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Balanced Translocations Disrupting SMARCB1 Are Hallmark Recurrent Genetic Alterations in Renal Medullary Carcinomas.
Calderaro, Julien; Masliah-Planchon, Julien; Richer, Wilfrid; Maillot, Laetitia; Maille, Pascale; Mansuy, Ludovic; Bastien, Claire; de la Taille, Alexandre; Boussion, Hélène; Charpy, Cécile; Jourdain, Anne; Bléchet, Claire; Pierron, Gaelle; Gentien, David; Choudat, Laurence; Tournigand, Christophe; Delattre, Olivier; Allory, Yves; Bourdeaut, Franck.
Afiliación
  • Calderaro J; APHP, Groupe Hospitalier Henri Mondor, Département de Pathologie, Créteil, France; INSERM, U955, Institut Mondor de Recherche Biomédicale, Créteil, France; Université Paris-Est Créteil, Créteil, France. Electronic address: juliencalderaro@yahoo.fr.
  • Masliah-Planchon J; Institut Curie, Unité de Génétique Somatique, Paris, France; INSERM U830, Génétique et Biologie des Cancers, Institut Curie, Paris, France.
  • Richer W; INSERM U830, Génétique et Biologie des Cancers, Institut Curie, Paris, France; SiRIC Institut Curie, Recherche Translationnelle en Oncologie Pediatrique, Paris, France.
  • Maillot L; Institut Curie, Unité de Génétique Somatique, Paris, France.
  • Maille P; APHP, Groupe Hospitalier Henri Mondor, Département de Pathologie, Créteil, France.
  • Mansuy L; CHU Nancy, Hôpital d'enfants, Service d'Hémato-oncologie pédiatrique, Vandoeuvre les Nancy, France.
  • Bastien C; CHU Nancy, Hôpital Brabois, Service d'Anatomie pathologique, Vandoeuvre les Nancy, France.
  • de la Taille A; INSERM, U955, Institut Mondor de Recherche Biomédicale, Créteil, France; Université Paris-Est Créteil, Créteil, France; APHP, Groupe Hospitalier Henri Mondor, Service d'Urologie, Créteil, France.
  • Boussion H; APHP, Groupe Hospitalier Henri Mondor, Service d'Oncologie médicale, Créteil, France.
  • Charpy C; APHP, Groupe Hospitalier Henri Mondor, Département de Pathologie, Créteil, France.
  • Jourdain A; CHU Tours, Hôpital Clocheville, Service d'oncologie et d'hématologie pédiatrique, Tours, France.
  • Bléchet C; CHU Tours, Service d'Anatomie et de cytologie pathologiques, Tours, France.
  • Pierron G; Institut Curie, Unité de Génétique Somatique, Paris, France.
  • Gentien D; Plateforme de Biologie Moléculaire, Département de Recherche Translationnelle, Institut Curie, Centre de Recherche, Paris, France.
  • Choudat L; APHP, Hôpital Bichat, Département de Pathologie, Paris, France.
  • Tournigand C; Université Paris-Est Créteil, Créteil, France; APHP, Groupe Hospitalier Henri Mondor, Service d'Oncologie médicale, Créteil, France.
  • Delattre O; Institut Curie, Unité de Génétique Somatique, Paris, France; INSERM U830, Génétique et Biologie des Cancers, Institut Curie, Paris, France.
  • Allory Y; APHP, Groupe Hospitalier Henri Mondor, Département de Pathologie, Créteil, France; INSERM, U955, Institut Mondor de Recherche Biomédicale, Créteil, France; Université Paris-Est Créteil, Créteil, France.
  • Bourdeaut F; INSERM U830, Génétique et Biologie des Cancers, Institut Curie, Paris, France; SiRIC Institut Curie, Recherche Translationnelle en Oncologie Pediatrique, Paris, France; Institut Curie, Département d'Oncologie Pédiatrique -Adolescents Jeunes Adultes, Paris, France.
Eur Urol ; 69(6): 1055-61, 2016 06.
Article en En | MEDLINE | ID: mdl-26433572
ABSTRACT

BACKGROUND:

Renal medullary carcinoma (RMC) is a rare and highly aggressive neoplasm that most often occurs in the setting of sickle cell trait or sickle cell disease (SCD). Most patients present with metastatic disease resistant to conventional chemotherapy, and therefore there is an urgent need for molecular insight to propose new therapies.

OBJECTIVE:

To determine the molecular alterations and oncogenic pathways that drive RMC development. DESIGN, SETTING, AND

PARTICIPANTS:

A series of five frozen samples of patients with RMC was investigated by means of gene expression profiling, array comparative genomic hybridization, and RNA and whole exome sequencing (WES). OUTCOME MEASUREMENTS AND STATISTICAL

ANALYSIS:

RNA and DNA sequencing read data were analyzed to detect gene fusions and somatic mutations. Gene fusions mutations were validated by real-time polymerase chain reaction and fluorescence in situ hybridization. Gene expression profiling was analyzed by unsupervised hierarchical clustering and Gene Set Enrichment Analysis (Broad Institute, Cambridge, MA, USA). RESULTS AND

LIMITATIONS:

We observed inactivation of the tumor suppressor gene SMARCB1 in all tumors. In all four cases developed in patients with SCD, we identified an original mechanism of interchromosomal balanced translocations that disrupt the SMARCB1 sequence and thus contribute to its inactivation. Gene expression profiling revealed that RMC shares common oncogenic pathways with pediatric malignant rhabdoid tumors, another tumor subtype characterized by SMARCB1 deficiency.

CONCLUSIONS:

RMCs are characterized by an original mechanism of interchromosomal balanced translocations that disrupt the SMARCB1 sequence. WES reveals that RMCs show no other recurrent genetic alteration and an overall stable genome, underscoring the oncogenic potency of SMARCB1 inactivation. PATIENT

SUMMARY:

Our comprehensive molecular study supports a pivotal role of the tumor suppressor gene SMARCB1 in the development of renal medullary carcinoma. The use of therapeutic strategies based on the biologic effects of its inactivation should now open new perspectives for this typically lethal malignancy.
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Texto completo: 1 Base de datos: MEDLINE Asunto principal: Translocación Genética / Carcinoma / Proteína SMARCB1 / Neoplasias Renales Tipo de estudio: Prognostic_studies Idioma: En Revista: Eur Urol Año: 2016 Tipo del documento: Article
Texto completo
Imprimir
XML
PubMed Links
Buscar en Google

Texto completo: 1 Base de datos: MEDLINE Asunto principal: Translocación Genética / Carcinoma / Proteína SMARCB1 / Neoplasias Renales Tipo de estudio: Prognostic_studies Idioma: En Revista: Eur Urol Año: 2016 Tipo del documento: Article