The control of maize spikelet meristem fate by the APETALA2-like gene indeterminate spikelet1

doi:10.1101/gad.12.8.1145

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Vol. 12, No. 8, pp. 1145-1154, April 15, 1998

RESEARCH PAPER
The control of maize spikelet meristem fate by the APETALA2-like gene indeterminate spikelet1

George Chuck,¹ Robert B. Meeley,² and Sarah Hake¹^,³^,⁴

¹ Department of Plant and Microbial Biology, University of California, Berkeley, California 94720, USA; ² Pioneer Hi-Bred International, Johnston, Iowa 50131, USA; ³ Plant Gene Expression Center, US Department of Agriculture-Agricultural Research Service (USDA-ARS), Albany, California 94710, USA

Abstract

Top
Abstract
Introduction
Results
Discussion
Materials & Methods
References

The orderly production of meristems with specific fates is crucial for the proper elaboration of plant architecture. The maizeinflorescence meristem branches several times to produce lateralmeristems with determinate fates. The first meristem formed, thespikelet pair meristem, produces two spikelet meristems, eachof which produces two floral meristems. We have identified a genecalled indeterminate spikelet1 (ids1) that specifies a determinatespikelet meristem fate and thereby limits the number of floralmeristems produced. In the absence of ids1 gene function, thespikelet meristem becomes indeterminate and produces additionalflorets. Members of the grass family vary in the number of floretswithin their spikelets, suggesting that ids1 may play a role ininflorescence architecture in other grass species. ids1 is a memberof the APETALA2 (AP2) gene family of transcription factors thathas been implicated in a wide range of plant development roles.Expression of ids1 was detected in many types of lateral organprimordia as well as spikelet meristems. Our analysis of the ids1mutant phenotype and expression pattern indicates that ids1 specifiesdeterminate fates by suppressing indeterminate growth within thespikelet meristem.

[Key Words: Meristem; spikelet; indeterminate spikelet1; APETALA2; determinacy]

	Introduction

Top Abstract Introduction Results Discussion Materials & Methods References

The development of the plant body is dependent on the activity of apical meristems, groups of indeterminate cells found atthe growing tips. The ability of shoot apical meristems to remainindeterminate allows them to continually initiate the organs,tissues, and secondary meristems required for normal development.This property requires that the meristem set aside a populationof cells to renew itself and replenish the cells lost to eachlateral organ or secondary meristem. The failure of this processto occur results in the termination of the growing tip. Some meristems,such as floral meristems, are consumed in the production of lateralorgans, and can be described as having a determinate fate. Theinflorescence of maize is particularly useful for studying meristemdeterminacy as it undergoes several well defined branching eventsto produce meristems with increasingly restricted fates.

Grass florets are organized into units called spikelets, each consisting of a pair of sterile bracts called glumes enclosinga fixed number of florets (Clifford 1987). The regulation of floretnumber per spikelet is a prime determinant of spikelet architectureamong members of the grass family. The spikelet of maize is determinate,producing only two florets in defined positions on an axis calledthe rachilla (Weatherwax 1923). Relatives of maize are characterizedby spikelets with an indeterminate number of florets, such aswheat, or contain only one floret per spikelet, as in barley.One classical criterion used to distinguish different grass speciesis whether their spikelets contain a determinate or indeterminatenumber of florets (Clifford and Watson 1977). The spikelet itselfis but one component of the complex branched inflorescence ofmaize. In contrast to dicotyledonous plants such as Arabidopsisin which flowers are produced directly by the apical and lateralmeristems (Hempel and Feldman 1994), there are at least two distinctinflorescence branching steps in maize before the spikelet meristemterminates in the production of two florets. These extra branchingsteps allow for greater morphological diversity among the grasses.

A number of mutants have been described in maize that result in an extra number of florets within the spikelet (Veit et al.1993). In the branched silkless mutants, extra florets are initiatedin male tassel spikelets (Kempton 1934), although a more extremetransformation is seen in female spikelets of the ear in whichflorets are transformed into long indeterminate branches (Veitet al. 1993). Studies of the Tasselseed6 mutation revealed thatthe spikelet meristem undergoes a delay in acquiring determinacy,allowing it to initiate florets for a longer period of time (Irishet al. 1994). The analysis of Tasselseed6 mutants led to a model(Irish 1997) in which the inflorescence meristem and its branchderivatives pass through an orderly, defined series of determinatedevelopmental states, ending with the conversion of the terminalspikelet meristem into the upper floret. Similar branching mutantshave also been described in other grass species and include themultiflorous mutation of barley (Bossinger et al. 1992) and thedominant Naked mutant of oats (Ougham et al. 1996).

