Journal of Experimental Botany, Vol. 65, No. 8, pp. 2137–2146, 2014 doi:10.1093/jxb/eru073  Advance Access publication 18 March, 2014 This paper is available online free of all access charges (see http://jxb.oxfordjournals.org/open_access.html for further details)

Research Paper

A dark–light transition triggers expression of the floral promoter CrFTL1 and downregulates CONSTANS-like genes in a short-day plant Chenopodium rubrum Jana Drabešová, David Cháb, Jan Kolář, Kateřina Haškovcová and Helena Štorchová* Institute of Experimental Botany, Academy of Sciences of the Czech Republic, v.v.i. Rozvojová 223, 165 02 Prague 6, Lysolaje, Czech Republic * To whom correspondence should be addressed. E-mail: [email protected] Received 20 December 2013; Revised 30 January 2014; Accepted 31 January 2014

Abstract The proper timing of flowering is essential for the adaptation of plant species to their ever-changing environments. The central position in a complex regulatory network is occupied by the protein FT, which acts as a florigen. We found that light, following a permissive period of darkness, was essential to induce the floral promoter CrFTL1 and to initiate flowering in seedlings of the short-day plant Chenopodium rubrum L. We also identified two novel CONSTANS-like genes in C.  rubrum and observed their rhythmic diurnal and circadian expressions. Strong rhythmicity of expression suggested that the two genes might have been involved in the regulation of photoperiod-dependent processes, despite their inability to complement co mutation in A. thaliana. The CrCOL1 and CrCOL2 genes were downregulated by dark–light transition, regardless of the length of a preceding dark period. The same treatment activated the floral promoter CrFTL1. Light therefore affected CrCOL and CrFTL1 in an opposite manner. Both CrCOL genes and CrFTL1 displayed expression patterns unique among short-day plants. Chenopodium rubrum, the subject of classical physiological studies in the past, is emerging as a useful model for the investigation of flowering at the molecular level. Key words:  Chenopodium rubrum, CONSTANS-like, flowering, FLOWERING LOCUS T-like, gene expression, light sensitivity, short-day plant.

Introduction Daylength, or photoperiod, is a key environmental factor responsible for flower induction particularly in plants growing in higher latitudes. The central position in a complex network regulating flowering in Arabidopsis thaliana is occupied by the protein FLOWERING LOCUS T (FT; reviewed by Amasino, 2010; Pin and Nilsson, 2012), which fulfils a role of florigen, a factor long predicted to be responsible for flower induction (Corbesier et  al., 2007; Zeevaart, 2008). FT gene expression is regulated by various environmental cues including daylength (Jaeger and Wigge, 2007). Information about daylength or photoperiod is mediated by the transcription factor CO (CONSTANS) (Putterill et  al., 1995). The CO

protein is produced under long days in A. thaliana and activates FT (Suarez-Lopez et al., 2001), whereas it is degraded under short days (Valverde et al., 2004; Jang et al., 2008). The CO protein contains two conserved B-box zinc finger domains at its N-terminus, which may be responsible for protein–protein interactions (Ben-Naim et  al., 2006; Wenkel et  al., 2006). The CCT (CONSTANS, CONSTANS-like, TIMING OF CAB EXPRESSION1) domain is located at the C-terminus and has been implicated in DNA binding (Robson et al., 2001). A large family of 17 CO-like (COL) genes exists in A. thaliana, divided into three subfamilies or groups according to gene structure (Griffiths et al., 2003). Group I contains

© The Author 2014. Published by Oxford University Press on behalf of the Society for Experimental Biology. This is an Open Access article distributed under the terms of the Creative Commons Attribution License (http://creativecommons.org/licenses/by/3.0/), which permits unrestricted reuse, distribution, and reproduction in any medium, provided the original work is properly cited.

2138 | Drabešová et al. the genes with two B-boxes, including CO. Only a minority of the AtCOL genes is involved in the control of flowering in A. thaliana. Besides CO, AtCOL5 was shown to induce flowering (Hassidim et al., 2009). In contrast, AtCOL3 (Datta et al., 2006) and AtCOL9 (Cheng and Wang, 2005) inhibit flowering. Some COL genes appear to be involved in the regulation of plant development other than flowering, e.g. AtCOL3 directs lateral root formation and shoot branching (Datta et al., 2006). A CO/FT regulatory module is conserved among shortday plants, which flower when night is longer than a critical period. FT and CO homologues were identified in rice and termed Hd3a and Hd1, respectively (Yano et al., 2001). Hd3a, like FT, activates flowering under permissive conditions, i.e. short-day in rice. Hd1, a CO homologue, fulfills dual roles: it downregulates Hd3a expression under long days but promotes it under short days (Yano et al., 2000). The mode of action of Hd1 is therefore partially distinct from CO in A. thaliana. A  CONSTANS homologue participates in the regulation of development, specifically in the induction of bud dormancy in trees (Bohlenius et al., 2006), grapevine (Almada et al., 2009) or in tuberization in potato (Gonzalez-Schain et al., 2012). To build a complex regulatory network managing the control of flowering, plants seem to utilize similar elements: genes with a conserved structure. However, their function or position in signalling pathways may be changed according to the specific demands of particular species. A recent example was provided by Harig et al. (2012), who found that three of four tobacco FT homologues functioned like floral inhibitors, which was atypical for FT-like proteins. A similar case was described by Pin et al. (2010) in sugar beet. Two FT homologues shared similar sequences, but displayed antagonistic functions. Whereas BvFT2 acted as a floral promoter, BvFT1 repressed flowering. Chenopodium rubrum belongs to the same family, Amaranthaceae, as sugar beet and is a short-day plant that can be induced to flower at a juvenile stage. Owing to this convenient manipulation, it became the subject of classical physiological studies of flowering (Cumming, 1967; Seidlová and Krekule, 1973). In the present study, we confirm CrFTL1’s function as a floral inducer (Cháb et al., 2008) by the complementation assay in A.  thaliana. We demonstrate its upregulation by a dark– light transition regardless of circadian phase, a mode of light response very unusual among short-day plants (Kojima et al., 2002; Hayama et al., 2007). We also describe two novel COL genes, termed CrCOL1 and CrCOL2. Their strong diurnal and circadian rhythmic expression suggest their possible role in the regulation of plant development, despite their failure to complement an A. thaliana co mutation. Both genes were downregulated by a dark–light transition at the same time when CrFTL1 was upregulated. Therefore, COL and CrFTL1 showed complementary expression levels.

