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Characterization of New Players in Planar
Polarity Establishment in Arabidopsis
Stefano Pietra
Umeå Plant Science Centre
Fysiologisk Botanik
Umeå 2014
Characterization of New Players
in Planar Polarity Establishment
in Arabidopsis
Stefano Pietra
Umeå Plant Science Centre
Fysiologisk Botanik
Umeå 2014
This work is protected by the Swedish Copyright Legislation (Act 1960:729)
ISBN: 978-91-7601-050-1
Front cover by: Stefano Pietra
E-version available at http://umu.diva-portal.org/
Printed by: Servicecenter KBC, Umeå University
Umeå, Sweden 2014
Table of Contents
Table of Contents
i
Abstract
iii
Sammanfattning
iv
List of Papers
v
Author contributions
vi
Abbreviations
vii
Introduction
1
A common paradigm for cell polarity establishment
1
Cell polarity in unicellular organisms: fission and budding yeast
1
Planar polarity, the coordinate polar organization of a tissue layer
2
The frizzled planar polarity pathway in Drosophila
3
Planar polarity in plants: coordinate positioning of root hairs
6
An auxin gradient directs root hair polarity
6
Ethylene affects root hair polarity upstream of auxin
7
Auxin transport fine-tunes the auxin gradient and affects planar polarity
8
Effects of intracellular vesicle trafficking and GNOM on planar polarity
9
Polarly localized proteins in the root epidermis
10
The actin cytoskeleton is not only an effector of planar polarity
10
Rho-of-plant GTPases are the earliest markers of root hair planar polarity 11
Additional factors influencing planar polarity of root hairs
12
Root hair initiation and tip growth
13
Initiation and morphogenesis of leaf trichomes
15
Planar morphogenesis of pavement cells
17
Microtubules and their organization at the cell cortex
19
Organization and dynamics of the actin cytoskeleton
22
The plant cytoskeleton during cell division
25
The microtubule-associated protein CLASP
28
Patterning of the root and leaf epidermis
30
Aim
34
Results and Discussion
35
The kreuz und quer mutant
35
kreuz und quer is mutated in the SABRE gene
35
Planar polarity defects of sab mutants
36
Cell polarity defects of sab trichomes
37
The SAB protein
38
Homologs of the SAB protein
38
Subcellular localization of the SAB protein
39
SAB interaction with the CLASP gene
41
SAB and CLASP interact genetically
41
SAB also has a role in PPB orientation
41
i
SAB is not involved in mitotic progression
42
Complex interaction of SAB and CLASP in the control of distinct processes 43
SAB function in the organization of cortical microtubules
44
Role of SAB in elongating epidermal cells
44
Bipolar growth of longitudinal microtubule arrays
45
Cortical microtubule organization at root hair initiation sites
45
Actin is an additional player in the planar polarity pathway
47
ACTIN7 genetically interacts with SAB
47
The actin cytoskeleton affects planar polarity of root hair positioning
48
AIP1-2 is an actin interactor in plants
49
AIP1-2 expression is restricted to hair-producing cells
50
Interplay of ethylene signalling and actin cytoskeleton in planar polarity
51
Patterned expression of AIP1-2 depends on WER function
51
SAB has a role in root epidermal patterning
52
sab mutants differentiate excessive ectopic root hairs
52
Longitudinal cell divisions are not responsible for sab patterning defects
53
Destabilized expression of fate markers in the sab root epidermis
53
SAB affects epidermal cell fate upstream of the core patterning pathway
54
SAB does not control patterning of leaf trichomes
55
SAB may act on transduction of patterning cues from the cortex
56
Conclusions and Future Perspectives
57
Acknowledgements
59
References
60
ii
Abstract
Coordinated polarity and differentiation of cells in the plane of a tissue layer
are essential to the development of multicellular organisms. Arabidopsis
thaliana root hairs and trichomes provide model systems to study the
pathways that control planar polarity and cell fate specification in plants. A
concentration gradient of the plant hormone auxin provides an instructive
cue that coordinates polar assembly of signalling complexes at plasma
membranes of root epidermal cells; however, knowledge about additional
players and cytoskeletal effectors driving cell polarization prior to hair
emergence remains limited. On the other hand, epidermal cell fate
specification is controlled by a well-characterized gene network of
transcription factors that translate positional signals and cell-to-cell
communication into tissue-wide patterning. Yet, new components are
continuously found to interact with the patterning pathway, shedding light
on its connections with diverse developmental processes.
This thesis presents the SABRE (SAB) gene as a novel player in planar
polarity establishment and root epidermal patterning. SAB is a large protein
with sequence similarity to proteins present in all eukaryotes and affects
planar polarity as well as orientation of cell divisions and cortical
microtubules. Genetic interaction with the microtubule-associated protein
gene CLASP further supports involvement of SAB in microtubule
arrangement, suggesting a role for this gene in cytoskeletal organisation.
Strikingly, SAB also interacts genetically with ACTIN7 (ACT7), and both
ACT7 and its modulator ACTIN INTERACTING PROTEIN 1-2 (AIP1-2)
contribute to planar polarity of root hair positioning. Cell-file specific
expression of AIP1-2 depends on the epidermal-patterning regulator
WEREWOLF (WER), revealing a connection between actin organization,
planar polarity and cell fate specification. Consistent with this finding, SAB
also functions in patterning of the root epidermis by stabilizing cell fate
acquisition upstream of the core patterning pathway. These results unveil
new roles for SAB in planar polarity and epidermal patterning and suggest
that organization of the microtubule and the actin cytoskeleton are
important to both planar polarity establishment and cell fate specification.
iii
Sammanfattning
Samordning av polaritet och differentiering av celler inom ett vävnadslager
är avgörande för utvecklingen av multicellulära organismer. Rothår och
bladhår hos Arabidopsis thaliana utgör modellsystem för att studera
signalvägar som kontrollerar planpolaritet och specifikation av cellers öde
hos växter. En koncentrationsgradient av växthormonet auxin ger en
instruktiv signal som koordinerar polär hopsättning av signalkomplex vid
plasmamembranet i rotepidermisceller; dock är kunskapen om ytterligare
aktörer och hur cytoskelettets aktörer påverkar cellpolaritet innan rothår
bildas begränsad. Vad gäller differentieringen av epidermala cellers öde
kontrolleras dessa genom ett väl karakteriserat nätverk av
transkriptionsfaktorer som överför positionssignaler och cell-till-cell
kommunikation till vävnadsomfattande mönsterbildning. Fortfarande hittas
dock nya komponenter som interagerar med signalvägarna för
mönsterbildning, vilket ger nya insikter om dess förbindelser med diverse
utvecklingsprocesser.
Denna avhandling presenterar genen SABRE (SAB) som en ny aktör i
etableringen av planpolaritet och mönsterbildning av rotepidermis. SAB är
ett stort protein som har sekvenslikhet med proteiner som finns i alla
eukaryoter och det påverkar planpolaritet, orientering av celldelning och
kortikala mikrotubler. Genetisk interaktion med genen för det mikrotubuliassocierade proteinet CLASP stärker ytterligare inblandningen av SAB i
organiserandet av mikrotubler och antyder att denna gen har en roll i
organiserandet av cytoskelettet. Slående är att SAB även interagerar
genetiskt med ACTIN7 (ACT7) och att både ACT7 och dess modulator
ACTIN-INTERACTING PROTEIN1-2 (AIP1-2) bidrar till planpolaritet vid
positionering av rothår. Cellfils-specifikt uttryck av AIP1-2 beror på den
epidermala mönsterbildande genen WEREWOLF (WER), vilket påvisar ett
samband mellan organisationen av aktin, planpolaritet och specifikationen
av cellers öde. SAB fungerar även i mönsterbildning av rotens epidermis och
stabiliserar förvärvet av cellöde uppströms av den centrala signalvägen för
mönsterbildning. Dessa resultat visar på nya roller för SAB i planpolaritet
och mönsterbildning av epidermis och indikerar att organiseringen av
mikrotubler och aktin-cytoskelettet är viktiga både för etablerandet av
planpolaritet och för specificeringen av cellers öde.
iv
List of Papers
I
Stefano Pietra, Anna Gustavsson, Christian Kiefer, Lothar Kalmbach, Per
Hörstedt, Yoshihisa Ikeda, Anna N. Stepanova, Jose M. Alonso and Markus
Grebe (2013). Arabidopsis SABRE and CLASP interact to stabilize cell
division plane orientation and planar polarity. Nature Communications 4
II
Christian S. Kiefer, Andrea R. Claes, Jean-Claude Nzayisenga, Stefano
Pietra, Thomas Stanislas, Anke Hüser, Yoshihisa Ikeda and Markus Grebe.
Arabidopsis AIP1-2 restricted by WER-mediated patterning modulates
planar polarity. Submitted manuscript
III
Stefano Pietra*, Patricia Lang* and Markus Grebe. SABRE is required for
stabilization of root hair patterning in Arabidopsis thaliana. Submitted
manuscript
* These authors contributed equally to this work.
The papers will be referred to by their Roman numbers in the text.
Publications by Stefano Pietra NOT included in this thesis:
Stefano Pietra and Markus Grebe (2010). Auxin paves the way for planar
morphogenesis. Cell 143, 29-31
v
Author contributions
I
Stefano Pietra performed the fine-mapping and the map-based identification
of the kuq mutation (summarized in Figure 2), characterization of the kuq
mutant and other sab alleles necessary for Figure 1a-c and Figure 3a-e, RTPCRs shown in Figure 3f-h, analyses for Figure 4, quantifications for Figure
5a-e, live imaging for Figure 6c,d,r-t, Figure 7a,b,d-p, Supplementary Figure
S4d-k and Supplementary Movies 1-6, recombineering work to generate the
SAB-3xYpet and 3xYpet-SAB complemented sab-5 lines, live imaging for
Figure 8j-l and Figure 9a-h,v,w. He additionally co-supervised Lothar
Kalmbach during his Diploma thesis work that produced Figure 1h-m and
Supplementary Figure S2e,f. Stefano Pietra generated all used transgenic
lines expressing fluorescent markers in the sab background, contributed to
analysis and statistical analysis of all experiments and wrote the manuscript
together with Markus Grebe.
II
Stefano Pietra performed the ROP immunolocalization experiments, the
imaging, the quantification and the statistical analysis required for Figure 5.
He read, commented on and improved the manuscript draft.
III
Stefano Pietra initially observed the patterning defects in sab-mutant roots.
He subsequently co-supervised and guided Patricia Lang during her master
thesis work that produced the results required for all Figures, Tables 1 and 2.
Stefano Pietra performed all quantitative and statistical analysis of
epidermal cell patterning displayed in Table 3 including analyses of the sab5;wer-1 and sab-5;cpc-1 mutants. He generated experimental materials,
contributed to analysis and interpretation of all results and wrote the
manuscript together with Markus Grebe.
Stefano Pietra also performed part of the experiments, imaging and
quantification required for Figure 10 presented in the results and discussion
section of this thesis. The remaining part was performed by Anna
Gustavsson.
vi
Abbreviations
2,4-D
+TIP
ABP1
ABP
ACT2
ACT7
ACT8
ADF
AIP1
AIR9
AN
APT1
ARF1
ARF-GEF
ARP2/3
AUX1
AVG
axr2-1
BFA
CAP
CDK
CDS
CESA6
CLASP
CLC2
CLC3
CP
CPC
CtBP/BARS
CTR1
Dgo
DIS1
Ds
Dsh
EB1
EF-1α
EGL3
EIN1
2,4-dichlorophenoxyacetic acid
plus-end tracking protein
AUXIN BINDING PROTEIN 1
actin-binding protein
ACTIN2
ACTIN7
ACTIN8
ACTIN DEPOLYMERIZATION FACTOR
ACTIN INTERACTING PROTEIN 1
AUXIN INDUCED IN ROOTS 9
ANGUSTIFOLIA
ABERRANT POLLEN TRANSMISSION 1
ADP-RIBOSYLATION FACTOR 1
guanine exchange factor for adenosyl
ribosylation factor
actin-related protein 2/3
AUXIN RESISTANT 1
aminoethoxyvinylglycine
auxin resistant 2-1
Brefeldin A
CYCLASE ASSOCIATED PROTEIN
cyclin-dependent kinase
cortical division site
CELLULOSE SYNTHASE 6
CLIP170-associated protein
CLATHRIN LIGHT CHAIN 2
CLATHRIN LIGHT CHAIN 3
capping protein
CAPRICE
C-terminal binding proteins/brefeldin A ADPribosylated substrates
CONSTITUTIVE TRIPLE RESPONSE 1
Diego
DISTORTED 1
Dachsous
Dishevelled
END BINDING 1
ELONGATING FACTOR-1α
ENHANCER OF GLABRA3
ETHYLENE INSENSITIVE 1
vii
EIN2
ERH2
ERH3
ETC1
ETO1
ETR1
F-actin
Fj
Flr
Fmi
Frtz
Ft
Fy
Fz
G-actin
GA
GCP2
GCP3
GEF
GL1
GL2
GL3
GST
H
IBA
In
JA
JKD
KCA1
KIP
KTN1
kuq
MAP
MOR1
Mwh
N
NADPH oxidase
P
PDR8
PEN3
PIN
ETHYLENE INSENSITIVE 2
ECTOPIC ROOT HAIR 2
ECTOPIC ROOT HAIR 3
ENHANCER OF TRY AND CPC 1
ETHYLENE OVERPRODUCER 1
ETHYLENE RESPONSE 1
Filamentous actin
Four-jointed
Flare
Flamingo
Fritz
Fat
Fuzzy
Frizzled
Globular actin
gibberellin
γ-tubulin complex protein 2
γ-tubulin complex protein 3
guanine nucleotide exchange factor
GLABRA 1
GLABRA 2
GLABRA 3
Glutathione-S-Transferase
hair
indole-3-butyric acid
Inturned
jasmonic acid
JACKDAW
KINESIN CDKA;1-ASSOCIATED 1
KINKY POLLEN
katanin
kreuz und quer
microtubule-associated protein
MICROTUBULE ORGANIZATION 1
Multiple Wing Hairs
non-hair
nicotinamide adenine dinucleotide phosphate
oxidase
phosphorus
PLEIOTROPIC DRUG RESISTANCE 8
PENETRATION 3
PIN-FORMED
viii
PIP5K3
Pk
PLD
PLDζ1
POK1
POK2
POM1
PPB
PRC1
PtdIns(4)P
PtdIns(4,5)P2
RanGAP1
RHD2
RHD4
RHD6
Rho-GDI
ROP
ROS
RSH
RT-PCR
SAB
SCAR
SCM
SCN1
SCZ
SIM
SMT1
SNX1
SPK1
SPR1
Stan
Stbm
TAN1
TMK
TON1A
TON1B
TON2
TRY
Tsr
TTG1
Vang
VLN4
PHOSPHATIDYLINOSITOL PHOSPHATE 5KINASE 3
Prickle
PHOSPHOLIPASE D
PHOSPHOLIPASE Dζ1
PHRAGMOPLAST ORIENTING KINESIN 1
PHRAGMOPLAST ORIENTING KINESIN 2
POM POM 1
preprophase band
PROCUSTE 1
phosphatidylinositol 4-phosphate
phosphatidylinositol 4,5-bisphosphate
Ran GTPase ACTIVATING PROTEIN 1
ROOT HAIR DEFECTIVE 2
ROOT HAIR DEFECTIVE 4
ROOT HAIR DEFECTIVE 6
Rho-GDP dissociation inhibitor
Rho-of-plants
reactive oxygen species
ROOT-SHOOT-HYPOCOTYL-DEFECTIVE
Reverse transcription PCR
SABRE
suppressor of cAMP receptor defects
SCRAMBLED
SUPERCENTIPEDE 1
SCHIZORIZA
SIAMESE
STEROL METHYLTRANSFERASE 1
SORTING NEXIN 1
SPIKE 1
SPIRAL 1
Starry Night
Strabismus
TANGLED 1
TRANSMEMBRANE KINASE
TONNEAU 1A
TONNEAU 1B
TONNEAU 2
TRIPTYCHON
Twinstar
TRANSPARENT TESTA GLABRA 1
Van Gogh
VILLIN 4
ix
WAVE
WEI2
WEI7
WER
Wg
ZWI
Wiskott-Aldrich Syndrome protein family
verprolin-homologous protein
WEAK ETHYLENE INSENSITIVE 2
WEAK ETHYLENE INSENSITIVE 7
WEREWOLF
Wingless
ZWICHEL
x
Introduction
A common paradigm for cell polarity establishment
Cell polarity can be defined as an asymmetry in the shape, organization, and
distribution of structures within a cell (Cove, 2000). Polarized cell growth is
essential for the development of both unicellular and multicellular
organisms (Nelson, 2003). In simple single-cell organisms, like bacteria and
yeast, cell polarity is fundamental for morphogenesis, proliferation, and
ultimately survival. Similarly, multicellular organisms that are unable to set
up a correct polarity face early death or severe perturbation in their
development: their cells need to polarize in order to acquire a specific fate or
morphology and carry out specialized functions (Yang, 2008).
Although some systems are able to establish their polarity in an
autonomous way (Cove, 2000), in most cases polarization requires a specific
internal (biological) or external (environmental) signal to break cell
symmetry and initiate asymmetrical organization and dynamics of cellular
components. Despite the great diversity among cell types that display polar
growth, a common set of mechanisms is used by evolutionarily distant
organisms, and it is possible to outline a paradigm that can be applied to all
eukaryotic systems (Nelson, 2003; Yang, 2008): in response to an initial cue,
a polarity landmark is established on the cell surface and determines the
localized aggregation of signalling complexes of Rho-family small GTPases
(Perez and Rincón, 2010; Nelson, 2003; Yang, 2008). These central
signalling components initiate cascades that activate the mobilization of
proteins from intracellular pools and direct the recruitment and oriented
assembly of cytoskeletal structures, which in turn lead to targeted vesicle
secretion. Polarized protein transport in combination with endocytic
recycling generates a positive feedback loop able to reinforce the initial
signal and sustain polar growth (Geldner, 2009; Grebe, 2004).
The simplest examples of how polarity is generated and translated into
polar growth are unicellular organisms. Studies from the model systems
fission and budding yeast provide excellent platforms to understand and
explore similar conserved mechanisms that are employed by more complex
multicellular organisms.
Cell polarity in unicellular organisms: fission and budding yeast
Cells of the fission yeast Schizosaccharomyces pombe have a cylindrical rod
shape and grow by polarized tip extension until they enter mitosis and divide
in two shorter symmetrical cells (Piel and Tran, 2009). Microtubules play an
essential role in directing growth at the cell tips: they are organized in
1
bundles parallel to the long axis of the cell and are uniformly polarized with
their plus ends growing away from the geometrical cell centre (Nelson,
2003). Dynamic microtubules deliver to cell ends the microtubule plus end
proteins Tea1p and Tea4p, essential for marking the growth site (Mata and
Nurse, 1997; Martin et al., 2005). Tea1p is anchored to the cell cortex
through the membrane-associated protein Mod5p (Snaith and Sawin, 2003)
and the complex then recruits the polarisome complex, which includes the
actin-binding protein Bud6p and the formin For3p (Martin et al., 2005). The
Rho GTPase Cdc42p activates For3p (Martin et al., 2007), which nucleates
actin cables thus establishing tracks for myosin-driven vesicular transport of
materials for cell growth and of additional polarity determinants (Piel and
Tran, 2009). The imbalance between this polarized delivery and their rate of
dispersion allows accumulation of the polarity factors, generating a feedback
loop that reinforces the initial polarity cue (Piel and Tran, 2009).
The budding yeast Saccharomyces cerevisiae has cells with round shape
that divide by formation on their surface of a single bud, which grows polarly
and then separates at maturation. Positional information from the former
budding cycle of the yeast cell establishes a landmark (bud scar),
determining anisotropic growth of the plasma membrane. Also in this case,
specific localization and activation of Cdc42p is crucial for oriented assembly
of the actin cytoskeleton and targeting of vesicles to the bud site (Nelson,
2003; Perez and Rincón, 2010). Initial stochastic increases in Cdc42p
clustering are reinforced by actin filaments through their effects on targeted
secretion and endocytosis, in a positive feedback loop that counteracts lateral
diffusion and stabilizes growth polarity (Marco et al., 2007; Valdez-Taubas
and Pelham, 2003).
