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对脊髓灰质炎病毒蛋白2C N端假定两亲性螺旋的研究。

Studies of a putative amphipathic helix in the N-terminus of poliovirus protein 2C.

作者信息

Paul A V, Molla A, Wimmer E

机构信息

Department of Microbiology, School of Medicine, State University of New York at Stony Brook 11794-5222.

出版信息

Virology. 1994 Feb 15;199(1):188-99. doi: 10.1006/viro.1994.1111.

Abstract

Poliovirus protein 2C contains near its N-terminus a putative amphipathic helix which is well conserved among picornaviruses. Three mutants were constructed within this region by site-directed mutagenesis. In the first mutant (pT7XL2-2C-N1) two glutamic acids were replaced with valines at the boundary of the charged and uncharged faces of the helix. The second mutant (pT7XL2-2C-N2) contains an isoleucine to lysine change in the hydrophobic half; in the third mutant (pT7XL2-2C-N3) two lysines were replaced with threonines in the hydrophilic half of the helix. Upon transfection of HeLa cells with RNA transcripts made from these plasmids only pT7XL2-2C-N1 yielded viable virus (W1-2C-N1) which had a small-plaque phenotype. A large-plaque revertant of this virus, W1-2C-N1R, was found to contain the original glutamic acid at one of the mutated sites (E19). There is no detectable minus-stranded RNA synthesis following transfection of HeLa cells with transcript RNAs of the other two plasmids, pT7XL2-2C-N2 and -N3. In vitro translation of these two mutant RNA transcripts in HeLa extracts revealed processing abnormalities in the P2/P3 region of the polyprotein. This leads to a nearly complete absence of 2C and 3AB, which might be the primary cause of defective viral RNA synthesis. The putative amphipathic helix was found to overlap a consensus binding site for double-stranded RNA.

摘要

脊髓灰质炎病毒蛋白2C在其N端附近含有一个假定的两亲性螺旋,该螺旋在小RNA病毒中高度保守。通过定点诱变在该区域构建了三个突变体。在第一个突变体(pT7XL2-2C-N1)中,螺旋带电荷面和不带电荷面边界处的两个谷氨酸被缬氨酸取代。第二个突变体(pT7XL2-2C-N2)在疏水半段含有异亮氨酸到赖氨酸的变化;在第三个突变体(pT7XL2-2C-N3)中,螺旋亲水半段的两个赖氨酸被苏氨酸取代。用这些质粒制备的RNA转录本转染HeLa细胞后,只有pT7XL2-2C-N1产生了具有小噬菌斑表型的活病毒(W1-2C-N1)。该病毒的一个大噬菌斑回复体W1-2C-N1R被发现其中一个突变位点(E19)含有原来的谷氨酸。用另外两个质粒pT7XL2-2C-N2和-N3的转录RNA转染HeLa细胞后,未检测到负链RNA合成。在HeLa提取物中对这两个突变RNA转录本进行体外翻译,结果显示多蛋白的P2/P3区域存在加工异常。这导致几乎完全没有2C和3AB,这可能是病毒RNA合成缺陷的主要原因。发现假定的两亲性螺旋与双链RNA的共有结合位点重叠。

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