Selection for improved subtiligases by phage display
AUTOR(ES)
Atwell, Shane
FONTE
The National Academy of Sciences
RESUMO
Engineering enzyme activity has been challenging because of uncertainties in structure–function relationships and difficulties in screening a large number of mutant enzymes. A product capture strategy using phage display is presented here for the selection of improved enzymes from a large library of variants (>109 independently derived mutants). Subtiligase, a double mutant of subtilisin BPN′ that catalyzes the ligation of peptides, was displayed on phage. Twenty-five active site residues were randomly mutated in groups of four or five to yield six different libraries that were independently sorted. Variants that ligated a biotin peptide onto their own extended N termini were selectively captured. Mutant subtiligases were identified that had increased ligase activity. The selection also yielded unexpected subtiligase mutants having residues known to improve the stability and oxidative resistance of wild-type subtilisin. These studies are exemplary for the use of phage to improve enzyme function when it is closely linked to a selectable catalytic event.
ACESSO AO ARTIGO
http://www.pubmedcentral.nih.gov/articlerender.fcgi?artid=22237Documentos Relacionados
- Expression cloning of cDNA by phage display selection.
- Selection of Recombinant Antibodies Specific for Pathogenic Streptococcus suis by Subtractive Phage Display
- An improved helper phage system for efficient isolation of specific antibody molecules in phage display
- Accelerating phage-display library selection by reversible and site-specific biotinylation
- Shotgun Phage Display - Selection for Bacterial Receptins or other Exported Proteins