Hence, these are perfect examples from unicellular organisms of how an
initial polarity cue, mediated by the microtubule cytoskeleton in one case
and by cell-membrane landmarks in the other, can induce polar activation of
Rho GTPase molecular switches and in turn (re)organization of actin
filaments, driving targeted secretion of more polarity determinants to the
growth site. The cytoskeleton and Rho-type GTPases are central actors in
polarization of all eukaryotic systems, and it is therefore fascinating to
compare the mechanisms regulating such an essential process in very
distantly related species.
Planar polarity, the coordinate polar organization of a tissue layer
Setting up and regulation of polarity can gain additional levels of complexity
in multicellular systems. Polar growth of individual cells often needs to be
coordinated in the context of tissues and of the whole organism. This implies
that each cell can be polarized along several axes, and needs mechanisms to
distinguish multiple membrane domains and organize them differently
2
(Nelson, 2003; Geldner, 2009). In addition, polarity can be coordinated
among cells within a single tissue layer, determining alignment of the whole
plane to the same polarity cues. This process is referred to as planar polarity
(Nübler-Jung et al., 1987).
Planar polarity is most obvious in animal epithelia, where structures like
scales, feathers and hairs offer a very convenient read-out to analyze the
mechanisms that regulate their orientation. One of the most commonly used
models for research on planar polarity is hair orientation on the wings of the
fruitfly Drosophila melanogaster (Adler, 2002). Genetic studies in this
system have accumulated a large body of knowledge over the past decades,
revealing many of the molecular components that control planar polarity
establishment in animals (Zallen, 2007).
The frizzled planar polarity pathway in Drosophila
Cells of the Drosophila wing epithelium each produce a single hair that
emerges at the distal end of the cell and points towards the tip of the wing
(Wong and Adler, 1993). Initial studies identified a set of genes that form the
core planar polarity pathway. The name reflects that mutations in any of the
components of the pathway lead to non-polar cells, with hairs initiating in
their centre (Goodrich and Strutt, 2011). These components control planar
polarity of wing hairs through asymmetrical subcellular localization in both
cell-autonomous and non-autonomous ways (Adler, 2002).
A key member of this pathway is the frizzled (fz) gene, encoding a sevenpass Wnt transmembrane receptor and lending its name to the whole gene
network, which is commonly termed “the frizzled pathway” (Vinson and
Adler, 1987; Adler, 2002). From early stages of wing development, Fz
localizes distally on apical cell surfaces and recruits the cytoplasmic proteins
Dishevelled (Dsh), required for signal transduction (Strutt, 2009), and Diego
(Dgo). At the same time, the four-pass transmembrane protein Strabismus
(Stbm, also known as Van Gogh; Vang) and the cytosolic protein Prickle (Pk)
associate and accumulate specifically at proximal cell ends (Fig. 1; Zallen,
2007). Asymmetrical protein distribution can be achieved through
intracellular antagonistic interactions, which stabilize the formation of
mutually exclusive complexes at the two ends of a cell, and intercellular
contacts between distal and proximal complexes in adjacent cells (Tree et al.,
2002). These latter are mediated by the formation of homodimers of the
transmembrane cadherin Flamingo (Fmi, also known as Starry Night; Stan),
which localizes to both poles of the cells and allows heterologous interaction
between Fz and Stbm (Fig. 1; Strutt and Strutt, 2009). Cell-cell
communication establishes a feedback loop that reinforces the asymmetrical
subcellular localization of core proteins in neighbouring cells and is likely to
coordinate intercellular polarity, as demonstrated by the fact that mutations
3
Figure 1. The Drosophila frizzled pathway.
Core planar polarity proteins localize asymmetrically
across the junction between two wing epidermal cells,
forming a proximal and a distal complex that interact
to coordinate planar polarity of wing hairs. Frizzled
(Fz), Dishevelled (Dsh) and Diego (Dgo) localize to the
distal end of cells, whereas Strabismus (Stbm) and
Prickle (Pk) accumulate at proximal ends and
Flamingo (Fmi) forms homodimers over the cell
junction. Image adapted from Strutt and Strutt (2009)
with permission of the publisher.
in fz and stbm have non-cell autonomous effects on surrounding cells (Adler,
2002).
Asymmetrical localization of the core proteins of the planar polarity
pathway is dependent on each other’s presence, in a system capable of selforganizing polarity locally (Strutt and Strutt, 2005). However, the nature of
the global signal that initiates polarization of the core module and aligns it
across an entire tissue has been the object of a long debate (Zallen, 2007).
One candidate for such a role has for several years been the Fat/Dachsous
system (Strutt and Strutt, 2005). Fat (Ft) and Dachsous (Ds) are both large
atypical cadherins that localize to the apical ends of epithelial cells and
interact heterophilically across cell boundaries (Thomas and Strutt, 2012).
Their activity and accumulation are affected by a Golgi kinase, Four-jointed
(Fj), which is expressed in a gradient along the wing and modulates their
binding, generating a bias in the orientation of the heterodimers and thus a
directional cue (Matis and Axelrod, 2013). The findings that loss of Ft, Ds, or
Fj activity caused the core proteins to lose their ability to coordinate polarity
at long distance suggested that they could function as the factor dictating
global polarity upstream of the core pathway (Yang et al., 2002). Further
studies however revealed discrepancies within this linear three-tiered model
and nowadays the relationship between the Ft/Ds and core systems is
controversial. Currently, the Ft/Ds module is thought to most likely act in
parallel to or downstream of another global signal (Strutt, 2009; Goodrich
and Strutt, 2011; Matis and Axelrod, 2013).
From the very beginning of studies on planar polarity, the presence of a
gradient of Fz activity along the wing has been an attractive candidate for the
role of global signal imposing and maintaining directional polarity. Because
fz expression is homogeneous though, the model required the presence of a
morphogen whose concentration gradient could modulate Fz activation over
the whole tissue layer (Lawrence, 1966). Taking into account that in several
4
signalling pathways proteins of the Frizzled family acted as receptors for
secreted Wnt ligands and that Dsh was already part of a signalling cascade in
a different Wnt pathway (Thomas and Strutt, 2012), it was easy to presume
that the long-range signal providing a polarizing cue could be a Wnt ligand
(Adler et al., 1997). However, despite several Wnts being implicated in
planar polarity signalling in vertebrates and Wnt gradients being present in
other polarized tissues, evidence of a Wnt ligand controlling planar polarity
of Drosophila wing hairs has been lacking for many years (Goodrich and
Strutt, 2011). Only recently the two redundant Wnt proteins Wingless (Wg)
and dWnt4 have been shown to modulate local intercellular interactions
between Fz and Stbm. Through their graded distribution Wg and dWnt4
generate an aligned gradient of Fz activity providing the long-sought global
cue that orients planar cell polarity in the wing (Wu et al., 2013).
In addition to its role in coordinating tissue polarity, Fz also functions in
the initiation and placement of wing hairs (Adler, 2002). This cellautonomous activity relies on signalling through tissue-specific effectors
acting downstream of the core pathway and specifying the site of hair
growth. Three effector proteins, Inturned (In), Fritz (Frtz) and Fuzzy (Fy)
localize proximally in wing cells in a Stbm-dependent manner and direct
accumulation as well as activation of the formin-homology domain protein
Multiple Wing Hairs (Mwh) to proximal cell edges (Strutt and Warrington,
2008). Mwh functions as a repressor of actin filament formation and
restricts actin polymerization and hair initiation to the opposite, distal
region of the cell. Mutations in any of these effectors lead to multiple hairs
emerging in various locations around the cell periphery (Strutt and Strutt,
2009).
The importance of actin dynamics in wing hair initiation is confirmed by
the role of Rho family GTPases, modulators of the actin cytoskeleton,
downstream of Dsh: mutations in RhoA or its effector Drok, which acts on
the myosin II regulatory light chain in the wing, determine the formation of
multiple hairs pointing distally (Strutt et al., 1997; Winter et al., 2001), and
expression of a dominant negative version of Rac1 gives rise to duplicated or
triplicated wing hairs (Eaton et al., 1996). Furthermore, actin dynamics are
not only an output of the planar polarity pathway, limiting the number and
position of hair outgrowths, but are also an essential component required for
the pathway to function (Ren et al., 2007). In fact, mutants of either of the
two actin severing factors twinstar (tsr) and flare (flr), which encode the
Drosophila homologs of Cofilin/Actin Depolymerization Factor (ADF) and
Actin Interacting Protein 1 (AIP1), display hair polarity defects and aberrant
Fmi localization (Blair et al., 2006; Ren et al., 2007). These findings strongly
suggests that actin remodelling has a role in establishing the polarity of core
components of the pathway, possibly affecting their intracellular transport or
localized stabilization (Blair et al., 2006).
5
Planar polarity has been studied for the longest time and in greatest depth
through analyses of the growth of hairs on the wing epithelium (Adler,
2002); however, the frizzled pathway indeed also has a role in establishing
planar polarity of other Drosophila structures, like bristles and eye
ommatidia (Goodrich and Strutt, 2011). Orthologs of the frizzled core and
global components are present in many other organisms, including
vertebrates, and regulate diverse processes from convergent extension
during gastrulation to patterning of hairs in mammals (Simons and Mlodzik,
2008). Strikingly, however, no homologs of fz or any other planar polarity
core protein are present in plants.
Planar polarity in plants: coordinate positioning of root hairs
Plant species certainly also possess an array of polarized tissues, and must
thus have evolved different mechanisms to coordinate their polarity. One of
the systems offering the clearest read-out of polarization over the plane of a
whole tissue in plants is the root epidermis with its pattern of outgrowing
hairs (Grebe, 2004). Root hairs are unicellular structures that distantly
resemble the Drosophila wing hairs in the fact that they emerge distally in
hair-bearing cells (trichoblasts), at a conserved position close to the root tip
(Schiefelbein and Somerville, 1990). The uniform polarity of these structures
has been already observed in the middle of last century (Sinnott and Bloch,
1939). When powerful genetic tools in the model system Arabidopsis
thaliana became available, researches started to dissect the mechanisms that
regulate polarization of root hair placement (Masucci and Schiefelbein,
1994). However, studies specifically focusing on how planar polarity of hair
positioning is established and maintained in plants have been conducted
only throughout the last decade (Grebe, 2004; Nakamura et al., 2012).
An auxin gradient directs root hair polarity
In Arabidopsis the plant hormone auxin has a central role in the control of
hair polarity in the root (Fig. 2; Masucci and Schiefelbein, 1994; Sabatini et
al., 1999; Grebe, 2004). An auxin gradient with its maximum in the root tip
provides vectorial information for the orientation of root hairs (Fig. 3;
Fischer et al., 2006), and modulating this gradient or its perception can
affect epidermal cell polarity (Masucci and Schiefelbein, 1994; Grebe, 2004;
Fischer et al., 2006). Exogenous auxin supply or auxin overproduction
induce hair initiation at a more basal (rootward) position within trichoblasts,
while mutants affecting the response of cells to auxin, as the auxin resistant
2-1 (axr2-1) mutant, display an apical (shootward) shift of hair positioning
(Masucci and Schiefelbein, 1994). In addition, application of a membranepermeable auxin directly to the root epidermis of a mutant lacking an
6
endogenous auxin gradient is able to orient root hair growth towards the
auxin source, demonstrating that a local auxin concentration gradient is
sufficient to direct root hair polarization (Fischer et al., 2006).
Figure 2. Genetic framework of planar polarity in the Arabidopsis root. Ethylene signalling
through CONSTITUTIVE TRIPLE RESPONSE 1 (CTR1) and ETHYLENE INSENSITIVE 2 (EIN2) affects local
auxin biosynthesis by WEAK ETHYLENE INSENSITIVE 2 (WEI2) and WEAK ETHYLENE INSENSITIVE 7
(WEI7). Auxin is transported polarly by the influx carrier AUXIN RESISTANT 1 (AUX1) and the efflux carrier
PIN-FORMED 2 (PIN2) and forms a root-tip oriented gradient that guides positioning of Rho-of-plant (ROP)
small GTPases. ROP positioning is further affected by the GNOM guanine exchange factor, which also acts
upstream of PIN2. ROP accumulation directs polar initiation of root hairs. Diagram based on data from
Fischer et al. (2006) and Ikeda et al. (2009).
Ethylene affects root hair polarity upstream of auxin
The hormone ethylene is known to interact with auxin in a multitude of
processes (Muday et al., 2012), and also has a role in planar polarity of root
hair positioning (Fig. 2; Masucci and Schiefelbein, 1994; Fischer et al., 2006;
Ikeda et al., 2009). Exogenous application of the ethylene precursor 1Aminocyclopropane-1-carboxylic acid (ACC) polarizes hair initiation towards
the basal cell ends, and a similar hyperpolarization is determined by
increases in endogenous ethylene biosynthesis in mutants like the dominant
ethylene overproducer 1 (eto1; Masucci and Schiefelbein, 1994). On the
contrary,
inhibiting
ethylene
production
with
the
chemical
7
aminoethoxyvinylglycine (AVG) or ethylene perception with mutations in
ETHYLENE RESPONSE 1/ETHYLENE INSENSITIVE 1 (ETR1/EIN1) or
ETHYLENE INSENSITIVE 2 (EIN2) induces an apical shift in root hair
positioning (Masucci and Schiefelbein, 1994; Fischer et al., 2006). Ethylene
signalling acts upstream of auxin biosynthesis in the planar polarity
pathway, as demonstrated by the inhibitory effect of the negative regulator of
ethylene signalling CONSTITUTIVE TRIPLE RESPONSE 1 (CTR1) on the
local expression of the auxin biosynthesis genes WEAK ETHYLENE
INSENSITIVE 2 (WEI2) and WEAK ETHYLENE INSENSITIVE 7 (WEI7) in
the root tip (Ikeda et al., 2009). Mutations in CTR1 increase auxin
biosynthesis and consequently the auxin gradient in the root, resulting in a
basal shift of root hair positioning (Ikeda et al., 2009).
Figure 3. Polar root hair positioning directed by an auxin gradient. Root hairs initiate close to the
basal end of epidermal cells. Arrows indicate trichoblast polarization towards the auxin concentration
maximum in the root tip. Image adapted from Grebe (2004) and Fischer et al. (2006) with permission of the
publishers.
Auxin transport fine-tunes the auxin gradient and affects planar polarity
Generation and maintenance of the root tip-oriented auxin gradient does
not, however, only depend on auxin biosynthesis in shoot or root, but also
strongly relies on redistribution of the hormone via membrane-localized
specialized transporters (Kramer and Bennett, 2006). These include among
others the auxin influx carrier AUXIN RESISTANT 1 (AUX1; Bennett et al.,
1996) and auxin efflux carriers of the PIN-FORMED (PIN) family (Petrášek
et al., 2006), responsible for the acropetal transport (downward through the
8
root centre toward the tip) and basipetal recycling (upward through the
epidermal layer) of auxin in the root (Kramer and Bennett, 2006).
Polar auxin transport is indeed essential for the fine-tuning of the auxinresponse gradient in the root apex (Blilou et al., 2005) and a crucial
component of the non-cell autonomous effect of auxin on root hair planar
polarity (Fig. 2; Grebe et al., 2002; Ikeda et al., 2009). Loss-of-function aux1
mutations induce hair initiation at a more apical position and insensitivity to
the effects of the auxin influx carrier substrate 2,4-dichlorophenoxyacetic
acid (2,4-D) on root hair polarity (Grebe et al., 2002). By contrast, single
mutants of the genes encoding the PIN1 and PIN2 auxin efflux carriers do
not show any planar polarity defects, and only the quadruple
pin1;pin2;pin3;pin7 mutant displays a weak but significant apical shift,
suggesting that polar hair positioning does not rely strongly on the activity of
PIN proteins (Grebe et al., 2002; Fischer et al., 2006). However, mutation of
PIN2 partially suppresses hair hyperpolarization of ctr1 mutants and
enhances the apical shift of ein2 mutants, revealing a subtle contribution of
PIN2 to planar polarity establishment (Ikeda et al., 2009).
Effects of intracellular vesicle trafficking and GNOM on planar polarity
Polar membrane localization of auxin transporters is based on polar
targeting, endocytic recycling, and transcytosis (Kleine-Vehn and Friml,
2008). AUX1 localizes to the apical membrane of protophloem cells and to
apical and basal ends of epidermal cells (Swarup et al., 2001), PIN1 localizes
basally in vascular cells (Gälweiler et al., 1998), and PIN2 accumulates on
the apical membrane of epidermal cells and elongating cortical cells (Müller
et al., 1998), while it is situated on the basal end of meristematic cortical
cells (Blilou et al., 2005).
Delivery of auxin carriers to correct membrane domains is dependent on a
subclass of guanine exchange factors for adenosyl ribosylation factor small G
proteins (ARF-GEFs) that mediate intracellular vesicle trafficking (Geldner
et al., 2003). The fungal toxin Brefeldin A (BFA) specifically inhibits the
ARF-GEFs responsible for basal targeting of auxin transporters (Steinmann
et al., 1999; Kleine-Vehn et al., 2008), abolishing for instance membrane
localization of PIN1 and AUX1 (Steinmann et al., 1999; Grebe et al., 2002).
BFA treatment thus induces a defect in auxin distribution and polar
localization of root hairs, which emerge at a more apical position (Grebe et
al., 2002).
One of the direct targets of BFA is the ARF-GEF GNOM, which mediates
basal membrane localization of PIN1 and PIN2 but not AUX1 (Steinmann et
al., 1999; Geldner et al., 2003; Fischer et al., 2006). Hypomorphic gnom
mutants display an apical shift in root hair initiation, and combining a
hypomorphic gnom transheterozygote mutant combination with mutations
9
in AUX1 and EIN2 reveals synergistic activity of the three genes in
modulating the auxin gradient and polar hair positioning in the root (Fischer
et al., 2006). GNOM acts upstream of PIN2, as confirmed by genetic
analyses and perturbed basal PIN2 localization in the cortex of weak gnom
mutants (Kleine-Vehn et al., 2008; Ikeda et al., 2009). However, its function
in planar root hair polarity is likely not limited to an effect on PIN proteins,
because the defects in hypomorphic gnom mutants are much stronger than
those detected in knock-outs of multiple PIN genes (Fig. 2; Fischer et al.,
2006).
Polarly localized proteins in the root epidermis
Auxin transporters are not the only proteins that localize polarly in the
Arabidopsis root epidermis. Several proteins are subject to specific
trafficking that allows them to accumulate at distinct membrane domains in
epidermal cells. An example is the PENETRATION 3/PLEIOTROPIC DRUG
RESISTANCE 8 (PEN3/PDR8) ATP binding cassette transporter, which is
involved in defence from pathogens and efflux of the auxin precursor indole3-butyric acid (IBA), and localizes to outer membranes at the root-soil
interface (Stein et al., 2006; Strader and Bartel, 2009; Łangowski et al.,
2010). On the opposite side of the cells, the boric acid/borate exporter BOR1
localizes polarly to the inner lateral membrane domain and translocates
boron from the epidermis toward the xylem in a tightly controlled manner
(Takano et al., 2010). Finally, the AGC protein kinase D6PK, which controls
efficient auxin transport and is able to phosphorylate PIN proteins, localizes
to the basal membrane of several meristematic root cell types, including
epidermal cells (Zourelidou et al., 2009). At the moment however, none of
these polarly localized proteins has been characterized for having any effect
on establishment or regulation of root hair planar polarity.
The actin cytoskeleton is not only an effector of planar polarity
Despite fundamental differences in the global polarizing cues as well as the
core genes that determine planar polarity of hairs between Arabidopsis and
Drosophila, the final effectors that control hair assembly and initiation at
polar sites appear surprisingly similar.
