Abstract The conventional procedure for the construction of recombinant expression vector of a target gene includes PCR cloning and restriction enzyme mediated subcloning, which is time-consuming and sometimes troublesome because of the inefficiency of ligation. A variety of ligase-independent PCR cloning strategies have been developed, but they either involve complicated PCR procedures or need other DNA modifying enzymes. In this study, we report the design, and construction of an omnipotent expression vector pOmni, with which a target gene can be easily cloned through innovative selection-free PCR recombination cloning strategy with only one pair of primer and two times of PCR in one work day, without using any restriction enzymes, ligase...
Abstract Background Recent developments in metabolic engineering and the need for expanded compatibi...
Herein, we describe a novel cloning strategy for PCR-amplified DNA which employs the type IIs restri...
For promoter studies the cloning, subcloning and transfer to different plasmid vectors usually requi...
Introducing PCR products into plasmids vectors is key for molecular techniques. Ideally cloning vect...
Use of Escherichia coli bacteria as a host for high-level expression of cloned genes has become comm...
Rapid and efficient construction of expression vectors and subsequent transformation are basic recom...
Rapid and efficient construction of expression vectors and subsequent transformation are basic recom...
Background: Expression and purification of correctly folded proteins typically require screening of ...
A multipurpose vector vas constructed which can be used for cloning DNA fragments of about 20 kb gen...
PCR fragments and linear vectors containing overlapping ends are easily assembled into a propagative...
A vector system is presented that allows generation of E. coli co-expression clones by a standardize...
<div><p>A robust method for the <i>in vivo</i> cloning of large gene clusters was developed based on...
Production of recombinant proteins is the starting point for biochemical and biophysical analyses an...
Most conditional expression vectors designed for mammalian cells have been valuable systems for stud...
A vector system is presented that allows generation of E. coli co-expression clones by a standardize...
Abstract Background Recent developments in metabolic engineering and the need for expanded compatibi...
Herein, we describe a novel cloning strategy for PCR-amplified DNA which employs the type IIs restri...
For promoter studies the cloning, subcloning and transfer to different plasmid vectors usually requi...
Introducing PCR products into plasmids vectors is key for molecular techniques. Ideally cloning vect...
Use of Escherichia coli bacteria as a host for high-level expression of cloned genes has become comm...
Rapid and efficient construction of expression vectors and subsequent transformation are basic recom...
Rapid and efficient construction of expression vectors and subsequent transformation are basic recom...
Background: Expression and purification of correctly folded proteins typically require screening of ...
A multipurpose vector vas constructed which can be used for cloning DNA fragments of about 20 kb gen...
PCR fragments and linear vectors containing overlapping ends are easily assembled into a propagative...
A vector system is presented that allows generation of E. coli co-expression clones by a standardize...
<div><p>A robust method for the <i>in vivo</i> cloning of large gene clusters was developed based on...
Production of recombinant proteins is the starting point for biochemical and biophysical analyses an...
Most conditional expression vectors designed for mammalian cells have been valuable systems for stud...
A vector system is presented that allows generation of E. coli co-expression clones by a standardize...
Abstract Background Recent developments in metabolic engineering and the need for expanded compatibi...
Herein, we describe a novel cloning strategy for PCR-amplified DNA which employs the type IIs restri...
For promoter studies the cloning, subcloning and transfer to different plasmid vectors usually requi...