Sequential filtering for clinically relevant variants as a method for clinical interpretation of whole exome sequencing findings in glioma

dc.contributor.authorUlgen, Ege
dc.contributor.authorCan, Ozge
dc.contributor.authorBilguvar, Kaya
dc.contributor.authorBoylu, Cemaliye Akyerli
dc.contributor.authorYuksel, Sirin Kilicturgay
dc.contributor.authorDanyeli, Ayca Ersen
dc.contributor.authorSezerman, O. Ugur
dc.contributor.authorYakicier, M. Cengiz
dc.contributor.authorPamir, M. Necmettin
dc.contributor.authorOzduman, Koray
dc.date.accessioned2023-02-21T12:35:06Z
dc.date.available2023-02-21T12:35:06Z
dc.date.issued2021-01-01
dc.description.abstractBackground In the clinical setting, workflows for analyzing individual genomics data should be both comprehensive and convenient for clinical interpretation. In an effort for comprehensiveness and practicality, we attempted to create a clinical individual whole exome sequencing (WES) analysis workflow, allowing identification of genomic alterations and presentation of neurooncologically-relevant findings. Methods The analysis workflow detects germline and somatic variants and presents: (1) germline variants, (2) somatic short variants, (3) tumor mutational burden (TMB), (4) microsatellite instability (MSI), (5) somatic copy number alterations (SCNA), (6) SCNA burden, (7) loss of heterozygosity, (8) genes with double-hit, (9) mutational signatures, and (10) pathway enrichment analyses. Using the workflow, 58 WES analyses from matched blood and tumor samples of 52 patients were analyzed: 47 primary and 11 recurrent diffuse gliomas. Results The median mean read depths were 199.88 for tumor and 110.955 for normal samples. For germline variants, a median of 22 (14-33) variants per patient was reported. There was a median of 6 (0-590) reported somatic short variants per tumor. A median of 19 (0-94) broad SCNAs and a median of 6 (0-12) gene-level SCNAs were reported per tumor. The gene with the most frequent somatic short variants was TP53 (41.38\%). The most frequent chromosome-/arm-level SCNA events were chr7 amplification, chr22q loss, and chr10 loss. TMB in primary gliomas were significantly lower than in recurrent tumors (p = 0.002). MSI incidence was low (6.9\%). Conclusions We demonstrate that WES can be practically and efficiently utilized for clinical analysis of individual brain tumors. The results display that NOTATES produces clinically relevant results in a concise but exhaustive manner.
dc.description.issue1
dc.description.issueFEB 23
dc.description.volume14
dc.identifier.doi10.1186/s12920-021-00904-3
dc.identifier.urihttps://hdl.handle.net/11443/1871
dc.identifier.urihttp://dx.doi.org/10.1186/s12920-021-00904-3
dc.identifier.wosWOS:000623213600003
dc.publisherBMC
dc.relation.ispartofBMC MEDICAL GENOMICS
dc.subjectWhole exome sequencing
dc.subjectNGS
dc.subjectGlioma
dc.subjectBrain tumor
dc.subjectClinical analysis
dc.titleSequential filtering for clinically relevant variants as a method for clinical interpretation of whole exome sequencing findings in glioma
dc.typeArticle

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