We developed a generic method for high-throughput cloning in bacteria that are less amenable to conventional DNA manipulations. The method involves ligation-independent cloning in an intermediary Escherichia coli vector, which is rapidly converted via vector-backbone exchange (VBEx) into an organism-specific plasmid ready for high-efficiency transformation. We demonstrated VBEx proof of principle for Lactococcus lactis, but the method can be adapted to all organisms for which plasmids are available.</p
Multiplex genome engineering is a standalone recombineering tool for large-scale programming and acc...
The 5.5 kb high-copy number cryptic plasmid pDI25 from Lactococcus lactis subsp. lactis 5136 was iso...
A tool kit of vectors was designed to manipulate and express genes from a wide range of gram-negativ...
We developed a generic method for high-throughput cloning in bacteria that are less amenable to conv...
Background: Homologous recombination mediated by the lambda-Red genes is a common method for making ...
<div><p>A robust method for the <i>in vivo</i> cloning of large gene clusters was developed based on...
Use of Escherichia coli bacteria as a host for high-level expression of cloned genes has become comm...
AbstractTargeted mutagenesis is one of the major tools for determining the function of a given gene ...
Here we present a modification of the widely used pET29 expression vector for use in rapid and strai...
Plasmid pSEUDO and derivatives were used to show that llmg_pseudo_10 in Lactococcus lactis MG1363 an...
Plasmids are important vectors for the transfer of genetic material among microbes. The transfer of ...
In the pUC18-derived integration plasmid pML336 there is a 5.3-kb chromosomal DNA fragment that carr...
A robust method for the in vivo cloning of large gene clusters was developed based on homologous rec...
AbstractThe genetic modification of primary bacterial disease isolates is challenging due to the lac...
AbstractCloning by homologous recombination (HR) in Saccharomyces cerevisiae is an extremely efficie...
Multiplex genome engineering is a standalone recombineering tool for large-scale programming and acc...
The 5.5 kb high-copy number cryptic plasmid pDI25 from Lactococcus lactis subsp. lactis 5136 was iso...
A tool kit of vectors was designed to manipulate and express genes from a wide range of gram-negativ...
We developed a generic method for high-throughput cloning in bacteria that are less amenable to conv...
Background: Homologous recombination mediated by the lambda-Red genes is a common method for making ...
<div><p>A robust method for the <i>in vivo</i> cloning of large gene clusters was developed based on...
Use of Escherichia coli bacteria as a host for high-level expression of cloned genes has become comm...
AbstractTargeted mutagenesis is one of the major tools for determining the function of a given gene ...
Here we present a modification of the widely used pET29 expression vector for use in rapid and strai...
Plasmid pSEUDO and derivatives were used to show that llmg_pseudo_10 in Lactococcus lactis MG1363 an...
Plasmids are important vectors for the transfer of genetic material among microbes. The transfer of ...
In the pUC18-derived integration plasmid pML336 there is a 5.3-kb chromosomal DNA fragment that carr...
A robust method for the in vivo cloning of large gene clusters was developed based on homologous rec...
AbstractThe genetic modification of primary bacterial disease isolates is challenging due to the lac...
AbstractCloning by homologous recombination (HR) in Saccharomyces cerevisiae is an extremely efficie...
Multiplex genome engineering is a standalone recombineering tool for large-scale programming and acc...
The 5.5 kb high-copy number cryptic plasmid pDI25 from Lactococcus lactis subsp. lactis 5136 was iso...
A tool kit of vectors was designed to manipulate and express genes from a wide range of gram-negativ...