1999
DOI: 10.1038/sj.leu.2401383
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Simple and reliably sensitive diagnosis and monitoring of Philadelphia chromosome-positive cells in chronic myeloid leukemia by interphase fluorescence in situ hybridization of peripheral blood cells

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Cited by 33 publications
(19 citation statements)
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“…[16][17] A limitation of interphase FISH method is the background of a variant proportion of false positive cells, depending on the probe/detection system used. [18][19][20][21] In practice, the limit of detection of CML cells is typically 1-5% and depends in part on which probes are used, the size of the nucleus, the precise position of the breakpoint within the ABL gene and the criteria used to define co-localization. 22 The advantage of FISH over conventional cytogenetics is the analysis of a larger number of nuclei, resulting in smaller sampling errors.…”
Section: Fluorescence In Situ Hybridization (Fish)mentioning
confidence: 99%
“…[16][17] A limitation of interphase FISH method is the background of a variant proportion of false positive cells, depending on the probe/detection system used. [18][19][20][21] In practice, the limit of detection of CML cells is typically 1-5% and depends in part on which probes are used, the size of the nucleus, the precise position of the breakpoint within the ABL gene and the criteria used to define co-localization. 22 The advantage of FISH over conventional cytogenetics is the analysis of a larger number of nuclei, resulting in smaller sampling errors.…”
Section: Fluorescence In Situ Hybridization (Fish)mentioning
confidence: 99%
“…[10][11][12][13][14][15] Previous studies focused on patients treated with IFN-based drug therapy, allogeneic and autologous stem cell transplantation. 10,13,16 While the correlation between I-FISH and BM metaphases is generally rather tight, there is considerable variation between studies, and there may be significant discrepancies between the two methods in individual patients.…”
Section: Introductionmentioning
confidence: 99%
“…Muhlmann et al (1998), in a study of 30 paired PB and BM specimens obtained simultaneously from patients with different cytogenetic responses, showed an excellent correlation between quantification of BCR-ABL-positive cells from bone marrow and peripheral blood. However, two other reports, on a total of 53 paired specimens, showed that the levels of BCR-ABL cells detected in PB for most of the specimens were lower than that in the BM (Buno et al, 1998;Yanagi et al, 1999). In one of these reports, it was shown that, in 10 patients, the quantitative changes in the PB over an approximately 12-month course of IFN␣ therapy paralleled that of the BM, suggesting that monitoring with PB specimens could provide sufficient information as to whether patients respond to therapy (Buno et al, 1998;Yanagi et al, 1999).…”
Section: Interferon-␣-based Therapymentioning
confidence: 93%
“…However, two other reports, on a total of 53 paired specimens, showed that the levels of BCR-ABL cells detected in PB for most of the specimens were lower than that in the BM (Buno et al, 1998;Yanagi et al, 1999). In one of these reports, it was shown that, in 10 patients, the quantitative changes in the PB over an approximately 12-month course of IFN␣ therapy paralleled that of the BM, suggesting that monitoring with PB specimens could provide sufficient information as to whether patients respond to therapy (Buno et al, 1998;Yanagi et al, 1999). Given these findings, it can be inferred, however, that in the later stages of therapy when the leukemic burden is further reduced to below what can be detected in the peripheral blood, a BM specimen is still required for detection of minimal residual disease.…”
Section: Interferon-␣-based Therapymentioning
confidence: 93%
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