A Role for Auxin in Flower Development

Auxin has long been implicated in many aspects of plant growth and development including flower development. However, the exact roles of auxin in flower development have not been well defined until the recent identification of auxin biosynthesis mutants. Auxin is necessary for the inltiation of floral primordia, and the disruption of auxin biosynthesis, polar auxin transport or auxin signaling leads to the failure of flower formation. Auxin also plays an essential role in specifying the number and Identity of floral organs. Further analysis of the relationship between the auxin pathways and the known flower development genes will provide critical information regarding mechanisms of organogenesis and pattern formation in plants.     

Exogenous Auxin Effects on Lateral Bud Outgrowth in Decapitated Shoots

In 1933 Thimann and Skoog demonstrated exogenous auxin repressionof lateral bud outgrowth in decapitated shoots ofVicia faba. This evidence has given strong support for a role of auxinin apical dominance. Most, but not all, investigators have confirmedThimann and Skoog's results. In the present study, auxin treatmentswere carried out on ten different species or plant types, manyof which were treated with auxin in different forms, media andunder different light conditions. The Thimann–Skoog experimentdid work for most species (i.e. exogenous auxin did repressbud outgrowth) including thedgt tomato mutant which is knownto be insensitive to auxin in certain responses. Toxic auxinsymptoms were observed in some but not all species. The Thimann–Skoogexperiment did not work for greenhouse-grownColeus or forArabidopsis. Light was shown to reduce apical dominance inColeus andIpomoeanil . apical dominance; lateral bud outgrowth; axillary bud; auxin; IAA; decapitation; Vicia faba ; Ipomoea nil ; Pisum sativum ; Phaseolus vulgaris ; Lycopersion exculentum ; dgt ; Coleus blumei ; Arabidopsis thaliana ; Helianthus annuus ; Thimann–Skoog     

Photosynthesis of Lamina and Sheath of Barley Leaves

Apparent photosynthesis, in mg. CO₂ absorbed per dm.² per hour,of the sheath and enclosed stem of a barley leaf was about 50per cent. of that of the lamina of the same leaf, when the photosynthesizingarea was measured as one side of the lamina and the outer exposedsurface of the sheath. Apparent photosynthesis of a particularlamina or sheath was about 70 per cent. of that of the one aboveon the same stem. Respiration per dm.², though not per g. dry weight, of sheathwith enclosed stem was greater than of lamina in one experimentdone with low-intensity illumination so that true rates of photosynthesisof lamina and sheath were similar. Differences in respirationrates per unit area of laminae and sheaths probably accountedfor most of the greater apparent photosynthesis of the formerin other experiments done with higher intensity illumination. It is suggested that for growth-analysis studies the size ofthe photosynthetic system of cereals should be measured as thatof one side of the leaf laminae plus the outer surface of thecombined leaf sheaths. In the later stages of growth the surfacearea of exposed stem and peduncle should also be included.     

Strigolactone Acts Downstream of Auxin to Regulate Bud Outgrowth in Pea and Arabidopsis

During the last century, two key hypotheses have been proposed to explain apical dominance in plants: auxin promotes the production of a second messenger that moves up into buds to repress their outgrowth, and auxin saturation in the stem inhibits auxin transport from buds, thereby inhibiting bud outgrowth. The recent discovery of strigolactone as the novel shoot-branching inhibitor allowed us to test its mode of action in relation to these hypotheses. We found that exogenously applied strigolactone inhibited bud outgrowth in pea (Pisum sativum) even when auxin was depleted after decapitation. We also found that strigolactone application reduced branching in Arabidopsis (Arabidopsis thaliana) auxin response mutants, suggesting that auxin may act through strigolactones to facilitate apical dominance. Moreover, strigolactone application to tiny buds of mutant or decapitated pea plants rapidly stopped outgrowth, in contrast to applying N-1-naphthylphthalamic acid (NPA), an auxin transport inhibitor, which significantly slowed growth only after several days. Whereas strigolactone or NPA applied to growing buds reduced bud length, only NPA blocked auxin transport in the bud. Wild-type and strigolactone biosynthesis mutant pea and Arabidopsis shoots were capable of instantly transporting additional amounts of auxin in excess of endogenous levels, contrary to predictions of auxin transport models. These data suggest that strigolactone does not act primarily by affecting auxin transport from buds. Rather, the primary repressor of bud outgrowth appears to be the auxin-dependent production of strigolactones.     

