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Preparation of mutants of Trichoderma reesei with enhanced cellulase production.

机译:制备具有增强的纤维素酶产量的里氏木霉突变体。

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摘要

The development of an agar plate screening technique has allowed the isolation of a range of mutants of Trichoderma reesei capable of synthesizing cellulase under conditions of high catabolite repression. The properties of one of these mutants (NG-14) is described to illustrate the use of this technique. NG-14 produced five times the filter paper-degrading activity per ml of culture medium and twice the specific activity per mg of excreted protein in submerged culture when compared with the best existing mutant, QM9414. NG-14 also showed enhanced endo-beta-glucanase and beta-glucosidase production. Although these mutants were isolated as cellulase producers in the presence of 5% glycerol on agar plates, in similar liquid medium, NG-14 exhibits only partial derepression of the cellulase complex. Since the proportions of filter paper activity, endo-beta-glucanase, and cellobiase were not the same in mutants NG-14 and QM9414, and the yields of each enzyme under conditions repressive for cellulase synthesis were different, differential control of each enzyme of the cellulase complex is implied. These initial results suggest that the selective technique for isolating hyper-cellulase-producing mutants of Trichoderma will be of considerable use in the development of commercially useful cellulolytic strains.
机译:琼脂平板筛选技术的发展已允许分离一系列能够在高分解代谢物阻抑条件下合成纤维素酶的里氏木霉突变体。描述了这些突变体之一(NG-14)的特性,以说明该技术的使用。与现有最佳的突变体QM9414相比,NG-14在每毫升培养基中产生的滤纸降解活性是其每毫升培养基的五倍,而每毫克分泌蛋白质的比活性是在淹没培养物中的两倍。 NG-14还显示出增强的内切β-葡聚糖酶和β-葡萄糖苷酶产量。尽管这些突变体在琼脂平板上存在5%甘油的情况下被分离为纤维素酶生产者,但在类似的液体培养基中,NG-14仅表现出部分的纤维素酶复合物阻抑作用。由于突变体NG-14和QM9414中滤纸活性,内切β-葡聚糖酶和纤维二糖酶的比例不同,并且在抑制纤维素酶合成的条件下每种酶的产量均不同,因此对每种酶的差异控制暗示纤维素酶复合物。这些初步结果表明,用于分离产生木霉属的超纤维素酶的突变体的选择性技术将在商业上有用的纤维素分解菌株的开发中大量使用。

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