Survey
* Your assessment is very important for improving the workof artificial intelligence, which forms the content of this project
* Your assessment is very important for improving the workof artificial intelligence, which forms the content of this project
Cell growth wikipedia , lookup
Cell encapsulation wikipedia , lookup
Cell culture wikipedia , lookup
Extracellular matrix wikipedia , lookup
Endomembrane system wikipedia , lookup
Signal transduction wikipedia , lookup
Tissue engineering wikipedia , lookup
Cellular differentiation wikipedia , lookup
Cytokinesis wikipedia , lookup
Journal of Experimental Botany, Vol. 64, No. 9, pp. 2579–2592, 2013 doi:10.1093/jxb/ert101 Advance Access publication 12 April, 2013 REVIEW PAPER Auxin and self-organization at the shoot apical meristem Massimiliano Sassi and Teva Vernoux* Laboratoire de Reproduction et Développement des Plantes, CNRS, INRA, ENS Lyon, UCBL, Université de Lyon, 46 Allée d’Italie, 69364 Lyon Cedex 07, France. * To whom correspondence should be addressed: Email: [email protected] Received 8 February 2013; Revised 7 March 2013; Accepted 13 March 2013 Plants continuously generate new tissues and organs throughout their life cycle, due to the activity of populations of specialized tissues containing stem cells called meristems. The shoot apical meristem (SAM) generates all the aboveground organs of the plant, including leaves and flowers, and plays a key role in plant survival and reproduction. Organ production at the SAM occurs following precise spatio-temporal patterns known as phyllotaxis. Because of the regularity of these patterns, phyllotaxis has been the subject of investigations from biologists, physicists, and mathematicians for several centuries. Both experimental and theoretical works have led to the idea that phyllotaxis results from a self-organizing process in the meristem via long-distance interactions between organs. In recent years, the phytohormone auxin has emerged not only as the central regulator of organogenesis at the SAM, but also as a major determinant of the self-organizing properties of phyllotaxis. Here, we discuss both the experimental and theoretical evidence for the implication of auxin in the control of organogenesis and self-organization of the SAM. We highlight how several layers of control acting at different scales contribute together to the function of the auxin signal in SAM dynamics. We also indicate a role for mechanical forces in the development of the SAM, supported by recent interdisciplinary studies. Key words: auxin, auxin signalling, mechanical forces, phyllotaxis, polar auxin transport, shoot apical meristem. Introduction One of the most striking differences between plants and animals lies in the regulation of their organogenetic capacity over time. Unlike most animals, in which organogenesis occurs during embryonic development, plants can form new organs throughout their life cycle. Post-embryonic development occurs thanks to specialized tissues containing stem-cell niches known as meristems. Plants possess different types of meristems that control both primary and secondary growth. Among the meristems controlling primary growth, the shoot apical meristem (SAM) is located at the apex of the shoot axis and is responsible for the generation of all the aerial organs, in particular leaves and flowers. The SAM is thus not only important for building up the plant architecture but also for plant photosynthetic uptake and reproductive fitness. The SAM is established during embryogenesis and remains active throughout the plant life, which can last for up to thousands of years, as in the case of the giant sequoia (Sequoiadendron giganteum). A high level of coordination between the reiterative process of organogenesis and the self-renewal activity of the stem cells is thus expected to maintain the SAM function over long periods of time. Coordination of cellular behaviours and cell fate is also evident when considering the spatio-temporal patterns of organogenesis at the SAM or phyllotaxis. Organs are indeed initiated sequentially and at relatively precise spatial positions in the SAM. A majority of plants, including the model species Arabidopsis thaliana, have a spiral phyllotaxis where organs are initiated one by one and at a 137° relative angle from the previous organ. The regularity of these patterns has intrigued not only biologists but also physicists and mathematicians for several centuries. Both experimental and theoretical works have led to the idea that phyllotaxis could arise from Abbreviations: CZ, central zone; IAA, indole-3-acetic acid; OC, organizing centre; PZ, peripheral zone; SAM, shoot apical meristem; TF, transcription factor. © The Author [2013]. Published by Oxford University Press [on behalf of the Society for Experimental Biology]. All rights reserved. For permissions, please email: [email protected] Downloaded from http://jxb.oxfordjournals.org/ at Smith College on July 9, 2014 Abstract 2580 | Sassi and Vernoux long-distance interactions between organs in a self-organization process. In this context, the phytohormone auxin is a central regulator of the SAM organogenetic capacities but also as an orchestrator of the spatio-temporal dynamics of the SAM patterning. After presenting some of the key molecular players involved in regulating SAM function, we will discuss here both the experimental and theoretical evidence for the implication of auxin in the control of organogenesis and self-organization of the SAM. We will highlight how several layers of control contribute together to the function of the auxin signal in SAM dynamics. We will also indicate a role for mechanical forces in SAM morphogenesis supported by recent interdisciplinary studies. Cellular organization and genetic regulation of the SAM Phyllotactic patterning as a self-organizing developmental process Phyllotaxis represents one of the most striking examples of geometrical regularities that can result from a developmental patterning process. In higher plants, different phyllotactic patterns can be observed, being defined by the number of organs formed at any given time and their relative spatial distribution. The geometry corresponding to each phyllotaxis is defined by precise mathematical rules. In the case of spiral phyllotaxis, the most common phyllotactic pattern, the divergence angle (i.e. the angle between two consecutive organs) approximates to 137.5°. This value corresponds to the golden Downloaded from http://jxb.oxfordjournals.org/ at Smith College on July 9, 2014 The structure of the SAM is relatively well conserved among angiosperms, on which this review will focus. In general, the SAM can be divided into an external layer called the tunica and an inner region called the corpus. These two regions are very well defined at a cellular level: the cells of the corpus divide without a preferential cell division plane, whereas the cells of the tunica mostly divide anticlinally (i.e. perpendicular to the SAM surface), generating a typical layered structure, as daughter cells usually remain in the same layer as their parents. The tunica can be composed of several layers of cells (two in the case of Arabidopsis, named L1 and L2), and the layered organization is maintained only in the epidermal layer once the cells are recruited in organ primordia. Superimposed on the tunica–corpus organization, different domains of the meristem can also be defined based on the rates of cell growth and division. In the central zone (CZ) of the SAM, cells divide infrequently and grow at a low rate. By contrast, in the peripheral zone (PZ) surrounding the CZ, cells grow and divide at much higher rates. The PZ corresponds to the organogenetic domain of the SAM. As soon as the organ primordia starts to bulge out, as a result of the increase in cell proliferation and growth of a small number of founder cells, another group of cells at the proximal end of the organ will slow down their growth rates. These cells will form the boundary between the organ and the SAM, providing a physical separation between these two structures (Traas and Doonan, 2001). Specific gene expression patterns also define functional regions in the SAM that partly overlap with the zonation of the SAM based on the structural organization and cellular behaviours. A large number of these genes have been identified from mutants affected in SAM function. We will present here only briefly the most important regulators, and we refer the reader to recent reviews for a more exhaustive view (Aida and Tasaka, 2006; Sablowski, 2007; Rast and Simon, 2008; Dodsworth, 2009; Perales and Reddy, 2012). The CZ is characterized by expression of the CLAVATA3 (CLV3) gene. CLV3 encodes a signalling peptide implicated in a well-defined self-regulatory feedback loop, composed of the CLV3 secreted ligand, a receptor signalling cascade implicating notably CLV1 and the WUSCHEL (WUS) homeodomain transcription factor (TF). The expression of CLV3 is specific to the stem cells found in the CZ. WUS is expressed in a small domain in the corpus of the SAM, below the stem cells. The WUS domain defines the organizing centre (OC), and WUS is involved in promoting the expression of CLV3. The CLV3 peptide directly binds the receptor kinase CLV1 and activates a signalling cascade that restricts the size of the OC underneath. This non-cell-autonomous regulatory network implicating antagonistic factors determines and maintains the integrity of the SAM stem-cell niche. Indeed, wus mutants are unable to maintain an active SAM, whereas the size of the SAM is dramatically increased in clv3 mutants (Laux et al., 1996; Mayer et al., 1998; Schoof et al., 2000; Brand et al., 2000; Ogawa et al., 2008; Yadav et al., 2011). To give rise to a new organ in the PZ, a group of cells loses its meristematic identity and acquire a new organ identity. The homeodomain TF SHOOT-MERISTEMLESS (STM), which plays a central role in meristem maintenance, is expressed throughout the SAM but is excluded from organ primordia (Endrizzi et al., 1996), and the loss of meristematic identity is in part achieved by repression of STM