A Role for Auxin and Auxin Transport Inhibitors on the Ca Content of Artificially Induced Parthenocarpic Fruits

Artificially induced parthenocarpic fruits of apples, pears and tomatoes, as well as seeded fruits treated with 2,3,5-triiodobenzoic acid, frequently show symptoms of Ca deficiency and a low Ca content. It was concluded that auxins, probably produced by the seeds, play a significant role in Ca translocation into fruits. Exogenous indoleacetic acid but not 4-chlorophenoxyacetic acid applications could replace the effect of seeds in this respect. Auxin transport, rather than auxin accumulation, seems to be necessary for Ca transport, as can be concluded from the effect of auxin transport inhibitors.     

Role for Apyrases in Polar Auxin Transport in Arabidopsis

Recent evidence indicates that extracellular nucleotides regulate plant growth. Exogenous ATP has been shown to block auxin transport and gravitropic growth in primary roots of Arabidopsis (Arabidopsis thaliana). Cells limit the concentration of extracellular ATP in part through the activity of ectoapyrases (ectonucleoside triphosphate diphosphohydrolases), and two nearly identical Arabidopsis apyrases, APY1 and APY2, appear to share this function. These findings, plus the fact that suppression of APY1 and APY2 blocks growth in Arabidopsis, suggested that the expression of these apyrases could influence auxin transport. This report tests that hypothesis. The polar movement of [³H]indole-3-acetic acid in both hypocotyl sections and primary roots of Arabidopsis seedlings was measured. In both tissues, polar auxin transport was significantly reduced in apy2 null mutants when they were induced by estradiol to suppress the expression of APY1 by RNA interference. In the hypocotyl assays, the basal halves of APY-suppressed hypocotyls contained considerably lower free indole-3-acetic acid levels when compared with wild-type plants, and disrupted auxin transport in the APY-suppressed roots was reflected by their significant morphological abnormalities. When a green fluorescent protein fluorescence signal encoded by a DR5:green fluorescent protein construct was measured in primary roots whose apyrase expression was suppressed either genetically or chemically, the roots showed no signal asymmetry following gravistimulation, and both their growth and gravitropic curvature were inhibited. Chemicals that suppress apyrase activity also inhibit gravitropic curvature and, to a lesser extent, growth. Taken together, these results indicate that a critical step connecting apyrase suppression to growth suppression is the inhibition of polar auxin transport.In both animals and plants, cells release nucleotides into their extracellular matrix, where they function as signaling agents, inducing rapid increases in the concentration of cytosolic calcium that are transduced into downstream changes in cell physiology (Kim et al., 2006; Burnstock, 2007; Roux and Steinebrunner, 2007; Tanaka et al., 2010a, 2010b; Demidchik et al., 2011). Prominent among these downstream changes in plants are changes in the growth of cells, including the growth of pollen tubes (Steinebrunner et al., 2003), root hairs (Clark et al., 2010b), and cotton (Gossypium hirsutum) fibers (Clark et al., 2010a). These results suggest the possibility that the signaling changes induced by extracellular nucleotides intersect with signaling changes induced by one or more of the hormones that regulate plant cell growth. Consistent with this possibility, Tang et al. (2003) showed that a concentration of applied nucleotides that inhibited the gravitropic growth of roots could block the transport of the growth hormone auxin and that this effect could not be attributed to either pH changes or chelation of divalent cations. Correspondingly, Clark et al. (2010a) showed that when the application of nucleotides to cotton ovules growing in culture altered the rate of cotton fiber growth, it also induced the production of ethylene, a hormone known to regulate the growth of cotton fibers.Given the potency of extracellular nucleotides to regulate cellular activities, it would be important for cells to control the concentration of these nucleotides. In both animals and plants, the principal enzymes that limit the buildup of extracellular ATP (eATP) and extracellular ADP are ectoapyrases (apyrase; EC 3.6.1.5). These enzymes, which are nucleoside triphosphate diphosphohydrolases, are characterized by apyrase-conserved regions whose peptide sequences are highly similar throughout the plant and animal kingdoms (Clark and Roux, 2009). Based on this structural criterion, there are seven apyrases in Arabidopsis (Arabidopsis thaliana; APY1–APY7), and two of these, APY1 and APY2, share 87% protein sequence identity but are less than 30% similar to the other five apyrases. These two apyrases partially complement each other’s function and play central roles in growth control in Arabidopsis, as judged both by genetic and biochemical criteria (Wolf et al., 2007; Wu et al., 2007). Polyclonal antibodies raised to APY1 (Steinebrunner et al., 2000) inhibit the apyrase activity released into the medium of growing pollen tubes, and when these antibodies were added to the culture medium of germinated pollen, they both blocked the growth of the pollen and raised the concentration of ATP in the medium (Wu et al., 2007). Similarly, treatment of cultured cotton ovules with antibodies that recognize cotton fiber apyrase both inhibits the growth of the fibers and increases the concentration of ATP in the medium, further establishing the link between apyrase activity and regulation of the extracellular ATP concentration ([eATP]) in growing tissues (Clark et al., 2010a).Because wild-type pollen tubes expressing active APY1 or APY2 and cultured cotton fibers with wild-type apyrase activity grow at a normal rate, and because the antibodies inhibit apyrase activity (Wu et al., 2007), the growth inhibition induced by the antibodies further implicated apyrase activity as critical for the growth of these tissues. The antibodies were unlikely to enter the pollen tubes or cotton fibers, so these results also suggested that the pollen and cotton apyrases were ectoapyrases. However, these data do not rule out a possible Golgi function for APY1 and APY2 and for the cotton APY(s), as discussed by Wu et al. (2007) and Clark and Roux (2011). In fact, there is strong evidence that APY1 and APY2 are localized in the Golgi and may function there to regulate protein glycosylation and/or affect polysaccharide synthesis (Chiu et al., 2012; Schiller et al., 2012).Although the suppression of APY1/APY2 or of apyrase activity has a dramatic effect on growth, overexpression of APY1 or APY2 has much less of an effect. Constitutive expression of APY1 induces a small but statistically significant increase in the growth of etiolated hypocotyls, while overexpressing APY2 has no effect on this growth (Wu et al., 2007). This is probably because the wild-type levels of apyrase expression are near optimal for growth (Roux and Steinebrunner, 2007).The double knockout apy1apy2 is sterile, because the pollen of this mutant does not germinate (Steinebrunner et al., 2003). However, when APY1 is suppressed only approximately 60% by an inducible RNA interference (RNAi) construct in apy2 null mutants, pollen of these mutants will germinate, permitting fertilization and subsequent normal development, although the adult plants of these mutants are dwarf (Wu et al., 2007). Suppression of ectoapyrase activity would be expected to raise the equilibrium concentration of eATP (Wu et al., 2007), and since higher levels of eATP can inhibit auxin transport in roots (Tang et al., 2003), it was reasonable to hypothesize that the suppression of apyrase by RNAi could suppress auxin transport. The experiments described in this report test this hypothesis. The results indicate that suppression of APY1/APY2 expression in an inducible RNAi line, R2-4A (Wu et al., 2007), results in a significant inhibition of polar auxin transport in Arabidopsis hypocotyls and roots, with a concomitant altered distribution of endogenous auxin. Consistent with this result and with the results of Tang et al. (2003), suppression of APY1/APY2 also blocks the asymmetric distribution of a GFP reporter encoded by a DR5:GFP construct in gravistimulated primary roots of Arabidopsis seedlings and diminishes the extent of the elongation zone in these roots. These results are consistent with the novel conclusion that inhibition of auxin transport is a key step in the signaling pathway that links the inhibition of apyrase expression to growth inhibition.     

A New Role for TIMP-1 in Modulating Neurite Outgrowth and Morphology of Cortical Neurons

Background

Tissue inhibitor of metalloproteinases-1 (TIMP-1) displays pleiotropic activities, both dependent and independent of its inhibitory activity on matrix metalloproteinases (MMPs). In the central nervous system (CNS), TIMP-1 is strongly upregulated in reactive astrocytes and cortical neurons following excitotoxic/inflammatory stimuli, but no information exists on its effects on growth and morphology of cortical neurons.