Materials and methods Plant material Seedlings of C.  rubrum ecotype 374 (Cumming, 1967) were cultivated in growth chambers at 20  °C with constant light or under various photoperiodic treatments essentially as described by Cháb

et  al. (2008). Sampling during darkness was performed under a dim green light. To estimate flower development, 15 individuals from each experimental treatment were left intact and grown under constant light until the age of 14  days. Morphological changes at the shoot apex associated with flowering were observed under a stereomicroscope. Seeds of A. thaliana were stratified for 3 days at 4 °C. Seeds were then sown onto Jiffy-7 pellets (41 mm diameter, manufactured by Jiffy Products International AS (Norway)). Five seeds were sown onto each pellet. Seedlings were later thinned to two average-sized individuals at the age of 10 days and then to a single plant in each pellet at the age of 17  days. Plants were cultivated in Microclima Arabidopsis Cabinet MCA1600E-6TL (Snijders Scientific, Netherlands) at 20 °C and 60% relative humidity. Light was provided by white fluorescent tubes. Daylength was 16 h of light (130 μmol m–2 s–1) daily. Cloning of CrCOL genes Degenerate primers designed by program CODEHOP (Rose et al., 1998; Supplementary Table S1, available at JXB online) were targeted to conserved regions of the first and second exons, respectively, of the CONSTANS gene. Genomic DNA from C. rubrum was amplified with AmpliTaq Gold DNA Polymerase (Applied Biosystems, CA, USA) under the following conditions: 9 min initial denaturation at 94 °C; 36 cycles 30 s at 94 °C, 40 s at 56 °C and 1.5 min at 72 °C; final extension 10 min at 72  °C. Resulting 1.5 kb PCR fragments were cloned in pGEM-T Easy vector (Promega, WI, USA) and sequenced. Based on this sequence, specific primers CrCON138for and CrCON1523rev (Supplementary Table S1 available at JXB online) were developed. These were used to amplify cDNA from C. rubrum seedlings using Taq polymerase (Promega, WI, USA) and conditions: 2 min at 94 °C; 35 cycles 40 s at 93 °C, 45 s at 58 °C and 2 min at 72°C; final extension 5 min at 72  °C. To obtain complete sequences of CrCOL cDNA, a modified RACE procedure (Cháb et  al., 2008) was employed. Briefly, cDNA was prepared from the mixture of RNA extracted from C. rubrum seedlings sampled at various times of day using SMART technology (Clontech, CA, USA). This was then cloned into pGEM-T Easy vector (Promega, WI, USA) and amplified with a combination of gene-specific and vectortargeted primers (Supplementary Table S1 available at JXB online) using PCR with Phusion high-fidelity DNA polymerase (Thermo Fisher Scientific, Finland): 30 s at 98 °C; 35 cycles for 10 s at 98 °C, 20 s at 58 °C and 45 s at 72 °C; final extension 5 min at 72 °C. As Phusion polymerase generates amplicons with blunt ends, A-tailing (Knoche and Kephart, 1999) with Taq polymerase (Promega, WI, USA) was performed to generate PCR fragments suitable for A/T cloning into the pGEM-T Easy vector. The introns were amplified with the specifically designed primers directed to adjacent exons (Supplementary Table S1 available at JXB online) and sequenced. Raw sequences were edited, stored and analysed using Vector NTI Suite 9. The newly obtained sequences were deposited in GenBank under the acccession numbers EU395770 and EU395771. Transformation of A. thaliana Full-length cDNAs of CrFTL1, CrFTL2, CrCOL1 and CrCOL2s were cloned into pGEM-T Easy vectors using the primers targeted to UTRs (Supplementary Table S1 available at JXB online), and confirmed by sequencing. The vector carrying CrFTL2 was digested with EcoRI (MBI Fermentas, Lithuania). This restriction fragment was inserted into the EcoRI site of pRT101 (Töpfer et  al., 1987) between the polyA signal and 35S promoter. The vectors bearing other genes were cut with NotI (MBI Fermentas, Lithuania), the resulting fragments were filled by Klenow polymerase fragment (MBI Fermentas, Lithuania), and subsequently inserted to bluntended pRT101. The gene casette was transferred from pRT101 to pGreenII0179 (Hellens et al., 2000) using HindIII site. To generate transgenic plants, the vector with a casette was transformed into

