Fibroblast growth factor receptor 3 (FGFR3) aberrations in muscle-invasive urothelial carcinoma

This study is a part of the Samsung Medical Center (SMC) Oncology Biomarker study (ClinicalTrials.​gov identifier: NCT01831609). Tumor samples were collected from 74 consecutive patients with UC who underwent radical cystectomy or nephroureterectomy between 2012 and 2014, and had adequate specimen for molecular analysis. All patients provided written informed consent for the use of tumor tissues as well as their clinical data. This study was performed in accordance with the Declaration of Helsinki and approved by the Institutional Review Board of SMC (Seoul, Korea).

Our dedicated genitourinary pathologist (G.Y.K.) reviewed all pathology specimens to ensure the samples contained > 80% tumor cells with < 20% necrosis. Genomic DNA was extracted from the primary tumor tissues using a QIAamp DNA Mini Kit (Qiagen, Valencia, CA, USA). After extraction, we measured concentration as well as 260/280 and 260/230 nm ratio by spectrophotometer (ND1000, Nanodrop Technologies, Thermo-Fisher Scientific, MA, USA). Each sample was then quantified with the Qubit fluorometer (Life technologies, Carlsbad, CA, USA). Genomic DNA with > 10 ng measured by Qubit fluorometer was subjected to library preparation.

We used the Ion Torrent Ampliseq™ cancer panel v2 to detect frequent somatic mutations that were selected based on a literature review. This panel examines 2855 mutations in 50 commonly mutated oncogenes and tumor suppressor genes (Additional file 1: Table S1). We constructed libraries using 10 ng of genomic DNA with the Ion AmpliSeq Library Kit and Ion Xpress Barcodes (Life Technologies). For barcoded library preparations, barcoded adapters from the Ion Xpress Barcode Adapters 1–96 Kit were substituted for the non-barcoded adapter mix in the Ion AmpliSeq Library Kit. Next, the multiplexed barcoded libraries were enriched by clonal amplification using emulsion polymerase chain reaction (PCR) on Ion Sphere Particles (Ion PGMTemplate 200 Kit) and loaded on an Ion 316 Chip. Massively parallel sequencing was carried out on an Ion PGM using the Ion PGM Sequencing 200 Kit v2. The primary filtering process was performed using Torrent Suite v3.6.0 and Ion Torrent Variant Caller v3.6 software. The pipeline included signaling processing, base calling, quality score assignment, adapter trimming, read alignment to 19 human genome references, mapping quality control, coverage analysis, and variant calling. For detection of copy number variations (CNV), nCounter Copy Number Variation CodeSets (NanoString Technologies, Seattle, WA, USA) were used with 300 ng of purified genomic DNA extracted from 2 to 3 sections of 4-μm-thick, formalin-fixed, paraffin-embedded (FFPE) representative tumor blocks using a QIAamp DNA FFPE Tissue Kit (Qiagen, Hilden, Germany). DNA was fragmented via AluI digestion and denatured at 95uC. Fragmented DNA was hybridized with the codeset of 257 genes (Additional file 2: Table S2) in the nCounter Cancer CN Assay Kit (Nanostring Technologies) for 18 h at 65uC and processed according to the manufacturer’s instructions. The nCounter Digital Analyzer counted and tabulated the signals of reporter probes.

We used cutoff values of greater than 6% variant frequency and more than 100X coverage to detect true mutational changes in accordance with previous reports and our own experience. Variant calls were further analyzed using the ANNOVAR, which included variant filtering and annotation using the Catalogue of Somatic Mutations in Cancer (COSMIC, http://​cancer.​sanger.​ac.​uk/​cancergenome/​projects/​cosmic) database, dbSNP build 137, and amino acid change information. Variant calls from Ion AmpliSeq were further evaluated to reduce potential false-positives. Coverage (> 100X) and quality score (> 30) were considered as filtering criteria. For gene expression data from the NanoString nCounter assay, filtering of samples using quality control criteria was performed according to the manufacturer’s recommendations. All statistical analyses were performed by the Biostatistics and Clinical Epidemiology Center at our institute. The R for Windows v2.11.1 software (R Core Team, Vienna, Austria; http://​www.​r-project.​org) was used for analysis of all data. We implemented the method found in the R “compound.Cox” package.