DNA methylation-based subtype prediction for pediatric acute lymphoblastic leukemia.

Abrahamsson, Jonas; Barbany, Gisela; Bäcklin, Christofer L; Cavelier, Lucia; Dahlberg, Johan; Flaegstad, Trond; Forestier, Erik; Gustafsson, Mats G; Heyman, Mats M; Jónsson, Ólafur G; Kanerva, Jukka; Larsson, Rolf; Lönnerholm, Gudmar; Nordgren, Ann; Nordlund, Jessica; Palle, Josefine; Schmiegelow, Kjeld; Syvänen, Ann-Christine; Zachariadis, Vasilios; Öfverholm, Ingegerd; Övernäs, Elin

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DNA methylation-based subtype prediction for pediatric acute lymphoblastic leukemia.

Authors: Jonas Abrahamsson
Gisela Barbany
Christofer L Bäcklin
Lucia Cavelier
Johan Dahlberg
Trond Flaegstad
Erik Forestier
Mats G Gustafsson
Mats M Heyman
Ólafur G Jónsson
Jukka Kanerva
Rolf Larsson
Gudmar Lönnerholm
Ann Nordgren
Jessica Nordlund
Josefine Palle
Kjeld Schmiegelow
Ann-Christine Syvänen
Vasilios Zachariadis
Ingegerd Öfverholm
Elin Övernäs
Publication date: 1 January 2015
Publisher: 'Springer Science and Business Media LLC'
Doi

Abstract

To access publisher's full text version of this article, please click on the hyperlink in Additional Links field or click on the hyperlink at the top of the page marked Files. This article is open access.We present a method that utilizes DNA methylation profiling for prediction of the cytogenetic subtypes of acute lymphoblastic leukemia (ALL) cells from pediatric ALL patients. The primary aim of our study was to improve risk stratification of ALL patients into treatment groups using DNA methylation as a complement to current diagnostic methods. A secondary aim was to gain insight into the functional role of DNA methylation in ALL.We used the methylation status of ~450,000 CpG sites in 546 well-characterized patients with T-ALL or seven recurrent B-cell precursor ALL subtypes to design and validate sensitive and accurate DNA methylation classifiers. After repeated cross-validation, a final classifier was derived that consisted of only 246 CpG sites. The mean sensitivity and specificity of the classifier across the known subtypes was 0.90 and 0.99, respectively. We then used DNA methylation classification to screen for subtype membership of 210 patients with undefined karyotype (normal or no result) or non-recurrent cytogenetic aberrations ('other' subtype). Nearly half (n = 106) of the patients lacking cytogenetic subgrouping displayed highly similar methylation profiles as the patients in the known recurrent groups. We verified the subtype of 20% of the newly classified patients by examination of diagnostic karyotypes, array-based copy number analysis, and detection of fusion genes by quantitative polymerase chain reaction (PCR) and RNA-sequencing (RNA-seq). Using RNA-seq data from ALL patients where cytogenetic subtype and DNA methylation classification did not agree, we discovered several novel fusion genes involving ETV6, RUNX1, and PAX5.Our findings indicate that DNA methylation profiling contributes to the clarification of the heterogeneity in cytogenetically undefined ALL patient groups and could be implemented as a complementary method for diagnosis of ALL. The results of our study provide clues to the origin and development of leukemic transformation. The methylation status of the CpG sites constituting the classifiers also highlight relevant biological characteristics in otherwise unclassified ALL patients.Swedish Foundation for Strategic Research RBc08-008 Swedish Cancer Society CAN2010/592 Swedish Childhood Cancer Foundation 11098 Swedish Research Council for Science and Technology 90559401 Swedish Research Council FORTE Swedish Research Council FORMAS Swedish Research Council VINNOVA Swedish Research Council VR 259-2012-2

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