AI Article Synopsis

  • The text discusses a new platform for creating antibodies with high effectiveness and diversity, building on a previously established single-chain fragment (scFv) library that used clinical antibodies as a base.
  • This advancement involves using Fab phage display followed by scFab yeast display, resulting in better expression balance of antibody chains and improved conversion rate to IgG antibodies, combining the benefits of scFvs and Fabs.
  • A quality-controlled Fab phage library was developed, showcasing its potential to produce a diverse range of binding scFabs with high efficiency, ultimately streamlining the path for these antibodies to become viable therapeutic options.

Article Abstract

We previously described an single-chain fragment (scFv) library platform originally designed to generate antibodies with excellent developability properties. The platform design was based on the use of clinical antibodies as scaffolds into which replicated natural complementarity-determining regions purged of sequence liabilities were inserted, and the use of phage and yeast display to carry out antibody selection. In addition to being developable, antibodies generated using our platform were extremely diverse, with most campaigns yielding sub-nanomolar binders. Here, we describe a platform advancement that incorporates Fab phage display followed by single-chain antibody-binding fragment Fab (scFab) yeast display. The scFab single-gene format provides balanced expression of light and heavy chains, with enhanced conversion to IgG, thereby combining the advantages of scFvs and Fabs. A meticulously engineered, quality-controlled Fab phage library was created using design principles similar to those used to create the scFv library. A diverse panel of binding scFabs, with high conversion efficiency to IgG, was isolated against two targets. This study highlights the compatibility of phage and yeast display with a Fab semi-synthetic library design, offering an efficient approach to generate drug-like antibodies directly, facilitating their conversion to potential therapeutic candidates.

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Source
http://www.ncbi.nlm.nih.gov/pmc/articles/PMC11352698PMC
http://dx.doi.org/10.1080/19420862.2024.2394230DOI Listing

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