抗黄瓜花叶病毒RNAi载体的构建及烟草的转化

抗黄瓜花叶病毒RNAi载体的构建及烟草的转化

[目的]构建抗黄瓜花叶病毒RNAi载体,并将载体转入烟草.[方法]采用RT-PCR方法,扩增黄瓜花叶病毒NS04加工番茄分离物的RNA2基因组的序列选取CMV RAN2基因组中的复制酶片段作为靶序列,构建pBi35SCR2真核表达载体,并对表达载体时行鉴定;通过农杆菌介导的方法将表达载体转入烟草,用PCR的方法检测载体是否转入.[结果]系统进化树分析结果表明,RNA2中编码CMV-2a的序列与中国浙江的DQ412731 分离物有较高核苷本乡酸及氨基酸同源性,分别达到98.0%和96.5%;RCR结果表明,试验成功构建了pBi35SCR2真核表达载体,并成功将表达载体转入烟草[结论]试验获得的转...

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Veröffentlicht in:Hunan agricultural science & technology newsletter : HASTN 2010 (5)
1. Verfasser: 张瑜 郑银英 赵峰玉 乔亚红 崔百明 向本春 Yin-ying Feng-yu Ya-hong Bai-ming Ben-chun
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Sprache:eng
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Cucumber
eukaryotic
experiment
expression
material
Mosaic
phylogenetic
results
RNA2
RNAi载体
RT-PCR
sequence
target
test
tobacco
Transformation
transgenic
tree
vector
Virus
加工番茄
真核表达载体
黄瓜花叶病毒
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creator 张瑜 郑银英 赵峰玉 乔亚红 崔百明 向本春 Yin-ying Feng-yu Ya-hong Bai-ming Ben-chun
description [目的]构建抗黄瓜花叶病毒RNAi载体,并将载体转入烟草.[方法]采用RT-PCR方法,扩增黄瓜花叶病毒NS04加工番茄分离物的RNA2基因组的序列选取CMV RAN2基因组中的复制酶片段作为靶序列,构建pBi35SCR2真核表达载体,并对表达载体时行鉴定;通过农杆菌介导的方法将表达载体转入烟草,用PCR的方法检测载体是否转入.[结果]系统进化树分析结果表明,RNA2中编码CMV-2a的序列与中国浙江的DQ412731 分离物有较高核苷本乡酸及氨基酸同源性,分别达到98.0%和96.5%;RCR结果表明,试验成功构建了pBi35SCR2真核表达载体,并成功将表达载体转入烟草[结论]试验获得的转基因烟草可作为后期攻毒试验的材料,并为研究加工番茄抗黄瓜花叶病毒奠定了基础. Abstract: [Objective] Aimed to construct RNAi vector resistant to cucumber mosaic virus and transferred this vector into tobacco.[Method]RT-PCR method was used to amplify cucumber mosaic virus NSO4 and process RNA2 gene sequen of tomato isolates.The analysis results of phylogenetic tree demonstrated that the sequence in RNA2 encoded CMV-2a had 98.0% and 96.5% homology with nucleotide and amino acid of DQ412731 isolate of Zhejiang,China.The replicase fragment in CMV RAN2 gene was taken as target sequence to construct pBi35SCR2 eukaryotic expression vector,then the expression vector was identified.Through agrobacterium-mediated method,the expression vector was transferred into tabacco and PCR method was used to check the transfer.The PCR results demonstrated that the experiment had successfully construct eukaryotic expression vector of pBi35SCR2 and the expression vector was successfully transferred into tabacco. [Conclusion] The obtained transgenic tobacco could be used as challenge test material in following experiment and provided foundation for studying processing tomato resist cucumber mosaic virus.
