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沙漠植物唐古特白刺果实发育和成熟过程中的基因转录谱

Gene transcript profiles in the desert plant Nitraria tangutorum during fruit development and ripening.

作者信息

Wang Jia, Dang Zhenhua, Zhang Huirong, Zheng Linlin, Borjigin Tebuqin, Wang Yingchun

机构信息

College of Life Sciences, Inner Mongolia University, Hohhot, 010021, People's Republic of China.

College of Mongolian Medicine, Inner Mongolia Medical University, Hohhot, 010110, People's Republic of China.

出版信息

Mol Genet Genomics. 2016 Feb;291(1):383-98. doi: 10.1007/s00438-015-1116-5. Epub 2015 Sep 20.

Abstract

Nitraria tangutorum Bobr., a valuable wild shrub distributed in Northwest China, produces edible and medicinal berries. However, little is known about the molecular mechanisms of its fruit development and ripening. We performed de novo transcriptome sequencing of N. tangutorum fruit using the Illumina HiSeq™ 2000 sequencing platform. More than 62.94 million reads were obtained and assembled into 69,306 unigenes (average length, 587 bp). These unigenes were annotated by querying against five databases (Nr, Swiss-Prot, GO, COG, and KEGG); 42,929 and 26,809 unigenes were found in the Nr and Swiss-Prot databases, respectively. In ortholog analyses, 33,363 unigenes were assigned with one or more GO terms, 15,537 hits were aligned to 25 COG classes, and 24,592 unigenes were classified into 128 KEGG pathways. Digital gene expression analyses were conducted on N. tangutorum fruit at the green (S1), yellow (S2), and red (S3) developmental stages. In total, 8240, 5985, and 4994 differentially expressed genes (DEGs) were detected for S1 vs. S2, S1 vs. S3, and S2 vs. S3, respectively. Cluster analyses showed that a large proportion of DEGs related to plant hormones and transcription factors (TFs) showed high expression in S1, down-regulated expression in S2, and up-regulated expression in S3. We analyzed the expression patterns of 23 genes encoding 12 putative enzymes involved in flavonoid biosynthesis. The expression profiles of 10 DEGs involved in flavonoid biosynthesis were validated by Q-PCR analysis. The assembled and annotated transcriptome sequences and gene expression profile analyses provide valuable genetic resources for research on N. tangutorum.

摘要

唐古特白刺是一种分布于中国西北的珍贵野生灌木,其果实可食用且具有药用价值。然而,关于其果实发育和成熟的分子机制却知之甚少。我们利用Illumina HiSeq™ 2000测序平台对唐古特白刺果实进行了从头转录组测序。共获得了超过6294万个读段,并组装成69306个单基因(平均长度为587 bp)。通过与五个数据库(Nr、Swiss-Prot、GO、COG和KEGG)进行比对,对这些单基因进行了注释;在Nr和Swiss-Prot数据库中分别发现了42929个和26809个单基因。在直系同源分析中,33363个单基因被赋予了一个或多个GO术语,15537个匹配结果与25个COG类别进行了比对,24592个单基因被分类到128个KEGG通路中。对唐古特白刺果实绿色(S1)、黄色(S2)和红色(S3)发育阶段进行了数字基因表达分析。分别在S1与S2、S1与S3以及S2与S3中检测到8240、5985和4994个差异表达基因(DEG)。聚类分析表明,与植物激素和转录因子(TF)相关的大部分DEG在S1中高表达,在S2中下调表达,在S3中上调表达。我们分析了编码参与类黄酮生物合成的12种假定酶的23个基因的表达模式。通过Q-PCR分析验证了参与类黄酮生物合成的10个DEG的表达谱。组装和注释的转录组序列以及基因表达谱分析为唐古特白刺的研究提供了有价值的遗传资源。

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