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*Substance via MeSH
Medline Plus Health Information
*Joint Disorders
*Salivary Gland Disorders
*Sjogren's Syndrome
The Journal of Immunology, 2001, 167: 5449-5456.
Copyright © 2001 by The American Association of Immunologists

Autoantibodies to the Amino-Terminal Fragment of {beta}-Fodrin Expressed in Glandular Epithelial Cells in Patients with Sjögren’s Syndrome1

Masataka Kuwana2,*, Tetsuroh Okano{dagger}, Yoko Ogawa*, Junichi Kaburaki{ddagger} and Yutaka Kawakami*

* Institute for Advanced Medical Research, Keio University School of Medicine, Shinjuku-ku, Tokyo, Japan; {dagger} Department of Clinical Immunology, Kitasato University School of Allied Health Science, Sagamihara, Japan; and {ddagger} Department of Internal Medicine, Tokyo Electric Power Company Hospital, Tokyo, Japan

Sjögrens’s syndrome (SS) is an autoimmune disease characterized by destruction of lacrimal and salivary glands, but the mechanisms underlying the disease process are unclear. By immunoscreening a HepG2 cDNA library with serum from an SS patient we isolated a cDNA encoding amino-terminal 616 aa of {beta}-fodrin, a membrane skeleton protein associated with ion channels and pumps. Serum Ab to the amino-terminal fragment of {beta}-fodrin was frequently detected in SS patients compared with rheumatic disease patients without SS or healthy controls (70 vs 12 or 4%; p < 0.00001). All the anti-{beta}-fodrin-positive sera recognized the amino-terminal fragment with no homology to {alpha}-fodrin. Anti-{beta}-fodrin Abs in patients’ sera as well as mouse polyclonal sera raised against the amino-terminal {beta}-fodrin fragment did not react with intact {beta}-fodrin, but recognized the 65-kDa amino-terminal fragment generated through cleavage by caspase-3 or granzyme B. When expression of intact and fragmented {beta}-fodrin in lacrimal glands was assessed by immunohistochemistry, the antigenic amino-terminal fragment was distributed diffusely in acinar epithelial cell cytoplasm, whereas the carboxyl-terminal fragment and/or intact {beta}-fodrin were localized in peripheral cytoplasm, especially at the basal membrane, in SS patients. In contrast, intact {beta}-fodrin was detected primarily at the apical membrane of epithelia, and the amino-terminal fragment was scarcely detected in control patients with chronic graft-vs-host disease. These findings suggest that cleavage and altered distribution of {beta}-fodrin in glandular epithelial cells may induce impaired secretory function and perpetuate an autoimmune response to {beta}-fodrin, leading to autoantibody production and glandular destruction in SS.




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