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Plasmids with E2 epitope tags: tagging modules for N- and C-terminal PCR-based gene targeting in both budding and fission yeast, and inducible expression vectors for fission yeast

机译:具有E2表位标签的质粒:在萌芽和裂变酵母中靶向N和C端基于PCR的基因的标记模块,以及裂殖酵母的诱导型表达载体

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摘要

A single-step PCR-based epitope tagging enables fast and efficient gene targeting with various epitope tags. This report presents a series of plasmids for the E2 epitope tagging of proteins in Saccharomyces cerevisiae and Schizosaccharomyces pombe.E2Tags are 10-amino acids (epitope E2a: SSTSSDFRDR)- and 12 amino acids (epitope E2b: GVSSTSSDFRDR)-long peptides derived from the E2 protein of bovine papillomavirus type 1. The modules for C-terminal tagging with E2a and E2b epitopes were constructed by the modification of the pYM-series plasmid. The N-terminal E2a and E2b tagging modules were based on pOM-series plasmid. The pOM-series plasmids were selected for this study because of their use of the Cre-loxP recombination system. The latter enablesa marker cassette to be removed after integration into the loci of interest and, thereafter, the tagged protein is expressed under its endogenous promoter. Specifically for fission yeast, high copy pREP plasmids containing the E2a epitope tag as an N-terminal or C-terminal tag were constructed. The properties of E2a and E2b epitopes and the sensitivity of two anti-E2 monoclonal antibodies (5E11 and 3F12) were tested using several S. cerevisiae and Sz. pombe E2-tagged strains.
机译:基于PCR的单步抗原决定簇标签可实现各种抗原决定簇标签的快速有效基因靶向。该报告提出了一系列用于酿酒酵母和粟酒裂殖酵母中蛋白质E2表位标签的质粒.E2标签是10个氨基酸(表位E2a:SSTSSDFRDR)和12个氨基酸(表位E2b:GVSSTSSDFRDR)长的肽1型牛乳头瘤病毒的E2蛋白通过修饰pYM系列质粒,构建了用E2a和E2b表位进行C末端标记的模块。 N端E2a和E2b标签模块基于pOM系列质粒。选择pOM系列质粒进行此项研究是因为它们使用了Cre-loxP重组系统。后者使得标记盒能够在整合到感兴趣的基因座中之后被去除,然后,标记的蛋白质在其内源启动子下表达。专门针对裂变酵母,构建了包含E2a表位标签作为N端或C端标签的高拷贝pREP质粒。 E2a和E2b表位的性质以及两种抗E2单克隆抗体(5E11和3F12)的敏感性使用几种酿酒酵母和Sz进行了测试。带有E2标签的pombe菌株。

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  • 来源
    《Yeast》 |2009年第1期|共12页
  • 作者

    Tamm T;

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  • 原文格式 PDF
  • 正文语种 eng
  • 中图分类 酿造工业;
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