2018
DOI: 10.18632/oncotarget.24950
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Cross-platform comparison for the detection of RAS mutations in cfDNA (ddPCR Biorad detection assay, BEAMing assay, and NGS strategy)

Abstract: CfDNA samples from colon (mCRC) and non-small cell lung cancers (NSCLC) (CIRCAN cohort) were compared using three platforms: droplet digital PCR (ddPCR, Biorad); BEAMing/OncoBEAM™-RAS-CRC (Sysmex Inostics); next-generation sequencing (NGS, Illumina), utilizing the 56G oncology panel (Swift Biosciences). Tissue biopsy and time matched cfDNA samples were collected at diagnosis in the mCRC cohort and during 1st progression in the NSCLC cohort. Excellent matches between cfDNA/FFPE mutation profiles were observed. … Show more

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Cited by 47 publications
(72 citation statements)
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“…This sample and three other samples only showed mutations in loci not covered by the KRAS Screening Multiplex Kit used for ddPCR ( KRAS codon 61, BRAF and TP53 ). Nonetheless, we observed good agreement between ddPCR and NGS, which was also reported in other studies …”
Section: Discussionsupporting
confidence: 91%
“…This sample and three other samples only showed mutations in loci not covered by the KRAS Screening Multiplex Kit used for ddPCR ( KRAS codon 61, BRAF and TP53 ). Nonetheless, we observed good agreement between ddPCR and NGS, which was also reported in other studies …”
Section: Discussionsupporting
confidence: 91%
“…All experiments were conducted at the Lyon Universitary Hospital. Briefly, as described previously, the cfDNA sample was diluted in 123 µL of AVE buffer (Qiagen). A PCR Master Mix, specifically targeting p.T790M was mixed with the cfDNA samples and split into six replicate of 65 µL reactions in the initial target‐specific spanning PCR.…”
Section: Methodsmentioning
confidence: 99%
“…After breaking the emulsion PCR reaction, WT and mutant‐specific probes were hybridized and flow cytometry analysis was conducted using a cytometer (BD Bioscience, Erembodegem, Belgium). The threshold of positivity is defined by two parameters: the MAF had to exceed 0.02% and the absolute number of mutant beads had to be greater than 50 . All samples with lower mutated bead counts were considered negative, even if the MAF exceeded 0.02%, this is most likely due to a low cfDNA input amount, typically below 2 ng.…”
Section: Methodsmentioning
confidence: 99%
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