Genome-wide methylation profiling and copy number analysis in atypical fibroxanthomas and pleomorphic dermal sarcomas indicate a similar molecular phenotype

被引:45
作者
Koelsche, Christian [1 ]
Stichel, Damian [2 ,3 ,4 ]
Griewank, Klaus G. [5 ,6 ,7 ]
Schrimpf, Daniel [2 ,3 ,4 ]
Reuss, David E. [2 ,3 ,4 ]
Bewerunge-Hudler, Melanie [4 ,8 ]
Vokuhl, Christian [9 ]
Dinjens, Winand N. M. [10 ]
Petersen, Iver [11 ]
Mittelbronn, Michel [12 ,13 ,14 ,15 ]
Cuevas-Bourdier, Adrian [13 ]
Buslei, Rolf [16 ]
Pfister, Stefan M. [4 ,17 ,18 ,19 ]
Flucke, Uta [20 ]
Mechtersheimer, Gunhild [1 ]
Mentzel, Thomas [21 ]
von Deimling, Andreas [2 ,3 ,4 ]
机构
[1] Heidelberg Univ Hosp, Inst Pathol, Dept Gen Pathol, Neuenheimer Feld 224, D-69120 Heidelberg, Baden Wurttembe, Germany
[2] Heidelberg Univ Hosp, Inst Pathol, Dept Neuropathol, Neuenheimer Feld 224, D-69120 Heidelberg, Baden Wurttembe, Germany
[3] German Canc Res Ctr, Clin Cooperat Unit Neuropathol, Heidelberg, Baden Wurttembe, Germany
[4] German Canc Consortium DKTK, Core Ctr Heidelberg, Heidelberg, Baden Wurttembe, Germany
[5] Univ Duisburg Essen, Wset German Canc Ctr, Univ Hosp Essen, Dept Dermatol, Essen, North Rhine Wes, Germany
[6] German Canc Consortium DKTK, Essen, North Rhine Wes, Germany
[7] Dermatopathol Mainz, Nieder Olm, Rhineland Palat, Germany
[8] German Canc Res Ctr, Microarray Unit, Genom & Prote Core Facil, Heidelberg, Baden Wurttembe, Germany
[9] Univ Hosp Schleswig Holstein, Dept Pediat Pathol, Kiel, Schleswig Holst, Germany
[10] Erasmus MC, Dept Pathol, Rotterdam, Netherlands
[11] SRH Poliklin Gera GmbH, Inst Pathol, Gera, Germany
[12] Luxembourg Ctr Neuropathol LCNP, Luxembourg, Luxembourg
[13] LNS, Dudelange, Luxembourg
[14] Univ Luxembourg, LCSB, Luxembourg, Luxembourg
[15] LIH, NORLUX Neurooncol Lab, Luxembourg, Luxembourg
[16] Sozialstiftung Bamberg, Inst Pathol, Bamberg, Germany
[17] NCT Heidelberg KiTZ, Hopp Childrens Canc Ctr, Heidelberg, Germany
[18] German Canc Res Ctr, Div Pediat Neurooncol, Heidelberg, Baden Wurttembe, Germany
[19] Heidelberg Univ, Dept Pediat Oncol Hematol & Immunol, Heidelberg, Baden Wurttembe, Germany
[20] Radboud Univ Nijmegen, Med Ctr, Dept Pathol, Nijmegen, Netherlands
[21] Dermatopathol Bodensee, Friedrichshafen, Baden Wurttembe, Germany
关键词
Pleomorphic dermal sarcoma; Atypical fibroxanthoma; Sarcomas; Melanomas; Carcinomas; Mimics; DNA methylation; Profiling; DNA METHYLATION; NERVOUS-SYSTEM; CLASSIFICATION; MELANOMA; CANCER; TUMORS; HEAD; CYTOKERATIN; MULTICENTER; MUTATIONS;
D O I
10.1186/s13569-019-0113-6
中图分类号
R73 [肿瘤学];
学科分类号
100214 ;
摘要
Background: Atypical fibroxanthomas (AFX) and pleomorphic dermal sarcomas (PDS) are lesions of the skin with overlapping histologic features and unspecific molecular traits. PDS behaves aggressive compared to AFX. Thus, a precise delineation, although challenging in some instances, is relevant. Methods: We examined the value of DNA-methylation profiling and copy number analysis for separating these tumors. DNA-methylation data were generated from 17 AFX and 15 PDS using the Illumina EPIC array. These were compared with DNA-methylation data generated from 196 tumors encompassing potential histologic mimics like cutaneous squamous carcinomas (cSCC; n = 19), basal cell carcinomas (n = 10), melanoma metastases originating from the skin (n = 11), leiomyosarcomas (n = 11), angiosarcomas of the skin and soft tissue (n = 11), malignant peripheral nerve sheath tumors (n = 19), dermatofibrosarcomas protuberans (n = 13), extraskeletal myxoid chondrosarcomas (n = 9), myxoid liposarcomas (n = 14), schwannomas (n = 10), neurofibromas (n = 21), alveolar (n = 19) and embryonal (n = 17) rhabdomyosarcomas as well as undifferentiated pleomorphic sarcomas (n = 12). Results: DNA-methylation profiling did not separate AFX from PDS. The DNA-methylation profiles of the other cases, however, were distinct from AFX/PDS. They reliably assigned to subtype-specific DNA-methylation clusters, although overlap occurred between some AFX/PDS and cSCC. Copy number profiling revealed alterations in a similar frequency and distribution between AFX and PDS. They involved losses of 9p (22/32) and 13q (25/32). Gains frequently involved 8q (8/32). Notably, a homozygous deletion of CDKN2A was more frequent in PDS (6/15) than in AFX (2/17), whereas amplifications were non-recurrent and overall rare (5/32). Conclusions: Our findings support the concept that AFX and PDS belong to a common tumor spectrum. We could demonstrate the diagnostic value of DNA-methylation profiling to delineating AFX/PDS from potential mimics. However, the assessment of certain histologic features remains crucial for separating PDS from AFX.
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