Download light control of seedling development

Annu. Rev. Plant Physiol. Plant Mol. Biol. 1996. 47:215–43
Copyright © 1996 by Annual Reviews Inc. All rights reserved
LIGHT CONTROL OF SEEDLING
DEVELOPMENT
Albrecht von Arnim and Xing-Wang Deng
Department of Biology, Yale University, New Haven, Connecticut 06520-8104
KEY WORDS: seedling, development, light, Arabidopsis, morphogenesis
ABSTRACT
Light control of plant development is most dramatically illustrated by seedling
development. Seedling development patterns under light (photomorphogenesis)
are distinct from those in darkness (skotomorphogenesis or etiolation) with respect to gene expression, cellular and subcellular differentiation, and organ morphology. A complex network of molecular interactions couples the regulatory
photoreceptors to developmental decisions. Rapid progress in defining the roles
of individual photoreceptors and the downstream regulators mediating light
control of seedling development has been achieved in recent years, predominantly because of molecular genetic studies in Arabidopsis thaliana and other
species. This review summarizes those important recent advances and highlights the working models underlying the light control of cellular development.
We focus mainly on seedling morphogenesis in Arabidopsis but include complementary findings from other species.
INTRODUCTION ......................................... ..........................................................................
COMPLEXITY OF LIGHT RESPONSES AND PHOTORECEPTORS................................
RESPONSES ....................................... ..........................................................................
Seed Germination .................................... ..........................................................................
Sketch of Seedling Photomorphogenesis . ..........................................................................
Formation of New Cell Types .................. ..........................................................................
Cell Autonomy and Cell-Cell Interactions .........................................................................
Unhooking and Separation of the Cotyledons ....................................................................
Cotyledon Development and Expansion .. ..........................................................................
Inhibition of Hypocotyl Elongation ......... ..........................................................................
Phototropism............................................ ..........................................................................
Plastid Development ................................ ..........................................................................
REGULATORS OF LIGHT RESPONSES IN SEEDLINGS..................................................
Positive Regulators ................................. ..........................................................................
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LIGHT CONTROL OF SEEDLING DEVELOPMENT
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Possible Roles of Plant Hormones........... .......................................................................... 231
Repressors of Light-Mediated Development....................................................................... 232
CONCLUSION.............................................. .......................................................................... 235
INTRODUCTION1
Seed germination and seedling development interpret the body plan with its
preformed embryonic organs, the cotyledons, the hypocotyl, and the root.
Whereas embryo and seed development take place in the shelter of the parental ovule, rather independently of the environmental conditions, seed germination and seedling development are highly sensitive and dramatically responsive to environmental conditions. Higher plants have evolved a remarkable
plasticity in their developmental pathways with respect to many environmental parameters. First, the embryonic axes of the root and the shoot orient
themselves in opposite directions in the field of gravity. Second, seedling development is highly responsive to light fluence rates over approximately six
orders of magnitude. The direction of incident light entices shoots and roots to
respond phototropically. Light intensity and wavelength composition are important factors in determining the speed of cell growth, of pigment accumulation, and of plastid differentiation.
Angiosperms, in particular, choose between two distinct developmental
pathways, according to whether germination occurred in darkness or in light.
The light developmental pathway, known as photomorphogenesis, leads to a
seedling morphology that is optimally designed to carry out photosynthesis.
The dark developmental pathway, known as etiolation, maximizes cell elongation in the shoot with little leaf or cotyledon development as the plant attempts to reach light conditions sufficient for photoautotrophic growth. Although the exact patterns of seedling morphogenesis vary widely among different taxa, the light-regulated developmental decision between the etiolated
and the photomorphogenic pathway transcends phylogenetic classification.
Arabidopsis thaliana, for example, is programmed to switch between the photomorphogenic and the etiolation pathway in the hypocotyl and the cotyledons. In the legumes, such as Pisum sativum, which use the cotyledons as
storage organs, the corresponding developmental switch is programmed in the
epicotyl and the primary leaves. Comparable phenomena of developmental
plasticity are observed in the mesocotyl, the coleoptile, and the first leaf of
monocotyledonous seedlings such as oat and rice (50, 99, 136). It is reasonable to speculate that the fundamental mechanism is similar in different plant
1
Abbreviations: UV-A, 320–400 nm light; UV-B, 280–320 nm light; HIR, high-irradiance response; LF, low fluence response; VLF, very low fluence response; Pr, phytochrome form with
absorbance maximum in the red; Pfr, phytochrome form with absorbance maximum in far-red.
We follow the phytochrome nomenclature proposed in Reference 141.
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species, though defined light signals are frequently coupled to individual responses in a species-dependent manner.
The contrasting developmental patterns are thought to be mediated primarily by changes in the expression level of light-regulated genes (reviewed in 5,
90, 168). The cellular events leading to the activation of these genes have
been studied intensively, and extensive progress in elucidating some of the
downstream steps in phytochrome and blue light receptor signaling has been
reviewed during the past two years (15, 115, 138, 140, 152). Use of Arabidopsis thaliana as a model organism has led to profound advances in understanding the light control of seedling development. We attempt to put these recent
genetic advances in perspective with traditional physiological data from other
species and focus on the overlap and the mutual fertilization between these
two lines of research.
Many valuable perspectives on photomorphogenesis have been described
in a series of recent reviews on, for example, responses to blue light (75, 97),
responses to UV light and high light stress (7, 40), ecological considerations
(154, 155, 157), progress based on transgenic plants (188), phytochrome
(138–140, 157, 176, 177), and mutational analysis (28, 45, 78, 86, 97, 134,
143, 188).
COMPLEXITY OF LIGHT RESPONSES AND
PHOTORECEPTORS
In a given species, the specific effects of light can differ drastically from one
organ or cell type to the other and even between neighboring cells. In Arabidopsis, light treatment of a dark-grown seedling will reduce the cell elongation rate in the hypocotyl while inducing cell expansion and cell division in
the cotyledon and the shoot apex. Meanwhile, stomata differentiation is promoted by light in both the growth-arrested hypocotyl and the expanding cotyledon. In light-exposed shoots, plastids differentiate from proplastids or etioplasts into chloroplasts, whereas in the adjacent cells of the root, plastids differentiate instead into amyloplasts under both light and dark conditions.
Light responses are also known to exhibit fundamental changes in sensitivity as development progresses, e.g. from responsiveness to red light to blue
light. This effect is conceptually most easily demonstrated at the level of gene
expression (18, 61, 64, 73).
