Pan-cancer analysis of somatic copy-number alterations implicates IRS4 and IGF2 in enhancer hijacking (original) (raw)
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Acknowledgements
This research project was funded in part through Network of Excellence funding by the European Commission (260791 to J.O.K. and A.H.), grants from the German Ministry for Science and Education (BMBF) (01KU1505F to J.O.K. and S.M.P.; 01ZX1303A to R.T. and M.P.; 01ZX1406 to M.P.), a European Research Council (ERC) Starting Grant (336045 to J.O.K.), the Danish Medical Research Council (DFF-4183-00233 to J.W.), the DFG (KFO 227/BA 4806/1-2 to C.R.B. and KFO 227/GL286/1-1 to H.G.), the Baden–Württemberg Stiftung (P-LS-ASII/33 to C.R.B. and H.G.), iMed (Helmholtz Initiative on Personalized Oncology to H.G.), the EU framework program Horizon2020 (TRANSCAN-2 ERA-NET to H.G.), and the German Cancer Aid (Colon-Resist-Net to C.R.B. and H.G.). S.M.W. received funding through an SNSF Early Postdoc Mobility Fellowship (P2ELP3_155365) and an EMBO Long-Term Fellowship (ALTF 755-2014). T.D. was supported by a scholarship from the German Cancer Research Center. S.M.D. was supported by the Heidelberg School of Oncology. The results reported here are in part based upon data generated by the TCGA Research Network (“URLs”), and we acknowledge the specimen donors as well as the research groups involved in the sampling, sequencing and processing of these data. We are grateful to the NCT Tissue Bank for providing samples in accordance with the regulations of the tissue bank and the approval of the ethics committee of Heidelberg University. We are grateful to the GeneCore, IT, mouse facility and Flow Cytometry core facilities at EMBL for excellent assistance. We thank E. Furlong and B. Klaus for valuable discussions during early stages of this project, N. Sidiropoulos for assistance with Hi-C plots, and N. Habermann for assistance with manuscript formatting and proofreading. pMD2.G and psPAX2 were gifts from D. Trono (EPFL, Lausanne, France).
Author information
Author notes
- Joachim Weischenfeldt, Taronish Dubash and Alexandros P Drainas: These authors jointly supervised this work.
Authors and Affiliations
- European Molecular Biology Laboratory (EMBL), Genome Biology Unit, Heidelberg, Germany
Joachim Weischenfeldt, Alexandros P Drainas, Balca R Mardin, Adrian M Stütz, Sebastian M Waszak, Benjamin Raeder, Theocharis Efthymiopoulos, Serap Erkek, Thomas Zichner & Jan O Korbel - The Finsen Laboratory, Rigshospitalet, University of Copenhagen, Copenhagen, Denmark
Joachim Weischenfeldt - Biotech Research and Innovation Centre (BRIC), Copenhagen, Denmark
Joachim Weischenfeldt - Department of Translational Oncology, National Center for Tumor Diseases (NCT), Heidelberg, Germany
Taronish Dubash, Christine Siegl, Sebastian M Dieter, Claudia R Ball & Hanno Glimm - Division of Translational Oncology, German Cancer Research Center (DKFZ), Heidelberg, Germany
Taronish Dubash, Christine Siegl, Sebastian M Dieter, Claudia R Ball & Hanno Glimm - Division of Molecular Thoracic Oncology, German Cancer Research Center (DKFZ), Heidelberg, Germany
Yuanyuan Chen & Rocio Sotillo - Department of Translational Genomics, Center of Integrated Oncology Cologne–Bonn, Medical Faculty, University of Cologne, Cologne, Germany
Graziella Bosco, Roman Thomas & Martin Peifer - Department of Cancer Genetics, Institute for Cancer Research, Oslo University Hospital–The Norwegian Radium Hospital, Oslo, Norway
