pZHK2, a bi-functional transformation vector, suitable for two step gene targeting

U. Kück, S. Pöggeler
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引用次数: 9

Abstract

Homologous recombination is a prerequisite for the generation of knock out strains by means of DNA-mediated transformation. In filamentous fungi however, the frequency of ectopic integration events is rather high and the actual efficiency of homologous recombination depends upon the length of homologous DNA flanking the transformation marker. Recently, d'Enfert and coworkers (Chaveroche et al., 2000) presented a two-step technology for the integration of a bi-functional zeocin-pyrG cassette into a target sequence of interest using an Escherichia coli strain expressing the phage lambda Red functions. In the resulting recombinant cosmids, the selection marker is flanked by fungal DNA sequences longer than 1 kb, which can be used to transform appropriate fungal recipient strains. For selection of fungal transformants, those workers used the A. nidulans pyrG gene encoding orotidine-5'monophosphate decarboxylase, which confers prototrophy in appropriate uridine/uracil auxotrophic recipient strains. Here, we describe the novel bi-functional transformation vector pZHK2, which carries in addition to the zeocin resistance gene the hygromycin B phosphotransferase gene often used as a dominant selectable marker gene in fungal recipient strains. The applicability of the vector is demonstrated by generating a ura3 knock out strain from Sordaria macrospora showing auxotrophy.
pZHK2是一种双功能转化载体,适用于两步基因靶向
同源重组是通过dna介导转化产生敲除菌株的先决条件。然而,在丝状真菌中,异位整合事件的频率相当高,同源重组的实际效率取决于转化标记侧同源DNA的长度。最近,d'Enfert及其同事(Chaveroche等人,2000)提出了一种两步技术,利用表达噬菌体lambda Red功能的大肠杆菌菌株,将双功能的zeocin-pyrG盒整合到感兴趣的目标序列中。在重组的cosmids中,选择标记的两侧有超过1kb的真菌DNA序列,可以用来转化合适的真菌受体菌株。为了选择真菌转化体,这些工人使用了A. nidulans pyg基因编码orotidine-5'单磷酸脱羧酶,该基因赋予适当的尿苷/尿嘧啶营养不良受体菌株原生营养。在这里,我们描述了新的双功能转化载体pZHK2,它除了携带zeocin抗性基因外,还携带潮霉素B磷酸转移酶基因,在真菌受体菌株中常被用作显性选择标记基因。通过从大孢子索达菌中产生一个ura3敲除菌株,证明了该载体的适用性。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
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