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褶皱链霉菌几丁质酶(几丁质酶-63)在大肠杆菌中的克隆与表达。

Cloning and expression of a Streptomyces plicatus chitinase (chitinase-63) in Escherichia coli.

作者信息

Robbins P W, Albright C, Benfield B

机构信息

Center for Cancer Research, Massachusetts Institute of Technology, Cambridge 02139.

出版信息

J Biol Chem. 1988 Jan 5;263(1):443-7.

PMID:3275646
Abstract

4-Methylumbelliferyl (4-MU) glycosides of N-acetylglucosamine oligosaccharides were used as substrates to detect expression of a Streptomyces chitinase in Escherichia coli. Low levels of enzyme were detected when S. plicatus DNA was cloned into a bacteriophage lambda vector (EMBL-4). Subcloning into E. coli plasmids also gave low but detectable levels of enzyme expression. High level expression was achieved by resection of the cloned S. plicatus DNA with Bal31 followed by in-frame fusion to the amino-terminal peptide sequence of beta-galactosidase found in the pUC vectors. The Streptomyces chitinase was secreted into the periplasmic space of E. coli, and its signal sequence was removed. We characterized the activity of the cloned enzyme and compared it to three other purified Streptomyces plicatus chitinases with respect to hydrolysis of the 4-MU oligosaccharides. We found that two of the enzymes form 4-methylumbelliferone much more rapidly from the 4-MU disaccharide than from the trisaccharide. These same enzymes convert the 4-MU trisaccharide primarily to diacetylchitobiose and the 4-MU monosaccharide, a nonfluorescent product. The latter compound is not hydrolyzed appreciably by any of the enzymes. On the basis of these results, we suggest a new definition of "exo" and "endo" chitinase that differs from that found in the literature. We propose that exochitinase activity be defined as processive action starting at the nonreducing ends of chitin chains with release of successive diacetylchitobiose units, and that endochitinase activity be defined as random cleavage at internal points in chitin chains.

摘要

以N - 乙酰葡糖胺寡糖的4 - 甲基伞形酮基(4 - MU)糖苷为底物,检测链霉菌几丁质酶在大肠杆菌中的表达。当将褶皱链霉菌DNA克隆到噬菌体λ载体(EMBL - 4)中时,检测到低水平的酶。亚克隆到大肠杆菌质粒中也产生了低但可检测水平的酶表达。通过用Bal31切除克隆的褶皱链霉菌DNA,然后与pUC载体中发现的β - 半乳糖苷酶的氨基末端肽序列进行读码框融合,实现了高水平表达。链霉菌几丁质酶分泌到大肠杆菌的周质空间中,并且其信号序列被去除。我们对克隆酶的活性进行了表征,并将其与其他三种纯化的褶皱链霉菌几丁质酶在水解4 - MU寡糖方面进行了比较。我们发现其中两种酶从4 - MU二糖形成4 - 甲基伞形酮的速度比从三糖快得多。这些相同的酶主要将4 - MU三糖转化为二乙酰壳二糖和4 - MU单糖,后者是一种无荧光的产物。任何一种酶都不会明显水解后一种化合物。基于这些结果,我们提出了一种与文献中不同的“外切”和“内切”几丁质酶的新定义。我们建议将外切几丁质酶活性定义为从几丁质链的非还原端开始的连续作用,释放连续的二乙酰壳二糖单元,而内切几丁质酶活性定义为在几丁质链内部点的随机切割。

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