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Efficiency of interphase fluorescence in situ hybridization for BCR/ABL on peripheral blood smears for monitoring of CML patients: a comparison with bone marrow findings

  1. Author:
    Akel, S.
    Kolialexi, A.
    Mavrou, A.
    Metaxotou, C.
    Loukopoulos, D.
    Yataganas, X.
  2. Author Address

    NCI, Basic Res Lab, CCR, Bldg 567,Rm 261, Frederick, MD 21702 USA Univ Athens, Sch Med, Dept Med 1, GR-11527 Athens, Greece Univ Athens, Sch Med, Dept Med Genet, GR-11527 Athens, Greece Akel S NCI, Basic Res Lab, CCR, Bldg 567,Rm 261, Frederick, MD 21702 USA
    1. Year: 2002
  1. Journal: Clinical and Laboratory Haematology
    1. 24
    2. 6
    3. Pages: 361-367
  2. Type of Article: Article
  1. Abstract:

    Conventional cytogenetic analysis (CCA) is the standard method for monitoring of the Philadelphia (Ph) chromosome in chronic myeloid leukemia (CML). Evaluation of breakpoint cluster region/abelson murine leukemia (BCR/ABL) fusion using interphase fluorescence in situ hybridization on peripheral blood smears (PB-FISH) might be another approach allowing more frequent and less invasive follow-up investigations. Herein, BCR/ABL fusion gene was assessed on 21 PB smears from 16 CML patients in chronic phase. Results of PB-FISH were compared with those of CCA and interphase FISH on bone marrow aspirates (BM-FISH). PB-FISH analysis was combined with CD3 immunophenotyping that allowed simultaneous investigation of the leukemic status of CD3(+) T lymphocytes and scoring CD3(-) cells for BCR/ABL fusion gene. Moreover, the frequency of BCR/ABL fusion in nonlymphoid PB cells was estimated according to the differential leukocyte counts. The incidence of BCR/ABL(+) fusion signals in CD3(+) T cells of CML patients was 5.3% (SD+/-1.9) and did not exceed the normal cut-off value of 8%. A significant correlation (P<0.001) was found between results of PB-FISH and methods of BM analysis (CCA or BM-FISH). Correction of PB-FISH results to include only nonlymphoid or CD3(-) cells reduced the mean of differences and improved agreement between PB-FISH and CCA or BM-FISH methods. The best agreement was noted between CCA and PB-FISH on nonlymphoid cells. On the other hand, results of BM-FISH agreed well with those of PB-FISH on CD3(-) cells. These findings imply that PB- FISH on nonlymphoid or CD3(-) cells is reliable and may replace BM analysis for monitoring of response to treatment in CML patients.

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