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小核糖核酸病毒的复制。I. 来自体外RNA合成的证据表明脊髓灰质炎病毒基因组的聚腺苷酸是由基因编码的。

Replication of picornaviruses. I. Evidence from in vitro RNA synthesis that poly(A) of the poliovirus genome is genetically coded.

作者信息

Dorsch-Häsler K, Yogo Y, Wimmer E

出版信息

J Virol. 1975 Dec;16(6):1512-7. doi: 10.1128/JVI.16.6.1512-1517.1975.

Abstract

A crude replication complex has been isolated from poliovirus-infected HeLa cells and used for synthesis of poliovirus replicative intermediate (RI) RNA, replicative form (RF) RNA, and single-stranded (SS) RNA in vitro. All three classes of virus-specific RNA synthesized in vitro are shown to contain poly(A). Poly(A) of RF and of SS RNA [RF-poly(A) and SS-poly(A)] has a chain length (50 to 70 nucleotides) that is shorter than that of poly(A) of in vivo-synthesized RNAs. Poly(A) of RI [RI-poly(A),] however, is at least 200 nucleotides long and, therefore, larger than poly(A) of RI isolated from HeLa cells 4 h after infection. The crude membrane-bound replication complex contains a terminal adenylate transferase activity that is stimulated by Mn2+ and the addition of an (Ap)2AOH primer. This transferase activity is found also in extracts of mock-infected cells. Partial purificaiton of the replication complex in a stepwise sucrose gradient, in which the viral replicase is associated with the smooth cytoplasmic membrane fraction, does not remove the terminal transferase. However, when the partially purified replication complex is treated with deoxycholate and sedimented through a sucrose gradient, a soluble replication complex can be isolated that is free from terminal adenylate transferase. This soluble replication complex was found to synthesize viral RNA-linked poly(A) longer in chain length than that synthesized by the crude replication complex. Taking into account the 5'-terminal poly(U) in poliovirus minus strands, our data suggest that polyadenylation of poliovirus RNA occurs by transcription and not by end addition. When compared to other viral systems, poliovirus and, probably, all picornaviruses appear to be unique in that the poly(A) of their genome is genetically coded.

摘要

已从感染脊髓灰质炎病毒的HeLa细胞中分离出一种粗制复制复合物,并用于体外合成脊髓灰质炎病毒复制中间体(RI)RNA、复制型(RF)RNA和单链(SS)RNA。体外合成的所有三类病毒特异性RNA均显示含有多聚腺苷酸(poly(A))。RF和SS RNA的poly(A) [RF-poly(A)和SS-poly(A)]的链长(50至70个核苷酸)比体内合成RNA的poly(A)短。然而,RI的poly(A) [RI-poly(A)]至少有200个核苷酸长,因此比感染后4小时从HeLa细胞中分离出的RI的poly(A)大。粗制的膜结合复制复合物含有一种末端腺苷酸转移酶活性,该活性受Mn2+和添加(Ap)2AOH引物的刺激。这种转移酶活性在模拟感染细胞的提取物中也能找到。在逐步蔗糖梯度中对复制复合物进行部分纯化,其中病毒复制酶与光滑的细胞质膜部分相关联,并不会去除末端转移酶。然而,如果用脱氧胆酸盐处理部分纯化的复制复合物并通过蔗糖梯度沉淀,则可以分离出一种不含末端腺苷酸转移酶的可溶性复制复合物。发现这种可溶性复制复合物合成的病毒RNA连接的poly(A)链长比粗制复制复合物合成的长。考虑到脊髓灰质炎病毒负链中的5'-末端多聚尿苷酸(poly(U)),我们的数据表明脊髓灰质炎病毒RNA的多聚腺苷酸化是通过转录而不是末端添加发生的。与其他病毒系统相比,脊髓灰质炎病毒以及可能所有小RNA病毒似乎都很独特,因为它们基因组的poly(A)是由基因编码的。

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