Finally, the kinetics of light-mediated effects allow for fast responses (in
minutes), such as the inhibition of hypocotyl elongation (37, 162) or the induction of early light-inducible transcripts (114), but also accommodate slow
responses (from hours to days), e.g. the entrainment of circadian rhythms by
light (3a, 12, 103, 106, 121, 192).
LIGHT CONTROL OF SEEDLING DEVELOPMENT
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Perhaps the most important component for encoding the complexity of responses is the multiple families of photoreceptors. Seedling responses to light
are mediated by at least three classes of regulatory photoreceptors: (a) phytochromes, which respond mainly to red and far-red light but which also absorb
blue and UV-light; (b) photoreceptors that are specific for blue and UV-A
light; and (c) UV-B photoreceptors. Photosynthetic pigments, for example
chlorophylls and carotenoids, have important roles as screening agents for the
regulatory photoreceptors. Surprisingly little is known about their direct effects on developmental responses (169).
Molecular cloning of the Arabidopsis CRY1/HY4 gene (3, 91a, 91b, 103a)
as well as characterization of photoreceptor mutants (80, 81, 83, 92) may help
to reveal the well-kept secrets of the blue light photoreceptors, which have
long been referred to as “cryptochromes.” The basis for the wide absorption
band of CRY1 in the blue and UV-A region of the spectrum has been resolved
by molecular analysis, which showed that CRY1 can bind two types of chromophores simultaneously, a flavin and a pterin (91b, 103a). It is conceivable
that both chromophore binding sites can be mutated independently, thus separating sensitivity to UV-A and blue light genetically, as has been demonstrated in Reference 191. In Arabidopsis (3, 87), and also in transgenic tobacco (103a), CRY1 is responsible for sensitivity of hypocotyl elongation to
green light, in addition to blue and UV-A. A possible explanation is provided
by the tendency of CRY1 to stabilize a reduced, green-light absorbing form of
the flavin chromophore (91b).
The phytochromes (phys), a family of dimeric, approximately 240-kDa
chromoproteins, are by far the best studied of all photoreceptors (62, 138–141,
176, 177). In all known phytochromes, absorption of light leads to a conformational shift (photoconversion) of a red light absorbing form (Pr, absorption
maximum around 660 nm) into a form with increased sensitivity to far-red
light (Pfr, 730 nm). Absorption of far-red light converts the molecule back to
the Pr form. Overlap in the absorption spectra of Pr and Pfr ensures that no
light condition can convert all phytochrome into exclusively one form. Only
phytochrome that is newly synthesized in complete darkness is present exclusively as Pr. It is generally approximated that the concentration of Pfr, rather
than Pr, is responsible for all of the photomorphogenic effects of phytochrome, although this view has recently been challenged (95, 142, 151, 154).
Phytochrome responses allow an operational distinction among different
levels of sensitivity: Low fluence (LF) responses are saturated by pulses with
a red fluence component of 1 to 1000 µmol photons/m2. They are at least partially reversible by a subsequent far-red light pulse. The effectiveness of the
far-red pulse is a function of the intervening period of darkness. This function
is known as the escape kinetic, a powerful tool to probe the chain of downstream signaling events. Very low fluence (VLF) responses (<1 µmol/m2 red)
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are inducible by pulses of far-red light alone. High-irradiance responses (HIR)
(typically >1 µmol/m2/s) require continuous irradiation, which precludes
analysis of far-red reversibility.
Phytochrome apoproteins are encoded by a small gene family with five
members in Arabidopsis (PHYA, PHYB, PHYC, PHYD, and PHYE) (34, 139).
Typically, phytochrome A (phyA) holoprotein is abundant in etiolated tissue
and is greatly reduced in green tissue because it is degraded with a half life of
approximately 1 h when in the Pfr form (177). Expression of the PHYA gene
in Arabidopsis and some other species is downregulated by light (38, 66, 149,
159). PHYB, C, D, and E are moderately expressed in both etiolated and green
tissues (34, 141, 158). Mutational analysis has revealed that phyA and phyB
have distinct, partially complementary and partially overlapping functions in
Arabidopsis (31, 71, 140, 142, 154, 155, 188). The absorption spectra of at
least phyA and phyB appear to be almost identical and can therefore not be responsible for the different physiological functions (179, 180). In addition, the
phytochromes that have been examined at the seedling stage seem to be expressed ubiquitously, albeit at different levels, and may contribute only quantitatively to the tissue specificity of many light responses (1, 34, 158).
Functionally distinct phytochromes have been similarly observed in many
other species (139, 188). Apart from Arabidopsis (Table 1) (86, 87), mutants
deficient in specific phytochromes have been described in cucumber (lh) (2,
102), Brassica (ein) (49), pea (lv) (186), tomato (85) (tri) (172, 173), and sorghum (27).
RESPONSES
Seed Germination
Seminal experiments on the light control of seed germination and its action
spectrum revealed the photoreversibility of the phytochrome photoreceptor
(13, 153). The recent availability of mutants affecting specific phytochromes
in Arabidopsis has allowed a critical evaluation of the roles of individual phytochromes on seed germination (35, 142, 151). Rapid germination of Ara bidopsis seeds imbibed in darkness is controlled primarily by phyB, stored in
the Pfr form (PfrB) in the seed, whereas phyA contributes little to the decision
to germinate in darkness. The seed germination rate in darkness is particularly
high in seeds overexpressing phyB (108). Moreover, short pulses of red light
increase the germination efficiency of the wild type further, which suggests
that a significant level of phyB is also present in the Pr form in at least a fraction of seeds (151). A prominent role for a light-stable phytochrome such as
phyB is consistent with the slow escape of the red response from reversibility
by a pulse of far-red light (14).
