A range of specific and unusual biological pathways are found in Gram-negative bacteria. It is possible to express the genes involved in these processes in Escherichia coli, however, some genes prove lethal when cloned into high copy number vectors in common usage. Conversely, various genetic functions remain silent in E. coli and require to be transferred into their original host for expression and subsequent analysis. To facilitate the cloning and the characterisation of bacterial genes, we have constructed CcdB 'positive-selection' vectors that possess one or more of the following properties: (i) low or medium copy number; (ii) narrow or broad replication host range; (iii) conjugational mobilisation. In this communication, we illustrate ...
Creation of defined genetic mutations is a power-ful method for dissecting mechanisms of bacterial d...
A simple procedure for cloning and stable insertion of foreign genes into the chromosomes of gram-ne...
Selbitschka W, NIEMANN S, Pühler A. CONSTRUCTION OF GENE REPLACEMENT VECTORS FOR GRAM- BACTERIA USIN...
Plasmids pKIL18/19 are positive-selection cloning vectors containing an active cytotoxic ccdB gene u...
Introducing PCR products into plasmids vectors is key for molecular techniques. Ideally cloning vect...
International audiencePlasmids play a central role in engineering recombinant bacteria because they ...
AbstractThe genetic modification of primary bacterial disease isolates is challenging due to the lac...
SCHAEFER A, Tauch A, JAEGER W, Kalinowski J, THIERBACH G, Pühler A. Small mobilizable multi-purpose ...
Most plasmids replicate only within a particular genus or family.Here we describe an engineered high...
Lack of suitable gene transfer techniques hampers genetic improvement and analysis of several indus...
Bacteria Conjugation is the primary means of transfer of genetic material among prokaryotes. We have...
Production of recombinant DNA in bacterial cells is an essential technique in molecular biology. Pla...
Infections due to antibiotic-resistant (AbR) bacteria are a major cause of morbidity and mortality t...
Production of recombinant DNA in bacterial cells is an essential technique in molecular biology. Pla...
Although many vectors exist for Escherichia coli and closely related species, there are few broad ho...
Creation of defined genetic mutations is a power-ful method for dissecting mechanisms of bacterial d...
A simple procedure for cloning and stable insertion of foreign genes into the chromosomes of gram-ne...
Selbitschka W, NIEMANN S, Pühler A. CONSTRUCTION OF GENE REPLACEMENT VECTORS FOR GRAM- BACTERIA USIN...
Plasmids pKIL18/19 are positive-selection cloning vectors containing an active cytotoxic ccdB gene u...
Introducing PCR products into plasmids vectors is key for molecular techniques. Ideally cloning vect...
International audiencePlasmids play a central role in engineering recombinant bacteria because they ...
AbstractThe genetic modification of primary bacterial disease isolates is challenging due to the lac...
SCHAEFER A, Tauch A, JAEGER W, Kalinowski J, THIERBACH G, Pühler A. Small mobilizable multi-purpose ...
Most plasmids replicate only within a particular genus or family.Here we describe an engineered high...
Lack of suitable gene transfer techniques hampers genetic improvement and analysis of several indus...
Bacteria Conjugation is the primary means of transfer of genetic material among prokaryotes. We have...
Production of recombinant DNA in bacterial cells is an essential technique in molecular biology. Pla...
Infections due to antibiotic-resistant (AbR) bacteria are a major cause of morbidity and mortality t...
Production of recombinant DNA in bacterial cells is an essential technique in molecular biology. Pla...
Although many vectors exist for Escherichia coli and closely related species, there are few broad ho...
Creation of defined genetic mutations is a power-ful method for dissecting mechanisms of bacterial d...
A simple procedure for cloning and stable insertion of foreign genes into the chromosomes of gram-ne...
Selbitschka W, NIEMANN S, Pühler A. CONSTRUCTION OF GENE REPLACEMENT VECTORS FOR GRAM- BACTERIA USIN...