Principal Findings

We found that 24 h incubation with recombinant TIMP-1 induced a 35% reduction in neurite length and significantly increased growth cones size and the number of F-actin rich microprocesses. TIMP-1 mediated reduction in neurite length affected both dendrites and axons after 48 h treatment. The effects on neurite length and morphology were not elicited by a mutated form of TIMP-1 inactive against MMP-1, -2 and -3, and still inhibitory for MMP-9, but were mimicked by a broad spectrum MMP inhibitor. MMP-9 was poorly expressed in developing cortical neurons, unlike MMP-2 which was present in growth cones and whose selective inhibition caused neurite length reductions similar to those induced by TIMP-1. Moreover, TIMP-1 mediated changes in cytoskeleton reorganisation were not accompanied by modifications in the expression levels of actin, βIII-tubulin, or microtubule assembly regulatory protein MAP2c. Transfection-mediated overexpression of TIMP-1 dramatically reduced neuritic arbour extension in the absence of detectable levels of released extracellular TIMP-1.

Conclusions

Altogether, TIMP-1 emerges as a modulator of neuronal outgrowth and morphology in a paracrine and autrocrine manner through the inhibition, at least in part, of MMP-2 and not MMP-9. These findings may help us understand the role of the MMP/TIMP system in post-lesion pre-scarring conditions.     

Directionality of Plasmodesmata-Mediated Transport in Arabidopsis Leaves Supports Auxin Channeling

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Polar Auxin Transport Is Essential for Medial versus Lateral Tissue Specification and Vascular-Mediated Valve Outgrowth in Arabidopsis Gynoecia