Ann Rita Halvorsen, Odd Terje Brustugun & Aslaug Helland - Division of Pediatric Neurooncology, German Cancer Research Center (DKFZ), Heidelberg, Germany
Serap Erkek & Stefan M Pfister - Division of Clinical Epidemiology and Aging Research, German Cancer Research Center (DKFZ), Heidelberg, Germany
Hermann Brenner - Department of Oncology, Oslo University Hospital–The Norwegian Radium Hospital, Oslo, Norway
Odd Terje Brustugun & Aslaug Helland - Developmental Neurobiology, St. Jude Children's Research Hospital, Memphis, Tennessee, USA
Paul A Northcott - Institute of Pathology, Jena University Hospital, Jena, Germany
Iver Petersen - General Surgery, Heidelberg University Clinics, Heidelberg, Germany
Martin Schneider - Department of Cardiothoracic Surgery, Oslo University Hospital–Rikshospitalet, Oslo, Norway
Steinar K Solberg - Department of Pathology, VU University Medical Center, Amsterdam, the Netherlands
Erik Thunissen - Institute of Pathology, Technical University Munich, Munich, Germany
Wilko Weichert - Department of Pathology, University Hospital Cologne, Cologne, Germany
Wilko Weichert & Roman Thomas - German Consortium for Translational Cancer Research (DKTK), German Cancer Research Center (DKFZ), Heidelberg, Germany
Wilko Weichert, Claudia R Ball & Hanno Glimm - Center for Molecular Medicine Cologne (CMMC), University of Cologne, Cologne, Germany
Martin Peifer - European Molecular Biology Laboratory (EMBL), Cell Biology Unit, Heidelberg, Germany
Martin Jechlinger - European Molecular Biology Laboratory–European Bioinformatics Institute (EMBL-EBI), Wellcome Trust Genome Campus, Cambridge, UK
Jan O Korbel
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Contributions
H.G. and J.O.K. share joint senior authorship. J.W. and J.O.K. developed the CESAM methodology; J.W., A.P.D., S.M.W., T.Z., S.E. and J.O.K. carried out computational pan-cancer analysis of the TCGA public resource data set; J.W., A.P.D., B.R.M., T.D., C.R.B., H.G. and J.O.K. designed experiments; A.P.D., B.R.M., A.M.S., T.D., B.R., T.E., G.B., R.T., M.P., A.R.H., A.H., C.R.B., J.W., H.G. and J.O.K. worked on experiments in primary cancer samples; A.P.D., B.R., A.M.S., T.E., B.R.M., J.W. and J.O.K. conducted experiments in cell lines; T.D., A.P.D., B.R.M., A.M.S., S.M.D., J.W., C.R.B., H.G. and J.O.K. conducted experiments in spheroid cultures; C.S., S.M.D., C.R.B. and H.G. carried out enhancer luciferase experiments; J.W., A.P.D., B.R.M., Y.C., T.D., C.R.B., H.G. and J.O.K. prepared manuscript display items; M.S., A.H., M.P., H.B., W.W., O.T.B., P.A.N., S.M.P., I.P., S.K.S. and E.T. provided clinical information and human cancer tissue; W.W. carried out pathology analysis of spheroids; Y.C., A.P.D. and S.M.W. performed mouse experiments; and R.S., M.J., A.P.D., Y.C., J.W. and J.O.K. designed mouse experiments.
Corresponding authors
Correspondence toHanno Glimm or Jan O Korbel.
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Competing interests
The authors declare no competing financial interests.
Integrated supplementary information
Supplementary Figure 1 P value distribution and relative distance to genomic features of CESAM hits.
(a) QQ plot depicting observed _P_-values (-log10) in comparison to expected _P_-values (-log10). (b) Shadow figure to Figure 1d. Relative proximity to genetic elements compared to background (mann-whitney U test) for CESAM hits (‘CESAM’) versus ‘CONTROL’.
