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Merck

Two-dimensional high-throughput on-cell screening of immunoglobulins against broad antigen repertoires.

Communications biology (2024-07-11)
Yakov A Lomakin, Leyla A Ovchinnikova, Stanislav S Terekhov, Samir S Dzhelad, Igor Yaroshevich, Ilgar Mamedov, Anastasia Smirnova, Tatiana Grigoreva, Igor E Eliseev, Ioanna N Filimonova, Yuliana A Mokrushina, Victoria Abrikosova, Maria P Rubtsova, Nikita N Kostin, Maria A Simonova, Tatiana V Bobik, Natalia L Aleshenko, Alexander I Alekhin, Vitali M Boitsov, Hongkai Zhang, Ivan V Smirnov, Yuri P Rubtsov, Alexander G Gabibov
RESUMEN

Identifying high-affinity antibodies in human serum is challenging due to extremely low number of circulating B cells specific to the desired antigens. Delays caused by a lack of information on the immunogenic proteins of viral origin hamper the development of therapeutic antibodies. We propose an efficient approach allowing for enrichment of high-affinity antibodies against pathogen proteins with simultaneous epitope mapping, even in the absence of structural information about the pathogenic immunogens. To screen therapeutic antibodies from blood of recovered donors, only pathogen transcriptome is required to design an antigen polypeptide library, representing pathogen proteins, exposed on the bacteriophage surface. We developed a two-dimensional screening approach enriching lentiviral immunoglobulin libraries from the convalescent or vaccinated donors against bacteriophage library expressing the overlapping set of polypeptides covering the spike protein of SARS-CoV-2. This platform is suitable for pathogen-specific immunoglobulin enrichment and allows high-throughput selection of therapeutic human antibodies.

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Sigma-Aldrich
IgG from human serum, reagent grade, ≥95% (HPLC), buffered aqueous solution
Sigma-Aldrich
Anticuerpo de cabra anti-IgG humana, Fc, conjugado HRP, Chemicon®, from goat
Sigma-Aldrich
Anti-Human IgG (whole molecule) antibody produced in goat, IgG fraction of antiserum, buffered aqueous solution