LIGHT CONTROL OF SEEDLING DEVELOPMENT
Table 1
Name
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Arabidopsis mutants defective in aspects of photomorphogenesisa
Other names
Gene
Phenotype
cloned
Mutants in photoreceptor apoprotein genes
phyA
hy8, fre1
Yes
long hy in FR
phyB
hy3
Yes
long hy in R and W
cry1
hy4
Yes
long hy in B and W
Mutants in genes for pleiotropic regulators
Negative regulators
cop1 to fus 12 in D:
cop1
fusl, embl68
Yes
–short hy
cop8
fus8, embl34
No
–open cotyledons
cop9
fus7, embl43
Yes
–green root
cop10
fus9, embl44
No
–thylakoid membranes
cop11
fus6, emb78
Yes
–cell differentiation
detl
fus2
Yes
–derepression of lightinducible genes
fus4, -5,
No
-11, -12
Positive regulators
fhy1, fhy3
hy5
No
No
long hy in FR
long hy under R and B
Mutants in genes regulating specific responses
Negative regulators
amp1
No
hook open, derepressed gene
expression in D
cop2
No
hook open
cop3
hls1
No
hook open
cop4
No
de-etiolated, nuclear gene
expression
agravitropic
det2
No
de-etiolated, nuclear gene
expression
det3
No
short hy, open cotyledons
doc1–doc3
No
elevated CAB
expression in D
gun1–gun
No
nuclear gene expression
3
uncoupled from plastid
icx1
No
CHS expression sensitized to
light
Positive regulators
cue1
No
low CAB expression
References
41, 120, 133, 142, 189
87, 118, 142, 160
3, 87, 91a,b, 98, 103a
46–48, 112, 116
116, 185
116, 183, 184
116, 185
24, 116, 185
30, 32, 33, 116, 135
88a, 116
189
87
25
68
51, 68
68
29
19a
89
165
68a
89a
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Table 1
Name
(continued)
Other names
Phototropism mutants
nph1
JK224
nph2, nph4
nph3
JK218
rpt1–rpt3
Gene
cloned
Phenotype
References
No
No
No
No
nonphototropic
“-”
“-”
nonphototropic
root
80, 81, 83, 92
92
80, 81, 92
129–131
Abbreviations: hy, hypocotyl; FR, far-red light; R, red light; B, blue light; W, white light; D, darkness; CAB, chlorophyll a/b–binding protein gene; CHS, chalcone synthase gene.
Other phytochromes, such as phyA, gradually accumulate in the imbibed
seed, promoting germination particularly under continuous far-red light. Under far-red light, phyB mutant seeds germinate more efficiently than wild
type. Thus, the wild-type PHYB allele appears to negate the action of phyA,
which provides an example for antagonistic control of the same response by
the two types of phytochrome (142, 151). Because the inhibitory effect of
PHYB is clearly retained in the phyA mutant (142), phyB probably does not
act directly on phyA but rather on a downstream effector of phyA. The level
of PfrB is extremely low in far-red light and suggests that the negative effect
of phyB on phyA-mediated seed germination may be conferred by its Pr form
(142, 151).
Sketch of Seedling Photomorphogenesis
Seedling development in complete darkness differs markedly from that in
continuous white light or under a light-dark cycle. Under light conditions, the
Arabidopsis seedling emerges from the seed coat, consisting of a hypocotyl
with an apical hook, two small folded cotyledons, and a short main root. After
an initial increase in volume, which is attributable primarily to hydration, the
apical hook starts to straighten, and, at the same time, the cotyledons open and
expand by cell division and cell expansion, accompanied by chlorophyll accumulation and greening. Meanwhile, the apical meristem gives rise to the first
pair of true leaves, which carry trichomes. The hypocotyl translates positive
phototropic and negative gravitropic cues into growth by differential cell
elongation, in order to position the cotyledons for optimal exposure to the
light source. In contrast, the root interprets the same signals in exactly the opposite manner, showing positive gravitropism and negative phototropism.
In darkness, the embryonic organs develop according to a completely different program. After an initial phase of moderate cell expansion due to hydration, the hypocotyl cells elongate rapidly while the apical hook persists for
LIGHT CONTROL OF SEEDLING DEVELOPMENT
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over a week and the cotyledons remain folded. The apical meristem remains
arrested in the dark. Only gravitropic cues position the hypocotyl upright in
anticipation of a light source.
At the subcellular level, plastids undergo drastic changes in morphology
and protein composition in both darkness and light. In darkness, proplastids in
the cotyledons develop into etioplasts, characterized by a paracrystalline prolamellar body and a poorly developed endomembrane system. Upon exposure
to light the prolamellar body quickly disappears and is replaced by an extensive network of unstacked and grana-stacked thylakoid membranes, similar to
those of the light-grown seedlings.
In contrast with the aerial portion of the seedling, roots develop in a similar
pattern in both light and darkness. During the first week of seedling development, chloroplast development remains repressed under both light and dark
conditions. However, if plants continue to expose their roots to light beyond
the seedling stage and into adulthood, chloroplast development can be observed in the older part of the root system.
Formation of New Cell Types
Under laboratory conditions, light-dependent decisions that affect cell shape
and differentiation during Arabidopsis seedling development only become apparent two days after germination and then lead quickly into diverging pathways (185). The first two days in light or darkness are accompanied by overall
cell enlargement in hypocotyl, root, and cotyledon, and root hairs develop.
During the following day in darkness, hypocotyl cells elongate enormously,
and the hypocotyl epidermis forms a smooth surface. In the light-grown sibling hypocotyl, cell enlongation is inhibited and cell-type differentiation proceeds. The most obvious examples are the initiation and maturation of stomata
in the epidermal layer of the hypocotyl, which are absent from the hypocotyl
in the dark (185). In Arabidopsis, epidermal hairs are confined to true leaves,
which are themselves dependent on light. The related crucifer Sinapis alba
(white mustard), however, shows that differentiation of epidermal hairs on the
hypocotyl can be under direct light control (181).
The cotyledon development in darkness is essentially arrested after two
days, whereas in the light, cotyledon cells differentiate into distinct cell types,
such as vascular, mesophyll, and epidermal cells. The most conspicuous
change in the expanding mesophyll cells is the differentiation of numerous
proplastids into green chloroplasts, although little differentiation between
palisade and spongy mesophyll cells occurs (32, 46). Meanwhile, the epidermal pavement cells expand into their characteristic lobed, jigsaw puzzle
shape. A set of guard-cell initials is present in the embryonic cotyledons and
will differentiate into guard-cell precursors regardless of light conditions during the first two days (185). While development of guard-cell precursors then
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arrests in darkness, it continues to completion under light conditions. In addition, only in the light-grown cotyledons do new guard-cell initials form, following polarized cell divisions of epidermal cells (185). Finally, the vasculature in dark-grown seedlings is rather undeveloped but is quite extensive in
light-grown seedlings. This has been clearly documented in Zinnia seedlings
by using three early markers for developing xylem and phloem cells (44).
