Leukemia Research
Volume 27, Issue 9 , Pages 803-805, September 2003

Flow cytometric measurement of phosphorylated STAT5 in AML: lack of specific association with FLT3 internal tandem duplications

Division of Haematology, Clinical Sciences Building, University of Nottingham and Nottingham City Hospital, Nottingham NG5 1PB, UK

Received 15 August 2002; accepted 21 December 2002.

Abstract 

STAT5 phosphorylation has been noted in 69–95% of AML cases by Western blotting. We used flow cytometry to measure phosphorylated STAT5 on a semi-quantitative scale. The method was validated on K562 cells, which constitutively express phosphorylated STAT5, but lose this when BCR-abl tyrosine kinase activity is blocked by STI571. Phosphorylated STAT5 was found to measure 2.22±0.09 relative fluorescence units (RFU) falling to 0.925±0.005RFU in the presence of STI571. Phosphorylated STAT5 expression was 0.99 to 2.09RFU in 28 primary AML samples. There was no logical cut-off point between positive and negative fluorescence. FLT3 internal tandem duplications, found in 11/28 samples, were not significantly associated with the level of phosphorylated STAT5 expression. We conclude that STAT5 phosphorylation can be measured sensitively by flow cytometry in AML and that its expression should not be dichotomised as present or absent.

Keywords: AML, Phosphorylated STAT5, FLT3 ITD

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PII: S0145-2126(03)00012-2

doi:10.1016/S0145-2126(03)00012-2

Leukemia Research
Volume 27, Issue 9 , Pages 803-805, September 2003