The actin cytoskeleton is the main candidate for initiating the final
morphological events that lead to emergence of root hairs, as filamentous
actin (F-actin) accumulates in root hair bulges just after hair initiation
(Baluška et al., 2000), although data on early stages have not been published
yet (Grebe, 2004). Furthermore, although no detailed experiments have
focused on placing actin within the planar polarity pathway, mutations in the
ACTIN2 (ACT2) gene have been shown to affect not only root hair growth
10
but also positioning of the hair initiation site, leading to slightly apicallyshifted hairs in addition to causing the occasional formation of multiple hairs
per trichoblast (Ringli et al., 2002).
Rho-of-plant GTPases are the earliest markers of root hair planar polarity
Actin organization is regulated in other systems by small GTPases of the Rho
family, and indeed in root hair initiation as well members of the Rho-ofplants (ROP) family seem to play a central role in coordinating actin at sites
of hair formation. ROPs relocalize polarly to hair initiation sites even prior to
any visible sign of hair outgrowth (Molendijk et al., 2001; Jones et al.,
2002), and ROP2 overexpression induces additional and often misplaced
hairs on single cells (Jones et al., 2002).
Loss-of-function evidence to complement these data is missing, but
knock-out of the gene encoding the Rho-GDP dissociation inhibitor (RhoGDI) SUPERCENTIPEDE 1 (SCN1) that limits ROP2 activation also leads to
multiple sites of hair growth on individual trichoblasts (Carol et al., 2005),
functionally supporting a role for ROPs in hair initiation site selection. ROP
patches are the earliest markers of future sites of hair formation, and their
positioning is dependent on the combined action of AUX1, of ethylene
signalling and of GNOM on the generation of an auxin gradient in the root
tip (Fig. 2; Fischer et al., 2006; Ikeda et al., 2009). Furthermore,
mathematical modelling studies of auxin-dependent ROP activation support
this view: given a specific cell length, ROP levels and active versus inactive
ROP diffusion rates, an intracellular gradient of auxin concentration is
sufficient to spontaneously drive polar placement of ROP patches (Payne and
Grierson, 2009).
In addition, auxin exogenously applied to leaf protoplasts can activate
ROP2 and ROP6 through AUXIN BINDING PROTEIN 1 (ABP1) and
members of the TRANSMEMBRANE KINASE (TMK) family of kinases,
leading to the reorganization of the actin and microtubule cytoskeleton (Xu
et al., 2010; Xu et al., 2014). This shows that auxin can indeed positively
regulate ROPs and their downstream effectors. Whether the same
mechanism exists in root cells and how it can generate a polarity cue from a
concentration gradient remains to be investigated.
Polar localization of ROP2 to hair initiation sites also depends on function
of ADP-RIBOSYLATION FACTOR 1 (ARF1) family members, central
components of the intracellular vesicle trafficking machinery whose activity
can be inhibited by BFA (Molendijk et al., 2001; Xu and Scheres, 2005). This
suggests another possible regulatory mechanism upstream of ROPs, but the
exact functional link between the polarizing signal and potential downstream
effectors of root hair polarity remains to be found.
11
Additional factors influencing planar polarity of root hairs
Additional processes and genes affect planar polarity of the root epidermis,
although it is not clear yet what their role is and at which stage they come
into play.
For instance, clathrin-mediated endocytosis, a mechanism controlling
membrane internalization and protein recycling from the plasma membrane
and the trans-Golgi network, has been proposed to be important for polar
positioning of root hairs. Double mutants of CLATHRIN LIGHT CHAIN 2
(CLC2) and CLATHRIN LIGHT CHAIN 3 (CLC3) initiate their hairs at a
more apical position in trichoblasts (Wang et al., 2013), and this defect has
been suggested to depend on aberrant auxin transport or signalling (Wang et
al., 2013). However, no direct evidence that the phenotype is caused by
altered auxin distribution is currently available, and endocytosis may as well
have non-auxin-related effects on planar polarity.
Furthermore, an important factor in modulating differential endocytosis
of polarly distributed proteins is membrane sterol composition (Men et al.,
2008). The sterol biosynthesis mutant sterol methyltransferase 1 (smt1) has
defects in cell polarity and polar auxin transport, and in addition displays
more randomized positioning of hairs in the root epidermis, suggesting that
sterols do as well have a role in planar polarity establishment (Willemsen et
al., 2003). This hypothesis is supported by the detection of sterols
accumulating to sites of root hair formation at very early stages of bulge
initiation, already before any structural sign of outgrowth is visible (Ovecka
et al., 2010). It is thus tempting to speculate that sterols are involved in
selection of the bulging site.
One of the first steps required for bulge formation in root hair cells is local
loosening of the cell wall. Altering the cell wall structure by mutating a gene
responsible for cellulose biosynthesis, as in the procuste 1 (prc1) mutant of
CELLULOSE SYNTHASE 6 (CESA6), can affect planar polarity of ROP and
root hair positioning (Singh et al., 2008). In prc1 mutants, hairs emerge
from both more basal and more apical positions along the trichoblasts, and a
similar defect is observed in localization of the ROP patches that mark the
future sites of hair initiation. It could be that cell wall composition influences
selection of the polar site for hair outgrowth, but the molecular mechanisms
that connect this contribution to the planar polarity pathway are currently
elusive.
PRC1 affects hair formation downstream of a transcription factor acting
very early in root hair initiation, ROOT HAIR DEFECTIVE 6 (RHD6;
Masucci and Schiefelbein, 1994; Singh et al., 2008). Mutants defective in
RHD6 display a reduced number of root hairs and were also the first
Arabidopsis mutants characterized for having defects in root hair polar
positioning: trichoblasts of rhd6 roots produce hairs from a more apical
12
position compared to wild type (Masucci and Schiefelbein, 1994). Auxin and
ACC application can rescue the rhd6 mutant phenotypes, indicating that
RHD6 function is most likely mediated by auxin and ethylene. However, the
exact role of RHD6 in planar polarity establishment is still unknown.
Root hair initiation and tip growth
Root hairs are a system of choice for studying planar polarity in plants. They
are long tubular projections that grow on the outer surface of epidermal
cells, and represent the main point of contact between roots and soil. Their
various roles include water and nutrient uptake, anchorage, and interaction
with microorganisms (Schiefelbein, 2000; Dolan, 2001; Grierson et al.,
2001).
Specification of root hairs takes place in the meristem based on positional
information from the underlying cortex, and epidermal cell fate is acquired
already during embryonic root development, although it is still possible for it
to change postembryonically (Berger et al., 1998a). Cells destined to produce
a hair have a denser cytoplasm and smaller vacuole compared to non-hair
cells, have a higher division rate but elongate more slowly than non-hair cells
(Dolan et al., 1994; Berger et al., 1998b).
Initiation of hairs in elongating cells is under the control of signalling
from ethylene and depends on auxin, whose transport from the root tip to
differentiating hair cells is facilitated by specific expression of the AUX1
auxin influx transporter in non-hair cells (Jones et al., 2009). Several
mutants related to ethylene or auxin perception show that hairs can be
initiated on cells with cytological characteristics of non-hair cells, and vice
versa. Regulation through ethylene and auxin may allow plants to modulate
root hair density in response to environmental stimuli and thus override the
positional cues (Schiefelbein, 2000).
The first morphological sign of hair outgrowth is the formation of a bulge
at a specific site on the lateral wall of an almost fully elongated epidermal
cell. Size and number of swellings are under tight genetic control (Grierson
et al., 2001), and bulge outgrowth results from an initial acidification of the
cell wall (Bibikova et al., 1998), which locally activates wall-loosening
proteins allowing directional turgor-driven deformation of the cell surface
(Rounds and Bezanilla, 2013).
Within a growing hair bulge, rearrangement of the cytoskeleton and
polarization of the cytoplasm prepare the cell for tip-oriented hair
elongation. Dense and dynamic F-actin meshworks assemble just below the
growing tip (Baluška et al., 2000) and long actin bundles at the cell cortex
and in the central region of the hair orient axially and are essential to drive
hair growth and reverse-fountain cytoplasmic streaming (Rounds and
Bezanilla, 2013). Accordingly, mutation of ACT2 (Ringli et al., 2002) and
13
mutation or inhibition of genes encoding proteins involved in actin filament
initiation like DISTORTED 1 (DIS1; Mathur et al., 2003a) and CROOKED
(Mathur et al., 2003b), in actin turnover like ACTIN INTERACTING
PROTEIN 1-1 (AIP1-1) and ACTIN INTERACTING PROTEIN 1-2 (AIP1-2;
Ketelaar et al., 2004), or in actin bundling like VILLIN 4 (VLN4; Zhang et
al., 2011) affect tip growth, leading to shorter root hairs. Cortical
microtubule arrays, which are transversal to the root axis in elongating
trichoblasts, reorganize at the onset of hair outgrowth (Van Bruaene et al.,
2004) and align to the root-hair shank to control growth direction and limit
the number of growth sites (Bibikova et al., 1999). Shortly after bulge
formation, the root hair starts elongating by tip growth and the nucleus is
driven into the hair by actin-regulated processes (Ketelaar et al., 2002).
Soon after tip growth initiated, a Ca2+ gradient focused towards the apical
end of the hair is established (Wymer et al., 1997), and reactive oxygen
species (ROS) accumulate close to the growing region (Foreman et al.,
2003). Calcium ions and ROS are part of a positive feedback loop including
the ROOT HAIR DEFECTIVE 2 (RHD2) nicotinamide adenine dinucleotide
phosphate oxidase (NADPH oxidase), which localizes to growing root hair
tips in an actin-dependent manner (Jones et al., 2007; Takeda et al., 2008)
and there produces ROS. These molecules activate hyperpolarizationactivated Ca2+ channels facilitating influx of Ca2+ (Foreman et al., 2003),
which in turn induces RHD2 activity (Takeda et al., 2008) and ensures a
robust mechanism for maintaining polar hair elongation.
While elongating, root hairs oscillate between periods of fast and slow
growth that are tightly correlated with oscillations in extracellular pH,
extracellular ROS accumulation, and cytosolic Ca2+ concentration
(Monshausen et al., 2007; Monshausen et al., 2008). Cyclic increases in pH
and ROS locally stiffen the cell wall, limiting tip growth and contributing to
restricting it spatially, while at the same time affecting organization of the
actin cytoskeleton (Ishida et al., 2008, Cárdenas, 2009). Ca2+ as well plays a
crucial role in fine-tuning actin dynamics, and in addition is implicated in
regulating exocytosis near the hair apex (Monshausen et al., 2008). During
root hair growth a large number of vesicles form close to the hair tip in what
is referred to as the clear zone, a region rich of endoplasmic reticulum and
Golgi bodies (Rounds and Bezanilla, 2013). Vesicles are polarly secreted and
fuse with the plasma membrane, delivering new cell wall material to the
growing tip in a process strictly dependent on a functional actin cytoskeleton
(Dolan, 2001; Grierson et al., 2001).
Phospholipids, and in particular phosphatidylinositols, also contribute to
the control of root hair elongation, acting as second messengers in
cytoskeletal
reorganization
and
membrane
trafficking:
PHOSPHATIDYLINOSITOL PHOSPHATE 5-KINASE 3 (PIP5K3), an
enzyme involved in the synthesis of phosphatidylinositol 4,5-bisphosphate
14
[PtdIns(4,5)P2], localizes to sites of root hair initiation even prior to bulge
formation, and pip5k3 mutants do not accumulate PtdIns(4,5)P2 at root hair
growing tips and display much shorter root hairs (Kusano et al., 2008).
Furthermore, the phosphatidylinositol 4-phosphate phosphatase ROOT
HAIR DEFECTIVE 4 (RHD4) regulates polarized secretion at growing root
hair tips, and rhd4 mutants accumulate phosphatidylinositol 4-phosphate
[PtdIns(4)P] and have short and bulged root hairs (Thole et al., 2008).
Wild-type root hairs rarely branch, but several conditions including
interference with the microtubule cytoskeleton (Bibikova et al., 1999) and
mutations of the Rho-GDI gene SCN1 (Parker et al., 2000) have been shown
to strongly induce hair branching. Hair elongation proceeds until the hair is
about 1 mm long and is promoted by auxin and ethylene signalling, as
demonstrated by the long hairs of seedlings treated with 2,4-D or ACC and
shorter hairs of mutants impaired in auxin or ethylene signal transduction
(Pitts et al., 1998).
Initiation and morphogenesis of leaf trichomes
Leaf trichomes represent a fine example of cells that coordinate their polarity
within the plane of a tissue layer: their branches orient along the leaf
proximo-distal axis over the whole leaf surface, offering a clear polar readout (Fig. 4; Hülskamp et al., 1994). These characteristics, and the possibility
for mutations to affect their coordinated orientation (Kirik et al., 2007),
make trichomes good potential models for studying planar polarity in the
leaf epidermis.
Figure 4. Trichome organization on the leaf epidermis. Trichomes emerge at regular intervals from
the leaf surface and undergo two branching events during their maturation, orienting their proximal side stem
to the leaf proximo-distal axis. Images adapted from Yang (2008) and Hülskamp et al. (1994) with permission
of the publishers.
15
In Arabidopsis, trichomes are large unicellular structures that
differentiate on the epidermis of several organs, including leaves, and their
functions are related to protection from insect herbivores, excessive
transpiration, and UV light (Hülskamp, 2004). Leaf trichome development
initiates near the distal end of young leaves from single protodermal cells
spaced at regular intervals of three to four cells from each other (Hülskamp,
2004). Specification of the trichome fate is carried out through a complex
activator-inhibitor mechanism that by intercellular communication is able to
reinforce stochastic fluctuations of trichome promoting and suppressing
factors thus establishing de novo patterning (Pesch and Hülskamp, 2004;
Schellmann and Hülskamp, 2005). Hormone signalling also affects trichome
density, as application of gibberellin (GA) and jasmonic acid (JA) stimulates
trichome formation, while salicylic acid decreases their number (An et al.,
2013).
Once trichomes are initiated they undergo four rounds of
endoreduplication, resulting in cells with increased size and 16 times the
DNA content of a diploid cell. The switch from mitotic division to
endoreduplication is controlled by the cyclin-dependent kinase (CDK)
inhibitor SIAMESE (SIM; Churchman et al., 2006), whose loss-of-function
induces multicellular trichomes. The number of endoreduplication cycles is
tightly regulated by several mechanisms, including protein degradation,
hormone signalling, DNA decatenation and cell-death regulation
(Schellmann and Hülskamp, 2005). Defects in trichome ploidy have
profound effects on trichome morphology, as the number of branches
positively correlates with the cellular DNA content (Hülskamp, 2004).
Surprisingly, recent studies revealed that endoreduplication also plays a role
in maintaining trichome cell identity, thus confirming the importance of a
precise control of the cell cycle (Bramsiepe et al., 2010).
Enlarged trichome cells with an increased DNA content start growing out
of the leaf surface and undergo two consecutive branching events (Hülskamp
et al., 1994). The first event results in a proximal side stem and a distal main
stem, which both align to the leaf proximo-distal axis; subsequently the main
stem splits into two branches, in a plane perpendicular to the primary
branching plane (Fig. 4; Folkers et al., 1997). Trichome branch initiation
depends on the microtubule cytoskeleton: cortical microtubules reorient
when a branch is formed, and mutants or treatments that affect de novo
synthesis or fragmentation and realignment of microtubules display reduced
branching or even completely isotropic growth (Mathur et al., 1999; Kirik et
al., 2002a; Kirik et al., 2002b; Webb et al., 2002). On the contrary, drug
treatments that stabilize microtubules are able to induce new branch points
in branching-defective mutants (Mathur and Chua, 2000).
In addition, specific transport along microtubules also seems to have an
important role in branch formation: the branching-related gene ZWICHEL
16
(ZWI) encodes a kinesin-like microtubule motor protein (Oppenheimer et
al., 1997) that interacts with the C-terminal binding proteins/brefeldin A
ADP-ribosylated substrates (CtBP/BARS) related protein ANGUSTIFOLIA
(AN; Folkers et al., 2002). Both zwi and an mutants display only two
branches as a consequence of no secondary branching event (Hülskamp et
al., 1994). AN may be involved in regulating vesicle budding from Golgi
stacks, and another kinesin protein, KINESIN-13A, has been found to play a
role in trichome branching and distribution of Golgi stacks at the cell
periphery (Lu et al., 2005). These findings have led to the formulation of a
“Golgi delivery model” (Smith and Oppenheimer, 2005) where KINESIN13A directs transport of Golgi stacks along cortical microtubules to branch
initiation sites and AN, which is targeted to the branching sites by ZWI,
facilitates fission of vesicles containing material for branch initiation.
After branches are initiated, trichomes continue increasing their size by
expanding along the whole cell surface, in a process that strictly depends on
an intact actin cytoskeleton (Hülskamp, 2004). Mutants affected in the
DISTORTED class of genes all display defects in the directionality of
trichome expansion, similar to those of plants treated with drugs interfering
with actin function (Mathur et al., 1999). Several of these genes encode
subunits of two complexes involved in control of the actin cytoskeleton: the
actin-related protein 2/3 (ARP2/3) complex and the suppressor of cAMP
receptor defects/Wiskott-Aldrich Syndrome protein family verprolinhomologous protein (SCAR/WAVE) complex, which regulates the activity of
ARP2/3 (Mathur et al., 2003a; Mathur et al., 2003b; Basu et al., 2005;
Szymanski, 2005). The ARP2/3 complex promotes nucleation of new F-actin
from pre-existing filaments, and could therefore be responsible for
organization of the cytoplasmic actin cables that extend through the
elongating trichome branches and contribute to cytoplasm organization,
organelle motility and spatial regulation of cell expansion (Szymanski, 2005;
Smith and Oppenheimer, 2005). Recent results have shown that activation
of the SCAR/WAVE complex is mediated by signalling from the ROP
guanine nucleotide exchange factor (GEF) SPIKE 1 (SPK1; Basu et al., 2008).
Mutation of SPK1 also affects trichome branching and arrangement of the
microtubule cytoskeleton (Qiu et al., 2002), thus suggesting
interdependence and integration of microtubules and F-actin organization in
trichome morphogenesis.
Planar morphogenesis of pavement cells
Pavement cells are unspecialized epidermal cells that coordinate their polar
growth within the plane of the leaf surface (Yang, 2008). Polarity of
pavement cells is multidirectional and the acquisition of a specific cell
morphology is based exclusively on cell-cell coordination of growth.
17
Therefore, interconnected shaping of pavement cells is referred to as planar
morphogenesis (Nakamura et al., 2012).
Pavement cells possess a characteristic jigsaw puzzle shape consisting of
interdigitating lobes and indentations whose development is
spatiotemporally mutually regulated in neighbouring cells (Fig. 5; Yang,
2008). The mechanisms that establish and modulate cell polarity in
pavement cells are strikingly similar to those that operate in other types of
polarly growing cells: they are based on organization of the actin and
microtubule cytoskeleton through ROP small GTPases, which in turn
transduce signals from the hormone auxin (Smith and Oppenheimer, 2005).
Feedback regulation within the signalling pathway ensures stability of the
system and allows for polarity to be integrated between adjacent cells (Xu et
al., 2011).
Figure 5. Interdigitated morphogenesis of pavement cells. The polarly localized auxin efflux carrier
PIN-FORMED 1 (PIN1) facilitates auxin accumulation in the cell wall between two developing pavement cells.
At the lobe of one cell, AUXIN BINDING PROTEIN 1 (ABP1) senses auxin and activates Rho-of-plant 2
(ROP2), which promotes assembly of cortical actin filaments (F-actin) through the RIC4 effector. In the
adjacent cell, auxin signalling activates Rho-of-plant 6 (ROP6), which triggers the association of the effector
RIC1 with cortical microtubules. This association promotes the formation of microtubule bundles that restrict
cell expansion and generate an indentation. The two pathways antagonize each other: ROP2 suppresses RIC1
activity in lobes, whereas microtubule bundles repress the interaction between ROP2 and RIC4 in
indentations. Image reproduced from Pietra and Grebe (2010) with permission of the publisher.
