- Research article
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Conserved roles for Polycomb Repressive Complex 2 in the regulation of lateral organ development in Aquilegia x coerulea ‘Origami’
BMC Plant Biology volume 13, Article number: 185 (2013)
Abstract
Background
Epigenetic regulation is necessary for maintaining gene expression patterns in multicellular organisms. The Polycomb Group (PcG) proteins form several complexes with important and deeply conserved epigenetic functions in both the plant and animal kingdoms. One such complex, the Polycomb Repressive Complex 2 (PRC2), is critical to many developmental processes in plants including the regulation of major developmental transitions. In addition, PRC2 restricts the expression domain of various transcription factor families in Arabidopsis, including the class I KNOX genes and several of the ABCE class MADS box genes. While the functions of these transcription factors are known to be deeply conserved, whether or not their regulation by PRC2 is similarly conserved remains an open question.
Results
Here we use virus-induced gene silencing (VIGS) to characterize the function of the PRC2 complex in lateral organ development of Aquilegia x coerulea ‘Origami’, a member of the lower eudicot order Ranunculales. Leaves with PRC2 down-regulation displayed a range of phenotypes including ruffled or curled laminae, additional lobing, and an increased frequency of higher order branching. Sepals and petals were also affected, being narrowed, distorted, or, in the case of the sepals, exhibiting partial homeotic transformation. Many of the petal limbs also had a particularly intense yellow coloration due to an accumulation of carotenoid pigments. We show that the A. x coerulea floral MADS box genes AGAMOUS1 (AqAG1), APETALA3-3 (AqAP3-3) and SEPALLATA3 (AqSEP3) are up-regulated in many tissues, while expression of the class I KNOX genes and several candidate genes involved in carotenoid production or degradation are largely unaffected.
Conclusions
PRC2 targeting of several floral MADS box genes may be conserved in dicots, but other known targets do not appear to be. In the case of the type I KNOX genes, this may reflect a regulatory shift associated with the evolution of compound leaves.
Background
Maintenance of proper gene expression in differentiated cells is essential for the development of multicellular organisms and epigenetic regulation is an important player in this process Reviewed in: [1–3]. One family of proteins with deeply conserved functions in epigenetic regulation is the Polycomb Group (PcG). The PcG was first discovered in Drosophila melanogaster as repressors of the HOX genes [4]. Several PcG complexes exist in both plants and animals, each with distinct functions in epigenetic silencing Reviewed in: [5, 6]. However, only the Polycomb Repressive Complex 2 (PRC2) has been well characterized in multiple plant models Reviewed in: [5, 7]. The main function of the PRC2 complex is trimethylation of lysine 27 of histone H3 (H3K27), a histone modification known to suppress gene expression [8]. The PRC2 contains four core proteins; the histone methyltransferase Enhancer of Zeste (E(z)), and three other proteins thought to enhance PRC2 binding to nucleosome [9]. These include Suppressor of Zeste 12 (Su(z)12) and Extra Sex Combs (ESC), known respectively as EMBRYONIC FLOWER 2 (EMF2) and FERTILIZATION INDEPENDENT ENDOSPERM (FIE) in plants, and Multi-Copy Suppressor of IRA 1 (MSI1) Reviewed in: [10]. The E(z) lineage in plants has experienced an ancient duplication such that most angiosperms have at least two paralogs, known as CURLY LEAF (CLF) and SWINGER (SWN) [11]. Many plant species have additional duplications in the core PRC2 loci that allow them to form several PRC2 complexes often with distinct developmental functions [12, 13].
PRC2 is involved in a number of important developmental transitions. In the plant model system A. thaliana, these functions include endosperm development, early repression of flowering to allow proper vegetative development, the eventual transition to flowering, and flower organogenesis [14–17]. In grasses, the PRC2 complex plays roles in floral induction (rice and barley), flower development (rice), suppressing cell divisions in the unfertilized ovule (rice), and endosperm development (rice and maize) [12, 18, 19]. In the moss model Physcomitrella patens, PRC2-dependent remodeling appear to be required for the switch from gametophyte to sporophyte development [20, 21].
In addition to its role in developmental transitions, PRC2 has been suggested to function in lateral organ development in A. thaliana. In fact, the first description of a plant PRC2 function was discovered with the characterization of the clf mutant in A. thaliana[17]. The clf plants had severely curled leaves, smaller narrower sepals and petals, and partial homeotic transformations of sepals and petals towards carpel and stamen identity, respectively. Two MADS box genes, the C class member AGAMOUS (AG) and the B class representative APETALA3 (AP3) were shown to be over-expressed in clf mutants, suggesting that the PRC2 complex was required for stable repression of these genes [17]. This was particularly interesting because MADS box genes regulate homeotic floral organ identity in plants somewhat analogously to the way HOX genes regulate segment identity in animals [22–25]. Further studies have subsequently shown that the E class MADS SEPALLATA3 (SEP3) is similarly up-regulated in clf mutants [26]. PRC2 has also been shown to regulate the expression of the class I KNOX genes during vegetative development. The class I KNOX genes are a family of homeobox domain-containing loci in plants that have conserved roles in promoting pluripotency in the shoot apical meristem and in compound leaf development [27, 28]. Katz et al [29] found that in addition to the phenotypes reported in clf mutant plants, FIE cosuppressed plants also had loss of apical dominance and fasciated stems, rolled leaves with varying degrees of serration, loss of phyllotaxy in the inflorescence, and many problems with ovary and ovule development. They further demonstrated that several class I KNOX genes, including BREVIPEDICELLUS (BP), KNOTTED-LIKE FROM ARABIDOPSIS THALIANA 2 (KNAT2), and SHOOTMERISTEMLESS (STM), were over-expressed in rosette leaves of FIE silenced plants. In clf mutants, STM and KNAT2 were over-expressed but BP was not, possibly because the CLF paralog SWN was acting redundantly. The class I KNOX genes MOSS KNOTTED1-LIKE 2 and 5 (MKN2 and MKN5) were also shown to be over-expressed in PpFIE mutant gametophytes [21, 30], suggesting that PRC2 targeting of the class I KNOX genes may be deeply conserved.
