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Transformation of the phytopathogenic bacterium Clavibacter michiganense subsp. michiganense by electroporation and development of a cloning vector.

机译:植物病原性细菌密歇根细杆菌亚种的转化。通过电穿孔和克隆载体的发展。

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摘要

We constructed a cloning vector for use in the plant pathogenic bacterium Clavibacter michiganense subsp. michiganense. The vector pDM100 consists of a 3.2-kb restriction fragment of the Clavibacter plasmid pCM1 joined to a pBR325 derivative carrying the neomycin phosphotransferase of transposon Tn5 and the gentamicin acetyltransferase of Tn1696. Both antibiotic resistance genes are efficiently expressed in C. michiganense subsp. michiganense. Although polyethylene glycol-mediated transfection of spheroplasts with the DNA of the C. michiganense subsp. michiganense-specific bacteriophage CMP1 yielded about 3 x 10(3) transfectants per microgram of DNA, in transformations with plasmid DNA only a very few transformants were obtained. However, the transformation efficiency could be improved by electroporation of intact cells, giving about 2 x 10(3) transformants per microgram of plasmid DNA. Since a transformation procedure and a cloning vector are now available, pathogenicity in C. michiganense subsp. michiganense can now be analyzed genetically.
机译:我们构建了一种克隆载体,可用于植物病原细菌密歇根州克氏杆菌亚种。密歇根州。载体pDM100由连接至带有转座子Tn5的新霉素磷酸转移酶和庆大霉素乙酰基转移酶的tBR1的pBR325衍生物的杆状细菌质粒pCM1的3.2kb限制性片段组成。两种抗生素抗性基因均在密歇根梭菌亚种中有效表达。密歇根州。虽然聚乙二醇介导的原生质球菌亚种DNA转染原生质球。密歇根州特定的噬菌体CMP1每微克DNA产生约3 x 10(3)个转染子,在质粒DNA的转化中,只获得了很少的转化子。但是,可以通过对完整细胞进行电穿孔来提高转化效率,每微克质粒DNA可产生约2 x 10(3)个转化子。由于现在有转化方法和克隆载体,所以密歇根梭菌亚种中的致病性。密歇根州现在可以进行遗传分析。

著录项

  • 作者

    Meletzus, D; Eichenlaub, R;

  • 作者单位
  • 年度 1991
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  • 原文格式 PDF
  • 正文语种 en
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