Recent findings suggest that in pavement cells extracellular auxin is sensed
by ABP1 and induces interaction between ABP1 and the TMK receptor at the
plasma membrane (Xu et al., 2014). This complex transduces the auxin
signal to activate two antagonistic membrane-associated ROPs (Fig. 5; Xu et
al., 2010): ROP2, through its effector RIC4, promotes the assembly of
cortical F-actin and induces polar outgrowth and the formation of a lobe (Fu
et al., 2005); ROP6 on the contrary, through its effector RIC1, organizes
18
parallel bundles of cortical microtubules that locally restrict cell expansion
and generate an indentation (Fu et al., 2009; Smith, 2003). Inhibition of
RIC1 by ROP2 and repression of ROP2 activation through RIC1-dependent
microtubule organization (Fu et al., 2005) ensure that only one of the two
antagonistic pathways is activated in a specific cortical region of a pavement
cell. This and another feedback mechanism, ROP2 stimulating PIN1 polar
accumulation at lobe tips to export more auxin into the cell wall (Xu et al.,
2010), enforce growth coordination between neighbouring cells and
determine the growth of lobes where the contiguous cell is forming
indentations, and indentations where there are lobes (Xu et al., 2011).
The example of pavement cells morphogenesis illustrates how tight
regulation of cytoskeletal organization through ROPs can modulate
anisotropic cell expansion to generate functional shapes. ROPs are essential
for the coordinated establishment of cell polarity in adjacent cells and are
key elements for transduction of polarizing signals like auxin and other
hormones (Li et al., 2013).
Microtubules and their organization at the cell cortex
Microtubules are multimeric structures composed of heterodimers of the
globular proteins α- and β-tubulin. One α-tubulin and one β-tubulin
molecule, of which the Arabidopsis genome encodes six and nine isoforms
respectively (Ishida et al., 2007), each bind a GTP molecule and then
associate forming active dimers that assemble into hollow cylindrical
structures. After polymerization, β-tubulin monomers hydrolyze their GTP
nucleotide to GDP, losing their ability to reassemble onto a microtubule until
GDP is exchanged for GTP. Subunit asymmetry determines the polar nature
of microtubules, whose two ends have different assembly and disassembly
rates: the faster growing end is designated as the plus or leading end, while
the less active one is referred to as the minus or lagging end (Desai and
Mitchison, 1997).
Microtubules are highly dynamic polymers, with the ability at steady state
to constantly add and lose subunits at each of their two ends. Initiation of
new microtubules requires nucleation complexes, whose role is to lower the
energetic barrier for assembling new polymers. In plants, these complexes
are composed of two molecules of γ-tubulin associated with one molecule
each of γ-tubulin complex protein 2 (GCP2) and γ-tubulin complex protein 3
(GCP3; Seltzer et al., 2007). While nucleation complexes of animal cells are
located on centrosomes during interphase, plant cells lack centrosomes, and
their nucleation sites localize at the nuclear surface and at the cell cortex
(Ehrhardt and Shaw, 2006). Cortical microtubules can initiate either from
widely dispersed locations devoid of other polymers or, more commonly,
branching at a defined angle from sites residing along existing microtubules
19
(Fig. 6; Nakamura et al., 2010; Murata et al., 2005). As microtubules
elongate, their minus end is released from the nucleation site through action
of a katanin-containing severing complex, and new dimers are added to the
plus end (Sedbrook and Kaloriti, 2008). New polymers that are created in
proximity to the cell cortex soon
establish
cortical
association
(Ehrhardt,
2008).
While
microtubules grow, they keep
being cross-linked to the cell
membrane through a mechanism
that may depend on the lipidhydrolyzing
enzyme
PHOSPHOLIPASE
D
(PLD;
Gardiner et al., 2001; Dhonukshe
et al., 2003).
At this stage both the plus and
minus end of microtubules
undergo dynamic instability, a
behaviour
that
alternates
moments of growth and periods of
depolymerization (Fig. 6; Chan et
al., 2003). The presence of a cap
of GTP-bound tubulin subunits at
the plus end favours the addition
of new tubulin dimers, while the
GDP-bound β-tubulin subunits at
the
minus
end
tend
to
disassemble,
promoting
depolymerization at this end. This
causes microtubules to relocate by
continuous addition and removal
of dimers, through a mechanism
that is termed hybrid treadmilling
Figure 6. Plant microtubule dynamics. Modes
(Fig. 6; Shaw et al., 2003).
of microtubule initiation, growth and relocation
Association
to
the
plasma
behaviours, and possible outcomes of microtubule
encounters. Image adapted from Müller et al. (2009)
membrane
ensures
that
with permission of the publisher.
microtubules do not slide laterally
or leave the cell cortex. Thus,
microtubules advance by treadmilling and explore the two-dimensional
cortical space until they encounter other microtubules.
Encounter of a growing microtubule end with another microtubule leads
to cross-over or catastrophe when the two meet at an angle greater than 3040°, and induces bundling when the angle of incidence is lower (Fig. 6; Dixit
20
and Cyr, 2004). Cross-over often determines severing of microtubules by the
severing protein katanin (KTN1; Wightman and Turner, 2007), while
catastrophe consists in the rapid switch from growth to shrinking. Loss of
the GTP-cap initiates depolymerization of the GDP-bound subunits from the
plus end and can only be reversed by addition of new GTP-activated tubulin
dimers, an event termed “rescue” (Sedbrook and Kaloriti, 2008). Bundling
after sharp-angle encounters is at the base of the self-organization of
microtubules into arrays of higher-order structures: collision at low angles
induces realignment of the microtubule trajectory leading the growing
microtubule to continue elongating parallel to the encountered microtubule
(Dixit and Cyr, 2004). While the growing microtubule advances by
treadmilling, its non-aligned minus end depolymerizes or “zips” to the
encountered microtubule, thus leading to perfectly coaligned structures that
are likely to induce other inciding microtubules to realign, and generate
progressively larger bundles (Ehrhardt, 2008).
Formation of stable bundles is essential for microtubules to provide an
enduring cortical scaffold for biochemical complexes that require support
over an extended period of time (Ehrhardt and Shaw, 2006). The main
example of such structures are cellulose synthase complexes, which need to
be guided while they deposit cellulose microfibrils in the cell wall (Paredez et
al., 2006). By reorienting microtubule bundles at different developmental
stages, in specific locations within the cell, or in response to specific
environmental signals (Lindeboom et al., 2013), cells are able to affect the
cell wall growth pattern and regulate their own morphology and growth
anisotropy. For instance, cortical microtubules of newly divided root
meristematic cells are relatively randomly arranged, and they organize into a
transversal pattern of bundles to drive directional cell expansion until the
cell reaches maturity, at which point the bundles slowly reorient and become
parallel to the root axis (Ehrhardt and Shaw, 2006). Despite their higher
stability compared to individual microtubules, cortical microtubule bundles
are still highly dynamic structures and are constantly disassembled and
recreated by means of the self-organizing dynamic interactions of the
individual microtubule polymers.
In order to be able to self-organize, microtubule arrays also require the
activity of a large variety of microtubule-associated proteins (MAPs). MAPs
are defined by their ability to bind directly to the microtubule lattice and to
decorate microtubules (Sedbrook and Kaloriti, 2008). They have roles that
range from nucleating to stabilizing or destabilizing, cross-linking, severing
and anchoring microtubules. Some MAPs are conserved between animals
and plants, while others belong to families that are only found in plant
species (Gardiner, 2013).
Prominent MAPs that are involved in the organization of cortical
microtubules include the already mentioned GCP2 and GCP3 (Nakamura
21
and Hashimoto, 2009), required for microtubule nucleation, and KTN1, the
homolog of the animal p60 katanin ATPase subunit that severs microtubules
releasing their minus ends (Burk et al., 2001; Bichet et al., 2001).
MICROTUBULE ORGANIZATION 1 (MOR1) is a MAP required for
construction of the microtubule array (Whittington et al., 2001), while
MAP65 is part of a family that creates bridges between microtubules and is
essential for their stability and bundling (Smertenko et al., 2000). A group of
MAPs localize to growing ends of microtubules and dissipate upon
microtubule shrinking, and are therefore called plus-end tracking proteins
(+TIPs). They include the plant homologs of END BINDING 1 (EB1; Chan et
al., 2003) and CLIP170-associated protein (CLASP; Kirik et al., 2007;
Ambrose et al., 2007), and the plant-specific SPIRAL 1 (SPR1; Sedbrook et
al., 2004; Nakajima et al., 2004). In animal cells, +TIPs stabilize plus ends
of microtubules in the so-called “search and capture” process, where they
promote recognition and association of microtubules with specific structures
(Sedbrook and Kaloriti, 2008). A similar role could be hypothesized in
plants, where +TIPs might regulate microtubule stability and mediate
binding of plus ends as well as association with the cell cortex (Sedbrook and
Kaloriti, 2008). Motor proteins are a specific class of MAPs whose role is to
utilize the energy released by ATP hydrolysis to transport cargoes along
microtubules. Animals possess two classes of motor proteins, kinesins and
dyneins. While apparently the Arabidopsis genome does not encode for any
dynein heavy chain gene (Wickstead and Gull, 2007), it possesses a large
variety of genes encoding kinesins, both able to travel towards the plus and
the minus end of microtubules (Gardiner, 2013; Struk and Dhonukshe,
2014).
Organization and dynamics of the actin cytoskeleton
The plant actin cytoskeleton is an array of long polymers of the globular
protein actin, called filaments. Actin filaments possess diverse functions and
in interphase cells are involved in cytoplasmic streaming, intracellular
movement of organelles, and trafficking of secretory and endocytic vesicles
(Hussey et al., 2006; Henty-Ridilla et al., 2013). By acting on these different
processes, actin controls cellular architecture and cell shape, polar growth,
and responses to external stimuli (Wasteneys and Galway, 2003; Hussey et
al., 2006). Actin filaments can form a diffuse meshwork of fine strands or
organize in thick parallel or antiparallel bundles, which serve as tracks for
motor proteins like myosins that hydrolyze ATP to transport organelles or
vesicles moving along the cytoskeletal scaffold (Staiger and Blanchoin,
2006).
Arabidopsis possesses eight actin isoforms that can be divided in two
classes according to their expression pattern: ACT2, ACT7 and ACT8 are
22
vegetative actins, while ACT1, ACT3, ACT4, ACT11 and ACT12 are
preferentially expressed in reproductive tissues (Kandasamy et al., 2009).
Different isoforms vary in their biochemical properties and ability to interact
with actin-binding proteins (ABPs), indicating a marked functional
specificity within each family (Wasteneys and Galway, 2003).
Globular actin (G-actin) binds one ATP nucleotide and polymerizes
forming actin filaments (F-actin). Because of the endogenous asymmetry of
actin monomers and of the lag between incorporation of an ATP nucleotide,
hydrolysis to ADP and release of inorganic phosphate, actin filaments are
polar and have two ends, named the barbed (or plus) end and the pointed (or
minus) end. The barbed end has a higher affinity for actin subunits and
grows faster, while the pointed end does not usually extend and displays a
prevalence of ADP-actin (Hussey et al., 2006).
The actin cytoskeleton needs to continuously rearrange in order to be
functional, and the highly dynamic actin filaments base their rapid turnover
on a mechanism termed stochastic dynamics (Staiger et al., 2009). Unlike
microtubule plus ends, growing ends of actin filaments almost never arrest
their growth or depolymerize, but rather keep elongating at high rates;
disassembly of the filaments does not depend on the loss of monomers from
the minus end as in treadmilling microtubules, but is instead achieved
through stochastic and frequent severing and loss of the aged region of the
filament (Staiger et al., 2009; Henty-Ridilla et al., 2013).
In all eukaryotic organisms, actin dynamics and remodelling strictly
depend on the coordinated activity of multiple classes of ABPs. Plants
possess a great variety of ABPs, diversified by their roles, expression patterns
and biochemical properties (Kandasamy et al., 2009). Their multiple
functions can often be inferred through sequence similarity with ABPs from
other organisms; however, in some cases their specific activities can be
substantially different (Staiger and Blanchoin, 2006).
Profilin is a small ABP that binds monomeric actin and has a central role
in organizing the actin cytoskeleton. Profilin forms 1:1 complexes with most
of the free G-actin monomers present in the cell (which represents over 90%
of the actin pool) and prevents both their incorporation at the pointed ends
of actin filaments and the spontaneous assembly of new filaments (Staiger
and Blanchoin, 2006). Nucleation of actin filaments initiates either freely in
the cytosol or, in most of the cases, on the side of another filament (Hussey
et al., 2006). Both these modes require the action of specific ABPs: formins
are able to bind profilin-actin monomers and generate new filaments, while
the ARP2/3 complex attaches to the side of existing filaments, initiating a
new F-actin branch (Henty-Ridilla et al., 2013). Activity of the ARP2/3
complex is modulated by the SCAR/WAVE complex (Szymanski, 2005). The
SCAR/WAVE complex may be an effector of ROP2, and therefore this could
be a pathway that integrates signals to organize the actin cytoskeleton (Basu
23
et al., 2008). Surprisingly though, while the ARP2/3 complex is essential in
yeast and animals, mutations in Arabidopsis genes encoding for ARP2/3
subunits only determine defects in the shape of trichomes and pavement
cells, suggesting that the complex may have a more limited role in plants
than in animals (Hussey et al., 2006; Mathur et al., 2003a; Mathur et al.,
2003b; Basu et al., 2005).
The rate of actin filament elongation is modulated by several ABPs that
bind with high affinity to barbed ends and block the incorporation of new
monomers. One of these ABPs is the heterodimeric capping protein (CP),
which ensures a small population of short F-actin is maintained in each cell
and regulates the availability of barbed ends controlling the number of
growing filaments (Hussey et al., 2006). CP inactivation by phosphoinositide
lipids or phosphatidic acid releases the growing end of a filament and allows
polymerization to proceed (Staiger and Blanchoin, 2006).
Disassembly of the filaments is driven by the severing activity of several
ABPs in the aged region, where all actin subunits are bound to ADP. The
most prominent severing ABPs are ACTIN DEPOLYMERIZATION
FACTORS (ADFs), also known as cofilins, and villins (Henty-Ridilla et al.,
2013). Activity of ADFs is modulated by several factors, including the ACTIN
INTERACTING PROTEIN 1 (AIP1) plant orthologs. Plant AIP1 has been
shown to enhance the activity of ADFs both in vitro (Allwood et al., 2002)
and in vivo (Augustine et al., 2011). Whereas ADFs remain attached to the
severed filaments but leave the barbed end free to potentially reinitiate
growth, villins and AIP1 cap the filament end, inhibiting further elongation
(Henty-Ridilla et al., 2013). The small fragments resulting from filament
severing mostly undergo depolymerization, leading to single ADP-bound
ADF-actin complexes. The exchange of ADP to ATP on actin subunits is most
likely favoured in plants by the CYCLASE ASSOCIATED PROTEIN (CAP),
which regenerates profilin-actin monomers capable of assembling to the
growing end of a new filament (Staiger and Blanchoin, 2006).
In most plant cells, a large part of the actin filaments organize in robust
bundles or cables that are generally less dynamic and longer-lived than actin
filaments (Wasteneys and Galway, 2003). Such structures can be initiated by
formins or generated by several classes of bundling ABPs, which collect
single filaments giving rise to higher-order structures (Hussey et al., 2006).
The actin filament cross-linkers fimbrins and villins, as well as
ELONGATING FACTOR-1α (EF-1α), can bind actin and bundle it (Wasteneys
and Galway, 2003; Hussey et al., 2006). Binding of fimbrins and villins to
actin filaments also prevents modification by other ABPs, protecting the
bundles from severing and disassembly and making them more stable
(Staiger and Blanchoin, 2006).
24
The plant cytoskeleton during cell division
In addition to their roles in providing a dynamic intracellular scaffold and
controlling cell growth and polarity, the microtubule and actin cytoskeleton
carry out essential functions also during cell division. Plant cells are
surrounded by a rigid cell wall and thus divide based on very different
mechanisms compared to animal cells and require a set of unique
cytoskeletal structures that enable mitosis and cytokinesis to occur.
The first sign of an approaching mitosis in plants is the appearance of the
preprophase band (PPB), a cortical band of microtubules and actin filaments
that mark the site of the future division plane (Fig. 7; Wasteneys, 2002). In
cells dividing symmetrically, the PPB is located at the cell equator just
beneath the plasma membrane and encircles the nucleus, which is centred
before mitosis through the action of actin filaments and microtubules
radiating from the nuclear surface (Rasmussen et al., 2011). Formation of
the PPB begins in the G2 phase of the cell cycle, when cortical microtubule
bundles become restricted to the cell midplane via selective
depolymerization and/or local stabilization (Dhonukshe and Gadella, 2003;
Vos et al., 2004). Accumulation of PPB actin filaments depends on an intact
microtubule cytoskeleton and contributes to constraining width of the PPB,
which becomes narrower as the cell approaches prophase (Rasmussen et al.,
2013).
Several proteins localize to the PPB during prophase and are required for
correct PPB formation. Among these are the regulatory B’’ subunit of the
protein phosphatase 2A complex TONNEAU 2 (TON2)/FASS (Camilleri et
al., 2002), the protein products of the tandem duplicated genes TONNEAU
1A (TON1A) and TONNEAU 1B (TON1B; Azimzadeh et al., 2008), as well as
the microtubule-binding proteins MOR1 (Whittington et al., 2001), CLASP
(Ambrose et al., 2007; Kirik et al., 2007) and MAP65 (Smertenko et al.,
2004). Mutations in TON2/FASS, TON1A/TON1B or MOR1 completely or
partially abolish PPB formation and result in cells dividing in abnormal
orientations (Camilleri et al., 2002; Azimzadeh et al., 2008; Whittington et
al., 2001).
At the onset of prometaphase, once chromosomes are condensed, the
nuclear envelope breaks down and the PPB dissolves leaving the cell cortex
without any microtubules (Müller et al., 2009). A memory of the position of
the PPB at the cell periphery is, however, preserved throughout mitosis as
the cortical division site (CDS) that during cytokinesis guides the orientation
of the newly formed cell division plane (Fig. 7; Rasmussen et al., 2011). After
the PPB is disassembled, a region with very low or no actin accumulation
and flanked by two thin bands of high actin density remains on the cell
cortex at the former location of the PPB and is termed the actin-depleted
zone (Müller et al., 2009). The actin-depleted zone coincides with a zone
25
Figure 7. Cell division in plant cells.
Microtubules (green) at the cell cortex become
restricted to the cell equator creating the
preprophase band (PPB). When the mitotic
spindle is formed, the PPB disassembles
leaving a mark (red semicircles) referred to as
the cortical division site (CDS). As
chromosomes later decondense forming
daughter nuclei (blue), microtubules of the
phragmoplast guide vesicles (white circles) to
the cell division plane marked by the CDS and
assemble the cell plate. The cell plate expands
from the centre of the cell until it fuses to the
plasma membrane (PM) to complete
cytokinesis. Preprophase is illustrated as whole
cell view, while other stages are sections
through the cell mid-plane. Image adapted
from Barr and Gruneberg (2007) with
permission of the publisher.
devoid of the KINESIN CDKA;1ASSOCIATED 1 (KCA1), which starts to
be depleted from the CDS even before
disappearance of the PPB (Vanstraelen et
al., 2006). Localized removal of actin
remodelling proteins and KCA1 from the
plasma membrane involves mechanisms
that are still unknown, but could be
mediated
by
clathrin-mediated
endocytosis (Karahara et al., 2009).
In addition to negative CDS markers,
there are also positive markers of the
CDS during mitosis and cytokinesis: one
of these proteins is TANGLED 1 (TAN1),
which is recruited by PPB microtubules
and persists at the CDS throughout
completion of cytokinesis (Walker et al.,
2007).
Also
the
Ran
GTPase
ACTIVATING PROTEIN 1 (RanGAP1)
localizes to the PPB and stays at the CDS
even after the PPB has disassembled (Xu
et al., 2008). The role of TAN1 and
RanGAP1 is to provide guidance for the
new cell wall that will form during
cytokinesis; accordingly, mutation of
TAN1 or depletion of RanGAP1 cause the
formation of cell wall stubs and
misoriented cell division planes (Cleary
and Smith, 1998; Xu et al., 2008).
