To further elucidate the functional roles of OsMADS51, we constructed a chimeric binary vector (Ubi:OsMADS51) by placing a OsMADS51 full-length cDNA under the maize ubiquitin (Ubi) promoter (Fig. 2A). This construct was introduced into Agrobacterium and transferred into plant cells via cocultivation (An et al., 1985; Hiei et al., 1997). Seven primary (T₁) transgenic plants were obtained and planted in a paddy field. All showed early flowering, albeit to varying degrees. For example, two lines flowered 2 weeks early, three lines about 10 d sooner, and two lines by just about 3 d compared with our control transgenic plants. The extent of early flowering was correlated with OsMADS51 expression levels when confirmed by northern-blot analyses (data not shown).We then chose two lines (3 and 4) that manifested early flowering by 10 d and selected homozygous plants and segregating wild type using hygromycin selection. T₃ progeny were reared in a growth room in either SDs (10 h light) or LDs (14 h light) to elucidate the daylength-dependent roles of OsMADS51. Homozygous plants exhibited early flowering by 9 d (line 3) and 7 d (line 4) in SDs. However, no significant phenotypic difference was observed between homozygous transgenic lines and wild-type plants grown in LDs (Table II). These results support our conclusion that OsMADS51 is a SD flowering activator.

In osmads51 mutants and UbiOsMADS51 transgenic plants, transcript levels of OsGI were unchanged (Figs. 3 and 4). Therefore, we believe that OsGI either functions upstream of OsMADS51 or is part of an independent pathway. Hayama et al. (2003) have previously reported that OsGI RNAi plants show delayed flowering in SDs, and we observed the same late-flowering phenotype in our OsGI antisense plants. Therefore, this SD-specific effect suggests that OsGI and OsMADS51 may function within the same pathway. To investigate the relationship between these two genes, we generated OsGI antisense plants and found that the OsMADS51 transcript level was reduced in plants grown under either SDs or LDs (Fig. 5A). As controls, we also examined expression levels from other flowering regulators—Ehd1, OsMADS14, and Hd3a—that had been demonstrated to function downstream of OsGI (Hayama et al., 2003; Doi et al., 2004). As expected, their transcript levels were reduced in our OsGI antisense plants (Fig. 5, E–G). These results indicate that OsGI does function in the same pathway as OsMADS51, with OsGI occurring upstream.

Because OsMAD51 functions between OsGI and Ehd1, the transcript level of a MADS-box gene may oscillate as do OsGI and Ehd1. Therefore, we measured OsMADS51 transcription in leaf blades from 55-DAG plants grown under SDs or LDs (Fig. 7). As reported previously (Hayama et al., 2003), the OsGI transcript level was low at the beginning of the day (Fig. 7A), but increased under light and reached a maximum at the end of the day. In darkness, that level was continuously reduced to a minimal amount. A similar rhythm was observed in LDs (data not shown). Under SDs, a similar induction curve was observed for OsMADS51 (Fig. 7B), increasing under light and decreasing in the dark. However, the change in transcript amounts was not as great as that for OsGI. Under LD, no such rhythm was found (data not shown).

The relationship between OsMADS51 and OsMADS50 was also investigated. We have previously reported that osmads50 plants show a late-flowering phenotype (delay of about 1 month), whereas overexpressors of OsMADS50 display an extreme early-flowering phenotype (Lee et al., 2004). Here, our mutations down-regulated the expression of OsMADS14 and Hd3a, suggesting that OsMADS50 functions upstream of OsMADS14. To evaluate whether OsMADS50 is another flowering activator that may influence OsMADS51, we examined whether OsMADS51 expression was altered in the osmads50 plants. However, that proved not to be the case (Supplemental Fig. S3). We also found that levels of OsMADS50 were unchanged in the osmads51 plants (Supplemental Fig. S3). Our results indicate that these two MADS-box genes function independently to control flowering time.

The osmads51 homozygous progeny were screened from T₁ seeds of the mutants. Genotyping was performed with 35 cycles of 95°C for 15 s, 55°C for 30 s, and 72°C for 40 s, using a combination of specific and T-DNA border primer sets as follows. The primer sets for osmads51-1 included F2 primer (5′-CAACAACTGACGAGGAGCAC-3′), R2 primer (5′-TAGATCATGACCTCCAGTAC-3′), and Gus2R primer in T-DNA (5′-TTGGGGTTTCTACAGGACGTAAC-3′). The osmads51-2 primer sets were F3 primer (5′-CCTCCCATGTTGTGTTCCTT-3′), R3 primer (5′-AAATGGCAAACCACTCGAAC-3′), and LB2R primer in T-DNA (5′-ACGTCCGCAATGTGTTATTAAG-3′). The Gus2R and LB2R primers were used to obtain the T-DNA flanking sequences by inverse PCR (An et al., 2003; Jeong et al., 2006).

