1q12 chromosome translocations form aberrant heterochromatic foci associated with changes in nuclear architecture and gene expression in B cell lymphoma

Fournier, Alice; McLeer-Florin, Anne; Lefebvre, Catherine Lemieux; Duley, Samuel; Barki, Leila; Ribeyron, Juliana; Kassambara, Alboukadel; Hamaidia, Sieme; Granjon, A; Gressin, Rémy; Lajmanovich, Alicia; Bonnefoix, Thierry; Chauvelier, Stéphanie; Debernardi, Alexandra; Rousseaux, Sophie; Fraipont, Florence de; Figeac, Martin; Kerckaert, Jean‐Pierre; Vos, John De; Usson, Yves; Delaval, Katia; Grichine, Alexeï; Vourc’h, Claire; Khochbin, Saadi; Feil, Robert; Leroux, Dominique; Callanan, Mary

doi:10.1002/emmm.201000067

Cited by 33 publications

(27 citation statements)

References 38 publications

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“…For example, in patient 17, we identified the focal amplification of 16q11 translocated to 18q as part of a second translocation of the same JT1q12 ( Figure 2A). The der (20) in this cell line did not show a signal for 16q11 and, therefore, was not a sequential JT1q12 (Figure 2A). In a second more complex example, patient 59, 2 sequential specimens were analyzed.…”

Section: Whole-arm Jt1q12 To 16q11mentioning

confidence: 87%

“…32 We and others have previously speculated that the cause of these duplications and jumping translocations of 1q may be region-specific hypomethylation of the 1q12 pericentromeric heterochromatin. [18][19][20][21][22] The 1q12 pericentromeric region is a distinctive region in the human genome in that it is the largest single block of late-replicating, highly repetitive satII/III DNA that is known to contain unstable segmental duplications (low copy repeats). It is thought that a 5-azacytidine fragile site at 1q12 may play a role in the incomplete replication (delayed condensation), breaks, and triradial configurations of 1q12.…”

Section: Discussionmentioning

confidence: 99%

“…17 The primary mechanism for amplification of 1q21 in MM is the whole-arm CN aberration known as the jumping translocation 1q (JT1q12). [18][19][20][21] A JT1q12 occurs when a duplication of the 1q12 pericentromeric region translocates (jumps) as a donor chromosome (DC) segment to one or more receptor chromosomes (RCs). In most cases, JT1q12 becomes a stable clonal aberration; however, the JT1q12 can also translocate to a second RC or, alternatively, "jump off" a RC and be lost from the cell in the form of a single or multiple micronuclei.…”

Section: Introductionmentioning

confidence: 99%

See 2 more Smart Citations

Jumping translocations of 1q12 in multiple myeloma: a novel mechanism for deletion of 17p in cytogenetically defined high-risk disease

Sawyer

Tian

Heuck

et al. 2014

Blood

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Section: Whole-arm Jt1q12 To 16q11mentioning

confidence: 87%

Section: Discussionmentioning

confidence: 99%

Section: Introductionmentioning

confidence: 99%

See 1 more Smart Citation

Jumping translocations of 1q12 in multiple myeloma: a novel mechanism for deletion of 17p in cytogenetically defined high-risk disease

Sawyer

Tian

Heuck

et al. 2014

Blood

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“…23 Cytogenetics, FISH, molecular analyses, and aCGH R-banded karyotyping, fluorescence in situ hybridization (FISH) analyses, and array comparative genomic hybridization (aCGH) were performed by standard methods, as previously described. 10,25 All cytogenetic and aCGH data were centrally reviewed by the Groupe Francophone de Cytogénétique Hématologique and the French BPDCN network. Karyotypes were described according to the International System for Human Cytogenetic Nomenclature.…”

Section: Bpdcn Patients and Cell Linesmentioning

confidence: 99%

“…Chromatin immunoprecipitation (ChIP) experiments were performed as described by Fournier et al 25 (native chromatin) or using the Magna ChIP kit (Millipore; cross-linked chromatin), following the manufacturer's instructions. Briefly, all ChIP assays were performed in triplicate in at least 2 independent chromatin preparations.…”