While the functions of the floral ABC class and type I KNOX genes are thought to be conserved across angiosperms, comparative studies of their regulation have largely focused on upstream transcription factors, such as LEAFY or ARP family members [31, 32]. In order to begin addressing the question of whether PRC2-targeting interactions are similarly conserved, we have examined the functions of PRC2 members in lateral organ development of the emerging model system Aquilegia. The genus Aquilegia is a member of an early diverging lineage of the eudicotyledonous flowering plants, the Ranunculales, that arose before the radiation of the core eudicots Reviewed in: [33]. It therefore can be used as a rough phylogenetic midpoint between A. thaliana and model systems in the grasses [34]. Additionally, many ecological, evolutionary and genetic studies have been conducted in Aquilegia over the past 50 years. These have taken advantage of its small genome (n = 7, approximately 300 Mbp) as well as a number of more recent genomic tools, including the fully sequenced Aquilegia x coerulea genome (http://www.phytozome.net/search.php?method=Org_Acoerulea) Reviewed in: [33, 35]. The reverse genetic tool virus-induced gene silencing (VIGS) has been optimized in several species of Aquilegia[36] for both leaf and floral development [37–40]. Previously we examined the evolution and expression of the PRC2 family in Aquilegia[41] and found that the genome contains a simple complement of PRC2 homologs: one copy each of the two plant E(z) homologs, AqCLF and AqSWN; an ESC homolog, AqFIE; a Su(z)12 homolog, AqEMF2; and a copy of MSI1, AqMSI1. We initially assessed gene expression throughout Aquilegia vulgaris development due to its strong vernalization dependency and found no obvious tissue or stage specialization. Furthermore, the ancient paralogs, AqCLF and AqSWN, are not imprinted in Aquilegia endosperm as is seen in other plant species [19, 41].
In the current study we have used VIGS to knock down the expression of AqFIE [Genbank: JN944599] and AqEMF2 [Genbank: JN944598] in unvernalized and vernalized Aquilegia coerulea ‘Origami’ plants using the ANTHOCYANIN SYNTHASE (AqANS) as a marker gene. Due to limitations of the VIGS approach, it is not possible to assess many life cycle transitions, most notably flowering time, but lateral organ development can still serve as a useful model for PRC2 function. We find that PRC2 plays a role in leaf and floral organ development in A. x coerulea, particularly via down-regulation of the floral MADS box genes. This has allowed us to identify PRC2 targets that appear to be conserved between Arabidopsis and Aquilegia as well as some novel PRC2-regulated pathways.
Methods
Virus-induced gene silencing
The Aquilegia VIGS protocol was preformed as described previously [36]. TRV2-AqCLF-AqANS, TRV2-AqSWN-AqANS, TRV2-AqFIE-AqANS and TRV2-AqEMF2-AqANS constructs were prepared by PCR amplifying approximately 300 bp regions of each gene using primers that added EcoR1 and XbaI restriction sites to the 5′ and 3′ ends of the PRC products (see Additional file 1). The PCR products were then purified and cloned into the TRV2-AqANS construct [36] and electroporated into Agrobacterium strain GV101. A. x coerulea seedlings were grown to approximately the 4 to 6 leaf stage and then either treated as described in Gould and Kramer [36] for unvernalized samples or as described in Sharma and Kramer [37] for plants that had been vernalized for approximately 4 weeks at 4°C [36, 37]. The TRV2-AqANS and TRV2-AqFIE-AqANS constructs were each used to treat approximately 400 plants over 4 rounds of VIGS. Approximately 250 of these plants were VIGS treated before vernalization and approximately 150 of these plants were treated after vernalization. The TRV2-AqEMF2-AqANS construct was used to treat approximately 100 plants; roughly 50 of these plants were treated before vernalization and 50 were treated after vernalization. Leaves, petals, and sepals showing AqANS silencing were photographed, collected, and stored at -80°C for RNA analysis.
RT-PCR
RNA was extracted from control (AqANS silenced) and experimental (AqFIE and AqEMF2 VIGS-treated) tissue. One half of the AqANS silenced (control) leaves were from separate unvernalized plants (C1 and C2) and half were from separate vernalized plants (C3 and C4). Five of the TRV2-AqFIE-AqANS treated leaves were from separate unvernalized plants (F2, F4, F5, F7, and F8) while three were collected from separate vernalized plants (F1, F3, and F6). All of the TRV2-AqEMF2-AqANS leaves were collected from separate vernalized plants (E1-E4). Sample numbers do not indicate order of leaf appearance but were collected at roughly the same stages of development. We selected a variety of observed phenotypes for each set of samples. For leaves, the RNeasy Mini Kit (Qiagen, Valencia, CA) was used. For petals and sepals RNA was extracted using the Pure-Link Plant RNA Reagent small scale RNA isolation protocol (Ambion, Austin, TX). RNA was treated with Turbo DNase (Ambion, Austin, TX) and cDNA was synthesized from 1 μg of total RNA using Superscript II reverse transcriptase (Invitrogen, Carlsbad, CA) and oligo (dT) primers. cDNA was diluted 1:5 prior to use.
Amplification was performed using AccuStart PCR SuperMix (Quanta Biosciences Inc, Gaithersburg, MD). The amplification program began with 1 minute activation step at 94°C, followed by a 20 second denaturing step at 94°C, a 15 second annealing step at 55°C, and a 15 second extension at 72°C, repeated for 30 cycles. This cycle number was chosen for optimal detection of AqFIE and AqEMF2, which are expressed at relatively low levels in mature organs, especially compared to the high expression levels of AqIPP2. All primers used are listed in Additional file 1. Amplification of ISOPENTYL PYROPHOSPHATE:DIMETHYLALLYL PYROPHOSPHATE ISOMERASE2 (AqIPP2) was used as a positive control [38, 42]. To test for expression of APETALA3-1 (AqAP3-1), APETALA3-2 (AqAP3-2), APETALA3-3 (AqAP3-3), and FUL-like- 1 (AqFL1) in VIGS-treated leaves, cDNA from several leaves were pooled together prior to amplification. The control pool consisted of AqANS-silenced control leaves C1-4, the AqFIE VIGS-treated pool consisted of AqFIE leaves F3-6, and the AqEMF2 VIGS-treated pool consisted of AqEMF2 leaves E1-4.
qRT-PCR
cDNA was prepared from VIGS-treated tissue as described above. For the carpel sample, carpels were collected from 3 anthesis stage wild type plants and pooled together. RNA was extracted using the RNeasy Mini Kit (Qiagen, Valencia, CA) and treated as described above. cDNA from VIGS-treated tissue was then pooled together and diluted 1:10. The control sepal pool consisted of AqANS-silenced control sepals C1-4, the control petal pool consisted of AqANS-silenced control petals C1-4, the AqFIE sepal pool consisted of AqFIE VIGS-treated sepals F2, 3, 5, and 6, the AqFIE petal pool consisted of AqFIE VIGS-treated petals F2, 3, 5, and 6, the AqEMF2 sepal pool consisted of AqEMF2 VIGS-treated sepals E2, 3, and 4 s, and the AqEMF2 petal pool consisted of AqEMF2 VIGS-treated petals E1 and E2. qRT-PCR was performed using PerfeCTa qPCR FastMix, Low ROX (Quant Biosciences Inc., Gaithersburg, MD) in the Stratagene Mx3005P QPCR system to study the relative expression of AqAG1 and AqAG2. AqIPP2 expression was used for value normalization. All primers are listed in Additional file 1.