Furthermore, analogous defects in cell
division orientation are found in
pok1;pok2 double mutants, defective in
the two kinesins PHRAGMOPLAST
ORIENTING KINESIN 1 (POK1) and
PHRAGMOPLAST
ORIENTING
KINESIN 2 (POK2), which are required
for keeping TAN1 and RanGAP1 at the
CDS during telophase (Müller et al.,
2006). The involvement of two kinesins
suggests that continuous transport via
microtubules may be necessary to
maintain the specific localization of CDS
components.
26
Already prior to complete disassembly of the PPB, cells begin to form the
mitotic spindle, the only mitotic structure whose function is to a large extent
conserved between plants and animals (Rasmussen et al., 2013). As opposed
to animal cells though, plants do not have a centrosome, and thus their
spindles have diffuse, broad poles that contain numerous microtubule foci
(Wasteneys, 2002). During prometaphase highly dynamic microtubules
radiate from each pole, with their plus ends attaching to the chromosomes
via kinetochores or overlapping at the spindle equator with microtubules
coming from the opposite pole (Fig. 7). These interactions align the
chromosomes during metaphase and, together with a cage of actin bundles
that surround the spindle and connect it to the cell periphery, help
stabilizing the spindle structure (Rasmussen et al., 2011). During mitosis
spindle orientation sometimes changes with respect to the pre-existing PPB;
however, as long as reorientation is subtle, it does not determine any
alteration in the final division plane, as the newly forming cell wall is later
able to track back to the CDS and align to it (Rasmussen et al., 2013).
At the anaphase-telophase transition, once chromosomes have been
pulled towards the poles and start to decondense, remnants of the
disassembling mitotic spindle begin to form the phragmoplast in the central
region of the cell, between the two sets of daughter chromosomes (Fig. 7;
Wasteneys, 2002). The spindle microtubules maintain their polarity and are
joined by new microtubules emanating from the poles and by newly
polymerized actin filaments. The phragmoplast consists of two compact
cylindrical bundles of parallel microtubules and actin filaments that face
each other with opposite polarities at the plane of cell division (Jürgens,
2005). Plus ends of the phragmoplast microtubules interdigitate, while actin
filaments do not overlap (Jürgens, 2005). Microtubules that form the
phragmoplast direct the delivery of Golgi-derived vesicles to the plane of cell
division, where the vesicles fuse synthesizing a transient membrane
compartment called cell plate. The cell plate initiates as a disc at the centre of
the cell division plane and progressively expands laterally and matures,
giving rise to the new cell wall that separates the two daughter cells (Fig. 7;
Samuels et al., 1995; Jürgens, 2005).
As the cell plate develops, excessive membrane is removed from its centre
by endocytosis (Samuels et al., 1995; Seguí-Simarro et al., 2004) and
microtubules begin disassembling in the central region of the phragmoplast
and translocating to the outer edges, where new actin filaments are
polymerized as well. This centrifugal growth drives the cell plate towards the
CDS, where eventually cell plate and parental membrane fuse completing
cytokinesis (Jürgens, 2005). Microtubules and F-actin, in addition to the
already mentioned TAN1 and RanGAP1, may have a role in directing the
phragmoplast to the CDS (Rasmussen et al., 2013). Moreover, cell plate
maturation and attachment to the mother cell wall is controlled by several
27
additional factors, including the microtubule-associated protein AUXIN
INDUCED IN ROOTS 9 (AIR9; Buschmann et al., 2006), the
adaptor/coatomer-like protein TPLATE (Van Damme et al., 2006), and the
extensin ROOT-SHOOT-HYPOCOTYL-DEFECTIVE (RSH; Hall and
Cannon, 2002). These proteins localize to the cell plate and/or the CDS
shortly before fusion of the two membranes, and mutation of RSH or knockdown of TPLATE cause misoriented and incomplete cell walls, implicating
them in the final steps of cytokinesis (Hall and Cannon, 2002; Cannon et al.,
2008; Van Damme et al., 2006; Van Damme et al., 2011). Recently,
downregulation of the TPLATE interactor TML has also been shown to
induce ectopic accumulation of the KNOLLE cell plate syntaxin at the CDS
and plasma membrane, further supporting a role for the TPLATE complex in
correct maturation and fusion of the cell plate (Gadeyne et al., 2014). As cells
complete division and enter interphase, microtubules first appear as a
transient array radiating from the nucleus towards the cell periphery and
soon afterwards repopulate the cell cortex and associate with the plasma
membrane (Wasteneys, 2002).
The microtubule-associated protein CLASP
CLASP1 and CLASP2 are two mammalian MAPs that have been identified as
interactors of the microtubule-binding protein CLIP170 (Akhmanova et al.,
2001). They belong to the class of +TIPs and are essential for controlling the
attachment of microtubule plus ends to various cellular structures both in
interphase and during cell division (Lansbergen et al., 2006; Maiato et al.,
2005). CLASPs stabilize subsets of microtubules by selectively binding to
their plus ends in response to positional cues and by promoting pause state
or rescue, thus effectively reducing microtubule dynamicity (Galjart, 2005;
Sousa et al., 2007; Al-Bassam et al., 2010). During mitosis instead, CLASPs
regulate kinetochore fibre dynamics by adding tubulin subunits at
microtubule plus ends (Maiato et al., 2005). CLASPs may also be hubs that
integrate cytoskeletal signalling, as they have been shown to associate
directly with actin filaments (Tsvetkov et al., 2007) and to be regulated by
processes dependent on Rho GTPases (Lansbergen et al., 2006).
Arabidopsis only possesses one CLASP gene and analyses of clasp loss-offunction mutants have shown that, similar to its non-plant orthologs, CLASP
in plants functions in promoting microtubule stability (Ambrose et al., 2007;
Kirik et al., 2007). Consistent with these findings, clasp mutants are
hypersensitive to microtubule-depolymerizing drugs, and overexpression of
CLASP leads to strong bundling of microtubules (Ambrose et al., 2007; Kirik
et al., 2007).
In plants, CLASP is constitutively expressed at low levels in all tissues
(Ambrose et al., 2007; Kirik et al., 2007). During mitosis, CLASP localizes to
28
the PPB, accumulating almost exclusively at the cell edges intersected by the
band (Ambrose et al., 2011), and is present on spindles and phragmoplasts
(Ambrose et al., 2007; Kirik et al., 2007). In newly divided root cells, CLASP
is enriched along the apical and basal cell sides, while it becomes distributed
along longitudinal edges in cells undergoing elongation (Ambrose et al.,
2011). CLASP localization on cortical microtubules is not uniform, but rather
consists of distinct domains at the cell periphery (Ambrose et al., 2011). In
plants, the CLASP protein labels the full length of microtubules, and despite
being a +TIP shows only a weak enrichment at the plus end; there it maps
just behind the +TIP EB1b (Ambrose et al., 2007; Kirik et al., 2007).
A prominent role of the Arabidopsis CLASP is to coordinate the
interaction of microtubules with the plasma membrane: CLASP mediates
close association of cortical microtubules with the cell cortex, and in mutants
defective for CLASP the microtubules detach more frequently from the
plasma membrane and subsequently form hyper-parallel and more
prominent bundles (Ambrose and Wasteneys, 2008). Another role for
CLASP at the cell periphery is to promote the growth of cortical microtubules
around sharp cell edges, counteracting barrier-induced microtubule
catastrophes (Ambrose et al., 2011). Enrichment of CLASP along specific cell
edges allows the extension of microtubules into adjacent cell faces and the
formation of transfacial bundles in meristematic root cells (Ambrose et al.,
2011). Regulation of local CLASP accumulation at cell edges can thus
modulate cell-wide organization of the cortical microtubule array, including
formation and orientation of the PPB (Ambrose et al., 2011).
Recently CLASP has also been connected to tethering of endosomal
compartments to cortical microtubules through direct interaction with the
retromer-complex component SORTING NEXIN 1 (SNX1; Ambrose et al.,
2013). SNX1 is involved in endosomal recycling of membrane proteins,
including the auxin transporter PIN2 (Jaillais et al., 2006). CLASPdependent recruitment of SNX1 vesicles to cortical microtubules modulates
targeting and abundance of PIN2 at the plasma membrane (Ambrose et al.,
2013). A role for CLASP in regulating PIN2 polarity remains controversial
and awaits further analyses (Brandizzi and Wasteneys, 2013).
Consistent with an effect of CLASP on PIN2 localization and auxin
transport, clasp mutants display an array of auxin-related defects: plants
have reduced apical dominance and abundant lateral roots, roots are shorter
and have smaller apical meristems, aberrant cellular organization, and
delayed gravitropic responses (Ambrose et al., 2013). Furthermore, root and
hypocotyl cells of clasp mutants are shorter, there are fewer cells in the root
meristem, rosette leaves are twisted, pavement cells are less interdigitated
and trichomes have less branches, indicating that CLASP in multiple ways
affects cell expansion and morphogenesis as well as cell division (Ambrose et
al., 2007; Kirik et al., 2007). Interestingly, trichome branches of clasp
29
mutants are also misoriented with respect to the leaf proximo-distal axis
(Kirik et al., 2007). This observation, together with the more frequent
occurrence of PPBs that are misaligned relative to the cell axis in clasp
mutants (Ambrose et al., 2007), suggests a potential role for CLASP in cell
and planar polarity.
Patterning of the root and leaf epidermis
The root and leaf epidermis of Arabidopsis are models for studying planar
polarity in plants. In addition, they are optimal systems also to analyze the
specification of cell fate in the context of a tissue layer (Ishida et al., 2008).
During their development, root and leaf epidermal cells are faced with the
option of whether to differentiate or not specialized structures, root hairs
and trichomes respectively. Cells do not choose their fate individually, but
rather receive specific signals that coordinate patterning of cell fate over the
whole tissue, transmitting positional cues and exploiting cell-to-cell
communication (Schiefelbein et al., 2009; Hülskamp, 2004).
In plants as in other organisms, body pattern is organized during
embryogenesis, where the apical-basal body axis is established, principal
tissues and organs are formed, and different cell types are specified (Jürgens
et al., 1991). This also holds true for epidermal cell patterning, which is set
up in the embryo and then influences postembryonic development, when
fates are translated into morphological outputs (Berger et al., 1998a). In
roots, fate patterning generates a characteristic alternation of parallel cell
files that produce either hair or non-hair cells (Galway et al., 1994), while on
the leaf surface trichomes occur almost never in clusters but rather initiate at
a fixed distance from each other (Hülskamp, 2004).
The longitudinal files that align over the root surface are derived from 16
meristematic initials that attain a specific fate according to the position they
occupy with respect to the underlying layer of 8 cortical cells (Dolan et al.,
1993). Cells located over the anticlinal walls of two cortical cells will usually
grow a hair and are thus referred to as hair (H) cells, or trichoblasts; on the
other hand, the cells lying over the outer periclinal wall of a single cortical
cell do not generally grow any hairs and are referred to as non-hair (N) cells,
or atrichoblasts (Fig. 8; Dolan and Costa, 2001). Cell files propagate by
transversal cell divisions, and files of hair-forming trichoblasts are normally
separated by either one or two files of hairless atrichoblasts (Dolan et al.,
1994). Rare occurrence of longitudinal cell divisions can alter the number of
epidermal cell files and possibly the fate of daughter cells; changes in
patterning can in fact still take place postembryonically and cells are
constantly assessing the positional information they receive from the
underlying cortex (Berger et al., 1998a; Costa and Shaw, 2006).
30
Figure 8. Cellular organization and epidermal
cell differentiation in the root of Arabidopsis
thaliana. Coloured transverse section of a root
displaying epidermal hair (H) cells that lie over the
cleft between two cortical cells in red and non-hair
(N) cells located on top of one single cortical cell in
blue.
Both the positional cues that direct root hair fate acquisition and the
intercellular communication that spaces trichomes over the leaf surface
converge onto a similar set of transcription factors that organize epidermal
patterning both in the root and in leaves (Fig. 9). The central component of
this pathway is a protein complex capable of activating the homeobox
transcription factor GLABRA 2 (GL2), which leads to non-root-hair and
trichome cells (Di Cristina et al., 1996, Masucci et al., 1996, Rerie et al.,
1994). Expression of GL2 represses transcription of the hair-initiating gene
RHD6 (Menand et al., 2007) and of PHOSPHOLIPASE Dζ1 (PLDζ1; Ohashi
et al., 2003), a gene controlling root hair initiation and morphogenesis. The
core components of the activator complex have been uncovered over the
years, and include the WD40-repeat protein TRANSPARENT TESTA
GLABRA 1 (TTG1; Galway et al., 1994), the homologous bHLH transcription
factors GLABRA 3 (GL3) and ENHANCER OF GLABRA3 (EGL3; Bernhardt
et al., 2003), and the R2R3 MYB transcription factor WEREWOLF (WER;
Lee and Schiefelbein 1999) or GLABRA 1 (GL1; Oppenheimer et al., 1991).
WER and GL1 are tissue-specific components and are expressed exclusively
in roots and leaves, respectively.
A group of proteins that include CAPRICE (CPC; Wada et al., 1997),
TRIPTYCHON (TRY; Schellmann et al., 2002) and ENHANCER OF TRY
AND CPC 1 (ETC1; Kirik et al., 2004) have the role of inhibiting the activity
of the complex (Simon et al., 2007; Wester et al., 2009). Synthesis of these
small MYB-like DNA-binding proteins takes place in N and trichome cells
and they later move to adjacent hair and trichome-less cells where they
compete with WER or GL1 for binding to the bHLH transcription factors
(Wada et al., 2002; Kurata et al., 2005). Lack of a transcriptional activation
domain in CPC, TRY and ETC1 means that whenever they bind to GL3/EGL3
the complex does not activate GL2 transcription, thus determining root-hair
31
or trichome-less fate (Ishida et al., 2008). In a mechanism of lateral
inhibition aimed at stabilizing fate determination and patterning in the
epidermis, transcription of CPC, TRY and ETC1 is induced by the activator
complex, which therefore both supports non-hair/trichome fate in a cell and
promotes hair/no-trichome fate in its neighbours (Koshino-Kimura et al.,
2005, Ryu et al., 2005). In addition to this, transcription of GL3 and EGL3 is
repressed by the activator complex in non-hair cells and stimulated by CPC
and TRY in hair cells; once expressed, the bHLH proteins move to non-hair
cells where they reinforce fate selection by generating more activator
complexes (Bernhardt et al., 2005). In root epidermal cells, an additional
level of feedback regulation is provided by the MYB23 gene, encoding a
transcription factor closely related to WER (Kang et al., 2009). MYB23 is
able to substitute for WER in the activator complex, which in turn can
induce expression of MYB23, therefore generating a positive loop that
stabilizes accumulation of the patterning determinants (Kang et al., 2009).
Figure 9. Simplified representation of the gene networks controlling patterning of the root
and leaf epidermis. The activator complex including the WD40-repeat protein TRANSPARENT TESTA
GLABRA 1 (TTG1), the homologous bHLH transcription factors GLABRA 3 (GL3) and ENHANCER OF
GLABRA3 (EGL3), and either the MYB transcription factor WEREWOLF (WER) or its homolog GLABRA 1
(GL1) promotes expression of the GLABRA 2 (GL2) homeobox transcription factor and induces differentiation
into non-hair (N) cells or trichome cells. The activator complex also activates expression of the CAPRICE
(CPC) or TRIPTYCHON (TRY) MYB-like DNA-binding proteins, which move to neighbouring cells and
compete with WER or GL1, respectively, for binding to GL3/EGL3. In root hair (H) cells, a positional cue from
the receptor-like kinase SCRAMBLED (SCM) represses WER expression. Image adapted from Ishida et al.
(2008) with permission of the publisher.
In trichome patterning, the so-called activator-depletion model described by
Bouyer et al. (2008) provides an additional option to the activator-inhibitor
model presented so far. The authors show that the activator TTG1 is
ubiquitously expressed in the leaf epidermis and its protein product is
capable of moving between cells. The GL3 transcription factor is present at
32
high concentrations in trichome cells and can interact directly with TTG1
and trap it in the nucleus, efficiently depleting a positive regulator of
trichome initiation from cells adjacent to trichomes (Balkunde et al., 2011).
This mechanism of lateral inhibition does, however, not exclude functioning
of the core patterning pathway and is instead likely to operate in parallel
with it (Pesch and Hülskamp, 2009; Balkunde et al., 2011). Moreover, a
similar process has been recently proposed also for epidermal cells in roots,
where CPC, an inhibitor of non-hair fate, could get trapped by EGL3 in H
cells, thus ensuring accumulation of a promoter of H fate and providing
stability to cell fate patterning (Kang et al., 2013).
Upstream of the core patterning pathway, specification of cell fate in the
root epidermis relies on signals from the underlying cortical layer. The
molecular nature of these positional cues and how exactly they are generated
and transmitted to epidermal cells still remains elusive; however, they likely
require signalling through the receptor-like kinase SCRAMBLED (SCM;
Kwak and Schiefelbein, 2007). SCM action inhibits transcription of WER
preferentially in H cells, on account of the higher amount of SCM in this
position (Kwak and Schiefelbein, 2008). This differential accumulation is
achieved through inhibition of SCM expression in N cells by the activator
complex, which in this manner negatively feeds on its own inhibitor and
gives additional robustness to cell fate decisions (Kwak and Schiefelbein,
2008). Additional factors non-cell-autonomously contribute to epidermal
fate specification prior to the patterning gene network. The zinc finger
protein JACKDAW (JKD) modulates epidermal patterning by acting from
the underlying cortical layer and asymmetrically distributing cell fate
determinants in an SCM-dependent manner (Hassan et al., 2010). As a
consequence, in jkd mutants the fate of epidermal cells is less tightly
connected with their position relative to the underlying cells, and ectopic
hairs and non-hairs form more frequently (Hassan et al., 2010). The heat
shock transcription factor SCHIZORIZA (SCZ) suppresses epidermal fate in
cortical cells and controls cell fate separation in ground tissue; mutants
defective in SCZ develop root hairs also from the cortical cell layer and,
moreover, display perturbations in the establishment of epidermal hair and
non-hair cell fates (Mylona et al., 2002; ten Hove et al., 2010).
Patterning of epidermal cell fate in Arabidopsis thaliana has been
extensively studied over the past 20 years, and many of the molecular
mechanisms and transcriptional networks that control cell fate specification
in the root and leaf epidermis have been elucidated (Schiefelbein et al.,
2014). However, new players are continuously discovered and challenge the
present knowledge about the establishment of cell differentiation patterns in
the epidermis. Adding new components to these pathways and investigating
their role will provide a clearer and more complete picture of the complex
regulation behind fate patterning.
33
Aim
The aim of this study was to employ polar initiation of Arabidopsis root hairs
as a model system to identify new components of the plant planar polarity
pathway. The work focussed on characterizing the novel planar polarity actor
SABRE and analyzing its functions in cell division orientation and
stabilization of microtubule arrays. Additional research concentrated on the
role that the actin cytoskeleton and a modulator of its organization have in
planar polarity of root hair positioning. Finally, further investigation
addressed the connection between planar polarity establishment and cell fate
patterning in the root epidermis.
34
Results and Discussion
Root hair positioning in Arabidopsis thaliana provides an easy-to-analyze
phenotype for studying the establishment of planar polarity in plants.
Genetic dissection of the mechanisms that control this process has helped
outlining a pathway that describes how plants set up and maintain polar hair
initiation (Masucci and Schiefelbein, 1994; Fischer et al., 2006; Ikeda et al.,
2009). Nonetheless, we still know relatively little about how polarity cues are
generated and translated into morphological outputs. This prompted us to
investigate the presence of additional players involved in root hair planar
polarity. To this end, we performed a genetic screen and isolated several
mutants affected in the polar outgrowth of hairs on their root epidermis. One
of the mutants identified was named kreuz und quer (kuq) [German for
criss-cross] on account of its intricate placement of hairs that emerged at
very diverse positions along trichoblasts, displaying clear defects in their
polar positioning (Paper I, Fig. 1a-c).
