AXR1 Acts after Lateral Bud Formation to Inhibit Lateral Bud Growth in Arabidopsis

doi:10.1104/pp.121.3.839

AXR1 Acts after Lateral Bud Formation to Inhibit Lateral Bud Growth in Arabidopsis¹

Petra Stirnberg, Steven P. Chatfield, and H.M. Ottoline Leyser^*

Department of Biology, University of York, P.O. Box 373, York YO10 5YW, United Kingdom

ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
LITERATURE CITED

The AXR1 gene of Arabidopsis is required for many auxin responses. The highly branched shoot phenotype of mature axr1 mutantplants has been taken as genetic evidence for a role of auxinin the control of shoot branching. We compared the developmentof lateral shoots in wild-type Columbia and axr1-12 plants. Inthe wild type, the pattern of lateral shoot development dependson the developmental stage of the plant. During prolonged vegetativegrowth, axillary shoots arise and develop in a basal-apical sequence.After floral transition, axillary shoots arise rapidly along theprimary shoot axis and grow out to form lateral inflorescencesin an apical-basal sequence. For both patterns, the axr1 mutationdoes not affect the timing of axillary meristem formation; however,subsequent lateral shoot development proceeds more rapidly inaxr1 plants. The outgrowth of lateral inflorescences from excisedcauline nodes of wild-type plants is inhibited by apical auxin.axr1-12 nodes are resistant to this inhibition. These resultsprovide evidence for common control of axillary growth in bothpatterns, and suggest a role for auxin during the late stagesof axillary shoot development following the formation of the axillarybud and several axillary leafprimordia.

	INTRODUCTION

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION LITERATURE CITED

In plants, the shoot apex has an inhibitory effect on the development of lateral shoots. The theory that the plant hormoneauxin (indole-3-acetic acid [IAA]) is a signal in this apicaldominance remains a matter of debate. This theory is based onthe effects of auxin application on decapitated plants and thediscovery of basipetal auxin transport. The mechanism by whichauxin acts is still obscure and is likely to be indirect (seePhillips, 1975; Trewavas, 1981; Cline, 1991, 1994).

The increasing number of mutations or transgenes that affect auxin content, transport, or sensitivity, especially in Arabidopsis,provides a different approach to investigate the role of auxinin apical dominance, and in particular which stages of lateralshoot development it regulates in vivo. Plants expressing theIAA biosynthetic genes from Agrobacterium tumefaciens have highendogenous IAA levels and increased apical dominance (Klee etal., 1987; Romano et al., 1993, 1995). The iaaL gene from Pseudomonassavastanoi, encoding an enzyme that conjugates IAA to Lys, hasbeen transformed into tobacco, resulting in reduced levels offree IAA and reduced apical dominance (Romano et al., 1991).

Several mutants with altered auxin sensitivity have been produced in Arabidopsis. One such locus, AXR1, is defined by an allelicseries of recessive mutations. The phenotype of axr1 mutant plantsis pleiotropic, with defects in root, hypocotyl, stamen, and stemelongation, vascular development, lateral root formation, androot gravitropism. Leaf morphology is altered and shoot branchingis increased at maturity (Estelle and Somerville, 1987; Lincolnet al., 1990). All axr1 tissues examined showed reduced auxinsensitivity in a variety of assays, including rapid gene inductionby auxin (Abel et al., 1995; Timpte et al., 1995). This suggeststhat the AXR1 protein is required for auxin signaling. The AXR1gene encodes a protein related to the amino-terminal half of ubiquitin-activatingenzyme; sequencing of severe mutant alleles such as axr1-12 indicatescomplete loss of protein function (Leyser et al., 1993).

Although these mutant and transgenic lines suggest that branching is regulated by auxin in vivo, they were only investigatedat a cursory level. Altered branching may be an indirect consequenceof other auxin-regulated phenotypes. axr1-12 plants produce morebranches than the wild type, and are less fertile (Lincoln etal., 1990). There is evidence that developing fruits limit lateralbranching (Tamas et al., 1979; Hensel et al., 1994). Therefore,the increased branching in mature axr1 plants may be a consequenceof theirinfertility.

The in vivo role of auxin is further called into question by examining the pattern of lateral shoot development in Arabidopsis.If apically derived auxin acts as an inhibitor of axillary branching,one might expect the lateral buds closest to the shoot apex tobe the most repressed, giving a basal-apical (acropetal) sequenceof bud growth. Arabidopsis shows this pattern during prolongedvegetative growth, e.g. in late-flowering ecotypes (Grbi $c'$ andBleecker, 1996). However, lateral inflorescences develop in anapical-basal (basipetal) sequence after floral transition (Alvarezet al., 1992; Hempel and Feldman, 1994).

