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在蛋白质上添加糖基磷脂酰肌醇过程中形成的活性羰基是转酰胺酶催化作用的证据。

An active carbonyl formed during glycosylphosphatidylinositol addition to a protein is evidence of catalysis by a transamidase.

作者信息

Maxwell S E, Ramalingam S, Gerber L D, Brink L, Udenfriend S

机构信息

Roche Institute of Molecular Biology, Roche Research Center, Nutley, New Jersey 07110-1199, USA.

出版信息

J Biol Chem. 1995 Aug 18;270(33):19576-82. doi: 10.1074/jbc.270.33.19576.

Abstract

Glycosylphosphatidylinositol (GPI) substitution is now recognized to be a ubiquitous method of anchoring a protein to membranes in eukaryotes. The structure of GPI and its biosynthetic pathways are known and the signals in a nascent protein for GPI addition have been elucidated. The enzyme(s) responsible for GPI addition with release of a COOH-terminal signal peptide has been considered to be a transamidase but has yet to be isolated, and evidence that it is a transamidase is indirect. The experiments reported here show that hydrazine and hydroxylamine, in the presence of rough microsomal membranes, catalyze the conversion of the pro form of the engineered protein miniplacental alkaline phosphatase (prominiPLAP) to mature forms from which the COOH-terminal signal peptide has been cleaved, apparently at the same site but without the addition of GPI. The products, presumable the hydrazide or hydroxamate of miniPLAP, have yet to be characterized definitively. However, our demonstration of enzyme-catalyzed cleavage of the signal peptide in the presence of the small nucleophiles, even in the absence of an energy source, is evidence of an activated carbonyl intermediate which is the hallmark of a transamidase.

摘要

糖基磷脂酰肌醇(GPI)取代现已被认为是真核生物中一种普遍存在的将蛋白质锚定到膜上的方法。GPI的结构及其生物合成途径已为人所知,并且新生蛋白质中用于添加GPI的信号也已阐明。负责添加GPI并释放COOH末端信号肽的酶被认为是一种转酰胺酶,但尚未分离出来,而且其作为转酰胺酶的证据是间接的。此处报道的实验表明,在糙面微粒体膜存在的情况下,肼和羟胺催化工程化蛋白微型胎盘碱性磷酸酶(pro-miniPLAP)的前体形式转化为成熟形式,其中COOH末端信号肽已被切割,显然是在同一位置,但未添加GPI。产物,可能是miniPLAP的酰肼或异羟肟酸,尚未得到明确表征。然而,我们证明即使在没有能量来源的情况下,在小分子亲核试剂存在时酶催化信号肽的切割,这是转酰胺酶标志性的活性羰基中间体的证据。

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