ATM deficiency impairs thymocyte maturation because of defective resolution of T cell receptor α locus coding end breaks

Vacchio, Melanie S.; Olaru, Alexandru; Livák, Ferenc; Hodes, Richard J.

doi:10.1073/pnas.0611222104

Cited by 67 publications

(69 citation statements)

References 34 publications

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“…This is an autosomal recessive disorder characterized by progressive cerebellar degeneration and an increased incidence of cancer. Importantly, ATM deficiency leads to a defect in thymocyte maturation that is associated with decreased efficiency in V‐J rearrangement of the endogenous TCRα locus, accompanied by increased frequency of unresolved TCR‐Jα coding end breaks 55. It was also shown that residual ATM kinase activity correlates with the severity of immune defects 56…”

Section: Genes and Diseases Associated With Defective Recombination Imentioning

confidence: 99%

Programmed DNA breaks in lymphoid cells: repair mechanisms and consequences in human disease

Procházková

Loizou

2015

Immunology

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SummaryIn recent years, several novel congenital human disorders have been described with defects in lymphoid B‐cell and T‐cell functions that arise due to mutations in known and/or novel components of DNA repair and damage response pathways. Examples include impaired DNA double‐strand break repair, as well as compromised DNA damage‐induced signal transduction, including phosphorylation and ubiquitination. These disorders reinforce the importance of genome stability pathways in the development of lymphoid cells in humans. Furthermore, these conditions inform our knowledge of the biology of the mechanisms of genome stability and in some cases may provide potential routes to help exploit these pathways therapeutically. Here we review the mechanisms that repair programmed DNA lesions that occur during B‐cell and T‐cell development, as well as human diseases that arise through defects in these pathways.

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Section: Genes and Diseases Associated With Defective Recombination Imentioning

confidence: 99%

Programmed DNA breaks in lymphoid cells: repair mechanisms and consequences in human disease

Procházková

Loizou

2015

Immunology

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“…In this regard, deficiency in the ataxia telangiectasia mutated (ATM) serine threonine kinase in both mice and humans leads to an increased incidence of lymphoid tumors with RAG-dependent translocations involving antigen receptor loci (17)(18)(19)(20)(21). In addition, mature, nontransformed Atm-deficient lymphocytes have an increased frequency of translocations and other chromosomal aberrations involving antigen receptor loci (18,19,(22)(23)(24).…”

mentioning

confidence: 99%

“…Inhibition of the abl kinase with STI571 leads to G 1 cell cycle arrest, induction of RAG expression, and robust rearrangement of the endoge-nous Ig (Ig) light (L) chain genes and chromosomally integrated retroviral recombination substrates (25)(26)(27). Induction of V(D)J recombination by STI571 treatment of Atm Ϫ/Ϫ abl pre-B cells leads to an accumulation of un-repaired coding ends and to the aberrant resolution of these coding ends, analogous to what is observed in Atm-deficient lymphocytes in vivo (19,(22)(23)(24)(25). Here, we describe an experimental approach that permits high-throughput cloning of breakpoint targets from aberrantly resolved RAG DSBs generated during V(D)J recombination in Atm Ϫ/Ϫ abl pre-B cells.…”

mentioning

confidence: 99%

Aberrantly resolved RAG-mediated DNA breaks in Atm-deficient lymphocytes target chromosomal breakpoints incis

Mahowald

Baron

Mahowald

et al. 2009

Proc. Natl. Acad. Sci. U.S.A.

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Canonical chromosomal translocations juxtaposing antigen receptor genes and oncogenes are a hallmark of many lymphoid malignancies. These translocations frequently form through the joining of DNA ends from double-strand breaks (DSBs) generated by the recombinase activating gene (RAG)-1 and -2 proteins at lymphocyte antigen receptor loci and breakpoint targets near oncogenes. Our understanding of chromosomal breakpoint target selection comes primarily from the analyses of these lesions, which are selected based on their transforming properties. RAG DSBs are rarely resolved aberrantly in wild-type developing lymphocytes. However, in ataxia telangiectasia mutated (ATM)-deficient lymphocytes, RAG breaks are frequently joined aberrantly, forming chromosomal lesions such as translocations that predispose (ATM)-deficient mice and humans to the development of lymphoid malignancies. Here, an approach that minimizes selection biases is used to isolate a large cohort of breakpoint targets of aberrantly resolved RAG DSBs in Atm-deficient lymphocytes. Analyses of this cohort revealed that frequently, the breakpoint targets for aberrantly resolved RAG breaks are other DSBs. Moreover, these nonselected lesions exhibit a bias for using breakpoints in cis, forming small chromosomal deletions, rather than breakpoints in trans, forming chromosomal translocations.ataxia telangiectasia mutated ͉ chromosomal translocation ͉ DNA double-strand break repair ͉ V(D)J recombination D ouble-strand breaks (DSBs) in DNA are generated by genotoxic agents and cellular endonucleases as intermediates in several important physiologic processes including V(D)J recombination, Ig class switch recombination (CSR), DNA replication, gene transcription, and meiosis. DNA DSBs activate a highly conserved cellular response that prevents cell cycle progression, initiates repair of the broken DNA ends, and promotes apoptosis of cells with persistent un-repaired DSBs (1, 2). Broken DNA ends from a single DSB are usually rejoined; however, in some processes, such as V(D)J recombination and CSR, DNA ends arising from two DSBs are joined in a regulated fashion, generating a new gene product (1-4). Broken DNA ends from distinct DSBs can also be joined aberrantly, leading to the formation of potentially dangerous chromosomal lesions such as translocations, deletions, and inversions.All developing lymphocytes generate programmed DNA DSBs during V(D)J recombination, a process that joins variable (V), joining (J), and in some cases, diversity (D) gene segments to generate the second exon of antigen receptor genes (4). The V(D)J recombination reaction is initiated by the recombinase activating gene (RAG)-1 and -2 proteins, which together form the RAG endonuclease (5). RAG introduces DNA DSBs at the border of two recombining gene segments and their flanking RAG recognition sequences, termed recombination signals (RSs) (5). DNA cleavage by RAG occurs after an appropriate RS pair (12/23 compatible) forms a synaptic complex, generating

