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用于凝乳酶和胃蛋白酶检测的合成肽:pH 效应及混合物中胃蛋白酶的独立测定

Synthetic peptides for chymosin and pepsin assays: pH effect and pepsin independent-determination in mixtures.

作者信息

Salesse R, Garnier J

出版信息

J Dairy Sci. 1976 Jul;59(7):1215-21. doi: 10.3168/jds.S0022-0302(76)84349-4.

Abstract

Peptide I [H-Phe-Gly-His-Phe(NO2)-Phe-Ala-Phe-OMe] hydrolyzed by chymosin with kcat=.3+/-.3 s-1 and KM=7+/-3 mM (pH 4.7) inhibited competitively peptide II [H-Leu-Ser-Phe(NO2)-Nle-Ala-Leu-OMe] hydrolysis by chymosin with KI=.23 +/- .12 mM at pH 4.7. In reference conditions (.4 mM peptide, .01 M acetate buffer pH 4.7), the specific activities of porcine pepsin and chymosin on peptide I were 470 +/- 70 nM S-1 and .8 nM S-1 per mg of enzyme. This difference in specific activity for peptide I allowed development of a chymosin-independent pepsin assay for mixtures of these enzymes. In addition, peptide II with a specific activity of 2400 +/- 300 nM S-1 and 154 +/- 20 nM S-1 per mg of porcine pepsin and chymosin provides an alternative to measurement of milk clotting for measurement of chymosin- and pepsin-like activities in commercial rennets. Hydrolysis products of peptide II by chymosin exhibited one ionized group of apparent pK of 3.5 +/- .2 and a molar absorption coefficient change of 1000 +/- 100 at pH 4.7 and at 310 nm. From measurements of the kinetic constants, kcat and KM, from pH 2.5 to 7 with peptide II, chymosin activity depends on the protonation of one group of apparent pK 5.3 +/- .2 in the free enzyme. Rennet powder proved to be fairly stable after a 17-month storage at 4 C. Within the same period, a crystalline chymosin solution kept at --18 C lost 30 to 50% of its activity.

摘要

肽I [H-苯丙氨酸-甘氨酸-组氨酸-对硝基苯丙氨酸-苯丙氨酸-丙氨酸-苯丙氨酸-甲氧基]在pH 4.7条件下被凝乳酶水解,催化常数kcat = 0.3±0.3 s-1,米氏常数KM = 7±3 mM,它在pH 4.7时竞争性抑制肽II [H-亮氨酸-丝氨酸-对硝基苯丙氨酸-正亮氨酸-丙氨酸-亮氨酸-甲氧基]被凝乳酶水解,抑制常数KI = 0.23±0.12 mM。在参考条件下(0.4 mM肽,0.01 M pH 4.7的乙酸盐缓冲液),猪胃蛋白酶和凝乳酶对肽I的比活性分别为每毫克酶470±70 nM s-1和0.8 nM s-1。肽I比活性的这种差异使得能够开发一种用于这些酶混合物的不依赖凝乳酶检测胃蛋白酶的方法。此外,肽II对猪胃蛋白酶和凝乳酶的比活性分别为每毫克2400±

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