Although it is generally accepted that auxin is important for the patterning of the female reproductive organ, the gynoecium, the flow as well as the temporal and spatial actions of auxin have been difficult to show during early gynoecial development. The primordium of the Arabidopsis (Arabidopsis thaliana) gynoecium is composed of two congenitally fused, laterally positioned carpel primordia bisected by two medially positioned meristematic regions that give rise to apical and internal tissues, including the ovules. This organization makes the gynoecium one of the most complex plant structures, and as such, the regulation of its development has remained largely elusive. By determining the spatiotemporal expression of auxin response reporters and localization of PINFORMED (PIN) auxin efflux carriers, we have been able to create a map of the auxin flow during the earliest stages of gynoecial primordium initiation and outgrowth. We show that transient disruption of polar auxin transport (PAT) results in ectopic auxin responses, broadened expression domains of medial tissue markers, and disturbed lateral preprocambium initiation. Based on these results, we propose a new model of auxin-mediated gynoecial patterning, suggesting that valve outgrowth depends on PIN1-mediated lateral auxin maxima as well as subsequent internal auxin drainage and provascular formation, whereas the growth of the medial domains is less dependent on correct PAT. In addition, PAT is required to prevent the lateral domains, at least in the apical portion of the gynoecial primordium, from obtaining medial fates.The gynoecium is a highly complex assembly comprised of different tissues that work together to support female reproductive competence in angiosperms. As such, studies of the regulatory networks controlling gynoecial development are essential to not only understand plant reproduction, but also increase our knowledge about intertissue-specific cross talk and coordinated development. A gynoecium is composed of one or more carpels, which may have evolved by the invagination of an ancestral leaf-like structure carrying spores along its edges (for review, see Hawkins and Liu, 2014). The Arabidopsis (Arabidopsis thaliana) gynoecium is a bilateral structure composed of two congenitally fused carpels likely derived from the fusion of two leaf-like structures in which the central domains became the lateral valves and the peripheral meristematic margins carrying the ovules became the medial tissues (Hawkins and Liu, 2014). It has been suggested that the medial domains of the Arabidopsis gynoecial primordium are partially differentiated quasi-meristems with maintained meristematic characteristics allowing for prolonged proliferation (Girin et al., 2009). Accordingly, many lateral domain-specific genes are associated with leaf development, while several genes active in the medial domains are related to meristematic activity (Dinneny et al., 2005; Alonso-Cantabrana et al., 2007; González-Reig et al., 2012).Arabidopsis gynoecium development has been described and reviewed extensively (Sessions, 1997; Bowman et al., 1999; Ferrándiz et al., 1999; Balanzá et al., 2006; Østergaard, 2009; Sundberg and Ferrandíz, 2009) and is summarized in Figure 1. Briefly, at early floral stage 5 (stages according to Smyth et al., 1990), after the initiation of outer floral organs, the remaining floral meristem becomes dome shaped. Although the meristem still appears radially symmetric, it is considered to have a medial plane (black dashed lines in Fig. 1) facing the inflorescence meristem and a lateral plane (white dashed lines in Fig. 1) perpendicular to the medial plane. The terminal floral meristem subsequently broadens in the lateral plane, resulting in a bilateral flattened plate (late floral stage 5). At floral stage 6, differential growth has resulted in a central invagination positioned along the lateral plane, and differential gene expressions indicate that initial patterning events distinguishing medial and lateral domains as well as inner (adaxial) and outer (abaxial) tissues have initiated (Bowman et al., 1999). By the end of floral stage 7, the adaxial medial tissues grow toward each other, forming two medial ridges, also called carpel margin meristems (CMMs). The CMMs will give rise to placentae and subsequently ovule primordia at floral stage 8 (Schneitz et al., 1995). By stage 9, the major tissue types of the mature gynoecium become morphologically distinct as the style and stigmatic papillae start to differentiate. Cell differentiation and cell expansion continue during stages 10 to 12, and the gynoecium is fully mature and ready to accept pollen approximately 10 d after it started to initiate from the terminal floral meristem.Open in a separate windowFigure 1.Arabidopsis gynoecium development. Transmitted light confocal images of the remaining floral meristem (stage [st] 5) and the first stages of gynoecial primordia development (stages 6 and 7), and