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在低温诱导的对数早期培养物中,有利于在大肠杆菌中生产可溶性真核重组蛋白。

Production of soluble eukaryotic recombinant proteins in E. coli is favoured in early log-phase cultures induced at low temperature.

作者信息

San-Miguel Teresa, Pérez-Bermúdez Pedro, Gavidia Isabel

机构信息

Departamento de Biología Vegetal, Facultad de Farmacia, Universidad de Valencia, Av. VA Estellés s/n, Burjasot, 46100 Spain.

出版信息

Springerplus. 2013 Dec;2(1):89. doi: 10.1186/2193-1801-2-89. Epub 2013 Mar 8.

Abstract

BACKGROUND

Producing recombinant plant proteins expressed in Escherichia coli produce in high yields and in a soluble and functional form can be difficult. Under overexpression conditions, proteins frequently accumulate as insoluble aggregates (inclusion bodies) within the producing bacteria. We evaluated how the initial culture density, temperature and duration of the expression stage affect the production of some eukaryotic enzymes in E. coli.

FINDINGS

A high yield of active soluble proteins was obtained by combining early-log phase cultures and low temperatures for protein induction. When IPTG was added at OD600 = 0.1 and cultures were maintained at 4°C for 48-72 h, the soluble protein yield was 3 fold higher than that obtained in the mid-log phase (OD600 = 0.6). Besides, the target protein expression increased and the endogenous bacterial proteins reduced, thus making the protein purification process easier and more efficient.

CONCLUSIONS

The protocol can be widely applied to proteins with a heterologous expression which was limited by loss of activity at high temperatures or by low soluble recombinant protein yield.

摘要

背景

在大肠杆菌中高产、以可溶且有功能的形式生产重组植物蛋白可能具有挑战性。在过表达条件下,蛋白质经常在生产细菌内以不溶性聚集体(包涵体)的形式积累。我们评估了初始培养密度、温度和表达阶段的持续时间如何影响大肠杆菌中某些真核酶的生产。

研究结果

通过将对数早期培养物与低温用于蛋白质诱导相结合,获得了高产的活性可溶性蛋白。当在OD600 = 0.1时添加IPTG并将培养物在4°C下维持48 - 72小时,可溶性蛋白产量比在对数中期(OD600 = 0.6)获得的产量高3倍。此外,目标蛋白表达增加,内源性细菌蛋白减少,从而使蛋白质纯化过程更轻松、更高效。

结论

该方案可广泛应用于因高温下活性丧失或可溶性重组蛋白产量低而受到限制的异源表达蛋白质。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/8427/3602615/3f9379ce74f1/40064_2012_152_Fig1_HTML.jpg

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