in the organ founder cells (Byrne et al., 2000; Heisler et al., 2005). In parallel, a number of transcriptional regulators are induced in the organ primordium and will determine organ fate and tissues identities. The expression of the TFs of the YABBY, KANADI, and HD-Zip III families regulates the patterning of the organ by establishing its dorso/ventral polarity (Bowman et al., 2002; Byrne, 2006), whereas the expression of AINTEGUMENTA (ANT) promotes organ growth at least partially by regulating cell proliferation (Mizukami and Fischer, 2000). The expression of the CUP-SHAPED COTYLEDON (CUC) TFs specifies the boundaries as soon as the primordium starts to bulge out and allows for the separation of the organ from the meristem (Furutani et al., 2004; Heisler et al., 2005). Moreover, the absolute expression level of LEAFY (LFY) determines whether the organ acquires a leaf (low LFY level) or a flower (high LFY level) identity (reviewed by Moyroud et al., 2010). This transcriptional programme is reiteratively started in the PZ at each time a new organ is formed. This implies a tight control of transcription in space and time in order to coordinate the continuous and regular production of the new organs in the SAM and to establish phyllotactic patterns. Auxin at the shoot apical meristem | 2581 Polar auxin transport and phyllotaxis at the SAM A possible mechanism explaining the inhibitory fields would be the diffusion or transport of a molecule that inhibits organogenesis (see, for example, Mitchison, 1977). However, so far, no such inhibitory molecule has been identified. By contrast, a number of experimental and theoretical evidence have shown that auxin is both necessary and sufficient for organ formation at the SAM and that polar auxin transport depletes auxin in the region surrounding an organ, thus creating inhibitory fields. After presenting the mechanisms that control polar auxin transport, we will discuss the data supporting this vision. The regulation of polar auxin transport The active polar transport of auxin in plant tissues has been the subject of intense investigation for several decades. The classical chemiosmotic hypothesis (Rubery and Sheldrake, 1974; Raven, 1975) proposed that the chemical properties of the natural occurring auxin indole-3-acetic acid (IAA) are at the basis of auxin transport in plants. As a weak acid, IAA charge is pH dependent: in acidic (pH 5.5) environments such as in the apoplast, IAA is protonated (IAAH) and can easily move and enter the cell via diffusion. At neutral intracellular pH, IAAH loses its proton and becomes ionized (IAA–). Due to its charge, IAA– is trapped inside the cells. The chemiosmotic hypothesis then predicts that auxin efflux from cells requires an active carrier-dependent transport and that the polarity of the efflux carrier determines the polarity of the auxin flux (Leyser, 2005; Vieten et al., 2007; Friml, 2010). Actually, several transmembrane carriers accounting for both cellular influx and efflux of auxin have been identified in Arabidopsis over the years. The cellular influx of auxin is mediated by the AUXIN RESISTANT1/LIKE AUX1 (AUX1/ LAX) family of amino acid permease-like proteins, whereas the efflux from the cells is controlled mainly by members of the PIN-FORMED (PIN) family of transmembrane proteins (Leyser, 2005; Vieten et al., 2007; Friml, 2010). Members of the subfamily B of ATP-binding cassette/P-glycoprotein (ABCB/ PGP) transporters have also been demonstrated to mediate cellular auxin efflux and to interact with PIN transporters at different levels (Blakeslee et al., 2007; Mravec et al., 2008). PIN proteins are transmembrane carriers that perform a rate-limiting step in auxin efflux (Petrásek et al., 2006). As implied by the chemiosmotic hypothesis, PIN carriers are localized polarly on the plasma membrane of the cells and their polar localization controls the direction of auxin transport (Wisniewska et al., 2006). Thus, by observing the patterns of PIN polar localization in a plant tissue, it is possible to predict the direction of the auxin movement. The regulation of polar PIN localization is still not fully understood, although possible mechanisms have been identified. PIN proteins undergo constitutive cycles of clathrin-mediated endocytocis and recycling back to the plasma membrane (Geldner et al., 2001; Dhonukshe et al., 2007). Endocytic recycling has been shown to allow for the polar localization of PINs after an initial apolar delivery of newly synthesized PIN proteins (Dhonukshe et al., 2008). Rapid changes in PIN polarity have been shown to be determined by a transcytosis-like mechanism in which, after an initial step of endocytosis, PIN proteins are recycled to a different polar targeting domain on the plasma membrane (Kleine-Vehn et al., 2008a, 2010). Moreover, reversible phosphorylation of PINs by the PINOID (PID) serine/threonine protein kinase and the regulatory subunits A of the protein phosphatase 2A (PP2AAs) has also been demonstrated to play a central role in the decision of targeting PINs to the apical versus the basal membrane of cells (Friml et al., 2004; Michniewicz et al., 2007). In particular, it was recently proposed that phosphorylation via PID and related AGC3 kinases WAG1 and WAG2 recruits PINs into an apical recycling pathway as opposed to the default basal recycling that occurs in the absence of phosphorylation (Dhonukshe et al., 2010). While PIN proteins regulate auxin distribution within a tissue, auxin can in turn regulate PIN activity in several different Downloaded from http://jxb.oxfordjournals.org/ at Smith College on July 9, 2014 angle defined from the Fibonacci series. Each term of the Fibonacci series is given by the sum of the two previous ones (mathematically defined by in=in–1 + in–2; i0=i1=1). The golden angle is then the smaller angle resulting from the division of the circumference of a circle according to the value of the limit of the series obtained by dividing two consecutive terms of the Fibonacci series, this value being known as the golden ratio. Spiral phyllotaxis also generates a geometric distribution of organs at the apex where higher-order clockwise and counterclockwise spirals, known as contact parastichies, can be visualized by connecting adjacent organs. The number of contact parastichies generated by a SAM generally corresponds to two consecutive terms of the Fibonacci series (Reinhardt, 2005a,b; Kuhlemeier, 2007). The seminal experiments from Snow and Snow, more recently re-explored using modern laser-ablation approaches, have suggested that existing organs inhibit the formation of new primordia in their vicinity (Snow and Snow, 1931; Reinhardt et al., 2005). These results, together with the observation that a new primordium forms in the largest available space in the SAM (Höfmeister 1868), have fuelled the formulation of a number of theoretical models, collectively known as inhibitory field models (reviewed by Adler et al., 1997). These models postulate that organs generate inhibitory fields that prevent new organ initiation occurring in their vicinity. Among these, abstract dynamic models are sometimes considered as a paradigm for phyllotaxis (Shipman and Newell, 2005) and have been instrumental in exploring the putative role of inhibitory fields in the dynamics of phyllotaxis (Douady and Couder, 1996a,b,c). Indeed, computer simulations using dynamic models of inhibitory fields suggest that both the interval of time between organ initiations (the plastochrone) and the relative spatial position of the organs emerges from the local repulsive interactions of organs and the growth in the SAM. In other words, this theoretical work suggests that the formation of regular phyllotactic patterns is a self-organizing process that only requires inhibitory fields produced by organs. 2582 | Sassi and Vernoux PIN1-mediated polar auxin transport is essential for organ initiation and phyllotaxis Although the Arabidopsis genome encodes at least five PIN efflux carriers active at the plasma membrane, only PIN1 plays a non-redundant role in auxin distribution at the SAM. While pin1 mutants are able to form leaves during the vegetative stage (Guenot et al., 2012), they hardly produce any lateral organs after the transition to the reproductive stage, resulting in pin-like inflorescences (Okada et al., 1991; Gälweiler et al., 1998; Vernoux et al., 2000; Reinhardt et al., 2000). This indicates a limiting role both for PIN1 in auxin transport and for auxin transport in organ initiation at the inflorescence SAM, while other mechanisms might be at work in the vegetative SAM. Moreover, local application of exogenous auxin at the periphery of the inflorescence SAM induces de novo primordium formation in pin1 mutants (Reinhardt et al., 2000, 2003). This suggests not only that auxin is necessary and sufficient to trigger organ initiation but also that polar auxin transport leads to auxin accumulation at the site of the incipient primordium, thus providing instructions for organogenesis. PIN1 has been shown to be expressed predominantly in the L1 layer and in the provascular cells in the SAM (Vernoux et al., 2000; Reinhardt et al., 2003; Benková et al., 2003; Heisler et al., 2005; Barbier de Reuille et al., 2006). Patterns of PIN1 polarity and expression on the SAM surface are highly dynamic but are also stereotypical at the location of the incipient primordia and early developing organ: PIN1 pumps converge towards the forming organ, delimiting a small cluster of cells that display higher PIN1 expression levels without a clear polarity (Heisler et al., 2005; Barbier de Reuille et al., 2006). These cells will be connected with the inner PIN1-expressing provascular tissue at a slightly later stage (Benková et al., 2003; Reinhardt et al., 2003; Heisler et al., 2005). The PIN1 patterns in the L1 around organs suggest that polar auxin transport concentrates auxin at the site of the primordium formation, thus providing a mechanism for auxin accumulation. This scenario is supported by the upregulation of the synthetic auxin-inducible DR5 marker during organ initiation, indicating an