To further assess the role of auxin in the regulation of Arabidopsis shoot branching, we compared axillary shoot developmentin the wild type and axr1-12 to determine the earliest stage whendifferences can be detected. In addition, we compared the auxinsensitivity of wild-type and axr1-12 lateral inflorescence outgrowthusing nodes excised from the primary inflorescence. The axr1-12mutation does not affect early stages of axillary shoot development;however, it promotes the subsequent growth of axillary shootsinitiated by the acropetal and basipetal pattern. It also rendersthe outgrowth of isolated lateral inflorescences resistant toauxin inhibition. These results suggest a role for auxin in thestages of lateral shoot development following axillary meristemformation.

	MATERIALS AND METHODS

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION LITERATURE CITED

Plants for Morphometric and Histological Analyses

Seeds of Arabidopsis (wild type and axr1-12, ecotype Columbia) were sown onto F2 compost (Levington Horticulture, Ipswich,UK) in shallow trays consisting of individual 4- × 4-cm pots (P40,Cookson Plantpak, Maldon, UK), with several seeds per pot. Compostfor short-day-grown plants was treated with systemic insecticide(Intercept 70WG, Levington Horticulture) before sowing. After2 to 5 d of cold treatment at 4°C, trays were transferred to 21°C,8-h (short) or 16-h (long) photoperiods and watered with tap water.Light intensities were 130 and 50 µmol m² s¹ for the short and long photoperiod, respectively. Seedlings werethinned out to one per pot aftergermination.

Histology

Tissue was fixed overnight in 3% (v/v) formaldehyde/1.25% (v/v) glutaraldehyde in 0.05 M sodium phosphate buffer (pH 7.0),dehydrated in a graded ethanol series, transferred to Histoclear(National Diagnostics, Atlanta), and embedded in Paraplast Plus(Sigma-Aldrich, Poole, UK). Microtome sections (8 µm) were affixedto glass microscope slides covered with adhesive (1% [w/v] gelatin,13% [v/v] glycerol), dewaxed in xylene, rehydrated in an ethanolseries, stained in 0.025% (w/v) aqueous toluidine blue, dehydratedin an ethanol series followed by xylene, and coverslips were mountedwith DPX (BDH Laboratory Supplies, Poole,UK).

Excised Node Experiments

Seeds were surface-sterilized for 15 min in 10% (v/v) Chloros bleach (Beveridge, Edinburgh, UK) followed by one wash with70% (v/v) ethanol and five washes with sterile distilled water,and cold treated in water at 4°C for 3 d. Four individual seedswere then sown into sterile 1-L jars containing 50 mL of ATS medium(0.8% [w/v] agar, 1% [w/v] Suc, and mineral nutrients accordingto Wilson et al. [1990]). Jars were incubated at 22°C to 27°Cin a 16-h photoperiod (50 µmol m² s¹) until the primary inflorescence elongated. To prepare splitagar plates, 25-mL aliquots of ATS medium were dispensed into9-cm Petri dishes and allowed to solidify for 45 to 60 min ina laminar flow hood with the lid open. A strip of agar about one-eleventhof the total by weight was then cut out along the diameter ofthe plate and removed, leaving a gap 6 to 8 mm wide. Dishes werefurther dried for 30 min. Half-plates containing the syntheticauxin 1-NAA were prepared by adding 100 µL of a 100 µM or 100µL of a 1 mM 1-NAA stock to give approximate final concentrationsof 1 or 10 µM, respectively. The added solution was spread overthe agar surface until it was absorbed. Plates were prepared atleast 1 d before node excision for diffusion of the applied 1-NAAinto the agar layer. Stem sections consisting of a node with avisible axillary bud between parts of the apical and the basalinternode and 8 to 15 mm long were excised from elongating primaryinflorescences. The length of the bud was measured and the nodewas placed over the gap of a split plate, with the apical endinserted into one agar half and the basal end into the other.Plates containing up to three excised nodes were incubated inthe conditions described above in near-vertical orientation. Thelengths of the axillary shoots were measured daily with a metricruler until d 8 following excision. Lengths were determined fromthe point where the adaxial side of the subtending petiole insertedinto the stem to the tip of the axillary leaves when the bud wasstill closed, or to the inflorescence apex when the branch hadstartedelongating.