Supplementary Figure 2 Pan-cancer and ACC-specific CESAM analysis of gene expression changes for _TERT_-locus-proximal genes.
Related to main Figure 2. (a) Pan-cancer CESAM analysis of expression for genes in the vicinity of TERT, which demonstrates TERT as plausible target. (b) ACC-specific CESAM analysis of expression for genes in the vicinity of TERT, which demonstrates TERT as plausible target. For tumor type abbreviations, see Supplementary Table 6.
Supplementary Figure 3 Recurrent deletions at a TAD boundary on chromosome X are associated with IRS4 dysregulation in different cancer types.
Related to main Figure 3. A genomic region near IRS4 (a gene transcribed from the (-) strand of the reference genome), highlighted in yellow, exhibiting clustered transcription factor binding sites is highlighted in gray. Each SCNA is accompanied with the depicted expression fold change of IRS4 (shown adjacent to each SCNA). Samples harboring the cis deletion, but not samples without the cis deletion, exhibit H3K27ac chromatin marks at IRS4 as well as at the candidate CRE nearby (highlighted in grey; asterisks indicate significant differential H3K27ac marks between carriers and non-carriers). 4C-Seq experiments using the candidate CRE as a viewpoint clearly demonstrate physical interaction with IRS4; a similar intensity in interaction was observed in samples harboring the cis deletion as in samples lacking the deletion. And also 4C-Seq experiments using the gene as a viewpoint show interaction between IRS4 and the putative CRE in both deletion carriers and non-carriers. LUSC samples S00086, S00473 and S00166 were verified, using semi-quantitative RT-PCR, to exhibit high-level upregulation of IRS4, whereas S00478 and S00198 showed merely baseline-level expression (data not shown). For all remaining carrier and non-carrier samples, we verified outlier and non-outlier expression, respectively, by qPCR (Supplementary Table 3).
Supplementary Figure 4 IRS4 CESAM pan-cancer frequency and association with IRS2 and FGFR1.
Related to main Figure 3. (a) Fraction of donors per cancer type for which CESAM inferred IRS4 dysregulation in conjunction with SCNAs in cis in at least 3 donors. For tumor type abbreviations, see Supplementary Table 6. (b) _IRS4_-IRS2 gene expression correlation plot, showing significantly anticorrelated expression (_P_=0.008, Pearson correlation; _r_=-0.11) (c) Co-occurrence heatmap of samples exhibiting IRS4 CESAM hits versus FGFR1 amplification in LUSC samples (ctrl: control). Significant co-occurrence was seen with _P_=0.006 (Pearson’s chi-square test).
Supplementary Figure 5 Cancer-type-specific CESAM analysis of gene expression changes for structural variants versus control of IRS4 locus-proximal genes.
Related to main Figure 3. IRS4, COL4A5, COL4A6, VSIG1, PSMD10 and ATG4A expression values (RSEM) for SVs and controls, shown for different cancer types as well as for the pan-cancer setting. IRS4 represents the most consistently upregulated gene, and SCNAs clearly appear to converge on IRS4 overexpression at this extended genomic locus, implicating IRS4 as a plausible candidate gene.
Supplementary Figure 6 Cancer-type-specific CESAM analysis of gene expression changes for _IRS4_-locus-proximal genes.
Related to main Figure 3 and Supplementary Figure 5. IRS4, COL4A5, COL4A6, VSIG1, PSMD10 and ATG4A expression values (RSEM) for deletions (del), duplications (dup), amplifications (amp) and controls for different cancer types as well as in a pan-cancer setting. IRS4 is the most consistently upregulated gene.
Supplementary Figure 7 Tumor progression of transplanted _IRS4_-overexpressing HCC-15 cells and mock control in mouse model.