Cell Autonomy and Cell-Cell Interactions
What is the role of cell-cell communication and the extent of cell autonomy
during the light control of seedling development? After microinjection of phytochrome into tomato hypocotyl cells, it was shown that the anthocyanin accumulation and the phytochrome-mediated gene expression pathways are cell
autonomous (123). Similar conclusions were reached for the anthocyanin accumulation pathway by irradiating mustard cotyledons with a microbeam of
red or far-red light (124). Microirradiation at one site, specifically on a vascular bundle or on a site in the lamina, could suppress anthocyanin accumulation
at a site distant from the irradiated site, such as the leaf margin. This demonstrates that long-range inhibitory signals are transmitted through the leaf upon
irradiation (124). Even under uniform irradiation, individual cells in the mustard cotyledons responded in an all-or-none fashion, which resulted in patchy
patterns for both anthocyanin synthesis and for the mRNA of the key enzyme
chalcone synthase (CHS). However, only a subset of those cells that accumulated CHS mRNA accumulated a significant level of anthocyanin. This indicates that, in addition to CHS mRNA, additional rate-limiting factors must be
distributed unevenly over the leaf as well. If those factors are themselves
light-dependent, then the mustard seedling’s competence for the stochastic
patterning may be interpreted as a means to preserve responsiveness over a
wide range of fluence rates, which is typical for light responses in plants
(124).
Unhooking and Separation of the Cotyledons
The separation of the cotyledons and the opening of the apical hook are stimulated by red light (23, 94); in some species, such as Arabidopsis, hook opening
is also promoted by far-red or blue light, which indicates that multiple photoreceptors mediate this response (94, 96). Cotyledons that are folded back on
the hypocotyl are formed initially during the late stage of embryogenesis, and
the apical hook is maintained at the top of the hypocotyl during etiolation. A
developmental problem is that the hypocotyl, but not the hook, responds to directional light with differential cell elongation and phototropic curvature,
while the hook manages to perform differential cell elongation in the complete absence of any directional light signal. Mutations in a number of Arabidopsis loci, such as hookless1 (hls1)/constitutively photomorphogenic 3
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(cop3), amp1, and cop2 (25, 51, 68), result in a loss of the apical hook in darkness. On the other hand, mutation to ethylene overproduction (eto) or to a constitutive ethylene response (ctr1), or external application of ethylene, all result
in an exaggerated hook. Therefore it is likely that ethylene, perhaps in conjunction with auxins, is required to maintain the apical hook (51). The effect
of ethylene on hook formation may well be counterbalanced by cytokinins, as
suggested by the hookless phenotype of the cytokinin overproducing mutant
amp1 (25), although external application of cytokinins can also facilitate hook
formation via ethylene (21). Light, however, overrides the effect of the ethylene signal (82).
In Arabidopsis, the response of the hook to both low fluence red and blue
light is phytochrome mediated and far-red reversible, whereas intense far-red
and blue light act through high-irradiance responses, which lack fluence reciprocity and far-red reversibility (94, 96). The latter involve phyA and a blue
light–specific pathway that is also involved in hypocotyl elongation (97). During the transition of dark-grown seedlings to light, unhooking and arrest of hypocotyl elongation follow similar fluence rate-response curves in Arabidopsis
(94). Both also require a functional HY5 gene (96) and may therefore depend
on similar signal transduction pathways, but in other species the two processes
are more easily separated (94).
Cotyledon Development and Expansion
The same light signals that inhibit cell elongation in the hypocotyl also promote cell expansion in the cotyledons and the leaf. How these differential responses to the same light environment are regulated remains poorly understood (39, 50, 174, 175). Blue and red light–mediated leaf expansion begins
after distinct short and long lag times, respectively, in leaves of Phaseolus,
which is reminiscent of the short and long lag times that pass between blue
and red irradiation, respectively, and the inhibition of hypocotyl cell elongation in cucumber (10, 37). Perhaps promotion and inhibition of cell expansion
are induced by similar pathways in the two organs. Under white light, phytochromes A and B appear almost dispensable individually for cotyledon expansion in Arabidopsis (142). Full cotyledon expansion in bright red and blue
light, however, depends on signals perceived by phytochrome B, as indicated
by reduced cotyledon expansion in the phyB mutant (142). This phytochromeB-mediated cotyledon expansion is organ autonomous (122). The cry1/hy4
mutants show a decrease in cotyledon expansion, which confirms the involvement of a blue light receptor (11, 87, 93). Detaching the cotyledons from the
hypocotyl rescues the cotyledon defect of cry1/hy4 in blue light, suggesting
that the cry1/hy4 mutant hypocotyl may exert an inhibitory effect on cotyledon expansion (11). The importance of light perception in the hypocotyl or the
hook for events in the cotyledons (126), and vice versa (9), has long been
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known. Overexpression of the photomorphogenic repressor COP1 leads to an
inhibition of cotyledon cell expansion under blue light only, similar to the effect in cry1/hy4 (113). This result indicates that COP1 contributes to the inhibition of cotyledon cell expansion that is alleviated by CRY1/HY4 activity.
Inhibition of Hypocotyl Elongation
The inhibition of hypocotyl elongation in response to illumination is one of
the most easily quantifiable developmental processes and has greatly facilitated our understanding of the roles of regulatory components (16, 65, 85, 87,
93, 113, 182). Inhibition of hypocotyl elongation shows a complex fluence dependence that combines inductive, i.e. phytochrome-photoreversible (50,
127), and high-irradiance responses (HIR) (6, 89, 191). The considerable
quantitative variation in the spectral sensitivity among different species is not
easily explained (104).
Multiple photoreceptors can control hypocotyl elongation, although with
distinct kinetics. In cucumber hypocotyls, for instance, cell wall extensibility
and subsequent cell elongation are inhibited extremely rapidly in response to
blue light, starting after a lag of less than 30 s (37, 161, 162). Such a fast response is unlikely to require gene expression. Following a lag of over 10 min,
the phytochrome-mediated response is considerably delayed (157).
In Arabidopsis, phytochromes A and B, the blue light receptor CRY1/HY4
and a genetically separable UV-A receptor have been shown to contribute to
the inhibition of hypocotyl cell elongation (65, 87, 188, 191). Different from,
for example, Sinapis alba, which is most sensitive to red and far-red light (6,
67), Arabidopsis hypocotyl elongation is most easily inhibited under blue
light, where phytochromes and blue light receptors appear to act additively,
specializing in low and high fluence responses, respectively (97, 91a).
Whether the species-specific differences in sensitivity reflect subtle differences in the spectral properties or concentrations of the photoreceptors, the
light environment inside the plant tissue, the mutual coupling of different phototransduction chains, or merely differences in the experimental protocol remains to be addressed.