	RESULTS

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION LITERATURE CITED

Development of the Branched Inflorescence in Long Photoperiods

To establish when differences in branching between axr1-12 and wild-type plants first arise, the development of their shootsystems was studied over time. Neither wild-type nor axr1-12 rosettesshowed visible axillary buds or branches during vegetative growthin long photoperiods. After the transition to reproductive growth,flower buds became visible in the center of the rosettes and theplants started to bolt, as defined by visible elongation of thelowermost internode of the primary inflorescence. The date ofbolting was noted for each individual plant. Samples of five toeight plants of each genotype were removed and subjected to morphometricanalysis covering a time course of 3-d intervals between 3 and18 d after bolting. The leaves (excluding the cotyledons) werenumbered in order of emergence, and first-order lateral developmentin each leaf axil was scored into three categories: (a) no axillarybud visible by eye, (b) visible bud, and (c) elongatinginflorescence.

For laterals in category (c), inflorescence length was measured and the number of vegetative nodes determined. The presenceof visible accessory inflorescences, which may arise between alateral inflorescence and the subtending leaf in cauline nodes(Talbert et al., 1995), was noted. In total, 40 wild-type and33 axr1-12 plants were analyzed. Wild-type plants bolted betweend 28 and 37 after the end of cold treatment, with a mean ± SEof 30.0 ± 0.4 d. axr1-12 plants bolted between d 29 and 35, onaverage slightly later than wild type (mean 32.0 ± 0.4 d). Wild-typeplants produced between 13 and 24 leaves (rosette and cauline)before floral transition, with a mean ± SE of 17.0 ± 0.4. Withaxr1-12, leaf numbers ranged from 16 to 27, with a mean ± SE of23.0 ± 0.5, significantly higher than wild type. Both mean rosetteand mean cauline leaf numbers were higher for the mutant. Wild-typeplants had on average 3.3 ± 0.2 cauline and 13.7 ± 0.3 rosetteleaves. Mutant plants had on average 6.6 ± 0.2 cauline and 16.0± 0.4 rosetteleaves.

In both the wild type and axr1-12, all of the cauline leaf axils on the primary inflorescence produced a lateral inflorescence.Some of these were clearly elongating on d 3 after the primaryinflorescence started bolting and all were elongating by d 6.Due to the higher total cauline leaf number described above, axr1-12plants had on average twice as many cauline inflorescences asthe wildtype.

The time course of first-order lateral development in the rosettes of both genotypes is shown in Figure 1A. As the wild typeand axr1-12 differed in the number of leaves (i.e. nodes) in therosette, the three categories of laterals scored were expressedas proportions of the total rosette node number for each individual.In the wild type, the mean proportion of nodes with no visiblebud varied between 19% and 31% without a clear trend between d3 and 18 after bolting. The same was true for axr1-12, exceptthat the percentages were lower (between 14% and 20%). The percentageof wild-type nodes with visible buds decreased from 81% to 40%between d 3 and 18, accompanied by a rise in the percentage ofnodes with elongating inflorescences from 0% to 31%. In axr1-12,the proportion of nodes with visible buds decreased from 81% to33% and the proportion of elongating inflorescences increasedfrom 0% to 54%. The proportion of elongating inflorescences inthe rosette was higher in axr1-12 than in the wild type from d12 after bolting.

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Figure 1. Morphometric analysis of lateral shoot development of wild-type and axr1-12 plants grown in long photoperiods. A, Time course of lateral shoot development in rosette leaf axils. For each genotype, five to eight plants were sampled every 3 d between d 3 and 18 after bolting of the primary inflorescence, and their rosette leaf axils were examined. Lateral shoot development was scored into three developmental stages (no visible bud [ $diamond$ ]; visible bud [

]; and elongating inflorescence [ $open circle$ ]), and the proportion of laterals at each stage calculated for each plant. The mean proportions ± SE for each time point are plotted. B, Lateral shoot development at consecutive nodes along the primary shoot axis, 6 d after bolting. For one wild-type (upper row) and one axr1-12 plant (lower row), cotyledons and leaves were dissected from the primary shoot axis with their attached axillary shoots and laid out in the sequence in which they developed (left to right = base to apex). The uppermost rosette leaves are marked by arrows. Bar = 5 cm. C, Mean lateral inflorescence lengths ± SE at consecutive nodes along the primary shoot axis 18 d after the primary inflorescence started bolting. Five plants were analyzed for each genotype (wild type [ $open circle$ ]; axr 1-12 [

]). Lateral inflorescence lengths for axils without a visible bud or with a vegetative bud were scored as zero. As the mean number of cauline leaves was 3 for wild-type and 6 for axr1-12 plants, plots for wild type were started three node positions basal from those of axr1-12. Thus, node position 0 represents on average the uppermost rosette leaf for both genotypes.

