Add to ORKGWe developed a simple, rapid and reliable method to delete DNA fragments in plasmids using a polymerase chain reaction based amplification of the circular DNA sequence that excludes the fragment to be deleted. The primers are designed to contain a non-complementary 5' sequence consisting of a restriction enzyme target sequence. Following PCR amplification, the plasmid is digested with Dpn I to eliminate the template DNA, with the chosen restriction enzyme, and ligated. The only limitation is the selection of the restriction enzyme target sequence that must not be present in the original plasmid. The method is straightforward in its execution and success relies on a meticulous primer design that permits us obtain 100% of transformants c...
A procedure for extracting plasmid DNA from bacterial cells 1s described. The method 1s simple enoug...
New bioactive proteins need to be screened from various microorganisms for the increasing need for i...
We describe a simple PCR-based method for the isolation of genomic DNA that lies adjacent to a known...
We developed a simple, rapid and reliable method to delete DNA fragments in plasmids using a polymer...
We developed a simple, rapid and reliable method to delete DNA fragments in plasmids using a polymer...
The PCR-mediated plasmid DNA deletion method is a simple approach to delete DNA sequences from plasm...
This data article contains supplementary figures and methods to the research article entitled, “Mult...
To generate DNA deletions, a tandem array of class IIS restriction enzyme recognition sites was clon...
A simple procedure is described for the efficient deletion of large DNA sequences. The method involv...
A simple and efficient method is described for the isolation of extension fragments of known DNA seq...
A simple and efficient method is described for the isolation of extension fragments of known DNA seq...
Plasmids are important tools for producing biological reagents and performing molecular biological i...
We describe a new rapid and efficient polymerase chain reaction (PCR)-based site-directed mutagenesi...
Site-specific mutagenesis at one or multiple sites has recently become an invaluable strategy in fun...
Site-specific mutagenesis at one or multiple sites has recently become an invaluable strategy in fun...
A procedure for extracting plasmid DNA from bacterial cells 1s described. The method 1s simple enoug...
New bioactive proteins need to be screened from various microorganisms for the increasing need for i...
We describe a simple PCR-based method for the isolation of genomic DNA that lies adjacent to a known...
We developed a simple, rapid and reliable method to delete DNA fragments in plasmids using a polymer...
We developed a simple, rapid and reliable method to delete DNA fragments in plasmids using a polymer...
The PCR-mediated plasmid DNA deletion method is a simple approach to delete DNA sequences from plasm...
This data article contains supplementary figures and methods to the research article entitled, “Mult...
To generate DNA deletions, a tandem array of class IIS restriction enzyme recognition sites was clon...
A simple procedure is described for the efficient deletion of large DNA sequences. The method involv...
A simple and efficient method is described for the isolation of extension fragments of known DNA seq...
A simple and efficient method is described for the isolation of extension fragments of known DNA seq...
Plasmids are important tools for producing biological reagents and performing molecular biological i...
We describe a new rapid and efficient polymerase chain reaction (PCR)-based site-directed mutagenesi...
Site-specific mutagenesis at one or multiple sites has recently become an invaluable strategy in fun...
Site-specific mutagenesis at one or multiple sites has recently become an invaluable strategy in fun...
A procedure for extracting plasmid DNA from bacterial cells 1s described. The method 1s simple enoug...
New bioactive proteins need to be screened from various microorganisms for the increasing need for i...
We describe a simple PCR-based method for the isolation of genomic DNA that lies adjacent to a known...