Spectrofluorometric Assays of Human Collagenase Activity Using Native Collagen and Acetyl-Peptide Substrates

酶研究进展(英文) Pub Date : 2015-03-02 DOI:10.4236/AER.2015.31003

Valon Ejupi, Shpend Dragusha, T. Kabashima, Qinchang Zhu, A. EL-Mahdy, Sheng Yin, T. Shibata, M. Kai

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引用次数: 1

Abstract

A selective, sensitive, and convenient assay for human collagenase is required because of its implication in diseases such as rheumatoid arthritis, osteoarthritis, and tumors. Here, a novel assay for human collagenase activity is described in which enzymatic degradation of native collagen or acetyl peptide is determined by using a fluorogenic reaction for oligopeptides. The oligopeptides are quantified spectrofluorometrically with either 3,4-dihydroxyphenylacetic acid or 1,2-dihydroxybenzen reaction in the presence of sodium periodate and sodium borate (pH 7 - 8). These reactions can selectively convert N-terminal Gly-containing oligopeptides and N-terminal Ile-containing oligopeptides to fluorescence (FL) compounds, respectively, but not proteins, acetyl peptides or amino acids. Under optimized conditions using 1.65 μM collagen IV or 1.5 mM Ac-GPQGI- AGQ as substrates, this assay exhibits a proportional relationship between FL intensities and human collagenase-3 (MMP-13) concentrations. It can assay endogenous collagenase activities in several biological samples, such as cultured human cells and cheek tissue.

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用天然胶原和乙酰肽底物测定人胶原酶活性的荧光光谱法

由于胶原酶与类风湿关节炎、骨关节炎和肿瘤等疾病有关，因此需要一种选择性、敏感和方便的测定方法。在这里，一种新的测定人类胶原酶活性的方法被描述，其中天然胶原蛋白或乙酰肽的酶降解是通过对寡肽的荧光反应来确定的。用3,4-二羟基苯基乙酸或1,2-二羟基苯在高碘酸钠和硼酸钠(pH 7 - 8)存在下的反应对寡肽进行荧光定量。这些反应可以选择性地将n端含甘氨酸寡肽和n端含甘氨酸寡肽分别转化为荧光(FL)化合物，但不能将蛋白质、乙酰肽或氨基酸转化为荧光(FL)化合物。在以1.65 μM胶原IV或1.5 mM Ac-GPQGI- AGQ为底物的优化条件下，该实验显示FL强度与人胶原酶-3 (MMP-13)浓度成正比关系。它可以测定几种生物样品中的内源性胶原酶活性，如培养的人类细胞和脸颊组织。

本文章由计算机程序翻译，如有差异，请以英文原文为准。

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酶研究进展(英文)

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