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黑曲霉胞外蛋白酶缺陷型突变体的分离与鉴定

Isolation and characterization of mutants of Aspergillus niger deficient in extracellular proteases.

作者信息

Mattern I E, van Noort J M, van den Berg P, Archer D B, Roberts I N, van den Hondel C A

机构信息

TNO Medical Biological Laboratory, Rijswijk, The Netherlands.

出版信息

Mol Gen Genet. 1992 Aug;234(2):332-6. doi: 10.1007/BF00283855.

DOI:10.1007/BF00283855
PMID:1508158
Abstract

In the present study, the extracellular protease activity in a strain of the filamentous fungus Aspergillus niger was investigated and mutant strains deficient in the production of extracellular proteases were isolated. The major protease, which is responsible for 80-85% of the total activity, is aspergillopepsin A, a protein of ca. 43 kDa, the activity of which is inhibited by pepstatin. In addition, a second protease, aspergillopepsin B, is produced, which is much less sensitive to inhibition by pepstatin. Several protease-deficient mutants were obtained by in vivo UV mutagenesis. In addition, a mutant lacking aspergillopepsin A was constructed by an in vitro gene replacement strategy. In this mutant, AB1.1, the entire coding region of the gene for aspergillopepsin A (pepA) is deleted. In three UV-induced mutants, aspergillopepsin A is also missing. One of these mutants, AB1.18, is mutated in the pepA gene, which is located on chromosome I. One of the other mutants, AB1.13, which has only 1-2% of the extracellular protease activity in the parent strain, is deficient in both aspergillopepsin A and aspergillopepsin B. The mutation involved, prt-13, has been localized to chromosome VI, and is probably a mutation in a regulatory gene. Another mutation involved in loss of protease function, prt-39, is located on chromosome VIII. Degradation of various heterologous proteins in culture media of the mutants is reduced but, even in strain AB1.13, not completely abolished.

摘要

在本研究中,对丝状真菌黑曲霉的一个菌株中的胞外蛋白酶活性进行了研究,并分离出了缺乏胞外蛋白酶产生能力的突变菌株。主要的蛋白酶是曲霉胃蛋白酶A,它占总活性的80 - 85%,是一种约43 kDa的蛋白质,其活性被胃蛋白酶抑制剂抑制。此外,还产生了第二种蛋白酶曲霉胃蛋白酶B,它对胃蛋白酶抑制剂的抑制作用不太敏感。通过体内紫外线诱变获得了几个蛋白酶缺陷型突变体。此外,通过体外基因替换策略构建了一个缺乏曲霉胃蛋白酶A的突变体。在这个突变体AB1.1中,曲霉胃蛋白酶A(pepA)基因的整个编码区被删除。在三个紫外线诱导的突变体中,曲霉胃蛋白酶A也缺失。其中一个突变体AB1.18,其pepA基因发生了突变,该基因位于染色体I上。另一个突变体AB1.13,其胞外蛋白酶活性仅为亲本菌株的1 - 2%,同时缺乏曲霉胃蛋白酶A和曲霉胃蛋白酶B。所涉及的突变prt - 13已定位到染色体VI上,可能是一个调控基因的突变。另一个与蛋白酶功能丧失有关的突变prt - 39位于染色体VIII上。突变体培养基中各种异源蛋白质的降解减少了,但即使在菌株AB1.13中,也没有完全消除。

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