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“…Other important aberrant translocations involving the Tcra/Tcrd locus include those that result in ataxia-telangiectasia mutations in the A-T mutated kinase (ATM) that cause chromosome instability and defects in DNA repair [69]. An important percent of A-T syndrome patients develop the disease due to translocations and inversions involving specific breakpoints at the Tcra/Tcrd locus and most of all ATM -/-mice die due to thymic lymphomas derived from and incorrect repair of the breaks that result from V(D)J recombination and aberrant Tcra/Tcrd locus translocations [70][71][72][73][74][75]. The knowledge of the precise mechanisms by which the Tcra/Tcrd locus transcription and recombination are regulated is important to understand the defective control of these processes that results in disease.…”

Section: Transcription and Recombinationmentioning

confidence: 99%

Insights into the Transcriptional Regulation of the Unrearranged and Rearranged Tcra and Tcrd Genes

Hernández-Munaín¹,

Casal²,

Juanes³

et al. 2016

J Clin Cell Immunol

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The combined T-cell receptor α and δ locus, Tcra/Tcrd, encodes the TCRα and TCRδ chains of the αβ or γδ T-cell receptors (TCRαβ and TCRγδ), respectively, which define the two distinct T-cell lineages, αβ and γδ T lymphocytes. Like other antigen receptor loci, this locus must recombine its variable (V), diversity (D), and joining (J) gene segments to generate a diverse range of TCR that allow vertebrates to respond to an unlimited number of antigens. The Tcra/Tcrd germline transcription and subsequent V(D)J gene segment rearrangements are strictly regulated by two distant transcriptional enhancers, Eα and Eδ, respectively, during thymocyte development. Once the Tcra locus is productively rearranged, it is assumed Eα remains active for the transcription of the rearranged locus and the expression of the functional TCRα chain in αβ T lymphocytes. However, our recent experiments have shown Eα is significantly inhibited during the final stage of thymocyte development, concomitantly with the expression of the rearranged Tcra locus, and remains inhibited in αβ T lymphocytes. These results imply the existence of an Eα-independent mechanism to activate transcription of the rearranged Tcra locus in αβ T lymphocytes. Interestingly, Eα is essential for the normal expression of the rearranged Tcrd locus in γδ T lymphocytes. In this review, the current knowledge about the regulation of Tcra/Tcrd germline transcription and gene segment rearrangement during thymocyte development and the possible mechanisms for transcription of the rearranged Tcra locus in mature αβ T lymphocytes are discussed. The knowledge of the detailed mechanisms involved in the regulation of transcription at the Tcra/Tcrd locus by distant enhancers is important to understand the cases in which deregulation this process results in disease. Keywords: Transcription; T-cell receptor; V(D)J recombination; Enhancer Abbreviations:A Temporal Control of TCR Gene RearrangementsDuring thymic T-cell development (Figure 1), early T-cell progenitors (ETP) arising from fetal liver or bone marrow enter to the thymus, where they mature progressively through different stages that can be distinguished based on the expression of the CD4 and CD8 surface markers: CD4-CD8-double-negative (DN) thymocytes, immature single-positive (ISP) CD8 + thymocytes, CD4 + CD8 + doublepositive (DP) thymocytes, and CD4 + or CD8 + single-positive (SP) thymocytes [1]. Among the DN thymocyte population, four subpopulations can be further distinguished based on the expression of CD25 and CD44 surface markers: DN1 (CD44 + CD25 -), DN2 (CD44 + CD25 + ), DN3 (CD44 -CD25 + ), and DN4 (CD44 -CD25 -) thymocytes. In addition, two DN3 subpopulations can be distinguished based on the expression of CD27: DN3a (CD27 low ) and DN3b (CD27 high ) thymocytes [2]. Furthermore, two DP thymocyte populations can be distinguished based on the expression of CD71: early DP (eDP) (CD71 + ) and late DP (lDP) (CD71 -) thymocytes [3]. For αβ T-cell development, thymocytes transition from DN1 to SP thymocytes by matu...

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ATM deficiency impairs thymocyte maturation because of defective resolution of T cell receptor α locus coding end breaks

Cited by 67 publications

References 34 publications

Programmed DNA breaks in lymphoid cells: repair mechanisms and consequences in human disease

Programmed DNA breaks in lymphoid cells: repair mechanisms and consequences in human disease

Aberrantly resolved RAG-mediated DNA breaks in Atm-deficient lymphocytes target chromosomal breakpoints incis

Insights into the Transcriptional Regulation of the Unrearranged and Rearranged Tcra and Tcrd Genes

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