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毕赤酵母中的荧光蛋白融合。

Fluorescent protein fusions in Candida guilliermondii.

机构信息

EA2106, Biomolécules et Biotechnologies Végétales, Université François-Rabelais de Tours, France.

出版信息

Fungal Genet Biol. 2011 Nov;48(11):1004-11. doi: 10.1016/j.fgb.2011.07.004. Epub 2011 Jul 23.

DOI:10.1016/j.fgb.2011.07.004
PMID:21807108
Abstract

Candida guilliermondii is an emerging fungal agent of candidiasis often associated with oncology patients. This yeast also remains a promising biotechnological model for the industrial production of value-added metabolites. In the present study, we developed a recipient strain as well as a set of plasmids for construction of fluorescent protein (FP) fusions in this species. We demonstrated that C. guilliermondii phosphoglycerate kinase transcription-regulating sequences allow a constitutive expression of codon-optimized green, cyan, yellow and mCherry FP genes in C. guilliermondii cells and the fluorescence signal could be directly observed at the colony and blastospore level by epifluorescence microcopy. To illustrate differential targeting of the FPs into specified cellular compartments, we studied and validated the expected subcellular localization of various C. guilliermondii predicted proteins fused to FPs. Furthermore, co-expression experiments of various couples of FP-tagged C. guilliermondii predicted proteins in the same cell showed that the fluorescence of each FP could be detected independently, providing firm evidences that YFP/CFP and GFP/mCherry pairs can be used for dual labeling in C. guilliermondii cells. This technical advance will facilitate future studies of protein co-expression and co-localization in C. guilliermondii and will give precious help for elucidating new molecular events supporting pathogenicity, antifungal resistance and for exploring the potential of yeast metabolic engineering.

摘要

假丝酵母是一种新兴的真菌病原体,常与肿瘤患者有关。这种酵母仍然是一种很有前途的生物技术模型,可用于工业生产增值代谢物。在本研究中,我们开发了一种受体菌株和一套质粒,用于在该物种中构建荧光蛋白(FP)融合。我们证明,假丝酵母磷酸甘油酸激酶转录调控序列允许在假丝酵母细胞中组成型表达密码子优化的绿色、青色、黄色和 mCherry FP 基因,并且荧光信号可以通过荧光显微镜直接在菌落和芽殖孢子水平上观察到。为了说明 FP 被靶向到特定的细胞区室,我们研究并验证了各种假丝酵母预测蛋白与 FP 融合后的预期亚细胞定位。此外,在同一细胞中表达各种 FP 标记的假丝酵母预测蛋白的共表达实验表明,每个 FP 的荧光都可以独立检测到,这为 YFP/CFP 和 GFP/mCherry 对可用于假丝酵母细胞的双标记提供了确凿的证据。这项技术进步将有助于假丝酵母中蛋白质共表达和共定位的未来研究,并为阐明支持致病性、抗真菌耐药性的新分子事件以及探索酵母代谢工程的潜力提供宝贵帮助。

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