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使用可裂解交联试剂鉴定大肠杆菌30S核糖体亚基中的相邻蛋白质。

The use of a cleavable crosslinking reagent to identify neighboring proteins in the 30-S ribosomal subunit of Escherichia coli.

作者信息

Peretz H, Towbin H, Elson D

出版信息

Eur J Biochem. 1976 Mar 16;63(1):83-92. doi: 10.1111/j.1432-1033.1976.tb10210.x.

Abstract

A cleavable bifunctional reagent, dimethyl 3,3'-dithiobispropionimidate, has been used to crosslink proteins that occupy neighboring positions in the 30-S ribosomal subunit of Escherichia coli. The crosslinked proteins were identified, fully or partly, by their positions in two two-dimensional gel electrophoretic systems, one diagonal and the other quasi-diagonal, in which the complexes were cleaved after the first-dimensional run. It was found to be necessary to block the protein sulfhydryl groups in order to prevent artifactual disulfide crosslinking after extraction of the protein from ribosome. Eleven crosslinked complexes were detected. Four were fully identified: the triplet S4-S5-S8, and the pairs S2-S3, S4-S5, and S5-S8. In five others one component was identified unambiguously. No additional complexes were seen when the longer homologous butyro and capro reagents were used.

摘要

一种可裂解的双功能试剂,3,3'-二硫代双丙酰亚胺二甲酯,已被用于交联在大肠杆菌30-S核糖体亚基中占据相邻位置的蛋白质。通过交联蛋白质在两种二维凝胶电泳系统中的位置,对其进行了全部或部分鉴定,一种是对角线系统,另一种是准对角线系统,其中复合物在一维电泳后被裂解。发现有必要封闭蛋白质的巯基,以防止从核糖体中提取蛋白质后出现人为的二硫键交联。检测到11种交联复合物。其中4种已完全鉴定:三联体S4-S5-S8,以及配对S2-S3、S4-S5和S5-S8。在另外5种复合物中,明确鉴定出了其中一个组分。当使用更长的同源丁酰和己酰试剂时,未观察到其他复合物。

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