Arabidopsis phyB mutants show a moderately elongated hypocotyl under
white light (87, 118, 144, 160), where phyA mutants exhibit no such defect
(41, 120, 133, 189). A drastic exaggeration of the long hypocotyl phenotype is
seen in phyA/phyB double mutants (142). Therefore, under white light, inhibition of hypocotyl elongation can be mediated not only by blue and UV-A light
but also by both phyA and phyB in an arrangement suggesting multiple, but
only partially redundant, control (22, 140, 142).
Under continuous red light, phyB is the active phytochrome species inhibiting hypocotyl elongation, whereas under continuous far-red light, phyA is
primarily responsible. However, supplementing a seedling growing in con-
LIGHT CONTROL OF SEEDLING DEVELOPMENT
227
stant red or white light with far-red light causes the hypocotyl to elongate
more rapidly than in constant red or white or in far-red light alone (110, 190).
This effect is apparent in many species and is part of the “shade avoidance”
response in adult plants, because a high ratio of far-red to red light is typical
for the light environment under a plant canopy (154, 155).
One simple model attempts to explain the rate of hypocotyl elongation
solely on the basis of the distinct steady-state levels of PfrB and PfrA, as estimated from their differential stability and expression levels: As discussed in
the section on Complexity of Light Responses and Photoreceptors, phyB is
relatively stable as Pfr and is expressed continuously at a moderate level,
fairly independent of light. In contrast, phyA expression is high in darkness
and low in the light, and PfrA is rapidly degraded (160, 177). Continuous redlight irradiation will therefore rapidly deplete the plant of phyA but not of
phyB. Little phyA-mediated signaling is expected under these conditions, and
continuous red light effects are attributed mainly to phyB. Continuous far-red
light, however, can lead to a relatively high steady-state level of PfrA and
hence can cause a pronounced developmental effect, because the low ratio of
active Pfr to inactive Pr may be compensated for by the high overall phyA
level. The low level of phyB in combination with the low Pfr-to-Pr ratio
makes signaling through phyB negligible under the continuous far-red light.
This model approximates the different roles of phyA and phyB on the basis of
their expression levels and degradation rates alone and does not take into account some possible differences in the coupling of phyA and phyB to regulators or downstream effectors.
Consistent with the overlapping roles of phyA and phyB as inferred from
mutant analysis, overexpression of cereal phyA in tobacco (26, 72, 76, 77,
107, 110, 111, 119), tomato (16), and Arabidopsis (17) or of phyB in Arabidopsis (108, 180) increases the seedlings’ sensitivity to light, as judged by an
extremely short hypocotyl under white light. Overexpression of heterologous
phyA increases the sensitivity to far-red, white, and red light, which suggests
that the elevated level of phyA persists even under prolonged irradiation with
red light, a condition that leads to rapid degradation of the endogenous phyA
(16, 25, 110, 111, 119). On the other hand, is sensitivity to far-red light also
increased in seedlings overexpressing the photostable phyB? Such an increase
would be expected according to the model put forward, on the basis of the essentially identical absorption spectra of phyA and phyB. However, this does
not seem to be the case. Overexpression of phyB does not sensitize hypocotyl
inhibition to far-red light (108, 109, 187). Therefore, phyA and phyB may interact with distinct sets of regulator or effector molecules. Similarly, phyB
overexpression does not disable the shade avoidance response in adult plants,
in contrast with the effect of phyA (110).
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VON ARNIM & DENG
Phototropism
Seedlings of higher plants orient their growth with regard to the direction of
light in an attempt to optimize exposure of the photosynthetic organs to light
(55). The phototropic curvature of the shoot is achieved by differential
growth, with cells on the shaded side elongating more strongly than cells on
the surface exposed to light. Phototropism in Arabidopsis is superimposed
over the light inhibition of hypocotyl elongation and over the negative gravitropic regulation of cell elongation in the hypocotyl (19). Therefore, a single
cell elongation event may integrate signals from three different transduction
chains simultaneously. The role of light on tropic responses is complicated
further by the interaction of a phytochrome-mediated pathway with the gravitropic pathway in both the hypocotyl (63) and the root (54, 95).
Typically, phototropism is mediated by blue and UV-A light, but green
light is effective in Arabidopsis as well (163). Red light absorbed by phytochrome stimulates phototropism directly in pea (132) and modulates the phototropic response to blue light in Arabidopsis (69, 70). Transduction of phototropic stimuli involves an early phosphorylation of a 120-kDa membraneassociated protein (152). Mutational analysis has identified four complementation groups of nonphototropic hypocotyl (nph) mutants (80, 92) and three
complementation groups for root phototropism (rpt) mutants (129–131).
Mutants defective in blue light–mediated hypocotyl cell elongation (cry1/
hy4) retain normal phototropic responses, and phototropic mutants (JK218/
nph3 and nph1-1) respond normally to light by inhibition of hypocotyl cell
elongation. Those results not only confirm that the two processes are genetically separable but also suggest that they are almost certainly mediated by distinct photoreceptors (92, 98), because CRY1/HY4 encodes a blue light receptor (3) and nph1 mutants are defective in an early signaling step of blue and
green light–mediated phototropism, most likely light perception (92). A conceptual similarity among the distinct roles of individual phytochrome family
members and the members of the family of blue light receptors becomes apparent.
Although nph1 mutants are defective in both shoot and root phototropism,
other phototropism mutants, such as rpt1 and rpt2, are specifically defective
in root—but not shoot—phototropism only (129, 130). This suggests that
nph1-mediated signals can be fed into at least two different pathways, depending on cell type, and that the signaling mechanisms in shoot and root are distinct. In support of this interpretation, shoot but not root phototropism is responsive to green light in Arabidopsis (131).
Plant hormones, especially auxins, have been implicated in differential cell
elongation processes, such as during phototropism and gravitropism in hypocotyls, coleoptiles, and roots. Whether phototropism requires redistribution of
auxins or modulation of auxin sensitivity is not well established (55, 125,
LIGHT CONTROL OF SEEDLING DEVELOPMENT
229
130), but investigation of phototropism in auxin-deficient, resistant, or overproducing strains could differentiate between different models. In fact, because the phototropic response is unaffected by the auxin resistance mutation
aux1 (130), root phototropism may not necessarily be compromised by defects in auxin signaling.
Roots and hypocotyls of Arabidopsis also exhibit differential cell elongation responses after gravitropic stimulation (129). Phototropism mutants now
enable us to dissect the relationship between phototropism and gravitropism
in Arabidopsis roots. Roots exhibit positive gravitropism and negative phototropism, and both responses rely on differential cell elongation. Three mutants
have been described that affect both photo- and gravitropism (80, 81), but
many mutations that affect one of the responses specifically are available.