An abundance of genetic and molecular studies have identified several genes important for floral development. One such gene,the APETALA2 (AP2) homeotic gene of Arabidopsis, has several functionsin flower, seed, and ovule development (Kunst et al. 1989; Jofukuet al. 1994; Modrusan et al. 1994). In addition to its role indetermining floral organ identity, AP2 affects the regulationof floral meristem identity. For example, double mutants of theweak ap2-1 allele with floral meristem identity mutants such asleafy or apetala1 produce more coflorescence side branches inthe place of flowers (Bowman et al. 1993). Also, weak ap2 allelesunder short days cause the formation of tertiary floral shootsin the axils of transformed sepals (Schultz and Haughn 1993).The AP2 gene belongs to a large gene family, 12 of which havebeen identified in Arabidopsis (Okamuro et al. 1997). Numeroushomologs have been identified in both monocots and dicots (Jofukuet al. 1994; Ohme-Takagi and Shinshi 1995; Moose and Sisco 1997).Mutations in the AP2-like gene, AINTEGUMENTA, are defective inovule development (Elliot et al. 1996; Klucher et al. 1996). Theglossy15 gene of maize has recently been shown to be an AP2-likegene that functions to repress adult leaf characters in juvenileleaves (Moose and Sisco 1997).

Here we describe a new branching mutant in maize, indeterminate spikelet1 (ids1), that we obtained by analyzing the phenotypeconditioned by loss of function of a maize AP2-like gene. ids1mutants have an indeterminate spikelet in which several floretsare produced instead of the two found in wild-type maize. ids1expression was observed in a variety of lateral organs as wellas the spikelet pair and spikelet meristems. Our analysis indicatesthat the ids1 gene is critical for the regulation of spikeletmeristem determinacy in maize.

	Results

Top Abstract Introduction Results Discussion Materials & Methods References

Isolation of the ids1 gene

The AP2 gene from Arabidopsis was used to screen two maize cDNA libraries at low stringency, one prepared from immature earsand the other from vegetative meristems. The same class of cDNAwas isolated from each library. The longest clone of this classwas 1967 nucleotides and contained an ORF of 433 amino acids (Fig.1) with several domains showing striking amino acid similarityto the AP2 gene of Arabidopsis (Jofuku et al. 1994). Two tandemlyrepeated 68 amino acid motifs were found that share 86% aminoacid identity with the AP2 domain of the Arabidopsis AP2 protein.The AP2 gene family can be classified into two groups, designatedas EREBP-like or AP2-like, on the basis of whether they possessone or two of the AP2 repeats, respectively (Okamuro et al. 1997).The IDS1 protein belongs to the latter class that includes theAP2, AINTEGUMENTA, GLOSSY15, and RAP2.7 proteins (Fig. 2) (Jofukuet al. 1994; Klucher et al. 1996; Moose and Sisco 1997; Okamuroet al. 1997). The tobacco ERE-BP proteins, which have only oneof these repeats, bind DNA (Ohme-Takagi and Shinshi 1995). Thus,by analogy it is likely that IDS1 functions as a transcriptionfactor. In support of this, a short stretch of basic amino acidsthat may function as a nuclear localization domain is presentin the IDS protein between animo acids 100 and 110 (Fig. 1). TheAP2 protein from Arabidopsis contains a serine-rich acidic domainat the amino terminus that may function as an activation domain(Jofuku et al. 1994). Although a similar region is found at theamino terminus of the IDS1 protein at positions 9-45, the regionis much smaller and has fewer acidic and serine residues comparedwith AP2. Outside the AP2 domain there is very little sequencesimilarity between AP2 and IDS1. Given this finding, it is surprisingthat the positions of six introns within the AP2 domain are conservedbetween ids1 and AP2 (Fig. 1). A similar result was found forthe gl15 gene of maize (Moose and Sisco 1997).

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Figure 1. Nucleotide and deduced amino acid sequence of IDS1. Amino acid numbers are shown to the left; nucleotides are numbered on the right. Underlined amino acid sequences represent the two AP2 domains (Jofuku et al. 1994

). Serines and acidic amino acids at the amino terminus are indicated with short underlines. Amino acid sequences in bold represent the basic region with putative nuclear localization activity. Bold nucleotide sequences correspond to the ZAP2-1 primer used for the PCR screen. ( $down-triangle$ ) The six intron positions conserved between IDS, AP2, and GL15; ( $black-down-triangle$ ) the other intron.

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Figure 2. Comparison between the AP2 domains of the AP2-like genes. The deduced amino acid sequences of the AP2 domains of IDS1 (GenBank accession no. AF048900), RAP2.7 (AF003100), GL15 (U41466), and ANT (U40256) are compared with AP2 (ATU12546). The region in between the two AP2 repeats, i.e., the linker region, starts at amino acid 78 and ends at 102. Gaps, represented by dots, were introduced to facilitate the alignment. Amino acids shared by all five proteins are shown in boldface type and on the consensus sequence at bottom.

ids1 was mapped to the long arm of chromosome one at position 192 by use of recombinant inbred lines (Burr et al. 1988) probedwith a nonrepetitive DNA fragment from the 3' end of ids1. Noknown morphological mutants have been mapped to this position.

