Leaky severe combined immunodeficiency and aberrant DNA rearrangements due to a hypomorphic RAG1 mutation

Giblin, William; Chatterji, Monalisa; Westfield, Gerwin; Masud, Tehmina; Theisen, Brian; Cheng, Hwei Ling; DeVido, Jeffrey; Alt, Frederick W.; Ferguson, David O.; Schatz, David G.; Sekiguchi, JoAnn

doi:10.1182/blood-2008-07-165167

Cited by 42 publications

(63 citation statements)

References 70 publications

(107 reference statements)

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“…In detail, after initial purification of DN4 stage T cells by flow sorting, single cells were resorted or isolated by using the CellCelector automated cell picking system (ALS Automated Lab Solutions GmbH, Jena, Germany); digested in a 20-l solution containing 10 mM Tris-HCl (pH 9.0), 50 mM KCl, 1.5 mM MgCl 2 , 3.0 g proteinase K (EM Science), and 0.1% Triton X-100 (Sigma); and incubated at 55°C for 60 min followed by 95°C for 15 min. First-round PCR amplified both V(D)Jrearranged alleles together in a 60-l final reaction mixture volume consisting of 20 l of the single-cell isolation solution described above, PCR buffer (10 mM Tris-HCl [pH 9.0], 50 mM KCl, and 2.0 mM MgCl 2 ), 200 M deoxynucleoside triphosphates (dNTPs), 0.5 U Taq DNA polymerase (New England BioLabs), and an oligonucleotide mixture (each at a 100 nM final concentration) (25,26,42,82) (Table 4) containing 22 forward primers corresponding to 23 V␤ exon families (2 primers were designed to amplify 2 V␤5 and 3 V␤8 multisequence families, respectively), the D␤1 and D␤2 diversity segment genes, 2 reverse primers matching joining-segment J␤1 and J␤2 sequences, as well as 1 primer set for ␤-actin. The PCR conditions were 94°C for 1 min and 5 cycles with the annealing temperature ramped from 66°C to 58°C, followed by 25 cycles of 94°C for 30 s, 56°C for 60 s, and 72°C for 60 s, with a final extension step at 72°C for 5 min.…”

Section: Methodsmentioning

confidence: 99%

GATA3 Abundance Is a Critical Determinant of T Cell Receptor β Allelic Exclusion

Sekiguchi

Panwar

et al. 2017

Molecular and Cellular Biology

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Allelic exclusion describes the essential immunological process by which feedback repression of sequential DNA rearrangements ensures that only one autosome expresses a functional T or B cell receptor. In wild-type mammals, approximately 60% of cells have recombined the DNA of one T cell receptor ␤ (TCR␤) V-to-DJ-joined allele in a functional configuration, while the second allele has recombined only the DJ sequences; the other 40% of cells have recombined the V to the DJ segments on both alleles, with only one of the two alleles predicting a functional TCR␤ protein. Here we report that the transgenic overexpression of GATA3 leads predominantly to biallelic TCR␤ gene (Tcrb) recombination. We also found that wild-type immature thymocytes can be separated into distinct populations based on intracellular GATA3 expression and that GATA3 LO cells had almost exclusively recombined only one Tcrb locus (that predicted a functional receptor sequence), while GATA3 HI cells had uniformly recombined both Tcrb alleles (one predicting a functional and the other predicting a nonfunctional rearrangement). These data show that GATA3 abundance regulates the recombination propensity at the Tcrb locus and provide new mechanistic insight into the historic immunological conundrum for how Tcrb allelic exclusion is mediated.KEYWORDS allelic exclusion, T cell receptor beta locus, GATA3, monoallelic-tobiallelic switch O ne enduring mystery in cellular immunology regards the underlying mechanisms that control antigen receptor allelic exclusion (1, 2), the process whereby B or T lymphocytes are programmed to express only one functional allele for each chain of their respective antigen receptors (B cell receptor [BCR] or T cell receptor [TCR]), thus avoiding the coexistence of multiple antigen specificities in a single immune cell. Lymphocytes acquire the diversity of antigen recognition (3) as well as a unique monospecificity for particular antigens (4) during development in the bone marrow (B cells) or the thymus (T cells).T lymphocyte development is generally characterized by division into multiple stages based on developmental timing and the location and expression of specific cell surface markers (5). T cell development begins when multipotential hematopoietic progenitor cells in the bone marrow migrate through the bloodstream to the thymus, where early T lineage progenitors (ETPs) are generated and later specified to become T cells (6-10). ETPs differentiate into double-negative (DN) cells (DN2 to DN4 stages) that express neither the CD4 nor the CD8 coreceptor, then into double-positive (DP)

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Section: Methodsmentioning

confidence: 99%

GATA3 Abundance Is a Critical Determinant of T Cell Receptor β Allelic Exclusion

Sekiguchi

Panwar

et al. 2017

Molecular and Cellular Biology

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“…Second, germline NHEJ/Tp53-deficient mice succumb to pro-B lymphomas with RAG-dependent Igh/c-myc or Igh/N-myc translocations (Difilippantonio et al, 2002;Zhu et al, 2002;Gladdy et al, 2003;Rooney et al, 2004). Third, Tp53 À/À mice expressing a RAG1 mutant that exhibits defects in DNA end joining develop thymic lymphomas with clonal antigen receptor locus translocations (Giblin et al, 2009). Fourth, Tp53 À/À mice containing a genetic block in thymocyte development succumb to thymic lymphomas with RAG-dependent genomic instability (Haines et al, 2006).…”

