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Blood, 1 September 2000, Vol. 96, No. 5, pp. 2002-2002

CORRESPONDENCE

To the editor:

Anticorresponding p15 promoter methylation and microsatellite instability in acute myeloblastic leukemia

We read with interest the paper on p15 promoter methylation in adult and childhood acute leukemias.1 Wong et al used methylation-specific polymerase chain reaction (MSP) to analyze p15 promoter methylation patterns in acute leukemia. Their study included an analysis of 38 adults and 4 children with acute myeloid leukemia (AML). In this group they found higher p15 methylation frequencies in patients with the M3, M4, M2, and M7 French-American-British (FAB) subtypes than in those with the M1, M6, or M5 subtypes. They also noted an association between p15 methylation and chromosomal translocations, inversions, and deletions, suggesting an interplay of these abnormalities and p15 methylation, but the number of patients with these abnormalities and p15 methylation in their cohort of patients with AML was small (n=3).

We have retrospectively analyzed p15 methylation in 73 patients with AML aged 16 to 96 years (median age 63 years). Our study also utilized MSP using the same primer sets as Wong et al. Data relating to FAB type are available on 55 of our cases (Table). Unlike Wong et al, we failed to find any association between p15 methylation frequencies and FAB subtype. We believe that the discrepancies between our results and those of Wong et al reflect the small numbers of patients involved in both studies and suggest that no correlations should be drawn between AML subtype and p15 methylation status until a larger cohort of patients has been analyzed.

                              
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  		Comparison of the frequency of p15 methylation as determined by Wong et al1 compared with that determined in the Nottingham study

We also have cytogenetic data available on 53 of our patients. These have been analyzed according to the 3 prognostic cytogenetic risk groups defined in the Medical Research Council AML 10 trial.2 According to these criteria, the inv(16)(q13q22), t(15;17)(q22;q12) and t(8;21)(q22;q22) abnormalities described by Wong et al are characterized as good-risk abnormalities. In our study, 0 of 3 patients with good-risk cytogenetics, 19 of 34 with intermediate-risk cytogenetics, and 8 of 16 with poor-risk cytogenetics had evidence of p15 methylation. The figures were compared using a Pearson chi-square test, and no correlation was found between p15 methylation status and cytogenetic risk group (= .178).

We have also examined the relationship between p15 methylation and functional evidence of a mismatch repair (MMR) gene defect as detected by microsatellite instability (MSI) using a panel of 11 microsatellite markers to compare constitutional DNA derived from mouthwash samples with that of leukemic DNA from the same patients.3 An analysis of MSI was successful in 61 of the 73 patients whose p15 methylation status was known. Six patients were found to have MSI, and this was shown to be associated with abnormal MSH2 protein expression as detected by Western blotting. Of the 6 MSI-positive cases, none had evidence of p15 methylation. In contrast, 30 of 55 MSI-negative cases had p15 methylation. Although the number of patients with MSI is small, the inverse correlation between MSI and p15 methylation is statistically significant using the Fisher exact test (= .024). These results represent an interesting and novel finding. p15 promoter hypermethylation appears to be a common late event in the pathogenesis of AML, whereas MMR gene defects are rare. The finding that MMR gene defects, when present, are not associated with p15 promoter hypermethylation implies a unique disease pathogenesis in those patients with MMR gene defects. In such cases leukemia is likely to evolve through novel pathways involving MMR gene defects and subsequent mutations in genes regulating growth and apoptosis independently of methylation defects.

Emma P. Das-Gupta and Nigel H. Russell
Academic Haematology Nottingham City Hospital Nottingham, England
Supported by a grant from the Leukaemia Research Fund, London, England.

References

1. Wong IHN, Ng MHL, Huang DP, Lee JCK. Aberrant p15 promoter methylation in adult and childhood leukemias of nearly all morphologic subtypes: potential prognostic implications. Blood. 2000;95:1942-1949[Abstract/Free Full Text].

2. Grimwade D, Walker H, Oliver F, et al. The importance of diagnostic cytogenetics on outcome in AML: analysis of 1,612 patients entered into the MRC AML 10 trial. Blood. 1998;92:2322-2333[Abstract/Free Full Text].

3. Zhu Y-M, Das-Gupta EP, Russell NH. Microsatellite instability and p53 mutations are associated with abnormal expression of the MSH2 gene in adult acute leukemia. Blood. 1999;94:733-740[Abstract/Free Full Text].


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Related Article in Blood Online:

Aberrant p15 promoter methylation in adult and childhood acute leukemias of nearly all morphologic subtypes: potential prognostic implications
Ivy H. N. Wong, Margaret H. L. Ng, Dolly P. Huang, and Joseph C. K. Lee
Blood 2000 95: 1942-1949. [Abstract] [Full Text] [PDF]




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