High-affinity lamprey VLRA and VLRB monoclonal antibodies

Lamprey are members of the ancestral vertebrate taxon (jawless fish), which evolved rearranging antigen receptors convergently with the jawed vertebrates. But instead of Ig superfamily domains, lamprey variable lymphocyte receptors (VLRs) consist of highly diverse leucine-rich repeats. Although VLRs...

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Bibliographic Details
Published in:Proceedings of the National Academy of Sciences - PNAS 2009-08, Vol.106 (31), p.12891-12896
Main Authors: Tasumi, Satoshi, Velikovsky, C. Alejandro, Xu, Gang, Gai, S. Annie, Wittrup, K. Dane, Flajnik, Martin F, Mariuzza, Roy A, Pancer, Zeev
Format: Article
Language:English
Subjects:
Adaptation, Physiological
Animals
Antibodies
Antibodies, Monoclonal - immunology
Antibody Affinity
Antigens
Base Sequence
Biological Sciences
Biotechnology
Health care industry
Immunoglobulins
Lampreys - immunology
Libraries
Lymphocyte receptors
Lymphocytes
Molecular Sequence Data
Monoclonal antibodies
Petromyzontidae
Proteins - immunology
Receptors
Receptors, Antigen - immunology
Receptors, Antigen - physiology
Titration
Vertebrates
Yeasts
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Summary:Lamprey are members of the ancestral vertebrate taxon (jawless fish), which evolved rearranging antigen receptors convergently with the jawed vertebrates. But instead of Ig superfamily domains, lamprey variable lymphocyte receptors (VLRs) consist of highly diverse leucine-rich repeats. Although VLRs represent the only known adaptive immune system not based on Ig, little is known about their antigen-binding properties. Here we report robust plasma VLRB responses of lamprey immunized with hen egg lysozyme and β-galactosidase (β-gal), demonstrating adaptive immune responses against soluble antigens. To isolate monoclonal VLRs, we constructed large VLR libraries from antigen-stimulated and naïve animals in a novel yeast surface-display vector, with the VLR C-terminally fused to the yeast Flo1p surface anchor. We cloned VLRB binders of lysozyme, β-gal, cholera toxin subunit B, R-phycoerythrin, and B-trisaccharide antigen, with dissociation constants up to the single-digit picomolar range, equivalent to those of high-affinity IgG antibodies. We also isolated from a single lamprey 13 anti-lysozyme VLRA clones with affinities ranging from low nanomolar to mid-picomolar. All of these VLRA clones were closely related in sequence, differing at only 15 variable codon positions along the 244-residue VLR diversity region, which augmented antigen-binding affinity up to 100-fold. Thus, VLRs can provide a protective humoral antipathogen shield. Furthermore, the broad range of nominal antigens that VLRs can specifically bind, and the affinities achieved, indicate a functional parallelism between LRR-based and Ig-based antibodies. VLRs may be useful natural single-chain alternatives to conventional antibodies for biotechnology applications.
ISSN:0027-8424
1091-6490
DOI:10.1073/pnas.0904443106