Section: Introductionmentioning

confidence: 99%

Tp53 deletion in B lineage cells predisposes mice to lymphomas with oncogenic translocations

et al. 2011

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Inactivating Tp53 mutations are frequent genetic lesions in human tumors that harbor genomic instability, including B lineage lymphomas with IG translocations. Antigen receptor genes are assembled and modified in developing lymphocytes by RAG/AID-initiated genomic rearrangements that involve the induction of DNA double strand breaks (DSBs). Although TP53 inhibits the persistence of DSBs and induces apoptosis to protect cells from genomic instability and transformation, the development of spontaneous tumors harboring clonal translocations has not been reported in mice that only lack wild-type Tp53 protein or express Tp53 mutants. Tp53-deficient (Tp53 À/À ) mice succumb to T lineage lymphomas lacking clonal translocations but develop B lymphoid tumors containing immunoglobulin (Ig) translocations upon combined inactivation of DSB repair factors, RAG mutation or AID overexpression; mice expressing apoptosis-defective Tp53 mutants develop B cell lymphomas that have not been characterized for potential genomic instability. As somatic rather than germline inactivating mutations of TP53 are typically associated with human cancers and Tp53 deletion has cellular context dependent effects upon lymphocyte transformation, we generated mice with conditional Tp53 deletion in lineage-committed B lymphocytes to avoid complications associated with defective Tp53 responses during embryogenesis and/or in multilineage potential cells and, thereby, directly evaluate the potential physiological role of Tp53 in suppressing translocations in differentiated cells. These mb1-cre:Tp53 flox/flox mice succumbed to lymphoid tumors containing Ig gene rearrangements and immunophenotypes characteristic of B cells from various developmental stages. Most mb1-cre: Tp53 flox/flox tumors harbored clonal translocations, including Igh/c-myc or other oncogenic translocations generated by the aberrant repair of RAG/AID-generated DSBs.Our data indicate that Tp53 serves critical functions in B lineage lymphocytes to prevent transformation caused by translocations in cell populations experiencing physiological levels of RAG/AID-initiated DSB intermediates, and provide evidence that the somatic TP53 mutations found in diffuse large B-cell lymphoma and Burkitt's lymphoma may contribute to the development of these human malignancies.

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“…14,15 Mouse models of OS and of leaky SCID have been generated, such as Rag1 R972Q, 16 the Rag1 S723C, 7 , and Rag2 R229Q 17 mice. In addition to the mouse, SCID and SCID variants have also been modeled in the dog and horse.…”

Section: Cd8mentioning

confidence: 99%

“…We and others have shown that hypomorphic RAG mutations that affect, but do not abolish, V(D)J recombination, are often associated with distinct immunologic and clinical phenotypes with residual presence of T, and in some cases B, lymphocytes. [6][7][8][9] The presence of autologous, auto-reactive, activated, and oligoclonal T cells that infiltrate and damage peripheral organs is a hallmark of Omenn syndrome (OS). In other cases, hypomorphic RAG mutations may cause delayed disease onset, granuloma formation, autoimmunity, and/or dysgammaglobulinemia.…”

Section: Introductionmentioning

confidence: 99%

Modeling altered T-cell development with induced pluripotent stem cells from patients with RAG1-dependent immune deficiencies

Brauer

Pessach

Clarke

et al. 2016

Blood

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• Upon in vitro differentiation, iPSCs obtained from patients with SCID and OS show a similar block in T-cell development.• Presence of unresolved single-strand DNA breaks in developing T cells from OS patient-derived iPSCs affects their differentiation.Primary immunodeficiency diseases comprise a group of heterogeneous genetic defects that affect immune system development and/or function. Here we use in vitro differentiation of human induced pluripotent stem cells (iPSCs) generated from patients with different recombination-activating gene 1 (RAG1) mutations to assess T-cell development and T-cell receptor (TCR) V(D)J recombination. RAG1-mutants from severe combined immunodeficient (SCID) patient cells showed a failure to sustain progression beyond the CD3residual mutant RAG1 recombination activity from an Omenn syndrome (OS) patient, similar impaired T-cell differentiation was observed, due to increased single-strand DNA breaks that likely occur due to heterodimers consisting of both an N-terminal truncated and a catalytically dead RAG1. Furthermore, deep-sequencing analysis of TCR-b (TRB) and TCR-a (TRA) rearrangements of CD3 2 CD4 1 CD8 2 immature single-positive and CD81 double-positive cells showed severe restriction of repertoire diversity with preferential usage of few Variable, Diversity, and Joining genes, and skewed length distribution of the TRB and TRA complementary determining region 3 sequences from SCID and OS iPSC-derived cells, whereas control iPSCs yielded T-cell progenitors with a broadly diversified repertoire. Finally, no TRA/d excision circles (TRECs), a marker of TRA/d locus rearrangements, were detected in SCID and OS-derived T-lineage cells, consistent with a pre-TCR block in T-cell development. This study compares human T-cell development of SCID vs OS patients, and elucidates important differences that help to explain the wide range of immunologic phenotypes that result from different mutations within the same gene of various patients. (Blood. 2016;128(6):783-793)

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Leaky severe combined immunodeficiency and aberrant DNA rearrangements due to a hypomorphic RAG1 mutation

Cited by 42 publications

References 70 publications

GATA3 Abundance Is a Critical Determinant of T Cell Receptor β Allelic Exclusion

GATA3 Abundance Is a Critical Determinant of T Cell Receptor β Allelic Exclusion

Tp53 deletion in B lineage cells predisposes mice to lymphomas with oncogenic translocations

Modeling altered T-cell development with induced pluripotent stem cells from patients with RAG1-dependent immune deficiencies

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