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RNA聚合酶I与糖皮质激素调节的转录因子IC的共纯化

Copurification of RNA polymerase I and the glucocorticoid-regulated transcription factor IC.

作者信息

Mahajan P B, Thompson E A

机构信息

Department of Human Biological Chemistry and Genetics, University of Texas Medical Branch, Galveston 77550.

出版信息

Protein Expr Purif. 1992 Oct;3(5):410-6. doi: 10.1016/s1046-5928(05)80043-9.

Abstract

A simple and rapid method to copurify RNA polymerase I and the glucocorticoid-regulated transcription factor, TFIC, is described. This protocol results in 1262-fold purification and 15% total recovery of the enzyme and factors needed to support faithful transcription in vitro from cloned mouse rRNA gene (rDNA). Using this method, proteins involved in rDNA transcription were purified from exponentially growing lymphosarcoma P1798 cells as well as cells treated with 0.1 microM dexamethasone. A combination of transcription and reconstitution assays using G-free cassette-containing constructs and polyacrylamide gel electrophoretic analysis upon silver staining were used to detect TFIC activity as well as the characteristic TFIC polypeptides in control and dexamethasone-treated cell extracts. Treatment of P1798 cells with 0.1 microM dexamethasone for 24 h results in an over 95% reduction of TFIC activity, but no significant differences in the amount of TFIC polypeptides in the final product purified from control and glucocorticoid-treated cells could be detected. Our data indicate that glucocorticoid regulation of transcription of rDNA is mediated via post-translational modulation of the activity of TFIC.

摘要

本文描述了一种简单快速的方法,用于共纯化RNA聚合酶I和糖皮质激素调节的转录因子TFIC。该方案可实现1262倍的纯化,体外支持从克隆的小鼠rRNA基因(rDNA)进行忠实转录所需的酶和因子的总回收率达15%。使用此方法,从指数生长的淋巴肉瘤P1798细胞以及用0.1微摩尔地塞米松处理的细胞中纯化参与rDNA转录的蛋白质。使用含无G盒构建体的转录和重组分析以及银染后的聚丙烯酰胺凝胶电泳分析相结合的方法,检测对照和地塞米松处理的细胞提取物中的TFIC活性以及特征性TFIC多肽。用0.1微摩尔地塞米松处理P1798细胞24小时会导致TFIC活性降低超过95%,但从对照细胞和糖皮质激素处理细胞中纯化的最终产物中,TFIC多肽的量未检测到显著差异。我们的数据表明,糖皮质激素对rDNA转录的调节是通过TFIC活性的翻译后调节介导的。

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