This proposal will describe studies aimed at exploring the regulation of Ig isotype switching by murine B cells stimulated through their antigen receptor, using a novel conjugate, dextran-linked anti-immunoglobulin D antibody (alpha/delta-dex). We have demonstrated that alpha/delta-dex induces resting murine B cells to proliferate at 1000-fold lower concentrations of alpha/delta-dex than that required for induction of comparable responses to unconjugated anti-IgD. T cell-derived cytokines induce alpha/delta-dex-activated B cells to secrete immunoglobulin (Ig) and switch to the expression of most Ig isotypes, but fail to stimulate detectable IgE. By contrast, Sepharose-bound anti-IgD (alpha/delta-seph), when cultured with B cells and T cell-derived cytokines stimulates a large IgE response. Furthermore, IFN-gamma selectively induces IgG3 secretion by alpha/delta-dex-activated, membrane (m)IgM+mIgG3-B cells in the presence of a maturation factor, such as IL-5. Alpha/delta-dex also potently and selectively inhibits LPS + ILA-4-mediated IgE secretion. In this proposal we will describe experiments designed to 1) determine the basis for the selective failure of alpha/delta-activated B cells to secrete IgE in order to delineate the non-IL-4-mediated signals necessary for IgE production, 2) explore the mechanism by which IFN-gamma simulates alpha/delta-dex-activated B cells to switch to the expression of IgG3, the major IgG isotype induced by bacterial-derived polysaccharides in vivo, and 3) investigate mechanisms underlying the selective alpha/delta-dex-mediated inhibition of LPS + IL-4-induced IgE production. The effects of cytokines and costimuli (alpha/delta-dex, alpha/delta-seph, LPS) on IgE and IgG3 class switching will be explored using traditional cell biologic methodology in parallel with studies of constant heavy (CH) gene regulation. The latter will include analyses of induction of regulatory DNA-binding proteins specific for CH gene loci, quantitation of CH gene germline transcription, and quantitation of switch recombination at the DNA level. These studies will clarify key parameters which regulate Ig class switching upon antigen receptor crosslinkage.

Agency
National Institute of Health (NIH)
Institute
National Institute of Allergy and Infectious Diseases (NIAID)
Type
Research Project (R01)
Project #
5R01AI032560-02
Application #
3147680
Study Section
Allergy and Immunology Study Section (ALY)
Project Start
1992-09-01
Project End
1997-04-30
Budget Start
1993-05-01
Budget End
1994-04-30
Support Year
2
Fiscal Year
1993
Total Cost
Indirect Cost
Name
Henry M. Jackson Fdn for the Adv Mil/Med
Department
Type
DUNS #
City
Rockville
State
MD
Country
United States
Zip Code
20817
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Vos, Q; Snapper, C M; Mond, J J (1999) Heterogeneity in the ability of cytotoxic murine NK cell clones to enhance Ig secretion in vitro. Int Immunol 11:159-68
Vos, Q; Ortaldo, J R; Conan-Cibotti, M et al. (1998) Phenotypic and functional characterization of a panel of cytotoxic murine NK cell clones that are heterogeneous in their enhancement of Ig secretion in vitro. Int Immunol 10:1093-101
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Zelazowski, P; Max, E E; Kehry, M R et al. (1997) Regulation of Ku expression in normal murine B cells by stimuli that promote switch recombination. J Immunol 159:2559-62
Zelazowski, P; Carrasco, D; Rosas, F R et al. (1997) B cells genetically deficient in the c-Rel transactivation domain have selective defects in germline CH transcription and Ig class switching. J Immunol 159:3133-9
Snapper, C M; Rosas, F R; Moorman, M A et al. (1997) Restoration of T cell-independent type 2 induction of Ig secretion by neonatal B cells in vitro. J Immunol 158:2731-5
Shparago, N; Zelazowski, P; Jin, L et al. (1996) IL-10 selectively regulates murine Ig isotype switching. Int Immunol 8:781-90
Snapper, C M; Rosas, F R; Zelazowski, P et al. (1996) B cells lacking RelB are defective in proliferative responses, but undergo normal B cell maturation to Ig secretion and Ig class switching. J Exp Med 184:1537-41
Snapper, C M; Rosas, F; Moorman, M A et al. (1996) IFN-gamma is a potent inducer of Ig secretion by sort-purified murine B cells activated through the mIg, but not the CD40, signaling pathway. Int Immunol 8:877-85

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