SETD2 mutations in primary central nervous system tumors

At our institutions, targeted NGS of brain tumor specimens is performed as part of routine patient care. Genomic tumor testing was performed at the Center for Personalized Diagnostics (CPD) at the University of Pennsylvania and the Division of Genomic Diagnostics (DGD) at the CHOP, both CLIA-approved laboratories. Genomic DNA from brain tumor specimens is extracted from fresh tissue, formalin-fixed paraffin-embedded tissues or frozen tissue. Tumor DNA is sequenced on an Illumina MiSeq or HiSeq, and the data are analyzed using in-house bioinformatics pipelines.

At the CPD, the Solid Tumor Sequencing panel uses a custom Agilent HaloPlex library preparation (Agilent, Santa Clara, CA) to cover approximately 0.5 megabases, including the entire exonic (coding) sequence of 152 genes, + 10 base pairs of intronic sequence. The 152 genes sequenced on the CPD panel may be found at (https://​www.​pennmedicine.​org/​departments-and-centers/​center-for-personalized-diagnostics/​gene-panels). The library preparation includes unique molecular identifiers to identify duplicate reads. Specimens are sequenced on the Illumina HiSeq 2500 platform (Illumina, San Diego, CA) using multiplexed, paired end reads. Analysis and interpretation is performed using a customized bioinformatics pipeline, Halo_v1.2. All variants are annotated with reference to the hg19 Genome build. Variants are reported according to HGVS nomenclature and classified into 3 categories: Disease-Associated Variants, Variants of Uncertain Significance, and Benign. Variant allele frequency (VAF) is defined as the number of reads of a variant from the reference sequence divided by the total number of reads at that base.

The Comprehensive Solid Tumor Panel v1 at CHOP includes sequence and copy number analyses of 237 cancer genes, and 586 known fusions and many more novel fusions associated with 106 fusion gene partners. The genes included in the panel can be found at (https://​www.​testmenu.​com/​chop/​Tests/​785967). Fusion genes were evaluated by targeted RNA-seq using anchored multiplex PCR with custom designed primers (ArcherDx, Boulder, CO). Full exonic and select intronic/promotor sequence of 237 cancer genes were evaluated by next generation sequencing. Regions of interest were captured using SureSelect^QTX target enrichment technology (Agilent Technologies, Santa Clara, CA). Sequencing was performed on Illumina MiSeq or HiSeq (San Diego, CA). Sequencing data were processed using the homebrew software ConcordS v1 and NextGENe v2 NGS Analysis Software (Softgenetics, State College, PA). Variant interpretation was performed according to AMP/ASCO/CAP standards and guidelines for somatic variant interpretation and reporting [15].

All tumors with nonsense or frameshift mutations in SETD2 and those with missense mutations with AF greater than 40% were used for immunohistochemical (IHC) studies. In addition, glioblastomas, anaplastic astrocytomas, pilocytic astrocytomas and meningiomas confirmed to be SETD2-wildtype by NGS were used as controls.

H3K36me3 (Abcam ab9050), H3K36ac (Abcam ab177179), and H3K27me3 (Cell Signaling 9733) antibodies were used to stain formalin fixed paraffin embedded slides. Staining was performed on a Bond Max automated staining system (Leica Biosystems). The Bond Refine polymer staining kit (Leica Biosystems) was used. The standard protocol was followed with the exception of the primary antibody incubation which was extended to 1 h at room temperature. The antibodies were used at 1:5 K (H3K36me3), 1:100 (H3K36ac) and 1:150 (H3K36me3) dilutions and antigen retrieval was performed with E1 (H3K36me3 & H3K36ac) or E2 (H3K27me3) (Leica Biosystems) retrieval solution for 20 min. Slides were rinsed, dehydrated through a series of ascending concentrations of ethanol and xylene, then coverslipped.

Immunohistochemistry was scored using the semiquantitative H-score system. H-scores were calculated as 3x the percentage of strongly staining nuclei +2x the percentage of moderately staining nuclei + the percentage of weakly staining nuclei (giving a range of 0 to 300). The H-scores were independently assessed by two neuropathologists board-certified by the American Board of Pathology (MPN and ANV) on de-identified slides.