Microscopy
Petals from wild type, AqANS VIGS-treated, and AqEMF2 VIGS-treated plants were stored at -80°C and then warmed to room temperature and mounted whole on glass slides in water. Cells were visualized in the Harvard Center for Biological Imaging on a Zeiss AxioImager Z2 microscope using trans-illumination with white light. Images were taken using a Zeiss AxioCam Mrc digital camera.
Results
We treated both unvernalized and vernalized plants with TRV2 constructs containing either AqANS-AqFIE or AqANS-AqEMF2 fragments. TRV2-AqANS treated plants were used as controls throughout. Phenotypes of AqFIE and AqEMF2 silenced plants were equivalent and will be discussed together. We also treated a small number of unvernalized plants with AqANS-AqCLF and AqANS-AqSWN VIGS constructs. Phenotypes from these plants were similar to those seen in AqFIE and AqEMF2, but were weaker (data not shown), most likely due to partial redundancy between AqCLF and AqSWN. Thus we chose to focus on AqFIE and AqEMF2 VIGS-treated tissue. As is common for VIGS-treated plants, we recovered a range of phenotypes in a small percentage of VIGS-treated plants (roughly 10-15% of plants in each round) [36]. In the current experiment there is the added component that phenotypes are likely due to mis-expression of PRC2 target genes, and are therefore likely to have an added complexity due to ectopic expression of a potentially wide range of target loci.
Vegetative phenotypes
Wild type Aquilegia leaves are compound, typically bearing three leaflets that are themselves divided into two to three lobes (Figure 1A). Although these leaflets are often relatively deeply lobed, they do not generally produce elongated, higher order petiolules within the leaflets. However, A. x coerulea does display heteroblasty over the course of its lifespan, varying leaf morphology as the individual progresses from the vegetative to the reproductive stage (Additional file 2). In late reproductive adult stages, higher order petiolules may be observed in which the central lobe of each leaflet becomes itself a separate leaflet borne its own petiolule (Additional file 2C). Using the terminology of Kim et al. 2003 [32], all of these leaf forms are non-peltately palmate in that the leaflets are not radially positioned around the terminus of the primary petiole.
We observed AqANS silencing in 10-15% of treated plants across the AqFIE- and AqEMF2-VIGS experiments. In addition to the AqANS-silencing, the leaves of these plants showed a complex set of phenotypes. The most consistently observed perturbation was curled or ruffled laminae that typically curled toward the abaxial surface (~10-12% of treated plants and, thus, the majority of silenced plants) (Figure 1F, H, J-L). We also observed an increased frequency of higher order branching in which fully formed petiolules developed within the leaflet, creating as many as ten or twelve distinct leaflets rather than the usual three (Figure 1B-F, H, L and Additional file 2E). While we have never observed such higher order branching in control leaves, either in the context of these experiments or others [40], we obtained 15 leaves from a total of 10 AqFIE- and AqEMF2-treated plants that exhibited increased branching. When quantified (Additional file 2E), the presence of higher order petiolules is significant at p < 0.05 for unvernalized lateral leaflets but not significant for the other stages/leaflet types. However, it is obvious that there is much more branching variation in silenced leaflets than in controls. In many cases, the margins of the laminae had additional lobing relative to control leaves (observed in 10% of treated plants) (Figure 1B-E, K) and, in a small number of cases, the central lobe of the terminal leaflet was severely reduced (seen in multiple leaves from 5 plants) (Figure 1D, M). Laminar area was highly variable with some leaflets appearing to have expanded area (~25 plants) (Figure 1F) while others seemed reduced (~8 plants) (Figure 1G, I, M). In two plants, ectopic finger-like projections were observed on the adaxial surface of laminae (Figure 1F), which was never observed in control leaflets.
Floral phenotypes
Wild type A. x coerulea flowers possess five organ types: sepals, petals, stamens, staminodia and carpels [39]. We have focused on the sepals and petals because they showed strong phenotypes in the silenced flowers. Wild type sepals are flat and ovate with an entire margin (Figure 2A-B). The petals are notable for the presence of a long hollow nectar spur, which forms near the attachment point (Figure 2A). This feature divides the organ into two regions, the proximal spur and the distal limb. Spurs in A. x coerulea are typically 5-6 cm in length and slightly curved. The limb region is relatively flat with a rounded, weakly lobed margin (Figure 2C). In 25 flowers from vernalized AqFIE- and AqEMF2-treated plants, we observed sepals that were narrower than wildtype organs and dramatically folded towards the adaxial surface (Figure 2D, F, L, P). In severely affected flowers, petals were narrowed and stunted (10 flowers, Figure 2D, G, Q) or exhibited sharply bent spurs (12 flowers, Figure 2H-I, K, M, Q). In two AqEMF2-silenced flowers, the sepals exhibited chimeric petal identity including ectopic spur formation (Figure 2M-N). Perhaps most surprising, many of the perianth organs had a definite yellow hue, with the petal limbs showing particularly intense yellow coloration (observed in at least one organ from 15 flowers) (Figure 2E, I-M, O). Such coloration was not observed in AqANS-silenced control flowers (Figure 2A-C). Examination of the AqFIE- and AqEMF2-silenced organs under high magnification reveals that yellow pigment is deposited in plastids (Additional file 3A), consistent with carotenoids rather than the vacuole-based aurones that are produced in some Aquilegia species [43, 44].
Assessment of AqFIE and AqEMF2 down-regulation
Due to limited RNA availability, we used standard RT-PCR to assess target gene down-regulation in leaves, sepals and petals compared to their expression in AqANS silenced control tissue. Even in AqANS silenced (control) tissue, AqFIE and AqEMF2 are expressed at low levels relative to the loading control AqIPP2. The experimental samples (F1-8 and E1-4) were selected to represent all of the observed phenotypes and were derived from separate plants. This analysis demonstrated that in the TRV2-AqFIE-AqANS treated plants, AqFIE was strongly down-regulated, being undetectable in a number of samples (Figure 3A and Figure 4). Likewise, AqEMF2 expression is reduced to undetectable levels in most tested AqEMF2-silenced samples (Figure 3A and Figure 4). We also tested for AqEMF2 in AqFIE-treated plants and vice versa, and found that AqEMF2 levels are often reduced in AqFIE-treated leaves, although the reciprocal is generally not true (Figure 3A). Furthermore, we tested the other PRC2-complex members, AqCLF and AqSWN, and found no consistent evidence of their down-regulation in either type of silenced tissue (Additional file 4A).