activation of auxin signalling (Benková et al., 2003; Heisler et al., 2005; Barbier de Reuille et al., 2006; Smith et al., 2006), and by the results of computer simulations predicting auxin distribution in the SAM based on the connectivity of the PIN1 network (Barbier de Reuille et al., 2006). More recently, the DII-VENUS synthetic auxin sensor, which was obtained by fusing the auxin-binding domain of an Aux/IAA (see below) to a nuclear-targeted fastmaturating YFP (VENUS), allowed clear demonstration of an accumulation of auxin starting from the earlier steps of organ initiation (Vernoux et al., 2011; Brunoud et al., 2012). If the primordium acts as a sink, attracting auxin from the neighbouring cells through PIN1-mediated auxin transport, this suggests that an auxin-depleted region surrounding the primordium will be generated (Reinhardt et al., 2003; Heisler et al., 2005; Barbier de Reuille et al., 2006). As a result, organ formation will be inhibited in this auxin-depleted region. Observation of the PIN1 polarity patterns thus leads to the proposal that polar auxin transport could control not only accumulation of auxin at the site of organ initiation but also the creation of inhibitory fields around organs (Reinhardt et al., 2003; Reinhardt, 2005a,b). In this scenario, polar auxin transport alone would drive phyllotaxis through a tight spatio-temporal control of auxin distribution in the SAM. Analysing the DII-VENUS signal indeed confirmed this depletion of auxin around the organ, starting from organ initiation onwards (Vernoux et al., 2011; Brunoud et al., 2012), thus providing strong experimental support to this hypothesis. It is interesting to note that the depletion of auxin around organs closely correlates with the expression of boundary genes such as the CUC genes (Vernoux et al., 2000; Heisler et al., 2005) and the specification of the organ boundary identity might participate in inhibiting organogenesis close to existing organs. Finally, further supporting the role of polar auxin transport in the control of phyllotaxis, the AUX1/ LAX-dependent auxin influx has been shown to play a role in promoting organ separation and stabilizing phyllotactic patterning against environmental fluctuations (Reinhardt et al., 2003; Bainbridge et al., 2008). Although AUX1/LAX influx carriers do not display clear cellular polarity, they are thought to facilitate PIN1-mediated polar transport, notably by conveying auxin from the inner tissues to the L1 layer (Reinhardt et al., 2003; Bainbridge et al., 2008). Cell-based models suggest that phyllotaxis emerges from the dynamics of PIN1 polarities The dynamics of PIN1 pumps could thus explain the phyllotactic patterning, but there are two key questions. How is this process coordinated throughout the SAM? And how can PIN1 polarity precisely reorient to determine the next site of primordium formation? Despite the substantial knowledge on the molecular mechanisms of PIN polarization at a cellular level, an overall mechanistic view of how this process Downloaded from http://jxb.oxfordjournals.org/ at Smith College on July 9, 2014 ways. Auxin has been shown to inhibit PIN endocytosis, thus enhancing its own efflux from the cell (Paciorek et al., 2005). The AUXIN BINDING PROTEIN 1 (ABP1) protein acts as an extranuclear auxin receptor and has been implicated in this regulation. In particular, ABP1 has been shown to inhibit clathrin-mediated endocytosis at the plasma membrane upon auxin binding (Robert et al., 2010). On the other hand, nuclear auxin signalling through the TRANSPORT INHIBITOR RESISTANT 1/AUXIN SIGNALLING F-BOX (TIR1/AFB) receptors (see below) has been shown to regulate the abundance of PINs by controlling both the transcriptional activity of the genes and the turnover of proteins (Vieten et al., 2005; Abas et al., 2006; Kleine-Vehn et al., 2008b; Baster et al., 2012). In some tissues, auxin has also been shown to promote shifts in PIN polarity in a TIR1/ AFB-dependent fashion (Sauer et al., 2006). Such feedback regulations between auxin and PINs are thought to be crucial for the establishment and maintenance of the instructive auxin gradients that regulate several developmental processes including organogenesis at the SAM (Benjamins and Scheres, 2008; Vanneste and Friml, 2009) Auxin at the shoot apical meristem | 2583 and can favour one mechanism depending on the intracellular auxin content. As a result, cells with low auxin concentration will promote a concentration-based transport mode, whereas cells with high auxin concentration will activate a flux-based mechanism. This combined model was also able to reproduce realistically PIN polarization behaviour in different transport-dependent developmental contexts (Bayer et al., 2009). To date, all the theoretical models that have been developed assume the existence of hypothetical molecular components that can sense extracellular auxin or the intensity of the auxin flux through the membrane and direct PIN polarization. These models clearly show that a cellular feedback loop between auxin and the polarity of PIN1 is a plausible mechanism to explain the emergence of a phyllotactic pattern and self-organization in the SAM. However, they do not permit conclusions on the actual mechanisms involved. A recent computational study might provide some first answers and support canalization as a plausible scenario explaining polarization of PINs in a multicellular context. Wabnik et al. (2010) tested whether the modulation of PIN trafficking by an extracellular auxin receptor could lead to PIN polarization as postulated in the canalization hypothesis. The authors hypothesized that auxin binding to its receptor in the apoplast (ABP1 being an obvious candidate for such a receptor) immobilizes the receptor and triggers inhibition of PIN internalization in the nearest cell, increasing the efflux locally. As two neighbouring cells compete for auxin receptors in their common walls, this model can lead to an asymmetric PIN internalization in the two facing membranes. The authors also included in the model the regulation of PIN transcription by auxin through nuclear signalling and auxin transport through both the influx and efflux carriers. The authors demonstrated that their model can reproduce PIN-driven vascular formation in leaves and during vascular tissue regeneration in stem, two biological contexts that are easily explained using the canalization hypothesis (Wabnik et al., 2010). A key characteristic of the model used in this work is that PIN polarization is driven by concentration sensors and not flux sensors, and still the model appears to be able to simulate canalization. It remains to be established whether the mechanism proposed by Wabnik et al. (2010) formally behaves like a canalization model and whether it also functions for phyllotaxis. This point is notably important, as analysis of the role of mechanics in the SAM (which we will discuss later) rather supports the concentration-based models of phyllotaxis. However, this work suggests that building mechanistic models in parallel with the exploration of the cellular mechanisms controlling PIN polarity holds the key to the understanding of the selforganizing properties of the PIN1 network. In this context, it should be stressed that the different PIN1-based models of phyllotaxis are prone to instabilities (Jönsson et al., 2006; Smith et al., 2006; Stoma et al., 2008) and that this might be in part due to our partial knowledge of the PIN1 polarization mechanisms. However, beyond that, it could also be because other mechanisms regulating auxin homeostasis have been left out. For example, none of the models have considered a positive-feedback Downloaded from http://jxb.oxfordjournals.org/ at Smith College on July 9, 2014 is developmentally regulated at the tissue level is still missing. Among the known regulators of PIN polarity, only PID has been shown to play a role in organogenesis at the SAM (Christensen et al., 2000; Friml et al., 2004). PID is expressed specifically in organ boundaries (Christensen et al., 2000; Furutani et al., 2004) and is unlikely to account for the complex dynamics of PIN polarization that underlie phyllotaxis (Vernoux et al., 2010). To overcome the limited biological information, and inspired by the self-organization properties predicted by the dynamical models of phyllotaxis, a number of cell-based theoretical models have been developed to test whether the PIN1 network self-organizes, and to explore plausible scenarios that could explain self-regulatory properties of the auxin transport system in the SAM (reviewed by Wabnik et al., 2011). Such models have been developed on the basis of very simple hypotheses. A first set of models, inspired by the seminal work of Tsvi Sachs (1969) on vascular development, is based on the assumption that cells can perceive the flux of auxin across the plasma membrane and enhance it by polarizing the efflux carriers in the direction of the preexisting flow (flux-based models). Such a feedback mechanism (canalization hypothesis) has the potential to canalize auxin transport from sites with high hormone concentration toward sites with low hormone concentration (Mitchison et al., 1981). Although an auxin flux sensing mechanism remains to be demonstrated (see below), flux-based models can accurately predict PIN expression domains in the leaf vasculature similar to those that have been observed experimentally (Rolland-Lagan and Prusinkiewicz, 2005; Scarpella et al., 2006). For phyllotactic patterning, Stoma et al. (2008) had to postulate two different canalization regimes (i.e. two different feedback functions linking auxin flux to PIN protein insertion in membranes) in order to explain polarization of PIN1 towards sites of high auxin concentration during organogenesis. The weak regime (linear function) is active on the SAM surface, while the strong regime (quadratic function) is active in the provasculature underneath. With the assumption that, once established, sites of high auxin concentration act as sink by pumping auxin downwards by triggering the establishment of provascular cells, the model can