First-order lateral development in the rosettes of both genotypes displayed a basipetal gradient. At the time of bolting,a number of leaves at the base of the rosette had no visible budsin their axils. More apical leaves carried visible buds. Duringthe 18 d after bolting, an increasing number of leaves in themost apical part of the rosette carried an elongating lateralinflorescence.

Figure 1B shows one representative plant for each genotype, dissected 6 d after bolting. Their cotyledons and leaves withattached axillary shoots were laid out in the sequence in whichthey had been produced by the primary shoot apex. The class "visiblebuds" in Figure 1A included very small buds with leaves just beginningto expand (which are not visible at the magnification of Fig.1B), up to buds with several expanded leaves and visible flowerbuds. Although the proportions of "visible buds" did not differbetween the wild type and axr1-12 during the 18 d following bolting(Fig. 1A), genotypes differed in the extent of bud growth as earlyas 6 d after bolting (Fig. 1B). The zone of nodes carrying budsshowing significant leaf expansion, clearly seen at the magnificationof Figure 1B, was extended to more basal node positions in axr1-12.Overall, axillary leaves had expanded further in the mutant thanin the wild type, which was most obvious in the oldest one totwo leaves of each bud, but also in the younger leaves in thecenter of thebuds.

To compare inflorescence outgrowth in the wild type and axr1-12, the average first-order lateral inflorescence lengths werecalculated for consecutive node positions along the primary shootaxis, starting with the uppermost cauline leaf node and proceedingbasipetally. The distribution of inflorescence lengths is shownin Figure 1C for d 18 after bolting. Lateral inflorescence lengthsfor axils without a visible bud or with a vegetative bud werescored as zero. As the mean number of cauline leaves was threefor wild-type and six for axr1-12 plants, plots for the wild typewere started three node positions basal from those of axr1-12.Thus, node position 0 represents on average the uppermost rosetteleaf for both genotypes. The wild-type inflorescence length distributionshowed a characteristic pattern. Branches at the three most apicalnodes (on average corresponding to the cauline nodes on the primaryinflorescence) were of similar length. Mean inflorescence lengthsthen decreased progressively through up to four more basal nodepositions. No elongating inflorescences were found further towardthe base. The inflorescence lengths of axr1-12 plants followeda comparable pattern, but the number of apical inflorescencesof similar length was increased to six (corresponding to the meannumber of cauline inflorescences in axr1-12) and the zone of decreasinglength comprised up to six nodes. The apical-basal gradient ofinflorescence length was less steep in the mutant. In apical nodes,the mean axr1-12 inflorescence length was clearly below that ofwild type, while in the more basal nodes, the mean inflorescencelength was slightly higher than that of the wild type. These inflorescencelength distributions of the wild type and axr1-12 were establishedas early as 6 d after bolting and were maintained while the primaryand lateral inflorescences elongated (data notshown).

Lateral inflorescence architecture displayed characteristic differences that were correlated with position along the shootaxis. Apical axillary meristems produced fewer leaves before floraltransition than basal meristems. In wild-type plants leaf numbersranged between two and four for the uppermost cauline inflorescence,and four to five for the lowermost. In axr1-12, the uppermostcauline inflorescences had two or three leaves and the lowermosthad between six and 10 leaves. Leaf numbers increased furthertoward the lowermost rosette inflorescence, which had leaf numbersbetween nine and 11 for wild type and between 10 and 14 for axr1-12.

Between a lateral shoot and its subtending leaf, an accessory axillary meristem may form and develop into an accessory budor inflorescence in Arabidopsis (Talbert et al., 1995). Accessoryshoots were first seen in the axils of cauline leaves 6 d afterbolting, occurring in 6.7% of the 20 wild-type cauline nodes andin 64% of the 39 axr1-12 cauline nodes examined. The percentagesincreased in both genotypes until d 18 after bolting, but remainedclearly lower (27% of 15 nodes) in the the wild type than in axr1-12(70% of 30 nodes). Thus, differences in accessory developmentin the two genotypes arose as early as 6 d after bolting. Accessorybuds were not detected in rosette leaf axils of either wild typeor axr1-12.

