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Transglutaminase activity is involved in Saccharomyces cerevisiae wall construction

机译:转谷氨酰胺酶活性参与酿酒酵母壁墙施工

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Transglutaminase activity, which forms the interpeptidic cross-link N?-(γ-glutamyl)-lysine, was demonstrated in cell-free extracts of Saccharomyces cerevisiae by incorporation of [14C]lysine into an exogenous acceptor, N,N′-dimethylcasein. Higher levels of the activity were present in the cell wall, which also contained endogenous acceptors. The enzyme activity in the wall was inhibited by cystamine, a known inhibitor of transglutaminase, and by EDTA, indicating a cation-dependent activity. After the endogenous wall acceptors were labelled radioactively by transglutaminase, extraction with SDS solubilized about 50% of the total radioactivity, while Zymolyase and chitinase each released a further 3%. The proteins solubilized by SDS had molecular masses less than 50?kDa, whereas the material released by Zymolyase or chitinase had molecular masses greater than 180?kDa, suggesting a precursor–product relationship. Cystamine inhibited the growth of several strains of S. cerevisiae. Treated cells showed increased sensitivity to Zymolyase and appeared as protoplasts, indicating gross alterations in the cell wall. These data suggest that transglutaminase may be involved in the formation of covalent cross-links between wall proteins during wall construction.
机译:通过将[14C]赖氨酸掺入外源受体,N,N'-二甲基壳蛋白,形成形成杂散的交联Nα - (γ-谷氨酸)-LYSINE的转基氨酰胺酶活性。细胞壁中存在较高水平的活性,其也包含内源性受体。壁中的酶活性被胱胺,已知的转谷氨酰胺酶,并通过EDTA抑制,表明依赖于依赖性活性。通过转谷氨酰胺酶放射性地放线地标记后,用SDS溶解的SDS溶解约50%的总放射性,而Zymolate和Chitinase各自释放出3%。通过SDS溶解的蛋白质的分子量小于50Ω·kda,而通过Zymolyase或丁质酶释放的材料的分子量大于180μl≤kda,表明前体 - 产品关系。胱胺抑制了几种酿酒酵母的生长。经处理的细胞显示对Zymolatase的敏感性增加,并出现为原生质体,表明细胞壁中的粗糙变化。这些数据表明转谷氨酰胺酶可以参与在壁构造期间壁蛋白之间的共价交联的形成。

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