Flowering in Chenopodium rubrum | 2139 Agrobacterium tumefaciens strain GV3101 carrying a helper plasmid pSoup. Arabidopsis thaliana wild type or mutants were transformed by floral dipping (Clough and Bent, 1998). T1 progeny was selected on a medium with hygromycin. Homozygous T2 plants were identified on the basis of the screening of their progeny on the medium with hygromycin. The presence and expression of transgenes were confirmed by PCR or qRT PCR, respectively, using EF1-α as a reference in A.  thaliana (Landa et  al., 2010). The average transcript levels of the transgenes were only about 2- to 8-fold lower than the EF1-α reference level. RNA extraction and reverse transcription Total RNA, extracted by means of RNeasy Plant Mini Kit (Qiagen, Germany), was treated with DNase I  (DNA-free; Ambion, TX, USA). One microgram of RNA and oligo dT primers (500 ng) were heated for 5 min at 65 °C, chilled on ice and mixed with Transcriptor buffer (Roche, Germany), 0.5 μl of Protector RNase Inhibitor (Roche, Germany), 2 μl of 10 mM dNTPs and 10 units of Transcriptor Reverse Transcriptase (Roche, Germany). The first strand of cDNA was synthesized at 55 °C for 30 min. RNA samples were reverse transcribed in two independent RT reactions and each cDNA was measured twice. qRT PCR measurement The first strand of cDNA was diluted 10–20 times and qPCR was performed using the LightCycler 480 SYBR Green I Master (Roche) in a final volume of 10 μl with 300 nM of each of the HPLC purified primers (Supplementary Table S1 available at JXB online), supplied by Metabion (Germany). The LightCycler LC 480 (Roche, Germany) was programmed as follows: 10 min of initial denaturation at 95 °C, then 40 cycles for 10 s at 95 °C, 8 s at 58 °C, and 15 s at 72  °C. PCR efficiencies were estimated from calibration curves generated from serial dilution of cDNAs. A  calibrator was used to correct for run-to-run variation. To distinguish CrCOL splice variants, TaqMan probes (FAM dye, TAMRA quencher) were designed by TIB Molbiol (Germany) (Supplementary Table S1 available at JXB online). LightCycler 480 Probes Master kit (Roche, Germany) was applied in a final volume of 10 μl with 300 nM of each of primers and 50 nM TaqMan probe under the following cycling conditions: 10 min of initial denaturation at 95 °C, then 45 cycles for 10 s at 95 °C, 30 s at 60 °C, and 1 s at 72 °C. The specificity of each Taqman assay was verified through qPCR reactions with plasmids carrying particular CrCOL inserts as a template. Crossing points obtained with non-specific targets were at least 15 cycles lower than with the corresponding splice variant. The relative ratio of the target and reference gene was calculated as follows:

ERC

pR

E TCpT 

(1)

where ET/ER represents the efficiency of target/reference amplification and CpT/CpR represents the cycle number at target/reference detection threshold (crossing point). Expression values were normalized with actin (Cháb et al., 2008). Its invariant expression was confirmed by direct quantification of cDNA as described by Libus and Štorchová (2006). Southern hybrization Genomic DNA (1 μg) extracted according to Štorchová et al. (2000) was digested with restriction enzymes, electrophoresed overnight on a 0.9% agarose gel, and transferred to a positively charged membrane (Roche, Germany) by capillary blotting. A  0.5-kb fragment of the first exon of the CrCOL1 gene was amplified and labelled with digoxigenin (DIG) using a PCR labelling kit (Roche, Germany) according to the manufacturer. The primers used to generate the probes are provided in Supplementary Table S1 (available at JXB online). The membranes were hybridized with non-radioactively labelled probes and visualized as described (Cháb et al., 2008).

Data analysis We estimated the number of days to first flower bud and first flower, and the number of stem and rosette leaves at time of flowering in transgenic, mutant, and wild-type lineages of A. thaliana. We performed one-way ANOVA implemented in IBM SPSS Statistics. Honestly significant differences (HSD) were determined by Tukey test. Mean values and standard errors of transcript abundances from two biological and two technical replicates were calculated using Microsoft Excel.

Results Overexpression of the CrFTL genes in A. thaliana We performed a complementation assay to verify the function of the CrFTL genes (Cháb et  al., 2008). CrFTL1 and CrFTL2 cDNAs driven by the CaMV 35S promoter were transformed into A. thaliana ft-2 mutant. Flowering was dramatically accelerated in the six independent homozygous lines carrying CrFTL1 gene. They flowered when only three rosette leaves were developed, about 2 weeks following germination (Table 1). In contrast, the five independent CrFTL2 transgene lines examined in detail (out of 10)  exhibited no effect on flowering, despite high transgene expression (Table 1). Similar results were observed when CrFTL1 and CrFTL2 were overexpressed in wild-type individuals. We conclude that CrFTL1 is a functional equivalent of the FT gene in A. thaliana, whereas no clue about possible function was provided by heterologous complementation in the case of CrFTL2.

Light triggers CrFTL1 expression We grew C.  rubrum seedlings under light for 6 d and then transferred them to dark for 4, 6, 12, 18, or 24 h. We measured transcript levels in 3-h intervals (Fig. 1). CrFTL1 expression was induced by light-on and always reached the maximum 6–8 h after a dark–light transition regardless of the extent of preceding darkness. Thus, it was light-on, not previous transition to dark, that determined the timing of the initial peak. CrFTL1 expression was highest if preceded by a 12-h dark period, lower in the case of 18 h of darkness, very low after 6-h and 24-h dark periods, and negligible after 4 h of darkness. CrFTL1 expression correlated with flower induction. The highest proportion of flowering individuals (87%) was found among seedlings exposed to a single 12-h dark period; 33% of plants flowered after 18 h of darkness, and no flowering was observed after 4-, 6- or 24-h periods of darkness. We may conclude that CrFTL1 expression was induced by lighton and its increase reflected the length of the dark period, being maximal after 12 h of darkness, which was also the most efficient for flower induction.

