Detection of R882 Mutations in DNMT3A Gene in Acute Myeloid Leukemia: A Method Comparison Study

نویسندگان

  • Ahmad kazemi Department of hematology, School of allied medical sciences, Iran university of medical sciences
  • Bahareh toosi Department of hematology, School of allied medical sciences, Iran university of medical sciences
  • farhad zaker Department of hematology, School of allied medical sciences, Iran university of medical sciences
  • Mohsen Nikbakht Cell Therapy and Hematopoietic Stem Cell Transplantation Research Center, Tehran University of medical sciences, Tehran, Iran.
  • Saeed Mohammadi Cell Therapy and Hematopoietic Stem Cell Transplantation Research Center, Tehran University of medical sciences, Tehran, Iran
چکیده مقاله:

Background: Somatic mutations in the hotspot region of the DNA-methyltransferase 3A (DNMT3A) gene were recurrently identified in acute myeloid leukemia (AML). It is believed that DNMT3A mutations confer an adverse prognosis for AML patients. These lines of evidence support the need for a rapid and cost-efficient method for the detection of these mutations. The present study aimed to establish high resolution melting (HRM) curve analysis as a rapid and sensitive test to identify DNMT3A gene mutations in AML patients. Materials and Methods: In this retrospective cohort study, a total of 220 AML patients who referred to hematology-oncology and stem cell transplantation centers (referral center) at Shariati hospital in Tehran, Iran, were included. AML-M3 and therapy-related AML patients were excluded. The HRM assay was used to identify R882 mutations in DNMT3A gene, and the results were compared with those of Sanger sequencing as the gold standard test for detection of such mutations. Results: Among 220 samples from AML patients, Sanger sequencing detected 25 (11.4%) patients as having DNMT3A R882 mutations. HRM assay detected mutations in 23 (92%) samples and reported two false-negative results that were related to poor-quality DNA samples. There was an overall good agreement between direct sequencing and HRM assay (kappa value of 0.95) (p<0.001). Sensitivity assay showed that the analytical detection limits for HRM were 10% for the detection of R882H mutation compared with Sanger sequencing at 25%. Both Sanger sequencing and HRM assay reported no false-positive results. Conclusion: HRM curve analysis can be considered as a sensitive, fast, and high-throughput method for the detection of DNMT3A R882 mutation in AML patients. These results validate HRM analysis as an alternative method to Sanger sequencing because of its simplicity along with the lower cost and less required time.

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عنوان ژورنال

دوره 8  شماره 3

صفحات  172- 179

تاریخ انتشار 2018-05

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