Abstract

This proposal is to continue studies intended to define the molecular and cellular processes responsible for expression of the B cell repertoire and the mechanisms and consequences of antigenic triggering of B cells. Although it is clear that the combinatorial association of multiple available V gene segments, junction flexibility, and somatic mutation could give rise to an enormous variable region repertoire, several findings now indicate that these processes may not be totally random. This is exemplified by findings indicating that: a) certain clonotypes recurr within the newly generated, sIg-, bone marrow precursor cell population of normal adult mice at disproportionately high frequencies; b) the repertoire of fetal and neonatal precursor cells reflects preferential Vh gene segment utilization; and c) the precursor cell repertoire of aged mice includes high frequencies of novel clonotypes that are rare or absent in younger animals. We will continue to identify and analyze, at the molecular level, clonotypic expression that evidences such non-randomness in V region utilization in neonates and sIg- populations of adult and aged mice in an effort to delineate the mechanisms that control variable region generation and expression in the primary B cell repertoire. Studies will also be conducted to analyze the progenitors of secondary B cells, the parameters of their stimulation, and the expression of variable region genes and somatic mutations in these cells and thier clonal progeny. Comparisons of repertoire expression in environmentally naive sIg- vs mature sIg+ precursor cell populations have revealed that several clonotype sets are much more highly represented within the sIg- precursor cell pool. It is likely that such disparities evidence environmental down-regulation in repertoire expression as B cells mature. We will investigate further these disparities in order to define the contribution to mature B cell repertoire expression of environmental immunoregulatory processes and the mechanisms by which such processes operate. Finally, we have been able to establish several experimental systems which give great promise for enabling a detailed analysis of B cell triggering. We will utilize these approaches to further examine the membrane and intracellular requisites for tolerance induction vs stimulation, and the basis for differences in the affinity threshold of receptor-antigen interactions required to trigger immature vs mature precursor cells.

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Institute of Allergy and Infectious Diseases (NIAID)
Type
Method to Extend Research in Time (MERIT) Award (R37)
Project #
4R37AI015797-14
Application #
3480856
Study Section
Special Emphasis Panel (NSS)
Project Start
1978-07-01
Project End
1996-06-30
Budget Start
1991-07-01
Budget End
1992-06-30
Support Year
14
Fiscal Year
1991
Total Cost
Indirect Cost

  Institution

Name
Scripps Research Institute
Department
Type
DUNS #
City
La Jolla
State
CA
Country
United States
Zip Code
92037

  Publications

Diaz, Marilyn; Watson, Nicholas B; Turkington, Gene et al. (2003) Decreased frequency and highly aberrant spectrum of ultraviolet-induced mutations in the hprt gene of mouse fibroblasts expressing antisense RNA to DNA polymerase zeta. Mol Cancer Res 1:836-47
Diaz, M; Verkoczy, L K; Flajnik, M F et al. (2001) Decreased frequency of somatic hypermutation and impaired affinity maturation but intact germinal center formation in mice expressing antisense RNA to DNA polymerase zeta. J Immunol 167:327-35
Kline, G H; Hartwell, L; Beck-Engeser, G B et al. (1998) Pre-B cell receptor-mediated selection of pre-B cells synthesizing functional mu heavy chains. J Immunol 161:1608-18
Decker, D J; Linton, P J; Zaharevitz, S et al. (1995) Defining subsets of naive and memory B cells based on the ability of their progeny to somatically mutate in vitro. Immunity 2:195-203
Stillman, C A; Linton, P J; Koutz, P J et al. (1994) Specific immunoglobulin cDNA clones produced from hybridoma cell lines and murine spleen fragment cultures by 3SR amplification. PCR Methods Appl 3:320-31
Linton, P J; Lo, D; Lai, L et al. (1992) Among naive precursor cell subpopulations only progenitors of memory B cells originate germinal centers. Eur J Immunol 22:1293-7
Linton, P J; Klinman, N R (1992) The generation of memory B cells. Semin Immunol 4:3-9
Decker, D J; Boyle, N E; Koziol, J A et al. (1991) The expression of the Ig H chain repertoire in developing bone marrow B lineage cells. J Immunol 146:350-61
Linton, P J; Rudie, A; Klinman, N R (1991) Tolerance susceptibility of newly generating memory B cells. J Immunol 146:4099-104
Decker, D J; Boyle, N E; Klinman, N R (1991) Predominance of nonproductive rearrangements of VH81X gene segments evidences a dependence of B cell clonal maturation on the structure of nascent H chains. J Immunol 147:1406-11

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