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Family of shuttle vectors for ruminal Bacteroides.
Wong, Cheryl M; Klieve, Athol V; Hamdorf, Brenton J; Schafer, Darren J; Bräu, Lambert; Seet, Shawn G M; Gregg, Keith.
  • Wong CM; Rumen Biotech, Murdoch University, Murdoch, WA, Australia.
J Mol Microbiol Biotechnol ; 5(2): 123-32, 2003.
Article en En | MEDLINE | ID: mdl-12736534
ABSTRACT
A family of shuttle plasmids was constructed for genetic transformation of Escherichia coli and of ruminal Bacteroides strains AR20 and AR29. Plasmids were based on the replicon from Bacteroides plasmid pBI191 and were designed for studies of chromosomal integration (pBA), for the identification and study of Bacteroides gene promoters (pPPR) and for the expression of heterologous genes in Bacteroides (pBAC). Electroporation efficiency of Bacteroides was up to 10(5) transformants/microg plasmid, depending on the source of the DNA. The largest plasmid, pBA, was maintained at approximately 8 copies per cell in AR20 and did not measurably alter in vitro growth of transformed cells. In the current work, pBA did not integrate into the chromosomes of AR20 or AR29. The ability of plasmid pPPR to select promoter sequences was demonstrated by removal and replacement of promoters that activate the clindamycin resistance gene. The suitability of pBAC for expression of heterologous genes was demonstrated by expression of the Moraxella species fluoroacetate dehalogenase gene H1 to give intracellular activity of 7 nmol fluoride released/min/mg soluble protein in AR20 and 4 nmol/min/mg in AR29. Spontaneous loss of pBAC under non-selective conditions was 0.11-0.165% per generation, significantly less than loss of the native Bacteroides plasmid pBI191, which was lost at 0.53% per generation.
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Banco de datos: MEDLINE Asunto principal: Plásmidos / Rumen / Transformación Bacteriana / Bacteroides / Vectores Genéticos / Hidrolasas Tipo de estudio: Evaluation_studies Límite: Animals Idioma: En Año: 2003 Tipo del documento: Article
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Banco de datos: MEDLINE Asunto principal: Plásmidos / Rumen / Transformación Bacteriana / Bacteroides / Vectores Genéticos / Hidrolasas Tipo de estudio: Evaluation_studies Límite: Animals Idioma: En Año: 2003 Tipo del documento: Article