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首页> 外文期刊>Yeast >Cloning and disruption of the PpURA5 gene and construction of a set of integration vectors for the stable genetic modification of Pichia pastoris
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Cloning and disruption of the PpURA5 gene and construction of a set of integration vectors for the stable genetic modification of Pichia pastoris

机译:PpURA5基因的克隆和破坏以及用于稳定毕赤酵母基因修饰的一组整合载体的构建

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A pair of degenerate primers was used for amplification and cloning of a DNA fragment containing parts of the P. pastoris URA5 and SEC65 genes. Using additional information from a partial genomic sequence of P. pastoris, we cloned and sequenced a 1.9 kb chromosomal fragment containing the complete orotate-phosphoribosyltransferase-encoding URA5 gene. A disruption cassette was constructed by replacing a small part of the open reading frame with a kanamycin-resistance gene. The P. pastoris wild-type strain NRRL Y-11430 was transformed with the disruption cassette and an ura5 auxotrophic strain was identified. To generate marker constructs that can be reused in successive transformations of a single strain, we constructed two lacZ-PpURA3-lacZ and lacZ-PpURA5-lacZ cassettes and used them to disrupt PpOCH1. The PpURA3 and PpURA5 genes in the disruptants were then successfully recycled by selecting for resistance to 5'-fluoro-orotic acid. We also assembled a set of modular plasmids that can be used for the stable genetic modification of P. pastoris via a double cross-over event. The sequence presented here has been submitted to the EMBL data library under Accession No. AY303544.
机译:一对简并引物用于扩增和克隆包含巴斯德毕赤酵母URA5和SEC65基因的一部分的DNA片段。使用来自巴斯德毕赤酵母的部分基因组序列的其他信息,我们克隆并测序了一个1.9 kb的染色体片段,其中包含完整的乳清酸-磷酸核糖基转移酶编码URA5基因。通过用卡那霉素抗性基因替换开放阅读框的一小部分来构建破坏盒。用破坏盒转化巴斯德毕赤酵母野生型菌株NRRL Y-11430,并鉴定出ura5营养缺陷型菌株。为了生成可在单个菌株的后续转化中重复使用的标记构建体,我们构建了两个lacZ-PpURA3-lacZ和lacZ-PpURA5-lacZ盒,并使用它们来破坏PpOCH1。然后,通过选择对5'-氟乳清酸的抗性,成功地破坏了突变体中的PpURA3和PpURA5基因。我们还组装了一套模块化质粒,可用于通过双重交换事件对巴斯德毕赤酵母进行稳定的遗传修饰。此处显示的序列已提交到EMBL数据库,登录号为AY303544。

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