A novel synthetic trivalent single chain variable fragment (tri-scFv) construction platform based on the SpyTag/SpyCatcher protein ligase system

Md Kausar Alam; Michelle Brabant; Raja Solomon Viswas; Kris Barreto; Humphrey Fonge; C Ronald Geyer

doi:10.1186/s12896-018-0466-6

A novel synthetic trivalent single chain variable fragment (tri-scFv) construction platform based on the SpyTag/SpyCatcher protein ligase system

BMC Biotechnol. 2018 Sep 10;18(1):55. doi: 10.1186/s12896-018-0466-6.

Authors

Md Kausar Alam¹, Michelle Brabant², Raja Solomon Viswas³, Kris Barreto¹, Humphrey Fonge³, C Ronald Geyer⁴

Affiliations

¹ Department of Pathology and Laboratory Medicine, College of Medicine, University of Saskatchewan, Room 2841, Royal University Hospital, 103 Hospital Drive, Saskatoon, S7N 0W8, Canada.
² Department of Biochemistry, College of Medicine, University of Saskatchewan, Saskatoon, SK, S7N 5E5, Canada.
³ Medical Imaging, University of Saskatchewan, Saskatoon, SK, S7N 5E5, Canada.
⁴ Department of Pathology and Laboratory Medicine, College of Medicine, University of Saskatchewan, Room 2841, Royal University Hospital, 103 Hospital Drive, Saskatoon, S7N 0W8, Canada. ron.geyer@usask.ca.

Abstract

Background: Advances in antibody engineering provide strategies to construct recombinant antibody-like molecules with modified pharmacokinetic properties. Multermerization is one strategy that has been used to produce antibody-like molecules with two or more antigen binding sites. Multimerization enhances the functional affinity (avidity) and can be used to optimize size and pharmacokinetic properties. Most multimerization strategies involve genetically fusing or non-covalently linking antibody fragments using oligomerization domains. Recent studies have defined guidelines for producing antibody-like molecules with optimal tumor targeting properties, which require intermediates size (70-120 kDa) and bi- or tri-valency.

Results: We described a highly modular antibody-engineering platform for rapidly constructing synthetic, trivalent single chain variable fragments (Tri-scFv) using the SpyCatcher/SpyTag protein ligase system. We used this platform to construct an anti-human epidermal growth factor receptor 3 (HER3) Tri-scFv. We generated the anti-HER3 Tri-scFv by genetically fusing a SpyCatcher to the C-terminus of an anti-HER3 scFv and ligating it to a synthetic Tri-SpyTag peptide. The anti-HER3 Tri-scFv bound recombinant HER3 with an apparent K_D of 2.67 nM, which is approximately 12 times lower than the K_D of monomeric anti-HER3 scFv (31.2 nM). Anti-HER3 Tri-scFv also bound endogenous cell surface expressed HER3 stronger than the monomer anti-HER3 scFv.

Conclusion: We used the SpyTag/SpyCatcher protein ligase system to ligate anti-HER3 scFv fused to a SpyCatcher at its C-termini to a Tri-SpyTag to construct Tr-scFv. This system allowed the construction of a Tri-scFv with all the scFv antigen-binding sites pointed outwards. The anti-HER3 Tri-scFv bound recombinant and endogenously expressed HER3 with higher functional affinity (avidity) than the monomeric anti-HER3 scFv. The Tri-scFv had the size, valency, and functional affinity that are desired for therapeutic and imaging applications. Use of the SpyTag/SpyCatcher protein ligase system allows Tri-scFvs to be rapidly constructed in a simple, modular manner, which can be easily applied to scFvs or other antibody fragments targeting other antigens.

Keywords: Avidity; HER3; Multimerization; SpyTag/SpyCatcher; Tri-scFv; scFv.

Publication types

Evaluation Study
Research Support, Non-U.S. Gov't

MeSH terms

Antibody Affinity
Humans
Ligases / chemistry*
Peptides / genetics*
Peptides / immunology
Protein Engineering / instrumentation
Protein Engineering / methods*
Receptor, ErbB-3 / genetics
Receptor, ErbB-3 / immunology*
Recombinant Fusion Proteins / genetics
Recombinant Fusion Proteins / immunology
Single-Chain Antibodies / genetics*
Single-Chain Antibodies / immunology

Substances

Peptides
Recombinant Fusion Proteins
Single-Chain Antibodies
SpyTag peptide
ERBB3 protein, human
Receptor, ErbB-3
Ligases