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一种用于脊椎动物胶原酶的便捷荧光检测方法。

A convenient fluorescent assay for vertebrate collagenases.

作者信息

Bond M D, Auld D S, Lobb R R

出版信息

Anal Biochem. 1986 Jun;155(2):315-21. doi: 10.1016/0003-2697(86)90440-9.

Abstract

A versatile, convenient assay for vertebrate collagenases has been developed using the fluorescent peptide substrate dansyl-Pro-Gln-Gly-Ile-Ala-Gly-D-Arg. This sequence resembles that of collagen at the site of cleavage but includes modifications designed to eliminate nonspecific hydrolysis by contaminating peptidases. Both human skin fibroblast and bovine corneal cell collagenases cleave the substrate specifically at the Gly-Ile bond. Plasmin, thrombin, trypsin, alpha-chymotrypsin, carboxypeptidase B, and bacterial collagenase do not cleave the substrate. Elastase and angiotensin converting enzyme display 20- and 400-fold less activity than the vertebrate collagenases, respectively, and cleave the peptide at different positions. The assay is performed by incubating a 5- to 25-microliters aliquot of trypsin-activated sample with an equal volume of 2 mM substrate overnight at 33 degrees C and pH 7.5. Thin-layer chromatography then separates the fluorescent product from the substrate in less than 20 min and allows the detection of subnanogram levels of collagenase. The assay is applicable to the screening of large numbers of samples under different conditions of pH and ionic strength and is readily adaptable for use in a variety of collagenase-dependent systems, such as assays for collagenase activating and/or inducing factors.

摘要

利用荧光肽底物丹磺酰 - 脯氨酸 - 谷氨酰胺 - 甘氨酸 - 异亮氨酸 - 丙氨酸 - 甘氨酸 - D - 精氨酸,开发了一种通用、便捷的脊椎动物胶原酶检测方法。该序列在切割位点类似于胶原蛋白,但包含旨在消除污染性肽酶非特异性水解的修饰。人皮肤成纤维细胞胶原酶和牛角膜细胞胶原酶均特异性地在甘氨酸 - 异亮氨酸键处切割底物。纤溶酶、凝血酶、胰蛋白酶、α - 糜蛋白酶、羧肽酶B和细菌胶原酶均不切割该底物。弹性蛋白酶和血管紧张素转换酶的活性分别比脊椎动物胶原酶低20倍和400倍,且在不同位置切割该肽段。检测方法是将5至25微升经胰蛋白酶激活的样品等分试样与等体积的2 mM底物在33℃和pH 7.5下孵育过夜。然后,薄层色谱法在不到20分钟的时间内将荧光产物与底物分离,并可检测到亚纳克水平的胶原酶。该检测方法适用于在不同pH和离子强度条件下对大量样品进行筛选,并且易于适用于各种依赖胶原酶的系统,例如胶原酶激活和/或诱导因子的检测。

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