Detection of t(4;14)(p16.3;q32) chromosomal translocation in multiple myeloma by reverse transcription-polymerase chain reaction analysis of IGH-MMSET fusion transcripts.

染色体易位 分子生物学 生物 荧光原位杂交 逆转录聚合酶链式反应 多发性骨髓瘤 不确定意义的单克隆抗体病 聚合酶链反应 断点 逆转录酶 融合基因 一致性 基因 单克隆 单克隆抗体 信使核糖核酸 遗传学 抗体 染色体 免疫学
作者
Ursula Malgeri,Luca Baldini,Vittorio Perfetti,Sonia Fabris,M C Vignarelli,Gualtiero I. Colombo,Virginia Lotti,Silvana Compasso,Silvia Bogni,L. Tallone Lombardi,Anna Teresa Maiolo,Antonino Neri
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期刊:PubMed 卷期号:60 (15): 4058-61 被引量:94
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We and others have recently identified a novel recurring t(4;14)(p16.3; q32) translocation in multiple myeloma (MM) that leads to an apparent deregulation of the FGFR3 and WHSC1/MMSET genes. Because the presence of IGH-MMSET hybrid transcripts has been found in MM cell lines with t(4;14), they may represent a specific tumor-associated marker in MM. In this study, we developed a reverse transcription-PCR (RTPCR) assay for detecting chimeric transcripts from all of the 4p16.3 breakpoints identified thus far, and we used it to investigate a representative panel of 53 MM patients and 16 patients with monoclonal gammopathy of uncertain significance; in addition, t(4;14) was investigated in all of the MM patients by means of two-color fluorescence in situ hybridization. IGH-MMSET transcripts were found in 11 of the 53 (20%) MM cases and 1 of 16 (6%) cases of monoclonal gammopathy of uncertain significance. There was complete concordance between the RT-PCR and fluorescence in situ hybridization analyses of the MM cases. The results of this study indicate that RT-PCR is a sensitive and reliable method of detecting t(4;14) and suggest that it may be useful for monitoring the disease in a significant proportion of patients.

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