Related to main Figure 3. (a) Boxplots depicting mouse tumor progression curves of HCC-15 cells containing _IRS4_-expressing lentiviral constructs (pLenti-IRS4) versus mock control (pLenti-empty HCC-15); 1x106 cells injected respectively; last time point: 1st _P_=0.046, 2nd _P_=0.03; two-tailed t-test; two-tailed t-test computed at last measured time point (day 39); _N_=8 for each group in first experiment, _N_=9 for control and _N_=12 for IRS4 overexpressing sample in second experiment. (b) RT-qPCR of the control HCC-15 and IRS4-HCC-15 tumors confirming IRS4 overexpression. (c) Flow cytometry of tumors injected with IRS4-IRES-GFP overexpressing vector HCC-15 cell line. (d) Representative immunohistochemistry experiment showing IRS4 overexpression in the harvested tumors (bottom panel) but not in the control tumors (top panel).
Supplementary Figure 8 Structural variant analysis of chromosome X from LUSC samples associated with IRS4 gene overexpression and controls.
Related to main Figure 3. Read depth plot and somatic SVs from mate-pair sequencing data of LUSC samples exhibiting IRS4 overexpression as well as LUSC controls samples with normal IRS4 expression level. The location of the IRS4 gene is indicated with a green arrow. Read depth changes and SV types are shown as colored graphs. IRS4 alterations included simple as well as more complex SV events including such showing evidence for chromosome shattering (also known as chromothripsis). IRS4 expression fold-change is shown for each sample.
Supplementary Figure 9 Proposed model for IRS4 overexpression by active chromatin spreading.
Related to main Figure 3. Proposed model for IRS4 overexpression by active chromatin spreading, resulting from clustered deletions at a TAD boundary in cis of IRS4.
Supplementary Figure 11 Recurrent somatic duplications at the IGF2 locus associated with IGF2 overexpression.
Related to main Figure 5. Recurrent somatic duplications at the IGF2 locus associating with IGF2 overexpression encompass a contact domain boundary and a non-cognate annotated super enhancer in the adjacent contact domain, but do not encompass the known IGF2 cognate enhancer (light blue). H3K27ac peaks show the presence of a non-cognate enhancer in the contact domain adjacent to the IGF2 locus. H2K27me3 marks for WT samples and samples harboring the duplication show absence of repressive chromatin at the adjacent non-cognate enhancer. 4C-Seq experiments using IGF2 as the viewpoint demonstrate a marked physical interaction between the IGF2 locus and the non-cognate enhancer in samples with the recurrent tandem duplication, but not in samples lacking the tandem duplication (WT). By comparison, no physical interaction is seen between IGF2 and its known cognate enhancer, neither in tandem duplication nor in WT samples. 4C-Seq experiments using the non-cognate enhancer as viewpoint verify the marked physical interaction with IGF2 in tandem duplication carriers and not in WT samples. Collectively, these results demonstrate that hijacking of a non-cognate super-enhancer, mediated by a contact domain spanning recurrent SCNA, drive overexpression of the IGF2 locus (see also Figure 5). CTCF marks for WT samples and samples harboring the duplication are consistent with the presence of TAD boundaries normally separating IGF2 and the non-cognate (super) enhancer. (b) IGF2 expression fold change versus copy number ratio (tumor/normal).
Supplementary Figure 12 Enhancer validation in primary CRC-derived spheroid cultures.
Related to main Figure 5. (a) Additional experiments to characterize the mechanism of gene dysregulation were pursued in (non-TCGA based) spheroid cultures obtained from primary CRC. (b) Distribution of IGF2 expression measurements in additional primary samples and spheroids. Two spheroids with marked overexpression, denoted CRCP5S and CRCP7S, were used for further characterization along with controls lacking IGF2 expression. Expression values are based on qPCR. (c) Functional activity of enhancer regions spanning the _IGF2_-interacting distal super-enhancer locus. Selected parts of the enhancer regions found to be interacting with the IGF2 locus in tandem-duplicated spheroid cells were amplified by PCR, cloned into a firefly luciferase reporter construct and co-transfected with a renilla luciferase control construct into the colon cancer cell line HCT116 as well as HeLa (cervical cancer cell line) cells used as a control. 48 h post transfection, cells were lysed and luciferase activities were measured. Firefly luciferase signal was normalized to renilla luciferase signal and displayed as fold activity normalized to empty vector control (Ctrl) (Mean ± SEM in triplicate).
