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Please use this identifier to cite or link to this item: https://swslhd.intersearch.com.au/swslhdjspui/handle/1/12347
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dc.contributor.authorNindra, U.-
dc.contributor.authorPal, A.-
dc.contributor.authorLea, V.-
dc.contributor.authorLim, S. H. S.-
dc.contributor.authorWilkinson, K.-
dc.contributor.authorAsghari, R.-
dc.contributor.authorRoberts, T. L.-
dc.contributor.authorBecker, T. M.-
dc.contributor.authorFarzin, M.-
dc.contributor.authorRutland, T.-
dc.contributor.authorLee, M.-
dc.contributor.authorMacKenzie, S.-
dc.contributor.authorNg, W.-
dc.contributor.authorWang, B.-
dc.contributor.authorSoon Lee, C.-
dc.contributor.authorChua, W.-
dc.date.accessioned2023-12-04T22:59:56Z-
dc.date.available2023-12-04T22:59:56Z-
dc.date.issued2023-
dc.identifier.issn19326203 (ISSN)-
dc.identifier.urihttps://swslhd.intersearch.com.au/swslhdjspui/handle/1/12347-
dc.description.abstractBackground Next generation sequencing (NGS) is increasingly used in standard clinical practice to identify patients with potentially actionable mutations. Stratification of NGS mutation tiers is currently based on the European Society of Medical Oncology (ESMO) Scale for Clinical Actionability of Molecular Targets (ESCAT[E]) Tier I?V & X. Allele frequency is also increasingly recognised as an important prognostic tool in advanced cancer. The aim of this study was to determine the genomic mutations in metastatic colorectal cancer (CRC) in an Australian multicultural population and their influence on survival outcomes. Methods Next generation sequencing with the 50-gene panel Oncomine Precision Assay? was used on 180 CRC tissue samples obtained across six Sydney hospitals between June 2021 and March 2022. Results From 180 samples, 147 (82%) had at least one gene mutation identified with 68 (38%) having two or more concurrent mutations. Tier I variants included RAS wild-type [EI] in 73 (41%) and BRAF V600E [EIA] in 27 (15%). Non-tier I variants include 2 (1%) ERBB2 amplification [EIIB], 26 (15%) PIK3CA hotspot mutations [EIIIA] and 9 (5%) MET focal amplifications [EIIIA]. NGS testing revealed an additional 22% of cases with Tier II & III mutations. 43% of patients also presented with potentially actionable Tier III & IV mutations. Patients with concurrent TP53 and RAS mutations had significantly reduced overall survival (6.1 months versus 21.1 months, p <0.01). High KRAS allele frequency, as defined by those with over 20% variant allele frequency (VAF), also demonstrated reduced overall survival (12.1 months versus 42.9 months, p = 0.04). Conclusions In addition to identifying patients with genomic alterations suitable for clinically proven standard of care therapeutic options, the 50 gene NGS panel has significant potential in identifying potentially actionable non-tier 1 mutations and therefore may become future standard clinical practice. Copyright: ? 2023 Nindra et al. This is an open access article distributed under the terms of the Creative Commons Attribution License, which permits unrestricted use, distribution, and reproduction in any medium, provided the original author and source are credited.-
dc.publisherPublic Library of Science-
dc.subjectAustralia Colonic Neoplasms Colorectal Neoplasms High-Throughput Nucleotide Sequencing Humans Mutation Rectal Neoplasms B Raf kinase epidermal growth factor receptor 2 K ras protein protein kinase B protein p53 adult aged allele Article Australian bioinformatics cancer survival clinical practice cohort analysis colorectal cancer copy number variation demographics DNA repair female gene gene amplification gene frequency gene mutation gene sequence genomic mutation high throughput sequencing human human tissue major clinical study male metastatic colorectal cancer mismatch repair observational study overall survival PIK3CA gene progression free survival retrospective study colon tumor colorectal tumor pathology rectum tumor-
dc.titleMultigene panel next generation sequencing in metastatic colorectal cancer in an Australian population-
dc.typeJournal Article-
dc.contributor.swslhdauthorNindra, Udit-
dc.contributor.swslhdauthorPal, Abhijit-
dc.contributor.swslhdauthorWilkinson, Kate-
dc.contributor.swslhdauthorFarzin, Mahtab-
dc.contributor.swslhdauthorRutland, Tristan-
dc.contributor.swslhdauthorNg, Weng-
dc.contributor.swslhdauthorWang, Bin-
dc.contributor.swslhdauthorLee, Cheok S.-
dc.contributor.swslhdauthorChua, Wei-
dc.contributor.swslhdauthorLea, Vivienne-
dc.contributor.swslhdauthorLim, Stephanie H.-
dc.description.affiliatesDepartment of Medical Oncology, Liverpool Hospital, Liverpool, NSW, Australia Department of Medical Oncology, Macarthur Cancer Therapy Centre, Campbelltown Hospital, Campbelltown, NSW, Australia Department of Medical Oncology, Bankstown-Lidcombe Hospital, Bankstown, NSW, Australia Ingham Institute for Applied Medical Research, Liverpool, Australia School of Medicine, Western Sydney University, Sydney, Australia Department of Anatomical Pathology, Liverpool Hospital, Liverpool, Sydney, Australia South Western Clinical School, University of New South Wales, Sydney, Australia-
dc.identifier.doi10.1371/journal.pone.0292087-
dc.identifier.departmentLiverpool Hospital, Department of Medical Oncology-
dc.identifier.departmentLiverpool Hospital, Department of Anatomical Pathology-
dc.identifier.departmentCampbelltown Hospital, Macarthur Cancer Therapy Centre-
dc.identifier.departmentCampbelltown Hospital, Department of Medical Oncology-
dc.type.studyortrialArticle-
dc.identifier.journaltitlePLoS ONE-
Appears in Collections:Bankstown-Lidcombe Hospital
Camden and Campbelltown Hospitals
Liverpool Hospital

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