Both rpt1 and rpt2 have apparently normal shoot gravitropism, which also
suggests that a specific signaling pathway for light exists in the root. However, the agravitropic mutants aux1 and agr1 show normal root phototropism
(130). In the shoot, photo- and gravitropism are clearly separable genetically,
because four different nph mutants, including nph1, are gravitropically normal (92).
Previous photophysiological analysis demonstrated separate photoreceptor
systems for blue/UV-A light (PI) and green light (PII) (75, 83, 84), but an allelic series of nph1 mutants suggests a new interpretation. The weak allele
nph1-2 (JK224) is merely defective in first (low light) positive phototropism
in blue light but is wild-type-like in green light, whereas more severe alleles,
for example nph1-1, are additionally defective in second positive curvature in
both blue light and green light. The allelic series of NPH1 indicates that both
types of signals are processed by a single gene product for a photoreceptor
apoprotein, possibly carrying two independently disruptable chromophores or
one chromophore in alternative chemical states (92). In this respect it is interesting to note that the CRY1/HY4 gene product may also bind two distinct
chromophores, namely a pterin and a flavin (3, 91b, 103a). A detailed comparison of the relationship between the two photoreceptor systems awaits molecular analysis of the NPH1 gene.
Plastid Development
Chlorophyll accumulation and the concomitant transition of the proplastid or
etioplast to the chloroplast are arguably the most striking responses to light
and certainly require the intricate cooperation between multiple biochemical
assembly and disassembly processes. In several species, pretreatment with red
light, perceived at least partially by phyA and phyB, potentiates the accumulation of chlorophyll (74, 91). A feedback mechanism that conditions nuclear
gene expression for a subset of plastid proteins operates via a biochemically
undefined plastid signal, which is depleted by photooxidative damage to the
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plastid (36, 166, 167). At least part of this regulatory circuit involves an inhibitory element, because nuclear gene expression has escaped from the control by the plastid in recessive mutant alleles of at least three Arabidopsis
complementation groups (GUN1–GUN3) (165). These mutants have few morphological defects, but have the tendency to green inefficiently when they are
transferred from darkness to light in the etiolated state (165).
Mutant analysis has further demonstrated a panel of negative regulators,
which keep chloroplast development suppressed in the cotyledons of darkgrown seedlings. Mutations at each of 10 loci known as Constitutively Photomorphogenic (COP1, COP8–COP11), De-etiolated (DET1), and Fusca
(FUS4, 5, 11, and 12) result in the absence of etioplasts and in partial chloroplast development in complete darkness, accompanied by cotyledon expansion, arrest of hypocotyl elongation, and light-specific cell type differentiation
(24, 30, 32, 46, 48, 88a, 112, 116, 184, 185). The same loci also suppress
chloroplast development in the roots of light-grown seedlings, because the
mutants’ roots develop chloroplasts and turn green.
Mutations at several other loci affect overall organ development and expression of light-inducible genes during seedling morphogenesis without resulting in plastid differentiation. For examples, cop4 and det2, both of which
display significant derepression of light-inducible genes in darkness, have no
impact on chloroplast development (29, 68). A group of mutants at three loci,
known as DOC1, DOC2, and DOC3 (dark overexpressors of CAB) accumulate mRNA from the chlorophyll a/b binding protein gene (CAB) promoter in
darkness, without a conspicuous morphological phenotype (89). The complementary mutant phenotype, namely opening of the cotyledons on a short hypocotyl accompanied by continued repression of light-inducible genes in
darkness, has been described for the det3 mutant (19a). In this mutant chlorplast, development remains tightly controlled by light.
The particular combinations of phenotypic defects in the various mutants
described to date present a dilemma for the geneticist, because no simple linear sequence of gene action is consistent with all the data. While it is tempting
and straightforward to invoke feedback circuits in order to solve the problem,
detailed evidence for them is scarce. Elucidating the logic of the light signal
transduction events may therefore require the mechanistic dissection of the
function of the various gene products.
REGULATORS OF LIGHT RESPONSES IN SEEDLINGS
Positive Regulators
It is a recurring theme that predominantly negative regulators of photomorphogenic seedling development are uncovered in various genetic screens,
LIGHT CONTROL OF SEEDLING DEVELOPMENT
231
whereas genetic identification of the positive regulators is sparse (see Figure
1) (28, 45).
The prevalent coaction between pigment systems (52, 70, 117, 128, 171)
and, in particular, the partial redundancy inherent in multiple photoreceptor
systems may be two reasons for the difficulty of establishing mutants in positive regulators. Remarkable exceptions are the genes FHY1 and FHY3, which
result in phenotypes similar to phyA mutants. These gene products may act
downstream of PHYA in transmitting a signal specific for phytochrome A (71,
189). A fruitful approach to identifying specific regulators genetically may include screening for modifiers, suppressors or enhancers, of established photomorphogenic mutations. As an example, a suppressor of the Arabidopsis
phytochrome-deficient hy2 mutation (shy1) with some specificity for suppressing the phenotype under red rather than far-red light has been uncovered
(BC Kim, MS Soh, BJ Kang, M Furuya & HG Nam, personal communication).
A second promising line of research is to screen for mutants defective in
the light-dependent expression of specific genes. Following this rationale,
the CUE1 gene has been identified as a positive regulator of light-dependent
nuclear and plastid gene expression (89a). Similarly, expression of the gene
for chalcone synthase (CHS) and genes for related enzymes in the anthocyanin synthesis pathway is sensitized to light in the Arabidopsis mutant icx1
(68a).
The HY5 gene product integrates signals from multiple photoreceptors to
mediate inhibition of hypocotyl cell elongation in response to blue, red, and
far-red light, but not UV-B light (4, 28, 87). These light conditions have also
been shown to cooperate in abolishing the activity of COP1, a negative regulator of light responses (113). Mutations of COP1 and the positive light regulatory component HY5 exhibit an allele-specific interaction. Although a strong
allele of cop1 is epistatic over a mutant hy5 allele, hy5 can suppress the phenotype of the weak allele cop1-6. The suppression of the cop1-6 phenotype by
hy5 could be attributed to compensating alterations in the surfaces of two in-
Figure 1 Scheme change of the sequence of events leading from light perception to developmental
response. Examples for relevant gene products that have been identified by mutation are indicated.
Please note that developmental and hormonal signals can modulate the light response by affecting
any step of the sequence.