predict PIN1 polarization towards the auxin gradient and the formation of inhibitory fields around the organ, as well as PIN1 polarization in the provasculature (Stoma et al., 2008). A second type of model was based on the hypothesis that, in a cell, PIN1 polarizes towards the cell neighbour that possesses the highest concentration of auxin (concentration-based models). Simulations using concentrationbased models could reproduce realistic PIN1 polarization and phyllotactic patterns in the SAM (Jönsson et al., 2006; Smith et al., 2006). As such, concentration-based models can also predict phyllotactic patterning, implying that flux-based mechanisms must co-exist in the plant to regulate other auxin transport-dependent patterning processes such provasculature development or leaf venation. Therefore, a third model, integrating both the concentration-based and fluxbased hypotheses was developed. This model assumes that cells are able to sense both auxin fluxes and concentrations 2584 | Sassi and Vernoux Spatio-temporal regulation of auxin signalling capacities also contributes to the SAM patterning The action of auxin in a patterning process depends not only on the distribution of auxin in a tissue but also on the cellular capacities to sense auxin and trigger specific transcriptional responses. Protein–protein interactions between the Aux/IAA and auxin response factors (ARF) transcriptional regulators are central to auxin signalling. There are 29 Aux/IAA genes that encode mostly short-lived repressors of auxin-induced transcription. The 23 ARF proteins can be either activators (the five Q-rich ARFs) or repressors of transcription. Aux/IAA and ARF proteins are able to form homo- and heterodimers both within and between the families. The instability of the Aux/IAAs is intrinsic to the so-called domain II, which interacts directly with SCFlike ubiquitin protein ligases harbouring TIR1 or one of the three related AFB F-box proteins (Dharmasiri et al., 2005a,b; Kepinski and Leyser, 2005; Tan et al., 2007). TIR1 and the AFBs act as auxin co-receptors together with the Aux/IAAs (Calderón-Villalobos et al., 2012), and their activation leads to auxin-dependent degradation of Aux/ IAAs. A model for auxin transduction is that Aux/IAAs dimerize with the ARF activators. These complexes bind to auxin-inducible genes, thus preventing transcription. By promoting the degradation of the Aux/IAAs, auxin would allow the ARFs to activate transcription. Most Aux/IAAs are themselves targets of the ARFs, thus establishing a negative-feedback loop. Treatment of pin1 meristems with exogenous auxin demonstrated that all the cells at the periphery of the meristem are competent to initiate organs in response to auxin (Reinhardt et al., 2000). However, auxin cannot trigger organogenesis at the centre of the meristem. Mutation in MONOPTEROS/ARF5 (MP/ARF5) induces a pin-like phenotype and also blocks the ability of the PZ cells to respond to exogenous auxin (Hardtke and Berleth, 1998; Reinhardt et al., 2003). MP/ARF5 has been shown to exert its function in organogenesis, in part, by directly inducing, in an auxin–dependent manner, the expression of LFY, ANT, and ANT-like 6 (AIL6) TFs (Yamaguchi et al., 2013). As MP/ ARF5 is only expressed at the meristem periphery (Hardtke and Berleth, 1998; Yamaguchi et al., 2013), the competence for organ initiation at the periphery of the meristem thus depends, at least in part, on a spatial modulation of auxin signal transduction. Using mostly in situ hybridization, a recent study identified TIR1, AFB1, and AFB5 and over 20 Aux/IAAs and ARFs as the effectors of auxin perception and signalling in the SAM. This analysis also demonstrated that most of these regulators are expressed differentially in the SAM, with a low expression at the centre of the SAM and high expression in the PZ. Notably, both ARF repressor and ARF activator expression followed this general trend. A full Aux/IAA–ARF interactome was obtained using a yeast twohybrid approach, and knowledge on the topology of the Aux/ IAA–ARF auxin signalling pathway was used to develop a mathematical model of the control of gene transcription by auxin in the SAM. This model predicted a role for the Aux/ IAA–ARF pathway in creating a differential sensitivity to auxin between the centre and the periphery of the SAM, together with a capacity to buffer fluctuations in the auxin signal to stabilize the transcriptional response. These two predictions could be validated by analysing the differences between the spatio-temporal patterns of fluorescence of DIIVENUS and DR5 (Vernoux et al., 2011). This work shows that the spatial distribution of ARF genes in the SAM is essential to restrict high transcriptional responses to auxin (including Aux/IAA expression) at the periphery of the meristem and is essential to the definition of the two main functional domains of the SAM, the CZ and the PZ. In addition, the role of the signalling pathway in stabilizing transcriptional responses to auxin probably contributes to the robustness of patterning at the SAM and thus of phyllotaxis (Vernoux et al., 2011). The dynamics of morphogenesis at the SAM thus appear to result from a dynamic integration of both spatial distribution of the auxin signal and local signalling capacities in the spatial control of morphogenesis (Fig. 1), similarly to what has been observed recently Downloaded from http://jxb.oxfordjournals.org/ at Smith College on July 9, 2014 mechanism between auxin transport and its biosynthesis that is supported by experimental evidence (Ljung et al., 2001; Cheng et al., 2007). Recent breakthrough experiments have shown that auxin biosynthesis is regulated mainly through a two-step pathway implicating the production of indole-3-pyruvic acid from tryptophan by members of the TRYPTOPHAN AMINOTRANSFERASE OF ARABIDOPSIS (TAA) family, followed by the conversion of indole-3-pyruvic acid to IAA by YUCCA (YUC) flavin monooxygenase-like proteins (Mashiguchi et al., 2011; Won et al., 2011). Several yuc mutant combinations display leaf and inflorescence developmental defects (Cheng et al., 2006). Pin-like structures are also observed in the yuc1,2,4,6 quadruple mutant and the expression patterns of the YUC genes indicate that the YUC pathway regulates lateral organ initiation and development of spatial and temporal control of auxin biosynthesis. Cheng et al. (2007) further observed that combining the pin1 mutation with yuc1 and yuc4 mutations enhanced the pin1 organogenesis phenotype, suggesting a coordinated action between auxin transport and biosynthesis in the SAM. Feedback between auxin transport and biosynthesis could provide robustness to the auxin distribution dynamics. Indeed, the expression YUC1 and YUC4 in the SAM is under the control of the AP2 transcription factors of the PLETHORA (PLT) family (Pinon et al., 2013). It was proposed that phyllotactic defects observed in the plt3plt5plt7 mutants arise from a perturbation in auxin biosynthesis in the SAM, which, in turn, alters PIN1 accumulation at the sites of incipient primordia (Pinon et al., 2013). Further work on the spatial control of auxin biosynthesis and incorporating auxin biosynthesis into the computational models of phyllotaxis are likely to be crucial in refining our understanding of the auxin-dependent self-organizing properties of patterning in the SAM. Auxin at the shoot apical meristem | 2585 for morphogen-driven developmental patterning in animal systems (Kicheva et al., 2012). Feedback between auxin-mediated patterning and morphogenesis: a role for biomechanics Cell-wall properties and morphogenesis at the SAM As discussed above, the coordinated regulation of auxin transport and signalling provides instructions for patterned organogenesis at the SAM. Such instructions will determine local changes in cell growth that underlie primordium formation, but how is this achieved? How are the initial instructions translated into a final shape? Plant cells are linked together by the cell wall, which prevents cell sliding and migration, and thus plant morphogenesis is the result of the coordination between localized cell division and selective cell growth (Somerville et al., 2004; Cosgrove, 2005). At the cellular level, growth is determined by the concerted action of the turgor pressure of the protoplasm and the mechanical properties of the cell wall. A plant cell can be abstracted as an inflated balloon inside a rigid but deformable box: the pressure inside the balloon will drive the growth of the whole structure if it can overcome the physical resistance of the box. As such, the water uptake into the plant cell will increase the turgor pressure, which, in turn, will trigger the extension of the pre-existing cell wall. At the same time, new polymers are synthesized by the cell and delivered to the wall to avoid an excessive thinning and weakening of the structure (Cosgrove, 2005; Murray et al., 2012). At the biochemical level, the cell wall is composed of stiff polysaccharides made of cellulose microfibrils that are embedded and cross-linked in a matrix of hemicelluloses, pectins, and structural proteins: the chemical interactions between these components are commonly thought to determine the mechanical properties of the cell wall (for reviews on cell-wall biochemistry, see Somerville et al., 2004; Cosgrove, 2005). The irreversible extension of the cell wall during growth (loosening) has so far been associated with acidic conditions and the activity of some wall-loosening proteins such as expansins that cleave the cross-links between polysaccharides complexes, causing wall relaxation (Cosgrove, 2005; Murray et al., 2012). Auxin-mediated cell growth has classically been Downloaded from http://jxb.oxfordjournals.org/ at Smith College on July 9, 2014 Fig. 1. Multiple feedback loops acting across different scales drive auxin-driven organ formation at the SAM. Auxin accumulation in cells at specific locations of the PZ in the SAM triggers both TIR1/AFB- and ABP1-mediated signalling. The activation of cellular auxin responses promotes: (1) PIN1-mediated auxin efflux that will in turn influence polar auxin transport patterns in the SAM; and (2) the level of auxin biosynthesis in the SAM. These will in turn feed back on the patterns of auxin accumulation amplifying the local growth responses that promote organ formation. 