Abstract

The goal of this research is to understand how B lymphocyte production is regulated and to characterize early B cell precursors. Two different long-term bone marrow cultures (LTBMC) are central to these analyses. The Dexter myeloid bone marrow cultures (MBMC) are optimal for myelopoiesis. No B cells are produced in this system but an early B cell precursor is maintained. The Whitlock-Witte lymphoid bone marrow cultures (LBMC) allow long-term B lymphopoiesis. The MBMC B cell precursor can be induced to differentiate into B cells following switching to LBMC conditions.
The first aim of the proposal is to characterize stromal cell lines isolated from the MBMC adherent layer. One, termed S17, supports B cell differentiation while another, S10, does not. The molecular weight of a factor secreted by S17 that induces Ig expression in pre-B cells will be determined by high pressure liquid chromatography. The relative contribution of the factor alone versus direct contact between developing B cells and stromal cells will be examined in diffusion chamber experiments.
This aim will also examine the effects of nonstromal factors as IL-1, IL-2, and gamma-interferon on B cell production by adding these agents to the MBMC to LBMC switch system. The second focus of this proposal will examine membrane interactions between B cells and the stromal cells. Initially, the interactions between S17 and developing B cells will be examined by transmission electron microscopy. Components of the stromal cell surface with which B cells interact will then be identified. Stromal cell membrane preparations will be made, separated on 1- D gels and the proteins transferred to nitrocellulose filters. B cells and their precursors from LBMC will be incubated on these and the ability of the cells to bind to membrane fractions, of a particular molecular weight determined. Once the relevant molecule is identified, monoclonal antibodies will be made to it. An alternative source of immunogen will be whole stromal cell populations.
A third aim of the work will be to identify intermediate stages of B lymphopoiesis. A detailed kinetic analysis of developing cells in the MBMC to LBMC switch system will be performed using antibodies to surface and cytoplasmic antigens. Preliminary observations indicate that cells that may be lymphocyte progenitors from these cultures form colonies in semisolid medium overlayed on a stromal cell feeder layer. The growth conditions of the system will be defined and phenotype of the colony forming cell(s) determined.
The final aim will use cells from the colonies to examine Ig gene utilization during development using DNA probes to the various Ig heavy chain variable regions. This will allow expression of the Ig repertoire in B cell precursors of defined maturational state to be studied. The data from these studies will provide a knowledge of the basic biology of normal B cell differentiation and contribute to understanding pathological B cell development.

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Institute of Allergy and Infectious Diseases (NIAID)
Type
Research Project (R01)
Project #
2R01AI021256-04
Application #
3131203
Study Section
Immunobiology Study Section (IMB)
Project Start
1984-07-01
Project End
1991-06-30
Budget Start
1987-07-01
Budget End
1988-06-30
Support Year
4
Fiscal Year
1987
Total Cost
Indirect Cost

  Institution

Name
University of California Riverside
Department
Type
Overall Medical
DUNS #
City
Riverside
State
CA
Country
United States
Zip Code
92521

  Publications

Montecino-Rodriguez, Encarnacion; Casero, David; Fice, Michael et al. (2018) Differential Expression of PU.1 and Key T Lineage Transcription Factors Distinguishes Fetal and Adult T Cell Development. J Immunol 200:2046-2056
Montecino-Rodriguez, Encarnacion; Fice, Michael; Casero, David et al. (2016) Distinct Genetic Networks Orchestrate the Emergence of Specific Waves of Fetal and Adult B-1 and B-2 Development. Immunity 45:527-539
Montecino-Rodriguez, Encarnacion; Li, Katy; Fice, Michael et al. (2014) Murine B-1 B cell progenitors initiate B-acute lymphoblastic leukemia with features of high-risk disease. J Immunol 192:5171-8
Sham, Caroline W; Chan, Ann M; Kwong, Jacky M K et al. (2012) Neuronal programmed cell death-1 ligand expression regulates retinal ganglion cell number in neonatal and adult mice. J Neuroophthalmol 32:227-37
Montecino-Rodriguez, Encarnacion; Dorshkind, Kenneth (2012) B-1 B cell development in the fetus and adult. Immunity 36:13-21
Yoshimoto, Momoko; Montecino-Rodriguez, Encarnacion; Ferkowicz, Michael J et al. (2011) Embryonic day 9 yolk sac and intra-embryonic hemogenic endothelium independently generate a B-1 and marginal zone progenitor lacking B-2 potential. Proc Natl Acad Sci U S A 108:1468-73
Barber, Chad L; Montecino-Rodriguez, Encarnacion; Dorshkind, Kenneth (2011) Reduced production of B-1-specified common lymphoid progenitors results in diminished potential of adult marrow to generate B-1 cells. Proc Natl Acad Sci U S A 108:13700-4
Montecino-Rodriguez, Encarnacion; Dorshkind, Kenneth (2011) Formation of B-1 B cells from neonatal B-1 transitional cells exhibits NF-?B redundancy. J Immunol 187:5712-9
Signer, Robert A J; Montecino-Rodriguez, Encarnacion; Witte, Owen N et al. (2010) Immature B-cell progenitors survive oncogenic stress and efficiently initiate Ph+ B-acute lymphoblastic leukemia. Blood 116:2522-30
Chen, Ling; Sham, Caroline W; Chan, Ann M et al. (2009) Role of the immune modulator programmed cell death-1 during development and apoptosis of mouse retinal ganglion cells. Invest Ophthalmol Vis Sci 50:4941-8

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