Enhancer hijacking determines extrachromosomal circular MYCN amplicon architecture in neuroblastoma

Author:

Helmsauer KonstantinORCID,Valieva Maria E.ORCID,Ali SalaheddineORCID,Chamorro González RocíoORCID,Schöpflin Robert,Röefzaad Claudia,Bei YiORCID,Dorado Garcia HeathcliffORCID,Rodriguez-Fos EliasORCID,Puiggròs MontserratORCID,Kasack Katharina,Haase KerstinORCID,Keskeny Csilla,Chen Celine Y.ORCID,Kuschel Luis P.ORCID,Euskirchen PhilippORCID,Heinrich Verena,Robson Michael I.ORCID,Rosswog Carolina,Toedling JoernORCID,Szymansky AnnabellORCID,Hertwig Falk,Fischer MatthiasORCID,Torrents David,Eggert Angelika,Schulte Johannes H.ORCID,Mundlos Stefan,Henssen Anton G.ORCID,Koche Richard P.ORCID

Abstract

AbstractMYCN amplification drives one in six cases of neuroblastoma. The supernumerary gene copies are commonly found on highly rearranged, extrachromosomal circular DNA (ecDNA). The exact amplicon structure has not been described thus far and the functional relevance of its rearrangements is unknown. Here, we analyze the MYCN amplicon structure using short-read and Nanopore sequencing and its chromatin landscape using ChIP-seq, ATAC-seq and Hi-C. This reveals two distinct classes of amplicons which explain the regulatory requirements for MYCN overexpression. The first class always co-amplifies a proximal enhancer driven by the noradrenergic core regulatory circuit (CRC). The second class of MYCN amplicons is characterized by high structural complexity, lacks key local enhancers, and instead contains distal chromosomal fragments harboring CRC-driven enhancers. Thus, ectopic enhancer hijacking can compensate for the loss of local gene regulatory elements and explains a large component of the structural diversity observed in MYCN amplification.

Publisher

Springer Science and Business Media LLC

Subject

General Physics and Astronomy,General Biochemistry, Genetics and Molecular Biology,General Chemistry

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