Potato Virus Y mRNA Expression Knockdown Mediated by siRNAs in Cultured Mammalian Cell Line

Potato Virus Y mRNA Expression Knockdown Mediated by siRNAs in Cultured Mammalian Cell Line

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摘要 RNA interference(RNAi) is a powerful tool for functional gene analysis which has been successfully used to downregulate the expression levels of target genes.The goal of this research was to provide a highly robust and concise methodology for in-vitro screening of efficient siRNAs from a bulk to be used as a tool to protect potato plants against PVY invasion.In our study,a 480bp fragment of the capsid protein gene of potato virus Y(CP-PVY) was used as a target to downregulate PVY mRNA expression in-vitro,as the CP gene interferes with viral uncoating,translation and replication.A total of six siRNAs were designed and screened through transient transfection assay and knockdown in expression of CP-PVY mRNA was calculated in CHO-k cells.CP-PVY mRNA knockdown efficiency was analyzed by RT-PCR and real-time PCR of CHO-k cells co-transfected with a CP gene construct and siRNAs.Six biological replicates were performed in this study.In our findings,one CP gene specific siRNA out of a total of six was found to be the most effective for knockdown of CP-PVY mRNA in transfected CHO-k cells by up to 80%-90%. RNA interference （RNAi） is a powerful tool for functional gene analysis which has been successfully used to downregulate the expression levels of target genes. The goal of this research was to provide a highly robust and concise methodology for in-vitro screening of efficient siRNAs from a bulk to be used as a tool to protect potato plants against PVY invasion. In our study, a 480bp fragment of the capsid protein gene of potato virus Y （CP-PVY） was used as a target to downregulate PVY mRNA expression in-vitro, as the CP gene interferes with viral uncoating, translation and replication. A total of six siRNAs were designed and screened through transient transfection assay and knockdown in expression of CP-PVY mRNA was calculated in CHO-k cells. CP-PVY mRNA knockdown efficiency was analyzed by RT-PCR and real-time PCR of CHO-k cells co-transfected with a CP gene construct and siRNAs. Six biological replicates were performed in this study. In our findings, one CP gene specific siRNA out of a total of six was found to be the most effective for knockdown of CP-PVY mRNA in transfected CHO-k cells by up to 80%-90%.

作者 Bushra Tabassum Idrees Ahmad Nasir Tayyab Husnain

机构地区 National Centre of Excellence in Molecular Biology(CEMB)

出处《Virologica Sinica》 SCIE CAS CSCD 2011年第2期105-113,共9页 中国病毒学（英文版）

关键词马铃薯Y病毒 SIRNAS 细胞株哺乳动物基因表达 CP基因 RNA干扰 PCR技术 RNAi Potato virus Y siRNA in-vitro Expression knockdown Transfection

分类号 Q78 [生物学—分子生物学]

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1Atreya P L, Atreya C D, Pirone T P. 1991. Amino acid substitutions in the coat protein result in loss of insect transmissibility of a plant virus. Proc Natl Acad Sci USA, 88: 7887-7891.
2Baulcombe D. 2004. RNA silencing in plants. Nature, 431: 356-363.
3Baulcombe D. 2001. RNA silencing. Diced defence. Nature, 409: 295-296.
4Brummeikamp T R, Bernards R, Agami R. 2002. A system for stable expression of short interfering RNAs in mammalian cells. Science, 296: 550-553.
5Bukovinszki A, Diveki Z, Csanyi M, et al. 2007. Engineering resistance to PVY in different potato cultivars in a marker-free transformation system using a"Shooter mutant" A. tumefaciens. Plant Cell Report, 26: 459-465.
6De Bokx J A, Huttinga H. 1981. Potato Virus Y. Potato virus Y (CMI/AAB Descriptions of Plant Viruses, no. 242). Kew, UK: Commonwealth Microbiology Institute and Association of Applied Biology.
7Elbashir S M, Harborth J, Lendeckel W, et al 2001. Duplexes of 21-nucleotide RNAs mediate RNA interference in cultured mammalian cells. Nature, 411: 494-498.
8English J J, Mueller E. Bauleombe D C. 1996. Suppression of virus accumulation in transgenic plants exhibiting silencing of nuclear genes. Plant Cell, 8: 179-188.
9Gargouri-bouzid R, Jaova L, Mansove R B, et al. 2005 PVY resistant transgenic potato plants (cv. Cloustar) expressing the viral coat protein. J Plant Biotechnol, 3: 1-5.
10Hamilton A, Baulcombe D C. 1999. A species of small antisense RNA in post transcriptional gene silencing in plants. Science, 286: 950-952.

1牛娜,牛成峰,胡有燕,张凌娇,迟胜起.源于马铃薯Y病毒CP基因的dsRNA原核表达及提取[J].青岛农业大学学报（自然科学版）,2009,26(3):184-187. 被引量：2
2张荔子.蛋白质组学:人类下一个目标[J].中国社区医师,2002,18(1):47-48.
3Minghao Dang,Xiangxi Wang,Quan Wang,Yaxin Wang,Jianping Lin,Yuna Sun,Xuemei Li,Liguo Zhang,Zhiyong Lou,Junzhi Wang,Zihe Rao.Molecular mechanism of SCARB2-mediatec attachment and uncoating of EV71[J].Protein & Cell,2014,5(9):692-703. 被引量：15
4沙鸥.花园工具保护四步骤[J].花木盆景（上半月）,2004(1):37-37.
5中国科学院院士张启发指出：绿色超级稻是下一个目标[J].福建农业科技,2005(5):68-68.
6袁军涛,黄增飞,叶慧燕,唐瑶,温荣辉.马铃薯Y病毒P3N-PIPO酵母双杂交诱饵载体的构建及鉴定[J].基因组学与应用生物学,2017,36(1):299-304. 被引量：1
7孙燕霞,张献军,刘兰伟,刘秀君,刘红梅.高温激活RNA沉默介导的心叶烟抗病毒防御反应[J].植物病理学报,2008,38(1):58-63. 被引量：1
8陈宏.热度不减说克隆[J].农友,2002(12):29-29.
9刘冰花,李小红,汴国宁,熊世娟,李红霞,余蓉.黏细菌的筛选及鉴定的初步研究[J].食品与药品,2007,9(03A):38-40. 被引量：3
10畅捷张利华 David Cook.转基因食品：魔鬼还是天使？[J].英语学习,2015,0(3):14-16.

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2011年第2期

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Potato Virus Y mRNA Expression Knockdown Mediated by siRNAs in Cultured Mammalian Cell Line

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