Assessment of candidate gene expression
We tested for ectopic expression of a wide panel of potential target genes, with a focus on the floral organ identity loci and type I KNOX homologs (Figure 3, Figure 5, and Additional file 4B). We again compared the expression of these genes to expression in AqANS-silenced control tissue. One of the two A. x coerulea the C class MADS box genes, AGAMOUS 1 (AqAG1) (see Additional file 1 for all gene identification numbers), is consistently up-regulated in silenced leaves and floral organs. The second AGAMOUS homologs, AGAMOUS2 (AqAG2) may also be slightly up-regulated in some of the leaves, although AqAG2 shows basal expression in control floral organs (Figures 3 and 5). The three A. x coerulea SEPALLATA paralogs (AqSEP1, AqSEP2, and AqSEP3) are somewhat difficult to assess because they are variably expressed in control leaves but AqSEP3 in particular seems to be up-regulated in AqEMF2-silenced leaves (Figure 3B). These genes were not assessed in floral organs because they are already broadly expressed in these tissues. A. x coerulea also has three paralogs of the B class MADS box gene, APETALA3 (AqAP3-1, AqAP3-2, and AqAP3-3). The petal-specific AqAP3-3 locus is highly up-regulated in AqEMF2-silenced sepals, which also showed chimeric sepal/petal identity in several cases (Figure 5A). Additionally two of the three AP3 paralogs are moderately up-regulated in PRC2 VIGS-treated leaves (Additional file 4B), but the expression of AqAP3-1 and AqAP3-2 is unaffected in mature sepals and petals (Figure 5A and B). We also looked at the expression of FUL-like 1 (AqFL1), which is normally expressed in early leaves, but no ectopic expression was detected (Figure 5 and Additional file 4B).
Next, we tested for up-regulation of three of the five A. x coerulea class I KNOX genes. No significant ectopic KNOX gene expression could be detected in the leaves. Weak expression of the SHOOTMERISTEMLESS 2 (AqSTM2) and KNOTTED (AqKN) homologs is detected in AqEMF2-silenced leaves (Figure 3C), however, we also occasionally detected comparable expression of these genes in control (AqANS-silenced) leaves, so it is difficult to ascribe significance to this expression. Given the lack of clear up-regulation in leaves and due to a limited amount of floral RNA, class I KNOX gene expression was not tested in the floral organs.
Although AqAG1 is consistently over-expressed in AqFIE and AqEMF2 silenced sepals and petals, we never saw any evidence of carpel identity in these organs. We therefore pooled cDNA from several AqANS- (control), AqFIE-, and AqEMF2-treated petals and sepals and used qRT-PCR to further examined the expression of AqAG1 and AqAG2 in these organs as well as in wild type carpels (Figure 5C and D). We found that while AqAG1 was clearly up-regulated in AqFIE and AqEMF2 silenced organs compared to the controls, AqAG1 expression was still much lower than in wild type carpels (about 0.05 to 0.2 fold). In contrast, AqAG2 expression was similar in control and PRC2 silenced tissue, but much lower than in wild type carpels.
Lastly, in an effort to investigate the carotenoid production, we identified the likely A. x coerulea homologs of a range of components of the carotenoid pathway in A. thaliana, including enzymes involved in production (PHYTOENE SYNTHASE (PSY) and CAROTENOID ISOMERASE (CRTISO)) and breakdown (CAROTENOID CLEAVAGE DIOXYGENASE 4 (CCD4) and 9-CIS-EPOXYCAROTENOID DIOXYGENASE 3 (NCED3)) of carotenoids [45]. A. x coerulea has two copies CCD4 (AqCCD4 and AqCCD4L) and two genes that are closely related to A. thaliana PSY (AqPSYL1 and AqPSYL2). Previous studies in A. thaliana have indicated that both CRTISO and NCED3 are positively epigenetically regulated by other SET domain containing proteins so we were particularly interested in the expression of these genes in AqFIE and AqEMF2 down-regulated tissue [46, 47]. We used RT-PCR to examine the expression of these six genes in AqANS- (control), AqFIE-, and AqEMF2-treated petals (Additional file 3B). Given the observed phenotypes, we might expect the expression of AqPSYL1, AqPSYL2, or AqCRTISO to be up-regulated or AqCCD4, AqCCD4L, or AqNCED3 to be down-regulated. Unfortunately, no clear patterns are apparent from these reactions.
Discussion
AqFIE and AqEMF2 VIGS-treated plants displayed a range of lateral organ phenotypes. Silenced leaves often had ruffled or curled lamina, additional lobing, and an increased frequency of higher order branching. The perianth organs were generally narrower than wild type organs. Sepals were also curled and petals were stunted or had bent spurs, while petal limbs also had a particularly intense yellow coloration seemingly due to an accumulation of carotenoid pigments in these cells. Many of the phenotypes we observed are similar to those seen in clf mutants and FIE cosuppressed A. thaliana, including curled leaves and narrow perianth organs [17, 29]. Unlike clf mutants and AG over-expressers in A. thaliana, dramatic transformation towards carpel identity was not observed in the AqFIE- and AqEMF2-treated sepals or petals. However, the level of AqAG1 expression in these organs was much less than what is seen in wild type Aquilegia carpels. Interestingly, the distinct folded morphology of the sepals may suggest slight transformation towards carpel identity as silenced leaves were folded towards the abaxial surface while the sepals were dramatically folded towards the adaxial surface, which is similar to the folding pattern of the Aquilegia carpel [48].
It is interesting to note that in AqFIE silenced leaves, AqEMF2 is also down-regulated. The reverse is not true in AqEMF2 silenced leaves, and AqEMF2 expression is not affected in AqFIE silenced floral organs. This result suggests that PRC2 may be directly or indirectly regulating AqEMF2 expression in A. x coerulea leaves, which could account for the generally more severe phenotypes observed in AqFIE silenced leaves compared to AqEMF2 silenced leaves. AqEMF2 is the only member of the complex that appears to be PRC2-regulated as the expression of AqCLF and AqSWN is not affected in PRC2 down-regulated leaves. In general, the potential for this type of cross-regulation is relatively unexplored in A. thaliana and, therefore, bears further study.
