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烟草蚀纹病毒NIa蛋白酶在病毒和外源蛋白序列中的自催化活性。

Autocatalytic activity of the tobacco etch virus NIa proteinase in viral and foreign protein sequences.

作者信息

Rorrer K, Parks T D, Scheffler B, Bevan M, Dougherty W G

机构信息

Department of Microbiology, Oregon State University, Corvallis 97331-3804.

出版信息

J Gen Virol. 1992 Apr;73 ( Pt 4):775-83. doi: 10.1099/0022-1317-73-4-775.

Abstract

The small nuclear inclusion (NIa) protein of the tobacco etch virus (TEV) is synthesized initially as part of a genome-derived high M(r) precursor. The NIa protein releases itself from this genome-derived precursor by self-cleavage, or an autocatalytic processing event. Cleavage between specific glutamine-glycine dipeptides at the N and C termini generates the 430 amino acid or 49,000 M(r) (49K) NIa protein. The requirements of this autocatalytic release, or cis cleavage, were examined by constructing gene cassettes encoding the TEV NIa protein which could be ligated into particular locations in cDNA of the TEV genome and also into foreign gene DNA sequences. Using cell-free transcription and translation systems, polyproteins containing TEV NIa sequences were synthesized and assayed for (i) autocatalysis and (ii) the ability of a functional NIa proteinase, purified from plant tissue, to cleave in bimolecular or trans reactions various artificial polyproteins which contained an inactive form of the NIa proteinase. The NIa self-cleavage events required an active proteinase sequence and a consensus TEV cleavage site sequence at the N and C termini. These results were consistent for NIa protein sequences placed at a foreign TEV cleavage site or in unrelated proteins. Differences were noted in the trans cleavage of these sites.

摘要

烟草蚀纹病毒(TEV)的小核内含物(NIa)蛋白最初作为基因组衍生的高分子量(M(r))前体的一部分被合成。NIa蛋白通过自我切割,即一种自催化加工事件,从这种基因组衍生的前体中释放出来。在N端和C端特定的谷氨酰胺-甘氨酸二肽之间进行切割,产生430个氨基酸或49,000分子量(49K)的NIa蛋白。通过构建编码TEV NIa蛋白的基因盒来研究这种自催化释放或顺式切割的要求,这些基因盒可以连接到TEV基因组cDNA的特定位置以及外源基因DNA序列中。利用无细胞转录和翻译系统,合成了含有TEV NIa序列的多蛋白,并对其进行了如下检测:(i)自催化作用;(ii)从植物组织中纯化的功能性NIa蛋白酶在双分子或反式反应中切割各种含有无活性形式NIa蛋白酶的人工多蛋白的能力。NIa自我切割事件需要一个活性蛋白酶序列以及在N端和C端的一个共有TEV切割位点序列。对于置于外源TEV切割位点或无关蛋白中的NIa蛋白序列,这些结果是一致的。在这些位点的反式切割中发现了差异。

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