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Autocloning and Amplification of LIP2 inYarrowia lipolytica

机译:解脂耶氏酵母中LIP2的自动克隆和扩增

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We synthesized a Yarrowia lipolytica strain overproducing lipase for industrial applications by using long terminal repeat (ζ) of the Y. lipolytica retrotransposon Ylt1 and an allele of URA3 with a promoter deletion to construct JMP3. JMP3 is a derivative of plasmid pHSS6 carrying aNotI-NotI cassette which contains a defectiveURA3 allele, a polylinker sequence, and the ζ region for targeting to multiple sites in the genome of the recipient. We inserted the LIP2 gene (encoding extracellular lipase) under the control of the strong POX2 promoter into JMP3 to generate JMP6. The pHSS6 region was removed by NotI digestion prior to transformation. Two Y. lipolytica strains transformed with the JMP6 LIP2 cassette had a mean of 10 integrated copies devoid of the Escherichia coli region, corresponding to an autocloning event. The copy number in the transformants was stable even after 120 generations in nonselective and lipase-inducing conditions. The resulting strains could produce 0.5 g of active lipase per liter in the supernatant, 40 times more than the single-copy strain with the LIP2 promoter. This work provides a new expression system in Y. lipolytica that results in strains devoid of bacterial DNA and in strains producing a high level of lipase for industrial uses, waste treatment, and pancreatic insufficiency therapy.
机译:我们使用解脂耶氏酵母逆转座子Ylt1和带有启动子缺失的URA3等位基因的长末端重复序列(ζ),合成了过量生产用于工业应用的脂肪酶的耶氏酵母脂肪酶菌株,以构建JMP3。 JMP3是携带NotI-NotI盒的质粒pHSS6的衍生物,该NotI-NotI盒包含有缺陷的URA3等位基因,多接头序列和用于靶向受体基因组中多个位点的ζ区。我们在强POX2启动子的控制下将LIP2基因(编码细胞外脂肪酶)插入JMP3以生成JMP6。在转化之前,通过NotI消化除去pHSS6区域。用JMP6 LIP2盒转化的两个解脂耶氏酵母菌株的平均整合拷贝数为10,缺少大肠杆菌区域,这与自动克隆事件相对应。即使在非选择性和脂肪酶诱导的条件下经过120代后,转化体中的拷贝数也是稳定的。所得菌株在上清液中每升可产生0.5 g活性脂肪酶,是具有LIP2启动子的单拷贝菌株的40倍。这项工作提供了一种在解脂耶氏酵母中的新表达系统,该系统可导致无细菌DNA的菌株以及产生高水平脂肪酶的菌株用于工业用途,废物处理和胰腺功能不全疗法。

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