Rapid and efficient construction of expression vectors and subsequent transformation are basic recombinant methods for the investigation of gene functionality. Although novel cloning methods have recently been developed, many laboratories worldwide continue to use traditional restriction digestion-ligation methods to construct expression vectors owing to financial constraints and the unavailability of appropriate vectors. We describe an improved restriction digestion-ligation (IRDL) cloning method that combines the advantage of directional cloning from double digestion-ligation with that of a low background observed by using a positive selection marker gene ccdB to facilitate digestion and ligation in a single tube. The IRDL cloning overcom...
International audienceCurrently, the most widely used strategies for molecular cloning are sticky-en...
Introducing PCR products into plasmids vectors is key for molecular techniques. Ideally cloning vect...
Direct cloning of PCR fragments by TA cloning or blunt end ligation are two simple methods which wou...
Rapid and efficient construction of expression vectors and subsequent transformation are basic recom...
<p>A, Schematic representation of one-step directional cloning of EGFP into a yeast expression vecto...
<p>A, Construct expression of one insert by IRDL cloning. The purified PCR products of GOI and expre...
<div><p>The precise assembly of specific DNA sequences is a critical technique in molecular biology....
The precise assembly of specific DNA sequences is a critical technique in molecular biology. Traditi...
Abstract The conventional procedure for the construction of recombinant expression vector of a targe...
<p>A, generation of sticky-end fragments and cloning into pWXY1.0 by IRDL cloning. The <i>JcDGAT2</i...
Plasmids are important tools for producing biological reagents and performing molecular biological i...
The precise assembly of specific DNA sequences is a critical technique in molecular biology. Traditi...
We report here a PCR-based cloning methodology that requires no post-PCR modifications such as restr...
Simple and low-cost recombinant enzyme-free seamless DNA cloning methods have recently become availa...
BACKGROUND: The cloning of gene sequences forms the basis for many molecular biological studies. One...
International audienceCurrently, the most widely used strategies for molecular cloning are sticky-en...
Introducing PCR products into plasmids vectors is key for molecular techniques. Ideally cloning vect...
Direct cloning of PCR fragments by TA cloning or blunt end ligation are two simple methods which wou...
Rapid and efficient construction of expression vectors and subsequent transformation are basic recom...
<p>A, Schematic representation of one-step directional cloning of EGFP into a yeast expression vecto...
<p>A, Construct expression of one insert by IRDL cloning. The purified PCR products of GOI and expre...
<div><p>The precise assembly of specific DNA sequences is a critical technique in molecular biology....
The precise assembly of specific DNA sequences is a critical technique in molecular biology. Traditi...
Abstract The conventional procedure for the construction of recombinant expression vector of a targe...
<p>A, generation of sticky-end fragments and cloning into pWXY1.0 by IRDL cloning. The <i>JcDGAT2</i...
Plasmids are important tools for producing biological reagents and performing molecular biological i...
The precise assembly of specific DNA sequences is a critical technique in molecular biology. Traditi...
We report here a PCR-based cloning methodology that requires no post-PCR modifications such as restr...
Simple and low-cost recombinant enzyme-free seamless DNA cloning methods have recently become availa...
BACKGROUND: The cloning of gene sequences forms the basis for many molecular biological studies. One...
International audienceCurrently, the most widely used strategies for molecular cloning are sticky-en...
Introducing PCR products into plasmids vectors is key for molecular techniques. Ideally cloning vect...
Direct cloning of PCR fragments by TA cloning or blunt end ligation are two simple methods which wou...