首页> 美国卫生研究院文献>Journal of Virology >Cell proteins bind specifically to West Nile virus minus-strand 3 stem-loop RNA.
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Cell proteins bind specifically to West Nile virus minus-strand 3 stem-loop RNA.

机译:细胞蛋白特异性结合西尼罗河病毒负链3茎环RNA。

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摘要

The first 96 nucleotides of the 5'noncoding region (NCR) of West Nile virus (WNV) genomic RNA were previously reported to form thermodynamically predicted stem-loop (SL) structures that are conserved among flaviviruses. The complementary minus-strand 3' NCR RNA, which is thought to function as a promoter for the synthesis of plus-strand RNA, forms a corresponding predicted SL structure. RNase probing of the WNV 3' minus-strand stem-loop RNA [WNV (-)3' SL RNA] confirmed the existence of a terminal secondary structure. RNA-protein binding studies were performed with BHK S100 cytoplasmic extracts and in vitro-synthesized WNV (-)3' SL RNA as the probe. Three RNA-protein complexes (complexes 1,2, and 3) were detected by a gel mobility shift assay, and the specificity of the RNA-protein interactions was confirmed by gel mobility shift and UV-induced cross-linking competition assays. Four BHK cell proteins with molecular masses of 108, 60, 50, and 42 kDa were detected by UV-induced cross-linking to the WNV (-)3' SL RNA. A preliminary mapping study indicated that all four proteins bound to the first 75 nucleotides of the WNV 3' minus-strand RNA, the region that contains the terminal SL. A flavivirus resistance phenotype was previously shown to be inherited in mice as a single, autosomal dominant allele. The efficiencies of infection of resistant cells and susceptible cells are similar, but resistant cells (C3H/RV) produce less genomic RNA than congenic, susceptible cells (C3H/He). Three RNA-protein complexes and four UV-induced cross-linked cell proteins with mobilities identical to those detected in BHK cell extracts with the WNV (-)3' SL RNA were found in both C3H/RV and C3H/He cell extracts. However, the half-life of the C3H/RV complex 1 was three times longer than that of the C3H/He complex 1. It is possible that the increased binding activity of one of the resistant cell proteins for the flavivirus minus-strand RNA could result in a reduced synthesis of plus-strand RNA as observed with the flavivirus resistance phenotype.
机译:先前已报道了西尼罗河病毒(WNV)基因组RNA的5'非编码区(NCR)的前96个核苷酸形成了黄病毒中保守的热力学预测茎环(SL)结构。互补的负链3'NCR RNA被认为起合成正链RNA的启动子的作用,形成了相应的预测SL结构。 WNV 3'负链茎环RNA [WNV(-)3'SL RNA]的RNase探测证实了末端二级结构的存在。使用BHK S100细胞质提取物并以体外合成的WNV(-)3'SL RNA作为探针进行RNA-蛋白质结合研究。通过凝胶迁移率变动测定法检测了三种RNA-蛋白质复合物(复合物1,2和3),并且通过凝胶迁移率变动和UV诱导的交联竞争测定法确认了RNA-蛋白质相互作用的特异性。通过UV诱导的WNV(-)3'SL RNA交联,检测到了四种分子量分别为108、60、50和42 kDa的BHK细胞蛋白。初步的作图研究表明,所有四种蛋白质均与WNV 3'负链RNA(包含末端SL的区域)的前75个核苷酸结合。以前显示出黄病毒抗性表型在小鼠中作为单个常染色体显性等位基因遗传。耐药细胞和易感细胞的感染效率相似,但耐药细胞(C3H / RV)产生的基因组RNA比同类易感细胞(C3H / He)少。在C3H / RV和C3H / He细胞提取物中均发现了3种RNA蛋白复合物和4种紫外线诱导的交联细胞蛋白,其迁移率与使用WNV(-)3'SL RNA在BHK细胞提取物中检测到的迁移率相同。但是,C3H / RV复合物1的半衰期是C3H / He复合物1的半衰期的三倍。很可能其中一种抗性细胞蛋白与黄病毒负链RNA的结合活性增加,导致黄病毒抗性表型所观察到的正链RNA合成减少。

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