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pH、温度和重水对猪滑膜胶原酶和明胶酶活性的影响。

The effect of pH, temperature, and D2O on the activity of porcine synovial collagenase and gelatinase.

作者信息

Stack M S, Gray R D

机构信息

Department of Biochemistry, University of Louisville, Kentucky 40292.

出版信息

Arch Biochem Biophys. 1990 Sep;281(2):257-63. doi: 10.1016/0003-9861(90)90441-z.

DOI:10.1016/0003-9861(90)90441-z
PMID:2168159
Abstract

The pH dependence of Vmax and Vmax/Km for hydrolysis of Dnp-Pro-Leu-Gly-Leu-Trp-Ala-D-Arg-NH2 at the Gly-Leu bond by porcine synovial collagenase and gelatinase was determined in the pH range 5-10. Both enzymes exhibited bell-shaped dependencies on pH for these two kinetic parameters, indicating that activity is dependent on at least two ionizable groups, one of which must be unprotonated and the other protonated. For collagenase, Vmax/Km data indicate that in the substrate-free enzyme, these groups have apparent pK values of 7.0 and 9.5, while the Vmax profile indicates similar pK values of 6.8 and 10.1 for the enzyme-substrate complex. The corresponding pH profiles of gelatinase were similar to those of collagenase, indicating the importance of groups with apparent pK values of 5.9 and 10.0 for the free enzyme and 5.9 and 11.1 for the enzyme-substrate complex. When these kinetic constants were determined in D2O using the peptide substrate, there was no significant effect on Vmax or Km for collagenase or Km for gelatinase. However, there was a deuterium isotope effect of approximately 1.5 on Vmax for gelatinase. These results indicate that a proton transfer step is not involved in the rate-limiting step for collagenase, but may be limiting with gelatinase. The Arrhenius activation energies for peptide bond hydrolysis of the synthetic peptide as well as the natural substrates were also determined for both enzymes. The activation energy (81 kcal) for hydrolysis of collagen by collagenase was nine times greater than that determined for the synthetic substrate (9.2 kcal). In contrast, the activation energy for hydrolysis of gelatin by gelatinase (26.3 kcal) was only 2.4 times greater than that for the synthetic substrate (11 kcal).

摘要

在pH值5 - 10范围内,测定了猪滑膜胶原酶和明胶酶对Dnp - Pro - Leu - Gly - Leu - Trp - Ala - D - Arg - NH₂中Gly - Leu键水解的Vmax和Vmax/Km的pH依赖性。这两种酶对这两个动力学参数均表现出钟形的pH依赖性,表明活性至少依赖于两个可电离基团,其中一个必须未质子化,另一个质子化。对于胶原酶,Vmax/Km数据表明,在无底物的酶中,这些基团的表观pK值为7.0和9.5,而Vmax曲线表明酶 - 底物复合物的类似pK值为6.8和10.1。明胶酶的相应pH曲线与胶原酶相似,表明表观pK值为5.9和10.0的基团对游离酶很重要,而表观pK值为5.9和11.1的基团对酶 - 底物复合物很重要。当使用肽底物在D₂O中测定这些动力学常数时,对胶原酶的Vmax或Km以及明胶酶的Km没有显著影响。然而,明胶酶的Vmax存在约1.5的氘同位素效应。这些结果表明,质子转移步骤不参与胶原酶的限速步骤,但可能是明胶酶的限速步骤。还测定了两种酶对合成肽以及天然底物的肽键水解的阿伦尼乌斯活化能。胶原酶水解胶原的活化能(81千卡)比合成底物(9.2千卡)的活化能大九倍。相比之下,明胶酶水解明胶的活化能(26.3千卡)仅比合成底物(11千卡)的活化能大2.4倍。

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