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过表达含有一个半胱氨酸的 Rhodanese PspE 可使缺乏 DsbA 的大肠杆菌菌株恢复二硫键形成。

Overexpression of the rhodanese PspE, a single cysteine-containing protein, restores disulphide bond formation to an Escherichia coli strain lacking DsbA.

机构信息

Department of Microbiology and Immunobiology, Harvard Medical School, Boston, MA 02115, USA.

出版信息

Mol Microbiol. 2012 Sep;85(5):996-1006. doi: 10.1111/j.1365-2958.2012.08157.x. Epub 2012 Jul 19.

Abstract

Escherichia coli uses the DsbA/DsbB system for introducing disulphide bonds into proteins in the cell envelope. Deleting either dsbA or dsbB or both reduces disulphide bond formation but does not entirely eliminate it. Whether such background disulphide bond forming activity is enzyme-catalysed is not known. To identify possible cellular factors that might contribute to the background activity, we studied the effects of overexpressing endogenous proteins on disulphide bond formation in the periplasm. We find that overexpressing PspE, a periplasmic rhodanese, partially restores substantial disulphide bond formation to a dsbA strain. This activity depends on DsbC, the bacterial disulphide bond isomerase, but not on DsbB. We show that overexpressed PspE is oxidized to the sulphenic acid form and reacts with substrate proteins to form mixed disulphide adducts. DsbC either prevents the formation of these mixed disulphides or resolves these adducts subsequently. In the process, DsbC itself gets oxidized and proceeds to catalyse disulphide bond formation. Although this PspE/DsbC system is not responsible for the background disulphide bond forming activity, we suggest that it might be utilized in other organisms lacking the DsbA/DsbB system.

摘要

大肠杆菌使用 DsbA/DsbB 系统将二硫键引入细胞包膜中的蛋白质中。删除 dsbA 或 dsbB 或两者都会减少二硫键的形成,但不会完全消除。这种背景中二硫键形成活性是否是酶催化的尚不清楚。为了确定可能有助于背景活性的细胞因子,我们研究了过表达内源性蛋白对周质中二硫键形成的影响。我们发现,过表达周质中的 rhodanese PspE 可部分恢复 dsbA 菌株中大量的二硫键形成。这种活性依赖于细菌二硫键异构酶 DsbC,但不依赖于 DsbB。我们表明,过表达的 PspE 被氧化为亚磺酸形式,并与底物蛋白反应形成混合二硫键加合物。DsbC 要么阻止这些混合二硫键的形成,要么随后将这些加合物解析。在此过程中,DsbC 本身被氧化并继续催化二硫键形成。尽管这个 PspE/DsbC 系统不是背景中二硫键形成活性的原因,但我们认为它可能在其他缺乏 DsbA/DsbB 系统的生物体中被利用。

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