Abstract

: First encounter with thymus-dependent antigen usually induces both a primary (1 primary) antibody response and B cell memory, thus providing a rationale for vaccination. However, the dichotomy in response to epitopes on (Tyr, Glu)-Ala--Lys [(T,G)-A--L] shows that B cell activation leading to the antibody forming cell (AFC) vs. memory pathways are separable events: the 1 primary antibody response is against GT, but upon memory recall, 20- 30% of the B cells respond to A-L, thus (T,G)-A--L-priming generated memory to A-L with no detectable early 1 primary effector phase. The long-term objectives are to understand the mechanisms that control cell fate determination (effector vs. memory) after 1 degree B cell activation. The proposed experiments will test the hypothesis that higher avidity 1 degree B cells (e. g., GT+) are activated to become AFC, whereas lower avidity B cells (e. g., A-L+) are activated only to enter the germinal center to memory pathway. V(D)J knock-in mice will be used to follow the cell fate of higher vs. lower avidity 1 primary B cells. The GT knock-in expresses a heavy chain from a 1 degree GT+ B cell. Two A-L+ knock-ins (AL-M, collectively) express mutated heavy chains from an A-L+ memory cell, whereas the AL-GL knock-in uses the same, but unmutated, heavy chain.
Aim 1 asks whether B cells differing in avidity have different cell fate outcomes after in vivo activation, and it will analyze different aspects of AFC or memory cell formation by GT, AL-M, and AL-GL 1 primary B cells using flow cytometry and adoptive transfer experiments.
Aim 2 asks whether in vitro correlates exist for differential signaling by BCRs differing in avidity, and it will analyze B cell antigen presentation ability, activation profiles, and BCR translocation to lipid rafts. If, as this hypothesis proposes, the signal threshold for memory cell generation is lower than that for AFC differentiation, then modifying strength of signal might modulate cell fate.
Aim 3 asks whether reducing CD22 negative regulation allows lower avidity cells to become AFC, and whether reducing Btk signals impedes AFC differentiation of higher avidity B cells. It will compare effector vs. memory cell generation in GT, AL-M, and AL-GL knock-ins on the CD22 -/- or .xid background. Understanding the relationships among B cell avidity, B cell activation signals, and B cell fate (effector vs. memory) will help in the design of vaccines that can elicit both protective, early 1 primary antibody and B cell memory after one priming event.

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Institute of Allergy and Infectious Diseases (NIAID)
Type
Research Project (R01)
Project #
5R01AI013725-26
Application #
7002194
Study Section
Immunobiology Study Section (IMB)
Program Officer
Ferguson, Stacy E
Project Start
1977-09-01
Project End
2008-12-31
Budget Start
2006-01-01
Budget End
2008-12-31
Support Year
26
Fiscal Year
2006
Total Cost
$378,394
Indirect Cost

  Institution

Name
Brandeis University
Department
Biology
Type
Schools of Arts and Sciences
DUNS #
616845814
City
Waltham
State
MA
Country
United States
Zip Code
02454

  Publications

Maul, Robert W; Cao, Zheng; Venkataraman, Lakshmi et al. (2014) Spt5 accumulation at variable genes distinguishes somatic hypermutation in germinal center B cells from ex vivo-activated cells. J Exp Med 211:2297-306
Giorgetti, C A; Press, J L (1998) Somatic mutation in the neonatal mouse. J Immunol 161:6093-104
Mainville, C A; Sheehan, K M; Klaman, L D et al. (1996) Deletional mapping of fifteen mouse VH gene families reveals a common organization for three Igh haplotypes. J Immunol 156:1038-46
Giorgetti, C A; Press, J L (1994) A peptide sequence mimics the epitope on the multideterminant antigen (Tyr,Glu)-Ala-Lys that induces the dominant H10/V kappa 1+ primary antibody response. J Immunol 152:136-45
Press, J L; Giorgetti, C A (1993) Molecular and kinetic analysis of an epitope-specific shift in the B cell memory response to a multideterminant antigen. J Immunol 151:1998-2013
Press, J L; Giorgetti, C A; Busby 3rd, W F (1991) A new germline VH36-60 gene is used in the neonatal primary and adult memory response to (T,G)-A--L. Mol Immunol 28:1217-24
Borriero, L; Giorgetti, C; Smith, G et al. (1990) Neonatal and adult primary B cells use the same germ-line VH and V kappa genes in their (T,G)-A-L-specific repertoire. J Immunol 144:583-92
Busto, P; Gerstein, R; Dupre, L et al. (1987) Molecular analysis of heavy and light chains used by primary and secondary anti-(T,G)-A--L antibodies produced by normal and xid mice. J Immunol 139:608-18
Press, J L; Giorgetti, C A (1986) Clonal analysis of the primary and secondary B cell responses of neonatal, adult, and xid mice to (T,G)-A--L. J Immunol 137:784-90
Busto, P; Giorgetti, C A; Gawoski, J et al. (1986) Xid and normal mice express a light chain-associated cross-reactive idiotype in response to (T,G)-A--L and (T,G)-A--L-mBSA. J Immunol 136:3734-43