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Molecular Screening in Anaplastic Lymphoma Kinase–Positive Anaplastic Large Cell Lymphoma: Anaplastic Lymphoma Kinase Analysis, Next-Generation Sequencing Fusion Gene Detection, and T-Cell Receptor Immunoprofiling

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Autor
Kalinová, MarkétaScopus Profile - 6701522367
Mrhalová, MarcelaScopus Profile - 6602309568
Kabíčková, EditaScopus Profile - 6602305248
Svatoň, MichaelORCiD Profile - 0000-0003-2966-3687WoS Profile - AAB-3869-2019Scopus Profile - 56440286100
Skotnicová, AnetaORCiD Profile - 0000-0001-7067-7795WoS Profile - FWF-8689-2022Scopus Profile - 57222366563
Prouzová, ZuzanaORCiD Profile - 0000-0002-7507-0797WoS Profile - AAB-4565-2021Scopus Profile - 6504770501
Křenová, Zdenka
Kolenová, Alexandra
Divoká, Martina
Froňková, EvaORCiD Profile - 0000-0002-6900-8145Scopus Profile - 8905682100
Kodet, RomanScopus Profile - 56045477600

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Datum vydání
2024
Publikováno v
Modern Pathology
Ročník / Číslo vydání
37 (3)
ISBN / ISSN
ISSN: 0893-3952
ISBN / ISSN
eISSN: 1530-0285
Informace o financování
UK//COOP
MZ0//NU20-03-00284
FN//V-VFN
UK/GAUK/GAUK318321
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Kolekce
  • 3. lékařská fakulta

Tato publikace má vydavatelskou verzi s DOI 10.1016/j.modpat.2024.100428

Abstrakt
Anaplastic lymphoma kinase-positive anaplastic large cell lymphoma (ALK+ ALCL) originates from the T-lineage and is marked by rearrangements of the ALK gene. Over ten fusion partners with the ALK gene are known, with the most common being the t(2;5)(p23;q35) translocation resulting in the NPM1::ALK fusion. In 10-20% of ALK+ ALCL cases, the ALK gene fuses with various other partners. Modern molecular techniques, especially next-generation sequencing (NGS), have eased the identification of ALK gene fusion partners and have allowed in-depth characterization of the TCR repertoire. We devised a quantitative RT-qPCR to measure the expression of the translocated portion of the ALK gene. Fusion partners for the ALK gene were analyzed using Rapid Amplification of 5'cDNA (RACE) or NGS. T-cell Receptor (TCR) immunoprofiling was performed by amplicon NGS. We studied 96 ALK+ ALCL patients. NPM1::ALK fusion gene was observed in 71 patients, ATIC::ALK in 9, and TPM3::ALK in 3. CLTC::ALK, MYH9::ALK, and RNF213::ALK fusions were identified in 2 patients each. We also discovered the TPM4::ALK and SATB1::ALK fusion genes, plus two previously unidentified ALK+ ALCL fusions: SQSTM1::ALK and CAPRIN1::ALK. High expression of the translocated ALK gene segment was observed in all 93 analyzed samples. TCR testing was conducted on 23 patients with available DNA. In 18 (78%), we discerned at least one (ranging from 1-4) clonal TCR rearrangement. In 59% of patients, clonal TCRB junctions corresponded with sequences previously observed in both healthy donors and under various pathological conditions. RT-qPCR detection of ALK expression is a fast and reliable method for both diagnosing and monitoring treatment response in ALK+ ALCL patients, irrespective of the ALK gene translocation. NGS reveals new ALK translocation partners. Both the malignant and reactive TCR repertoires in ALK+ ALCL patients are unique and do not consistently occur among different patients.
Klíčová slova
ALK expression, Anaplastic large cell lymphoma (ALCL), fusion genes ALCL, gene/protein ALK, immunoglobulin and T-cell receptor gene rearrangements, next generation sequencing (NGS)
Trvalý odkaz
https://hdl.handle.net/20.500.14178/2561
Zobraz publikaci v dalších systémech
WOS:001185168200001
SCOPUS:2-s2.0-85185557554
PUBMED:38266918
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Licence pro užití plného textu výsledku: Creative Commons Uveďte původ 4.0 International

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