Section: Chipmentioning

confidence: 99%

Haploinsufficiency for NR3C1, the gene encoding the glucocorticoid receptor, in blastic plasmacytoid dendritic cell neoplasms

Emadali

Hoghoughi

Duley

et al. 2016

Blood

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Key Points• NR3C1 haploinsufficiency is found in patients with a plasmacytoid dendritic cell neoplasm characterized by very poor clinical outcome.• Overexpression of lincRNA3q is a consistent feature of malignant cells in these patients and can be abrogated by BET protein inhibition.Blastic plasmacytoid dendritic cell neoplasm (BPDCN) is a rare and highly aggressive leukemia for which knowledge on disease mechanisms and effective therapies are currently lacking. Only a handful of recurring genetic mutations have been identified and none is specific to BPDCN. In this study, through molecular cloning in an index case that presented a balanced t(3;5)(q21;q31) and molecular cytogenetic analyses in a further 46 cases, we identify monoallelic deletion of NR3C1 (5q31), encoding the glucocorticoid receptor (GCR), in 13 of 47 (28%) BPDCN patients. Targeted deep sequencing in 36 BPDCN cases, including 10 with NR3C1 deletion, did not reveal NR3C1 point mutations or indels. Haploinsufficiency for NR3C1 defined a subset of BPDCN with lowered GCR expression and extremely poor overall survival (P 5 .0006). Consistent with a role for GCR in tumor suppression, functional analyses coupled with gene expression profiling identified corticoresistance and loss-of-EZH2 function as major downstream consequences of NR3C1 deletion in BPDCN. Subsequently, more detailed analyses of the t(3;5)(q21;q31) revealed fusion of NR3C1 to a long noncoding RNA (lncRNA) gene (lincRNA-3q) that encodes a novel, nuclear, noncoding RNA involved in the regulation of leukemia stem cell programs and G1/S transition, via E2F. Overexpression of lincRNA-3q was a consistent feature of malignant cells and could be abrogated by bromodomain and extraterminal domain (BET) protein inhibition. Taken together, this work points to NR3C1 as a haploinsufficient tumor suppressor in a subset of BPDCN and identifies BET inhibition, acting at least partially via lncRNA blockade, as a novel treatment option in BPDCN. (Blood. 2016;127(24):3040-3053)

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Histone crotonylation specifically marks the haploid male germ cell gene expression program

et al. 2011

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The haploid male germ cell differentiation program controls essential steps of male gametogenesis and relies partly on a significant number of sex chromosome-linked genes. These genes need to escape chromosome-wide transcriptional repression of sex chromosomes, which occurs during meiosis and is largely maintained in post-meiotic cells. A newly discovered histone lysine modification, crotonylation (Kcr), marks X/Y-linked genes that are active in post-meiotic male germ cells. Histone Kcr, by conferring resistance to transcriptional repressors, could be a dominant element in maintaining these genes active in the globally repressive environment of haploid cell sex chromosomes. Furthermore, the same mark was found associated with post-meiotically activated genes on autosomes. Histone Kcr therefore appears to be an indicator of the male haploid cell gene expression program and a notable element of genome programming in the post-meiotic phases of spermatogenesis.

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1q12 chromosome translocations form aberrant heterochromatic foci associated with changes in nuclear architecture and gene expression in B cell lymphoma

Cited by 33 publications

References 38 publications

Jumping translocations of 1q12 in multiple myeloma: a novel mechanism for deletion of 17p in cytogenetically defined high-risk disease

Jumping translocations of 1q12 in multiple myeloma: a novel mechanism for deletion of 17p in cytogenetically defined high-risk disease

Haploinsufficiency for NR3C1, the gene encoding the glucocorticoid receptor, in blastic plasmacytoid dendritic cell neoplasms

Histone crotonylation specifically marks the haploid male germ cell gene expression program

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