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Agrobacterium-mediated transformation of Ceratocystis albifundus

机译:农杆菌介导的Ceratocystis albifundus的转化

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摘要

Functional association between genomic loci and specific biological traits remains lacking in many fungi, including the African tree pathogen Ceratocystis albifundus. This is mainly because of the absence of suitable transformation systems for allowing genetic manipulation of this and other fungi. Here, we present an optimized protocol for Agrobacterium tumefaciens-mediated transformation of C. albifundus. Strain AGL-1 of A. turnefaciens and four binary T-DNA vectors (conferring hygromycin B or geneticin resistance and/or expressing the green fluorescent protein [GFP]) were used for transforming germinated conidia of three isolates of C. albifundus. Stable expression of these T-DNA-encoded traits was confirmed through sequential sub-culturing of fungal transformants on selective and non-selective media and by using PCR and sequence analysis. Single-copy integration of the respective T-DNAs into the genomes of these fungi was confirmed using Southern hybridization analysis. The range of experimental parameters determined and optimised included: (i) concentrations of hygromycin B and geneticin required for inhibiting growth of the wild type fungus and (ii) the dependence of transformation on acetosyringone for inducing the bacterium's virulence genes, as well as (iii) the duration of fungus-bacterium co-cultivation periods and (iv) the concentrations of fungal conidia and bacterial cells used for the latter. The system developed in this study is stable with a high-efficiency, yielding up to 400 transformants per 10(6) conidia. This is the first report of a transformation protocol for C. albifundus and its availability will be invaluable for functional studies in this important fungus.
机译:基因组基因座和特异性生物学性质之间的功能关系仍然缺乏许多真菌,包括非洲树病原菌Ceratocystis albifundus。这主要是因为没有合适的转化系统,用于允许遗传操作和其他真菌。在这里,我们为农杆菌癌症介导的C.Bolifundus的转化提供了优化方案。用于A.Turnfaciens和四个二进制T-DNA载体的菌株AgL-1(赋予Hygromycin B或遗传蛋白抗性和/或表达绿色荧光蛋白[GFP])用于转化C.Bolifundus的三个分离株的发芽结合。通过在选择性和非选择性介质上的真菌转化体和使用PCR和序列分析来证实这些T-DNA编码性状的稳定表达。使用Southern杂交分析证实了各自的T-DNA对这些真菌的基因组的单拷贝集成。确定和优化的实验参数范围包括:(i)纯霉素B和抑制野生型真菌生长所需的纯血清素和(ii)转化对乙酰血酮诱导细菌的毒力基因的依赖性,以及(III )真菌 - 细菌共培养期的持续时间和(iv)用于后者的真菌分类和细菌细胞的浓度。该研究中开发的系统具有高效率稳定,含量高达400例,每10(6)个分类。这是C.Blifundus的转型协议的第一个报告,其可用性对于这一重要真菌的功能研究将是无价的。

著录项

  • 来源
    《Microbiological Research》 |2019年第2019期|共10页
  • 作者单位

    Univ Pretoria Dept Biochem Genet &

    Microbiol Forestry &

    Agr Biotechnol Inst ZA-0002 Pretoria South Africa;

    Univ Pretoria Dept Biochem Genet &

    Microbiol Forestry &

    Agr Biotechnol Inst ZA-0002 Pretoria South Africa;

    Univ Pretoria Dept Biochem Genet &

    Microbiol Forestry &

    Agr Biotechnol Inst ZA-0002 Pretoria South Africa;

    Univ Pretoria Dept Biochem Genet &

    Microbiol Forestry &

    Agr Biotechnol Inst ZA-0002 Pretoria South Africa;

    Univ Pretoria Dept Biochem Genet &

    Microbiol Forestry &

    Agr Biotechnol Inst ZA-0002 Pretoria South Africa;

    Univ Pretoria Dept Biochem Genet &

    Microbiol Forestry &

    Agr Biotechnol Inst ZA-0002 Pretoria South Africa;

  • 收录信息
  • 原文格式 PDF
  • 正文语种 eng
  • 中图分类 生物科学;
  • 关键词

    Agrobacterium; Ceratocystis; GFP; Hygromycin; Geneticin;

    机译:农杆菌;Ceratocystis;GFP;潮霉素;遗传霉素;

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