Construction of IgG–Fab2 bispecific antibody via intein-mediated protein trans-splicing reaction

Author:

Yamada Risa,Nakahara Ishin,Kumagai Izumi,Asano Ryutaro,Nakanishi Takeshi,Makabe Koki

Abstract

AbstractA bispecific antibody (bsAb) is a class of engineered antibody molecules that simultaneously binds to two different antigens by having two kinds of antigen-binding domains. One of the major obstacles for the bsAb production is the incorrect chain-pairing problem, wherein each heavy and light chain should form pairings with the correct counterpart’s chains, but the structural similarity of the incorrect partners also forms the incorrect pairings. This study aimed to demonstrate a bsAb construction method using intein-mediated protein trans-splicing to create IgG–Fab2–type bsAbs, which is a modified antibody with a structure in which two additional Fabs are linked to the N-terminus of the heavy chain of an IgG molecule. The chain-paring problem between a heavy chain and a light chain is circumvented by separate expression and purification of the IgG part and the Fab part. We found that the deletion of a possible glycosylation residue improved the reaction yield and side-reaction cleavage in the protein ligation step. The resulting bsAb, IgG–Fab2 (Her2/CD3), demonstrated target binding activity and cytotoxicity mediated by activated T cells. These results indicate that the use of the protein ligation to produce the IgG–Fab2 type bsAb will expand the bsAb production method.

Funder

Grant-in-Aid from JSPS for Scientific Research, KAKENHI Category B

AMED

JST PRESTO

Takahashi Industrial and Economic Research Foundation

Hokuto Foundation for Bioscience, Japan

Foundation for Applied Enzymology

Astellas Foundation for Research on Metabolic Disorders

Publisher

Springer Science and Business Media LLC

Subject

Multidisciplinary

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