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An improved Agrobacterium-mediated transformation system for the functional genetic analysis of Penicillium marneffei.

机译:一种改良的农杆菌介导的转化系统,用于马尔尼菲青霉的功能遗传分析。

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摘要

We have developed an improved Agrobacterium-mediated transformation (AMT) system for the functional genetic analysis of Penicillium marneffei, a thermally dimorphic, human pathogenic fungus. Our AMT protocol included the use of conidia or pre-germinated conidia of P. marneffei as the host recipient for T-DNA from Agrobacterium tumefaciens and co-cultivation at 28 degrees C for 36 hours. Bleomycin-resistant transformants were selected as yeast-like colonies following incubation at 37 degrees C. The efficiency of transformation was approximately 123 +/- 3.27 and 239 +/- 13.12 transformants per plate when using 5 x 10(4) conidia and pre-germinated conidia as starting materials, respectively. Southern blot analysis demonstrated that 95% of transformants contained single copies of T-DNA. Inverse PCR was employed for identifying flanking sequences at the T-DNA insertion sites. Analysis of these sequences indicated that integration occurred as random recombination events. Among the mutants isolated were previously described stuA and gasC defective strains. These AMT-derived mutants possessed single T-DNA integrations within their particular coding sequences. In addition, other morphological and pigmentation mutants possessing a variety of gene-specific defects were isolated, including two mutants having T-DNA integrations within putative promoter regions. One of the latter integration events was accompanied by the deletion of the entire corresponding gene. Collectively, these results indicated that AMT could be used for large-scale, functional genetic analyses in P. marneffei. Such analyses can potentially facilitate the identification of those genetic elements related to morphogenesis, as well as pathogenesis in this medically important fungus.
机译:我们已经开发了一种改良的农杆菌介导的转化(AMT)系统,用于对马尔尼菲青霉菌(一种热双态人类致病性真菌)进行功能遗传分析。我们的AMT方案包括使用马尼菲假孢子的分生孢子或预萌生的分生孢子作为来自根癌农杆菌的T-DNA的宿主,并在28摄氏度共培养36小时。在37°C下孵育后,选择抗博来霉素的转化子作为酵母样菌落。使用5 x 10(4)分生孢子和pre-conidia时,每个平板的转化效率约为123 +/- 3.27和239 +/- 13.12个转化子。发芽的分生孢子分别作为起始原料。 Southern印迹分析表明95%的转化体含有单拷贝的T-DNA。反向PCR用于鉴定T-DNA插入位点的侧翼序列。这些序列的分析表明整合发生为随机重组事件。在分离的突变体中,先前描述的是stuA和gasC缺陷菌株。这些AMT衍生的突变体在其特定的编码序列内具有单个T-DNA整合。另外,分离了具有各种基因特异性缺陷的其他形态和色素沉着突变体,包括在推定的启动子区域内具有T-DNA整合的两个突变体。后一种整合事件伴随着整个相应基因的缺失。总的来说,这些结果表明AMT可以用于马尼菲疟原虫的大规模,功能性遗传分析。这样的分析可以潜在地促进与这些在医学上重要的真菌中的形态发生以及发病机理相关的遗传元件的鉴定。

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