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细菌视紫红质的结构-功能研究。II. 细菌视蛋白基因在大肠杆菌中的表达优化。

Structure-function studies on bacteriorhodopsin. II. Improved expression of the bacterio-opsin gene in Escherichia coli.

作者信息

Karnik S S, Nassal M, Doi T, Jay E, Sgaramella V, Khorana H G

出版信息

J Biol Chem. 1987 Jul 5;262(19):9255-63.

PMID:3298253
Abstract

The aims of this work have been to express bacterio-opsin with minimal variation from the native primary structure and to improve the level of expression in Escherichia coli. We describe the construction of plasmids in which the bacterio-opsin gene contains only an additional methionine residue at the N terminus and in which the C-terminal aspartic acid encoded in the gene has been deleted to conform to the mature protein. In attempts to improve bacterio-opsin expression, a variety of expression plasmids were constructed in which the promoters and the ribosome-binding sequences were varied. Invariably, in these plasmids, translation but not transcription of the bacterio-opsin gene was limiting. A striking increase in expression of the gene occurred when the codons for several of the N-terminal amino acids were changed to increase the A = T content. Bacterio-opsin expressed in E. coli was degraded with a half-life of 8-10 min. The addition of hydrophobic signal sequences at the N terminus increased the half-life and overall yield of the protein. Bacterio-opsin thus produced regenerated the native bacteriorhodopsin-like chromophore and carried out light-dependent proton translocation at a rate comparable to that of the native bacterio-opsin prepared from the purple membrane.

摘要

这项工作的目标是表达与天然一级结构差异最小的细菌视紫红质,并提高其在大肠杆菌中的表达水平。我们描述了质粒的构建,其中细菌视紫红质基因在N端仅含有一个额外的甲硫氨酸残基,并且为了符合成熟蛋白,基因中编码的C端天冬氨酸已被删除。为了提高细菌视紫红质的表达,构建了多种表达质粒,其中启动子和核糖体结合序列各不相同。在这些质粒中,细菌视紫红质基因的翻译而非转录总是受到限制。当几个N端氨基酸的密码子被改变以增加A=T含量时,该基因的表达显著增加。在大肠杆菌中表达的细菌视紫红质以8-10分钟的半衰期降解。在N端添加疏水信号序列增加了蛋白质的半衰期和总产量。由此产生的细菌视紫红质再生了天然细菌视紫红质样发色团,并以与从紫膜制备的天然细菌视紫红质相当的速率进行光依赖性质子转运。

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