In our analysis of candidate target genes, we found that AqAG1 is often ectopically expressed in PRC2 down-regulated tissue. AqAP3-3 and AqSEP3 are also up-regulated in some organs, but expression of the class I KNOX genes and several candidate genes involved in carotenoid production or degradation seem largely unaffected. Mutations in AG and SEP3 are known to suppress the curled leaf phenotype in clf mutant plants while over-expression of these MADS box genes, which themselves function together in a complex [49], is thought to be the cause of the curled leaf phenotype [26]. It is, therefore, possible that over-expression of AqAG1 and AqSEP3 is similarly responsible for many of the observed phenotypes in AqFIE and AqEMF2 silenced leaves. These findings lead us to conclude that PRC2-based regulation of AG and SEP3 homologs is deeply conserved in eudicots. It has recently been shown that several chromatin remodeling factors associate with MADS complexes and one model is that an important function of MADS domain complexes may be to recruit chromatin remodeling complexes to target loci in order to alter transcription of these genes and direct organ development [50, 51]. For example, RELATIVE OF EARLY FLOWERING 6 (REF6) was enriched in protein complexes that were isolated via immunoprecipitation using tagged ABCE class MADS box proteins [50]. REF6 has been shown to specifically demethylate H3K27me3, the histone modification deposited by PRC2 [52]. Activation of SEP3 by APETALA1 (AP1) in A. thaliana results in the reduction of H3K27me3 at the SEP3 promoter, suggesting that AP1 may recruit REF6 to the SEP3 promoter in order to help induce SEP3 gene function [50]. Our data suggests that this key dependency on epigenetic regulation for the switch from vegetative to floral development may be important outside of A. thaliana. There are some complications, however. Of the two A. x coerulea AG homologs, only one, AqAG1, is strongly regulated by PRC2. Perhaps consistent with this observation, sequencing of the Aquilegia genome (http://www.phytozome.net/search.php?method=Org_Acoerulea) reveals that AqAG1 does contain the large regulatory second intron that is common to AG homologs [53, 54] while AqAG2’s second intron is much smaller. These results suggest that PRC2 regulation can be directed in a paralog-specific fashion and may even play some role in the distinct expression patterns observed among these gene copies [39].
The class I KNOX genes are directly or indirectly regulated by PRC2 in both A. thaliana and Physcomitrella, however, we detected little or no increase in KNOX gene expression in our AqFIE and AqEMF2 silenced leaves. This is somewhat surprising because of the higher order branching that we observed in silenced leaves, including several of the tested RNA samples. The class I KNOX genes are thought to play a role in compound leaf development in a number of species. In many, but not all, compound leafed taxa where KNOX gene expression has been studied, including Aquilegia, it has been shown that the genes are expressed in the shoot apical meristem and down-regulated in incipient leaf primordia (P0), but subsequently turned back on in early leaf primordia [28]. Down-regulation of class I KNOX genes in the leaves of models such as tomato or Cardamine causes reduced branching while over-expression leads to increased branching [55, 56], suggesting that KNOX genes act to maintain indeterminacy in compound leaves and promote leaflet initiation.
There are several possible explanations for why we did not observe significant ectopic KNOX gene expression in our VIGS-treated leaves. First, it is possible the KNOX genes were ectopically expressed early in leaf development when the higher order branching actually developed, but were later down-regulated by redundant mechanisms, such as ASYMMETRIC LEAVES 1 (AS1)-mediated repression [57, 58]. In A. thaliana AS1 mediated silencing of some of the KNOX genes has been shown to require the PRC2 complex and it is thought that AS1 and AS2 directly recruit the PRC2 complex to KNOX loci [59]. However, it is important to remember that in other taxa with compound leaves, the KNOX and AS1 homologs have lost their mutually exclusive regulatory interactions and are expressed together at later stages [32]. This may suggest that the AS1-dependent epigenetic silencing of KNOX genes that has been described in several simple-leafed models [57, 58] does not hold for plants with compound leaves. Along these lines, it is also possible that the increased branching phenotypes are due to other factors, such as accelerated phase change or novel genetic mechanisms regulating leaflet branching in Aquilegia. For instance, a recent functional study of the gene AqFL1 in A. x coerulea revealed that it promotes proper leaf margin development, a unique finding for homologs of this gene lineage [40]. This raises the possibility that factors other than the KNOX genes contribute to compound leaf branching in Aquilegia.
In addition to the conserved role in regulating AG, AP3, and SEP3, A. x coerulea PRC2 may target novel pathways, including those regulating carotenoid production or degradation. In A. thaliana patches of yellow anther-like tissue are observed on clf mutant petals [17]. However, the yellow pigmentation we observed is due to the accumulation of carotenoids in the plastids rather than to a partial homeotic transformation. While genes in the carotenoid pathway are not known to be suppressed by PRC2, some loci are positively epigenetically regulated in A. thaliana. Previous studies have shown that a major enzyme in the carotenoid biosynthesis pathway, CRTISO, requires the chromatin modifying enzyme SET DOMAIN GROUP 8 (SDG8) to maintain its expression [46]. NCED3, an enzyme that cleaves some types of carotenoids as a part of abscisic acid (ABA) synthesis, is similarly epigenetically regulated by the A. thaliana trithorax homolog ATX1 [47]. While none of the genes we tested were consistently up- or down-regulated in AqFIE and AqEMF2 silenced petals, carotenoid production is very genetically complex and we were unable to test all of the candidate loci [60]. Thus, it seems likely that PRC2 regulates an as yet unidentified enzyme in this pathway in A. x coerulea.
Conclusions
-
A critical role for PRC2 in maintaining the repression of AG, SEP3, and possibly AP3 appears to be conserved across eudicots. This conservation underscores the importance of chromatin remodeling factors in regulating the floral transition and the proper localization of floral organ identity.
-
Class I KNOX genes are not ectopically expressed in PRC2 down-regulated tissue in A. x coerulea, possibly due to a regulatory shift associated with the evolution of compound leaves.
-
A. x coerulea PRC2 plays a significant role in regulating the carotenoid pathway in floral organs, which has not been observed in other taxa.
-
This study, the first to examine PRC2 function in angiosperms outside A. thaliana or the grasses, highlights how little we still know about the general conservation or targeting mechanisms underlying PRC2 function in major developmental transitions.