The full-length cDNA clone of OsMADS51 (GenBank accession no. AB003327; Shinozuka et al., 1999) was amplified by PCR using a forward primer (5′-aagcttggggagctagggtttttcg-3′) and a reverse primer (5′-ggtaccaaacttatgcacaggacacc-3′). These primers contained one of two restriction enzyme sites, HindIII or Asp-718 (underlined in the primer sequences), for subsequent cloning. The PCR product was first cloned into pBluescript SK− (Stratagene). Afterward, cDNA was subcloned into the pGA1611 binary vector (Lee et al., 1999; Kim et al., 2003) between the maize (Zea mays) Ubi promoter and the nopaline synthase (nos) terminator to generate the UbiOsMADS51 construct. To create the Ehd1-RNAi construct, we PCR amplified the 346-bp Ehd1 cDNA fragment (724–1,069 bp from the translation initiation site of the Ehd1 cDNA clone; GenBank accession no.AB092506), using a forward primer (5′-gttgccagtcatctgcag-3′) and a reverse primer (5′-ggatgtggatcatgagacat-3′). The PCR product was first cloned into pGA2960, a Gateway vector modified from pENTR 1A (Invitrogen). Afterward, the product was subcloned into the pANDA (p2K-1) binary vector by a clonase reaction (Miki and Shimamoto, 2004). Our OsGI antisense construct was generated by inserting a partial cDNA clone into the binary vector pGA1611 in the antisense orientation. The cDNA clone of OsGI (GenBank accession no. AJ133787mRNA) was amplified by PCR using a forward primer (5′-agacagcaaatttgactgcggcag-3′) and a reverse primer (5′-gacatgctgagtgcacggacatgcg-3′). The PCR product was first cloned into a pGEM-T vector (Promega). This OsGI cDNA product was then digested with restriction enzymes XhoI (991 bp from start codon) and XbaI (2,374 bp from start codon). The digested product was cloned into pBluescript SK− and subcloned into the pGA1611 binary vector using KpnI and SacI. Rice transformation was performed according to Agrobacterium-mediated cocultivation methods (Lee et al., 1999). All transgenic rice plants were grown in the greenhouse and then transferred to a confined paddy field.

Total RNA was isolated with Tri Reagent (MRC). First-strand cDNA was synthesized from 2 μg of total RNA, using Moloney murine leukemia virus reverse transcriptase (Promega), with 10 ng of the oligo(dT)₁₅ primer and 2.5 mm deoxyriboneucleotide triphosphate, as described by Han et al. (2006). Actin1 was used for normalization of the cDNA quantity. Primers included 5′-GTTTGCTCTGCTCCTACTC-3′ and 5′-ACTCCTCCTCCAGCATTGAA-3′ for OsMADS51; 5′-TGGAGAAAGGTTGTGGATGC-3′ and 5′-CATAGACGGCACTTCAGCAGAT-3′ for OsGI; 5′-GTTGCCAGTCATCTGCAGAA-3′ and 5′-GGATGTGGATCATGAGACAT-3′ for Ehd1; 5′-TTCTCCTCTCCAAAGATTCC-3′ and 5′-CATACGCCTTTCTTGTTTCA-3′ for Hd1; 5′-TCCTATGCAGAAAAGGTCCTT-3′ and 5′-GGACGAAGCCAAAATATACAC-3′ for OsMADS14; 5′-ATGGCCGGAAGTGGCAGGGAC-3′ and 5′-ATCGATCGGGATCATCGTTAG-3′ for Hd3a; and 5′-GTATCCATGAGACTACATACATACAACT-3′ and 5′-TACTCAGCCTTGGCAATCCACA-3′ for Actin1. The reactions included an initial 5 min of denaturation at 95°C, followed by 95°C for 15 s, 55°C for 30 s, and 72°C for 40 s. PCR cycles numbered 28 for the flowering-regulator genes and 25 for Actin1.