The chromosomal breakpoints of t(4;11) translocation of acute lymphoblastic leukemia (ALL) have been recently identified at molecular level and shown to involve the AF4 (FEL) gene on chromosome 4 and the ALL-1 (MLL, Hrx) gene on chromosome 11. The ALL-1/AF4 fusion gene is transcribed into a chimeric mRNA. Using primer sets derived from ALL-1 and AF4 cDNAs by reverse transcription-polymerase chain reaction (RT-PCR), we were able to amplify the breakpoint sites of the fusion transcript of all 15 ALL cases with karyotypic or molecular evidence of the t(4;11). DNA fragments of different size were obtained as the consequence of different breakpoints on chromosome 11 and the presence of alternative splicing of ALL-1 exon 8. The feasibility of monitoring the residual cells carrying the t(4;11) in 2 ALL patients with different clinical outcome was evaluated. Overall, the presented results provide evidence that RT-PCR can be used as a rapid method for detecting this chromosomal abnormality and following the patient's response to therapy
DETECTION OF ALL-1/AF4 FUSION TRANSCRIPT BY REVERSE TRANSCRIPTION-POLYMERASE CHAIN-REACTION FOR DIAGNOSIS AND MONITORING OF ACUTE LEUKEMIAS WITH THE T(4 11) TRANSLOCATION / Biondi, A; Rambaldi, A; Rossi, V; Elia, L; Caslini, C; Basso, G; Battista, R; Barbui, T; Mandelli, Franco; Masera, G; Croce, C; Canaani, E; Cimino, Giuseppe. - In: BLOOD. - ISSN 0006-4971. - STAMPA. - 82:(1993), pp. 2943-2947.
DETECTION OF ALL-1/AF4 FUSION TRANSCRIPT BY REVERSE TRANSCRIPTION-POLYMERASE CHAIN-REACTION FOR DIAGNOSIS AND MONITORING OF ACUTE LEUKEMIAS WITH THE T(4 11) TRANSLOCATION
MANDELLI, Franco;CIMINO, Giuseppe
1993
Abstract
The chromosomal breakpoints of t(4;11) translocation of acute lymphoblastic leukemia (ALL) have been recently identified at molecular level and shown to involve the AF4 (FEL) gene on chromosome 4 and the ALL-1 (MLL, Hrx) gene on chromosome 11. The ALL-1/AF4 fusion gene is transcribed into a chimeric mRNA. Using primer sets derived from ALL-1 and AF4 cDNAs by reverse transcription-polymerase chain reaction (RT-PCR), we were able to amplify the breakpoint sites of the fusion transcript of all 15 ALL cases with karyotypic or molecular evidence of the t(4;11). DNA fragments of different size were obtained as the consequence of different breakpoints on chromosome 11 and the presence of alternative splicing of ALL-1 exon 8. The feasibility of monitoring the residual cells carrying the t(4;11) in 2 ALL patients with different clinical outcome was evaluated. Overall, the presented results provide evidence that RT-PCR can be used as a rapid method for detecting this chromosomal abnormality and following the patient's response to therapyI documenti in IRIS sono protetti da copyright e tutti i diritti sono riservati, salvo diversa indicazione.