Development of Vegetative Lateral Shoots in Short Photoperiods

Our observations with plants grown in long photoperiods show that the axr1-12 mutation affects the growth of lateral shootsdeveloping in the basipetal pattern early after floral transition.The development of lateral shoots initiated by the acropetal patternwas compared by dissecting wild-type and axr1-12 plants (six pergenotype) that had undergone prolonged vegetative growth in 49to 58 short photoperiods. Figure 2 shows one plant of each genotypedissected 49 d after sowing, with the oldest 27 leaves and attachedaxillary shoots laid out in the sequence of emergence. In thewild type, a small axillary bud not visible at the magnificationof Figure 2 was associated with most leaves, and only a few budsscattered along the primary shoot axis showed some leaf expansion.In axr1-12, most buds showed considerable leaf expansion. Mutantbud development displayed a clear acropetal gradient, with budsize increasing toward the base, excluding some of the oldestjuvenile leaves, where buds were either small or not visible.

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Figure 2. Lateral shoot development at consecutive nodes along the primary shoot axis in short photoperiods 49 d after the end of cold treatment. For one wild-type (upper row) and one axr1-12 plant (lower row), the oldest 27 leaves (without the cotyledons that had senesced) were dissected from the primary shoot axis with their attached axillary shoots and laid out in the sequence in which they developed (left to right = base to apex). The undissected apical parts of the rosettes are shown on the right. Bar = 5 cm.

Timing of Axillary Shoot Formation

The experiment described above shows that axr1-12 buds in the axils of rosette leaves are further developed than their wild-typecounterparts. To determine whether axillary shoots were formedearlier in the mutant, we sectioned plants grown in long and shortphotoperiods and examined their leafaxils.

Plants grown in long days were fixed 15 and 20 d after the end of cold treatment, and longitudinal sections of both genotypeswere compared. For both genotypes, we found vegetative plantsand plants that had recently undergone floral transition amongthe plants fixed on d 15. Virtually all of the plants fixed ond 20 had undergone floral transition. During vegetative growth,the shoot apical meristem is relatively small and is situateddirectly on the short primary shoot axis (Vaughan, 1954; Mikscheand Brown, 1965; Hempel and Feldman, 1994). For both genotypes,axillary meristems were not detected in the axils of either youngor old leaves in vegetative plants (Fig. 3, A and E).

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Figure 3. Longitudinal sections of wild-type (A-D) and axr1-12 (E-H) shoots grown in long photoperiods stained with toluidine blue. Plants in A and C and E to G were fixed on d 15, and plants in B, D, and H were fixed on d 20 after the end of cold treatment. Bar in A (for A and E) and in bar in B (for B-D and F-H) = 100 µm. A and E, Vegetative shoots. m, Vegetative shoot apical meristem. Arrowheads point to the axils of leaf primordia and more mature leaves sectioned in a median plane and lacking axillary meristems. B and F, Shoots at floral transition. Elongation of the primary inflorescence is initiated by cell divisions in the region underlying the inflorescence meristem (m). Arrowheads mark clusters of meristematic cells in the axils of leaf primordia. C and G, Shoots at floral transition. Arrowheads point to meristematic cells at the base of the petiole of more mature leaves. D and H, Shoots whose inflorescence meristems (m) have produced flower primordia (f). Axillary meristematic regions (marked by arrowheads) are of increased size or have started to bulge out.

The early stages of reproductive growth are characterized by enlargement of the shoot apical meristem and by cell divisionsin the rib meristem at its base, which is the first step in theformation of the primary inflorescence axis (Vaughan, 1954; Mikscheand Brown, 1965; Hempel and Feldman, 1994). In both wild-typeand axr1-12 plants at this stage, clusters of very small, stronglystaining meristematic cells were observed at the base of youngleaf primordia (Fig. 3, B and F), as well as at the base of thepetiole of older leaves (Fig. 3, C and G). In plants in whichthe first flower primordia had been formed by the primary shootapical meristem, the axillary meristematic zone had increasedin size in both genotypes, but axillary leaf formation had notyet started (Fig. 3, D and H). The early stages of axillary shootformation in axr1-12 (Fig. 3, E-H) were indistinguishable fromthose of the wild type (Fig. 3, A-D). Accessory axillary meristemsat cauline nodes were observed in older plants of both genotypes,fixed at least 25 d after the end of cold treatment, but the frequencieswere insufficient for a detailedcomparison.

