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分离乳糖阻遏物与DNA结合所必需的氨基末端片段。

Isolation of amino-terminal fragment of lactose repressor necessary for DNA binding.

作者信息

Geisler N, Weber K

出版信息

Biochemistry. 1977 Mar 8;16(5):938-43. doi: 10.1021/bi00624a020.

Abstract

lac repressor can be dissected by trypsin into a homogenous tetrameric core (accounting for residues 60 to 347), carrying inducer binding activity, and the monomeric amino-terminal peptides ("headpieces") accounting for residues 1 to 59 and 1 to 51, respectively. This restriction of the action of trypsin on lac repressor is obtained in 1 M Tris-HCl (pH 7.5)-30% in glycerol at 25 degrees C since only the peptide bonds at lysine-59 and to a lesser extent after at arginine-51 are cleaved under these conditions. The headpieces can be purified by gel filtration. They have ordered secondary structure as revealed by circular dichroism studies. The monomeric headpieces show the relatively weak binding to nonoperator DNA but not the highly specific and strong binding to operator DNA typical for tetrameric lac repressor.

摘要

乳糖阻遏蛋白可被胰蛋白酶切割成一个具有诱导剂结合活性的同源四聚体核心(由60至347位残基组成),以及分别由1至59位残基和1至51位残基组成的单体氨基末端肽段(“头部”)。在25℃下,于1 M Tris-HCl(pH 7.5)-30%甘油中可实现胰蛋白酶对乳糖阻遏蛋白作用的这种限制,因为在这些条件下,只有赖氨酸-59处的肽键以及程度较小的精氨酸-51之后的肽键会被切割。这些头部肽段可通过凝胶过滤进行纯化。圆二色性研究表明它们具有有序的二级结构。单体头部肽段对非操纵基因DNA显示出相对较弱的结合,但不具有四聚体乳糖阻遏蛋白典型的对操纵基因DNA的高度特异性和强结合。

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