Characterization of CrCOL genes In a search for additional homologues of important flowering-related genes, we identified two full-length clones corresponding to two distinct CONSTANS-like genes termed CrCOL1 and CrCOL2 in the cDNA library prepared from total RNA of C. rubrum ecotype 374. The predicted CrCOL proteins contain two B-boxes, four motifs (M1–M4) in the

2140 | Drabešová et al. Table 1.  Flowering time (mean number of rosette leaves at time of flowering) of A. thaliana transformed with the C. rubrum genes under the control of the 35S promoter Data were collected from at least 10 homozygous T3 plants grown under long days. Asterisks denote honestly significant difference (HSD) estimated by Tukey test. Genotype Experiment 1 ft mutant (ft-2) 35S::CrFTL1 (ft-2) 35S::CrFTL2 (ft-2) Wild type Ler-0 35S::CrFTL1 (Ler-0) 35S::CrFTL2 (Ler-0) Experiment 2 Wild type Ler-0 35S::CrCOL1 (Ler-0) 35S::CrCOL2s (Ler-0) co mutant (co-2) 35S::CrCOL1 (co-2) 35S::CrCOL2s (co-2)

Number of rosette leaves (range of mean values) 10.4 2.5***–3.2*** 8.4–12.0 6.9 2.4***–3.5*** 5.9–7.5

6 5 3 4

6.7 6.0–8.2 5.4–7.7 17.5 17.3–18.4 17.3–18.4

Fig. 1.  The CrFTL1 gene is activated after the transfer from dark to light. Five-day-old C. rubrum seedlings grown under light were treated by a dark period of various lengths (specified in black boxes). The RNA samples were taken every 3 h. Mean values and standard errors (shown as bars) were calculated from four independent measurements of two seedlings (two technical and two biological replicates).

middle region, CCT and COOH domains (Fig. 2). This structure is specific to Group I, sub-group Ia of COL proteins (Griffiths et al., 2003). CrCOL1 and CrCOL2 are highly similar at both nucleotide (97%) and protein (98%) levels. Their closest homologue is BvCOL1 from sugar beet (Chia et al., 2008), which shows 89% and 90% similarity at nucleotide and protein level, respectively. Just like BvCOL1, CrCOL genes are closer to AtCOL2 (67% and 58% similarity at nucleotide and protein level, respectively) than to AtCO (63% and 54% similarity at nucleotide and protein level). To estimate the number of CrCOL variants, we performed a Southern hybridization with a 0.5-kb probe corresponding to B-boxes and an M1–M2 region under highly stringent conditions. Genomic DNA digested with HindIII provided six strong and two weak bands, whereas EcoRI digest produced

Number of T1 lineages

4 4 5 5

two strong and six weaker bands (Fig.  3). As there are no HindIII or EcoRI sites in a probe-covered area in known COL genes, two bands in the HindIII digest should correspond to CrCOL1 and CrCOL2. The remaining four bands are likely derived from two to four additional COL variants. The exact number of gene variants depends on whether or not a HindIII site is present in the area covered by the probe in the sequences of so far unidentified COL genes. If HindIII cleaves the unknown gene copy, two bands instead of one would correspond to one gene. The strong EcoRI bands might be derived from two or more restriction fragments of similar sizes, not separated on the gel. We interpret the results of Southern hybridization as the evidence for two to four additional, yet unknown COL variants present in a C. rubrum genome besides CrCOL1 and CrCOL2 genes.

CrCOL genes are alternatively spliced CrCOL1 and CrCOL2 genes possess a single intron located at the same position as in other members of the sub-group Ia COL genes. The sizes of the CrCOL1 and CrCOL2 introns are 769 bp and 752 bp, respectively. They are 93% identical, which reflects a close relatedness of both CrCOL genes. In the course of sequencing individual clones from the cDNA library obtained by RACE, we revealed two cDNAs corresponding to CrCOL transcripts that were significantly shorter. They were missing 87-bp (or 90-bp) stretches encoding amino acids between positions 152 and 181 (or 182)  of CrCOL1 (or CrCOL2) protein (see Fig.  2). The sequence of the missing region, which partially overlapped the M2 domain, started with GT and ended with AG. This suggested the possibility that it might have been an intron spliced out from the primary transcript by alternative splicing. To verify this notion, we performed qRT PCR with primers and probes specific for short transcripts (Supplementary Table S1 available at JXB online) with genomic DNA instead of cDNA

Flowering in Chenopodium rubrum | 2141

Fig. 2.  Multiple sequence alignment of CrCOL, BvCOL1, and AtCOL proteins. Conserved domains are marked by the lines above the alignment. Alternatively spliced regions of CrCOL proteins are underlined by XXX. Biochemically similar amino acids are shown on a grey background.

to reveal a shorter form of the CrCOL gene, if it exists. No amplification was observed. In addition, PCR with genomic DNA and the primers targeted to the sequences on both sides of the putative intron produced a single band (not shown). If a shorter form of the CrCOL gene was present in C. rubrum genome, two bands differing by 90 bp would be found. Thus, the transcripts, denoted CrCOL1s and CrCOL2s, which lack 31 or 30 amino acids, respectively, originated by alternative splicing.

Overexpression of the CrCOL genes in A. thaliana

Fig. 3.  Southern hybridization of EcoRI and HindIII digested DNA with a COL probe. Molecular weights in kb are shown on the right.

To assess a possible role of the CrCOL genes in flower induction we performed a complementation assay of late-flowering co-2 mutant of A.  thaliana. We chose one full-length transcript (CrCOL1) and one alternatively spliced variant (CrCOL2s). The constructs containing particular cDNA under the control of the strong CaMV 35S promoter were transformed into wild type or co-2 mutants. Between 5 and 15 T1 kanamycin-resistant transformants were obtained for each transgene, and four to five homozygous transgenic lines were selected for detailed analysis. The expression of the transgene was confirmed by qRT PCR measurement. No significant decrease in rosette leaf numbers at time of flowering (Table  1) was observed in transformants compared with recipient plants (wild type or co-2 mutant) grown under long-day conditions. Three of four lineages 35S::CrCOL1 in Ler-0 background exhibited a slight but statistically non-significant increase in rosette leaf numbers.

2142 | Drabešová et al. The levels of FT expression were comparable in all transgenic lineages 35S::CrCOL1, 35S::CrCOL2 and in wild type. Thus, CrCOL1 and CrCOL2s cannot complement co mutation in A. thaliana and do not seem to confer flowering suppression.

