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Induction of RNA interference genes by double-stranded RNA; implications for susceptibility to RNA interference

机译:双链RNA诱导RNA干扰基因;对RNA干扰敏感性的影响

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Gene silencing by RNA interference (RNAi) can be a useful reverse genetics tool in eukaryotes. However, some species appear refractory to RNAi. To study the role of the differential expression of RNAi proteins in RNAi, we isolated partial dicer-2, argonaute-2 translin, vasa intronic gene (VIG) and tudor staphylococcus/micrococcal nuclease (TSN) genes from the tobacco hornworm, Manduca sexta, a well-studied insect model which we have found to be variably sensitive to RNAi. We found that the RNAi gene, translin, was expressed at minimal levels in M. sexta tissue and that there is a specific, dose-dependent upregulation of dicer-2 and argonaute-2 expression in response to injection with dsRNA, but no upregulation of the other genes tested. Upregulation of gene expression was rapid and transient. In order to prolong the upregulation we introduced multiple doses of dsRNA, resulting in multiple peaks of dicer-2 gene expression. Our results have implications for the design of RNAi experiments and may help to explain differences in the sensitivity of eukaryotic organisms to RNAi
机译:RNA干扰(RNAi)使基因沉默可能是真核生物中有用的反向遗传学工具。但是,某些物种似乎对RNAi不利。为了研究RNAi蛋白差异表达在RNAi中的作用,我们从烟草角虫曼杜卡氏菌中分离了部分dicer-2,argonaute-2转蛋白,vasa内含子基因(VIG)和tudor葡萄球菌/微球菌核酸酶(TSN)基因,一个经过充分研究的昆虫模型,我们发现它对RNAi具有不同的敏感性。我们发现,RNAi基因translin在六分枝杆菌组织中以最低水平表达,并且响应于dsRNA的注射,dicer-2和argonaute-2表达有特定的,剂量依赖性上调,但没有上调。其他测试的基因。基因表达的上调是快速且短暂的。为了延长上调,我们引入了多剂量的dsRNA,导致dicer-2基因表达的多个峰。我们的结果对RNAi实验的设计有影响,并可能有助于解释真核生物对RNAi敏感性的差异

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