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由腺病毒2型-猴病毒40杂交体Ad2+ND1 dp2所指定的融合蛋白的特性分析

Characterization of a fused protein specified by the adenovirus type 2-simian virus 40 hybrid Ad2+ND1 dp2.

作者信息

Fey G, Lewis J B, Grodzicker T, Bothwell A

出版信息

J Virol. 1979 Apr;30(1):201-17. doi: 10.1128/JVI.30.1.201-217.1979.

Abstract

The adenovirus type 2-simian virus 40 (SV40) hybrid virus Ad2+ND1 dp2 (E. Lukanidin, manuscript in preparation) specified two proteins (molecular weights, 24,000 and 23,000) that are, in part, products of an insertion of SV40 early DNA sequences. This was demonstrated by translation in vitro from viral mRNA that had been selected by hybridization to SV40 DNA. These two phosphorylated, nonvirion proteins were produced late in infection in amounts similar to adenovirus 2 structural proteins and were closely related to each other in tryptic peptide composition. The portion of SV40 DNA (map units 0.17 to 0.22 on the SV40 genome) coding for these proteins was joined to sequences coding for the amino-terminal part of the adenovirus type 2 structural protein IV (fiber). The Ad2+ND1 dp2 23,000- and 24,000-molecular-weight proteins were hybrid polypeptides, with about two-thirds of their tryptic peptides contributed by the fiber protein and the remainder contributed by SV40 T-antigen. They shared with T-antigen (molecular weight, 96,000) a carboxy-terminal proline-rich tryptic peptide. Together, the tryptic peptide composition of these proteins and the known SV40 DNA sequences suggested the reading frame for the translation of T-antigen. The carboxy terminus for T-anigen would then be located on the SV40 genome map next to the TAA terminator triplet at position 0.175, 910 bases away from the cleavage site of the restriction endonuclease EcoRI. Seven host range mutants from Ad2+ND1 dp2 were isolated that had lost the capacity to propagate on monkey cells. They did not induce detectable levels of the hybrid proteins. Three of these mutants had lost the SV40 DNA insertion that codes in part for these proteins. Thus, in analogy to the Ad2+ND1 30,000-molecular-weight protein, the presence of these proteins correlates with the presence of the helper function for adenovirus replication on monkey cells.

摘要

2型腺病毒-猴病毒40(SV40)杂交病毒Ad2+ND1 dp2(E.卢卡尼丁,正在准备手稿)产生了两种蛋白质(分子量分别为24,000和23,000),它们部分是SV40早期DNA序列插入的产物。这通过从与SV40 DNA杂交选择的病毒mRNA进行体外翻译得到了证明。这两种磷酸化的非病毒粒子蛋白质在感染后期产生,其数量与2型腺病毒结构蛋白质相似,并且在胰蛋白酶肽组成上彼此密切相关。编码这些蛋白质的SV40 DNA部分(在SV40基因组上的图谱单位为0.17至0.22)与编码2型腺病毒结构蛋白质IV(纤维)氨基末端部分的序列相连。Ad2+ND1 dp2的23,000和24,000分子量蛋白质是杂合多肽,其胰蛋白酶肽约三分之二由纤维蛋白贡献,其余由SV40 T抗原贡献。它们与T抗原(分子量96,000)共享一个富含羧基末端脯氨酸的胰蛋白酶肽。这些蛋白质的胰蛋白酶肽组成和已知的SV40 DNA序列共同表明了T抗原翻译的阅读框。T抗原的羧基末端将位于SV40基因组图谱上,紧挨着位于0.175位置的TAA终止三联体,距离限制性内切酶EcoRI的切割位点910个碱基。从Ad2+ND1 dp2中分离出七个宿主范围突变体,它们失去了在猴细胞上繁殖的能力。它们没有诱导出可检测水平的杂合蛋白质。其中三个突变体失去了部分编码这些蛋白质的SV40 DNA插入片段。因此,类似于Ad2+ND1的30,000分子量蛋白质,这些蛋白质的存在与腺病毒在猴细胞上复制的辅助功能的存在相关。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/3be4/353314/355003f280df/jvirol00184-0214-a.jpg

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