2586 | Sassi and Vernoux The process of morphogenesis is not only determined by the growth rates of the cells within a tissue, as oriented cell expansion along a preferential axis (anisotropy) also plays an important role in the acquisition of the final shape (Coen et al., 2004; Baskin, 2005; Murray et al., 2012). At a cellular level, anisotropy is established via the spatial distribution of the microfibrillar component of the cell wall. In fact, the ordered deposition of cellulose microfibrils in transverse hoops around the cell will direct the growth towards the axis that is perpendicular to the orientation of cellulose deposition (Lloyd and Chan, 2004). Compelling evidence indicates that the microtubular cytoskeleton plays an important role in determining cell anisotropy: microtubules control the insertion and movement of cellulose synthase complexes on the plasma membrane, thereby guiding the spatial deposition of cellulose microfibrils in the cell wall (Paredez et al., 2006; Crowell et al., 2009; Gutierrez et al., 2009; Bringmann et al., 2012; Li et al., 2012). The functional link between microtubules and cellulose deposition provides an easy way to investigate the contribution of anisotropy to plant morphogenesis. Microtubules can easily be tagged with fluorescent proteins, allowing indirect visualization of cellulose deposition and growth anisotropy in the SAM in live imaging experiments (Hamant et al., 2008; Heisler et al., 2010; Uyttewaal et al., 2012). Moreover, the use of microtubule-depolymerizing drugs as well as of mutants with defective microtubule dynamics allow easy manipulation of the growth anisotropy (Hamant et al., 2008; Uyttewaal et al., 2012). By using a combination of these experimental approaches, it was demonstrated that growth anisotropy plays a relevant role in morphogenesis at the SAM. Ordered microtubule alignment marks the boundary cells that physically separate the SAM and the primordium (Hamant et al., 2008; Uyttewaal et al., 2012). In the absence of microtubules, the tissue folding that allows organ separation from the SAM is abolished, despite a correct specification of the boundary cells (Hamant et al., 2008). Growth anisotropy was also shown to contribute to the pin-like shape of the SAM in the absence of organ formation. In a naked meristem, microtubules align circumferentially around the SAM periphery, imposing cell anisotropic growth along the vertical axis of the stem. When microtubules are depolymerized, growth becomes isotropic, leading the SAM to acquire a globular shape that has the geometric properties of soap froth (Grandjean et al., 2004; Hamant et al., 2008; Corson et al., 2009). Microtubules might mediate a mechanical feedback during morphogenesis While the mechanical changes associated with morphogenesis have classically been considered to be downstream of the genetic and biochemical inputs, an opposite trend proposing a direct role of mechanical forces on developmental patterning has been gaining strong support over the years (Selker et al., 1992; Hamant et al., 2010; Uyttewaal et al., 2010; Mirabet et al., 2011). The hypothesis of a biophysical patterning mechanism is based on the assumption that the SAM surface is under tension. This is because cells in the L1 Downloaded from http://jxb.oxfordjournals.org/ at Smith College on July 9, 2014 explained by the acid growth hypothesis: auxin would promote the acidification of the cell wall, presumably by activating some plasma membrane H+-ATPases that release protons outside the cell (Christian et al., 2006). The low cell-wall pH would in turn increase the activity of expansins, causing cellwall relaxation (Cosgrove, 2005; Sánchez-Rodríguez et al., 2010; Murray et al., 2012). While this mechanism would account for very fast and transcription-independent loosening responses, evidence also shows that auxin regulates the expression of a number of cell-wall-modifying proteins including expansins and pectin methyl estherases (PMEs) (Overvoorde et al., 2005), probably promoting sustained loosening effects. Concerning the SAM, an increasing amount of evidence suggests that cell-wall modifications underlie organ formation. First, local application of exogenous expansins on the SAM surface has been shown to promote the formation of outgrowths that do not develop into proper organs but have the potential to alter phyllotaxis (Fleming et al., 1997). More recently, PMEs and their inhibitors (PMEIs) have been involved in the control of SAM morphogenesis (Peaucelle et al., 2008, 2011). PMEs and PMEIs are thought to modify the fluidity of the pectin matrix and, in turn, the permeability to wall-loosening agents, presumably leading to softer or stiffer walls, respectively (Peaucelle et al., 2008). Accordingly, local PME treatments on the SAM surface could promote organ outgrowth, whereas PMEI overexpression inhibits organogenesis at the SAM, leading to pin-like phenotypes (Peaucelle et al., 2008). Together, these pieces of evidence suggest a scenario in which auxin accumulation at the site of incipient primordia triggers cell-wall loosening via acidic growth and subsequent induction of wall-modifying enzymes, thereby promoting organogenesis. This idea is further supported by recent measurements of cell-wall mechanical properties on the SAM surface, as well as by finite-element modelling, suggesting that the slow-growing cells at the top of the SAM might have stiffer cell walls compared with the fast-growing cells at the periphery (Milani et al., 2011; Kierzkowski et al., 2012). However, cell-wall remodelling might not occur only at the meristem surface. Changes in the cell-wall elastic properties of subepidermal cells at the site of incipient primordia have also been reported, suggesting that cell expansion is initiated in the internal cell layers (Peaucelle et al., 2011). These results are in line with previous works showing that transgenic expression of expansins in the inner tissues of the SAM is capable of initiating the entire programme of leaf development in tomato (Solanum lycopersicon) apices (Pien et al., 2001). While all these elements suggest an interesting framework that links auxin to cell-wall-controlled morphogenesis, it has to be pointed out that clear genetic evidence causally linking cell-wall loosening to in planta morphogenesis is still missing. However, auxin action on cell growth at the SAM might not be limited to cell-wall loosening, but might also involve changes in turgor pressure (Christian et al., 2006). An attractive hypothesis is that auxin could regulate the activity of aquaporins, as has been demonstrated recently for lateral root formation (Péret et al., 2012), although this remains to be proven in the SAM. Auxin at the shoot apical meristem | 2587 membrane have been shown to limit the lateral diffusion of PIN proteins, thus contributing in the maintenance of PIN polarity (Feraru et al., 2011). Along the same line, it has been shown that in tomato (S. lycopersicon) apices, PIN1 levels and intracellular localization can be altered by treatments that cause cell-wall deformation or that modify plasma membrane properties. These findings suggest that cell-wall deformations caused by mechanical stress are sensed via the plasma membrane and affect PIN1 intracellular localization, possibly by altering the endocytosis/exocytosis ratio (Nakayama et al., 2012). Taken together, these lines of evidence support a scenario in which morphogenesis is the result of the coordinated action not only of genetic and biochemical pathways but also of the mechanical forces at the SAM surface (Fig. 2). This vision is also supported by theoretical works that suggest a plausible scenario in which biophysical and biochemical mechanisms compete and cooperate to generate robust phyllotactic patterns: fluctuations of auxin concentrations could modify the mechanical properties of the L1, causing uneven tissue growth that would further alter the stress distribution, eventually driving changes in auxin distribution (Newell et al., 2008a,b). It is likely that only through the integration of both biochemical and mechanical pathways will the mechanisms controlling the dynamics of PIN polarization in SAM tissues be elucidated. Conclusions From the body of work we have discussed in this review, the SAM can be viewed as a typical complex system in which interactions between elements that constitute the system at a given scale (e.g. the cells) allow the emergence of a behaviour at a higher scale (e.g. the tissue). Phyllotaxis provides a perfect illustration of this vision: the dynamics of tissue patterning emerge from repulsive interactions between organs that are themselves determined by rules of signal exchange between individual cells. Auxin is a central signal that acts at these different scales, but it is probably not the only one. We have indeed seen that different feedback mechanisms are key to controlling the self-organization properties of the SAM system: feedback between auxin concentration or flux and the polarity of the PIN1 pumps, feedback between auxin transport and auxin biosynthesis that remain to be fully analysed, feedback between auxin and its signalling pathways, and feedback between auxin and the geometry of the tissue through mechanics. At this point, the complexity of this developmental system clearly exceeds what can be understood intuitively, explaining why modelling approaches have been so instrumental in extracting plausible hypotheses from the data. Thus, we anticipate that modelling will remain central in the analysis of SAM function and phyllotaxis, together with further dissections of the molecular mechanisms implicated. We have already discussed the fact that understanding the cellular mechanisms of PIN polarity and the control of auxin biosynthesis are likely to be crucial to understand how robust phyllotactic patterns can be generated. Concerning Downloaded