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通过在原肽 C 端引入连接肽来提高链霉菌转谷氨酰胺酶的活性和原肽的切割效率。

Enhancement of Streptomyces transglutaminase activity and pro-peptide cleavage efficiency by introducing linker peptide in the C-terminus of the pro-peptide.

机构信息

School of Biotechnology, Jiangnan University, 1800 Lihu Road, Wuxi, China.

出版信息

J Ind Microbiol Biotechnol. 2013 Apr;40(3-4):317-25. doi: 10.1007/s10295-012-1221-y. Epub 2013 Jan 24.

Abstract

Streptomyces transglutaminase (TGase) has been widely used in food, pharmaceutical and textile industries. Streptomyces TGase is naturally synthesized as zymogen (pro-TGase), which is then processed to produce active enzyme by removing its N-terminal pro-peptide. Although the pro-peptide is essential for TGase folding and secretion, few studies have been reported on improving the properties of TGase by pro-peptide engineering. In this study, we developed a new approach to improve the properties of TGase based on pro-peptide engineering. When the α-helix(37G-42S) in pro-peptide was substituted with three glycines and three alanines respectively, the mutants exhibited higher specific activity and the efficiency of pro-peptide cleavage was enhanced. To further improve the properties of TGase, relevant mutations were constructed by introducing linker peptides in the C-terminus of the pro-peptide. Mutants with GS (GGGGS) and PT (PTPPTTPT) linker peptide exhibited 1.28 fold and 1.5 fold higher specific activity than the wild-type enzyme, respectively. This new method could be used to improve the properties of TGase by pro-peptide modification, which is a promising technology for creating unique TGase with various beneficial properties.

摘要

链霉菌转谷氨酰胺酶(TGase)已广泛应用于食品、制药和纺织工业。链霉菌 TGase 天然合成时为酶原(前 TGase),然后通过去除其 N 端前肽来加工产生活性酶。尽管前肽对于 TGase 的折叠和分泌是必不可少的,但很少有研究报道通过前肽工程来改善 TGase 的性质。在这项研究中,我们开发了一种基于前肽工程来改善 TGase 性质的新方法。当前肽中的α-螺旋(37G-42S)分别被三个甘氨酸和三个丙氨酸取代时,突变体表现出更高的比活性,并且前肽切割的效率得到增强。为了进一步改善 TGase 的性质,通过在前肽的 C 端引入连接肽构建了相关突变体。具有 GS(GGGGS)和 PT(PTPPTTPT)连接肽的突变体的比活性分别比野生型酶高 1.28 倍和 1.5 倍。这种新方法可用于通过前肽修饰来改善 TGase 的性质,这是一种具有广阔前景的技术,可用于创造具有各种有益性质的独特 TGase。

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