Plants grown in short photoperiods were fixed 37 d after the end of cold treatment, and series of transverse sections throughsix individual shoots were analyzed for each genotype. Leaveswere numbered from apex to base, with 1 being the youngest leafprimordium. In both genotypes, the morphology of axillary shootsobserved at consecutive node positions suggested that buds wereformed and developed in an acropetal sequence. The axils of anumber of the youngest leaf primordia close to the vegetativeshoot apical meristem were morphologically indistinguishable fromthe rest of the leaf primordium. Further basal, the first indicationof axillary bud formation was a region of strongly staining meristematiccells at the base of the leaf primordium. This increased in sizein leaf primordia further basal until an axillary bud could bedistinguished as a zone of meristematic cells bulging out fromthe petiole of the subtending leaf. Axillary buds at more basalnode positions showed increasing numbers of axillary leaf primordia.The most apical node showing axillary cell division, a clear axillarybud, and a bud with at least one leaf primordium was determinedfor each series of sections (Table I). The mean node positionsat which these stages were first observed were not significantlydifferent between the wild type and axr1-12. We also counted axillaryleaf primordia at nodes 32, 36, and 40. Node 40 was the oldestnode for which an accurate determination could be made. Belowthis node, axillary buds were often sectioned in an oblique planeand leaf primordia could not be counted. The mean numbers of leafprimordia up to node 40 were slightly but not significantly higherfor axr1-12 than for the wild type (data not shown).

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Table I. Early stages of axillary shoot formation in wild-type and axr1-12 plants grown in short photoperiods
Data are means ± SE of six plants per genotype fixed 37 d after the end of cold treatment.

Thus, the pattern and timing of the early stages of axillary bud formation in axr1-12 was indistinguishable from that of thewild type in both long and shortphotoperiods.

Auxin Inhibition of Inflorescence Outgrowth from Excised Nodes

The above observations suggest that the axr1-12 mutation affects lateral shoot growth after axillary meristem formation. Todetermine whether auxin can regulate lateral shoot growth in Arabidopsis,we studied its effect on the outgrowth of cauline lateral inflorescences.Nodes whose lateral inflorescences had not yet started to elongatewere excised from the primary inflorescence of plants grown insterile conditions and placed with the cut ends of their apicaland basal internodes contacting two separate slabs of agar mediumin a Petri dish. This allowed us to apply auxin either apicallyor basally. We used the synthetic auxin 1-NAA in these experimentsbecause of its greater stability compared with the natural auxinIAA. Nodes were excised as soon as internode elongation of theprimary inflorescence permitted adjacent internodes of suitablelength to be obtained. At this time, buds were typically between0.5 and 2 mm long. Figure 4 shows results obtained using the lowermostcauline node.

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Figure 4. Effect of the synthetic auxin 1-NAA on lateral inflorescence outgrowth from excised nodes of the wild type and axr1-12. The lowermost cauline node was excised from the elongating primary inflorescence of axenically grown plants and inserted between two separate agar slabs. Slabs contained either no 1-NAA or 1 or 10 µM 1-NAA in contact with the apical or with the basal part of the stem. Mean lateral shoot lengths ± SE were determined each day until d 8 following excision. Measurements for some lateral shoots that wilted and ceased elongating after d 5 were included in the earlier time points but were excluded from the later time points. Node numbers tested for each treatment are: $open circle$ , 0 µM 1-NAA apical/0 µM 1-NAA basal, 5 to 8 wild type and 14 to 16 axr1-12; $triangle$ , 0 µM 1-NAA apical/1 µM 1-NAA basal, 4 to 6 wild type and 5 axr1-12;

, 0 µM 1-NAA apical/10 µM 1-NAA basal, 4 wild type and 5 to 6 axr1-12; $black-triangle$ , 1 µM 1-NAA apical/0 µM 1-NAA basal, 12 to 15 wild type and 10 axr1-12; $black-square$ , 10 µM 1-NAA apical/0 µM 1-NAA basal, 8 wild type and 12 to 13 axr1-12.

When excised wild-type nodes were inserted between two slabs of hormone-free agar, the lateral inflorescences elongated andreached a mean length of 5.5 mm on d 4 and 30.6 mm on d 8 afterexcision (Fig. 4, left). 1-NAA (1 and 10 µM) inhibited elongationwhen applied to the agar in contact with the apical internode.Elongation was completely inhibited until d 4 after excision.After this time, some buds started to elongate, especially withthe lower 1-NAA concentration. 1-NAA (1 or 10 µM) had no effectwhen contacting the basal internode. When nodes excised from axr1-12plants (Fig. 4, right), were tested in the absence of auxin orwith 1 or 10 µM basal 1-NAA, lateral inflorescence outgrowth showeda time course very similar to that of the wild type under thesetreatments. However, in contrast to wild type, elongation of axr1-12inflorescences was not significantly inhibited by apically applied1-NAA at 1 or 10 µM.

