Abstract

Normal lymphocyte development relies on a series of cues from cell surface receptors. This includes receptors for important cytokines, such as IL-7 and receptors (pre-BCR and pre-TCR) generated after successful assembly of antigen receptor genes. We have demonstrated that the activation of DNA damage responses (DDR) by DNA double strand breaks (DSBs) generated by RAG during V(D)J recombination also provides important cues for developing lymphocytes. Like all DSBs, RAG DSBs activate the ATM kinase, which coordinates canonical DDR including repair by non-homologous end joining (NHEJ), initiation of cell cycle arrest and activation of cell death if the DSBs persist unrepaired. However, we demonstrated that in response to RAG DSBs ATM also activates a genetic program that includes many genes encoding proteins that have no function in canonical DDR. Rather these proteins function in lymphocyte-specific processes that could be important for normal development. From this we proposed that RAG DSBs, and possibly other types of physiologic DSBs, provide important signals that regulate cell-type-specific processes. In the last period of this grant we focused on understanding how RAG DSB signals activate distinct transcription pathways and how the resulting genetic program influences B cell development. In this regard, we have shown that the activation of ATM by RAG DSBs generated during immunoglobulin light (Igl) chain gene assembly in pre-B cells leads to the induction of both NF-kB1 and NF-kB2. NF-kB2 up-regulates the expression of the SpiC transcriptional repressor, which inhibits pre-BCR signaling by down-regulating the expression of Syk and BLNK. We find that while NF-kB1 can be activated by both RAG DSBs and genotoxic DSBs (from ionizing radiation), NF-kB2 is only activated by RAG DSBs. This is a very important finding as it demonstrates that the DSBs generated during antigen receptor gene assembly can specifically activate some transcriptional pathways that are not generally activated by all DSBs. In the current proposal we will establish the mechanistic basis for the selective activation of NF-kB2 by RAG DSBs. This will provide an important paradigm for our understanding of the activation of tissue-specific responses by different types of physiologic DSBs. Moreover, our finding that RAG DSB signals inhibit pre-BCR signals has led us to propose a ?toggle? model for pre-BCR and DDR signaling in pre-B cells. We envision that pre-B cells toggle between pre-BCR signals that promote Igl chain gene assembly and the activation of DDR by the resulting RAG DSBs that inhibit pre-BCR signaling and thus additional Igl chain gene rearrangements. This toggling between pre-BCR and DDR signals would provide for ordering of Igl chain gene assembly and promote genome stability in developing B cells.

Public Health Relevance

All developing lymphocytes generate DNA double strand breaks (DSBs) as intermediates in the generation of complete antigen receptor genes. We have demonstrated that these DSBs activate a genetic program that includes genes encoding proteins with broad cellular functions including processes that are important for normal lymphocyte development. The goal of this project is to understand how these DSBs specifically activate transcription pathways and how the resulting genetic program participates in lymphocyte development.

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Institute of Allergy and Infectious Diseases (NIAID)
Type
Research Project (R01)
Project #
2R01AI047829-16A1
Application #
9307412
Study Section
Cellular and Molecular Immunology - B Study Section (CMIB)
Program Officer
Nasseri, M Faraz
Project Start
2000-09-30
Project End
2021-03-31
Budget Start
2017-04-01
Budget End
2018-03-31
Support Year
16
Fiscal Year
2017
Total Cost
$423,750
Indirect Cost
$173,750

  Institution

Name
Weill Medical College of Cornell University
Department
Pathology
Type
Schools of Medicine
DUNS #
060217502
City
New York
State
NY
Country
United States
Zip Code
10065

  Publications

Fistonich, Chris; Zehentmeier, Sandra; Bednarski, Jeffrey J et al. (2018) Cell circuits between B cell progenitors and IL-7+ mesenchymal progenitor cells control B cell development. J Exp Med 215:2586-2599
Hung, Putzer J; Johnson, Britney; Chen, Bo-Ruei et al. (2018) MRI Is a DNA Damage Response Adaptor during Classical Non-homologous End Joining. Mol Cell 71:332-342.e8
Morales, Abigail J; Carrero, Javier A; Hung, Putzer J et al. (2017) A type I IFN-dependent DNA damage response regulates the genetic program and inflammasome activation in macrophages. Elife 6:
Bednarski, Jeffrey J; Pandey, Ruchi; Schulte, Emily et al. (2016) RAG-mediated DNA double-strand breaks activate a cell type-specific checkpoint to inhibit pre-B cell receptor signals. J Exp Med 213:209-23
Tubbs, Anthony T; Dorsett, Yair; Chan, Elizabeth et al. (2014) KAP-1 promotes resection of broken DNA ends not protected by ?-H2AX and 53BP1 in G?-phase lymphocytes. Mol Cell Biol 34:2811-21
KC, Wumesh; Satpathy, Ansuman T; Rapaport, Aaron S et al. (2014) L-Myc expression by dendritic cells is required for optimal T-cell priming. Nature 507:243-7
Dose, Marei; Emmanuel, Akinola Olumide; Chaumeil, Julie et al. (2014) ?-Catenin induces T-cell transformation by promoting genomic instability. Proc Natl Acad Sci U S A 111:391-6
Dorsett, Yair; Zhou, Yanjiao; Tubbs, Anthony T et al. (2014) HCoDES reveals chromosomal DNA end structures with single-nucleotide resolution. Mol Cell 56:808-18
Sandoval, Gabriel J; Graham, Daniel B; Bhattacharya, Deepta et al. (2013) Cutting edge: cell-autonomous control of IL-7 response revealed in a novel stage of precursor B cells. J Immunol 190:2485-9
Steinel, Natalie C; Lee, Baeck-Seung; Tubbs, Anthony T et al. (2013) The ataxia telangiectasia mutated kinase controls Ig? allelic exclusion by inhibiting secondary V?-to-J? rearrangements. J Exp Med 210:233-9

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