The diurnal and circadian pattern of CrCOL expression in light and dark Because we identified four different transcripts derived from two CrCOL genes, we wondered how they were expressed. We developed qRT PCR assays specific to each transcript with the aid of TaqMan probes. At first, we examined CrCOL expression in C.  rubrum seedlings grown under the flower-inductive photoperiodic regime of 12 h light, 12 h dark (Fig. 4A). The expression profiles of the four transcripts were similar. Expression of all CrCOL transcripts peaked before dawn and reached minima in the middle of day. A  floral inducer CrFTL1 exhibited diurnal fluctuation, showing peaks of expression anti-phasic to CrCOL transcripts, with maxima in the afternoon and minima at night. To explore free running rhythmicity without continuing entrainment by dark–light cycles, gene expression in C.  rubrum seedlings grown under permanent light followed by one 12-h dark period was examined (Fig. 4B). The levels of all CrCOL transcripts peaked before dawn and showed circadian fluctuation with a period of about 27–30 h under permanent light. The main maximum was preceded by a smaller peak at night. A trend toward double peaks was also visible during the first dark period in Fig. 4A. The most prominent feature of CrCOL expression under permanent light was its low amplitude. The maxima during light exposure were about five times lower than the peaks achieved in the dark. Expression of the CrCOL genes in C.  rubrum seedlings grown under constant light for 5 d and then transferred to permanent dark oscillated with a period of about 24–27 h (Fig.  4C). The second maximum was about 40% lower than the initial one; a gradual reduction continued across the third peak. However, the decrease was much weaker than under constant light after a 12-h period of darkness (Fig.  4B), when CrCOL expression was about five times lower. As in previous experiments, no marked differences were observed among the four transcripts derived from the CrCOL genes. Control seedlings grown under permanent light since the initial dark period necessary for germination exhibited very low CrCOL expression with slight circadian rhythmicity (Fig.  4C). In conclusion, CrCOL expression rhythmically oscillated under constant dark as well as under constant light after entrainment by a single dark period. CrCOL transcript levels were always much lower in light than in dark. High levels of CrCOL transcripts during darkness were in sharp contrast with CrFTL1 expression, which also rhythmically oscillated in dark, but with very low amplitudes (Cháb et al., 2008). If plotted onto Fig. 4C, CrFTL1 expression would follow the zero line. To investigate the effect of light on CrCOL gene expression in more detail, their transcript profiles during and after dark periods of different lengths were estimated.

Light downregulates CrCOL transcript levels CrCOL expression was measured in the seedlings during and after a single dark period lasting 4, 6, 12, 18, or 24 h, as described previously to examine CrFTL1 transcripts (see Fig. 1). As all four transcripts showed similar patterns, only CrCOL1 transcript levels are given in Fig.  5. A  dramatic decrease in CrCOL expression was observed after light-on. A  dark–light transition downregulated CrCOL expression regardless of the length of the preceding dark period. Light exhibited the exactly opposite effect on CrCOL than on CrFTL1, supressing the former and activating the latter.

Discussion A permissive period of darkness followed by light-on is necessary to induce CrFTL1 expression and flowering in C. rubrum Homologues of the FT gene (Kardailsky et  al., 1999) have been recognized as floral inducers in many plant species (Carmel-Goren et al., 2003; Hecht et al., 2005; reviewed by Pin and Nilsson, 2012). They are the regulatory targets of CO-like transcription factors located upstream in a signalling pathway and mediate photoperiod information both in long-day (D’Aloia et  al., 2009) and short-day (Hayama et al., 2007) plants. We have previously identified the CrFTL1 gene, a putative floral promoter in C.  rubrum (Cháb et  al., 2008). In this study, we employed a complementation assay to demostrate that it is indeed a functional equivalent of FT in A. thaliana. CrFTL1 is the closest homologue of the sugar beet floral inducer BvFT2 (Pin et al., 2010), whereas its paralogue CrFTL2, which was not capable of complementing ft mutant of A. thaliana, is closely related to the sugar beet floral repressor BvFT1 (Pin et al., 2010; Harig et al., 2012). Rhythmic expression of CrFTL1 in constant darkness was set up by a light–dark transition (Cháb et al., 2008), analogous to other short-day plants (Kojima et al., 2002; Hayama et al., 2007). However, unlike other short-day plants, the amplitudes were very low or negligible. The high increase in CrFTL1 transcript level, necessary for flower induction, was always observed several hours after the end of a dark period, regardless of how long it lasted, and thus regardless of the phase of the circadian oscillation at lights-on. In contrast, the duration of a period of darkness determined how pronounced the increase in CrFTL1 transcript level was. A  12-h dark period which resulted in the highest elevation of CrFTL1 transcript level also led to the highest proportion of flowering individuals. A  recent study of the GmFT2a and GmFT5a genes in short-day soybean (Kong et al., 2010) revealed diurnal oscillation of their expression peaking in late afternoon, similar to CrFTL1. The expression of soybean FT homologues in constant darkness was not investigated, hence we cannot determine whether their expression pattern was analogous to CrFTL1. Interestingly, both soybean (Buzzell, 1971) and C. rubrum (Cummings, 1967) are very efficiently induced to flowering by a 12-h dark period, which is otherwise less efficient for rice or Pharbitis. It will be of interest to compare the flower induction pathways of soybean and C. rubrum in greater detail.

Flowering in Chenopodium rubrum | 2143

Fig. 4.  Diurnal and circadian pattern of expression of four splice variants derived from CrCOL genes. Five-day-old C. rubrum seedlings were grown in the light and then transferred to 12-h dark/12-h light photoperiodic regime (A) or treated by a single period of 12-h darkness followed by constant light (B). Expression of CrCOL genes in permanent dark to which 5-day-old seedlings grown under light were transferred is shown in (C). The RNA samples were taken every 3 h for 72 h. CrFTL1 also exhibits diurnal rhythmicity, but with opposite amplitudes. Mean values were calculated from two independent measurements of two seedlings (two technical and two biological replicates).