Isolation of recessive ids1 mutations

To elucidate the function of ids1, we used a reverse genetic strategy to generate loss-of-function alleles. PCR was used ona large population of plants carrying Mutator (Mu) transposonsto find insertions into ids1 (Bensen et al. 1995; Meeley and Briggs1995). Primers flanking the AP2 domain of ids1 in combinationwith Mu primers yielded two independent insertion events throughthis screen. Sequencing of the PCR products localized the insertionsmore precisely. As shown in Figure 3, the Mu insertion in ids1-mum1was localized to the fifth conserved intron of the AP2 domain,whereas the ids1-mum2 insertion was localized to the first conservedintron 6 bp away from a splice acceptor site. Because Mu elementsgenerate a 9-bp duplication upon insertion (Bennetzen et al. 1993),the splice acceptor site is also found at the 5' end of Mu.

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Figure 3. Localization of the Mu elements in ids1-mum1 and ids1-mum2. ids1 intron and exon sequences are shown in normal and boldface lettering, respectively. Intron and exon numbers are shown above the DNA sequences. The underlined sequences represent the characteristic 9-bp duplication associated with Mu insertions.

Lines carrying the ids1-mum1 and ids1-mum2 alleles displayed a recessive floral phenotype that was more severe in ids1-mum2lines. To verify that the insertions into ids1 were responsiblefor the floral phenotype, we analyzed DNA from 104 F2 plants usingthe ids1 gene as a probe on DNA gel blots. Cosegregation of novelRFLPs with the floral phenotype was observed for 29 chromosomescontaining the ids1-mum1 allele and 91 chromosomes containingids1-mum2 (data not shown). No recombinants between the floralphenotype and ids1-mum-specific polymorphisms were found for eitherallele.

We analyzed the phenotypes of ids1-mum plants following a backcross into A632 and self-pollination. The most consistent phenotypein ids1-mum mutants was a defect in the spikelet. Mature wild-typetassel spikelets contain two florets each consisting of threestamens and two lodicules enclosed within palea and lemma bracts(Fig. 4B). The palea is distinguishable from the lemma by virtueof its position and the fact that it is bi-keeled with a doublemidrib (Clifford and Watson 1977). The spikelets of the ids1-mum2tassels are larger than those of wild type (Fig. 4A) because ofthe fact that extra florets are present (Fig. 4C). The numberof florets ranges from at least 3 in ids1-mum1 plants to as manyas 10 in ids1-mum2 plants. In addition to these florets, a thinrachilla containing several smaller florets can usually be seenin between the two uppermost florets (Fig. 4F). These smallerflorets tend to become progressively reduced, such that the onesremaining at the tip of the rachilla are barely visible. The largerextra florets show the normal pattern of sexual differentiationand have the correct number of stamens and lodicules surroundedby palea and lemma (Fig. 4C).

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Figure 4. Phenotypes in ids1-mum male and female spikelets. (A) Normal A632 tassel spikelet (left) and ids1-mum2 tassel spikelet (right). (B) Dissected normal A632 tassel spikelet showing lateral organs of upper and lower florets. (C) Dissected ids1-mum2 tassel spikelet showing four florets instead of two. Each floret has three stamens surrounded by palea and lemma as in A632. (D) Normal A632 ear spikelet (left) and ids-mum1 ear spikelet (right). Arrowheads point to silks. (E) Median longitudinal sections through unfertilized 25-day-old ids1-mum2 ear spikelet (left) and A632 ear spikelet (right). Black arrows point to florets. A632 spikelets have a single floret with an enlarged nucellus; ids1-mum2 ear spikelets have at least three florets with greatly reduced lateral organ development. (F) ids1-mum2 ear spikelet with an elongating rachilla containing two florets. The single arrowhead points to the tip of the rachilla. (st) Stamen; (il) inner lemma; (pa) palea; (ol) outer lemma; (ig) inner glume; (og) outer glume; (uf) upper floret; (lf) lower floret; (ra) rachilla; (fl) floret.

The ids1-mum female spikelets also exhibit a larger size as a result of the presence of extra florets (Fig. 4D,E). Normalfemale spikelets contain only a single mature floret because ofthe abortion of the lower floret (Delong et al. 1993). The developmentof secondary sexual characteristics in the female florets includethe abortion of stamens and the development of the gynoecium,as exemplified by the formation of long silks composed of twofused carpels (Randolph 1936). ids1-mum1 female spikelets oftencontain more than one silk located at ectopic positions (Fig.4D). These silks, however, usually do not develop normally; theyare often unfused and fail to elongate to their proper length.If the developing ear is manually opened and pollinated, a fewkernels develop, suggesting that all other aspects of fertilizationand fruit development are normal. When grown to maturity, thesekernels display ids1-mum homozygous phenotypes, and so do notrepresent germinal excisions of the Mu elements. The ids1-mum2allele appears more severe, in that most of the extra floretsfail to develop fully formed lateral organs (Fig. 4E, left). Approximately5% of the ids1-mum2 female spikelets show an elongating rachillathat emerges from the spikelet (Fig. 4F). In such cases, it canbe observed that the rachilla does not terminate in the uppermostfloret further confirming its indeterminate nature. No obviousand consistent phenotypes were seen in the leaves and roots ofids1 mutants despite the fact that ids1 is expressed in thoseorgans.

