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腺体激肽释放酶通过切割唾液蛋白C中的单键在富含脯氨酸的唾液蛋白A形成过程中的作用。

The role of glandular kallikrein in the formation of a salivary proline-rich protein A by cleavage of a single bond in salivary protein C.

作者信息

Wong R S, Madapallimattam G, Bennick A

出版信息

Biochem J. 1983 Apr 1;211(1):35-44. doi: 10.1042/bj2110035.

Abstract

An enzyme was purified from human parotid saliva that can cleave a single arginine-glycine peptide bond between residues 106 and 107 in human salivary proline-rich protein C, hereby giving rise to another proline-rich protein A, which is also found in saliva. The enzyme was purified 2400-fold. It cleaved salivary protein C at the rate of 59 micrograms of protein/h per microgram of enzyme and had amino acid composition, molecular weight and inhibition characteristics similar to those reported for human salivary kallikrein. Confirmation that the enzyme was kallikrein was demonstrated by its kinin-generating ability. Histochemical evidence indicates that a post-synthetic cleavage of protein C by kallikrein would have to take place during passage of saliva through the secretory ducts. In secreted saliva, cleavage of salivary protein C can only be observed after 72 h incubation. In addition, there is no effect of salivary flow rate on the relative amounts of proteins A and C in saliva. On the basis of the experimental observations, it is proposed that in vivo it is unlikely that kallikrein secreted from ductal cells plays a significant role in converting protein C into protein A.

摘要

从人腮腺唾液中纯化出一种酶,它能切割人唾液富含脯氨酸蛋白C中第106和107位残基之间的单个精氨酸 - 甘氨酸肽键,从而产生另一种富含脯氨酸的蛋白A,这种蛋白也存在于唾液中。该酶被纯化了2400倍。它以每微克酶每小时59微克蛋白质的速率切割唾液蛋白C,其氨基酸组成、分子量和抑制特性与报道的人唾液激肽释放酶相似。该酶产生激肽的能力证实了它是激肽释放酶。组织化学证据表明,唾液通过分泌导管时,激肽释放酶对蛋白C的合成后切割必定会发生。在分泌的唾液中,只有在孵育72小时后才能观察到唾液蛋白C的切割。此外,唾液流速对唾液中蛋白A和蛋白C的相对含量没有影响。基于实验观察结果,有人提出在体内,导管细胞分泌的激肽释放酶不太可能在将蛋白C转化为蛋白A的过程中发挥重要作用。

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