扩展工具箱:毛霉菌定向基因整合的另一种辅助营养标记。

Q1 Agricultural and Biological Sciences
Paul Primerano, Melani Juric, Robert Mach, Astrid Mach-Aigner, Christian Derntl
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引用次数: 0

摘要

背景:丝状赤霉菌雷氏毛霉菌(Trichoderma reesei)被用于纤维素酶的工业化生产,由于其出色的高蛋白质分泌率及其在工业和科学领域的长期应用,它有望实现异源基因表达。异源基因表达成功的先决条件是能够在雷氏菌基因组的合适位点插入相应的表达盒:在这项研究中,我们测试并证明了 his1 基因[编码 ATP 磷酸核糖转移酶(EC 2.4.2.17),组氨酸生物合成途径的一部分]和基因座对定向基因插入的适用性。删除 his1 启动子和部分编码区会导致组氨酸营养不良。重建 his1 基因座可恢复原营养。我们设计了一种匹配质粒,可以在 his1 基因座上整合表达盒。使用报告基因 EYFP(增强黄色荧光蛋白)证明了这一点。此外,我们还介绍了一种省力且无缝的标记回收方法。最后,我们通过比较三个在不同基因座上带有相同 EYFP 表达构建体的菌株,测试了整合位点对基因表达的影响:随着 his1 作为整合位点和辅助营养标记的确立,我们可以扩展雷氏菌株设计的工具箱。结论:随着 his1 作为整合位点和辅助营养标记的确立,我们可以扩大雷氏菌菌株设计的工具箱,这有助于未来以异源基因表达为目的的菌株构建。
本文章由计算机程序翻译,如有差异,请以英文原文为准。

Expanding the toolbox: another auxotrophic marker for targeted gene integrations in Trichoderma reesei.

Expanding the toolbox: another auxotrophic marker for targeted gene integrations in Trichoderma reesei.

Expanding the toolbox: another auxotrophic marker for targeted gene integrations in Trichoderma reesei.

Expanding the toolbox: another auxotrophic marker for targeted gene integrations in Trichoderma reesei.

Background: The filamentous ascomycete Trichoderma reesei is used for the industrial production of cellulases and holds the promise for heterologous gene expression due to its outstandingly high protein secretion rates and its long-term application in industry and science. A prerequisite for successful heterologous gene expression is the ability to insert a corresponding expression cassette at suitable loci in the genome of T. reesei.

Results: In this study, we test and demonstrate the applicability of the his1 gene [encoding for the ATP phosphoribosyltransferase (EC 2.4.2.17), part of the histidine biosynthesis pathway] and locus for targeted gene insertion. Deletion of the his1 promoter and a part of the coding region leads to histidine auxotrophy. Reestablishment of the his1 locus restores prototrophy. We designed a matching plasmid that allows integration of an expression cassette at the his1 locus. This is demonstrated by the usage of the reporter EYFP (enhanced yellow fluorescence protein). Further, we describe a minimal effort and seamless marker recycling method. Finally, we test the influence of the integration site on the gene expression by comparing three strains bearing the same EYFP expression construct at different loci.

Conclusion: With the establishment of his1 as integration locus and auxotrophic marker, we could expand the toolbox for strain design in T. reesei. This facilitates future strain constructions with the aim of heterologous gene expression.

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来源期刊
Fungal Biology and Biotechnology
Fungal Biology and Biotechnology Agricultural and Biological Sciences-Ecology, Evolution, Behavior and Systematics
CiteScore
10.20
自引率
0.00%
发文量
17
审稿时长
9 weeks
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