Highly Sensitive Detection of IDH2 Mutations in Acute Myeloid Leukemia

被引:11
|
作者
Petiti, Jessica [1 ]
Rosso, Valentina [1 ]
Croce, Eleonora [1 ]
Franceschi, Vanessa [1 ]
Andreani, Giacomo [1 ]
Dragani, Matteo [1 ]
De Gobbi, Marco [1 ]
Lunghi, Monia [2 ]
Saglio, Giuseppe [1 ]
Fava, Carmen [1 ]
Lo Iacono, Marco [1 ]
Cilloni, Daniela [1 ]
机构
[1] Univ Turin, San Luigi Gonzaga Hosp, Dept Clin & Biol Sci, Reg Gonzole 10, I-10043 Turin, Italy
[2] Univ Piemonte Orientale, Dept Translat Med, Div Hematol, Corso Giuseppe Mazzini 18, I-28100 Novara, Italy
关键词
AML; IDH2; R140Q; R172K; PNA-PCR clamping; droplet digital PCR; diagnostic assay; POLYMERASE-CHAIN-REACTION; MINIMAL RESIDUAL DISEASE; ONCOMETABOLITE; 2-HYDROXYGLUTARATE; EPIDEMIOLOGY; CANCER; ADULTS;
D O I
10.3390/jcm9010271
中图分类号
R5 [内科学];
学科分类号
1002 ; 100201 ;
摘要
Background: Acute myeloid leukemia is a heterogeneous hematological disease, characterized by karyotypic and molecular alterations. Mutations in IDH2 have a role in diagnosis and as a minimal residue disease marker. Often the variant allele frequency during follow up is less than 20%, which represents the limit of detection of Sanger sequencing. Therefore, the development of sensitive methodologies to identify IDH2 mutations might help to monitor patients' response to therapy. We compared three different methods to identify and monitor IDH2 mutations in patients' specimens. Methods: Performances of PNA-PCR clamping, droplet digital PCR and Sanger for IDH2 status identification were evaluated and compared in 96 DNA patients' specimens. Results: In contrast with Sanger sequencing, our results highlighted the concordance between PNA clamping and digital PCR. Furthermore, PNA-PCR clamping was able to detect more mutated DNA with respect to Sanger sequencing that showed several false negatives independently from the allelic frequency. Conclusions: We found that PNA-PCR clamping and digital PCR identified IDH2 mutations in DNA samples with comparable results in a percentage significantly higher compared to Sanger sequencing. PNA-PCR clamping can be used even in laboratories not equipped for sophisticated analyses, decreasing cost and time for IDH2 characterization.
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页数:11
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