The kreuz und quer mutant
kreuz und quer is mutated in the SABRE gene
Positional cloning of the kuq mutation revealed that it was located in the
large SABRE (SAB) gene and consisted of a single nucleotide deletion likely
to introduce a premature stop codon in the last sixth of the coding sequence
(Paper I, Fig. 2). Analysis of T-DNA insertion lines in the SAB gene revealed
homozygous mutants with phenotypes identical to those of kuq and unable
to complement the kuq mutation, thus confirming that the planar polarity
defects of kuq were caused by disruption of SAB function (Paper I, Fig. 3a-e).
Reverse transcription PCR (RT-PCR) analysis of three sab mutant lines
confirmed that they did not produce any full-length SAB transcript (Paper I,
Fig. 3f-h). This finding, together with the observation that 9 out of 11 T-DNA
insertion lines analyzed had indistinguishable phenotypes, suggested that
they were null alleles. We thus adopted one of these lines, named sab-5, for
further analyses.
Two of the analyzed T-DNA insertion lines in the SAB gene displayed
phenotypes similar to, but weaker than kuq and the other sab alleles. One of
them carried a T-DNA insertion in the promoter region of SAB, suggesting
that it might affect SAB expression rather than protein functionality. In the
other line the T-DNA was inserted only 300 nucleotides away from the end
of the 7824 nucleotides coding sequence, indicating a hypomorphic mutation
that might be producing a truncated, yet still partially functional version of
the SAB protein (Paper I, Fig. 2 and Fig. 3a,b,e). These two weak alleles have
35
not been further analyzed yet, but in the future could prove valuable tools for
dissecting SAB function: in addition to opening the way for studies on
dosage-dependence of SAB function and for serial-deletion analyses, they are
also the only two self-fertile sab mutants identified in this study and could be
used in genetic screens for SAB interactors.
Mutants defective in SAB have first been described in 1993 (Benfey et al.,
1993) and were isolated in a genetic screen for genes affecting root
morphogenesis. sab-mutant seedlings displayed shorter roots with increased
diameter, and more detailed analyses revealed that their increased radial
expansion when compared to the wild type was mainly a consequence of
defects in anisotropic growth of the cortical layer (Benfey et al., 1993;
Aeschbacher et al., 1995). Pharmacological and genetic interference with
ethylene biosynthesis or perception could partially rescue the sab phenotype
and this led the authors to hypothesize that SAB was involved in limiting
radial cell expansion by antagonizing ethylene action (Aeschbacher et al.,
1995). Antagonistic interaction of SAB with ethylene signalling was also
suggested recently in a study that identified sab mutants as hypersensitive to
phosphate starvation (Yu et al., 2012). Both studies report that ethylene
biosynthesis is not altered by mutations in SAB. However, the molecular
nature of the interplay between SAB and this hormone remains elusive and
requires further investigation.
Planar polarity defects of sab mutants
Quantitative analysis of root hair positioning in kuq and other sab mutants
revealed an irregular distribution of hair position compared to wild-type
seedlings, with hairs initiating more frequently both at the very basal end
and towards the middle of trichoblasts (Paper I, Fig. 1a-c and Fig. 3c-e). We
observed similar defects in the localization of ROPs at hair initiation sites
prior to root hair emergence: patches of ROP proteins accumulated either at
the basal-most end of the cells or at a more apical position with respect to
the wild type (Paper I, Fig. 1d-g and Fig. S2a-d). ROPs are the earliest
markers of polar hair initiation (Molendijk et al., 2001; Jones et al., 2002),
and these findings are consistent with an involvement of SAB in planar
polarity establishment upstream of ROP positioning.
The root-hair and ROP phenotypes of sab mutants are intriguing
concerning their display of both a basal and an apical shift in hair initiation.
Most of the mutants with planar polarity defects described so far in plants
have either a basal or an apical shift: for instance enhanced biosynthesis or
signalling of either ethylene or auxin determine hyperpolarization of root
hair initiation, while defects in perception of the hormones shift hair
outgrowth towards a more apical position (Masucci and Schiefelbein, 1994;
Grebe et al., 2002; Fischer et al., 2006; Ikeda et al., 2009). The fact that
36
mutations in SAB provoke a shift in both directions suggests that the effect of
this gene cannot be limited to a linear interaction with one of the two main
hormone pathways. This hints towards a more complex involvement of SAB
in planar polarity establishment, possibly through multiple contributions to
independent pathways.
In addition to the positioning of hairs in the root epidermis, we analyzed
the alignment of trichomes on leaves of sab mutants as a second system to
study polar orientation of cells within the plane of a tissue layer. The
proximal side stem, which in wild type aligns to the proximo-distal axis of
the leaf (Folkers et al., 1997), had a much more variable orientation in both
kuq and sab-5 mutants (Paper I, Fig. 1h-j and Fig. S1e,f). A similar
misalignment had only been reported for mutants defective in the MAP gene
CLASP (Kirik et al., 2007), and indicates that the effect of SAB on planar
polarity is not limited to the root but extends to aerial tissues. Trichoblasts
align to an auxin gradient in the root; however, a similar uniform auxin
gradient over the whole leaf surface has not yet been described (Mattsson et
al., 2003). Auxin certainly has instructive roles in leaf initiation and
vascularization (Leyser, 2005; Scarpella et al., 2006), and it will be
interesting to investigate if it also contributes to planar polarity of leaf
trichomes or whether this tissue relies on different, yet to be identified
polarizing cues. The discovery that SAB functions in establishment of
polarity in both the root and the leaf epidermis suggests that the
mechanisms are at least in part conserved between the two tissues.
Cell polarity defects of sab trichomes
When observing the morphology of leaf trichomes in kuq and sab-5 mutants,
we noticed a higher frequency of trichomes with only two branches, and a
higher incidence of trichomes with abnormal distance between the two
branching points and/or aberrant orientation of the branches with respect to
the leaf surface (Paper I, Fig. 1k-m and Fig. 5a). Initiation of trichome
branches depends on the microtubule cytoskeleton (Mathur et al., 1999), and
these defects indicated that SAB could act on microtubules to control the
correct cell polarity of leaf trichomes. Trichome branching of sab mutants is
not as severely inhibited as in seedlings treated with microtubuledepolymerizing drugs (Mathur et al., 1999) or mutants defective in the
assembly of tubulin subunits (Kirik et al., 2002a; Kirik et al., 2002b), but
rather resembles mutants affected in genes responsible for the microtubule
stabilization or severing and realignment (Kirik et al., 2007; Burk et al.,
2001). Therefore the role of the SAB gene might be in reorganization rather
than assembly of the microtubule cytoskeleton.
37
The SAB protein
Homologs of the SAB protein
The SAB gene encodes a protein of 2607 amino acids with a predicted
molecular weight of 290 kDa. The Arabidopsis genome harbours a gene for
one other protein of similar size with high sequence similarity to SAB,
named KINKY POLLEN (KIP) after the defects in pollen tube elongation of
mutants lacking its function (Procissi et al., 2003). Similarly, a Zea mays
homolog of SAB, the ABERRANT POLLEN TRANSMISSION 1 (APT1) gene,
is involved in growth of pollen tubes after pollen germination (Xu and
Dooner, 2006). Whereas APT1 is only expressed in mature pollen and its
loss-of-function does not affect any other tissues, KIP is required for tip
growth of both pollen tubes and root hairs (Procissi et al., 2003; Xu and
Dooner, 2006). Pollen tubes of kip mutants are twisted and branched, and
root hairs are shorter and thicker. Defects in root hair elongation are
sometimes related to incorrect functionality of the actin cytoskeleton
(Baluška et al., 2000; Ringli et al., 2002), and hair waving or branching is
normally caused by interference with the microtubule cytoskeleton (Bibikova
et al., 1999) or ROP signalling (Parker et al., 2000). Thus, although actin
filaments and microtubules of kip pollen tubes are reported not to differ
from wild-type (Procissi et al., 2003), it is difficult to rule out an
involvement of KIP in cytoskeletal organization.
The morphology of sab pollen tubes and root hairs does not differ from
wild type, and on the other hand kip seedlings do not display the strong
growth impairment of sab mutants (Procissi et al., 2003). However, despite
apparently controlling unrelated cellular processes, SAB and KIP seem to at
least partially interact genetically because sab;kip double mutants have more
severe defects both in seedling development and tip growth compared to the
two single mutants (Procissi et al., 2003).
The expression pattern of SAB and KIP is also relatively similar, with
mRNA of both genes expressed in all plant tissues and KIP enriched in tipgrowing cells (Procissi et al., 2003). The low and mostly homogeneous levels
of SAB expression are in agreement with previous findings (Aeschbacher et
al., 1995), with data from Genevestigator (Zimmermann et al., 2004), and
with a recent report using quantitative real-time PCR to analyze levels of
SAB transcripts (Yu et al., 2012). Transcriptional fusion of SAB regulatory
sequences with GUS further confirmed SAB expression in all the analyzed
tissues and revealed strongest signals in hypocotyl, cotyledons and leaves
(Yu et al., 2012).
Intriguingly, either one or two proteins with similar size and high
sequence similarity to SAB are present in most plant species whose genome
has been sequenced (Paper I, Fig. 4). SAB-related proteins can also be found
38
in most other eukaryotes, even distantly related ones such as yeasts and
primates. Sequence homology among plants is distributed over the whole
SAB protein, while in non-plant species the similarity is restricted to two
regions of about 700 and 300 amino acids in the central and C-terminal
parts of the protein. Such level of conservation strongly points towards the
requirement for SAB in an essential process, one needed for organisms with
very diverse organization and morphology. The two regions of homology
have not been characterized nor are predicted to have any catalytic or
structural role, and will indeed be primary targets for understanding the
function of the SAB protein. In addition, the presence of these sequences in
diverse eukaryotes could allow studies on protein conservation and
evolution, performed by exchanging domains between different species and
testing for protein functionality.
Unfortunately, apart from KIP and APT1 none of the SAB-related proteins
have been functionally characterized. SAB does not contain any predicted
functional domains or conserved motifs, and the only hint on the role of a
SAB-related protein comes from the SAB human homolog KIAA0100, which
produces antigens overexpressed in several types of cancer cells (Song et al.,
2006; Zhou et al., 2008).
Subcellular localization of the SAB protein
Analyses with bioinformatic tools gave a range of predictions on the
subcellular localization and membrane topology of the SAB protein. All of
the algorithms we employed agreed on the presence of a transmembrane
domain close to the protein’s N-terminus and following a short stretch of
cytosolic amino acids. This indicates that SAB is likely to be a
transmembrane protein. Nevertheless, predictions are in disagreement
concerning the total number of putative transmembrane domains and
consequently the localization of the protein’s C-terminus. The presence of
SAB peptides among membrane-associated proteins isolated from
Arabidopsis suspension cells has been previously reported and would
support SAB membrane localization (Benschop et al., 2007). On the other
hand, different studies have suggested that both KIP and SAB, as well as
their yeast and Drosophila homologs, do not contain membrane spanning
domains but rather a signal peptide directing them towards the secretory
pathway and extracellular matrix (Procissi et al., 2003). This discrepancy
may be attributed to the evolution of algorithms for membrane topology
predictions, which are likely to be more accurate at the time of our analysis.
Additionally, fluorescent fusions of C-terminal fragments of the maize APT1
protein have been shown to localize to Golgi bodies, suggesting that the APT1
protein and its homologs may be targeted to these organelles (Xu and
Dooner, 2006). However, evidence for localization of the full-length APT1
39
protein in stably transformed plants is lacking and thus these observations
are not very informative.
In order to directly elucidate the subcellular localization of the SAB
protein, we attempted to clone the SAB gene with the aim of fusing it to
fluorescent proteins and expressing the resulting constructs in plants.
Unfortunately, the extremely large size of the SAB genomic region (about 20
kb including the predicted regulatory sequences) hampered the success of
conventional molecular cloning. We thus adopted the alternative strategy of
recombination-mediated genetic engineering (recombineering; Zhou et al.,
2011) to fuse SAB with three tandem copies of the gene encoding the bright
fluorescent protein Ypet and transformed plants with the tagged SAB within
its genomic context. This allowed SAB expression under the control of its
endogenous regulatory sequences, circumventing problems related to gene
overexpression and providing a reliable read-out of its endogenous
expression pattern. In order to further identify any possible effect of the
fluorescent tag on localization of the SAB protein, we introduced the tag at
either end of the gene.
Both SAB-3xYpet and 3xYpet-SAB were expressed at very low levels in all
cell types of the root meristem and in elongating and differentiating
epidermal cells (Paper I, Fig. 8h-l and Fig. 9a,b,v,w). The protein fusions
localized to the plasma membrane, to unidentified endomembrane
compartments and to the nuclear envelope in interphase cells, whereas
during cell division they associated closely with PPBs and mitotic spindles
and labelled the cell plate and plasma membranes of the daughter cells
(Paper I, Fig. 9a-u). These findings are in agreement with the prediction that
SAB could be a membrane-associated or transmembrane protein, and
disprove the hypotheses of a secreted or primarily Golgi-localized protein.
Additionally, the observation that Ypet fusions at the N- and C-terminus
display similar fluorescence intensity is strongly supportive of orientation of
both ends of the SAB protein in the cytoplasm; fluorescent proteins are in
fact sensitive to acidic conditions and the intensity of their emission would
be reduced if they were exposed to the low pH of the root apoplastic space
(Swarup et al., 2004). Expression of SAB in all cell types, including cells
initiating root hairs, implies that SAB may act directly on polar root hair
initiation in a cell-autonomous way. We however cannot exclude non-cellautonomous effects, and expression of SAB under the control of cell-type
specific promoters or generation of mosaics of SAB expression would allow
to determine whether SAB also contributes to planar polarity establishment
in a non-cell-autonomous manner. It is interesting to note that SAB
localization at the plasma membrane is strongly enriched in the apical and
basal domains of root meristematic cells. This accumulation indicates the
presence of a mechanism for polarization of SAB distribution immediately
after cell division and supports an involvement of SAB in the generation or
40
maintenance of apical-basal polarity biases in root cells. Finally, SAB is not
evenly spread on membranes but rather preferentially confined to patches,
dots with relatively stronger signal intensity. Such a pattern suggests either
the presence of a yet unknown mechanism for SAB accumulation in specific
membrane compartments or association of SAB to discrete structures at the
cell cortex, although their identity remains elusive. Uncovering the nature of
SAB-labelled endomembrane compartments, clarifying mechanisms and
function of SAB membrane localization and revealing the role of SAB in
proximity to and in association with mitotic structures present challenges for
future functional studies on SAB localization.
SAB interaction with the CLASP gene
SAB and CLASP interact genetically
Since analysis of the SAB protein and its localization did not provide many
hints about the role of SAB in plants, we set out to search for possible genetic
interactors that could reveal SAB functions. Mutants defective in the MAP
gene CLASP are the only ones so far characterized for aberrant trichome
orientation and branching similar to sab mutants. Our analyses of sab;clasp
double mutants revealed a strong effect on trichome branching and overall
development of seedlings and plants, suggesting synergistic interaction
between SAB and CLASP (Paper I, Fig. 5a,b and Fig. S3a-c). This prompted
us to investigate whether CLASP could also be involved in planar polarity of
root hair positioning. Indeed, we uncovered that loss of CLASP function
results in a basal shift of both hair initiation and polar ROP positioning
(Paper I, Fig. 5c-h).
SAB also has a role in PPB orientation
The roles of CLASP in plants comprise microtubule stabilization (Ambrose et
al., 2007; Kirik et al., 2007) and organization of cortical microtubule arrays
(Ambrose and Wasteneys, 2008; Ambrose et al., 2011), including orientation
of the PPB microtubules at the cortex of dividing cells (Ambrose et al.,
2007). We thus employed tubulin immunolocalization and live imaging to
analyze PPBs and other mitotic structures in sab and clasp mutants. Our
observations revealed that kuq- and sab-5-mutant PPBs were often
misaligned with respect to the cell axis, and that this defect was accompanied
by aberrant orientation of mitotic spindles, phragmoplasts and cell division
planes (Paper I, Fig. 6a-q and Fig. S3d-h). Live imaging allowed us to assess
that mutation of SAB affected positioning of the PPB in the initial phases of
cell division, and that the orientation defects were then maintained in the
same cell until formation of the cell division plane (Paper I, Fig. 6c,d and
41
Supplementary Movies 1 and 2). These findings unveiled a role for SAB in
cell division already at the stage of PPB formation, and suggested that SAB
acts on the initial cell division plane alignment and not on maintenance of
this alignment during mitosis and cytokinesis.
PPB formation is driven by restriction of interphase cortical microtubule
bundles to the cell equator, and its correct set up requires a group of proteins
that localize to the cell division plane during prophase (Dhonukshe and
Gadella, 2003; Vos et al., 2004; Rasmussen et al., 2013). Mutations in the
TON2/FASS or TON1A/TON1B genes abolish PPB formation and determine
strongly altered cellular organization and positioning of cell division planes
(Camilleri et al., 2002; Azimzadeh et al., 2008). SAB function is not
equivalent to that of TON2/FASS or TON1A/TON1B, because mutation of
SAB does not impair assembly of the PPB but rather its orientation.
Similarly, SAB is not analogous to proteins that define the cortical division
site like TAN1 or RanGAP1: these markers localize to the PPB and stay at the
CDS after PPB disassembly to guide growth of the cell plate towards the
parental plasma membrane (Cleary and Smith, 1998; Walker et al., 2007; Xu
et al., 2008). First of all SAB does not localize to the PPB, and secondly
misoriented cell division planes in sab mutants are the consequence of
misoriented PPBs, rather than being caused by lack of guiding signals from
correctly aligned PPBs.
On the other hand, mutants defective in the gene encoding the MAP
katanin display a phenotype more reminiscent of the one observed in sab
and clasp mutants: fra2 and lue1 mutants of katanin have correctly oriented
PPBs but a high frequency of oblique spindles and phragmoplasts, resulting
in oblique cell walls and disordered cell organization (Panteris et al., 2011).
Interestingly, the proportion of misaligned spindles in katanin mutants is
much higher than the proportion of misoriented phragmoplasts, supporting
the notion that phragmoplasts are often able to track back to the CDS and
align to it (Rasmussen et al., 2013). No correction of phragmoplast
orientation takes place in sab mutants though, confirming that cell division
planes are misaligned already at the stage of CDS establishment. Similar to
CLASP, katanin colocalizes with PPB, spindle and phragmoplast
microtubules (Panteris et al., 2011) and thus differs from SAB also in this
regard. Nonetheless, resemblance of sab phenotypes to phenotypes of clasp
and katanin mutants points towards a possible role also for SAB in
microtubule modification or organization.
SAB is not involved in mitotic progression
Live imaging of dividing cells additionally offered us the opportunity to
compare the timing of mitosis and cytokinesis between wild type and sab-5
mutants. Advancement through mitotic phases was similar in all the cell
42
division events that we followed, in both wild-type and sab-5 cells, and
cytokinesis was complete approximately 70 minutes after break down of the
nuclear envelope (Paper I, Fig. 6c,d and Supplementary Movies 1 and 2).
This result indicates that SAB is not likely to be involved in mitotic
progression, although it does not exclude a role for SAB at other stages of the
cell cycle.
Complex interaction of SAB and CLASP in the control of distinct processes
When comparing the defects of sab-5 and clasp-1 in seedling development,
in trichome branching, and in misorientation of PPB, spindle and
phragmoplast, sab-5 mutants were always more strongly affected (Paper I,
Fig. 5a,b and Fig. 6o-q). Mutations in the two genes determined different
phenotypes with respect to planar polarity of root hairs and ROPs, with sab5 causing both an apical and a basal shift of hair and ROP positioning and
clasp-1 inducing an exclusively basal shift (Paper I, Fig. 3c and Fig. S2a-d
and Fig. 5c-h). Combining the two mutations led to strongly enhanced
defects in overall growth and in trichome branching (Paper I, Fig. 5a,b and
Fig. S3a-c), indicating synergistic action. However, with respect to ROP
positioning and orientation of mitotic structures the sab-5;clasp-1 double
mutants did not statistically differ from sab-5 (Paper I, Fig. 5k and Fig. 6oq), suggesting that SAB is epistatic to CLASP in the control of these
processes. These findings are sign of a complex interaction between SAB and
CLASP, which may combine their functions differently in distinct pathways.
