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Exploiting recombination in single bacteria to make large phage antibody libraries

SBLATTERO, DANIELE
•
Bradbury, Andrew
2000
  • journal article

Periodico
NATURE BIOTECHNOLOGY
Abstract
The creation of large phage antibody libraries has become an important goal in selecting antibodies against any antigen. Here we describe a method for making libraries so large that the complete diversity cannot be accessed using traditional phage technology. This involves the creation of a primary phage scFv library in a phagemid vector containing two nonhomologous lox sites. Contrary to the current dogma, we found that infecting Cre recombinase-expressing bacteria by such a primary library at a high multiplicity of infection results in the entry of many different phagemid into the cell. Exchange of Vh and Vl genes between such phagemids creates many new V h/Vl combinations, all of which are functional. On the basis of the observed recombination, the library is calculated to have a diversity of 3x1011. A library created using this method was validated by the selection of high affinity antibodies against a large number of different protein antigens
DOI
10.1038/71958
WOS
WOS:000084699900030
Archivio
http://hdl.handle.net/11368/2856418
info:eu-repo/semantics/altIdentifier/scopus/2-s2.0-0033987925
Diritti
metadata only access
Soggetti
  • Antibody engineering

  • Cre recombinase

  • Filamentous phage

  • Phage display

  • Recombination

  • Single-chain Fv (scFv...

  • Antibodie

  • Antibody Specificity

  • Antigen

  • Attachment Sites, Mic...

  • Bacteriophage

  • Binding Sites, Antibo...

  • Cloning, Molecular

  • Escherichia coli

  • Gene Rearrangement

  • Genetic Vector

  • Human

  • Immunoglobulin Fragme...

  • Integrase

  • Recombination, Geneti...

  • Reproducibility of Re...

  • Sequence Analysis, DN...

  • Antibody Diversity

  • Peptide Library

  • Viral Protein

  • Microbiology

Scopus© citazioni
276
Data di acquisizione
Jun 15, 2022
Vedi dettagli
Web of Science© citazioni
257
Data di acquisizione
Mar 16, 2024
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