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温度梯度凝胶电泳。纯化形式及细胞提取物中核酸与蛋白质的热力学分析。

Temperature-gradient gel electrophoresis. Thermodynamic analysis of nucleic acids and proteins in purified form and in cellular extracts.

作者信息

Rosenbaum V, Riesner D

出版信息

Biophys Chem. 1987 May 9;26(2-3):235-46. doi: 10.1016/0301-4622(87)80026-1.

Abstract

A temperature-gradient gel electrophoresis technique and its application to the study of structural transitions of nucleic acids and protein-nucleic acid complexes are described. The temperature gradient is established in a slab gel by means of a simple ancillary device for a commercial horizontal gel apparatus. The gradient may be freely selected between 10 and 80 degrees C, and is highly reproducible and linear. In a normal application the biopolymers migrate perpendicular to the temperature gradient so that every individual molecule is at constant temperature throughout electrophoresis. The structural transition of a biopolymer is seen as a continuous band which is retarded or speeded up in the temperature range of the transition. Dissociation processes are mostly irreversible under the conditions of electrophoresis and, therefore, show up as discontinuous transitions from a slow-moving to fast-moving band. As examples the conformational transitions of viroids, double-stranded RNA from reovirus, double-stranded satellite RNA from cucumber mosaic virus and repressor-operator complexes have been studied. It could be shown that by this method dsRNA molecules may be differentiated which differ only in one base-pair, or proteins differing in one amino acid only. As a particular advantage, temperature-gradient gel electrophoresis allows the study of conformational transitions of biopolymers which have not been purified. The biopolymer may either be identified by silver staining as a specific band among many others or, if the study is carried out on nucleic acids, these may be recorded by hybridization with a radioactive probe.

摘要

本文描述了一种温度梯度凝胶电泳技术及其在核酸和蛋白质 - 核酸复合物结构转变研究中的应用。通过一种用于商用水平凝胶装置的简单辅助装置,在平板凝胶中建立温度梯度。该梯度可在10至80摄氏度之间自由选择,且具有高度的可重复性和线性。在常规应用中,生物聚合物垂直于温度梯度迁移,使得每个分子在整个电泳过程中处于恒定温度。生物聚合物的结构转变表现为一条连续的带,在转变温度范围内其迁移速度会减慢或加快。在电泳条件下,解离过程大多是不可逆的,因此表现为从慢速迁移带到快速迁移带的不连续转变。作为实例,研究了类病毒、呼肠孤病毒的双链RNA、黄瓜花叶病毒的双链卫星RNA以及阻遏物 - 操纵子复合物的构象转变。结果表明,通过这种方法可以区分仅相差一个碱基对的双链RNA分子,或仅相差一个氨基酸的蛋白质。一个特别的优点是,温度梯度凝胶电泳允许研究未纯化的生物聚合物的构象转变。生物聚合物既可以通过银染作为众多条带中的特定条带进行鉴定,或者,如果是对核酸进行研究,这些核酸可以通过与放射性探针杂交进行记录。

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