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半胱氨酸残基的突变增加了桃扩张蛋白在甲基营养型酵母中的异源表达。

Mutation of cysteine residues increases heterologous expression of peach expansin in the methylotrophic yeast .

作者信息

Matsuyama Kaori, Sunagawa Naoki, Igarashi Kiyohiko

机构信息

Department of Biomaterial Sciences, Graduate School of Agricultural and Life Sciences, The University of Tokyo, 1-1-1 Yayoi, Bunkyo-ku, Tokyo 113-8657, Japan.

VTT Technical Research Centre of Finland, PO Box 1000, Tietotie 2, Espoo FI-02044 VTT, Finland.

出版信息

Plant Biotechnol (Tokyo). 2020 Dec 25;37(4):397-403. doi: 10.5511/plantbiotechnology.20.0713a.

Abstract

The study of Carbohydrate-Active enZymes (CAZymes) associated with plant cell wall metabolism is important for elucidating the developmental mechanisms of plants and also for the utilization of plants as a biomass resource. The use of recombinant proteins is common in this context, but heterologous expression of plant proteins is particularly difficult, in part because the presence of many cysteine residues promotes denaturation, aggregation and/or protein misfolding. In this study, we evaluated two phenotypes of methylotrophic yeast as expression hosts for expansin from peach ( (L.) Batsch, EXP1), which is one of the most challenging targets for heterologous expression. cDNAs encoding wild-type expansin (EXP1_WT) and a mutant in which all cysteine residues were replaced with serine (EXP1_CS) were each inserted into expression vectors, and the protein expression levels were compared. The total amount of secreted protein in EXP1_WT culture was approximately twice that of EXP1_CS. However, the amounts of recombinant expansin were 0.58 and 4.3 mg l, corresponding to 0.18% and 2.37% of total expressed protein, respectively. This 13-fold increase in production of the mutant in indicates that the replacement of cysteine residues stabilizes recombinant EXP1.

摘要

研究与植物细胞壁代谢相关的碳水化合物活性酶(CAZymes)对于阐明植物的发育机制以及将植物作为生物质资源加以利用都很重要。在这种情况下,使用重组蛋白很常见,但植物蛋白的异源表达特别困难,部分原因是许多半胱氨酸残基的存在会促进变性、聚集和/或蛋白质错误折叠。在本研究中,我们评估了两种甲基营养型酵母表型作为桃((L.) Batsch)扩张蛋白(EXP1)的表达宿主,EXP1是异源表达最具挑战性的目标之一。将编码野生型扩张蛋白(EXP1_WT)和所有半胱氨酸残基都被丝氨酸取代的突变体(EXP1_CS)的cDNA分别插入表达载体,并比较蛋白质表达水平。EXP1_WT培养物中分泌蛋白的总量约为EXP1_CS的两倍。然而,重组扩张蛋白的量分别为0.58和4.3 mg l,分别占总表达蛋白的0.18%和2.37%。突变体产量增加13倍表明半胱氨酸残基的取代使重组EXP1稳定。

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