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通过冻干法浓缩和保存核雄激素受体。

Concentration and preservation of nuclear androgen receptor by lyophilisation.

作者信息

de Larminat M A, Bruchovsky N, Rennie P S

出版信息

J Steroid Biochem. 1982 Jun;16(6):811-6. doi: 10.1016/0022-4731(82)90039-5.

Abstract

Nuclei from rat ventral prostate were disrupted by sonication and treated with micrococcal nuclease to precipitate nuclear proteins including the androgen receptor. The precipitate was dissolved in 0.6--1.2 M ammonium bicarbonate buffer, pH 7.6, with no loss of receptor when compared to the conventional Tes buffer, pH 7.0 containing 0.6--1.2 M NaCl. Lyophilisation of the solubilised protein did not produce any qualitative or quantitative differences in the recovery of receptor relative to a non-lyophilised control preparation, both of which were analysed for binding properties by Sephadex G-25/G-100 dual-column chromatography. Over longer periods of storage at -80 degrees C, the rate of inactivation of receptor was found to be 6% per week. The stability of the lyophilised receptor was improved by the inclusion of MgCl2 and SH-reducing agents in the ammonium bicarbonate buffer. Recovery improved also with increasing ionic strength of the buffer used to dissolve the lyophilised receptor.

摘要

大鼠腹侧前列腺的细胞核经超声破碎后,用微球菌核酸酶处理,以沉淀包括雄激素受体在内的核蛋白。将沉淀物溶解于pH 7.6的0.6 - 1.2 M碳酸氢铵缓冲液中,与含有0.6 - 1.2 M NaCl、pH 7.0的传统Tes缓冲液相比,受体没有损失。相对于未冻干的对照制剂,冻干溶解后的蛋白质在受体回收率上未产生任何定性或定量差异,二者均通过Sephadex G - 25/G - 100双柱色谱法分析结合特性。在-80℃下储存较长时间后,发现受体的失活速率为每周6%。通过在碳酸氢铵缓冲液中加入MgCl2和SH还原剂,冻干受体的稳定性得到改善。用于溶解冻干受体的缓冲液离子强度增加,回收率也有所提高。

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