Abstract

We generated a single chain Fv fragment of an antibody (scFv) with a binding affinity of about 5 pm to a short peptide by applying rigorous directed evolution. Starting from a high affinity peptide binder, originally obtained by ribosome display from a murine library, we generated libraries of mutants with error-prone PCR and DNA shuffling and applied off-rate selection by using ribosome display. Crystallographic analysis of the scFv in its antigen-bound and free state showed that only few mutations, which do not make direct contact to the antigen, lead to a 500-fold affinity improvement over its potential germ line precursor. These results suggest that the affinity optimization of very high affinity binders is achieved by modulating existing interactions via subtle changes in the framework rather than by introducing new contacts. Off-rate selection in combination with ribosome display can evolve binders to the low picomolar affinity range even for peptide targets.

Highlights

  • Directed evolution of proteins in vitro has become a widely applied strategy to generate proteins with a desired property [1]

  • Ribosome display offers a significant advantage since bound binders must not be eluted, but the ribosomally bound mRNA can be recovered by the addition of chelating agents, which destabilize the ribosomal complex [1]

  • Library Construction—In a previous study, we selected a group of single chain Fv fragment of an antibody (scFv) fragments from a murine library by using ribosome display, a selection method that works entirely in vitro and allows the selection from very large libraries (Fig. 1)

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Summary

EXPERIMENTAL PROCEDURES

Expression and Purification of Single Chain Fv Fragments—The scFv1 genes were cloned into the periplasmic expression vector pAK400 [12] introducing a His tag, expressed in Escherichia coli SB536 [13],.

Free scFv
RESULTS
NDe ND
DISCUSSION
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