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黄曲霉中丝氨酸蛋白酶基因(sep)的破坏导致金属蛋白酶基因(mep20)表达的代偿性增加。

Disruption of the serine proteinase gene (sep) in Aspergillus flavus leads to a compensatory increase in the expression of a metalloproteinase gene (mep20).

作者信息

Ramesh M V, Kolattukudy P E

机构信息

Neurobiotechnology Center, Ohio State University, Columbus, Ohio 43210, USA.

出版信息

J Bacteriol. 1996 Jul;178(13):3899-907. doi: 10.1128/jb.178.13.3899-3907.1996.

DOI:10.1128/jb.178.13.3899-3907.1996
PMID:8682796
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC232652/
Abstract

The serine proteinase gene (sep) in Aspergillus flavus was disrupted by homologous recombination with a hygromycin resistance gene as the marker. The gene-disrupted mutant GR-2 contained a single-copy insertion of the marker gene and did not express the sep gene. Serine proteinase activity, 36-kDa protein labeled by 3H-diisopropylfluorophosphate, and immunologically detectable proteinase were not detected in the culture fluid of GR-2. Despite the absence of the serine proteinase, the total elastinolytic activity levels in the mutant and the wild-type A.flavus were comparable. Immunoblots revealed that the mutant secreted greater amounts of an elastinolytic metalloproteinase gene (mep20) product than did the wild type. Furthermore, mep20 mRNA levels, measured by RNase protection assay, in the mutant were higher than those in the wild type. Inhibition of the serine proteinase by Streptomyces subtilisin inhibitor (SSI) in the culture medium of wild-type A.flavus also resulted in an elevation of mep20 gene products. Although no serine proteinase activity could be detected, the level of elastinolytic activity of the SSI-treated culture was comparable to that of the control. Immunoblots revealed that the addition of SSI caused an elevation in the levels of metalloproteinase and its mRNA. These results suggest that the expression of the genes encoding serine and metalloproteinases are controlled by a common regulatory system and the fungus has a mechanism to sense the status of extracellular proteolytic activities.

摘要

用潮霉素抗性基因作为标记,通过同源重组破坏了黄曲霉中的丝氨酸蛋白酶基因(sep)。基因破坏突变体GR-2含有标记基因的单拷贝插入,且不表达sep基因。在GR-2的培养液中未检测到丝氨酸蛋白酶活性、经3H-二异丙基氟磷酸标记的36-kDa蛋白以及免疫可检测的蛋白酶。尽管不存在丝氨酸蛋白酶,但突变体和野生型黄曲霉中的总弹性蛋白酶活性水平相当。免疫印迹显示,突变体分泌的弹性蛋白酶金属蛋白酶基因(mep20)产物比野生型多。此外,通过核糖核酸酶保护试验测量,突变体中的mep20 mRNA水平高于野生型。在野生型黄曲霉的培养基中用枯草芽孢杆菌蛋白酶抑制剂(SSI)抑制丝氨酸蛋白酶,也导致mep20基因产物增加。尽管未检测到丝氨酸蛋白酶活性,但SSI处理的培养液的弹性蛋白酶活性水平与对照相当。免疫印迹显示,添加SSI导致金属蛋白酶及其mRNA水平升高。这些结果表明,编码丝氨酸蛋白酶和金属蛋白酶的基因表达受一个共同的调节系统控制,并且该真菌有一种机制来感知细胞外蛋白水解活性的状态。

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本文引用的文献

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Erwinia chrysanthemi EC16 Produces a Second Set of Plant-Inducible Pectate Lyase Isozymes.菊欧文氏菌 EC16 产生第二组植物诱导性果胶裂解酶同工酶。
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