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通过噬菌体溶菌酶和 DNA/RNA 内切酶赋予的自溶和自动 DNA/RNA 水解的双重诱导作用,改进了两阶段蛋白表达和纯化。

Improved two-stage protein expression and purification via autoinduction of both autolysis and auto DNA/RNA hydrolysis conferred by phage lysozyme and DNA/RNA endonuclease.

机构信息

Department of Biomedical Engineering, Duke University, Durham, North Carolina.

Department of Chemistry, Duke University, Durham, North Carolina.

出版信息

Biotechnol Bioeng. 2020 Sep;117(9):2852-2860. doi: 10.1002/bit.27444. Epub 2020 Jun 20.

Abstract

We report improved release of recombinant proteins in Escherichia coli, which relies on combined cellular autolysis and DNA/RNA autohydrolysis, conferred by the tightly controlled autoinduction of both phage lysozyme and the nonspecific DNA/RNA endonuclease from Serratia marcescens. Autoinduction occurs in a two-stage process wherein heterologous protein expression and autolysis enzymes are induced upon entry into stationary phase by phosphate depletion. Cytoplasmic lysozyme and periplasmic endonuclease are kept from inducing lysis until membrane integrity is disrupted. After cell harvest, the addition of detergent (0.1% Triton X-100) and a single 30 min freeze-thaw cycle results in >90% release of protein, green fluorescent protein. This cellular lysis is accompanied by complete oligonucleotide hydrolysis. The approach has been validated for shake flask cultures, high-throughput cultivation in microtiter plates, and larger scale stirred-tank bioreactors. This tightly controlled system enables robust growth and resistance to lysis in routine media when cells are propagated and autolysis/hydrolysis genes are only induced upon phosphate depletion.

摘要

我们报告了一种在大肠杆菌中提高重组蛋白释放效率的方法,该方法依赖于噬菌体溶菌酶和来自粘质沙雷氏菌的非特异性 DNA/RNA 内切酶的紧密控制的自动诱导,从而导致细胞自动裂解和 DNA/RNA 自动水解。自动诱导分两个阶段进行,当进入静止期时通过磷酸盐耗尽诱导异源蛋白表达和自裂解酶。细胞质溶菌酶和周质内切酶在膜完整性被破坏之前不会诱导裂解。细胞收获后,添加洗涤剂(0.1%Triton X-100)并进行一次 30 分钟的冻融循环,可导致超过 90%的蛋白质(绿色荧光蛋白)释放。这种细胞裂解伴随着完整的寡核苷酸水解。该方法已在摇瓶培养、微孔板高通量培养和更大规模的搅拌罐生物反应器中得到验证。当在常规培养基中进行细胞繁殖和仅在磷酸盐耗尽时诱导自裂解/水解基因时,这种紧密控制的系统可实现稳健的生长和对裂解的抗性。

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