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细胞蛋白TIA-1和TIAR与西尼罗河病毒互补负链RNA的3'茎环相互作用,并促进病毒复制。

Cell proteins TIA-1 and TIAR interact with the 3' stem-loop of the West Nile virus complementary minus-strand RNA and facilitate virus replication.

作者信息

Li W, Li Y, Kedersha N, Anderson P, Emara M, Swiderek K M, Moreno G T, Brinton M A

机构信息

Department of Biology, Georgia State University, Atlanta, Georgia 30303, USA.

出版信息

J Virol. 2002 Dec;76(23):11989-2000. doi: 10.1128/jvi.76.23.11989-12000.2002.

Abstract

It was reported previously that four baby hamster kidney (BHK) proteins with molecular masses of 108, 60, 50, and 42 kDa bind specifically to the 3'-terminal stem-loop of the West Nile virus minus-stand RNA [WNV 3'(-) SL RNA] (P. Y. Shi, W. Li, and M. A. Brinton, J. Virol. 70:6278-6287, 1996). In this study, p42 was purified using an RNA affinity column and identified as TIAR by peptide sequencing. A 42-kDa UV-cross-linked viral RNA-cell protein complex formed in BHK cytoplasmic extracts incubated with the WNV 3'(-) SL RNA was immunoprecipitated by anti-TIAR antibody. Both TIAR and the closely related protein TIA-1 are members of the RNA recognition motif (RRM) family of RNA binding proteins. TIA-1 also binds to the WNV 3'(-) SL RNA. The specificity of these viral RNA-cell protein interactions was demonstrated using recombinant proteins in competition gel mobility shift assays. The binding site for the WNV 3'(-) SL RNA was mapped to RRM2 on both TIAR and TIA-1. However, the dissociation constant (K(d)) for the interaction between TIAR RRM2 and the WNV 3'(-) SL RNA was 1.5 x 10(-8), while that for TIA-1 RRM2 was 1.12 x 10(-7). WNV growth was less efficient in murine TIAR knockout cell lines than in control cells. This effect was not observed for two other types of RNA viruses or two types of DNA viruses. Reconstitution of the TIAR knockout cells with TIAR increased the efficiency of WNV growth, but neither the level of TIAR nor WNV replication was as high as in control cells. These data suggest a functional role for TIAR and possibly also for TIA-1 during WNV replication.

摘要

先前有报道称,四种分子量分别为108、60、50和42 kDa的幼仓鼠肾(BHK)蛋白可特异性结合西尼罗河病毒负链RNA的3'-末端茎环[WNV 3'(-) SL RNA](P.Y. Shi、W. Li和M.A. Brinton,《病毒学杂志》70:6278 - 6287,1996)。在本研究中,利用RNA亲和柱纯化了p42,并通过肽段测序鉴定为TIAR。用抗TIAR抗体免疫沉淀了在与WNV 3'(-) SL RNA孵育的BHK细胞质提取物中形成的42-kDa紫外线交联病毒RNA-细胞蛋白复合物。TIAR和密切相关的蛋白TIA-1都是RNA结合蛋白的RNA识别基序(RRM)家族成员。TIA-1也结合WNV 3'(-) SL RNA。在竞争凝胶迁移率变动分析中使用重组蛋白证明了这些病毒RNA-细胞蛋白相互作用的特异性。WNV 3'(-) SL RNA的结合位点在TIAR和TIA-1上均被定位到RRM2。然而,TIAR RRM2与WNV 3'(-) SL RNA之间相互作用的解离常数(K(d))为1.5×10(-8),而TIA-1 RRM2的解离常数为1.12×10(-7)。在鼠TIAR基因敲除细胞系中,WNV的生长效率低于对照细胞。对于另外两种RNA病毒或两种DNA病毒未观察到这种效应。用TIAR重建TIAR基因敲除细胞可提高WNV的生长效率,但TIAR的水平和WNV的复制水平均不如对照细胞高。这些数据表明TIAR以及可能还有TIA-1在WNV复制过程中具有功能作用。

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