Scanning electron microscopy analysis

Scanning electron microscopy was used to determine the point at which ids1-mum spikelet meristem development diverges fromthat of wild type. The inflorescence meristem normally initiatesspikelet pair meristems acropetally, which, in turn, branch toform two spikelet meristems (Fig. 5A) (Cheng et al. 1983). Thespikelet meristems also branch to form the lower and upper florets.These florets initiate in a distichous pattern, that is, alternating180 degrees from one another (Fig. 5B). Although the lower floralmeristem initiates first, lateral organ development occurs inthe upper floret much earlier than in the lower floret (Fig. 5C,D).The palea is the first lateral organ to differentiate, and thethree stamens develop soon after (Cheng et al. 1983). Sexual differentiationoccurs at later stages in which the gynoecium aborts in male floretsand the stamens abort in female florets (Dellaporta and Calderon-Urrea1993).

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Figure 5. Scanning electron microscopy of normal and ids1-mum2 ears. (A) A632 ear primordium with initiating spikelet pair primordia and spikelet primordia. Bar, 300 µm. (B) A632 unbranched spikelet meristem (top) and slightly older branched spikelet meristem (bottom). The older spikelet meristem undergoes lateral branching to initiate the lower floret. Bar, 102 µm. (C) Development of lateral organs in A632 ear spikelets. The lateral organs of the upper floret develop first. Bar, 80 µm. (D) Maturing lateral organs of the upper floret of A632 ear spikelets with initiating gynoecial ridge. Bar, 104 µm. (E) Branching ids1-mum2 spikelet meristems. The uppermost spikelet meristem has not branched yet and appears elongated. Simultaneous floret branching and lemma initiation occurs on opposite sides of the middle and lower spikelet meristems. Bar, 156 µm. (F) Further development of ids1-mum2 spikelet meristems with glumes removed showing development of the floral meristems within the axils of the lemmas. The spikelet meristem persists after each branching event. Bar, 58 µm. (G) Older ids1-mum2 spikelet meristem with glumes removed. The residual spikelet meristem elongates to initiate another floret. Bar, 60 µm. (H) ids1-mum2 spikelet showing maturing lateral organs. There is no distinction between upper and lower floret in terms of lateral organ development. The youngest floret branching from the spikelet meristem is obscured by the lemma. Bar, 171 µm. (spm) Spikelet pair meristem; (sm) spikelet meristem; (lfm) lower floral meristem; (gy) gynoecium; (fm) floral meristem; (le) lemma.

ids1-mum mutants show normal development until the stage at which the spikelet meristem begins to branch. At this point, theids1-mum spikelet meristems appear slightly elongated (Fig. 5E,top). In slightly older spikelet meristems (Fig. 5E, middle),two distinct branching events can be seen as shown by the presenceof two lemmas (arrows). Floral meristems then form in the axilsof these lemmas (Fig. 5E, bottom, and F). These branching eventsoccur on opposite sides of the spikelet meristem in a distichouspattern. The spikelet meristem persists after each branching eventand remains in between the two last formed florets (Fig. 5G,H).This residual spikelet meristem continues to initiate extra lemmasand florets distichously (Fig. 5F,G). The rate of lateral organdevelopment between the first two ids1-mum florets is similar(Fig. 5H), in contrast to wild type in which the organs in theupper floret develop first.

We used the knotted1 (kn1) homeobox gene of maize, which is expressed in meristems and not in determinate lateral organs,to follow the branching events in ids1-mum spikelets. kn1 is expressedin the spikelet and floral meristems of maize (Fig. 6A,B) (Jacksonet al. 1994). Hybridization with a kn1 anti-sense probe on ids1-mum2spikelet meristems showed normal expression within the spikeletmeristem (Fig. 6C). However, as soon as the ids1-mum2 spikeletmeristem branches to form florets, the spikelet meristem becomeslarger, and consequently, the domain of kn1 expression expands(Fig. 6D). Strong kn1 expression is observed within the extraflorets initiating from the spikelet meristem at later stages(Fig. 6E, arrowheads) confirming the meristematic origins of theextra florets. All other aspects of kn1 expression within theflorets, including absence from the lateral organs and the L1layer, appear normal.

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Figure 6. In situ localization of kn1 within A632 and ids1-mum2 spikelet meristems. (A) kn1 expression within an unbranched A632 spikelet meristem. Bar, 50 µm. (B) kn1 expression within a branching A632 spikelet meristem. Expression can be seen in the initiating lower floret. Bar, 50 µm. (C) kn1 expression within an unbranched ids1-mum2 spikelet meristem. Bar, 50 µm. (D) kn1 expression within an early branching ids1-mum2 spikelet meristem. Initiating florets can be seen on both sides of the spikelet meristem. Bar, 60 µm. (E) kn1 expression within an older ids1-mum2 spikelet. Strong expression persists within the developing florets. Bar, 80 µm. Arrowheads point to initiating florets in B, D, and E.

