DETECTION OF BCR-ABL AND E2A-PBX1 FUSION GENES BY RT-PCR IN ACUTE LYMPHOBLASTIC-LEUKEMIA WITH FAILED OR NORMAL CYTOGENETICS

To evaluate the use of molecular analysis as a complement to karyotypi c analysis in the detection of specific chromosomal abnormalities, the occurrence of t(1;19)(q23;p13) and t(9;22)(q34;q11) was investigated by RT-PCR in 43 diagnostic acute lymphoblastic leukaemia cases in whom cytogenetic investigations had failed (32 cases) or showed only a nor mal karyotype (greater than or equal to 20 normal metaphases, 11 cases ). One child (aged 14 years) and five adults (aged 18-60 years) were B CR-ABL positive on first round for M-BCR-ABL (one case) or m-BCR-ABL ( one case), or on nested PCR for m-BCR-ABL (three cases). Co-expression of M-BCR-ABL (first-round PCR) and m-BCR-ABL (nested PCR was seen in one case. One m-BCR-ABL-positive case also expressed the E2A-PBX1 fusi on transcript. Patients positive for the transcript(s) were older, had higher white brood cell counts and a significantly poorer event-free survival (P<0.001) than those negative for the transcript.