Synergy between two genes is generally the product of non-linear interplay,
whereas epistasis usually indicates that they act sequentially in one pathway.
Non-linearity could imply that SAB and CLASP reciprocally feed on each
other’s function, act together with additional common partners or form a
protein complex to control plant development and trichome morphology. To
date, we have no data supporting any of these scenarios and thus further
studies are needed to assess the likelihood of each hypothesis. For instance,
genetic interaction between SAB and CLASP does not strictly imply direct
protein interaction: association between SAB and CLASP could only be
confirmed through additional essays, which will however be complicated by
the considerable size of both proteins. Different localization also does not
suggest direct stable interaction, considering that SAB and CLASP, despite
partial potential overlap (at cell edges, in regions at the periphery of mitotic
spindles and phragmoplasts), overall display quite dissimilar distribution:
CLASP accumulates on PPBs (Ambrose et al., 2007; Kirik et al., 2007)
whereas SAB localized only in proximity to them (Paper I, Fig. S5); CLASP
labels cortical microtubules (Ambrose et al., 2007; Kirik et al., 2007)
whereas the membrane-associated SAB patches did not seem to colocalize
43
with microtubule bundles (Pietra, Gustavsson and Grebe, preliminary
observations).
In processes where the interaction between SAB and CLASP seemed
linear, we studied whether SAB function influenced CLASP expression and
vice versa, in order to determine which one of the two genes could act further
upstream. GFP-CLASP accumulated on aberrant PPBs in sab-5 mutants,
indicating that its localization to mitotic structures was affected by SABdependent orientation of the cortical microtubules in preprophase (Paper I,
Fig. 6s,t). On the contrary, SAB-3xYpet and 3xYpet-SAB localization were
completely unaltered in clasp-1 mutant seedlings (Pietra and Grebe, data not
shown). These results strongly support a role for SAB upstream of CLASP in
orientation of cell division planes and planar polarity of the root epidermis.
SAB may act through CLASP to control the cortical microtubule array, while
playing a broader role in these processes via interaction with other potential
partners.
SAB function in the organization of cortical microtubules
Role of SAB in elongating epidermal cells
Considering the role of SAB in orientation of microtubule arrays during
mitosis, we decided to investigate whether this gene also has an effect at later
stages of differentiation, when cells elongate and start to differentiate a hair
bulge.
Right after division in the meristem, root epidermal cells have their
microtubules distributed randomly at the cell cortex, without a specific
arrangement (Ehrhardt and Shaw, 2006). In order to drive anisotropic cell
expansion, microtubules organize into cortical bundles that orient
transversally to the root axis and to the direction of cell growth (Baskin,
2001). They do so by exploring the two-dimensional cortical environment
and modifying their alignment upon encounters with other microtubules at
sharp angles (Dixit and Cyr, 2004), and by interacting with MAPs that can
finely tune the organization, stability and orientation of the array (Ehrhardt,
2008). When we observed sab-5 epidermal cells that were either beginning
to expand or rapidly elongating, we noticed that their cortical microtubule
lattice was not regularly transversal as in wild-type cells but rather appeared
irregular, more crisscrossed and less aligned to the root apical-basal axis
(Paper I, Fig. S4a-c and Fig. 7a-c). Microtubule growth was bidirectional in
both wild-type and sab-5 cells (Paper I, Supplementary Movies 3 and 4);
however, the orientation of the cortical array of mutant cells did not seem
suited for supporting correct directional cell expansion. This could be one of
the causes of the reduced final length of sab epidermal cells and overall small
size of sab plants (Paper I, Fig. 3a,b). A possible explanation for the aberrant
44
alignment of cortical microtubules in sab elongating cells is that SAB is
involved in controlling the dynamics, interactions or bundling of
microtubules. Thus, lack of SAB function may not allow formation of the
bundles needed for reorganizing the cortical array after cell division. Such a
remodelling of cortical microtubule arrays through activity of a protein that
affects microtubule interactions would closely resemble the recently
described mechanism that is based on the severing protein katanin
(Lindeboom et al., 2013). Alternatively, SAB could function in cell-wide
arrangement and directionality of microtubule bundles and hence in sab
mutants the bundles would not be uniformly aligned and capable of driving
expansion in a single direction.
Bipolar growth of longitudinal microtubule arrays
At later stages, when epidermal cells have fully elongated and cease growth,
cortical microtubules reorient from transversal to oblique, and finally form a
more longitudinal array (Granger and Cyr, 2001). Longitudinal microtubule
arrays have been shown to be strongly bipolarized in hypocotyl cells, both
prior to and after bursts of growth (Sambade et al., 2012). We observed a
similar bipolar growth in root epidermal cells, with microtubule plus ends
elongating towards the shoot apex in the apical part of the cell and towards
the root tip in the basal part of the cell (Paper I, Fig. 7d-f and Supplementary
Movie 5). A functional explanation for this dynamic behaviour of cortical
microtubules is still lacking; however, bipolar growth was maintained also in
sab-5 cells, and the main difference compared to the wild type was rather in
the longitudinal orientation of microtubules and in their alignment to the
growth axis (Paper I, Fig. 7g and Supplementary Movie 6). SAB therefore is
not likely to be involved in directionality of microtubule growth, but instead
seems to modify alignment of their growth pattern, in meristematic as well
as in elongated cells.
Cortical microtubule organization at root hair initiation sites
Shortly before completing elongation, trichoblasts begin differentiating root
hairs on their surface. Bao et al. (2001) reported that reducing α-tubulin
expression induces the formation of ectopic root hairs and multiple hairs on
individual cells, thus indicating that microtubule dynamics could have a role
in establishment of root hair initiation sites. Indeed microtubules have been
shown to be disorganized in the apical region of emerging root hairs (Van
Bruaene et al., 2004); however, so far no specific microtubule organization
seemed to be required for root hair initiation. Our observations of the
microtubule cytoskeleton in combination with the root hair initiation site
marker PIP5K3-YFP uncovered the presence in 45% of the observed cells of a
45
characteristic radial array of cortical microtubules labelling the future site of
hair outgrowth prior to any morphological sign of bulge formation (Paper I,
Fig.7h-l and Fig. S4d,e). Radial organization of microtubules has already
been described for actively elongating tip-growing cells like moss
protonemata and conifer pollen tubes (Doonan et al., 1985; Anderhag et al.,
2000). Moreover, microtubules are known to play a role during later phases
of root hair tip-growth, as they control growth direction and avoid branching
(Bibikova et al., 1999). However, our finding identified specific microtubule
reorganization at root hair initiation sites at an earlier stage than described
before. The reason why not all of the analyzed cells presented this radial
array of microtubules still needs to be investigated, nonetheless one possible
explanation is that the radial rearrangement is transient and can only be
observed in a limited number of cells unless the hair initiation process is
entirely followed over time. Alternatively, the radial array might not be
strictly required for root hair initiation, and cells could begin hair formation
regardless of this arrangement. Similarly, longitudinal orientation of
microtubules might be frequent but not necessary for the earliest stages of
hair initiation: 4/71 cells expressing PIP5K3-YFP still had transversally
oriented microtubules. This seems to contradict earlier findings stating that
microtubule disorganization is necessary for root hair outgrowth in
Arabidopsis (Van Bruaene et al., 2004); however, previous studies have
employed the formation of a bulge as morphological sign of hair initiation,
while we observed the accumulation of a fluorescent marker at the hair
initiation site and thus have captured earlier stages of hair formation.
When analyzing the organization of cortical microtubules in sab-5 mutant
trichoblasts about to initiate a root hair, we could detect sites with radially
arranged microtubules that corresponded to PIP5K3-YFP patches (Paper I,
Fig. 7m-o). Therefore the mechanisms for generating radial arrays seemed to
still be functional in the absence of SAB. However, we could not find any cell
where microtubules displayed a clear and unique radial arrangement at the
site of hair initiation (Paper I, Fig. 7m-o and Fig. S4h-k). This result
indicated that SAB activity could be necessary for directing and limiting the
degree of microtubule organization and the formation of radial arrays
marking sites of polar root hair initiation. Determining the functional role of
microtubule rearrangement at hair initiation sites and the link between
radial arrays and establishment of polarity on the lateral membrane of root
epidermal cells could give a more precise hint towards SAB function in the
planar polarity pathway.
46
Actin is an additional player in the planar polarity pathway
ACTIN7 genetically interacts with SAB
After finding out that SAB genetically interacted with a MAP gene in planar
polarity establishment and affected the orientation and organization of
microtubules during cell division and elongation, we decided to investigate
whether SAB also interacted with the actin cytoskeleton, which is known to
regulate cell shape, architecture and polarity. To this end, we generated
double mutants between sab and a mutant defective in the gene encoding the
vegetative actin ACTIN7 (ACT7), and obtained seedlings with much shorter,
radially swollen roots and delayed growth compared to each of the single
mutants (Fig. 10a,b). These severe defects suggested that SAB and ACT7 may
interact synergistically in determining overall seedling development, and
prompted us to analyze whether ACT7 was also involved in planar polarity of
the root epidermis. We thus immunolocalized ROPs, the earliest markers of
planar root hair polarity, in trichoblasts of sab-5, act7-6 and sab-5;act7-6
mutants. Both sab-5 and act7-6 single mutants displayed a basal and an
apical shift in ROP localization compared to wild-type seedlings (Paper I,
Fig. S2a-d and Paper II, Fig. 5a,c,f). However, the apical shift was
significantly more pronounced in sab-5;act7-6 double mutants (Fig. 10c).
These results indicated that SAB and ACT7 are likely to have a combined
effect in the planar polarity pathway, and uncovered a potential, previously
unknown, interaction of a SAB-related protein with the actin cytoskeleton.
This finding led us to investigate the contribution of the actin cytoskeleton to
planar polarity of root hair positioning in more detail.
Figure 10. SAB and ACT7 interact genetically to determine seedling development and mediate
polar ROP positioning in trichoblasts. (a,b) Strongly impaired development of 5-day-old sab-5;act7-6
seedlings with respect to act7-6 and sab-5 single mutants. Note, extremely short and radially swollen roots.
(c) Quantitative analysis of polar positioning of ROP protein patches along the apical-basal axis of epidermal
cells in act7-6, sab-5 and sab-5;act7-6 seedlings. Number of cells in classes (frequency) showing ROP
positions between basal (0) and apical (1) ends is shown (**P = 0.009 act7-6 versus sab-5, **P = 0.002 sab-5
versus sab-5;act7-6, **P = 0.000 act7-6 versus sab-5;act7-6 by Kolmogorov-Smirnov test, n = 50 cells from
26 to 29 roots per genotype). Data for act7-6 are the same presented in Paper II Fig. 5f. For experimental
procedures, see Paper II. Scale bar, 2 mm.
47
The actin cytoskeleton affects planar polarity of root hair positioning
Actin is essential for tip growth of root hairs, and thick actin bundles as well
as dense F-actin meshworks have been localized to the central region and
just below the tip of elongating hairs (Rounds and Bezanilla, 2013; Baluška
et al., 2000). However, we could observe F-actin strands already during the
first morphological signs of hair initiation and even in proximity to sites of
hair emergence prior to formation of a bulge (Paper II, Fig. 1j,k). These
localization data support a role for actin organization in early events of root
hair initiation and potentially in selection of the polar site of hair outgrowth
on the lateral membrane of trichoblasts.
In order to examine the effects of interference with the actin cytoskeleton,
we analyzed the planar polarity phenotypes of mutants defective in various
vegetatively-expressed actins. Previous experiments have shown that
mutants of the ACT2 gene display a weak apical shift of root hair initiation
compared to wild type (Ringli et al., 2002), and this was confirmed by our
analysis of hair positioning in act2 mutants (Paper II, Fig. 1a,b,g). Stronger
defects were though uncovered in act7 mutant seedlings, both in distribution
of hair initiation sites (Paper II, Fig. 1a,c,g and Fig. S1a,b) and in positioning
of ROP patches on the trichoblast lateral membrane (Paper II, Fig. 5a,c,f): in
addition to a pronounced apical shift, act7 seedlings also presented a basal
shift of hair and ROP positioning, when compared to wild type. These
findings, combined with the lack of effects in actin8 (act8) loss-of-function
mutants (Paper II, Fig. S1d), suggest that ACT7 is the actin isoform that
contributes most strongly to planar polar establishment. Nevertheless, ACT2
also plays a role in this process, as demonstrated by the enhanced root hair
positioning defects of act7;act2 double mutants with respect to both single
mutants (Paper II, Fig.1b-d,h).
Furthermore, the mislocalization of ROPs in act7 mutants indicates that
the actin cytoskeleton is likely to have an effect upstream of ROP GTPases in
planar polarity of root hairs. This scenario is intriguing because in other
processes, like pavement cell morphogenesis and distribution of auxin
transporters, the actin cytoskeleton has been suggested as a downstream
effector of signals mediated by ROP molecular switches (Fu et al., 2005; Lin
et al., 2012). A tempting hypothesis is that the effect of the actin cytoskeleton
on ROP localization is part of a feedback meant to reinforce the formation of
polar membrane domains by recruiting additional polarity determinants,
similar to how polarity establishment is regulated in yeast cells (Piel and
Tran, 2009; Marco et al., 2007; Valdez-Taubas and Pelham, 2003).
Interference with actin organization may destabilize the set up of hair
initiation sites and randomize the positioning of ROPs and eventually root
hairs. The observation that mutation of an actin gene results in ROP
misplacement is in apparent disagreement with the reported unaffected
48
polar ROP localization upon pharmacological disruption of the actin
cytoskeleton (Molendijk et al., 2001). It is thus possible that the role of actin
in polar ROP positioning is indirect. Alternatively, interfering with actin
organization might not influence the formation of discrete ROP patches at
the plasma membrane but only alter their polar positioning along the apicalbasal cell axis: no quantification of ROP distribution following drug
treatment has in fact been provided in previous studies (Molendijk et al.,
2001).
AIP1-2 is an actin interactor in plants
In an effort to clarify the mechanisms of actin control over planar polarity,
we looked for interactors of plant actins by conducting a yeast two-hybrid
screen. Yeast two-hybrid analyses indicated AIP1-2, the product of one of the
two isoforms of the AIP1 gene in Arabidopsis, as a strong interactor of all
vegetative actins and ACT1 (Paper II, Fig. 2a). Similar results were obtained
with the product of the other AIP1 isoform, AIP1-1, and were confirmed in
vitro by Glutathione-S-Transferase (GST) pull-down assays with ACT2 and
ACT7 (Paper II, Fig. 2b,c and Fig. S2a-f). Significance of the interaction
between AIP1-2 and ACT7 was further assessed in planta through analysis of
act7;aip1-2 double mutants: germination was significantly reduced and
plants that did germinate presented shoot morphological defects that were
absent in both of the single mutants (Paper II, Fig. 3c-g and Fig. S3a-f). The
synthetic lethality of act7;aip1-2 mutants is indicative of a strong synergistic
effect of the two mutations and resembles the lethality that results from
combining the yeast homolog of AIP1, whose mutation does not cause severe
growth defects on its own, with mutations in ACT1 (Rodal et al., 1999).
AIP1 is a modulator of ADF severing activity that was first isolated in yeast
in a screen for Act1p interactors (Amberg et al., 1995). Consistent with the
role of AIP1 in F-actin disassembly, mutants defective in AIP1 homologs
display excessive actin stability and bundling in Drosophila, Physcomitrella
patens, and Arabidopsis lines where both AIP1 genes are knocked-down by
RNA interference (Ren et al., 2007; Augustine et al., 2011; Ketelaar et al.,
2004). Compromised AIP1 activity causes dramatic developmental defects
and strongly affects the elongation of tip growing cells in these organisms
(Ren et al., 2007; Augustine et al., 2011; Ketelaar et al., 2004). Interestingly,
mutants defective in the Drosophila AIP1 homolog Flare show aberrant
polarity of wing hair positioning, suggesting that in flies actin remodelling is
also involved in setting up planar polarity (Ren et al., 2007).
In order to test if Arabidopsis AIP1-2 also had an effect on planar polarity
establishment, we analyzed hair and ROP positioning in the root epidermis
of aip1-2 mutants, and discovered that hair initiation as well as ROP patches
were basally shifted with respect to wild type (Paper II, Fig. 4a,b,d and Fig.
49
5a,b,e and Fig. S4a). The difference in effect between the aip1-2 mutation,
causing a basal shift, and mutations in actin genes, act2 determining an
apical shift and act7 both an apical and a basal shift, may be attributed to the
opposite results that the mutations have on the actin cytoskeleton: whereas
aip1-2 likely determines stabilization and bundling of F-actin, although the
probable subtlety of this phenotype does not allow detection of any bundles
in aip1-2 seedlings, mutations in actin genes destabilize actin filaments and
thus reduce the formation of bundles.
Considering the effect we observed on plant survival and growth by
combining aip1-2 with the act7 mutation, we further investigated whether
AIP1-2 interacted synergistically with ACT7 also in planar polarity
establishment. Strikingly, positioning of both root hairs and ROPs in
act7;aip1-2 double mutants was not different from act7 single mutants
(Paper II, Fig. 4e and Fig. 5c,d,g and Fig. S4c). This result indicated that in
these processes act7 is epistatic to aip1-2, supporting the idea that ACT7 is
the actin isoform providing the strongest contribution to planar polarity and
that therefore F-actin stabilization does not affect root hair distribution in
the absence of ACT7.
AIP1-2 expression is restricted to hair-producing cells
With the aim of verifying whether AIP1-2 could interact with actin filaments
at root hair initiation sites, we analyzed the localization of a functional AIP12 fluorescent protein fusion. We observed prevalent AIP1-2 expression in the
epidermal layer of roots and strong accumulation at future sites of hair
emergence and especially in outgrowing hair bulges, where it coincided with
an enrichment of F-actin (Paper II, Fig. 4f-h). This finding corroborated the
interaction between AIP1-2 and actins, and supported the role of AIP1-2 in
planar polarity of root hair positioning. Surprisingly, AIP1-2 expression in
epidermal cells was specifically enriched in hair files and displayed a pattern
of alternating stripes starting from the early root elongation zone (Paper II,
Fig. 4f and Fig. 6a). To test if AIP1-2 enrichment was associated with the
differentiation of root hair cells, we employed mutation of the CTR1 gene
and treatments with ACC or synthetic auxins to induce the formation of
ectopic root hairs. Both ethylene and auxin signalling stimulate root hair
initiation (Schiefelbein, 2000), and either ctr1 mutation or application of
exogenous ethylene are known to determine an increased proportion of roothair-forming cells by acting downstream of the patterning pathway (Dolan et
al., 1994; Tanimoto et al., 1995; Masucci and Schiefelbein, 1996).
Intriguingly, we observed enhanced ectopic AIP1-2 expression in cells in the
non-hair position and in cells growing ectopic root hairs (Paper II, Fig. 6c-g).
This finding demonstrates that heterogeneous expression of AIP1-2 in the
root epidermis is affected by ethylene and auxin signalling.
50
Interplay of ethylene signalling and actin cytoskeleton in planar polarity
In addition to controlling root hair initiation, ethylene is also one of the main
actors in the pathway determining planar polarity of root hair positioning
(Masucci and Schiefelbein, 1994; Fischer et al., 2006; Ikeda et al., 2009).
The effect of ACC treatment and mutation of the CTR1 gene on AIP1-2
expression prompted us to further explore the genetic relationship between
ethylene signalling and the actin cytoskeleton in polar initiation of root hairs.
Mutation of the two vegetative actin genes ACT2 and ACT7 completely
suppressed the hyperpolar phenotype of the ctr1btk mutant (Paper II, Fig. 1df,i), indicating that ACT2 and ACT7 are epistatic to CTR1 in root hair
positioning. However, when combining the ctr1btk mutation with an aip1-2
mutant, the ctr1 phenotype was epistatic to aip1-2 and double mutant
seedlings were indistinguishable from ctr1btk single mutants (Paper II, Fig.