from http://jxb.oxfordjournals.org/ at Smith College on July 9, 2014 layer are subject to an upward pressure caused by the turgor of inner cells. The unbalance between the inner turgor pressure and surface tension leads to the buckling of the L1 that underlies the formation of an organ. The resulting physical deformation of the SAM surface generates folded areas where organogenesis is prevented, thus generating physicsbased inhibitory fields (Selker et al., 1992; Green, 1996, 1999). Deformations of the SAM surface might arise at the cellular level when neighbouring cells grow at very different rates (i.e. boundary cells versus primordium cells), triggering changes in surface tension that could feed back on local cellexpansion rates (Murray et al., 2012). Hamant et al. (2008) indeed showed that microtubule alignment on the SAM surface matched the theoretical distribution of the main force directions, calculated on a purely geometrical basis. This would suggest that microtubules might sense, through an unknown mechanism, the physical stress on the SAM surface and align accordingly to guide the anisotropic cellulose deposition, thus counteracting the stress. As a result, the oriented microtubule pattern in boundary cells that underlies organ separation would be generated by the action of mechanical forces (Hamant et al., 2008). The idea that microtubules react to mechanical changes at the SAM surface is also supported by SAM compressions, laser ablations, and pharmacological treatments weakening the cell wall, which all trigger a reorientation within a few hours of the microtubules according to the predicted stress patterns generated by the treatments (Hamant et al., 2008; Heisler et al., 2010; Uyttewaal et al., 2012). This stress-driven microtubule reorientation has been shown to depend on the action of the microtubule-severing protein katanin (AtKTN1) (Uyttewaal et al., 2012). In addition, patterns of microtubule orientation at the SAM surface have also been suggested to feed back on the auxin transport system. Indeed, in SAM cells, a negative correlation between microtubule alignment and PIN1 polarity has been observed: PIN1 localizes to anticlinal walls parallel to the main microtubule orientation (Heisler et al., 2010). Although PIN localization is unlikely to be under the direct control of microtubules (Geldner et al., 2001; Heisler et al., 2010), PIN1 has been shown to lose its cellular polarity after long treatments with microtubule-depolymerizing drugs (Heisler et al., 2010). In addition, PIN1 also reorients its polarity away from wounded cells in laser-ablation experiments with a dynamic similar to that observed for microtubules (Heisler et al., 2010). This would suggest that mechanical forces might influence PIN polarity and, as a result, auxin transport patterns. Computer simulations showed that a mechanism that distributes PIN1 polarity according to cell-wall stress behaves like a concentration-based model for auxin transport and is indeed capable of generating phyllotactic patterns (Heisler et al., 2010). This is in contrast to the results of Wabnik et al. (2010), which instead support canalization, thus questioning again which mechanism best explains phyllotactic patterning. However, further supporting the idea of a mechanical control of the auxin transport system, evidence that the cell wall plays a role in determining PIN polarity has been reported. In particular, cellulose-based mechanical connections between the extracellular matrix and the polar domains of the plasma 2588 | Sassi and Vernoux the role of mechanics, it should be pointed out that the contribution of biophysical pathways to plant morphogenesis is still controversial, because of the difficulty of experimentally measuring mechanical forces in the SAM (Kuhlemeier, 2007; Besnard et al., 2011). New technological developments will be necessary to convincingly demonstrate the role of mechanical forces in phyllotaxis at the SAM alongside auxin. Sensor mechanisms for mechanical forces are also required and remain to be identified. Finally, it should be noted that the theoretical approaches to phyllotaxis have led to an idealistic view of this developmental process. However, it can be expected that the phyllotactic patterning will be prone to noise like any developmental system and will thus show a certain level of variability. Recent analyses have indeed demonstrated deviations from the Fibonacci angle in Arabidopsis (Peaucelle et al., 2007, Refahi et al., 2011), which probably reflect the impact of noise on phyllotaxis (Mirabet et al., 2012). A proper quantification of the dynamics of organ initiation at the SAM using, for example, data obtained from live imaging (Grandjean et al., 2004, Heisler et al., 2005, Fernandez et al., 2010) is undoubtedly necessary to define the characteristics of the phyllotactic system. Such an analysis will be crucial to evaluate the predictive capacities of the models that will be used to understand how the different levels of control, from auxin to mechanics, are integrated in the SAM to generate robust phyllotactic patterns. Acknowledgements We apologize to all colleagues whose original works could not be cited for space constraints. We would like to thank Olivier Hamant for critical reading of the manuscript. The work of the authors is funded by the Agence National de la Recherche and the iSAM ERASysBIO+ programme. References Abas L, Benjamins R, Malenica N, et al... 2006. Intracellular trafficking and proteolysis of the Arabidopsis auxin-efflux facilitator Downloaded from http://jxb.oxfordjournals.org/ at Smith College on July 9, 2014 Fig. 2. Cross-talks between auxin and mechanical signalling in the regulation of morphogenesis at the SAM. Auxin-induced cell-wall loosening is thought to cause mechanical stress that in turn feeds back on PIN1-mediated auxin transport to amplify local growth responses (see text for details). Dashed lines represent putative interactions: (1) auxin might also regulate the turgor pressure of the SAM cells, probably by modulating aquaporins activity, as observed recently in the process of lateral root formation (Peret et al., 2012); (2) the mechanical stresses that determine microtubule orientation (Hamant et al., 2008; Heisler et al., 2010; Uyttewaal et al., 2012) might be sensed via the plasma membrane, as proposed recently for the mechanical stress-driven changes in PIN1 intracellular distribution (Nakayama et al., 2012). Auxin at the shoot apical meristem | 2589 PIN2 are involved in root gravitropism. Nature Cell Biology 8, 249–256. Adler I, Barabe D, Jean R. 1997. A history of the study of phyllotaxis. Annals of Botany 80, 231–244. Calderón-Villalobos LI, Lee S, De Oliveira C, et al. 2012. A combinatorial TIR1/AFB-Aux/IAA co-receptor system for differential sensing of auxin. Nature Chemical Biology 8, 477–485. Aida M, Tasaka M. 2006. Morphogenesis and patterning at the organ boundaries in the higher plant shoot apex. Plant Molecular Biology 60, 915–928. Cheng Y, Dai X, Zhao Y. 2006. Auxin biosynthesis by the YUCCA flavin monooxygenases controls the formation of floral organs and vascular tissues in Arabidopsis. Genes & Development 20, 1790–1799. Bainbridge K, Guyomarc’h S, Bayer E, Swarup R, Bennett M, Mandel T, Kuhlemeier C. 2008. Auxin influx carriers stabilize phyllotactic patterning. Genes & Development 22, 810–823. Cheng Y, Dai X, Zhao Y. 2007. Auxin synthesized by the YUCCA flavin monooxygenases is essential for embryogenesis and leaf formation in Arabidopsis. Plant Cell 19, 2430–2439. Barbier de Reuille P, Bohn-Courseau I, Ljung K, Morin H, Carraro N, Godin C, Traas J. 2006. Computer simulations reveal properties of the cell-cell signaling network at the shoot apex in Arabidopsis. Proceedings of the National Academy of Sciences, USA 103, 1627–1632. Christensen SK, Dagenais N, Chory J, Weigel D. 2000. Regulation of auxin response by the protein kinase PINOID. Cell 100, 469–478. Baskin TI. 2005. Anisotropic expansion of the plant cell wall. Annual Review of Cell and Developmental Biology 21, 203–222. Bayer EM, Smith RS, Mandel T, Nakayama N, Sauer M, Prusinkiewicz P, Kuhlemeier C. 2009. Integration of transportbased models for phyllotaxis and midvein formation. Genes & Development 23, 373–384. Benjamins R, Scheres B. 2008. Auxin: the looping star in plant development. Annual Review of Plant Biology 59, 443–465. Benková E, Michniewicz M, Sauer M, Teichmann T, Seifertová D, Jürgens G, Friml J. 2003. Local, efflux-dependent auxin gradients as a common module for plant organ formation. Cell 115, 591–602. Besnard F, Vernoux T, Hamant O. 2011. Organogenesis from stem cells in planta: multiple feedback loops integrating molecular and mechanical signals. Cellular and Molecular Life Sciences 68, 2885–2906. Blakeslee JJ, Bandyopadhyay A, Lee OR, et al. 2007. Interactions among PIN-FORMED and P-glycoprotein auxin transporters in Arabidopsis. Plant Cell 19, 131–147. Bowman JL, Eshed Y, Baum SF. 2002. Establishment of polarity in angiosperm lateral organs. Trends in Genetics 18, 134–141. Brand U, Fletcher JC, Hobe M, Meyerowitz EM, Simon R. 2000. Dependence of stem cell fate in Arabidopsis on a feedback loop regulated by CLV3 activity. Science 289, 617–619. Bringmann M, Li E, Sampathkumar A, Kocabek T, Hauser MT, Persson S. 2012. POM-POM2/cellulose synthase interacting1 is essential for the functional association of cellulose synthase and microtubules in Arabidopsis. Plant Cell 24, 163–177. Brunoud G, Wells DM, Oliva M, et al. 2012. A novel sensor to map auxin response and distribution at high spatio-temporal resolution. Nature 482, 103–106. Byrne ME, Barley R, Curtis M, Arroyo JM, Dunham M, Hudson A, Martienssen RA. 2000. Asymmetric leaves1 mediates leaf patterning and stem cell function in Arabidopsis. Nature 408, 967–971. Byrne ME. 2006. Shoot meristem function and leaf polarity: the role of class III HD-ZIP genes. PLoS Genetics 2, e89. Coen E, Rolland-Lagan AG, Matthews M, Bangham JA, Prusinkiewicz P. 2004. The genetics of geometry. Proceedings of the National Academy of Sciences, USA 101, 4728–4735. Corson F, Hamant O, Bohn S, Traas J, Boudaoud A, Couder