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甲状腺激素受体的滤膜结合测定法

Filter-binding assay procedure for thyroid hormone receptors.

作者信息

Inoue A, Yamakawa J, Yukioka M, Morisawa S

出版信息

Anal Biochem. 1983 Oct 1;134(1):176-83. doi: 10.1016/0003-2697(83)90280-4.

Abstract

An assay procedure for thyroid hormone receptor activity which used nitrocellulose membrane filters was developed. Receptor proteins, extracted from washed rat liver nuclei with a 0.4 M NaCl solution, were incubated with 125I-labeled thyroid hormone (T3), and filtered on the cellulose ester membranes under suction at 2 degrees C. The filters were subsequently washed with cold buffer and counted for 125I radioactivity. The method allowed an accurate estimation of the receptor activity, satisfying a linear relationship between the activity and the receptor protein concentrations. The usefulness of this filter-binding method became evident when it was compared with the conventional procedure that employs Sephadex G-25 columns. For practical application to routine assays, various filtration conditions were examined, and a standard procedure was established. Using this technique, the isolated receptors were determined to possess an apparent Kd of 1.38 X 10(-10) M and a pH optimum of T3 binding at 8.2-8.4.

摘要

开发了一种使用硝酸纤维素膜过滤器的甲状腺激素受体活性测定方法。用0.4M NaCl溶液从洗涤过的大鼠肝核中提取的受体蛋白,与125I标记的甲状腺激素(T3)一起孵育,并在2℃下抽滤于纤维素酯膜上。随后用冷缓冲液洗涤过滤器,并对125I放射性进行计数。该方法能够准确估计受体活性,活性与受体蛋白浓度之间呈线性关系。当将这种滤膜结合法与采用葡聚糖G - 25柱的传统方法进行比较时,其有效性变得明显。为了实际应用于常规测定,研究了各种过滤条件,并建立了标准程序。使用该技术,确定分离出的受体的表观解离常数(Kd)为1.38×10(-10)M,T3结合的最适pH为8.2 - 8.4。

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