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首页> 外文期刊>Journal of Microbiological Methods >A new recombinant protein expression system for high-throughput screening in the yeast Yarrowia lipolytica
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A new recombinant protein expression system for high-throughput screening in the yeast Yarrowia lipolytica

机译:用于酵母Yarrowia Lipolytica的高通量筛选的新重组蛋白表达系统

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Development of a high-throughput eukaryotic screening procedure is important to increase success in obtaining improved enzymes through directed enzyme evolution. This procedure was developed for the yeast Yarrowia lipolytica which becomes the second eukaryotic host for this purpose. The extracellular lipase Lip2 was used as expressed enzyme but this system will be easily adjusted for other enzymes. We adapted and optimized the protocol for protein expression by Y. lipolytica in 96-well microplates. Yeast transformation efficiency and expression cassette insertion were increased by constructing a strain containing a zeta docking platform for targeted integration into the genome. The coefficient of variance of the full process was reduced from 36.3% to 18.9%. The main part of the variability (11.7%) arises from the specific lipase enzyme assay whereas the coefficient of variance concerning transformation, growth and expression steps represents only 7.2%. The rate of clone with no activity was reduced from 5.8% to 0.2%. Both transformation efficiency and variability are then compatible with high-throughput screening in the yeast Y. lipolytica.
机译:高通量真核筛选程序的发展对于通过定向酶进化获得改善的酶来增加成功是重要的。为酵母YarraWia Lipolytica开发了该程序,其成为目的的第二真核宿主。使用细胞外脂肪酶LiP2如表达酶,但该系统将容易地调节其他酶。我们通过在96孔微孔板中调整并优化了Y. Lipolytica的蛋白质表达方案。通过构建含有Zeta对接平台的诱导菌株来增加酵母转化效率和表达盒插入,用于靶向整合到基因组中。完整过程的变异系数从36.3%降至18.9%。可变性的主要部分(11.7%)由特定的脂肪酶测定法产生,而有关转化,生长和表达步骤的差异系数仅为7.2%。没有活性的克隆率从5.8%降至0.2%。转化效率和可变性均与酵母Y. Lipolytica中的高通量筛选相容。

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