TRANSFER OF PLASMID DNA TO BREVIBACTERIUM-LACTOFERMENTUM BY ELECTROTRANSFORMATION

被引:36
作者
BONNASSIE, S
BURINI, JF
OREGLIA, J
TRAUTWETTER, A
PATTE, JC
SICARD, AM
机构
[1] CNRS,CTR RECH BIOCHIM & GENET CELLULAIRES,118 ROUTE NARBONNE,F-31062 TOULOUSE,FRANCE
[2] INST UNIV TECHNOL,MICROBIOL FROID LAB,F-27000 EVREUX,FRANCE
[3] LAB GENET & PHYSIOL MICROBIENNES,F-35042 RENNES,FRANCE
[4] CNRS,CHIM BACTERIENNE LAB,CNRS,F-13402 MARSEILLE 9,FRANCE
来源
JOURNAL OF GENERAL MICROBIOLOGY | 1990年 / 136卷
关键词
D O I
10.1099/00221287-136-10-2107
中图分类号
Q93 [微生物学];
学科分类号
071005 ; 100705 ;
摘要
The Escherichia coli-Brevibacterium lactofermentum shuttle vector pBLA was introduced into intact cells of B. lactofermentum by electrotransformation. Several parameters of this procedure such as voltage and cell concentration were analysed. Optimal conditions gave an efficiency of 106 transformants per μg of DNA. Two recalcitrant strains could be electrotransformed when an ampicillin pretreatment step was used. Electrotransformation experiments using DNAase or different structural forms of plasmid DNA showed that the electrotransformation process is quite different from natural transformation involving competence development. Restriction-modification-proficient B. lactofermentum could be efficiently electrotransformed with pBLA DNA isolated from E. coli. This restriction-modification system therefore seems to be overcome by electrotransformation. Thus electrotransformation may efficiently replace the protoplast bacterial transformation method.
引用
收藏
页码:2107 / 2112
页数:6
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