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裂殖酵母表达和分泌 CB4-1 scFv-GFP 融合蛋白。

Expression and secretion of a CB4-1 scFv-GFP fusion protein by fission yeast.

机构信息

PomBioTech GmbH, Campus Building A1-1, Saarbrücken, Germany.

出版信息

Appl Biochem Biotechnol. 2011 Jan;163(1):80-9. doi: 10.1007/s12010-010-9018-9. Epub 2010 Jul 10.

DOI:10.1007/s12010-010-9018-9
PMID:20617397
Abstract

There is a rapidly growing demand for fluorescent single-chain Fv (scFv) antibody fragments for many applications. Yeasts have developed into attractive hosts for recombinant production of these functionalized proteins because they provide several advantages over prokaryotes and higher eukaryotes as expression systems, e.g., being capable of high-level secretion of heterologous proteins. In this study, we report Schizosaccharomyces pombe as a new host organism for secretory production of scFv-green fluorescent protein (GFP) fusions and compare it with previously described yeast expression systems. We cloned a plasmid for the expression and secretion of the anti-p24 (human immunodeficiency virus 1) CB4-1 scFv fused to GFP. After expression of the scFv-GFP fused to an N-terminal Cpy1 secretion signal sequence, fluorescence microscopy of living yeast cells indicated that the heterologous protein entered the secretory pathway. Western blot analysis of cell-free culture supernatants confirmed that the scFv-GFP was efficiently secreted with yields up to 5 mg/L. In addition, fluorescence measurements of culture supernatants demonstrated that the GFP moiety of the scFv-GFP protein is fully functional after secretion. Our data suggest that S. pombe has the potential for being used as alternative expression host in recombinant antibody fragment production by ensuring efficient protein processing and secretion.

摘要

人们对用于多种应用的荧光单链 Fv(scFv)抗体片段的需求正在迅速增长。与原核生物和高等真核生物相比,酵母作为表达系统具有许多优势,例如能够高水平分泌异源蛋白,因此已成为这些功能化蛋白重组生产的有吸引力的宿主。在这项研究中,我们报告了裂殖酵母(Schizosaccharomyces pombe)作为 scFv-绿色荧光蛋白(GFP)融合蛋白分泌生产的新宿主生物,并将其与之前描述的酵母表达系统进行了比较。我们克隆了一个用于表达和分泌与 GFP 融合的抗 p24(人类免疫缺陷病毒 1)CB4-1 scFv 的质粒。在表达 scFv-GFP 融合到 N 端 Cpy1 分泌信号序列后,活酵母细胞的荧光显微镜观察表明该异源蛋白进入了分泌途径。无细胞培养上清液的 Western blot 分析证实 scFv-GFP 被有效地分泌,产量高达 5mg/L。此外,培养上清液的荧光测量表明,scFv-GFP 蛋白的 GFP 部分在分泌后仍具有完全功能。我们的数据表明,裂殖酵母具有作为重组抗体片段生产替代表达宿主的潜力,可确保高效的蛋白质加工和分泌。

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