false-colored DIC images of floral stages 8 to 12 gynoecia along a developmental time scale showing the time in days after floral initiation at the end of each stage. Early and late stage 5 as well as upper images at floral stages 6 and 7 are viewed from above. Lower floral stage 6 image is viewed from the lateral side. Lower images of floral stages 7 to 12 gynoecia are viewed from the medial side. Upper images of floral stages 8 to 12 gynoecia show transverse sections. Stages and time scale are adapted after Smyth et al. (1990) and Sessions (1997). White dashed lines indicate lateral plane, black dashed lines indicate medial plane, arrowheads indicate lateral crease, and asterisks indicate CMM. Bars = 10 µm (stages 5–7), 25 µm (stages 8–10), and 50 µm (stages 11 and 12).It is commonly accepted that the plant hormone auxin is important for gynoecium development, and several models have been put forward to explain this on a mechanistic level (Nemhauser et al., 2000; Østergaard, 2009; Sundberg and Østergaard, 2009; Nole-Wilson et al., 2010; Marsch-Martínez et al., 2012; Hawkins and Liu, 2014). However, we still lack a clear picture of the auxin dynamics and response sites during the earliest developmental stages when the major patterning decisions are made. During lateral organ development, instructive auxin peaks or gradients are formed by site-specific auxin biosynthesis and polar auxin transport (PAT), which results in procambium formation, organ outgrowth, and tissue differentiation (Sachs, 1969; Benková et al., 2003; Mattsson et al., 2003; Heisler et al., 2005; Scarpella et al., 2006; Furutani et al., 2014). The plasma membrane-bound PINFORMED (PIN) proteins as well as at least four members of the ATP-binding cassette subfamily B (ABCB)/MULTI-DRUG RESISTANT/P-GLYCOPROTEIN (PGP) protein family show auxin efflux capacity (for review, see Habets and Offringa, 2014). The PIN proteins are often polarly localized at the plasma membrane, whereas the ABCB/PGP proteins are generally localized apolarly. Therefore, the PINs are largely responsible for the net directional flow of auxin, while the ABCB proteins most likely contribute to PAT by regulating the effective cellular auxin available for polar transport (Mravec et al., 2008; Wang et al., 2013). The phytotropin 1-N-naphtylphthalamic acid (NPA) is a well established and widely used PAT inhibitor, although its exact mode of action is obscure (Petrásek et al., 2003). NPA treatment mimics the pin-like shoot phenotype of pin1 loss-of-function mutants (Okada et al., 1991), and even though NPA appears not to directly interact with PIN proteins, it may influence subcellular dynamics and has been shown to bind to ABCB family members, thereby blocking their transport capacity (Noh et al., 2001; Murphy et al., 2002; Geisler et al., 2003; Nagashima et al., 2008; Kim et al., 2010). This suggests that NPA may reduce PAT in part by restricting the amount of auxin available for PIN-mediated polar transport.Although the pin1-1 knockout mutant rarely produces flowers (Okada et al., 1991), gynoecia of the hypomorphic pin1-5 mutant form elongated styles and reduced or even missing carpels (Bennett et al., 1995; Sohlberg et al., 2006). Auxin biosynthesis mutants also produce disproportionate gynoecial tissues (Cheng et al., 2006; Stepanova et al., 2008), suggesting that auxin peaks and fluxes are important for the coordinated development of gynoecial domains. However, because the gynoecium is the last organ to initiate from the floral meristem, the abnormal gynoecial development in auxin-related mutants may result from developmental defects that occurred prior to gynoecium formation. By transiently treating inflorescences with NPA, Nemhauser et al. (2000) showed that PAT in the gynoecial primordia is important for differential development. However, the whole gynoecium was regarded as one entity with apical-basal polarity, and the possibility that the lateral carpels and the medial meristematic tissues could respond differently to the treatment was never discussed. Thus, where and how NPA affects PAT-regulated development has remained elusive.To understand how local auxin activities influence the outgrowth and patterning events of young gynoecial primordia, we determined the localization of PIN and PGP auxin efflux proteins and the resulting auxin response domains. This allowed us to map the directional flow and auxin response peaks during the earliest stages of gynoecium development. In addition, we induced transient disruptions in PAT and assessed the response of auxin signaling and domain-specific markers to establish how auxin signaling and vascular, lateral, and medial domains are affected by alterations in PAT. Based on our data, we propose a new model for auxin-regulated gynoecial patterning in which the medial versus lateral identity is dependent on correct auxin localization, and subsequent carpel valve outgrowth is dependent on transport-mediated apical auxin drainage.     