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Abstract: [Objective] Aimed to construct RNAi vector resistant to cucumber mosaic virus and transferred this vector into tobacco.[Method]RT-PCR method was used to amplify cucumber mosaic virus NSO4 and process RNA2 gene sequen of tomato isolates.The analysis results of phylogenetic tree demonstrated that the sequence in RNA2 encoded CMV-2a had 98.0% and 96.5% homology with nucleotide and amino acid of DQ412731 isolate of Zhejiang,China.The replicase fragment in CMV RAN2 gene was taken as target sequence to construct pBi35SCR2 eukaryotic expression vector,then the expression vector was identified.Through agrobacterium-mediated method,the expression vector was transferred into tabacco and PCR method was used to check the transfer.The PCR results demonstrated that the experiment had successfully construct eukaryotic expression vector of pBi35SCR2 and the expression vector was successfully transferred into tabacco. [Conclusion] The obtained transgenic tobacco could be used as challenge test material in following experiment and provided foundation for studying processing tomato resist cucumber mosaic virus.</description><identifier>ISSN: 1009-4229</identifier><language>eng</language><subject>Cucumber ; eukaryotic ; experiment ; expression ; material ; Mosaic ; phylogenetic ; results ; RNA2 ; RNAi载体 ; RT-PCR ; sequence ; target ; test ; tobacco ; Transformation ; transgenic ; tree ; vector ; Virus ; 加工番茄 ; 真核表达载体 ; 黄瓜花叶病毒</subject><ispartof>Hunan agricultural science &amp; technology newsletter : HASTN, 2010 (5)</ispartof><woscitedreferencessubscribed>false</woscitedreferencessubscribed></display><links><openurl>$$Topenurl_article</openurl><openurlfulltext>$$Topenurlfull_article</openurlfulltext><thumbnail>$$Uhttp://image.cqvip.com/vip1000/qk/87034A/87034A.jpg</thumbnail><link.rule.ids>314,776,780,4010</link.rule.ids></links><search><creatorcontrib>张瑜 郑银英 赵峰玉 乔亚红 崔百明 向本春 Yin-ying Feng-yu Ya-hong Bai-ming Ben-chun</creatorcontrib><title>抗黄瓜花叶病毒RNAi载体的构建及烟草的转化</title><title>Hunan agricultural science &amp; technology newsletter : HASTN</title><addtitle>Agricultural Science & Technology</addtitle><description>[目的]构建抗黄瓜花叶病毒RNAi载体,并将载体转入烟草.[方法]采用RT-PCR方法,扩增黄瓜花叶病毒NS04加工番茄分离物的RNA2基因组的序列选取CMV RAN2基因组中的复制酶片段作为靶序列,构建pBi35SCR2真核表达载体,并对表达载体时行鉴定;通过农杆菌介导的方法将表达载体转入烟草,用PCR的方法检测载体是否转入.[结果]系统进化树分析结果表明,RNA2中编码CMV-2a的序列与中国浙江的DQ412731 分离物有较高核苷本乡酸及氨基酸同源性,分别达到98.0%和96.5%;RCR结果表明,试验成功构建了pBi35SCR2真核表达载体,并成功将表达载体转入烟草[结论]试验获得的转基因烟草可作为后期攻毒试验的材料,并为研究加工番茄抗黄瓜花叶病毒奠定了基础. Abstract: [Objective] Aimed to construct RNAi vector resistant to cucumber mosaic virus and transferred this vector into tobacco.[Method]RT-PCR method was used to amplify cucumber mosaic virus NSO4 and process RNA2 gene sequen of tomato isolates.The analysis results of phylogenetic tree demonstrated that the sequence in RNA2 encoded CMV-2a had 98.0% and 96.5% homology with nucleotide and amino acid of DQ412731 isolate of Zhejiang,China.The replicase fragment in CMV RAN2 gene was taken as target sequence to construct pBi35SCR2 eukaryotic expression vector,then the expression vector was identified.Through agrobacterium-mediated method,the expression vector was transferred into tabacco and PCR method was used to check the transfer.The PCR results demonstrated that the experiment had successfully construct eukaryotic expression vector of pBi35SCR2 and the expression vector was successfully transferred into tabacco. [Conclusion] The obtained transgenic tobacco could be used as challenge test material in following experiment and provided foundation for studying processing tomato resist cucumber mosaic virus.