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通过亲和层析和光亲和标记法纯化苯并[a]芘结合蛋白

Purification of a benzo[a]pyrene binding protein by affinity chromatography and photoaffinity labeling.

作者信息

Collins S, Marletta M A

出版信息

Biochemistry. 1986 Jul 29;25(15):4322-9. doi: 10.1021/bi00363a022.

Abstract

Binding proteins for the polycyclic aromatic hydrocarbon carcinogen benzo[a]pyrene (B[a]P) have been purified from C57B1/6J mouse liver. Following affinity chromatography on aminopyrene-Sepharose, a single polypeptide of 29,000 daltons was isolated. The photolabile compound 1-azidopyrene was developed as a photoaffinity labeling agent to identify the protein during its purification. 1-Azidopyrene was found to be a competitive inhibitor of [3H]B[a]P binding. Affinity labeling studies with [3H]-1-azidopyrene in unfractionated cytosol, and in purified preparations, yielded a single covalently labeled protein of 29,000 daltons. The formation of this labeled species was blocked by preincubation with excess unlabeled B[a]P. A native molecular weight of 30,000 was estimated by gel filtration chromatography of [3H]B[a]P- and [3H]-1-azidopyrene-labeled cytosol proteins. An equilibrium dissociation constant of 2.69 +/- 0.66 nM and a maximum number of binding sites of 2.07 +/- 0.10 nmol of [3H]B[a]P bound/mg of protein were estimated for the pure protein. Two-dimensional gel electrophoresis further resolved the purified 29,000-dalton protein into three major isoelectric variants, each of which was specifically labeled by [3H]-1-azidopyrene.

摘要

多环芳烃致癌物苯并[a]芘(B[a]P)的结合蛋白已从C57B1/6J小鼠肝脏中纯化出来。在氨基芘-琼脂糖上进行亲和层析后,分离出一种分子量为29,000道尔顿的单一多肽。光不稳定化合物1-叠氮芘被开发为一种光亲和标记剂,用于在纯化过程中鉴定该蛋白。发现1-叠氮芘是[3H]B[a]P结合的竞争性抑制剂。用[3H]-1-叠氮芘在未分级的细胞溶质和纯化制剂中进行亲和标记研究,产生了一种分子量为29,000道尔顿的单一共价标记蛋白。这种标记物的形成可通过与过量未标记的B[a]P预孵育来阻断。通过对[3H]B[a]P和[3H]-1-叠氮芘标记的细胞溶质蛋白进行凝胶过滤层析,估计其天然分子量为30,000。对于纯蛋白,估计其平衡解离常数为2.69±0.66 nM,最大结合位点数为2.07±0.10 nmol [3H]B[a]P结合/mg蛋白。二维凝胶电泳进一步将纯化的29,000道尔顿蛋白解析为三个主要的等电变体,每个变体都被[3H]-1-叠氮芘特异性标记。

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