Analysis of ids1 expression

An initial characterization of ids1 expression by use of RNA gel blots indicated that the gene was expressed in both vegetativeand floral tissues. An RNA gel blot probed with the 3' portionof the ids1 cDNA shows that ids1 transcript is present in alltissues tested (Fig. 7A). The lowest amount of expression wasseen in embryo tissue and the highest in inflorescence tissue.

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Figure 7. Analysis of ids1 expression in different organs of B73 maize. (A) An RNA gel blot containing 1 µg of poly(A)⁺ RNA isolated from embryos 17 days postpollination (E), shoot meristems including unexpanded stem and the youngest leaf primordia (M), ear inflorescence primordia up to 2 cm long (I), primary roots from seeds germinated in humid air (R), and the blade portion of fully expanded juvenile leaves (L) was blotted and hybridized to the 3' portion of the ids1 cDNA that does not include the AP2 domain. (B) Control hybridization. The blot in A was probed with the maize ubiquitin cDNA to show relative loading.

To determine the levels of ids1 transcript in ids1-mum mutants, poly(A)⁺ RNA was isolated from mutant ears and compared with RNA fromwild-type ears. As shown in Figure 8A, no wild-type size transcriptwas found in either ids1-mum allele. Instead, faint, higher molecularweight transcripts were observed that may be the result of chimericor alternatively spliced transcripts. This result demonstratesthat the Mu element insertions into ids1 are not spliced out,and that both ids1-mum1 and ids1-mum2 may represent loss-of-functionalleles.

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Figure 8. Analysis of ids1 expression in ids1-mum mutant ears. (A) An RNA gel containing 1 µg of poly(A)⁺ RNA isolated from 2-cm ears from A632 (1), ids1-mum2 (2), and ids1-mum1 (3) was blotted and hybridized to the 3' portion of the ids1 cDNA. (B) Control hybridization. The blot in A was probed with the maize ubiquitin cDNA to show relative loading.

To localize the temporal and spatial pattern of ids1 expression more precisely, we used in situ hybridization. Figure 9A showslongitudinal sections of a wild-type vegetative shoot apex probedwith digoxigenin labeled anti-sense RNA made from the 3' end ofthe ids1 clone. The positions of leaves within the maize shoothave been described in terms of the plastochron index (Lamoreauxet al. 1978) in which the youngest leaf is referred to as plastochron1 or P₁ and successive leaves as P₂, P₃, etc. The position ofthe incipient leaf in the meristem is referred to as P₀. ids1expression is detected on the flanks of the meristem in a discretezone (Fig. 9A). From the position of the youngest leaf (labeledas P₁), we assume this zone of meristem expression is in the positionin which the next leaf will initiate (labeled as P₀). Expressionis also seen in the tips of the next two older leaves, P₁ andP₂.

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Figure 9. In situ localization in B73 vegetative and floral apices by use of the 3' portion of the ids1 cDNA. (A) Shoot apical meristem with young leaf primordia (P₁ and P₂) and incipient leaf primordia (P₀). Bar, 65 µm. (B) Young ear inflorescence. ids1 expression can be seen in the acropetally initiating spikelet pair primordia. Bar, 70 µm. (C) Unbranched spikelet meristems. Expression can be seen in the spikelet meristem but not in the glumes. Bar, 36 µm. (D) Branching spikelet meristems. Strong expression can be seen in the inner and outer lemmas as well as the zone in between the initiating upper and lower florets (unlabeled arrow). This zone of expression gradually disappears in the older spikelet below. No expression is detected in the initiating floral meristems. Bar, 70 µm. (E) Upper floret with initiating stamens. Discrete areas of ids1 expression can be observed in the initiating stamen primordia and palea. ids1 expression persists in the expanding inner and outer lemmas. Bar, 70 µm. (F) Older floret with lodicules. Stamen expression now localizes to the locule chambers of the anther. No expression can be seen in the lodicules (lo). Bar, 70 µm. (G) ids1-mum2 spikelet probed with ids1. Little or no ids1 transcript can be detected. Arrowheads point to florets. Bar, 130 µm.

