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米曲霉中脯氨酰二肽基肽酶基因(dppIV)的特性分析

Characterization of the prolyl dipeptidyl peptidase gene (dppIV) from the koji mold Aspergillus oryzae.

作者信息

Doumas A, van den Broek P, Affolter M, Monod M

机构信息

Nestlé Research Center, 1000 Lausanne 26, Switzerland.

出版信息

Appl Environ Microbiol. 1998 Dec;64(12):4809-15. doi: 10.1128/AEM.64.12.4809-4815.1998.

Abstract

The koji mold Aspergillus oryzae secretes a prolyl dipeptidyl peptidase (DPPIV) when the fungus is cultivated in a medium containing wheat gluten as the sole nitrogen and carbon source (MMWG). We cloned and sequenced the DPPIV gene from an A. oryzae library by using the A. fumigatus dppIV gene as a probe. Reverse transcriptase PCR experiments showed that the A. oryzae dppIV gene consists of two exons, the first of which is only 6 bp long. The gene encodes an 87.2-kDa polypeptide chain which is secreted into the medium as a 95-kDa glycoprotein. Introduction of this gene into A. oryzae leads to overexpression of prolyl dipeptidyl peptidase activity, while disruption of the gene abolishes all prolyl dipeptidyl peptidase activity in MMWG. The dppIV null mutants did not exhibit any change in phenotype other than the absence of prolyl dipeptidyl peptidase activity, suggesting that this activity is not essential. This loss of activity diminished the number of dipeptides and increased the number of larger peptides present in the MMWG culture broth. These effects were reversed by the addition of purified, recombinant DPPIV from the methylotrophic yeast expression vector Pichia pastoris. Our results suggest that the DPPIV enzyme may be of importance in industrial hydrolysis of what gluten-based substrates, which are rich in Pro residues.

摘要

当米曲霉在以小麦面筋作为唯一氮源和碳源的培养基(MMWG)中培养时,该霉菌会分泌一种脯氨酰二肽基肽酶(DPPIV)。我们以烟曲霉的dppIV基因作为探针,从米曲霉文库中克隆并测序了DPPIV基因。逆转录酶PCR实验表明,米曲霉的dppIV基因由两个外显子组成,其中第一个外显子仅6个碱基对长。该基因编码一条87.2 kDa的多肽链,它作为一种95 kDa的糖蛋白分泌到培养基中。将该基因导入米曲霉会导致脯氨酰二肽基肽酶活性的过表达,而该基因的破坏则会消除MMWG中的所有脯氨酰二肽基肽酶活性。dppIV基因敲除突变体除了缺乏脯氨酰二肽基肽酶活性外,没有表现出任何表型变化,这表明该活性并非必需。这种活性的丧失减少了MMWG培养液中二肽的数量,并增加了较大肽的数量。通过添加来自甲基营养酵母表达载体毕赤酵母的纯化重组DPPIV,这些影响得以逆转。我们的结果表明,DPPIV酶可能在富含Pro残基的小麦面筋基底物的工业水解中具有重要作用。

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