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尿素和盐酸胍诱导噬菌体F2衣壳的解离和变性。

Urea and guanidine hydrochloride induced dissociation and denaturation of bacteriophage F2 capsid.

作者信息

Kitchell B B, Henkens R W

出版信息

Int J Pept Protein Res. 1979 Jul;14(1):21-6. doi: 10.1111/j.1399-3011.1979.tb01916.x.

Abstract

A single, low molecular weight protein is found after urea or guanidine hydrochloride (Gdn.HCl) treatment of empty capsids derived from bacteriophage f2. The final product of denaturation is apparently a monomer, existing as a random coil in larger than or equal to 4.0 M Gdn.HCl but in a less extended form in 8.0 M urea. In contrast, an 11 S protein component is isolated after treatment of the intact virus with 4.0 M Gdn.HCl (Zelazo & Haschemeyer, 1969), indicating that RNA plays a role in stabilizing larger subunits. Denaturation by Gdn.HCl occurs in two stages as measured by changes in CD and Stokes radius: dissociation that involves a structural perturbation of aromatic side chains, followed by a major, cooperative transition that evidently results in the loss of all noncovalent structure. Denaturation by urea appears to be a much less cooperative process that occurs in several steps over a wide range of urea concentration (1--7 M). In both urea and Gdn.HCl, dissociation into subunits begins at a lower concentration of denaturant than the major changes in conformation.

摘要

在用尿素或盐酸胍(Gdn.HCl)处理源自噬菌体f2的空衣壳后,发现了一种单一的低分子量蛋白质。变性的最终产物显然是一种单体,在大于或等于4.0 M的Gdn.HCl中以无规卷曲形式存在,但在8.0 M尿素中则以伸展程度较小的形式存在。相比之下,用4.0 M Gdn.HCl处理完整病毒后分离出一种11 S蛋白质组分(Zelazo和Haschemeyer,1969),这表明RNA在稳定较大亚基中起作用。通过圆二色性(CD)和斯托克斯半径的变化测量,Gdn.HCl引起的变性分两个阶段发生:解离涉及芳香族侧链的结构扰动,随后是一个主要的协同转变,显然导致所有非共价结构的丧失。尿素引起的变性似乎是一个协同性低得多的过程,在很宽的尿素浓度范围(1 - 7 M)内分几步发生。在尿素和Gdn.HCl中,亚基解离开始时的变性剂浓度都低于构象的主要变化时的浓度。

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