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PDI可改善氧化还原无活性β-葡萄糖苷酶的分泌。

PDI improves secretion of redox-inactive beta-glucosidase.

作者信息

Powers Sara Lawrence, Robinson Anne Skaja

机构信息

Department of Chemical Engineering, University of Delaware, 150 Academy Street, Newark, Delaware 19716, USA.

出版信息

Biotechnol Prog. 2007 Mar-Apr;23(2):364-9. doi: 10.1021/bp060287p. Epub 2007 Feb 22.

Abstract

Although manipulation of the endoplasmic reticulum (ER) folding environment in the yeast Saccharomyces cerevisiae has been shown to increase the secretory productivity of recombinant proteins, the cellular interactions and processes of native enzymes and chaperones such as protein disulfide isomerase (PDI) are still unclear. Previously, we reported that overexpression of the ER chaperone PDI enabled up to a 3-fold increase in secretion levels of the Pyrococcus furiosus beta-glucosidase in the yeast S. cerevisiae. This result was surprising since beta-glucosidase contains only one cysteine per monomer and no disulfide bonds. Two possible mechanisms were proposed: PDI either forms a transient disulfide bond with the lone cysteine residue of the nascent beta-glucosidase during the folding and assembly process or acts as a chaperone to aid in proper folding. To discern between the two mechanisms, the single cysteine residue was mutated to serine, and the secretion of the two protein variants was determined. The serine mutant still showed increased secretion in vivo when PDI levels were elevated. When the folding bottleneck is removed by increasing expression temperatures to 37 degrees C rather than 30 degrees C, PDI no longer has an improvement on secretion. These results suggest that, unexpectedly, PDI acts in a chaperone-like capacity or possibly cooperates with the cell's folding or degradation mechanisms regardless of whether the protein is redox-active.

摘要

尽管在酿酒酵母中对内质网(ER)折叠环境进行调控已被证明可提高重组蛋白的分泌效率,但诸如蛋白二硫键异构酶(PDI)等天然酶和伴侣蛋白的细胞内相互作用及过程仍不清楚。此前,我们报道过在内质网伴侣蛋白PDI过表达的情况下,嗜热栖热菌β-葡萄糖苷酶在酿酒酵母中的分泌水平提高了多达3倍。这一结果令人惊讶,因为β-葡萄糖苷酶每个单体仅含一个半胱氨酸且没有二硫键。我们提出了两种可能的机制:在折叠和组装过程中,PDI要么与新生β-葡萄糖苷酶唯一的半胱氨酸残基形成一个瞬时二硫键,要么作为伴侣蛋白协助其正确折叠。为区分这两种机制,我们将单个半胱氨酸残基突变为丝氨酸,并测定了这两种蛋白变体的分泌情况。当PDI水平升高时,丝氨酸突变体在体内仍表现出分泌增加。当将表达温度提高到37摄氏度而非30摄氏度以消除折叠瓶颈时,PDI对分泌不再有促进作用。这些结果表明,出乎意料的是,无论蛋白质是否具有氧化还原活性,PDI都以类似伴侣蛋白的能力发挥作用,或者可能与细胞的折叠或降解机制协同作用。

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