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通过物理化学和体外重折叠研究提高活性重组壳二糖酶的产量

Enhancing the Yield of Active Recombinant Chitobiase by Physico-Chemical and In Vitro Refolding Studies.

作者信息

Dangi Arun Kumar, Rishi Praveen, Tewari Rupinder

机构信息

Department of Microbial Biotechnology, Panjab University, Sector 14, Chandigarh, 160014, India.

Department of Microbiology, Panjab University, Chandigarh, India.

出版信息

Protein J. 2016 Feb;35(1):72-9. doi: 10.1007/s10930-016-9648-z.

Abstract

Chitobiase (CHB) is an important enzyme for the production of N-acetyl-D-glucosamine from the chitin biopolymer in the series of chitinolytic enzymes. Majority of over-expressed CHB (58%) in E. coli expression system led to formation of inclusion bodies. The production and soluble yield of active CHB was enhanced by co-expression with GroEL/ES chaperonin, optimizing culture conditions and solubilization followed by refolding of remaining inactive chitobiase present in the form of inclusion bodies. The growth of recombinant E. coli produced 42% CHB in soluble form and the rest (~58%) as inclusion bodies. The percentage of active CHB was enhanced to 71% by co-expression with GroEL/ES chaperonin system and optimizing culture conditions (37 °C, 200 rpm, IPTG--0.5 mM, L-arabinose--13.2 mM). Of the remaining inactive CHB present in inclusion bodies, 37% could be recovered in active form using pulsatile dilution method involving denaturants (2 M urea, pH 12.5) and protein refolding studies (1.0 M L-arginine, 5% glycerol). Using combinatorial approach, 80% of the total CHB expressed, could be recovered from cells grown in one litre of LB medium is a step forward in replacing hazardous chemical technology by biotechnological process for the production of NAG from chitinous waste.

摘要

几丁质酶(CHB)是几丁质分解酶系列中从几丁质生物聚合物生产N-乙酰-D-葡萄糖胺的一种重要酶。在大肠杆菌表达系统中,大多数过表达的CHB(58%)会导致包涵体的形成。通过与GroEL/ES伴侣蛋白共表达、优化培养条件以及对以包涵体形式存在的剩余无活性几丁质酶进行溶解和复性,活性CHB的产量和可溶性产量得到了提高。重组大肠杆菌生长时产生的CHB有42%为可溶形式,其余(约58%)为包涵体。通过与GroEL/ES伴侣蛋白系统共表达并优化培养条件(37℃,200转/分钟,IPTG - 0.5 mM,L-阿拉伯糖 - 13.2 mM),活性CHB的比例提高到了71%。对于包涵体中剩余的无活性CHB,使用涉及变性剂(2 M尿素,pH 12.5)的脉冲稀释法和蛋白质复性研究(1.0 M L-精氨酸,5%甘油),37%可以以活性形式回收。采用组合方法,从在一升LB培养基中生长的细胞中回收了所表达总CHB的80%,这是在利用生物技术工艺从含几丁质废物生产NAG方面取代危险化学技术的一个进步。

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