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蜡蚧轮枝菌几丁质酶的分离与特性分析

Isolation and characterization of chitinases from Verticillium lecanii.

作者信息

Lu Zhen-Xiang, Laroche André, Huang Hung Chang

机构信息

Lethbridge Research Centre, Agriculture and Agri-Food Canada, AB, Canada.

出版信息

Can J Microbiol. 2005 Dec;51(12):1045-55. doi: 10.1139/w05-088.

DOI:10.1139/w05-088
PMID:16462863
Abstract

Degenerate PCR primers corresponding to conserved domains of fungal chitinases were designed, and PCR was performed on genomic DNA of the entomogenous fungus Verticillium lecanii (Zimmermann) Viegas. Two distinct PCR fragments, chf1 and chf2, were isolated and used to identify two DNA contigs. Analyses of these two contigs revealed that we had obtained the full-length DNA sequence including the promoter, 5' untranslated region, open reading frame (ORF), and 3' untranslated regions for two distinct chitinase-like genes. These two genomic DNA sequences exhibited 51% identity at the amino acid (aa) level and were designed as acidic (chi1) and basic (chi2) chitinase-like genes. The isolated cDNA for chi1 gene is 1110 bp with a predicted protein of 370 aa and molecular mass of 40.93 kDa, and its ORF was uninterrupted in its corresponding genomic DNA sequence. The cDNA for the chi2 gene is 1269 bp, a predicted ORF of 423 aa and molecular mass of 45.95 kDa. In contrast, the ORF was interrupted by three introns in its corresponding genomic DNA. The basic chitinase gene (chi2) was successfully expressed in the Pichia pastoris system; optimum enzymatic activity was observed at 22 degrees C and at pH 7.5. CHI1 and CHI2 were clustered into two different phylogenetic groups according to their sequence alignments with 28 other fungal chitinases. A chitin-binding domain, comprising two sub-domains that exhibit similarities at the aa level to chitin binding domains in bacteria, was identified in 30 fungal chitinase sequences examined.

摘要

设计了与真菌几丁质酶保守结构域对应的简并PCR引物,并对昆虫病原真菌蜡蚧轮枝菌(齐默尔曼)维加斯的基因组DNA进行了PCR。分离出两个不同的PCR片段chf1和chf2,并用于鉴定两个DNA重叠群。对这两个重叠群的分析表明,我们获得了两个不同的几丁质酶样基因的全长DNA序列,包括启动子、5'非翻译区、开放阅读框(ORF)和3'非翻译区。这两个基因组DNA序列在氨基酸(aa)水平上具有51%的同一性,并被设计为酸性(chi1)和碱性(chi2)几丁质酶样基因。分离出的chi1基因cDNA为1110 bp,预测蛋白质为370 aa,分子量为40.93 kDa,其ORF在相应的基因组DNA序列中是不间断的。chi2基因的cDNA为1269 bp,预测ORF为423 aa,分子量为45.95 kDa。相比之下,其ORF在相应的基因组DNA中被三个内含子打断。碱性几丁质酶基因(chi2)在毕赤酵母系统中成功表达;在22℃和pH 7.5时观察到最佳酶活性。根据CHI1和CHI2与其他28种真菌几丁质酶的序列比对,它们被聚类到两个不同的系统发育组中。在30个检测的真菌几丁质酶序列中鉴定出一个几丁质结合结构域,该结构域由两个在aa水平上与细菌几丁质结合结构域相似的亚结构域组成。

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