2006
DOI: 10.1128/aem.02750-05
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Phage Display of an Intracellular Carboxylesterase of Bacillus subtilis : Comparison of Sec and Tat Pathway Export Capabilities

Abstract: Using the phage display technology, a protein can be displayed at the surface of bacteriophages as a fusion to one of the phage coat proteins. Here we describe development of this method for fusion of an intracellular carboxylesterase of Bacillus subtilis to the phage minor coat protein g3p. The carboxylesterase gene was cloned in the g3p-based phagemid pCANTAB 5E upstream of the sequence encoding phage g3p and downstream of a signal peptide-encoding sequence. The phage-bound carboxylesterase was correctly fol… Show more

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Cited by 19 publications
(11 citation statements)
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“…Fisher et al [159] addressed this very issue and, using an ingenious tripartite fusion with a Tat signal at the N-terminus, a β-lactamase at the C-terminus and the protein of interest sandwiched in the middle, were able to actively select for variant fusion proteins with increased water solubility. The Tat system has also been exploited in several other protein-engineering projects, including a novel two-hybrid system for screening for protein-protein interactions [160], production and engineering of single-chain antibodies [64,161] and for phage display [162,163]. Some bacteria, in particular Gram-positive Streptomyces spp., export large numbers of diverse substrates by the Tat system and might be ideal hosts for the heterologous production of pharmaceutically important proteins that are incompatible with secretion by the Sec pathway [17].…”
Section: Medical and Biotechnological Applicationsmentioning
confidence: 99%
“…Fisher et al [159] addressed this very issue and, using an ingenious tripartite fusion with a Tat signal at the N-terminus, a β-lactamase at the C-terminus and the protein of interest sandwiched in the middle, were able to actively select for variant fusion proteins with increased water solubility. The Tat system has also been exploited in several other protein-engineering projects, including a novel two-hybrid system for screening for protein-protein interactions [160], production and engineering of single-chain antibodies [64,161] and for phage display [162,163]. Some bacteria, in particular Gram-positive Streptomyces spp., export large numbers of diverse substrates by the Tat system and might be ideal hosts for the heterologous production of pharmaceutically important proteins that are incompatible with secretion by the Sec pathway [17].…”
Section: Medical and Biotechnological Applicationsmentioning
confidence: 99%
“…For protein localization assays, pvdP_H6 was PCR amplified from pET26B-pvdP_H6 and cloned in the shuttle vector pME6032 (17), obtaining the plasmid pME-pvdP_H6. This plasmid was then transformed in the E. coli HB2151 wild type (WT) and the E. coli HB2151 ⌬tatC mutant (18).…”
Section: Methodsmentioning
confidence: 99%
“…This plasmid was electroporated into the E. coli HB2151 WT and the E. coli HB2151 ⌬tatC mutant (18). The two strains were grown overnight in 2ϫ TY of LB medium at 37°C and 250 rpm.…”
Section: Pvdp Cell Localization (I) Cell Fractionationmentioning
confidence: 99%
See 1 more Smart Citation
“…[27,40,41]. The examples of enzymes that have been phage-displayed to study their action mechanisms include trypsin [42], b-lactamases [43], metallo-b-lactamase b LII from Bacillus cereus [44], amylases [45], subtilisin [46,47], and carboxylesterase of Bacillus subtilis [48]. The mutant variant of 4 0 -phosphopantetheinyl transferase showing a more than 300-fold increase in catalytic efficiency toward 3 0 -dephospho-CoA was selected by co-displaying peptide substrates and enzyme mutants on the M13 phage surface as fusions to the phage capsid protein pIII [49].…”
Section: Discussionmentioning
confidence: 99%