CrCOL genes are rhythmically expressed and downregulated by light in C. rubrum We identified two novel COL genes termed CrCOL1 and CrCOL2 with a remarkable expression pattern in a shortday plant C.  rubrum. They belong to the sub-group Ia, which also contains the gene CO, an important element of a

photoperiodic regulatory pathway in A. thaliana. Expression of CrCOL1 and CrCOL2 exhibited diurnal and circadian rhythms, similar to other COL genes (Hayama et  al., 2007; Almada et  al., 2009). However, unlike CO in A.  thaliana (Suarez-Lopez et  al., 2001) or Hd1 in rice (Kojima et  al., 2002), it peaked not at the end of the day or at midnight, but

2144 | Drabešová et al. Numerous CrCOL transcripts in C. rubrum

Fig. 5.  The CrCOL genes are downregulated after transfer from dark to light. Five-day-old C. rubrum seedlings grown under light were treated by a dark period of various lengths (specified in black boxes). The samples were taken every 3 h. All four CrCOL splice variants displayed a similar pattern, but only CrCOL1 is shown for clarity. Mean values and standard errors (showed as bars) were calculated from four independent measurements of two seedlings (two technical and two biological replicates).

rather before dawn. This characteristic resembled the rhythmic expression of AtCOL1 and AtCOL2 (Ledger et al., 2001), genes not related to flowering. A similar transcript profile is also specific to the BvCOL1 gene in sugar beet (Chia et al., 2008), a functional equivalent of CO, which represented the closest homologue of CrCOL genes found in GenBank (October 2012). The transition from dark to light dramatically downregulated CrCOL transcript levels regardless of the length of a dark period or a phase of rhythmic oscillation. If light persisted after initial darkness, CrCOL expression fluctuated with a free running period, but with much lower amplitudes than in the dark. This contrasted with BvCOL1 in sugar beet, which showed slowly declining expression under constant light (Chia et al., 2008). Light positively influences CO transcription in A.  thaliana under long days and is responsible for its biphasic expression pattern, with an additional peak at dusk (Suarez-Lopez et  al., 2001). A  higher level of CO mRNA and a higher stability of CO protein under long days (Valverde et al., 2004) leads to FT activation and then flower induction. Thus, CO expression transmits information about day length. It is possible that downregulation of the CrCOL genes by a dark–light transition contributes to the perception of night length in short-day C. rubrum. The rhythmic expression pattern of the CrCOL genes suggested that they may be involved in perceiving dark periods and thus in control of processes dependent on day–night cycles, e.g. flower induction. However, the examined CrCOL genes did not complement co mutants of A. thaliana, unlike BvCOL1 (Chia et al., 2008) and other COL homologues (Liu et al., 2001). A negative result of heterologous complementation cannot exclude the possibility that the CrCOL genes were involved in flowering control in C. rubrum, but could not function properly in A. thaliana. Overexpression and silencing of the CrCOL genes in C. rubrum will provide more conclusive evidence about the function of these genes.

Alternative splicing generated shorter transcripts derived from the CrCOL1 and CrCOL2 genes that lacked a region encoding a part of the M2 domain. The examination of expression of CrCOL splice variants under various photoperiodic regimes in C.  rubrum seedlings did not provide a clue about a possible role of this phenomenon. All CrCOL splice variants displayed very similar expression profiles. The M2 domain, affected by alternative splicing, is one of four evolutionary conserved motifs located between the B-boxes and the CCT region. Its function is not known, but some segments in this area, particularly glutamine-rich sequences, play a role in transcriptional activation and are capable of binding to DNA (Tiwari et  al., 2010). It is possible that alternative splicing may influence the choice of the genes controlled by CrCOL factors. Alternative splicing contributes to the notable richness of COL transcripts in C. rubrum. Two to four additional COL genes, highly similar to known CrCOL genes, were revealed by Southern hybridization. This contrasts with only one subgroup Ia gene, BvCOL1, found by means of Southern hybridization in sugar beet by Chia et al. (2008). The larger number of COL genes in C. rubrum may reflect their functional diversification. COL genes in higher plants are involved in the control of various developmental processes, not only flower induction (Datta et al., 2006; Almada et al., 2009) but also in response to abiotic stresses (Winter et al., 2007). Chenopodium rubrum is tolerant to relatively high salt and nitrate concentrations (Wisskirchen, 2006). Some members of the numerous COL transcripts may help the plant to cope with osmotic or drought stresses. CrCOL1 and CrCOL2 are 97% identical and share similar introns. They may therefore represent homeologs originating from diploid parents of tetraploid C. rubrum. Polyploidy certainly contributed to increased number of CrCOL genes. To decipher the roles of individual members of this family, complementation assays in A. thaliana are helpful. However, silencing or overexpression of the genes under study in C. rubrum (Veit et al., 2006) will be necessary to reveal their functions.

CrCOL and CrFTL1 expression profiles show complementary expression levels The comparison of CrCOL and CrFTL1 expression in C.  rubrum seedlings revealed an interesting juxtaposition: CrCOL maxima corresponded to CrFTL1 minima in diurnal oscillation of transcript levels and vice versa. Also, when the CrCOL genes were downregulated by light-on after various periods of darkness (Fig.  5), CrFTL1 was upregulated. If CrCOL genes were involved in flowering control, they would play the role of a suppressor rather than a promoter. The investigation of FT and COL homologues in C. rubrum uncovered noteworthy features of their expression not reported in other short-day plants. Expression of the floral promoter CrFTL1 was induced by light-on and depended on the length of a preceding dark period. Expression of the

Flowering in Chenopodium rubrum | 2145 CrCOL genes exhibited diurnal and circadian rhythmicity and also light sensitivity, suggesting their role in the processes is controlled by day–night cycles, although more research is needed to understand their function. Thus the short-day plant C. rubrum deserves scientific attention as a suitable model for comparison with the long-day sugar beet in the same family, Amaranthaceae.

