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工程化里氏木霉木聚糖酶 3 启动子以实现高效酶表达。

Engineering of the Trichoderma reesei xylanase3 promoter for efficient enzyme expression.

机构信息

Department of Bioengineering, Nagaoka University of Technology, 1603-1, Kamitomioka, Nagaoka, Niigata, 940-2188, Japan.

Graduate School of Life and Environmental Sciences, Osaka Prefecture University, 1-1, Gakuen-cho, Naka-ku, Sakai, Osaka, 599-8531, Japan.

出版信息

Appl Microbiol Biotechnol. 2018 Mar;102(6):2737-2752. doi: 10.1007/s00253-018-8763-5. Epub 2018 Feb 7.

Abstract

The GH10 xylanase XYNIII is expressed in the hyper-cellulase-producing mutant PC-3-7, but not in the standard strain QM9414 of Trichoderma reesei. The GH11 xylanase gene xyn1 is induced by cellulosic and xylanosic carbon sources while xyn3 is induced only by cellulosic carbon sources in the PC-3-7 strain. In this study, we constructed a modified xyn3 promoter in which we replaced the cis-acting region of the xyn3 promoter by the cis-acting region of the xyn1 promoter. The resulting xyn3 chimeric promoter exhibited improved inductivity against cellulosic carbon over the wild-type promoter and acquired inductivity against xylanosic carbon. Furthermore, PC-3-7 expressing the heterologous β-glycosidase gene, Aspergillus aculeatus bgl1, under the control of the xyn3 chimeric promoter, showed enhanced saccharification ability through increased cellobiase activity. We also show that the xyn3 chimeric promoter is also functional in the QM9414 strain. Our results indicate that the xyn3 chimeric promoter is very efficient for enzyme expression.

摘要

GH10 木聚糖酶 XYNIII 在产超纤维素酶的突变株 PC-3-7 中表达,但不在里氏木霉 QM9414 的标准菌株中表达。GH11 木聚糖酶基因 xyn1 被纤维素和木聚糖碳源诱导,而 xyn3 仅在 PC-3-7 菌株中被纤维素碳源诱导。在这项研究中,我们构建了一个修饰的 xyn3 启动子,其中我们用 xyn1 启动子的顺式作用区替换了 xyn3 启动子的顺式作用区。所得的 xyn3 嵌合启动子对纤维素碳源的诱导活性高于野生型启动子,并获得了对木聚糖碳源的诱导活性。此外,在 xyn3 嵌合启动子的控制下,表达异源β-糖苷酶基因 Aspergillus aculeatus bgl1 的 PC-3-7 表现出通过增加纤维二糖酶活性而提高的糖化能力。我们还表明,xyn3 嵌合启动子在 QM9414 菌株中也是有效的。我们的结果表明,xyn3 嵌合启动子对于酶表达非常有效。

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