Volume 23, Issue 2 pp. 175-182
Research Article

Detection of t(11;14) using interphase molecular cytogenetics in mantle cell lymphoma and atypical chronic lymphocytic leukemia

Hervé Avet-Loiseau

Corresponding Author

Hervé Avet-Loiseau

Laboratory of Hematology, University Hospital, Nantes, France

Unité de Cytogénétique Hématologique, Institut de Biologie, 9 quai Moncousu, 44093 Nantes Cédex, FranceSearch for more papers by this author
Richard Garand

Richard Garand

Laboratory of Hematology, University Hospital, Nantes, France

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Fanny Gaillard

Fanny Gaillard

Laboratory of Pathology, University Hospital, Nantes, France

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Axelle Daviet

Axelle Daviet

Laboratory of Hematology, University Hospital, Nantes, France

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Marie-Paule Mellerin

Marie-Paule Mellerin

Laboratory of Hematology, University Hospital, Nantes, France

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Nelly Robillard

Nelly Robillard

Laboratory of Hematology, University Hospital, Nantes, France

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Isabelle Bouyge

Isabelle Bouyge

INSERM U463, Nantes, France

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Santosh Arcot

Santosh Arcot

Human Genome Center, Lawrence Livermore National Laboratory, Livermore, California

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Mark Batzer

Mark Batzer

Department of Pathology, Stanley Scott Cancer Center, New Orleans, Louisiana

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Pascaline Talmant

Pascaline Talmant

Laboratory of Hematology, University Hospital, Nantes, France

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Jean-Luc Harousseau

Jean-Luc Harousseau

Department of Clinical Hematology, University Hospital, Nantes, France

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Noël Milpied

Noël Milpied

Department of Clinical Hematology, University Hospital, Nantes, France

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Régis Bataille

Régis Bataille

Laboratory of Hematology, University Hospital, Nantes, France

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Abstract

The chromosomal translocation t(11;14)(q13;q32) fuses the IGH and CCND1 genes and leads to cyclin D1 overexpression. This genetic abnormality is the hallmark of mantle cell lymphoma (MCL), but is also found in some cases of atypical chronic lymphocytic leukemia (CLL), characterized by a poor outcome. For an unequivocal assessment of this specific chromosomal rearrangement on interphase cells, we developed a set of probes for fluorescence in situ hybridization (FISH). Northern blotting was performed for analysis of the cyclin D1 expression in 18 patients. Thirty-eight patients, with either a typical MCL leukemic phase (17 patients) or atypical CLL with an MCL-type immunophenotype, i.e., CD19+, CD5+, CD23−/low, CD79b/sIgM(D)++, and FMC7+ (21 patients), were analyzed by dual-color interphase FISH. We selected an IGH-specific BAC probe (covering the JH and first constant regions) and a commercially available CCND1 probe. An IGHCCND1 fusion was detected in 28 of the 38 patients (17 typical MCL and 11 cases with CLL). Cyclin D1 was not overexpressed in two patients with typical MCL and an IGHCCND1 fusion. In view of the poor prognosis associated with MCL and t(11;14)-positive CLL, we conclude that this set of probes is a valuable and reliable tool for a rapid diagnosis of these entities. Genes Chromosomes Cancer 23:175–182, 1998. © 1998 Wiley-Liss, Inc.

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