Abbreviations
- AG:
-
AGAMOUS
- ANS:
-
Anthocyanin synthase
- AP1:
-
APETALA1
- AP3:
-
APETALA3
- Aq:
-
Aquilegia
- BP:
-
Brevipedicellus
- bp:
-
Base pair(s)
- CCD:
-
CAROTENOID CLEAVAGE DIOXYGENASE
- cDNA:
-
DNA complementary to RNA
- CLF:
-
CURLY LEAF
- cm:
-
Centimeter
- CRTISO:
-
CAROTENOID ISOMERASE
- DNA:
-
Deoxyribonucleic acid
- DNase:
-
Deoxyribonuclease
- E(z):
-
Enhancer of zeste
- EMF2:
-
EMBRYONIC FLOWER 2
- ESC:
-
Extra sex combs
- Eudicots:
-
Eudicotyledonous
- FIE:
-
FERTILIZATION INDEPENDENT ENDOSPERM
- FIS:
-
FERTILIZATION INDEPENDENT SEED
- FLC:
-
FLOWERING LOCUS c
- FL1:
-
FRUITFUL-like 1
- H3K27:
-
Histone H3 Lysine 27
- HOX:
-
Homeobox
- IPP2:
-
Isopentyl pyrophosphatedimethylallyl pyrophosphate isomerase:
- KN:
-
KNOTTED
- KNAT2:
-
KNOTTED-like from Arabidopsis thaliana 2
- KNOX:
-
knotted1 homeobox gene
- MADS:
-
MCM1, agamous, deficiens, SRF
- MEA:
-
Medea
- MKN:
-
Moss knotted1-like
- MSI1:
-
Multi copy suppressor of IRA 1
- n:
-
Chromosome number
- NCED:
-
9-CIS-epoxycarotenoid dioxygenase
- oligo:
-
Oligodeoxyribonucleotide
- PcG:
-
Polycomb group
- Pp:
-
Physcomitrella patens
- PCR:
-
Polymerase chain reaction
- PRC1:
-
Polycomb repressive complex1
- PRC2:
-
Polycomb repressive complex2
- PSY:
-
Phytoene Synthase
- qRT-PCR:
-
Quantitative real time polymerase chain reaction
- REF6:
-
Relative of early flowering 6
- RNA:
-
Ribonucleic acid
- RT-PCR:
-
Reverse transcriptase PCR
- SEP:
-
SEPALLATA
- STM:
-
SHOOTMERISTEMLESS
- Su(z)12:
-
Suppressor of zeste12
- SWN:
-
SWINGER
- TRV:
-
Tobacco rattle virus
- VIGS:
-
Virus-induced gene silencing.
References
Holliday R: Epigenetics: an overview. Dev Gen. 1994, 15 (6): 453-457. 10.1002/dvg.1020150602.
Russo VEA, Martienssen R, Riggsm AD: Epigenetic Mechanisms of Gene Regulation. Woodbury, NY, USA: Cold Spring Harbor Laboratory Press: 1996.
Feil R: Epigenetics, an emerging discipline with broad implications. C R Biol. 2008, 331 (11): 837-843. 10.1016/j.crvi.2008.07.027.
Lewis EB: A gene complex controlling segmentation in Drosophila. Nature. 1978, 276: 565-570. 10.1038/276565a0.
Hennig L, Derkacheva M: Diversity of Polycomb group complexes in plants: same rules, different players?. Trends Genet. 2009, 25 (9): 414-423. 10.1016/j.tig.2009.07.002.
Sawarkar R, Paro R: Interpretation of developmental signaling at chromatin: The polycomb perspective. Dev Cell. 2010, 19 (5): 651-661. 10.1016/j.devcel.2010.10.012.
Kohler C, Hennig L: Regulation of cell identity by plant Polycomb and trithorax group proteins. Curr Opin Genet Dev. 2010, 20 (5): 541-547. 10.1016/j.gde.2010.04.015.
Schubert D, Primavesi L, Bishopp A, Roberts G, Doonan J, Jenuwein T, Goodrich J: Silencing by plant Polycomb-group genes requires dispersed trimethylation of histone H3 at lysine 27. Embo Journal. 2006, 25 (19): 4638-4649. 10.1038/sj.emboj.7601311.
Nekrasov M, Wild B, Muller J: Nucleosome binding and histone methyltransferase activity of Drosophila PRC2. EMBO Rep. 2005, 6 (4): 348-353. 10.1038/sj.embor.7400376.
Pien S, Grossniklaus U: Polycomb group and trithorax group proteins in Arabidopsis. Biochimica Et Biophysica Acta-Gene Structure and Expression. 2007, 1769 (5–6): 375-382.
Spillane C, Schmid KJ, Laoueille-Duprat S, Pien S, Escobar-Restrepo JM, Baroux C, Gagliardini V, Page DR, Wolfe KH, Grossniklaus U: Positive darwinian selection at the imprinted MEDEA locus in plants. Nature. 2007, 448 (7151): 349-U348. 10.1038/nature05984.
Luo M, Platten D, Chaudhury A, Peacock WJ, Dennis ES: Expression, imprinting, and evolution of rice homologs of the Polycomb group genes. Mol Plant. 2009, 2 (4): 711-723. 10.1093/mp/ssp036.
Whitcomb SJ, Basu A, Allis CD, Bernstein E: Polycomb Group proteins: an evolutionary perspective. Trends Genet. 2007, 23: 494-502. 10.1016/j.tig.2007.08.006.
Kohler C, Hennig L, Spillane C, Pien S, Gruissem W, Grossniklaus U: The Polycomb-group protein MEDEA regulates seed development by controlling expression of the MADS-box gene PHERES1. Genes Dev. 2003, 17 (12): 1540-1553. 10.1101/gad.257403.
Yoshida N, Yanai Y, Chen L, Kato Y, Hiratsuka J, Miwa T, Sung ZR, Takahashi S: EMBRYONIC FLOWER2, a novel polycomb group protein homolog, mediates shoot development and flowering in Arabidopsis. Plant Cell. 2001, 13 (11): 2471-2481.
Gendall AR, Levy YY, Wilson A, Dean C: The VERNALIZATION2 gene mediates the epigenetic regulation of vernalization in Arabidopsis. Cell. 2001, 107: 525-535. 10.1016/S0092-8674(01)00573-6.
Goodrich J, Puangsomlee P, Martin M, Long D, Meyerowitz EM, Coupland G: A polycomb-group gene regulates homeotic gene expression in Arabidopsis. Nature. 1997, 386 (6620): 44-51. 10.1038/386044a0.
Oliver SN, Finnegan EJ, Dennis ES, Peacock WJ, Trevaskis B: Vernalization-induced flowering in cereals is associated with changes in histone methylation at the VERNALIZATION1 gene. Proc Natl Acad Sci USA. 2009, 106 (20): 8386-8391. 10.1073/pnas.0903566106.
Rodrigues J, Luo M, Berger F, Koltunow A: Polycomb group gene function in sexual and asexual seed development in angiosperms. Sex Plant Reprod. 2010, 23 (2): 123-133. 10.1007/s00497-009-0131-2.
Okano Y, Aono N, Hiwatashi Y, Murata T, Nishiyama T, Ishikawa T, Kubo M, Hasebe M: A Polycomb Repressive Complex 2 gene regulates apogamy and gives evolutionary insights into early land plant evolution. Proc Natl Acad Sci USA. 2009, 106 (38): 16321-16326. 10.1073/pnas.0906997106.
