Comprehensive genetic characterization of pediatric T-cell acute lymphoblastic leukemia

Karrman, Kristina; Castor, Anders; Behrendtz, Mikael; Forestier, Erik; Olsson, Linda; Ehinger, Mats; Biloglav, Andrea; Fioretos, Thoas; Paulsson, Kajsa; Johansson, Bertil

Comprehensive genetic characterization of pediatric T-cell acute lymphoblastic leukemia

Mark

Karrman, Kristina ^LU ; Castor, Anders ^LU ; Behrendtz, Mikael ; Forestier, Erik ; Olsson, Linda ^LU ; Ehinger, Mats ^LU ; Biloglav, Andrea ^LU ; Fioretos, Thoas ^LU ; Paulsson, Kajsa ^LU and Johansson, Bertil ^LU (2014) 56th Annual Meeting of the American Society of Hematology In Blood 124(21). p.1084-1084

Abstract: A comprehensive genetic characterization comprising conventional chromosome banding, fluorescence in situ hybridization (FISH), and single nucleotide polymorphism (SNP) array analyses as well as large-scale sequencing of 75 genes were performed on a consecutive series of 47 pediatric T-cell acute lymphoblastic leukemia (T-ALL) patients. An abnormal karyotype was identified in 46% of the cases. Recurrent cytogenetic aberrations comprised T-cell receptor (TCR) translocations and deletions of 6q and 9p. FISH analyses of TCR rearrangements were positive in 26% of the investigated cases. The vast majority (37/39; 95%) of cases analyzed by SNP arrays displayed aberrations, with a median of 3 changes (range 0-11) per case. The genes recurrently... (More); A comprehensive genetic characterization comprising conventional chromosome banding, fluorescence in situ hybridization (FISH), and single nucleotide polymorphism (SNP) array analyses as well as large-scale sequencing of 75 genes were performed on a consecutive series of 47 pediatric T-cell acute lymphoblastic leukemia (T-ALL) patients. An abnormal karyotype was identified in 46% of the cases. Recurrent cytogenetic aberrations comprised T-cell receptor (TCR) translocations and deletions of 6q and 9p. FISH analyses of TCR rearrangements were positive in 26% of the investigated cases. The vast majority (37/39; 95%) of cases analyzed by SNP arrays displayed aberrations, with a median of 3 changes (range 0-11) per case. The genes recurrently deleted were CDKN2A, CDKN2B, LEF1, PTEN, RBI, and STIL. One case displayed chromothripsis involving 6q. No case had a whole chromosome uniparental isodisomy (wUPID); in fact, only one T-ALL of 123 informative cases in the literature has had a wUPID. However, segmental UPIDs (sUPIDs) were seen in 44% of the present cases, with most being sUPID9p. CDKN2A was homozygously deleted in all cases with sUPID9p, with a heterozygous deletion occurring prior to the sUPID9p in all instances. There was no evidence for chromosomal instability when comparing diagnostic and relapse samples. Among the genes sequenced, 14 were mutated in 28 cases. The genes targeted are involved in signaling transduction, epigenetic regulation, and transcription. In some cases, NOTCH1 mutations were seen in minor subclones and lost at relapse, showing that such mutations also can be secondary events. These findings support a multistep leukemogenic process. (Less)

Please use this url to cite or link to this publication: https://lup.lub.lu.se/record/9a2db845-1024-4d8a-a0ee-36ef5d5bf279

author

Karrman, Kristina ^LU ; Castor, Anders ^LU ; Behrendtz, Mikael ; Forestier, Erik ; Olsson, Linda ^LU ; Ehinger, Mats ^LU ; Biloglav, Andrea ^LU ; Fioretos, Thoas ^LU ; Paulsson, Kajsa ^LU and Johansson, Bertil ^LU

organization

publishing date

2014-12-06

type

Contribution to journal

publication status

published

subject

Medical Genetics

keywords

T lymphocyte receptor, T lymphocyte, acute lymphoblastic leukemia, American, society, hematology, gene, mutation, relapse, chromosome, chromosome aberration, human, patient, single nucleotide polymorphism, fluorescence in situ hybridization, diagnosis, chromosomal instability, uniparental disomy, chromosome banding pattern

in

Blood

volume

124

issue

21

pages

1084 - 1084

publisher

American Society of Hematology

conference name

56th Annual Meeting of the American Society of Hematology

conference location

San Francisco, United States

conference dates

2014-12-06 - 2014-12-09

ISSN

1528-0020

language

English

LU publication?

yes

id

9a2db845-1024-4d8a-a0ee-36ef5d5bf279

date added to LUP

2017-09-10 22:03:42

date last changed

2018-11-21 21:34:31

@misc{9a2db845-1024-4d8a-a0ee-36ef5d5bf279,
  abstract     = {{A comprehensive genetic characterization comprising conventional chromosome banding, fluorescence in situ hybridization (FISH), and single nucleotide polymorphism (SNP) array analyses as well as large-scale sequencing of 75 genes were performed on a consecutive series of 47 pediatric T-cell acute lymphoblastic leukemia (T-ALL) patients. An abnormal karyotype was identified in 46% of the cases. Recurrent cytogenetic aberrations comprised T-cell receptor (TCR) translocations and deletions of 6q and 9p. FISH analyses of TCR rearrangements were positive in 26% of the investigated cases. The vast majority (37/39; 95%) of cases analyzed by SNP arrays displayed aberrations, with a median of 3 changes (range 0-11) per case. The genes recurrently deleted were CDKN2A, CDKN2B, LEF1, PTEN, RBI, and STIL. One case displayed chromothripsis involving 6q. No case had a whole chromosome uniparental isodisomy (wUPID); in fact, only one T-ALL of 123 informative cases in the literature has had a wUPID. However, segmental UPIDs (sUPIDs) were seen in 44% of the present cases, with most being sUPID9p. CDKN2A was homozygously deleted in all cases with sUPID9p, with a heterozygous deletion occurring prior to the sUPID9p in all instances. There was no evidence for chromosomal instability when comparing diagnostic and relapse samples. Among the genes sequenced, 14 were mutated in 28 cases. The genes targeted are involved in signaling transduction, epigenetic regulation, and transcription. In some cases, NOTCH1 mutations were seen in minor subclones and lost at relapse, showing that such mutations also can be secondary events. These findings support a multistep leukemogenic process.}},
  author       = {{Karrman, Kristina and Castor, Anders and Behrendtz, Mikael and Forestier, Erik and Olsson, Linda and Ehinger, Mats and Biloglav, Andrea and Fioretos, Thoas and Paulsson, Kajsa and Johansson, Bertil}},
  issn         = {{1528-0020}},
  keywords     = {{T lymphocyte receptor; T lymphocyte; acute lymphoblastic leukemia; American; society; hematology; gene; mutation; relapse; chromosome; chromosome aberration; human; patient; single nucleotide polymorphism; fluorescence in situ hybridization; diagnosis; chromosomal instability; uniparental disomy; chromosome banding pattern}},
  language     = {{eng}},
  month        = {{12}},
  note         = {{Conference Abstract}},
  number       = {{21}},
  pages        = {{1084--1084}},
  publisher    = {{American Society of Hematology}},
  series       = {{Blood}},
  title        = {{Comprehensive genetic characterization of pediatric T-cell acute lymphoblastic leukemia}},
  volume       = {{124}},
  year         = {{2014}},
}

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Comprehensive genetic characterization of pediatric T-cell acute lymphoblastic leukemia