In longitudinal sections of floral tissue, ids1 expression is detected in several different lateral organ primordia as wellas the spikelet pair and spikelet meristems. In Figure 9B, longitudinalsections of early inflorescence meristems probed with ids1 showstripes of expression in a repeating pattern that evidently correspondsto spikelet pair primordia. At a later stage, after the pedicellateand sessile spikelets form, ids1 expression is found throughoutthe spikelet meristem but not in the first two lateral organ primordiaformed from the spikelet meristem, the outer and inner glumes(Fig. 9C). Soon after floral meristems initiate (Fig. 9D), ids1expression is present in the initiating inner and outer lemmabract leaves subtending the florets, but is absent from the floralmeristem itself. In addition, a strong band of expression is seenin the region between the upper and lower florets (Fig. 9D, unlabeledarrow). In slightly older spikelets as shown at the bottom ofFigure 9D, this band of expression begins to disappear. A scanningelectron micrograph of spikelets at equivalent stages is shownin Figure 5B. In more mature tassel florets (Fig. 9E), discretegroups of cells of the floral meristem that are positioned toform the stamens and palea express ids1. Expression persists atlater stages in the older expanded palea and lemma and also thelocule chambers of the anther (Fig. 9F). Little or no expressionwas seen in the lodicules or the gynoecium of the ear (Fig. 9F;data not shown). As shown in Figure 9G, when an anti-sense ids1probe is used on ids1-mum spikelets, no ids1 expression is detected.

	Discussion

Top Abstract Introduction Results Discussion Materials & Methods References

Regulating the number of florets initiated by the spikelet meristem is a critical step in the determination of spikelet morphology.Mutations within the ids1 gene affect spikelet meristem determinacy.Instead of producing only an upper and lower floret, the ids1-mumspikelet meristem continues to initiate additional florets ina distichous phyllotaxy. Understanding how ids1 promotes spikeletmeristem determinacy requires an examination of different modelsfor maize floret initiation.

One model for floret initiation suggests that the lower floret is initiated laterally whereas the upper floret is terminal,produced by the transformation of the spikelet meristem into theupper floret (Fig. 10A) (Irish 1997). In some grass species suchas anthoxanthum, the spikelet terminates in a flower with theovule being the terminal structure (Clifford 1987). If the upperfloret is a terminal structure in normal maize development, theIDS1 protein may function to promote the transformation of thespikelet meristem into the upper floret. IDS1 may do this alone,or through the activation of floral meristem identity genes suchas orthologs of LEAFY and APETELA1 that can transform inflorescencemeristems into floral meristems (Mandel and Yanofsky 1995; Weigeland Nilsson 1995). If this were the case, we would speculate thatthe transformation of spikelet meristem to floral meristem isdelayed in ids1-mum mutants, allowing the spikelet meristem topersist and initiate more florets. Such an interpretation hasbeen invoked to explain the phenotype of the dominant Ts6 mutantsof maize in which extra florets form (Irish 1997). Ts6 mutantsdiffer from ids1-mum mutants, however, in that they also affectsex determination and cause an absence of carpel suppression withinthe tassel, but not in the ear.

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Figure 10. Models for maize floret initiation. (A) Terminal upper floret model. The spikelet meristem branches once laterally to form the lower floret. The residual spikelet meristem (shown in black) is then transformed into the upper floret (black). (B) Lateral branching model. The spikelet meristem undergoes lateral branching to form the lower and then upper florets. The residual spikelet meristem (shown in black) is found in a small region in between the florets. A rudiment of the spikelet meristem in found in the rachilla in the mature spikelet (black).

An alternative model would suggest that both upper and lower florets are lateral products of the spikelet meristem. The twoflorets of maize have been interpreted as lateral branches ofthe rachilla with little or no remnant of the axis left in betweenthe florets (Bonnett 1953). If upper floret branching is lateral,then a greatly reduced rudiment of the spikelet meristem mightbe found in the rachilla after upper floret initiation (Fig. 10B).According to this model, IDS1 would participate in suppressionof indeterminate growth within the spikelet meristem, thus preventingthe spikelet meristem from regenerating after upper floret branching.In ids-mum mutants the residual spikelet meristem proliferatesand continues to initiate florets.

On the basis of the expression pattern of ids1 and the timing of the ids1-mum defects, we favor the second model and hypothesizethat IDS1 functions to suppress indeterminate growth within thespikelet meristem. According to the first model, the switch inspikelet meristem fate occurs only after the lower floret is initiated.However, defects in ids1-mum spikelet meristems were first observedin the spikelet meristem prior to lower floret initiation (Fig.5E). The timing of the defect suggests that the change in fatedetermination occurs earlier, in agreement with the ids1 expressionobserved in the spikelet meristem before floret branching occurs(Fig. 9C). The first model also suggests that the entire spikeletmeristem becomes transformed into an upper floret, leaving noresidual spikelet meristem. Yet, ids1 expression was detectedin a zone between the upper and lower florets in wild type (Fig.9D) in which the residual spikelet meristem would be expectedto be located. Additional evidence that this region representsthe residual spikelet meristem comes from the observation thatit regenerates after floret branching in ids1-mum mutants (Fig.5F,G). Furthermore, an expectation of the first model is thatids1 would be expressed throughout the future upper floret topromote its transformation to floral identity. Instead, as shownin Figure 9D, we see no ids1 expression in either the upper orlower floral meristems. Finally, if determinacy of the spikeletmeristem were simply being delayed in ids1-mum mutants in accordancewith the first model, one would expect to see the rachilla eventuallyterminate in a floret. This was not observed in either male andfemale ids1-mum spikelets (Fig. 4F; data not shown).