	DISCUSSION

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION LITERATURE CITED

To study the regulation of shoot branching, we characterized lateral shoot development in the Columbia ecotype of Arabidopsisgrown in long and short photoperiods. Under either photoperiod,the development in Arabidopsis leaf axils follows a similar sequencefrom empty axil through vegetative axillary shoot to floral shoot.The branching patterns observed in Arabidopsis plants must reflectthe rates of initiation and progress between these states. Inthis study we investigated the role of the AXR1 gene in theseevents.

Loss of AXR1 Function Does Not Affect Axillary Meristem Formation

In most respects, axillary meristem formation in the ecotype Columbia is identical to other ecotypes of Arabidopsis. In youngleaf primordia the axils appear to be completely empty (Hempeland Feldman, 1994; Grbi $c'$ and Bleecker, 1996; Fig. 3, A and E).The observed origin of the axillary meristem in the subtendingleaf (Fig. 3, B, C, F, and G) is in accordance with clonal studies(Furner and Pumfrey, 1992; Irish and Sussex, 1992; Schnittgeret al., 1996). A subepidermal origin with the epidermis beingrecruited later (Fig. 3C) is also consistent with clonal analysis(Schnittger et al., 1996). In contrast to Arabidopsis, the axillarymeristems of some other angiosperm species (maize, sunflower)appear to arise in the primary shoot apical meristem above thenascent leaf primordia (Garrison, 1955; Johri and Coe, 1983; McDanieland Poethig 1988; Jegla and Sussex, 1989; Sussex, 1989).

Studies of Arabidopsis ecotypes other than Columbia indicate that the sequence of axillary shoot formation along the primaryshoot axis is acropetal during (prolonged) vegetative growth,but basipetal after floral transition (Hempel and Feldman, 1994;Grbi $c'$ and Bleecker, 1996). Vegetative ecotype Columbia plantsshowed a clear acropetal pattern of axillary meristem formation,with detectable axillary cell divisions on average 17 nodes fromthe shoot apical meristem (Table I). After floral transitionin long days, axillary cell divisions were seen all along theshoot axis (Fig. 3). Temporal resolution in our experiment maynot have been sufficient to detect the basipetal sequence reportedby Hempel and Feldman (1994) and Grbi $c'$ and Bleecker (1996). Inany case, floral transition coincides with a switch from the completeinhibition of axillary meristem development near the shoot apicalmeristem to the formation of axillary meristems in close proximityto it (from 17 nodes to less than three nodes distance in ourexperiments). This shows that axillary meristem formation is regulatedindependently of leafage.

Early axillary shoot development in axr1-12 was indistinguishable from that of the wild type. In particular, the experimentin short photoperiods suggests that the axillary meristem andthe first axillary leaf primordia were formed at a similar rateup to 40 nodes from the shoot apical meristem. Thus, AXR1 is notrequired to specify either of the opposing patterns of axillarymeristem formation or the switch between them. AXR1 is also notinvolved in regulating the onset of axillary shoot formation ineither pattern. Our observations were not sufficient to comparethe formation of accessory axillary meristems in detail. Theywere detected in sections of both genotypes, which does not contradictthe hypothesis that their formation is also unaffected by theaxr1-12mutation.

Loss of AXR1 Function Promotes Axillary Shoot
Growth after Axillary Meristem Formation

After axillary meristem formation, lateral shoots develop in a manner similar to the primary shoot apical meristem. Thereappears to be an obligatory vegetative phase in that all of theaxillary meristems initiate at least two leaves before undergoingfloral transition, even if the primary shoot apical meristem isfloral. Our results suggest that axillary shoot growth duringthese stages is repressed in the wild type, and that repressionis relieved by the axr1-12 mutation (Figs. 1 and 2).

In short photoperiods, mutant buds were more advanced than those of the wild type before visible bolting of the primary shootapex. Furthermore, differences between wild-type and axr1-12 lateralshoot development in long-day-grown plants were detected soonafter floral transition and before significant fruit development(data not shown). Therefore, the effects of the axr1-12 mutationon lateral branching cannot just be the result of reducedfertility.

