Constructing SSH Library of Cotton Under Drought Stress and Analysis of Drought Associated Genes

Q3 Agricultural and Biological Sciences
De-Long WANG, Wu-Wei YE, Jun-Juan WANG, Li-Yan SONG, Wei-Li FAN, Yu-Peng CUI
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引用次数: 9

Abstract

A forward cDNA-SSH library was constructed from a drought-tolerant cotton (Gossypium hirsutum L.) inbred line, Handan 177, to understand the expressions of drought-induced genes. Using suppression subtractive hybridization method, a total of 2300 positive clones were obtained, of which 300 clones were selected for PCR validation and sequencing. Among these clones, 284 were available sequences. According to clustering analysis of the expressed sequence tag (EST), 202 uniESTs were found, including 28 contigs and 174 singlets. The result of BlastN showed that 156 uniESTs had homologous sequences in GenBank database. The result of BlastX indicated that 116 uniESTs had high homology with proteins with known functions, and 40 uniESTs showed high similarities with unknown proteins or putative proteins. Thirty-three uniESTs were located into 55 KEGG pathways using KOBAS software, including 23 pathways at a significant level (P < 0.05). These significant pathways were mainly related to pyruvate metabolism (15%) and glyoxylate and dicarboxylate metabolism (12%). A large group of drought-induced genes were detected in the cDNA library, which were involved in signal transduction, energy metabolism, protein metabolism, nucleic acid metabolism, photosynthesis, and transmembrane transport. Some of them were associated with drought tolerance, such as malate synthase genes (MS1, 0001_C12 and MS2, 0002_F01), malate dehydrogenase genes (Md1, 001_C12 and Md2, 002_F01), NAC type transcription factor (001_C08), BZR1/BES1 (003_G04), zinc finger protein gene (zfp, 003_C06), and translationally controlled tumor protein gene (tctp, 002_C04).

干旱胁迫下棉花SSH文库构建及干旱相关基因分析
以抗旱棉花(Gossypium hirsutum L.)自交系邯郸177为材料,构建了正向cDNA-SSH文库,以了解抗旱诱导基因的表达。采用抑制减法杂交法,共获得2300个阳性克隆,筛选出300个克隆进行PCR验证和测序。其中可利用序列284个。对表达序列标签(EST)进行聚类分析,共发现202个单元,其中contigs 28个,singlets 174个。BlastN结果显示,156个uniest在GenBank数据库中有同源序列。BlastX结果表明,116个uniESTs与已知功能蛋白具有高度同源性,40个uniESTs与未知蛋白或推测蛋白具有高度同源性。利用KOBAS软件将33个单元定位到55个KEGG通路中,其中23个通路处于显著水平(P <0.05)。这些重要途径主要与丙酮酸代谢(15%)、乙醛酸盐和二羧酸盐代谢(12%)有关。在cDNA文库中检测到大量干旱诱导基因,涉及信号转导、能量代谢、蛋白质代谢、核酸代谢、光合作用和跨膜运输等。其中,苹果酸合成酶基因(MS1, 0001_C12和MS2, 0002_F01)、苹果酸脱氢酶基因(Md1, 001_C12和Md2, 002_F01)、NAC型转录因子(001_C08)、BZR1/BES1 (003_G04)、锌指蛋白基因(zfp, 003_C06)和翻译控制肿瘤蛋白基因(tctp, 002_C04)与耐旱性相关。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
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来源期刊
CiteScore
1.50
自引率
0.00%
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审稿时长
30 weeks
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