The development of a critical meristem size in maize is thought to provide the cue for branching to occur (Sundberg and Orr1996). One mechanism by which IDS1 may suppress indeterminategrowth is to restrict the size of the residual spikelet meristemsuch that it can no longer initiate florets. In ids1-mum mutants,the size of the residual spikelet meristem may be deregulatedand expand to larger than normal. A larger spikelet meristem couldpotentially allow greater numbers of branching events to produceextra florets. In support of this idea, the ids1-mum spikeletmeristem appears more elongated than normal before florets areinitiated (Fig. 5E). Also, a larger spikelet meristem diameteris observed soon after the first floret is initiated in ids1-mummutants (Fig. 6D).

It is important to recognize, however, that meristem fate is not always dependent on meristem size. For example, the upperfloral meristem is much larger that the lower floral meristemat the time of initiation (Fig. 5B), and yet both are equallydetermined to make florets. Thus, having a larger spikelet meristemwould not necessarily endow it with greater indeterminacy. Anequally important component of the distinction between determinateand indeterminate spikelet meristem fates is the ability to regenerateafter floret initiation. Meristems with indeterminate fates mayshow a greater ability at self-regeneration regardless of theirinitial size. The altered morphology seen in the spikelet meristemsof the ids1-mum mutants may simply be a reflection of this ability.

It is possible that one way IDS1 functions to maintain spikelet meristem determinacy is to repress those factors necessaryfor maintaining indeterminacy. The kn1 homeobox gene is expressedin several types of indeterminate meristematic tissues and notin determinate organs such as leaves (Smith et al. 1992; Jacksonet al. 1994). Loss-of-function mutants of kn1 in maize show reducedtassel branching and fewer spikelets. This phenotype has beenpostulated to result from a loss of indeterminate inflorescencecells which, in the absence of kn1, have adopted determinate fates(Kerstetter et al. 1997). If kn1 is in fact maintaining meristemindeterminacy, then kn1 expression should persist within the ids1-mumspikelet meristem and show an expanded domain. Although this wasobserved (Fig. 6D), it is important to note that kn1 is normallyexpressed in both spikelet and floral meristems (Fig. 6A,B). Thus,the fact that the domain of kn1 expression is expanded in ids1-mummutants may simply reflect extra areas of floret initiation.

The ids1 gene was cloned by homology to the AP2 gene of Arabidopsis and shown to contain two repeats of the highly conservedAP2 domain. Although the IDS1 protein shows greater similarityto AP2 compared with all other AP2-like genes cloned thus far,the ids1 gene may not represent the actual AP2 ortholog of maize.The amino acid homology between IDS1 and AP2 does not extend outsideof the AP2 domain. Furthermore, the expression of ids1 was notdetected in carpels, as is found for AP2 (Jofuku et al. 1994).Finally, preliminary experiments show that the overexpressionof the ids1 cDNA in Arabidopsis does not complement the ap2-1mutant phenotype (G. Chuck unpubl.). Additional AP2 gene familymembers are likely to be present in the maize genome, becauselow stringency hybridizations with the ids1 AP2 domain as a probeon maize Southern blots show several hybridizing bands (data notshown). In addition, several expressed sequence tags from maizecDNA libraries have been shown to have AP2 domains (Klucher etal. 1996).

Even though ids1 is expressed in vegetative and floral lateral organ primordia, no obvious mutant phenotypes were detectedin those organs. A certain level of genetic redundancy may operatein these organs, which can only be uncovered through the analysisof double mutants. For example, double mutants of ap2 and aintegumentashow floral organ phenotypes not seen in either single mutantin Arabidopsis (Elliot et al. 1996). Considering the large numberof AP2-like genes present in the genome of Arabidopsis (Okamuroet al. 1997), it would not be surprising to find such functionalredundancy occurring in maize. Recently, it has been suggestedthat two closely related MADS box genes, zag1 and zmm2, play redundantroles in specifying carpel and stamen identity in maize (Menaet al. 1996).

Although floral organs of ids1-mum tassel florets are fully functional and resemble those of wild type, floral organ defectswere observed in ids1-mum female spikelets. A possible explanationfor this defect may lie in the fact that the lower floret abortsin normal female spikelets. If the distinction between upper andlower florets is lost in ids1-mum mutants, then all the floretsmay receive the abortion signal that is normally only presentin the lower floret in wild type. Double-mutant analysis withthe tasseled 2 mutant, in which lower floret abortion does notoccur (DeLong et al. 1993) will be useful to test this model.