Effects of Loss of AXR1 Function Indicate That Auxin Regulates the Growth of Axillary Shoots after Axillary Meristem Formation

A role of auxin as a signal in apical dominance has been questioned for several species including Arabidopsis, because evenhigh concentrations of auxin did not inhibit lateral outgrowthafter decapitation (Cline, 1996). However, with Arabidopsis nodesexcised from the primary inflorescence, the outgrowth of caulineinflorescences was completely inhibited for at least 4 d by 1-NAAapplied apically at micromolar concentrations (Fig. 4). The lackof response to auxin in buds on decapitated plants in contrastto excised nodes was also observed in bean (Tamas et al., 1989).This could either reflect a variation in sensitivity to auxinor the presence of factors produced in the root that promote budoutgrowth.

Involvement of AXR1 in the control of apical dominance had been proposed by Estelle and Somerville (1987) and Lincoln et al.(1990), based on the bushy phenotype of mature axr1 mutant plants.The AXR1 gene has been isolated (Leyser et al., 1993) and ourpresent understanding of the mechanism of action of the AXR1 proteinsuggests that it modulates the ubiquitin-mediated degradationof regulatory proteins (del Pozo et al., 1998; Leyser, 1998; Rueggeret al., 1998). Although all of the phenotypes of axr1 loss-of-functionmutants may be explained in terms of reduced auxin sensitivity,AXR1 might regulate the degradation of other proteins not involvedin the auxin response. However, it has been reported that increasedbranching conferred by the axr1-3 mutation is epistatic to theIAA-M auxin over-producing transgene (Romano et al., 1995). Weshow that detectably enhanced lateral growth after axillary meristemformation in vivo correlates with auxin resistance of isolatedlateral inflorescences in axr1. This suggests an AXR1-mediatedrole for auxin in regulating Arabidopsis shoot branching afteraxillary meristemformation.

No differences in the timing or the pattern of axillary meristem formation between axr1-12 and wild type were detected. Thismay be because axillary meristem formation is auxin independent.Alternatively, auxin may regulate axillary meristem formationin an AXR1-independent manner. Analogy with yeast signaling systemssuggests that the AXR1 protein may increase the efficiency ofthe degradative pathway, rather than being absolutely requiredfor it (Leyser, 1998). AXR1 may therefore only be necessary fora subset of auxin signaling events, for example, those triggeredby low levels ofauxin.

The axr1-12 mutation affects axillary shoot growth independently of the prevailing pattern of axillary shoot formation andgrowth along the shoot axis. This suggests that growth is regulatedby a common factor, and the fact that the axr1-12 mutant is auxinresistant suggests that this factor may be auxin. If this is thecase, then the switch in the pattern of lateral shoot growth withfloral transition might be due to a change in auxin distribution.At floral transition, the primary shoot apex ceases producingleaves and it is these that are thought to be the source of axillarygrowth inhibition and the site of auxin production rather thanthe apical meristem itself (White et al., 1975; Weiss and Shillo,1988). With technical advances in auxin analysis (Uggla et al.,1996), detailed information on the temporal and tissue distributionof auxin in Arabidopsis may be obtained in thefuture.

Previous studies indicate that auxin does not act directly in the axillary bud, since apically applied radiolabeled IAA isnot transported into inhibited buds (Hall and Hillman, 1975; Morris,1977). To address the question of where auxin acts, we are currentlyexpressing the wild-type AXR1 gene in an axr1-12 mutant backgroundunder the control of a variety of tissue-specific promoters. Wehope to establish which tissues require the wild-type AXR1 proteinto repress axillary shootgrowth.

	ACKNOWLEDGMENTS

We thank Dr. Voijslava Grbi $c'$ for helpful discussions, Dr. Karin van de Sande, Dr. Jon Booker, and Stephen Day for criticalreading of the manuscript, Megan Stark for photographic work,and the horticultural technicians at the University of York forexcellent plantcare.

	FOOTNOTES

Received February 17, 1999; accepted July 14, 1999.

¹ This work was supported by a grant from the Biotechnology and Biological Sciences Research Council of the UnitedKingdom.

^* Corresponding author; e-mail hmol1{at}york.ac.uk; fax 44-1904-434312.

LITERATURE CITED

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
LITERATURE CITED

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AXR1 Acts after Lateral Bud Formation to Inhibit Lateral Bud Growth in Arabidopsis1

AXR1 Acts after Lateral Bud Formation to Inhibit Lateral Bud Growth in Arabidopsis¹