Y. 2009. Turning a plant tissue into a living cell froth through isotropic growth. Proceedings of the National Academy of Sciences, USA 106, 8453–8458. Cosgrove DJ. 2005. Growth of the plant cell wall. Nature Reviews Molecular Cell Biology 6, 850–861. Crowell EF, Bischoff V, Desprez T, Rolland A, Stierhof YD, Schumacher K, Gonneau M, Höfte H, Vernhettes S. 2009. Pausing of Golgi bodies on microtubules regulates secretion of cellulose synthase complexes in Arabidopsis. Plant Cell 21, 1141–1154. Dharmasiri N, Dharmasiri S, Estelle M. 2005a. The F-box protein TIR1 is an auxin receptor. Nature 435, 441–445. Dharmasiri N, Dharmasiri S, Weijers D, Lechner E, Yamada M, Hobbie L, Ehrismann JS, Jürgens G, Estelle M. 2005b. Plant development is regulated by a family of auxin receptor F box proteins. Developmental Cell 9, 109–119. Dhonukshe P, Aniento F, Hwang I, Robinson DG, Mravec J, Stierhof YD, Friml J. 2007. Clathrin-mediated constitutive endocytosis of PIN auxin efflux carriers in Arabidopsis. Current Biology 17, 520–527. Dhonukshe P, Huang F, Galvan-Ampudia CS, et al. 2010. Plasma membrane-bound AGC3 kinases phosphorylate PIN auxin carriers at TPRXS(N/S) motifs to direct apical PIN recycling. Development 137, 3245–3255. Dhonukshe P, Tanaka H, Goh T, et al. 2008. Generation of cell polarity in plants links endocytosis, auxin distribution and cell fate decisions. Nature 456, 962–966. Dodsworth S. 2009. A diverse and intricate signalling network regulates stem cell fate in the shoot apical meristem. Developmental Biology 336, 1–9. Douady S, Couder Y. 1996a. Phyllotaxis as a dynamical self organizing process. Part I: the spiral modes resulting from timeperiodic iterations. Journal of Theoretical Biology 178, 255–274. Downloaded from http://jxb.oxfordjournals.org/ at Smith College on July 9, 2014 Baster P, Robert S, Kleine-Vehn J, Vanneste S, Kania U, Grunewald W, De Rybel B, Beeckman T, Friml J. 2012. SCFTIR1/AFB-auxin signalling regulates PIN vacuolar trafficking and auxin fluxes during root gravitropism. EMBO Journal 32, 260–274. Christian M, Steffens B, Schenck D, Burmester S, Böttger M, Lüthen H. 2006. How does auxin enhance cell elongation? Roles of auxin-binding proteins and potassium channels in growth control. Plant Biology 8, 346–352. 2590 | Sassi and Vernoux Douady S, Couder Y. 1996b. Phyllotaxis as a dynamical selforganizing process. Part II: the spontaneous formation of a periodicity and the coexistance of spiral and whorled patterns. Journal of Theoretical Biology 178, 275–294. Douady S, Couder Y. 1996c. Phyllotaxis as a dynamical self organizing process. Part III: the simulation of the transient regimes of ontogeny. Journal of Theoretical Biology 178, 295–312. Endrizzi K, Moussian B, Haecker A, Levin JZ, Laux T. 1996. The SHOOT MERISTEMLESS gene is required for maintenance of undifferentiated cells in Arabidopsis shoot and floral meristems and acts at a different regulatory level than the meristem genes WUSCHEL and ZWILLE. The Plant Journal 10, 967–979. Feraru E, Feraru MI, Kleine-Vehn J, Martinière A, Mouille G, Vanneste S, Vernhettes S, Runions J, Friml J. 2011. PIN polarity maintenance by the cell wall in Arabidopsis. Current Biology 21, 338–343. Fleming AJ, McQueen-Mason S, Mandel T, Kuhlemeier C. 1997. Induction of leaf primordia by the cell wall protein expansin. Science 276, 1415–1418. Friml J. 2010. Subcellular trafficking of PIN auxin efflux carriers in auxin transport. European Journal of Cell Biology 89, 231–235. Friml J, Yang X, Michniewicz M, et al. 2004. A PINOID-dependent binary switch in apical-basal PIN polar targeting directs auxin efflux. Science 306, 862–865. Furutani M, Vernoux T, Traas J, Kato T, Tasaka M, Aida M. 2004. PIN-FORMED1 and PINOID regulate boundary formation and cotyledon development in Arabidopsis embryogenesis. Development 131, 5021–5030. Gälweiler L, Guan C, Müller A, Wisman E, Mendgen K, Yephremov A, Palme K. 1998. Regulation of polar auxin transport by AtPIN1 in Arabidopsis vascular tissue. Science 282, 2226–2230. Geldner N, Friml J, Stierhof YD, Jürgens G, Palme K. 2001. Auxin transport inhibitors block PIN1 cycling and vesicle trafficking. Nature 413, 425–428. Grandjean O, Vernoux T, Laufs P, Belcram K, Mizukami Y, Traas J. 2004. In vivo analysis of cell division, cell growth, and differentiation at the shoot apical meristem in Arabidopsis. Plant Cell 16, 74–87. Green PB. 1996. Transductions to generate plant form and pattern: an essay on cause and effect. Annals of Botany 78, 269–281. Green PB. 1999. Expression of pattern in plants: combining molecular and calculus-based biophysical paradigms. American Journal of Botany 86, 1059–1076. Guenot B, Bayer E, Kierzkowski D, Smith RS, Mandel T, Žádníková P, Benková E, Kuhlemeier C. 2012. PIN1-independent leaf initiation in Arabidopsis. Plant Physiology 159, 1501–1510. Gutierrez R, Lindeboom JJ, Paredez AR, Emons AM, Ehrhardt DW. 2009. Arabidopsis cortical microtubules position cellulose synthase delivery to the plasma membrane and interact with cellulose synthase trafficking compartments. Nature Cell Biology 11, 797–806. Hamant O, Traas J, Boudaoud A. 2010. Regulation of shape and patterning in plant development. Current Opinion in Genetics & Development 20, 454–459. Hardtke CS, Berleth T. 1998. The Arabidopsis gene MONOPTEROS encodes a transcription factor mediating embryo axis formation and vascular development. EMBO Journal 17, 1405–1411. Heisler MG, Hamant O, Krupinski P, Uyttewaal M, Ohno C, Jönsson H, Traas J, Meyerowitz EM. 2010. Alignment between PIN1 polarity and microtubule orientation in the shoot apical meristem reveals a tight coupling between morphogenesis and auxin transport. PLoS Biology 8, e1000516. Heisler MG, Ohno C, Das P, Sieber P, Reddy GV, Long JA, Meyerowitz EM. 2005. Patterns of auxin transport and gene expression during primordium development revealed by live imaging of the Arabidopsis inflorescence meristem. Current Biology 15, 1899–1911. Höfmeister W. 1868. Allgemeine Morphologie der Gewachse. In: de Bary A, Irmisch TH, Sachs J, eds. Handbuch der Physiologischen Botanik . Leipzig: Engelmann, 405–664. Jönsson H, Heisler MG, Shapiro BE, Meyerowitz EM, Mjolsness E. 2006. An auxin-driven polarized transport model for phyllotaxis. Proceedings of the National Academy of Sciences, USA 103, 1633–1638. Kepinski S, Leyser O. 2005. The Arabidopsis F-box protein TIR1 is an auxin receptor. Nature 435, 446–451. Kicheva A, Cohen M, Briscoe J. 2012. Developmental pattern formation: insights from physics and biology. Science 338, 210–212. Kierzkowski D, Nakayama N, Routier-Kierzkowska AL, Weber A, Bayer E, Schorderet M, Reinhardt D, Kuhlemeier C, Smith RS. 2012. Elastic domains regulate growth and organogenesis in the plant shoot apical meristem. Science 335, 1096–1099. Kleine-Vehn J, Dhonukshe P, Sauer M, Brewer PB, Wiśniewska J, Paciorek T, Benková E, Friml J. 2008a. ARF GEF-dependent transcytosis and polar delivery of PIN auxin carriers in Arabidopsis. Current Biology 18, 526–531. Kleine-Vehn J, Ding Z, Jones AR, Tasaka M, Morita MT, Friml J. 2010. Gravity-induced PIN transcytosis for polarization of auxin fluxes in gravity-sensing root cells. Proceedings of the National Academy of Sciences, USA 107, 22344–22349. Kleine-Vehn J, Leitner J, Zwiewka M, Sauer M, Abas L, Luschnig C, Friml J. 2008b. Differential degradation of PIN2 auxin efflux carrier by retromer-dependent vacuolar targeting. Proceedings of the National Academy of Sciences, USA 105, 17812–17817. Kuhlemeier C. 2007. Phyllotaxis. Trends in Plant Science 12, 143–150. Laux T, Mayer KF, Berger J, Jürgens G. 1996. The WUSCHEL gene is required for shoot and floral meristem integrity in Arabidopsis. Development 122, 87–96. Leyser O. 2005. Auxin distribution and plant pattern formation: how many angels can dance on the point of PIN? Cell 121, 819–822. Downloaded from http://jxb.oxfordjournals.org/ at Smith College on July 9, 2014 Fernandez R, Das P, Mirabet V, Moscardi E, Traas J, Verdeil JL, Malandain G, Godin C. 2010. Imaging plant growth in 4D: robust tissue reconstruction and lineaging at cell resolution. Nature Methods 7, 547–553. Hamant O, Heisler MG, Jönsson H, et al. 2008. Developmental patterning by mechanical signals in Arabidopsis. Science 322, 1650–1655. Auxin at the shoot apical meristem | 2591 Li S, Lei L, Somerville CR, Gu Y. 2012. Cellulose synthase interactive protein 1 (CSI1) links microtubules and cellulose synthase complexes. Proceedings of the National Academy of Sciences, USA 109, 185–190. Ljung K, Bhalerao RP, Sandberg G. 2001. Sites and homeostatic control of auxin biosynthesis in Arabidopsis during vegetative growth. The Plant Journal 28, 465–474. Ogawa M, Shinohara H, Sakagami Y, Matsubayashi Y. 2008. Arabidopsis CLV3 peptide directly binds CLV1 ectodomain. Science 319, 294. Okada K, Uedalb J, Komaki MK, Bell CJ, Shimura Y. 1991. Requirement of the auxin polar transport system in early stages of Arabidopsis floral bud formation. Plant Cell 3, 677–684. Overvoorde PJ, Okushima Y, Alonso JM, et al. 2005. Functional genomic analysis of the AUXIN/INDOLE-3-ACETIC ACID gene family members in Arabidopsis thaliana. Plant Cell 17, 3282–3300. Mashiguchi K, Tanaka K, Sakai T, et al. 2011. The main auxin biosynthesis pathway in Arabidopsis. Proceedings of the National Academy of Sciences USA 108, 18512–18517. Paciorek T, Zazímalová E, Ruthardt N, et al. 2005. Auxin inhibits endocytosis and promotes its own efflux from cells. Nature 435, 1251–1256. Mayer KF, Schoof H, Haecker A, Lenhard M, Jürgens G, Laux T. 1998. Role of WUSCHEL in regulating stem cell fate in the Arabidopsis shoot meristem. Cell 95, 805–815. Paredez AR, Somerville CR, Ehrhardt DW. 2006. Visualization of cellulose synthase demonstrates functional association with microtubules. Science 312, 1491–1495. Michniewicz M, Zago MK, Abas L, et al. 2007. Antagonistic regulation of PIN phosphorylation by PP2A and PINOID directs auxin flux. Cell 130, 1044–1056. Peaucelle A, Braybrook SA, Le Guillou L, Bron E, Kuhlemeier C, Höfte H. 2011. Pectin-induced changes in cell wall mechanics underlie organ initiation in Arabidopsis. Current Biology 21, 1720–1726. Milani