Improvement of bacterial two-hybrid vectors for detection of fusion proteins and transfer to pBAD-tandem affinity purification, calmodulin binding peptide, or 6-histidine tag vectors

Improvement of bacterial two-hybrid vectors for detection of fusion proteins and transfer to pBAD-tandem affinity purification, calmodulin binding peptide, or 6-histidine tag vectors

The original vectors of the bacterial two-hybrid technique developed by Karimova et al. in 1998 did not enable detection of the recombinant proteins. Here, we propose two methods resolving this problem, either using new plasmids containing the Flag epitope, or using a trick to detect the T18 domain...

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Veröffentlicht in:Proteomics (Weinheim) 2008-11, Vol.8 (22), p.4768-4771
Hauptverfasser: Battesti, Aurélia, Bouveret, Emmanuelle
Format: Artikel
Sprache:eng
Schlagworte:
Analytical, structural and metabolic biochemistry
Bacterial two-hybrid
Bacteriology
Biological and medical sciences
Blotting, Far-Western
Calmodulin-Binding Proteins - chemistry
Fundamental and applied biological sciences. Psychology
Histidine
Microbiology
Miscellaneous
Oligopeptides
Peptides - chemistry
Plasmids
Protein detection
Protein-protein interaction
Proteins
Recombinant Fusion Proteins - analysis
Two-Hybrid System Techniques
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Zusammenfassung:The original vectors of the bacterial two-hybrid technique developed by Karimova et al. in 1998 did not enable detection of the recombinant proteins. Here, we propose two methods resolving this problem, either using new plasmids containing the Flag epitope, or using a trick to detect the T18 domain of adenylate cyclase. Furthermore, we describe a set of vectors for TAP, CBP or 6-histidine tagging that possess the same cloning site as our two-hybrid vectors.
ISSN:1615-9853
1615-9861
DOI:10.1002/pmic.200800270