</description><subject>Cucumber</subject><subject>eukaryotic</subject><subject>experiment</subject><subject>expression</subject><subject>material</subject><subject>Mosaic</subject><subject>phylogenetic</subject><subject>results</subject><subject>RNA2</subject><subject>RNAi载体</subject><subject>RT-PCR</subject><subject>sequence</subject><subject>target</subject><subject>test</subject><subject>tobacco</subject><subject>Transformation</subject><subject>transgenic</subject><subject>tree</subject><subject>vector</subject><subject>Virus</subject><subject>加工番茄</subject><subject>真核表达载体</subject><subject>黄瓜花叶病毒</subject><issn>1009-4229</issn><fulltext>true</fulltext><rsrctype>article</rsrctype><creationdate>2010</creationdate><recordtype>article</recordtype><recordid>eNpjYeA0NDCw1DUxMrLkYOAtLs4yMDAwNDMzMrS04GSwetY1_eXulueT57zo2vi0f9vz6a3P1k8K8nPMfLF375O9k5_Pank2r-Xp7l1P-7ueN89_0dsJFHmxd83Tnmk8DKxpiTnFqbxQmptBxc01xNlDNzkjPy-9MDMvPT4pMTk7LTMnNd7IAGSpgaG5oTGRygCXZ0hB</recordid><startdate>2010</startdate><enddate>2010</enddate><creator>张瑜 郑银英 赵峰玉 乔亚红 崔百明 向本春 Yin-ying Feng-yu Ya-hong Bai-ming Ben-chun</creator><scope>2RA</scope><scope>92L</scope><scope>CQIGP</scope><scope>W95</scope><scope>~WA</scope></search><sort><creationdate>2010</creationdate><title>抗黄瓜花叶病毒RNAi载体的构建及烟草的转化</title><author>张瑜 郑银英 赵峰玉 乔亚红 崔百明 向本春 Yin-ying Feng-yu Ya-hong Bai-ming Ben-chun</author></sort><facets><frbrtype>5</frbrtype><frbrgroupid>cdi_FETCH-chongqing_backfile_20000101713</frbrgroupid><rsrctype>articles</rsrctype><prefilter>articles</prefilter><language>eng</language><creationdate>2010</creationdate><topic>Cucumber</topic><topic>eukaryotic</topic><topic>experiment</topic><topic>expression</topic><topic>material</topic><topic>Mosaic</topic><topic>phylogenetic</topic><topic>results</topic><topic>RNA2</topic><topic>RNAi载体</topic><topic>RT-PCR</topic><topic>sequence</topic><topic>target</topic><topic>test</topic><topic>tobacco</topic><topic>Transformation</topic><topic>transgenic</topic><topic>tree</topic><topic>vector</topic><topic>Virus</topic><topic>加工番茄</topic><topic>真核表达载体</topic><topic>黄瓜花叶病毒</topic><toplevel>online_resources</toplevel><creatorcontrib>张瑜 郑银英 赵峰玉 乔亚红 崔百明 向本春 Yin-ying Feng-yu Ya-hong Bai-ming Ben-chun</creatorcontrib><collection>中文科技期刊数据库</collection><collection>中文科技期刊数据库-CALIS站点</collection><collection>中文科技期刊数据库-7.0平台</collection><collection>中文科技期刊数据库-农业科学</collection><collection>中文科技期刊数据库- 镜像站点</collection><jtitle>Hunan agricultural science &amp; technology newsletter : HASTN</jtitle></facets><delivery><delcategory>Remote Search Resource</delcategory><fulltext>fulltext</fulltext></delivery><addata><au>张瑜 郑银英 赵峰玉 乔亚红 崔百明 向本春 Yin-ying Feng-yu Ya-hong Bai-ming Ben-chun</au><format>journal</format><genre>article</genre><ristype>JOUR</ristype><atitle>抗黄瓜花叶病毒RNAi载体的构建及烟草的转化</atitle><jtitle>Hunan agricultural science &amp; technology newsletter : HASTN</jtitle><addtitle>Agricultural Science & Technology</addtitle><date>2010</date><risdate>2010</risdate><issue>5</issue><issn>1009-4229</issn><abstract>[目的]构建抗黄瓜花叶病毒RNAi载体,并将载体转入烟草.[方法]采用RT-PCR方法,扩增黄瓜花叶病毒NS04加工番茄分离物的RNA2基因组的序列选取CMV RAN2基因组中的复制酶片段作为靶序列,构建pBi35SCR2真核表达载体,并对表达载体时行鉴定;通过农杆菌介导的方法将表达载体转入烟草,用PCR的方法检测载体是否转入.[结果]系统进化树分析结果表明,RNA2中编码CMV-2a的序列与中国浙江的DQ412731 分离物有较高核苷本乡酸及氨基酸同源性,分别达到98.0%和96.5%;RCR结果表明,试验成功构建了pBi35SCR2真核表达载体,并成功将表达载体转入烟草[结论]试验获得的转基因烟草可作为后期攻毒试验的材料,并为研究加工番茄抗黄瓜花叶病毒奠定了基础. Abstract: [Objective] Aimed to construct RNAi vector resistant to cucumber mosaic virus and transferred this vector into tobacco.[Method]RT-PCR method was used to amplify cucumber mosaic virus NSO4 and process RNA2 gene sequen of tomato isolates.The analysis results of phylogenetic tree demonstrated that the sequence in RNA2 encoded CMV-2a had 98.0% and 96.5% homology with nucleotide and amino acid of DQ412731 isolate of Zhejiang,China.The replicase fragment in CMV RAN2 gene was taken as target sequence to construct pBi35SCR2 eukaryotic expression vector,then the expression vector was identified.Through agrobacterium-mediated method,the expression vector was transferred into tabacco and PCR method was used to check the transfer.The PCR results demonstrated that the experiment had successfully construct eukaryotic expression vector of pBi35SCR2 and the expression vector was successfully transferred into tabacco. [Conclusion] The obtained transgenic tobacco could be used as challenge test material in following experiment and provided foundation for studying processing tomato resist cucumber mosaic virus.</abstract></addata></record>
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source Alma/SFX Local Collection
subjects Cucumber
eukaryotic
experiment
expression
material
Mosaic
phylogenetic
results
RNA2
RNAi载体
RT-PCR
sequence
target
test
tobacco
Transformation
transgenic
tree
vector
Virus
加工番茄
真核表达载体
黄瓜花叶病毒
title 抗黄瓜花叶病毒RNAi载体的构建及烟草的转化
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