Maftahi M, Gaillardin C, Nicaud J M
Institut National Agronomique Paris-Grignon, Laboratoire de Génétique Moléculaire et Cellulaire, INRA CNRS, Thiverval-Grignon, France.
Yeast. 1996 Jul;12(9):859-68. doi: 10.1002/(SICI)1097-0061(199607)12:9%3C859::AID-YEA978%3E3.0.CO;2-Q.
We describe a new procedure for the generation of plasmids containing a large promoter and terminator region of a gene of interest, useful for gene disruption. In a two-step polymerase chain reaction (PCR), a fragment, corresponding to the terminator and promoter regions separated by a 16 bp sequence containing a rare restriction site (e.g. AscI), is synthesized (T-P fragment). This PCR fragment is cloned in vectors presenting a rare blunt-end cloning site and a yeast marker for selection in Saccharomyces cerevisiae (TRP1, HIS3 and KanMX). The final plasmids are used directly for gene disruption after linearization by the enzyme (e.g. AscI) specific for the rare restriction site. This approach was used to disrupt three open reading frames identified during the sequencing of COS14-1 from chromosome XIV of S. cerevisiae.
我们描述了一种生成质粒的新方法,该质粒含有感兴趣基因的大片段启动子和终止子区域,可用于基因破坏。在两步聚合酶链反应(PCR)中,合成一个片段(T-P片段),该片段对应于由包含稀有限制性位点(如AscI)的16bp序列隔开的终止子和启动子区域。将该PCR片段克隆到具有稀有平端克隆位点和用于在酿酒酵母中进行选择的酵母标记(TRP1、HIS3和KanMX)的载体中。最终的质粒在通过针对稀有限制性位点的酶(如AscI)线性化后直接用于基因破坏。该方法用于破坏在酿酒酵母第十四号染色体的COS14-1测序过程中鉴定出的三个开放阅读框。
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