Mosquna A, Katz A, Decker EL, Rensing SA, Reski R, Ohad N: Regulation of stem cell maintenance by the Polycomb protein FIE has been conserved during land plant evolution. Development. 2009, 136 (14): 2433-2444. 10.1242/dev.035048.
Bowman J, Smyth DR, Meyerowitz E: The ABC model of flower development: then and now. Development. 2012, 139 (22): 4095-4098. 10.1242/dev.083972.
Bowman JL, Drews GN, Meyerowitz EM: Expression of the Arabidopsis floral homeotic gene agamous is restricted to specific cell types late in flower development. Plant Cell. 1991, 3: 749-758.
Bowman JL, Smyth DR, Meyerowitz EM: Genes directing flower development in Arabidopsis. Plant Cell. 1989, 1: 37-52.
Foronda D, de Navas LF, Garaulet DL, Sanchez-Herrero E: Function and specificity of Hox genes. Int J Dev Biol. 2009, 53 (8–10): 1409-1419.
Lopez-Vernaza M, Yang SX, Muller R, Thorpe F, de Leau E, Goodrich J: SEPALLATA3, FT and FLC genes as targets of the Polycomb group gene CURLY LEAF. PLoS ONE. 2012, 7 (2): e30715. 10.1371/journal.pone.0030715.
Wagner D: Chromatin regulation of plant development. Curr Opin Plant Biol. 2003, 6 (1): 20-28. 10.1016/S1369526602000079.
Bharathan G, Goliber TE, Moore C, Kessler S, Pham T, Sinha NR: Homologies in leaf form inferred from KNOXI gene expression during development. Science. 2002, 296 (5574): 1858-1860. 10.1126/science.1070343.
Katz A, Oliva M, Mosquna A, Hakim O, Ohad N: FIE and CURLY LEAF polycomb proteins interact in the regulation of homeobox gene expression during sporophyte development. Plant Journal. 2004, 37 (5): 707-719. 10.1111/j.1365-313X.2003.01996.x.
Singer SD, Ashton NW: Revelation of ancestral roles of KNOX genes by a functional analysis of Physcomitrella homologues. Plant Cell Reports. 2007, 26: 2039-2054. 10.1007/s00299-007-0409-5.
Maizel A, Busch MA, Tanahashi T, Perkovic J, Kato M, Hasebe M, Weigel D: The floral regulator LEAFY evolves by substitutions in the DNA binding domain. Science. 2005, 308 (5719): 260-263. 10.1126/science.1108229.
Kim M, McCormick S, Timmermans M, Sinha N: The expression domain of PHANTASTICA determines leaflet placement in compound leaves. Nature. 2003, 424: 438-443. 10.1038/nature01820.
Hodges SA, Kramer EM: Columbines. Curr Biol. 2007, 17 (23): R992-R994. 10.1016/j.cub.2007.09.034.
Kramer EM, Hodges SA: Aquilegia as a model system for the evolution and ecology of petals. Philos Trans R Soc Lond B Biol Sci. 2010, 365: 477-490. 10.1098/rstb.2009.0230.
Kramer EM: Aquilegia: A new model for plant development, ecology, and evolution. Ann Rev Plant Biol. 2009, 60: 261-277. 10.1146/annurev.arplant.043008.092051.
Gould B, Kramer EM: Virus-induced gene silencing as a tool for functional analyses in the emerging model plant Aquilegia (columbine, Ranunculaceae). Plant Methods. 2007, 3: 6. 10.1186/1746-4811-3-6.
Sharma B, Kramer EM: Sub- and neofunctionalization of APETALA3 paralogs have contributed to the evolution of novel floral organ identity in Aquilegia (columbine, Ranunculaceae). New Phytol. 2013, 197: 949-957. 10.1111/nph.12078.
Sharma B, Guo C, Kong H, Kramer EM: Petal-specific subfunctionalization of an APETALA3 paralog in the Ranunculales and its implications for petal evolution. New Phytol. 2011, 190: 870-883.
Kramer EM, Holappa L, Gould B, Jaramillo MA, Setnikov D, Santiago P: Elaboration of B gene function to include the identity of novel floral organs in the lower eudicot Aquilegia (Ranunculaceae). Plant Cell. 2007, 19 (3): 750-766. 10.1105/tpc.107.050385.
Pabón-Mora N, Sharma B, Holappa L, Kramer EM, Litt A: The Aquilegia FRUITFULL-like genes play key roles in leaf morphogenesis and inflorescence development. Plant J. 2013, 74 (2): 197-212. 10.1111/tpj.12113.
Gleason E, Kramer EM: Characterization of Aquilegia Polycomb Repressive Complex 2 homologs reveals absence of imprinting. Gene. 2012
Ballerini ES, Kramer EM: The control of flowering time in the lower eudicot Aquilegia formosa. EvoDevo. 2011, 2: 4. 10.1186/2041-9139-2-4.
Vishnevetsky M, Ovadis M, Vainstein A: Carotenoid sequestration in plants: the role of carotenoid-associated proteins. Trends Plant Sci. 1999, 4 (6): 232-235. 10.1016/S1360-1385(99)01414-4.
Ono E, Hatayama M, Isono Y, Sato T, Watanabe R, Yonekura-Sakakibara K, Fukuchi-Mizutani M, Tanaka Y, Kusumi T, Nishino T, et al: Localization of a flavonoid biosynthetic polyphenol oxidase in vacuoles. Plant J. 2006, 45 (2): 133-143. 10.1111/j.1365-313X.2005.02625.x.
Cazzonelli CI: Carotenoids in nature: insights from plants and beyond. Funct Plant Biol. 2011, 3 (1): 833-847.
Cazzonelli CI, Roberts AC, Carmody ME, Pogson BJ: Transcriptional control of SET domain group 8 and carotenoid isomerase during Arabidopsis development. Mol Plant. 2010, 3 (1): 174-191. 10.1093/mp/ssp092.
Ding Y, Avramova Z, Fromm M: The Arabidopsis trithorax-like factor ATX1 functions in dehydration stress responses via ABA-dependent and ABA-independent pathways. Plant J. 2011, 66 (5): 735-744. 10.1111/j.1365-313X.2011.04534.x.
Tucker SC, Hodges SA: Floral ontogeny of Aquilegia, Semiaquilegia, and Isopyrum (Ranunculaceae). Int J Plant Sci. 2005, 166 (4): 557-574. 10.1086/429848.
Honma T, Goto K: Complexes of MADS-box proteins are sufficient to convert leaves into floral organs. Nature. 2001, 409 (6819): 525-529. 10.1038/35054083.
