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支链氨基酸结合蛋白的体外合成与加工

The in vitro synthesis and processing of the branched-chain amino acid binding proteins.

作者信息

Daniels C J, Anderson J J, Landick R, Oxender D L

出版信息

J Supramol Struct. 1980;14(3):305-11. doi: 10.1002/jss.400140305.

Abstract

The synthesis of the leucine-specific and LIV-binding proteins was examined in vitro in a coupled transcription/translation system using the hybrid plasmids pOX7 and pOX13 as templates. Plasmid pOX7 contains the livK gene coding for the leucine-specific binding protein and pOX13 contains the livJ gene coding for the LIV-binding protein. Both binding proteins were synthesized in vitro as precursor forms with molecular weights approximately 2,500 greater than their respective mature forms. Conversion of the precursor forms to their mature forms occurred during post-translational incubation following synthesis in the presence of membrane. The precursor of the LIV-binding protein was processed more rapidly than the leucine-specific binding protein precursor. Processing activity could be removed from the in vitro synthesis system by centrifugation, suggesting that the processing activity was membrane associated. Restoration of post-translational processing activity was achieved by adding inside-out membrane vesicles to membrane-depleted reaction mixtures.

摘要

使用杂交质粒pOX7和pOX13作为模板,在体外偶联转录/翻译系统中检测亮氨酸特异性结合蛋白和LIV结合蛋白的合成。质粒pOX7含有编码亮氨酸特异性结合蛋白的livK基因,pOX13含有编码LIV结合蛋白的livJ基因。两种结合蛋白在体外均以前体形式合成,其分子量比各自的成熟形式大约大2500。在膜存在的情况下合成后,前体形式在翻译后孵育期间转化为成熟形式。LIV结合蛋白的前体比亮氨酸特异性结合蛋白前体加工得更快。加工活性可通过离心从体外合成系统中去除,这表明加工活性与膜相关。通过向耗尽膜的反应混合物中添加内翻膜囊泡,实现了翻译后加工活性的恢复。

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