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Genes associated with thermosensitive genic male sterility in rice identified by comparative expression profiling

机译:通过比较表达谱鉴定与水稻热敏性雄性不育相关的基因

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Thermosensitive genic male sterile (TGMS) lines and photoperiod-sensitive genic male sterile (PGMS) lines have been successfully used in hybridization to improve rice yields. However, the molecular mechanisms underlying male sterility transitions in most PGMS/TGMS rice lines are unclear. In the recently developed TGMS-Co27 line, the male sterility is based on co-suppression of a UDP-glucose pyrophosphorylase gene (Ugp1), but further study is needed to fully elucidate the molecular mechanisms involved. Microarray-based transcriptome profiling of TGMS-Co27 and wild-type Hejiang 19 (H1493) plants grown at high and low temperatures revealed that 15462 probe sets representing 8303 genes were differentially expressed in the two lines, under the two conditions, or both. Environmental factors strongly affected global gene expression. Some genes important for pollen development were strongly repressed in TGMS-Co27 at high temperature. More significantly, series-cluster analysis of differentially expressed genes (DEGs) between TGMS-Co27 plants grown under the two conditions showed that low temperature induced the expression of a gene cluster. This cluster was found to be essential for sterility transition. It includes many meiosis stage-related genes that are probably important for thermosensitive male sterility in TGMS-Co27, inter alia: Arg/Ser-rich domain (RS)-containing zinc finger proteins, polypyrimidine tract-binding proteins (PTBs), DEAD/DEAH box RNA helicases, ZOS (C2H2 zinc finger proteins of Oryza sativa), at least one polyadenylate-binding protein and some other RNA recognition motif (RRM) domain-containing proteins involved in post-transcriptional processes, eukaryotic initiation factor 5B (eIF5B), ribosomal proteins (L37, L1p/L10e, L27 and L24), aminoacyl-tRNA synthetases (ARSs), eukaryotic elongation factor Tu (eEF-Tu) and a peptide chain release factor protein involved in translation. The differential expression of 12 DEGs that are important for pollen development, low temperature responses or TGMS was validated by quantitative RT-PCR (qRT-PCR). Temperature strongly affects global gene expression and may be the common regulator of fertility in PGMS/TGMS rice lines. The identified expression changes reflect perturbations in the transcriptomic regulation of pollen development networks in TGMS-Co27. Findings from this and previous studies indicate that sets of genes involved in post-transcriptional and translation processes are involved in thermosensitive male sterility transitions in TGMS-Co27.
机译:热敏基因雄性不育系(TGMS)和光周期敏感性雄性不育系(PGMS)已成功用于杂交以提高水稻产量。然而,在大多数PGMS / TGMS水稻品系中,雄性不育转变的分子机制尚不清楚。在最近开发的TGMS-Co27品系中,雄性不育是基于共抑制UDP-葡萄糖焦磷酸化酶基因(Ugp1),但需要进一步研究以充分阐明涉及的分子机制。在高温和低温下生长的TGMS-Co27和野生型合江19(H1493)植物的基于芯片的转录组谱分析表明,在两种条件下或在两种条件下或两者下,代表8303个基因的15462个探针集差异表达。环境因素强烈影响了全球基因表达。 TGMS-Co27在高温下强烈抑制了一些对花粉发育重要的基因。更重要的是,在两种条件下生长的TGMS-Co27植物之间的差异表达基因(DEG)的序列聚类分析表明,低温诱导了基因簇的表达。发现该簇对于无菌过渡是必不可少的。它包括许多与减数分裂阶段相关的基因,这些基因可能对TGMS-Co27中的热敏雄性不育很重要,尤其是:含Arg / Ser富集域(RS)的锌指蛋白,多嘧啶束结合蛋白(PTB),DEAD / DEAH盒RNA解旋酶,ZOS(水稻的C2H2锌指蛋白),至少一种参与转录后过程的聚腺苷酸结合蛋白和一些其他包含RNA识别基序(RRM)域的蛋白,真核起始因子5B(eIF5B) ,核糖体蛋白(L37,L1p / L10e,L27和L24),氨酰基-tRNA合成酶(ARS),真核生物延伸因子Tu(eEF-Tu)和参与翻译的肽链释放因子蛋白。通过定量RT-PCR(qRT-PCR)验证了对花粉发育,低温反应或TGMS重要的12个DEG的差异表达。温度强烈影响全球基因表达,可能是PGMS / TGMS水稻品系中常见的育性调节剂。鉴定出的表达变化反映了TGMS-Co27中花粉发育网络的转录组调控中的干扰。从本研究和以前的研究中发现,转录后和翻译过程中涉及的基因集与TGMS-Co27中的热敏雄性不育转变有关。

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