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[利用反义RNA技术下调酿酒酵母中羊毛甾醇合酶基因的表达]

[Downregulation of lanosterol synthase gene expression by antisense RNA technology in Saccharomyces cerevisiae].

作者信息

Wang Qing-hua, Gao Li-li, Liang Hui-chao, Du Guo-hua, Gong Ting, Yang Jin-ling, Zhu Ping

出版信息

Yao Xue Xue Bao. 2015 Jan;50(1):118-22.

PMID:25924486
Abstract

The cyclization of 2,3-oxidosqualene is the key branch point of ergosterol and triterpenoid biosynthesis. Downregulation of 2,3-oxidosqualene metabolic flux to ergosterol in Saccharomyces cerevisiae may redirect the metabolic flux toward the triterpenoid synthetic pathway. In our study, primers were designed according to erg7 gene sequence of S. cerevisiae. Three fragments including 5' long fragment, 5' short fragment and erg7 coding region fragment were amplified by PCR. 5' long fragment consists of the promoter and a part of erg7 coding region sequence. 5' short fragment consists of a part of promoter and a part of erg7 coding region sequence. These fragments were inserted reversely into pESC-URA to construct antisense expression plasmids. The recombinant plasmids were transformed into S. cerevisiae INVSc1 and recombinant strains were screened on the nutritional deficient medium SD-URA. The erg7 expression level of recombinant strains, which harbored antisense expression plasmid of erg7 coding region, was similar to that of INVScl by semi-quantitative PCR detection. But erg7 expression level of recombinant strains, which harbored 5' long antisense fragment and 5' short antisense fragment, was significantly lower than that of the control. The results of TLC and HPLC showed that the ergosterol content of recombinant strains, which harbored 5' long antisense fragment, decreased obviously. The ergosterol contents of the others were almost equal to that of INVSc1. Lanosterol synthase gene expression was downregulated by antisense RNA technology in S. cerevisiae, which lays a foundation for reconstructing triterpenoid metabolic pathway in S. cerevisiae by synthetic biology technology.

摘要

2,3-氧化角鲨烯的环化作用是麦角固醇和三萜生物合成的关键分支点。酿酒酵母中2,3-氧化角鲨烯向麦角固醇的代谢通量下调可能会使代谢通量转向三萜合成途径。在我们的研究中,根据酿酒酵母的erg7基因序列设计引物。通过PCR扩增出包括5'长片段、5'短片段和erg7编码区片段在内的三个片段。5'长片段由启动子和一部分erg7编码区序列组成。5'短片段由一部分启动子和一部分erg7编码区序列组成。将这些片段反向插入pESC-URA构建反义表达质粒。将重组质粒转化到酿酒酵母INVSc1中,并在营养缺陷型培养基SD-URA上筛选重组菌株。通过半定量PCR检测,含有erg7编码区反义表达质粒的重组菌株的erg7表达水平与INVScl相似。但是,含有5'长反义片段和5'短反义片段的重组菌株的erg7表达水平明显低于对照。TLC和HPLC结果表明,含有5'长反义片段的重组菌株的麦角固醇含量明显降低。其他菌株的麦角固醇含量几乎与INVSc1相等。通过反义RNA技术下调了酿酒酵母中羊毛甾醇合酶基因的表达,这为利用合成生物学技术重建酿酒酵母中的三萜代谢途径奠定了基础。

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