Supplementary material Supplementary data are available at JXB online. Table S1. The primers and probes.

Acknowledgements We are grateful to Professor Ove Nilsson for reading and commenting on the manuscript. We thank Nagavalli S. Kiran for providing pGreenII and pRT101 vectors and advice on CrFTL2 cloning, and Helena Mašterová for assistance with plant cultivation. We appreciate linguistic help and valuable comments by Amanda L.  Robertson, James D.  Stone and two anonymous reviewers. Financial support was provided through grants of the Grant Agency of the Czech Republic 522/05/0300 and P506/12/1359 to HS.

References Almada R, Cabrera N, Casaretto JA, Ruiz-Lara S, Villanueva EG. 2009. VvCO and VvCOL1, two CONSTANS homologous genes, are regulated during flower induction and dormancy in grapevine buds. Plant Cell Reports 28, 1193–1203. Amasino R. 2010. Seasonal and developmental timing of flowering. The Plant Journal 61, 1001–1013. Ben-Naim O, Eshed R, Parnis A, Teper-Bamnolker P, Shalit A, Coupland G, Samach A, Lifschitz E. 2006. The CCAAT binding factor can mediate interactions between CONSTANS-like proteins and DNA. The Plant Journal 46, 462–476. Bohlenius H, Huang T, Charbonnel-Campaa L, Brunner AM, Jansson S, Strauss SH, Nilsson O. 2006. CO/FT regulatory module controls timing of flowering and seasonal growth cessation in trees. Science 312, 1040–1043. Buzzell RI. 1971. Inheritance of a soybean flowering response to fluorescent-daylength conditions. Canadian Journal of Genetics and Cytology 13, 703–707. Carmel-Goren L, Liu YS, Lifschitz E, Zamir D. 2003. The SELFPRUNING gene family in tomato. Plant Molecular Biology 52, 1215–1222. Cháb D, Kolář J, Olson MS, Štorchová H. 2008. Two Flowering Locus T (FT) homologs in Chenopodium rubrum differ in expression patterns. Planta 228, 929–940. Cheng XF, Wang ZY. 2005. Overexpression of COL9, a CONSTANSLIKE gene, delays flowering by reducing expression of CO and FT in Arabidopsis thaliana. The Plant Journal 43, 758–768. Chia TYP, Muller A, Jung, C, Mutasa-Gottgens ES. 2008. Sugar beet contains a large CONSTANS-LIKE gene family including a CO homologue that is independent of the early-bolting (B) gene locus. Journal of Experimental Botany 59, 2735–2748. Clough SJ, Bent AF. 1998. Floral dip: a simplified method for Agrobacterium-mediated transformation of Arabidopsis thaliana. The Plant Journal 16, 735–743. Corbesier L, Vincent C, Jang SH et al. 2007. FT protein movement contributes to long-distance signaling in floral induction of Arabidopsis. Science 316, 1030–1033. Cumming BG. 1967. Early-flowering plants. In: Wilt FH, Wessels NK, eds. Methods in developmental biology . New York: Crowell Co., 277–299. D’Aloia M, Tamseddak K, Bonhomme D, Bonhomme F, Bernier G, Perilleux C. 2009. Gene activation cascade triggered by a single

photoperiodic cycle inducing flowering in Sinapis alba. The Plant Journal 59, 962–973. Datta S, Hettiarachchi GH, Deng XW, Holm M. 2006. Arabidopsis CONSTANS-LIKE3 is a positive regulator of red light signaling and root growth. The Plant Cell 18, 70–84. Gonzalez-Schain ND, Diaz-Mendoza M, Zurczak M, Suarez-Lopez P. 2012. Potato CONSTANS is involved in photoperiodic tuberization in a graft-transmissible manner. The Plant Journal 70, 678–690. Griffiths S, Dunford RP, Coupland G, Laurie DA. 2003. The evolution of CONSTANS-like gene families in barley, rice, and Arabidopsis. Plant Physiology 131, 1855–1867. Harig L, Beinecke FA, Oltmanns J, Muth J, Müller O, Rüping B, Twyman RW, Fischer R, Prüfer D, Noll GA. 2012. Proteins from the FLOWERING LOCUS T-like subclade of the PEBP family act antagonistically to regulate floral initiation in tobacco. The Plant Journal 72, 908–921. Hassidim M, Harir Y, Yakir E, Kron Y, Green RM. 2009. Overexpression of CONSTANS-LIKE 5 can induce flowering in short-day grown Arabidopsis. Planta 230, 481–491. Hayama R, Agashe B, Luley E, King R, Coupland G. 2007. A circadian rhythm set by dusk determines the expression of FT homologues and the short-day photoperiodic flowering response in Pharbitis. The Plant Cell 19, 2988–3000. Hecht V, Foucher F, Ferrandiz C et al. 2005. Conservation of Arabidopsis flowering genes in model legumes. Plant Physiology 137, 1420–1434. Hellens RP, Edwards EA, Leyland NR, Bean S, Mullineaux PM. 2000. pGreen: a versatile and flexible binary Ti vector for Agrobacteriummediated plant transformation. Plant Molecular Biology 42, 819–832. Jaeger KE, Wigge PA. 2007. FT protein acts as a long-range signal in Arabidopsis. Current Biology 17, 1050–1054. Jang S, Marchal V, Panigrahi KCS, Wenkel S, Soppe W, Deng XW, Valverde F, Coupland G. 2008. Arabidopsis COP1 shapes the temporal pattern of CO accumulation conferring a photoperiodic flowering response. EMBO Journal 27, 1277–1288. Kardailsky I, Shukla V, Ahn JH, Dagenais N, Christensen SK, Nguyen JT, Chory J, Harrison MJ, Weigel D. 1999. Activation tagging of the floral inducer FT. Science 286, 1962–1965. Knoche K, Kephart D. 1999. Cloning blunt-end Pfu DNA polymerasegenerated PCR fragments into pGEM®-T Vector Systems. Promega Notes 71, 10–13. Kojima S, Takahashi Y, Kobayashi Y, Monna L, Sasaki T, Araki T, Yano M. 2002. Hd3a, a rice ortholog of the Arabidopsis FT gene, promotes transition to flowering downstream of Hd1 under short day conditions. Plant and Cell Physiology 43, 1096–1105. Kong F, Liu B, Xia Z et al. 2010. Two coordinately regulated homologs of FLOWERING LOCUS T are involved in the control of photoperiodic flowering in soybean. Plant Physiology 154, 1220–1231. Landa P, Štorchová H, Hodek J, Vanková R, Podlipná R, Maršik P, Ovesná J, Vaněk T. 2010. Transferases and transporters mediate the detoxification and capacity to tolerate trinitrotoluene in Arabidopsis. Functional and Integrative Genomics 10, 547–559. Ledger S, Strayer C, Ashton F, Kay SA, Putterill J. 2001. Analysis of the function of two circadian-regulated CONSTANS-LIKE genes. The Plant Journal 26, 15–22. Libus J, Štorchová H. 2006. Quantification of cDNA generated by reverse transcription of total RNA provides a simple alternative tool for quantitative RT-PCR normalization. BioTechniques 41, 156–164. Liu J, Yu J, McIntosh L, Kende H, Zeevaart JA. 2001. Isolation of a CONSTANS ortholog from Pharbitis nil and its role in flowering. Plant Physiology 125, 1821–1830. Pin PA, Nilsson O. 2012. The multifaceted roles of FLOWERING LOCUS T in plant development. Plant, Cell and Environment 35, 1742–1755. Pin PA, Benlloch R, Bonnet D, Wremerth-Weich E, Kraft T, Gielen JJL, Nilsson O. 2010. An antagonistic pair of FT homologs mediates the control of flowering time in sugar beet. Science 330, 1397–1400. Putterill J, Robson F, Lee K, Simon R, Coupland G. 1995. The CONSTANS gene of Arabidopsis promotes flowering and encodes a protein showing similarities to zinc-finger transcription factors. Cell 80, 847–857.

