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通过噬菌体展示实现单链cro的功能表达及亲和力筛选:新型DNA结合蛋白的分离

Functional expression and affinity selection of single-chain cro by phage display: isolation of novel DNA-binding proteins.

作者信息

Nilsson M T, Mossing M C, Widersten M

机构信息

Department of Biochemistry, Uppsala University, Biomedical Center, Box 576, SE-751 23 Uppsala, Sweden.

出版信息

Protein Eng. 2000 Jul;13(7):519-26. doi: 10.1093/protein/13.7.519.

Abstract

A robust selection system affording phage display of the DNA-binding helix-turn-helix protein Cro is presented. The aim of the work was to construct an experimental system allowing for the construction and isolation of Cro-derived protein with new DNA-binding properties. A derivative of the phage lambda Cro repressor, scCro8, in which the protein subunits had been covalently connected via a peptide linker was expressed in fusion with the gene 3 protein of Escherichia coli filamentous phage. The phage-displayed single-chain Cro was shown to retain the DNA binding properties of its wild-type Cro counterpart regarding DNA sequence specificity and binding affinity. A kinetic analysis revealed the rate constant of dissociation of the single-chain Cro-phage/DNA complex to be indistinguishable from that of the free single-chain Cro. Affinity selection using a biotinylated DNA with a target consensus operator sequence allowed for a 3000-fold enrichment of phages displaying single-chain Cro over control phages. The selection was based on entrapment of phage/DNA complexes formed in solution on streptavidin-coated paramagnetic beads. The expression system was subsequently used to isolate variant scCro8 proteins, mutated in their DNA-binding residues, that specifically recognized new, unnatural target DNA ligands.

摘要

本文介绍了一种强大的筛选系统,该系统可实现DNA结合型螺旋-转角-螺旋蛋白Cro的噬菌体展示。这项工作的目的是构建一个实验系统,用于构建和分离具有新DNA结合特性的Cro衍生蛋白。噬菌体λ Cro阻遏物的衍生物scCro8,其中蛋白质亚基通过肽接头共价连接,与大肠杆菌丝状噬菌体的基因3蛋白融合表达。噬菌体展示的单链Cro在DNA序列特异性和结合亲和力方面保留了其野生型Cro对应物的DNA结合特性。动力学分析表明,单链Cro-噬菌体/DNA复合物的解离速率常数与游离单链Cro的解离速率常数没有区别。使用具有目标共有操纵序列的生物素化DNA进行亲和筛选,使得展示单链Cro的噬菌体比对照噬菌体富集了3000倍。该筛选基于溶液中形成的噬菌体/DNA复合物被捕获在链霉亲和素包被的顺磁性珠子上。随后,该表达系统被用于分离在其DNA结合残基处发生突变的变体scCro8蛋白,这些蛋白能够特异性识别新的、非天然的目标DNA配体。

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