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一种用于内皮素转化酶的荧光检测法。

A fluorogenic assay for endothelin-converting enzyme.

作者信息

von Geldern T W, Holleman W H, Opgenorth T J

机构信息

Cardiovascular Research Division, Abbott Laboratories, Abbott Park, IL 60064.

出版信息

Pept Res. 1991 Jan-Feb;4(1):32-5.

PMID:1802235
Abstract

The potent vasoconstrictor peptide endothelin-1 is proposed to arise via proteolysis of a precursor molecule, "big endothelin," at a unique cleavage site. To aid in the identification of a putative endothelin-converting enzyme, we have developed an assay that mimics the relevant cleavage reaction. The assay takes advantage of the intramolecular fluorescence energy transfer between the scissile-site tryptophan and a dansyl moiety present in the same synthetic substrate. Cleavage of the peptide chain separates the fluorophore and quencher, resulting in an increase in fluorescence. The assay has been validated using chymotrypsin as a model protease and has been employed in the identification of novel endothelin-converting enzyme activities.

摘要

强效血管收缩肽内皮素-1被认为是通过前体分子“大内皮素”在一个独特的切割位点进行蛋白水解而产生的。为了帮助鉴定一种假定的内皮素转化酶,我们开发了一种模拟相关切割反应的检测方法。该检测方法利用了在同一种合成底物中存在的可切割位点色氨酸与丹磺酰部分之间的分子内荧光能量转移。肽链的切割使荧光团和猝灭剂分离,导致荧光增强。该检测方法已使用胰凝乳蛋白酶作为模型蛋白酶进行了验证,并已用于鉴定新型内皮素转化酶活性。

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