Human LPP gene is fused to MLL in a secondary acute leukemia with a t(3;11) (q28;q23)

被引:40
|
作者
Dahéron, L
Veinstein, A
Brizard, F
Drabkin, H
Lacotte, L
Guilhot, F
Larsen, CJ
Brizard, A
Roche, J
机构
[1] Poitiers Univ Hosp, CNRS FRE 2224, Hematol Lab, Poitiers, France
[2] Poitiers Univ Hosp, Dept Hematol & Oncol Med, Poitiers, France
[3] Univ Poitiers, IBMIG, CNRS FRE 2224, Poitiers, France
[4] UCHSC, Div Med Oncol, Denver, CO USA
来源
GENES CHROMOSOMES & CANCER | 2001年 / 31卷 / 04期
关键词
D O I
10.1002/gcc.1157
中图分类号
R73 [肿瘤学];
学科分类号
100214 ;
摘要
The mixed lineage leukemia, MLL, gene is frequently rearranged in patients with secondary leukemia following treatment with DNA topoisomerase II inhibitors. By FISH and Southern blot analyses we identified a rearrangement in the MLL gene due to a novel t(3;11)(q28;q23) chromosomal translocation in a patient who developed AML-M5 3 years after treatment for a follicular lymphoma. Through inverse PCR, the LPP (lipoma preferred partner) gene on 3q28 was identified as the MLL fusion partner. LPP contains substantial identity to the focal adhesion protein, zyxin, and is frequently fused to HMGIC in lipomas. The breakpoint occurred in intron 8 of MLL and LPP. Two in-frame MLL-LPP transcripts, which fuse MLL exon 8 to LPP exon 9, were detected by RT-PCR, although the smaller of these contained a deletion of 120 bp from the MLL sequence. The predicted MLL-LPP fusion protein includes the A/T hook motifs and methyltransferase domain of MLL joined to the two last LIM domains of LPP. A reciprocal LPP-MLL transcript, predicted to include the proline-rich and leucine zipper motifs, and the first LIM domain of LPP were also detected by RT-PCR. In summary, LPP is a newly identified MLL fusion partner in secondary leukemia resulting from topoisomerase inhibitors. The MLL-LPP and LPP-MLL predicted proteins contain many of the features present in other MLL rearrangements. (C) 2001 Wiley-Liss, Inc.
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页码:382 / 389
页数:8
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