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VON ARNIM & DENG
teracting proteins (4). Molecular cloning of the HY5 gene should allow a direct test of this hypothesis.
Possible Roles of Plant Hormones
Many of the light-regulated seedling developmental responses, such as the inhibition of hypocotyl cell elongation (21, 101, 150), stem elongation (8), the
cell division in the shoot apex (33), opening of the apical hook (51), and the
induction or repression of nuclear gene expression, also respond to treatment
with one or more of a variety of plant hormones (38, 42, 56). We have briefly
alluded to possible contributions of ethylene and auxins to the control of
tropic responses (51, 55, 125, 130). The question arises how hormonal and
light effects are integrated with each other: Are hormones second messengers
in light responses? Or do they transmit another signal that shares a common
target with light? Or do they serve as integrators of distinct signaling pathways by “cross talk?”
CYTOKININS The relationship between light on the one hand and cytokinins
and giberellins on the other has received the most thorough attention. For example, control of a wheat kinase gene homolog (WPK4) by light may require the
presence of cytokinin, because a putative cytokinin antagonist (2-chloro-4cyclobutylamino-6-ethylamino-s-triazine) specifically prevented the induction
of WPK4 mRNA (148). Even more intriguing is that de-etiolation of dark-grown
Arabidopsis seedlings can be mimicked partially by supplementing seedlings
with cytokinins under defined laboratory conditions (33). Moreover, the typically light-inducible genes for a chlorophyll a/b binding protein (CAB) (64, 73)
and for chalcone synthase (CHS) (53, 88) were moderately activated by cytokinin treatment, although the effective levels of applied cytokinins were about tenfold higher than the endogenous level in these experiments. Tentative links
between a high cytokinin level and a suppressed etiolation response are suggested because of the correlation of a hook opening phenotype with a significantly elevated cytokinin level in the amp1 mutant, epistasis of amp1 over hy2
(25), and the aberrant response of det1 and det2 to cytokinin (33). However, endogenous cytokinin levels in dark- and light-grown seedlings and in det1 and
det2 mutants were not consistent with the notion that light signals are transmitted simply by a change in cytokinin concentration (33). Furthermore, an additive and probably independent co-action of cytokinin and light has been
demonstrated for the control of hypocotyl elongation (163a).
Cytokinin may act posttranscriptionally on CAB mRNA levels in Lemna
gibba, while light clearly has a transcriptional component, indicating independent and probably additive action of cytokinin and light (56, 57). Stimulatory effects by moderate concentrations of applied cytokinins on the expres-
LIGHT CONTROL OF SEEDLING DEVELOPMENT
233
sion of light-inducible, circadian clock–regulated genes have also been observed under light conditions, which again suggests additive effects (42, 43).
In conclusion, although light effects may not be mediated primarily by cytokinin levels, any drastic alteration of the cellular cytokinin level by any
stimulus other than light would be expected to modulate the seedling’s responsiveness to light.
Although both light and giberellins control hypocotyl elongation, e.g. in cucumber (101), and mesocotyl elongation, for example, in rice
(170), few genetic studies support the simple hypothesis that light acts through
altering the levels of active giberellins (145–147). However, alterations in phytochrome levels have been shown to affect giberellin levels in tobacco (72), Sorghum (58, 59), and Brassica (49). One phenotype of the long hypocotyl mutant
lh of cucumber, which has a deficiency in a B-type phytochrome and a constitutive shade avoidance response (100–102, 156), is an increase in the responsiveness to giberellin. Conversely, in the wild type, depletion of Pfr increases the
responsiveness to giberellin (101). Phytochrome may similarly inhibit the sensitivity of the rice mesocotyl to giberellin (170).
The careful dissection of the signaling chains for light on the one hand and
hormones on the other by use of defined mutations and by molecular and
physiological analysis will allow researchers to pry apart the intertwined pathways and will finally reveal the role of cytokinin, giberellins, and other hormones in the light control of seedling development.
GIBERELLINS
Repressors of Light-Mediated Development
PLEIOTROPIC COP, DET, AND FUS GENES Combined efforts in photomorphogenic mutant screens (cop or det mutants) and purple seed color screens (fusca
mutants) have yielded a set of at least ten loci that are required for the full establishment of the dark developmental pathway and suppression of photomorphogenic development in darkness. The ten loci have been designated as
COP1/FUS1, DET1/FUS2, COP8/FUS8, COP9/FUS7, COP10/FUS9,
COP11/FUS6, FUS4, FUS5, FUS11, and FUS12, and mutations in each result
in dark-grown seedlings with a pleiotropic de-etiolated or constitutively photomorphogenic phenotype (24, 32, 46, 88a, 116, 184, 185). The mutants display
chloroplast-like plastids containing thylakoid membrane systems and lacking a
prolamellar body in the dark-grown cotyledons and show a pattern of lightregulated gene expression in the dark resembling their light-grown siblings. The
wild-type COP/DET/FUS genes also contribute to the repression of photomorphogenic responses in seedling roots under light conditions, because greening
and chloroplast development have been consistently observed in the lightgrown mutants. The elevated expression of nuclear- and plastid-encoded lightinducible genes in the dark-grown mutants is a direct or indirect loss in the abil-
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VON ARNIM & DENG
ity to repress nuclear gene promoter activity as indicated by analysis of transgenic promoter-reporter gene fusions in the mutant backgrounds (29, 46, 184,
185). Consistent with a widespread evolution of COP/DET/FUS-like functions,
a pea mutant with light-independent photomorphogenesis (lip) has been described (60). On the basis of the recessive nature of those mutations and their
pleiotropic phenotype, it has been proposed that the photomorphogenic pathway constitutes the default route of development, whereas the etiolation pathway is an evolutionarily recent adaptation pioneered by the angiosperms (185).
It is important to point out that for certain light-regulated processes, the
pleiotropic COP/DET/FUS loci are clearly not required. For instance, severe
loss-of-function alleles of all ten loci seem to retain normal phytochrome control of seed germination (46, 88a, 185).
The immediate downstream target of any of the COP, DET, and FUS repressor molecules remains unknown. It is possible that they directly inhibit
the transcription of photosynthetic genes or that they modulate expression of
an intermediate set of regulatory genes, which in turn regulate the final target
genes. Some indirect evidence is consistent with the latter possibility. For example, COP1 is a regulator of the PHYA gene itself (46). Further, it was recently reported that the normally light-inducible homeobox gene ATH1 was
derepressed in dark-grown cop1 and det1 mutants (137). Together, ATH1 and
two other homeobox genes, ATHB-2 and -4, exhibit light-regulated expression
patterns (20, 137) and may act as downstream effectors of the COP/DET/FUS
proteins. In addition, the DNA binding factor CA-1, which binds to a region
of the CAB promoter important for light regulation, was absent in the det1-1
mutant allele, consistent with its function as a downstream target of inactivation by DET1 (79, 164).