The Interactions among DWARF10, Auxin and Cytokinin Underlie Lateral Bud Outgrowth in Rice

Previous studies have shown that DWARF10 (D10) is a rice ortholog of MAX4/RMS1/DAD1, encoding a carotenoid cleavage dioxygenase and functioning in strigolactones/strigolactone-derivatives (SL)biosynthesis. Here we use D10- RNA interference (RNAi) transgenic plants similar to d10 mutant in phenotypes to investigate the interactions among D10, auxin and cytokinin in regulating rice shoot branching. Auxin levels in node 1 of both decapitated D10-RNAi and wild type plants decreased significantly, showing that decapitation does reduce endogenous auxin concentration, but decapitation has no clear effects on auxin levels in node 2 of the same plants. This implies that node 1 may be the location where a possible interaction between auxin and D10 gene would be detected. D10 expression in node 1 is inhibited by decapitation, and this inhibition can be restored by exogenous auxin application,indicating that D10 may play an important role in auxin regulation of SL. The decreased expression of most OsPINs in shoot nodes of D10- RNAi plants may cause a reduced auxin transport capacity.Furthermore, effects of auxin treatment of decapitated plants on the expression of cytokinin biosynthetic genes suggest that D10 promotes cytokinin biosynthesis by reducing auxin levels. Besides, in D10- RNAi plants, decreased storage cytokinin levels in the shoot node may partly account for the increased active cytokinin contents, resulting in more tillering phenotypes.     

生长素在植物胚胎早期发育中的作用

有性生殖是有花植物的一个重要特征, 胚胎则是实现有性生殖和世代交替的重要载体。植物胚胎从双受精开始, 经历了合子极性建立、顶基轴形成、细胞层分化和器官形成等过程, 这些过程都受到生长素的调控。近年来的研究表明, 生长素在生物合成、极性运输和信号转导3个层面上调控胚胎的发育过程。该文以双子叶植物拟南芥(Arabidopsis thaliana)为例, 综述了生长素对胚胎早期发育过程, 包括合子极性和顶基轴建立、表皮原特化和对称模式转变、胚根原特化和根尖分生组织形成及茎尖分生组织形成等发育的调控机制。