The Cancer Genome Atlas (TCGA) dataset was retrieved from cbioportal (http://​www.​cbioportal.​org) by searching for SETD2 mutations in “CNS/Brain” tumors (headings: diffuse glioma, glioblastoma, oligodendroglioma, pilocytic astrocytoma and medulloblastoma). The search was performed 11/30/2017.

Statistical analysis was performed using SPSS version 23.0 (IBM Corp.). Statistical significance was defined as p <  .05 and based on two-tailed tests. For the analysis of the number of co-occurring mutations in SETD2-mutant tumors, only data from the CPD were used in calculations.

Immunohistochemistry for H3K36me3, H3K36ac and H3K27me3 expression were assessed with H-scores by two neuropathologists (ANV and MPN) on SETD2-mutant tumors and histologic controls confirmed to be wildtype for SETD2 by NGS. Gliomas with SETD2 mutations showed significantly lower H-scores for H3K36me3 compared to wildtype controls (140.8 ± 65.4 vs. 228.8 ± 29.1, p < 0.01) (Fig. 3). In contrast, statistically significant differences in staining for H3K36ac and H3K27me3 between SETD2 mutants and controls were not observed (H3K36ac: 140.1 ± 35.7 vs. 160.0 ± 41.8, p = 0.13; H3K27me3: 206.1 ± 24.2vs. 190.8 ± 33.5, p = 0.23). There was no correlation between AF and H-score for any of the immunohistochemical markers [H3K36me3: F_1,8 = 0.55, p = .48 with an R² of 0.06 (Fig. 3c); H3K36ac: F_1,8 = 0.54, p = .48 with an R² of 0.06; H3K27me3: F_1,8 = 0.46, p = .53 with an R² of 0.08]. The concordance correlation coefficients for the three antibodies were as follows: H3K36me3 concordance correlation coefficient of 0.88 [95% CI 0.69–0.96]; H3K36ac concordance correlation coefficient of 0.58 (95% CI 0.12–0.83); H3K27me3: concordance correlation coefficient of 0.51 (95% CI 0.16–0.75).

The results shown here are based upon data generated by the TCGA Research Network: http://​cancergenome.​nih.​gov/​, via http://​www.​cbioportal.​org/​ [4, 7]. A total of 22 CNS tumors with SETD2 mutations were identified across the cohorts included in the TCGA datasets, with 0–14% of CNS tumors harboring a SETD2 mutation depending on the cohort (Fig. 4). Eleven tumors had truncating mutations, ten had missense mutations and one had a splice-site mutation. The age of the patients ranged from 2 to 74 years (mean 40.1 ± 23.6 years) with a male to female ratio of 2.3:1. There was no statistically significant difference (p = 0.22) in age between patients with truncating mutations and those with missense mutations. SETD2 mutations were found in high grade gliomas (n = 14, 63%), low grade gliomas (n = 3, 14%), and medulloblastomas (n = 5, 23%). The low grade gliomas included two pilocytic astrocytomas and an IDH-mutant, 1p/19q-codeleted, WHO grade II oligodendroglioma. Data on the location of the tumors is limited; a study of glioblastomas found that all tumors with SETD2 mutations were located in the cerebral hemispheres [6]. However, it is likely SETD2 mutant tumors were also present in the posterior fossa as mutations were seen in 5 medulloblastomas and 2 pilocytic astrocytomas, tumors which both have a strong association with the posterior fossa. In total, 26 SETD2 mutations were seen among the 22 tumors with one medulloblastoma having 3 SETD2 missense mutations. For the 11 tumors for which data on AF was available, the frequency ranged from 5 to 48%. No statistically significant difference in AF was seen between truncating mutations and missense mutations (p = 0.82). The mutations were distributed throughout SETD2 (Fig. 2 aii). Survival data is available on 16 patients (15 patients with gliomas and 1 patient with medulloblastoma). The average follow-up was 19.1 ± 17.3 months (range 5 to 72 months) for all tumors and 15.8 ± 11.4 months (range 5 to 45 months) for patients with high grade gliomas. Twelve patients were still living. High grade gliomas with TM had an average follow-up of 13.2 ± 10.8 months and those with MM had an average follow-up of 17.7 ± 12.3 months (p = .52). Four deceased patients all had high grade gliomas (two of which were recurrent) with an average survival of 16.3 ± 10.0 months (range 7 to 30 months). Two of the deceased patients had TM (survival 7 months and 30 months) and two patients had MM (survivals of 11 and 17 months).