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通过DNA-纤维素色谱法最大限度地纯化活化的糖皮质激素受体。

Maximizing the purification of the activated glucocorticoid receptor by DNA-cellulose chromatography.

作者信息

Eisen H J, Glinsmann W H

出版信息

Biochem J. 1978 Apr 1;171(1):177-83. doi: 10.1042/bj1710177.

Abstract

With heat treatment (20 degrees C for 30 min), the glucocorticoid-receptor complex becomes 'activated' and undergoes an increase in affinity for DNA. A two-stage procedure was used to separate sequentially the rat liver glucocorticoid-receptor complex from proteins with high and low affinity for DNA. DNA-cellulose column chromatography of unheated cytosol resulted in the retention of DNA-binding proteins, but not the unactivated receptor complex. Heat treatment of the column eluate resulted in increased affinity of the receptor complex to DNA, and chromatography on DNA-cellulose then yielded receptor complex free from proteins with low affinity for DNA. Removal of DNA-binding proteins during the first chromatographic step was critically dependent on ionic conditions and the ratio of cytosol chromatographed to DNA-cellulose. A purification of 11000-fold (85% yield) was achieved by this procedure. The partially purified receptor complex was taken up by rat liver nuclei.

摘要

经过热处理(20摄氏度,30分钟),糖皮质激素受体复合物被“激活”,对DNA的亲和力增加。采用两阶段程序依次从对DNA具有高亲和力和低亲和力的蛋白质中分离大鼠肝脏糖皮质激素受体复合物。未加热的细胞溶质经DNA-纤维素柱色谱法处理后,DNA结合蛋白被保留,但未活化的受体复合物未被保留。对柱洗脱液进行热处理导致受体复合物对DNA的亲和力增加,然后在DNA-纤维素上进行色谱分离,得到的受体复合物不含对DNA具有低亲和力的蛋白质。在第一步色谱分离过程中去除DNA结合蛋白关键取决于离子条件以及进行色谱分离的细胞溶质与DNA-纤维素的比例。通过该程序实现了11000倍的纯化(产率85%)。部分纯化的受体复合物被大鼠肝细胞核摄取。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/fed9/1184147/3e2b6362cfc9/biochemj00489-0183-a.jpg

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