Puig O, Rutz B, Luukkonen B G, Kandels-Lewis S, Bragado-Nilsson E, Séraphin B
EMBL, Heidelberg, Germany.
Yeast. 1998 Sep 15;14(12):1139-46. doi: 10.1002/(SICI)1097-0061(19980915)14:12<1139::AID-YEA306>3.0.CO;2-B.
Gene disruption and tagging can be achieved by homologous recombination in the yeast genome. Several PCR-based methods have been described towards this end. However these strategies are often limited in their applications and/or their efficiencies and may be technically demanding. Here we describe two plasmids for C-terminal tagging of proteins with the IgG binding domain of the Staphylococcus aureus protein A. We also present simple and reliable strategies based on PCR to promote efficient integration of exogenous DNA into the yeast genome. These simple methods are not limited to specific strains or markers and can be used for any application requiring homologous recombination such as gene disruption and epitope tagging. These strategies can be used for consecutive introduction of various constructs into a single yeast strain.
基因破坏和标记可通过酵母基因组中的同源重组来实现。为此已描述了几种基于PCR的方法。然而,这些策略在其应用和/或效率方面往往受到限制,并且可能在技术上要求较高。在此,我们描述了两种用于用金黄色葡萄球菌蛋白A的IgG结合结构域对蛋白质进行C端标记的质粒。我们还提出了基于PCR的简单可靠策略,以促进外源DNA高效整合到酵母基因组中。这些简单方法不限于特定菌株或标记,可用于任何需要同源重组的应用,如基因破坏和表位标记。这些策略可用于将各种构建体连续引入单个酵母菌株。