2146 | Drabešová et al. Robson F, Costa MM, Hepworth SR, Vizir I, Pineiro M, Reeves PH, Putterill J, Coupland G. 2001. Functional importace of conserved domains in the flowering-time gene CONSTANS demonstrated by analysis of mutant alleles and transgenic plants. The Plant Journal 28, 619–631. Rose TM, Schultz ER, Henikoff JG, Pietrokovski S, McCallum CM, Henikoff S. 1998. Consensus degenerate hybrid oligonucleotide primers for amplification of distantly-related sequences. Nucleic Acids Research 26, 1628–1635. Seidlová F, Krekule J. 1973. The negative response of photoperiodic floral induction in Chenopodium rubrum L. to preceding growth. Annals of Botany 37, 605–614. Štorchová H, Hrdličková R, Chrtek Jr J, Tetera M, Fitze D, Fehrer J. 2000. An improved method of DNA isolation from plants collected in the field and conserved in saturated NaCl/CTAB solution. Taxon 49, 79–84. Suarez-Lopez P, Wheatley K, Robson K, Onouchi H, Valverde F, Coupland G. 2001. CONSTANS mediates between the circadian clock and the control of flowering in Arabidopsis. Nature 410, 1116–1119. Tiwari, SB, Shen Y, Chang HC et al. 2010. The flowering time regulator CONSTANS is recruited to the FLOWERING LOCUS T promoter via a unique cis-element. New Phytologist 187, 57–66. Töpfer R, Matzeit V, Gronenborg B, Schell J, Steinbiss HH. 1987. A set of plant expression vector for transcriptional and translational fusions. Nucleic Acids Research 15, 5890.

Valverde F, Mouradov A, Soppe W, Ravenscroft D, Samach A, Coupland G. 2004. Photoreceptor regulation of CONSTANS protein in photoperiodic flowering. Science 303, 1003–1006. Veit J, Wagner E, Albrechtova JTP. 2006. Floral dip transformation of Chenopodium rubrum. In: Teixeira da Silva JA, ed. Floriculture, ornamental and plant biotechnology: advances and topical issues . Isleworth, UK: Global Science Books, 49–53. Wenkel S, Turck F, Singer K, Gissot L, Le Gourrierec J, Samach A, Coupland G. 2006. CONSTANS and the CCAAT box binding complex share a functionally important domain and interact to regulate flowering of Arabidopsis. The Plant Cell 18, 2971–2984. Winter D, Vinegar B, Nahal H, Ammar R, Wilson GV, Provart NJ. 2007. An ‘electronic fluorescent pictograph’ browser for exploring and analyzing large-scale biological data sets. PloS ONE 2, e718. Wisskirchen R. 2006. An experimental study on the growth and flowering of riparian pioneer plants under long- and short-day conditions. Flora 201, 3–23. Yano M, Katayose Y, Ashikari M et al. 2000. Hd1, a major photoperiod sensitivity quantitative trait locus in rice, is closely realated to the Arabidopsis flowering time gene CONSTANS. The Plant Cell 12, 2473–2483. Yano M, Kojima S, Takahashi Y, Lin HX, Sasaki T. 2001. Genetic control of flowering time in rice, a short-day plant. Plant Physiology 127, 1425–1429. Zeevaart JAD. 2008. Leaf-produced floral signals. Current Opinion in Plant Biology 11, 541–547.

A dark-light transition triggers expression of the floral promoter CrFTL1 and downregulates CONSTANS-like genes in a short-day plant Chenopodium rubrum.

The proper timing of flowering is essential for the adaptation of plant species to their ever-changing environments. The central position in a complex...
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