In light of the fact that many members of the grass family possess indeterminate spikelets, it is tempting to speculate thatAP2-like genes play a role in regulating floret number in othergrasses. Spikelets with many florets are assumed to be an ancienttrait given that derived species have almost universally evolveda reduction in floret number (Stebbins 1987). A possible mechanismfor such a reduction may have involved a change in the functionor domain of expression of the ids1 gene to include the spikeletmeristem in addition to the various lateral organs where it isnormally expressed. The analysis of ids1 expression in both modernand ancient grasses will be interesting to analyze in this regard.

	Materials and methods

Top Abstract Introduction Results Discussion Materials & Methods References

Cloning the ids1 gene

Forty thousand plaques of a B73 cDNA library constructed from 1- to 3-cm inflorescence ears (Jackson et al. 1994) were probedat reduced stringency at 55°C in 50% formamide (Schmidt et al.1993) with the full-length AP2 cDNA from Arabidopsis (Jofuku etal. 1994). Approximately 75 positive clones were isolated. Onlythe strongest hybridizing class was analyzed further. A representativeclone from this class was used to probe a B73 vegetative meristemcDNA library (Lambda ZapII, Stratagene) from which a full-length1.9-kb cDNA was isolated. The cDNA was subcloned into pSK- andboth strands sequenced with an ABI sequencer. Sequence analysiswas done by use of GCG (Wisconsin Genetics Group) and the NationalCenter for Biotechnology Information Blast E-MAIL server.

RNA gel blots and in situ hybridization

RNA was isolated from embryos, ears, vegetative meristems, and roots as described previously (Kerstetter et al. 1994). Insitu hybridization was performed as described by Jackson et al.(1994) by use of a 3' end probe between nucleotides 1330 and 1835outside the conserved AP2 domain. This same DNA fragment was usedto probe all RNA gel blots. A single band is observed to hybridizeto this probe on DNA gel blots (data not shown), therefore, crosshybridization with other AP2 family members is unlikely.

Isolation of recessive ids1 alleles by PCR

Approximately 42,000 F₁ plants from crosses between stocks containing active Mu transposable elements were grown and screenedby PCR by Pioneer Hi-Bred International for insertion into ids1(Bensen et al. 1995) with the ZAP2-1 primer (5'-CCGGTGGCGCCAGCGAAGAA-3')and Mu-9242 (5'-CCCTGAGCTCTTCGTC(CT)ATAATGGCAATTATCTC-3'), a degenerateprimer that binds to the terminal inverted repeat of Mu. PCR reactionswere run on gels, blotted, and probed with the ids1 cDNA. PCRproducts that hybridize to the ids1 cDNA identified individualsthat likely have Mu insertions into the ids1 gene. Such a screenidentified nine candidates by use of the ZAP2-1 primer. DNA gelblot analysis of digested DNA made from self-pollinated progenyof each candidate revealed polymorphisms for only two of the ninefamilies when probed with the ids1 cDNA. These same two familieswere the only ones that generated ids1 PCR products by use ofthe ZAP2-1 and Mu 9242 primers. It is likely that the seven otherfamilies that showed no polymorphisms represent somatic insertionevents of Mu into ids1 that did not transmit into the germ line.Each ids1-mum allele was generated from a cross between a Mu activeline and the A632 inbred line. Both alleles were backcrossed toA632 once and self-pollinated to observe phenotypes in the homozygotes.The phenotypes were also observed after a second backcross toA632 and a backcross to inbred W23.

Scanning electron microscopy

Tissue was fixed in FAA (50% ethanol, 5% acetic acid, 3.7% formaldehyde) at 4°C overnight and dehydrated in a graded ethanolseries to 100%. The samples were then critical point dried andsputter coated with palladium. Samples were viewed on an ISI 30SEM at 10 kV accelerating voltage.

	Acknowledgments

We thank J. Okamuro and D. Jofuku (University of California, Santa Cruz) for the gift of the AP2 cDNA, R. Kerstetter for theuse of his RNA blot, and K. Canada (Pioneer Hi-Bred International)for identifying ids1 insertions. We are also grateful to E. Vollbrecht,P. McSteen, L. Reiser, F. Hempel, and the members of the Hakelaboratory for reviewing the manuscript and providing helpfuldiscussions. G.C. was supported by a University of Californiafellowship. This work was supported by the U.S. Department ofAgriculture and performed, in part, under a Cooperative Researchand Development Agreement with Pioneer Hi-Bred International,Inc.

The publication costs of this article were defrayed in part by payment of page charges. This article must therefore be herebymarked "advertisement" in accordance with 18 USC section 1734solely to indicate this fact.

	Footnotes

Received November 3, 1997; revised version accepted February 26, 1998.

⁴ Corresponding author.

E-MAIL maizesh{at}nature.berkeley.edu; FAX (510) 559-5678.

References

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Abstract
Introduction
Results
Discussion
Materials & Methods
References

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RESEARCH PAPER The control of maize spikelet meristem fate by the APETALA2-like gene indeterminate spikelet1

RESEARCH PAPER
The control of maize spikelet meristem fate by the APETALA2-like gene indeterminate spikelet1