Generation of protein lineages with new sequence spaces by functional salvage screen

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A variety of different methods to generate diverse proteins, including random mutagenesis and recombination, are currently available and most of them accumulate the mutations on the target gene of a protein, whose sequence space remains unchanged. On the other hand, a pool of diverse genes, which is generated by random insertions, deletions and exchange of the homologous domains with different lengths in the target gene, would present the protein lineages resulting in new fitness landscapes. Here we report a method to generate a pool of protein variants with different sequence spaces by employing green fluorescent protein (GFP) as a model protein. This process, designated functional salvage screen (FSS), comprises the following procedures: a defective GFP template expressing no fluorescence is first constructed by genetically disrupting a predetermined region(s) of the protein and a library of GFP variants is generated from the defective template by incorporating the randomly fragmented genomic DNA from Escherichia coli into the defined region(s) of the target gene, followed by screening of the functionally salvaged, fluorescence-emitting GFPs. Two approaches, sequence-directed and PCR-coupled methods, were attempted to generate the library of GFP variants with new sequences derived from the genomic segments of E.coli. The functionally salvaged GFPs were selected and analyzed in terms of the sequence space and functional properties. The results demonstrate that the functional salvage process not only can be a simple and effective method to create protein lineages with new sequence spaces, but also can be useful in elucidating the involvement of a specific region(s) or domain(s) in the structure and function of protein.
Publisher
OXFORD UNIV PRESS
Issue Date
2001-09
Language
English
Article Type
Article
Keywords

GREEN FLUORESCENT PROTEIN; DIRECTED EVOLUTION; MOLECULAR EVOLUTION; ESCHERICHIA-COLI; HYBRID ENZYMES; FAMILY; DOMAIN; OLIGOMERIZATION; MUTAGENESIS; INSERTION

Citation

PROTEIN ENGINEERING, v.14, no.9, pp.647 - 654

ISSN
0269-2139
URI
http://hdl.handle.net/10203/18147
Appears in Collection
CH-Journal Papers(저널논문)BS-Journal Papers(저널논문)
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