P, Gholamirad M, Traas J, Arnéodo A, Boudaoud A, Argoul F, Hamant O. 2011. In vivo analysis of local wall stiffness at the shoot apical meristem in Arabidopsis using atomic force microscopy. The Plant Journal 67, 1116–1123. Peaucelle A, Louvet R, Johansen JN, Höfte H, Laufs P, Pelloux J, Mouille G. 2008. Arabidopsis phyllotaxis is controlled by the methyl-esterification status of cell-wall pectins. Current Biology 18, 1943–1948. Mirabet V, Besnard F, Vernoux T, Boudaoud A. 2012. Noise and robustness in phyllotaxis. PLoS Computational Biology 8, e1002389. Peaucelle A, Morin H, Traas J, Laufs P. 2007. Plants expressing a mir164-resistant CUC2 gene reveal the importance of postmeristematic maintenance of phyllotaxy in Arabidopsis. Development 134, 1045–1050. Mirabet V, Das P, Boudaoud A, Hamant O. 2011. The role of mechanical forces in plant morphogenesis. Annual Review of Plant Biology 62, 365–385. Mitchison GJ. 1977. Phyllotaxis and the Fibonacci series. Science 196, 270–275. Mitchison GJ, Hanke DE, Sheldrake AR. 1981. The polar transport of auxin and venation patterns in plants. Philosophical Transactions of the Royal Society of London B 295, 461–471. Mizukami Y, Fischer RL. 2000. Plant organ size control: AINTEGUMENTA regulates growth and cell numbers during organogenesis. Proceedings of the National Academy of Sciences, USA 97, 942–947. Perales M, Reddy GV. 2012. Stem cell maintenance in shoot apical meristems. Current Opinion in Plant Biology 15, 10–16. Péret B, Li G, Zhao J, et al. 2012. Auxin regulates aquaporin function to facilitate lateral root emergence. Nature Cell Biology 14, 991–998. Petrásek J, Mravec J, Bouchard R, et al. 2006. PIN proteins perform a rate-limiting function in cellular auxin efflux. Science 312, 914–918. Moyroud E, Kusters E, Monniaux M, Koes R, Parcy F. 2010. LEAFY blossoms. Trends in Plant Science 15, 346–352. Pien S, Wyrzykowska J, McQueen-Mason S, Smart C, Fleming A. 2001. Local expression of expansin induces the entire process of leaf development and modifies leaf shape. Proceedings of the National Academy of Sciences, USA 98, 11812–11817. Mravec J, Kubes M, Bielach A, Gaykova V, Petrásek J, Skůpa P, Chand S, Benková E, Zazimalova E, Friml J. 2008. Interaction of PIN and PGP transport mechanisms in auxin distribution-dependent development. Development 135, 3345–3354. Pinon V, Prasad K, Grigg SP, Sanchez-Perez GF, Scheres B. 2013. Local auxin biosynthesis regulation by PLETHORA transcription factors controls phyllotaxis in Arabidopsis. Proceedings of the National Academy of Sciences, USA 110, 1107–1112. Murray JAH, Jones A, Godin C, Traas J. 2012. Systems Analysis of Shoot Apical Meristem Growth and Development: Integrating Hormonal and Mechanical Signaling. The Plant Cell 24, 3907–3919. Rast MI, Simon R. 2008. The meristem-to-organ boundary: more than an extremity of anything. Current Opinion in Genetics & Development 18, 287–294. Nakayama N, Smith RS, Mandel T, Robinson S, Kimura S, Boudaoud A, Kuhlemeier C. 2012. Mechanical regulation of auxinmediated growth. Current Biology 22, 1468–1476. Raven JA. 1975. Transport of indoleacetic acid in plant cells in relation to pH and electrical potential gradients, and its significance for polar IAA transport. New Phytologist 74, 163–172. Newell AC, Shipman PD, Sun Z. 2008a. Phyllotaxis: cooperation and competition between mechanical and biochemical processes. Journal of Theoretical Biology 251, 421–439. Refahi Y, Farcot E, Guedon Y, Besnard F, Vernoux T, Godin C. (2011) A combinatorial model of phyllotaxis perturbations in Arabidopsis thaliana. In: 22nd Annual Symposium on Combinatorial Pattern Matching , Palermo, Italy, vol. 6661, 323–335. http:// www-sop.inria.fr/virtualplants/Publications/2011/RFGBVG11/. Last accessed date : March 26, 2013. Newell AC, Shipman PD, Sun Z. 2008b. Phyllotaxis as an example of the symbiosis of mechanical forces and biochemical processes in living tissue. Plant Signaling & Behavior 3, 586–589. Downloaded from http://jxb.oxfordjournals.org/ at Smith College on July 9, 2014 Lloyd C, Chan J. 2004. Microtubules and the shape of plants to come. Nature Reviews Molecular Cell Biology 5, 13–22. 2592 | Sassi and Vernoux Reinhardt D, Frenz M, Mandel T, Kuhlemeier C. 2005. Microsurgical and laser ablation analysis of leaf positioning and dorsoventral patterning in tomato. Development 132, 15–26. Reinhardt D. 2005a. Regulation of phyllotaxis. International Journal of Developmental Biology 49, 539–46. Reinhardt D. 2005b. Phyllotaxis—a new chapter in an old tale about beauty and magic numbers. Current Opinion in Plant Biology 8, 487–493. Reinhardt D, Mandel T, Kuhlemeier C. 2000. Auxin regulates the initiation and radial position of plant lateral organs. Plant Cell 12, 507–518. Reinhardt D, Pesce ER, Stieger P, Mandel T, Baltensperger K, Bennett M, Traas J, Friml J, Kuhlemeier C. 2003. Regulation of phyllotaxis by polar auxin transport. Nature 426, 255–260. Robert S, Kleine-Vehn J, Barbez E, et al. 2010. ABP1 mediates auxin inhibition of clathrin-dependent endocytosis in Arabidopsis. Cell 143, 111–121. Rubery PH, Sheldrake AR. 1974. Carrier-mediated auxin transport. Planta 121, 101–121. Sablowski R. 2007. Flowering and determinacy in Arabidopsis. Journal of Experimental Botany 58, 899–907. Sachs T. 1969. Polarity and the induction of organized vascular tissues. Annals of Botany 33, 263–275. Sánchez-Rodríguez C, Rubio-Somoza I, Sibout R, Persson S. 2010. Phytohormones and the cell wall in Arabidopsis during seedling growth. Trends in Plant Science 15, 291–301. Sauer M, Balla J, Luschni, C, Wisniewska J, Reinöhl V, Friml J. Benková E. 2006. Canalization of auxin flow by Aux/IAA-ARFdependent feedback regulation of PIN polarity. Genes & Development 20, 2902–2911. Scarpella E, Marcos D, Friml J, Berleth T. 2006. Control of leaf vascular patterning by polar auxin transport. Genes & Development 20, 1015–1027. Schoof H, Lenhard M, Haecker A, Mayer KF, Jürgens G, Laux T. 2000. The stem cell population of Arabidopsis shoot meristems in maintained by a regulatory loop between the CLAVATA and WUSCHEL genes. Cell 100, 635–644. Selker JM, Steucek GL, Green PB. 1992. Biophysical mechanisms for morphogenetic progressions at the shoot apex. Developmental Biology 153, 29–43. Shipman PD, Newell AC. 2005. Polygonal planforms and phyllotaxis on plants. Journal of Theoretical Biology 236, 154–197. Smith RS, Guyomarc’h S, Mandel T, Reinhardt D, Kuhlemeier C, Prusinkiewicz P. 2006. A plausible model of phyllotaxis. Proceedings of the National Academy of Sciences, USA 103, 1301–1306. Snow M, Snow R. 1931. Experiments on phyllotaxis. I. The effect of isolating a primordium. Philosophical Transactions of the Royal Society London B 221, 1–43. Somerville C, Bauer S, Brininstool G, et al. 2004. Toward a systems approach to understanding plant cell walls. Science 306, 2206–11. Tan X, Calderón-Villalobos LI, Sharon M, Zheng C, Robinson CV, Estelle M, Zheng N. 2007. Mechanism of auxin perception by the TIR1 ubiquitin ligase. Nature 446, 640–645. Traas J, Doonan H. 2001. Cellular basis of shoot apical meristem development. International Review of Cytology 208, 161–206. Uyttewaal M, Burian A, Alim K, et al. 2012. Mechanical stress acts via katanin to amplify differences in growth rate between adjacent cells in Arabidopsis. Cell 149, 439–451. Uyttewaal M, Traas J, Hamant O. 2010. Integrating physical stress, growth, and development. Current Opinion in Plant Biology 13, 46–52. Vanneste S, Friml J. 2009. Auxin: a trigger for change in plant development. Cell 136, 1005–1016. Vernoux T, Besnard F, Traas J. 2010. Auxin at the shoot apical meristem. Cold Spring Harbor Perspectives in Biology 2, a001487. Vernoux T, Brunoud G, Farcot E, et al. 2011. The auxin signalling network translates dynamic input into robust patterning at the shoot apex. Molecular Systems Biology 7, 508. Vernoux T, Kronenberger J, Grandjean O, Laufs P, Traas J. 2000. PIN-FORMED 1 regulates cell fate at the periphery of the shoot apical meristem. Development 127, 5157–5165. Vieten A, Sauer M, Brewer PB, Friml J. 2007. Molecular and cellular aspects of auxin-transport-mediated development. Trends in Plant Science 12, 160–168. Vieten A, Vanneste S, Wisniewska J, Benková E, Benjamins R, Beeckman T, Luschnig C, Friml J. 2005. Functional redundancy of PIN proteins is accompanied by auxin-dependent cross-regulation of PIN expression. Development 132, 4521–4531. Wabnik K, Govaerts W, Friml J, Kleine-Vehn J. 2011. Feedback models for polarized auxin transport: an emerging trend. Molecular BioSystems 7, 2352–2359. Wabnik K, Kleine-Vehn J, Balla J, Sauer M, Naramoto S, Reinöhl V, Merks RMH, Goaverts W, Friml J. 2010. Emergence of tissue polarization from synergy of intracellular and extracellular auxin signaling. Molecular Systems Biology 6, 447. Wisniewska J, Xu J, Seifertová D, Brewer PB, Ruzicka K, Blilou I, Rouquié D, Benková E, Scheres B, Friml J. 2006. Polar PIN localization directs auxin flow in plants. Science 312, 883. Won C, Shen X, Mashiguchi K, Zheng Z, Dai X, Cheng Y, Kasahara H, Kamiya Y, Chory J, Zhao Y. 2011. Conversion of tryptophan to indole-3-acetic acid by TRYPTOPHAN AMINOTRANSFERASES OF ARABIDOPSIS and YUCCAs in Arabidopsis. Proceedings of the National Academy of Sciences, USA 108, 18518–18523. Yadav RK, Perales M, Gruel J, Girke T, Jönsson H, Reddy GV. 2011. WUSCHEL protein movement mediates stem cell homeostasis in the Arabidopsis shoot apex. Genes & Development 25, 2025–2030. Yamaguchi N, Wu MF, Winter CM, Berns MC, Nole-Wilson S, Yamaguchi A, Coupland G, Krizek BA, Wagner D. 2013. A molecular framework for auxin-mediated initiation of flower primordia. Developmental Cell 24, 271–282. Downloaded from http://jxb.oxfordjournals.org/ at Smith College on July 9, 2014 Rolland-Lagan AG, Prusinkiewicz P. 2005. Reviewing models of auxin canalization in the context of leaf vein pattern formation in Arabidopsis. The Plant Journal 44, 854–865. Stoma S, Lucas M, Chopard J, Schaedel M, Traas J, Godin C. 2008. Flux-based transport enhancement as a plausible unifying mechanism for auxin transport in meristem development. PLoS Computational Biology 4, e1000207.