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首页> 外文期刊>Enzyme and Microbial Technology >Cloning of cellulase genes from Melanocarpus albomyces and their efficient expression in Trichoderma reesei
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Cloning of cellulase genes from Melanocarpus albomyces and their efficient expression in Trichoderma reesei

机译:黑果木霉纤维素酶基因的克隆及其在里氏木霉中的高效表达

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In our previous study, three purified cellulases of Melanocarpus albomyces proved to be effective in biostoning application at neutral pH [Enzyme Microb. Technol., accepted for publication]. We cloned and sequenced three genes of M. albomyces, which encode a 20 kDa and two 50-kDa polypeptides. The 20-kDa protein (Cel45A) and one of the 50-kDa proteins (Cel7A) are endoglucanases of the glycosyl hydrolase families 45 and 7, respectively. The other 50-kDa protein (Cel7B) is a family 7 cellobiohydrolase. None of the cellulases harbors a cellulose binding domain (CBD). These genes were expressed in Trichoderma reesei under the control of the T reesei cbh1 promoter and the proteins detected in the culture medium. The endoglucanase production levels of the cel45A- and cel7A-transformants were several times higher than those of the parental M. albomyces strain. The sizes of Cel45A, Cel7A and Cel7B proteins produced by the transformants were the same as the sizes of the corresponding proteins purified from M. albomyces. Cellulase preparations produced by the cel45A transformants performed well at neutral pH in stone-washing of denim fabric and caused considerably less backstaining as compared to the acid cellulase product of T reesei
机译:在我们之前的研究中,三种纯化的黑果果纤维素纤维素被证明在中性pH下有效用于生物石化[酶微生物学。技术,已接受出版]。我们克隆和测序了3个基因的M. albomyces,它们编码一个20 kDa和两个50 kDa的多肽。 20 kDa蛋白(Cel45A)和50 kDa蛋白之一(Cel7A)分别是糖基水解酶家族45和7的内切葡聚糖酶。另一个50 kDa蛋白(Cel7B)是7家族纤维二糖水解酶。没有纤维素酶具有纤维素结合域(CBD)。这些基因在里氏木霉cbh1启动子的控制下在里氏木霉中表达,并在培养基中检测到蛋白质。 cel45A和cel7A转化子的内切葡聚糖酶生产水平比亲本分枝杆菌菌株高出几倍。由转化体产生的Cel45A,Cel7A和Cel7B蛋白的大小与从高山分枝杆菌纯化的相应蛋白的大小相同。 cel45A转化子产生的纤维素酶制剂在中性pH下在牛仔布的石洗中表现良好,与里氏木霉的酸性纤维素酶产物相比,造成的反染少得多

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