International Immunology, Vol 9, 1311-1318, Copyright © 1997 by Oxford University Press
J Farrar, S Portolano, N Willcox, A Vincent, L Jacobson, J Newsom-Davis, B Rapoport and SM McLachlan
The muscle weakness in myasthenia gravis (MG) is caused by heterogeneous
high-affinity IgG autoantibodies to the nicotinic acetylcholine receptor
(AChR), a complex ion channel glycoprotein. These antibodies are clearly
responsible for reducing AChR numbers at the neuromuscular junction in
myasthenia; however, the origins, diversity, specificity and pathogenicity
of individual antibodies have not yet been established. We have cloned and
characterized four different AChR-specific Fab from an MG patient's thymus
by screening an IgG1/kappa gene combinatorial lambda phage library with
soluble human AChR labeled with [125I] alpha-bungarotoxin. Unlike most
previously cloned human antibodies, all four Fab immunoprecipitated soluble
human muscle AChR. Two Fab strongly inhibited binding of mAb to the main
immunogenic region on the alpha subunits and one Fab bound to an epitope on
the fetal-specific gamma subunit. In sensitivity and fine specificity,
these Fab resembled the anti-AChR antibodies found in many MG patients,
including the donor. The closest germline counterparts for their heavy
chains were in VH families 1, 3 and 4; however, there were many differences
consistent with an antigen-driven response of diverse B cell clones. The
combinatorial approach holds promise for further analysis of human
autoantibodies.
ARTICLES
Diverse Fab specific for acetylcholine receptor epitopes from a myasthenia gravis thymus combinatorial library
Institute of Molecular Medicine, Department of Clinical Neurology, University of Oxford, UK.
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