Supplementary Figure 13 Single-copy super-enhancer juxtaposing tandem duplications result in IGF2 overexpression.
Related to main Figure 5. (a) Four IGF2 single copy gene duplications not associated with stark levels of IGF2 overexpression (orange bars) are shown next to IGF2 single-copy tandem duplications leading to ~300-fold IGF2 upregulation. Based on analyzing their relative position with respect to preexisting contact domains/TADs (black bars), 3/4 of these larger duplications are not able to bring IGF2 and the super-enhancer (SE) depicted in Fig. 5 into a single de novo contact domain – the lack of associated IGF2 overexpression is hence consistent with our new model of IGF2 dysregulation by enhancer hijacking (Fig. 5d). For the fourth duplication, juxtaposition of IGF2 and the SE is inferred to occur at a larger distance. (b) Gene expression fold-change for single-copy duplicated genes on chromosome 11. Single-copy IGF2 duplications not inferred to bring the SE and IGF2 into a de novo contact domain (denoted class A) and duplications inferred to juxtapose the SE and IGF2 bringing both elements into a de novo contact domain (class B) are depicted separately. For the observed 58 single-copy duplicated genes on chromosome 11 in CRC samples, the median gene expression increase was ~1.4-fold. (c) Panel supporting (b), showing significant difference in IGF2 expression between class A and class B single-copy IGF2 duplications (_P=_0.01; Wilcoxon rank-sum test). (d) RNA expression of IGF2 (y-axis) for class A (green dots) and class B (purple dots) versus the estimated distance in basepairs (bp) between IGF2 and the SE upon tandem duplication (x-axis).
Supplementary information
Supplementary Text and Figures
Supplementary Figures 1–13, Supplementary Table 7 and Supplementary Note (PDF 3005 kb)
Supplementary Table 1
Full list of CESAM hits in tumor-specific analysis (sheet 1) and tumor-type abbreviations (XLSX 44 kb)
Supplementary Table 2
SCNAs and fold-change expression from TERT, IRS4 and IGF2 CESAM analyses (XLSX 58 kb)
Supplementary Table 3
Xenograft mouse experiment data with _IRS4_-overexpressing HCC-15 LUSC cell lines and control. Data include tumor volume measurements, statistics and qPCR measurements. (XLSX 37 kb)
Supplementary Table 4
RT-qPCR data from LUSC samples to identify IRS4 overexpressors (separate Excel file). First, all 94 samples were tested in duplicate with IRS4 primers only; the results are provided in the “IRS4 Ct raw” column. Then, the 15 highest _IRS4_-expressing samples (taking the known RIN value into account) and 7 representative normal-expression samples were selected, and tests were repeated in another experiment using both IRS4 and globulin primers. The fold-change results after normalization with the housekeeping gene are reported. (XLSX 9 kb)
Supplementary Table 5
Patient characteristics and RT-qPCR data from CRC samples to identify IGF2 overexpressors (XLSX 12 kb)
Supplementary Table 6
Luciferase enhancer reporter experiment measurements (XLSX 12 kb)
Supplementary Table 8
Primer sequences (XLSX 10 kb)
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Weischenfeldt, J., Dubash, T., Drainas, A. et al. Pan-cancer analysis of somatic copy-number alterations implicates IRS4 and IGF2 in enhancer hijacking.Nat Genet 49, 65–74 (2017). https://doi.org/10.1038/ng.3722
- Received: 26 April 2016
- Accepted: 19 October 2016
- Published: 21 November 2016
- Issue Date: January 2017
- DOI: https://doi.org/10.1038/ng.3722