A recombination based method to rapidly assess specificity of two- hybrid clones in yeast | Zendy

Robert Petermann | Zendy

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A recombination based method to rapidly assess specificity of two- hybrid clones in yeast

Author(s) -

Robert Petermann

Publication year - 1998

Publication title -

nucleic acids research

Language(s) - English

Resource type - Journals

SCImago Journal Rank - 9.008

H-Index - 537

eISSN - 1362-4954

pISSN - 0305-1048

DOI - 10.1093/nar/26.9.2252

Subject(s) - biology , insert (composites) , plasmid , yeast , two hybrid screening , dna , genomic library , cloning (programming) , gene , genetics , molecular cloning , saccharomyces cerevisiae , recombinant dna , reporter gene , computational biology , microbiology and biotechnology , peptide sequence , gene expression , mechanical engineering , programming language , computer science , engineering

The yeast two-hybrid system is frequently used to identify protein-protein interactions. Confirming the specificity of candidate clones requires separation and isolation of yeast plasmids, propagation in bacteria and testing combinations of DNA-binding and activation domain hybrids in yeast. In order to simplify this procedure, we developed a rapid method based on PCR amplification of library insert DNAs and in vivo cloning into the activation domain hybrid vector. Reporter gene activity is assayed in parallel for combinations with different DNA-binding domain hybrids. Further characterization of inserts does not require plasmid isolation and intermediate hosts.

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