OVEREXPRESSION STUDIES The molecular cloning of four pleiotropic
COP/DET/FUS loci (24, 47, 135, 183) permitted a direct test using overexpression studies of the genetic model that their gene products act as repressors of the
photomorphogenic pathway. To date, overexpression of COP1 has produced
the clearest evidence for a photomorphogenic suppressor (113). Moderate twoto fourfold overexpression resulted in two responses typical for the etiolation
pathway, namely, an elongation of the hypocotyl under blue and far-red light
and under a dark/light cycle and a reduction in cotyledon expansion under blue
light. These effects of COP1 overexpression under far-red or blue light resemble
those of the phyA or cry1/hy4 mutants, which supports the notion that COP1 acts
downstream of multiple photoreceptors (11, 113). Overexpression of COP9 resulted in a similar but less dramatic elongation of the hypocotyl, again most pronounced under blue and far-red light, although no inhibitory effect on cotyledon
cell expansion could be discerned (N Wei & X-W Deng, unpublished data).
Therefore, the overexpression results in general confirm the conclusion that the
LIGHT CONTROL OF SEEDLING DEVELOPMENT
235
pleiotropic COP/DET/FUS gene products are repressors of photomorphogenic
development.
REGULATION OF COP/DET/FUS ACTIVITY BY LIGHT Limited sequence identity
of COP9, COP11/FUS6, and DET1 to other eukaryotic protein sequences submitted in databases suggests that they participate in a highly conserved, but as
yet undefined, cellular process (24a). For COP1, sequence similarity to the
Ring-finger class of zinc binding proteins and the β-subunit of trimeric G proteins is consistent with a role as a nuclear regulator of gene expression (47). This
alone, however, does not clarify the mechanism of light regulation. COP1 and
COP9 protein are detected in dark-grown seedlings, when the proteins are active, and also in the light-grown seedlings, when they are photomorphogenically
inactive (112, 183). Similarly, DET1 mRNA is expressed in both dark- and
light-grown seedlings (135). Therefore, the light inactivation of DET1, COP1,
and COP9 is probably not mediated by the expression level but by some other
means of posttranslational regulation. Recent studies with COP1 and COP9
point out some interesting insights. Our laboratory has shown that COP9 is a
subunit of a large nuclear-localized protein complex whose apparent molecular
weight can be shifted upon exposure of dark-grown seedlings to light (183).
This may reflect light regulation of COP9 activity through modulation of
protein-protein interactions in the COP9 complex. While DET1 (135) and the
COP9 complex (N Wei & X-W Deng, unpublished data) appear to have the potential for nuclear localization, examination of the subcellular localization of fusion proteins between COP1 and β-glucuronidase (GUS) reporter enzyme
suggested that the nucleocytoplasmic partitioning of COP1 is regulated by light
in a cell type–dependent manner (178). In root cells, where COP1 is constitutively active and helps to repress chloroplast development (48), GUS-COP1 is
found in the nucleus under all light conditions. In hypocotyl cells, however,
GUS-COP1 is nuclear in darkness but excluded from the nucleus under constant
white light. Upon a switch in illumination conditions from darkness to light, the
protein slowly repartitions in the hypocotyl from a nuclear to a cytoplasmic location, and vice versa (178). Complementation of the cop1-mutant phenotype
by the GUS-COP1 transgene suggests that it is a functional substitute of COP1
(our unpublished data). GUS-COP1 nucleocytoplasmic repartitioning coincides with light-regulated developmental redifferentiation processes, but their
initiation clearly precedes any noticeable shift of GUS-COP1 (178). Further, the
kinetics of repartitioning seem independent of the presence or absence of wildtype COP1 in the genetic background (our unpublished data). It is therefore
likely that COP1 relocalization serves to maintain a developmental commitment that has previously been communicated to the cell by means other than
COP1 partitioning.
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VON ARNIM & DENG
Evidence for a role of the cytoskeleton in modulating COP1 partitioning
has been obtained following the isolation of a COP1-interacting protein, CIP1
(105). The subcellular localization of CIP1 is cell type–dependent. While
CIP1 shows a fibrous, cytoskeleton-like distribution in protoplasts derived
from hypocotyl and cotyledons, it is localized to discrete foci in protoplasts
derived from roots. The cell type–dependent localization pattern of CIP1 may
provide a mechanism to regulate access of COP1 to the nucleus by specific
protein-protein interactions with a cytoplasmic anchor protein (105).
CONCLUSION
In the past few years a combination of molecular genetic, biochemical, and
cell biological studies has brought us remarkable progress in defining the
critical players and their specific roles in mediating the light control of seedling development. The basic network of signaling events seems remarkably
conserved throughout the angiosperm species examined. Therefore the focus
on a model organism will prove to be continuously fruitful.
How light signals perceived by distinct photoreceptors are integrated to
control cellular development and differentiation decisions may become a major focus in the coming years. A comprehensive understanding will not only
reveal the players involved but also how those players interact with other
stimuli, such as hormones, to reach a precise response according to the exact
light environmental cues. In particular, many decisions in the natural environment are not simply all-or-none but quantitative. Therefore, physiological
studies will probably play increasingly greater roles in the future work.
Moreover, individual light responses vary significantly among different species. Explaining the evolutionary flexibility on the basis of conserved modules
of protein function will be a major challenge in the future. In addition, most of
the key players identified to date seem to be present in most if not all cell
types, though each cell type produces a distinct response to a particular light
stimulus. Answers to the questions presented here will bring further insights
into the light control of seedling development.
ACKNOWLEDGMENTS
We thank Jeffrey Staub for a critical review of the manuscript and Peter Quail,
Ning Wei, Steve Kay, and Hong Gil Nam for communicating unpublished results. Research in this laboratory was supported by grants from the National
Science Foundation and by the National Institutes of Health.
Any Annual Review chapter, as well as any article cited in an Annual Review chapter,
may be purchased from the Annual Reviews Preprints and Reprints service.
1-800-347-8007; 415-259-5017; email: [email protected]
LIGHT CONTROL OF SEEDLING DEVELOPMENT
237
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