Smaczniak C, Immink RGH, Angenent GC, Kaufmann K: Developmental and evolutionary diversity of plant MADS-domain factors: insights from recent studies. Development. 2012, 139 (17): 3081-3098. 10.1242/dev.074674.
Immink RGH, Kaufmann K, Angenent GC: The ‘ABC’ of MADS domain protein behaviour and interactions. Semin Cell Dev Biol. 2010, 21 (1): 87-93. 10.1016/j.semcdb.2009.10.004.
Lu FL, Cui X, Zhang SB, Jenuwein T, Cao XF: Arabidopsis REF6 is a histone H3 lysine 27 demethylase. Nat Genet. 2011, 43 (7): 715-719. 10.1038/ng.854.
Deyholos MK, Sieburth LE: Separable whorl-specific expression and negative regulation by enhancer elements within the AGAMOUS second intron. Plant Cell. 2000, 12 (10): 1799-1810.
Hong RL, Hamaguchi L, Busch M, Weigel D: Regulatory elements of the floral homeotic gene AGAMOUS identified by phylogenetic footprinting and shadowing. Plant Cell. 2003, 15: 1296-1309. 10.1105/tpc.009548.
Hareven D, Gutfinger T, Parnis A, Eshed Y, Lifschitz E: The making of a compound leaf: genetic manipulation of leaf architecture in tomato. Cell. 1996, 84 (5): 735-744. 10.1016/S0092-8674(00)81051-X.
Hay A, Barkoulas M, Tsiantis M: ASYMMETRIC LEAVES1 and auxin activities converge to repress BREVIPEDICELLUS expression and promote leaf development in Arabidopsis. Development. 2006, 133 (20): 3955-3961. 10.1242/dev.02545.
Guo M, Thomas J, Collins G, Timmermans MCP: Direct repression of KNOX loci by the ASYMMETRIC LEAVES1 complex of Arabidopsis. Plant Cell. 2008, 20 (1): 48-58. 10.1105/tpc.107.056127.
Phelps-Durr TL, Thomas J, Vahab P, Timmermans MCP: Maize rough sheath2 and its Arabidopsis orthologue ASYMMETRIC LEAVES1 interact with HIRA, a predicted histone chaperone, to maintain knox gene silencing and determinacy during organogenesis. Plant Cell. 2005, 17 (11): 2886-2898. 10.1105/tpc.105.035477.
Lodha M, Marco CF, Timmermans M: The ASYMMETRIC LEAVES complex maintains repression of KNOX homeobox genes via direct recruitment of Polycob-repressive complex2. Genes Dev. 2013, 27: 596-601. 10.1101/gad.211425.112.
Lu S, Li L: Carotenoid metabolism: biosynthesis, regulation and beyond. J Integr Plant Biol. 2008, 50 (7): 778-785. 10.1111/j.1744-7909.2008.00708.x.
Acknowledgements
The authors would like to thank members of the Kramer lab and 2 anonymous reviewers for critical comments on the manuscript.
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Authors’ contributions
EJG helped to conceive of the study, carried out the experiments, and drafted the manuscript. EMK helped to conceive of the study, supervised the experiments, and helped draft the manuscript. Both authors read and approved the final manuscript.
Electronic supplementary material
12870_2013_1383_MOESM2_ESM.jpeg
Additional file 2: Heteroblasty in A. x coerulea leaves. A. Unvernalized leaf with 3 major lobes in the lateral leaflets. B. Unvernalized leaf with 2 major lobes in the lateral leaflets. C. Vernalized leaf with higher order petiolules where the central lobe of each leaflet is a separate leaflet borne on a petiolule (asterisks). D. Vernalized leaf with 2 major lobes in the lateral leaflets. These leaves are more deeply lobed than similar unveralization leaves. E. Average number of higher order petiolules within medial or lateral leaflets in wild type unvernalized, AqFIE silenced unvernalized, wild type vernalized, and AqFIE silenced leaves with standard deviations. Both unvernalized and vernalized AqFIE silenced lateral leaflets had on average more higher order petiolules than the wild type. Unvernalized AqFIE silenced lateral leaflets also had a slightly higher average number of higher order petiolules compared to wild type, but vernalized AqFIE silenced leaves had a slightly lower number of petiolules per medial leaflet. When quantified, this increase is significant (*) at p < 0.05 for unvernalized lateral leaflets but not significant for the other stages/leaflet types.3 (JPEG 335 KB)
12870_2013_1383_MOESM3_ESM.jpeg
Additional file 3: The PRC2 regulates carotenoid production in A. coerulea petals. A. High magnification views of epidermal cells in A. x coerulea petal limbs. From left to right: Anthocyanin of untreated petal limb (anthocyanin is deposited in the vacuole, resulting in a very even distribution of color), almost complete lack of color in AqANS-silenced petal limb, and punctate pattern of carotenoid deposition in plastids of AqEMF2-silenced petal limb. B. Expression of several A. x coerulea homologs of genes important in carotenoid production (CRTISO and PSY) and degradation (CCD4 and NCED3) in AqANS-silenced control petals (C1-C4) and AqFIE (F1-F6) and AqEMF2 (E1 and E2) treated petals. Petals with strong yellow pigment are highlighted in dark yellow (F1, F5, and E1) and petals with pale yellow pigment are highlighted in light yellow (F2-F4). The expression of these genes is not consistently affected in the AqFIE and AqEMF2 silenced petal samples. It is possible that other genes in the carotenoid pathway are being misexpressed. Scale bars: 10 μm. (JPEG 534 KB)
12870_2013_1383_MOESM4_ESM.jpeg
Additional file 4: Additional candidate gene expression in PRC2 VIGS-treated leaves. A. Expression of AqCLF and AqSWN in AqFIE- and AqEMF2-treated leaves. Although AqEMF2 appears to be down-regulated in some AqFIE-silenced leaves, the expression of AqCLF and AqSWN in these leaves is not affected. B. Expression of AqAG1, AqFL1, AqAP3-1, AqAP3-2, and AqAP3-3 in pooled AqANS silenced control leaves (C) and AqFIE (F) and AqEMF2 (E) silenced leaves. AqAP3-1 AqAP3-2 and AqAP3-3 is moderately up-regulated in both AqFIE and AqEMF2 silenced tissue while AgFL1 expression is unaffected. (JPEG 206 KB)
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Gleason, E.J., Kramer, E.M. Conserved roles for Polycomb Repressive Complex 2 in the regulation of lateral organ development in Aquilegia x coerulea ‘Origami’. BMC Plant Biol 13, 185 (2013). https://doi.org/10.1186/1471-2229-13-185
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DOI: https://doi.org/10.1186/1471-2229-13-185