7a-e). These findings are consistent with ACT7 being epistatic to AIP1-2
(Paper II, Fig. 4e and Fig. 5c,d,g and Fig. S4c), and could outline a scenario
where ethylene can control F-actin stability and bundling in hair cells by
affecting the expression of AIP1-2, while at the same time proper formation
of actin filaments is necessary downstream of ethylene and actin organizing
proteins to direct the correct placement of root hairs. Although ethylene
signalling has long been known to affect organization of the microtubule
cytoskeleton (Steen and Chadwick, 1981), our observations point out an
additional genetic link with actin. No direct connection between ethylene
signalling and actin is however demonstrated, and thus this effect could be
indirect or mediated for instance by auxin synthesis and perception.
Patterned expression of AIP1-2 depends on WER function
Upon finding that ethylene and auxin affected the patterned expression of
AIP1-2 in the root epidermis, we set out to further determine factors
restricting AIP1-2 accumulation to root hair files. In the root epidermis,
ethylene and auxin modulate gene expression and cell differentiation
downstream of a network of transcription factors that translate positional
signals into hair and non-hair cell patterning (Schiefelbein, 2000; Dolan,
2001). One of the central components of this patterning gene network is the
Myb transcription factor WER (Lee and Schiefelbein, 1999). We thus
investigated whether AIP1-2 expression was under the control of WER by
analyzing AIP1-2 localization in the roots of wer mutant seedlings, which are
defective in non-hair fate specification and thus form ectopic hairs on most
of their non-hair cells. Strikingly, in wer mutants all epidermal cell files
evenly expressed AIP1-2, indicating that preferential accumulation of this
protein in hair files depends on WER function (Paper II, Fig. 6a-c). The
reason for enrichment of AIP1-2 in hair cells is elusive, as no role has been
51
described so far for AIP1-2 downstream of WER. However, controlling the
expression of an actin modulating protein like AIP1-2 could be a strategy to
restrict the energy-consuming reorganization of the actin cytoskeleton to
cells that are going to initiate outgrowth of a root hair.
In Drosophila, expression of the core components of the frizzled planar
polarity pathway and of the effectors that control reorganization of the actin
cytoskeleton is homogeneous in all cells of the tissues whose polarity they
control (Goodrich and Strutt, 2011). Together with RHD6 (Menand et al.,
2007), AIP1-2 is therefore one of the few reported examples of patterned
expression of a gene affecting planar polarity. Although no role has been
described for AIP1-2 in patterning of the root epidermis, the finding that
restriction of its expression depends on WER suggested interplay between
planar polarity establishment and epidermal cell fate specification. We thus
decided to further investigate common features between planar polarity
formation and epidermal patterning. To this end, we started analyzing
mutants of the planar polarity gene SAB for defects in patterning of the root
epidermis.
SAB has a role in root epidermal patterning
sab mutants differentiate excessive ectopic root hairs
The root epidermis of wild-type Arabidopsis seedlings is patterned by the
alternation of longitudinal files of hair-forming and non-hair-forming cells,
whose fate is determined by their position with respect to the underlying
cortex: epidermal cells on top of two cortical cell files produce a hair and are
considered in hair (H) position, while cells over a single cortical cell file do
not differentiate a hair and are thus referred to as non-hair (N) cells (Dolan
et al., 1994). In two mutant alleles of the SAB gene we observed a
significantly higher number of hairs emerging from cells in the N position,
causing the seedlings to display about four times more ectopic hairs than
wild type and strongly suggesting that SAB has a role in root epidermal
patterning (Paper III, Fig. 1a-c and Table 1). Ectopic hairs are characteristic
of mutants defective in genes that promote non-hair fate within the
patterning pathway, but are frequent also in mutant seedlings of the
ECTOPIC ROOT HAIR 2/POM POM 1 (ERH2/POM1) and ECTOPIC ROOT
HAIR 3 (ERH3) genes (Schneider et al., 1997). Roots of erh2/pom1 seedlings
have radially swollen cortical cells similar to sab (Hauser et al., 1995; Benfey
et al., 1993), and erh3 mutants are also deficient in anisotropic cell growth
(Schneider et al., 1997; Uyttewaal et al., 2012), indicating that control of cell
expansion could be involved in patterning of the root epidermis and may be
one of the mechanisms through which SAB affects this process.
Furthermore, ERH3 is the KTN1 katanin, which severs and reorganizes
52
microtubule arrays, contributing to formation of mitotic structures and
orientation of cell division (Bichet et al., 2001; Panteris et al., 2011; Webb et
al., 2002); the similarity with the role of SAB in microtubule rearrangement
suggests that manipulation of microtubule dynamics and orientation may
also have a function in determining cell fate of epidermal cells.
Longitudinal cell divisions are not responsible for sab patterning defects
Once cell fate has been established in the root meristem, hair and non-hair
cells generally divide transversally to the root axis, and daughter cells
assume the same fate as their parent. However, in rare instances cells divide
longitudinally and generate daughter cells that initiate two new cell files that
do not necessarily have the same fate (Berger et al., 1998b). Considering the
role of SAB in orientation of mitotic structures and cell division planes, we
investigated whether the increased amount of ectopic hairs in sab mutants
could be caused by a greater number of longitudinal cell divisions and
subsequent H-fate duplications. This was however not the case, as the
number of cell file divisions in sab mutants was comparable to wild-type
seedlings, indicating that SAB function in cell division orientation is not
likely to play a role in patterning of the root epidermis (Paper III, Fig. 2).
Moreover, in sab seedlings about 40% of the longitudinal divisions took
place in N cells, whereas in wild type the file duplications initiated in most of
the cases from H cells (Paper III, Fig. 2). It is difficult to point out a
functional reason for the preferential occurrence of aberrant longitudinal
divisions in cells with a specific fate. Nevertheless, selection of the files
undergoing duplication seems to be under the control of a mechanism that
requires SAB function. Interestingly, similar defects have been reported for
mutants of genes belonging to the core cell fate patterning pathway (Berger
et al., 1998b), and this result therefore supports the involvement of SAB in
specification of epidermal cell fate.
Destabilized expression of fate markers in the sab root epidermis
We employed cell fate and differentiation markers to visualize the stability of
fate selection within root epidermal cell files. We expected homogeneous
expression of the markers among cells of the same lineage; however, we
noticed that cells would sometimes switch fate with respect to the file they
belonged to, determining a disparity between their position over the cortex
and the marker they expressed. We observed sporadic fate switches in
epidermal cell files of wild-type roots carrying both hair differentiation and
non-hair fate markers. Strikingly though, all of the analyzed markers
revealed substantially more frequent fate alternations in sab-mutant
seedlings than in wild type, suggesting that SAB function is required for
53
uniform fate specification within files of root epidermal cells (Paper III, Fig.
3 and Fig. S1).
One of the employed reporter constructs, pWER:GFP, indicates
expression of a core component of the patterning pathway and positive
regulator of non-hair cell fate (Lee and Schiefelbein, 1999). Considering the
increase of ectopic root hairs in sab mutants (Paper III, Fig. 1a-c and Table
2), SAB may be expected to negatively affect WER expression in epidermal
cells. However, we could not find any preference in the cell fate of epidermal
files undergoing switches of pWER:GFP expression, indicating that the sab
mutation apparently has no effect on the overall number of cells expressing
WER and adopting the N fate. Further studies will thus be needed to clarify
how SAB acts on WER expression and to explain how lack of SAB function
translates into root hair patterning defects, since we currently cannot
exclude an additional effect of the core patterning pathway on SAB. The
unstable expression of fate markers suggests that SAB controls fate
maintenance within cell files rather than being involved in the specification
of one or the other fate, and that the role of SAB is therefore in pattern
stability within the root and not in selection of single cell fate.
SAB affects epidermal cell fate upstream of the core patterning pathway
We further explored the function of SAB in epidermal fate specification by
analyzing genetic interaction between SAB and genes of the core patterning
pathway. Hair patterning defects of mutants lacking function of either the
WER or CPC genes, which promote non-hair and hair fate respectively, were
epistatic to the phenotype of sab mutants, and led to either very hairy or
hairless double mutant seedlings (Paper III, Fig. 4 and Table 3). These
results suggested that SAB acts in the same pathway as WER and CPC and
may function upstream of them. The latter hypothesis is supported by the
observation that mutation of SAB can affect the expression of WER and of
genes further downstream in the cell fate specification and differentiation
pathway (Paper III, Fig. 3 and Fig. S1). Additionally, the finding that
mutation of SAB in the cpc background determines hairless seedlings
indicates that activity of the non-hair-fate-promoting complex is not
impaired in sab mutants and hence SAB is not likely to be one of its
components.
The function of SAB upstream of the core epidermal patterning pathway
further rules out that the excessive amount of ectopic root hairs in sab
mutants may be a consequence of enhanced sensitivity to phosphorus (P)
starvation or an effect of ethylene signalling. Recent studies have
demonstrated that sab mutants are highly sensitive to P starvation (Yu et al.,
2012), and this physiological stress is known to promote the formation of
root hairs (Schmidt and Schikora, 2001). Moreover, SAB seems to counteract
54
ethylene signalling, which is known to stimulate root hair development
(Aeschbacher et al., 1995; Yu et al., 2012; Tanimoto et al., 1995). However,
both P and ethylene have been shown to affect differentiation of epidermal
cells downstream of the core patterning gene network (Müller and Schmidt,
2004; Masucci and Schiefelbein, 1996). Placing SAB upstream of WER and
CPC action excludes that the patterning defects of sab mutants depend on
the effect of SAB on P and ethylene signalling, and further supports a role for
SAB upstream of the pathway that controls patterning of epidermal cell fate.
SAB does not control patterning of leaf trichomes
After discovering that SAB is involved in root epidermal patterning, we
investigated whether this gene does also have a role in specification of leaf
trichomes, whose regular spacing on the leaf surface is controlled by a gene
network that employs components very similar to the ones determining root
epidermal fate (Hülskamp, 2004; Ishida et al., 2008). To calculate the
proportion of leaf epidermal cells that differentiate into trichomes, we
quantified the number of trichomes on leaves of wild-type and sab-5 plants
and compensated for differences in leaf size and cell density between the two
genotypes. Surprisingly, values were very similar for wild-type and mutant
leaves, suggesting that SAB does not affect trichome density and that its role
in epidermal cell fate specification is likely to be restricted to the root (Paper
III, Fig. 1d-g and Table 2).
This finding may be explained in several ways: first, SAB could be a rootspecific component of the cell fate specification pathway, similar to the MYB
transcription factor WER that is only present in the root and hypocotyl (Lee
and Schiefelbein, 1999). SAB function might not be required for patterning
of the leaf epidermis, or may be executed by another shoot-specific
component. However, considering the role that SAB has in planar polarity
and branching of leaf trichomes (Paper I, Fig. 1h-m and Fig. 5a and Fig.
S2e,f) and the strong defects in leaf size observed in sab mutants (Paper I,
Fig. 8a,b and Paper III, Fig. 1d,f), it is unlikely that the SAB protein is absent
from leaf tissues. It could however be that SAB function in the shoot is
restricted to other roles and that SAB in the leaf is not part of the patterning
pathway. Alternatively, there could be a shoot-specific redundant factor with
functions similar to SAB in leaf epidermal patterning. This factor would be
able to compensate for SAB loss-of-function in leaves but not in roots,
determining the absence of a visible shoot patterning phenotype in sab
mutants. Finally, the SAB gene might play a role that is independent of the
core network of patterning transcription factors and is required only for
epidermal patterning of roots. The main difference within epidermal fate
specification is that root cells receive positional cues from the underlying
cortical layer, while patterning of leaf cells is only driven by stochastic
55
fluctuations and cell-to-cell interactions (Balkunde et al., 2010; Schiefelbein
et al., 2009). If indeed SAB were implicated in generating, perceiving,
and/or transmitting the positional signals from the cortex, there would be no
role for it in patterning of the leaf epidermis, regardless of its expression in
aerial tissues.
SAB may act on transduction of patterning cues from the cortex
Strikingly, sab mutants display various similarities to mutants of genes that
are involved in radial communication between the root cortex and epidermis.
For instance, mutants defective in either the SCM or JKD gene show an
increase in the number of ectopic root hairs similar to sab mutants (Kwak et
al., 2005; Hassan et al., 2010; Paper III, Fig. 1a-c and Table 1). Additionally,
scm and jkd mutants also have a higher amount of non-hair cells in the H
position (Kwak et al., 2005; Hassan et al., 2010). Although in sab mutants
the number of H cells not producing a hair was not significantly different
from wild type, thorough observation revealed that both analyzed sab alleles
also had a subtle defect in specification of the H fate (Paper III, Table 1).
Furthermore, expression of two non-hair fate markers in the root epidermis
is unstable and randomized in scm and jkd, similar to what we observed in
sab seedlings (Kwak et al., 2005; Hassan et al., 2010; Paper III, Fig. 3).
Finally, the effect of the wer and cpc mutations on scm seedlings strongly
resembles what we observed for sab;wer and sab;cpc in that the epidermal
patterning of scm;wer and scm;cpc double mutants is indistinguishable from
the single wer and cpc mutants (Kwak and Schiefelbein, 2007; Paper III,
Table 3).
These considerations support the idea that, similar to SCM and JKD, SAB
functions in stabilizing fate acquisition upstream of the core patterning
pathway. In the hypothetical scenario that, like SCM and JKD, SAB may be
involved in the interaction between root epidermis and cortex, interesting
considerations could come from comparison of the localization of the three
proteins. JKD, which modulates root hair specification upstream of the
patterning pathway, is not present in epidermal cells and operates non-cellautonomously from the cortex (Hassan et al., 2010). In contrast, both SCM
and SAB are expressed in all root cell types (Kwak et al., 2005; Paper I, Fig.
8i), suggesting that the role of SAB might be more similar to that of SCM.
However, neither scm nor jkd mutants have defects in the density of root
hairs on their epidermis (Kwak et al., 2005; Hassan et al., 2010), while sab
seedlings display an overall increased proportion of hair-bearing cells (Paper
III, Fig. 1a-c and Table 1). Therefore, even on the assumption that SAB may
have a position analogous to either SCM or JKD in the pathway, its role and
mechanism of action are likely to differ markedly.
56
Conclusions and Future Perspectives
Similar mechanisms for establishment of polarity are present in all
eukaryotic systems. They involve an initial polarity cue, polar accumulation
of signalling complexes and, as a last step, organization of the cytoskeleton to
orient cells and their structures. Here we have identified SABRE as a novel
player in the Arabidopsis planar polarity pathway and have shown that this
gene also functions in organization of cortical microtubules, orientation of
mitotic structures, and patterning of the root epidermis. Genetic interaction
with CLASP and ACT7 supports an involvement of SAB in arrangement of
microtubule arrays and in actin function. Accordingly, SAB acts on planar
polarity upstream of ROPs, which have been shown to control organization
of both microtubules and F-actin in other processes (Fu et al., 2005; Fu et
al., 2009; Lin et al., 2013). Actin and its organization have been suggested to
play a role in planar polarity (Ringli et al., 2002; Ren et al., 2007); we
further characterize their contribution, identify new interactions and reveal a
connection with the pathway for epidermal cell patterning. On the other
hand, our findings of specific cortical microtubule arrays at root hair
initiation sites, of planar polarity defects in clasp mutants, and of roles of the
SAB planar polarity gene in microtubule organization strongly encourage
further studies on the involvement of the microtubule cytoskeleton during
coordination of planar polarity.
Treatment with microtubule inhibitors and mutations in MAP genes or
actin have been shown to induce misorientation of mitotic structures or cell
division planes resembling those we observed for sab mutants (Baskin et al.,
2004; Ambrose et al., 2007; Panteris et al., 2011; Gilliland et al., 2003). This
resemblance is further indicative of a likely role for SAB in connection with
both cytoskeletal arrays. In addition, the phenotypic similarities between sab
and act7, which in contrast to most published planar polarity mutants
display both an apical and a basal shift of root hair distribution, suggest an
analogous mechanism of SAB and ACT7 action on root hair positioning.
Crosstalk between microtubule and actin dynamics in Arabidopsis has
already been demonstrated (Sampathkumar et al., 2011), thus it is
reasonable to assume that SAB could have an effect on both arrays and to
imagine a strong interplay between microtubules and F-actin in both planar
polarity and epidermal patterning. Additional studies on the functional
interaction between SAB and components or modulators of the microtubule
and actin cytoskeleton may help understanding the exact role of SAB in
organization of these arrays.
The large size of the SAB protein makes it a good candidate for acting as
an organizing hub or scaffold for cytoskeletal structures. This hypothesis is
intriguing also in light of the localization of SAB at the cell cortex and in
57
proximity to mitotic arrays. A structural role for SAB might also explain the
partial conservation of its sequence, as its function and interactors would be
similar among distantly related species. Mapping of functional protein
domains could help to elucidate roles and mechanisms of action of the SAB
protein. These would additionally be clarified by uncovering potential SAB
interactors; so far the yeast two-hybrid screens we conducted with five
different SAB bait proteins including the full-length sequence have not
identified any candidate for direct interaction with SAB (Pietra and Grebe,
unpublished results), but biochemical methods such as coimmunoprecipitation might prove more successful in the future.
Mechanisms of SAB action as well as its effect on microtubule and actin
organization at the molecular level are still unknown, and future studies may
reveal whether the SAB protein can directly bind to microtubules or F-actin.
An effect of SAB on microtubule organization exclusively through CLASP
would not explain the synergistic interaction between SAB and CLASP and
the stronger phenotypes of sab compared to clasp mutants. Therefore, SAB
may either affect microtubule arrays directly or through genetic interaction
with other modulators of their dynamics. A direct role for SAB on
microtubule dynamics would be intriguing, considering the analogies
between SAB action and the microtubule severing protein katanin, which
similarly to SAB is widely conserved and affects cell division orientation,
anisotropic cell expansion and epidermal patterning (Panteris et al., 2011;
Schneider et al., 1997; Webb et al., 2002). Strikingly, despite its local effect
on individual microtubules, katanin is able to coordinate global organization
of cortical arrays within an entire cell, in events such as response to
mechanical stress or rapid reorientation of cortical microtubule arrays upon
light perception (Uyttewaal et al., 2012; Lindeboom et al., 2013).
Analogously, SAB could act on microtubule dynamics to direct cell-wide
cytoskeletal organization.
Taken together, our findings identify SAB as a novel planar polarity and
epidermal patterning player involved in organization of microtubule arrays
and actin function. This study opens the way for understanding the function
of SAB-related proteins in eukaryotic organisms and stimulates further
analyses on the roles of the microtubule and actin cytoskeleton in planar
polarity and epidermal cell fate specification.
58
Acknowledgements
Thank you to Prof. Dr. Markus Grebe for conceiving this project, supervising
me during my doctoral studies, and for critically reading and commenting on
this thesis.
I am grateful to all the past and present group members for fruitful
discussions, suggestions, and nice times during and after work. Thank you to
Yoshi who initiated the work on kuq and guided me in the lab when I got
started, and a big thank you to Anna for all her work on the SAB project, and
for swedish translations.
Thank you to the three incredibly talented master students I had the
pleasure to work with, who allowed me to achieve results that would not
have been possible had I been working on my own.
A big thank you to Jose and Anna and all the members of the AlonsoStepanova lab, who gave me an amazingly warm welcome in Raleigh and
made my stay there so enjoyable.
Thank you to all my office mates for their tolerance during the long
unexpected meeting, and to Kriszta and Carole in particular for the good
mood and laughters.
Thanks a lot to all those helping UPSC to run smoothly and efficiently and to
those that keep it such a lively and stimulating environment.
Thanks to Benni for the help with practical issues concerning the thesis and
for all the motivating messages, and to Paola for drawing Figure 8.
A great thank you to my family and friends, for their constant support and
affection, even from a distance.
Thanks to Matilda for her patience when I couldn’t dedicate to her the time
she deserved, and for inspiring discussions during the preparation of this
thesis.
And the biggest thank you to Anna, for always helping me to put things in
perspective and see the real priorities, for the butt kicking to help me
writing, and for always being convinced that I would make it, even when I
didn’t believe it myself.
59
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