The potential of combined mutation sequencing of plasma circulating cell‐free DNA and matched white blood cells for treatment response prediction

Leest, Paul van der; Schuuring, Ed

doi:10.1002/1878-0261.12646

Cited by 11 publications

(5 citation statements)

References 18 publications

(27 reference statements)

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“…Longitudinal monitoring of a single tumor‐derived variant beyond the currently proposed interval might assist in early detection of disease progression and its clinical applicability, probably in combination with multiple available biomarkers, should be investigated in future (prospective) studies. Besides, as ccfDNA is shed into circulation from various tissues, DNA fragments from hematopoietic and germline origin are prone to affect analytical results with NGS, as well as inconsistent preanalytical handling and sample processing [ 23 , 49 , 50 , 51 ]. Although the majority of clonal hematopoietic variants occur in nontargetable genes, these variants are also identified in targetable genes such as KRAS , BRAF , and PIK3CA as well [ 16 ].…”

Section: Discussionmentioning

confidence: 99%

“…Deep sequencing of plasma may therefore identify more mutations, but these might not all be derived from the tumor. To this extent, parallel sequencing of a patient‐matched bloodborne reference material, for example, white blood cells, is of importance [ 50 ], further increasing the costs for routine clinical practice. Therefore, monitoring ctDNA with a ddPCR assay is as sensitive as NGS to monitor therapy response but in a cost‐effective manner.…”

Section: Discussionmentioning

confidence: 99%

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Circulating tumor DNA as a biomarker for monitoring early treatment responses of patients with advanced lung adenocarcinoma receiving immune checkpoint inhibitors

et al. 2021

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Section: Discussionmentioning

confidence: 99%

Section: Discussionmentioning

confidence: 99%

Circulating tumor DNA as a biomarker for monitoring early treatment responses of patients with advanced lung adenocarcinoma receiving immune checkpoint inhibitors

et al. 2021

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“…This makes it possible to encounter genomic alterations in cfDNA but not in tissue DNA. Those unique plasma variations were thought to be entirely because of tumor heterogeneity and clonal evolution, but recent reports have added clarification to the complex picture: such events might reflect clonal hematopoiesis [25] or simply are reported because of technical errors [26]. By analyzing replicate sets of tissue‐plasma samples through four NGS‐based plasma assays, Stetson et al documented variability among results from the four plasma NGS vendors revealing technical errors or differences in sensitivities as potential causes of discrepant alterations between the plasma NGS vendors [26].…”

Section: Discussionmentioning

confidence: 99%

Validation of a Circulating Tumor DNA-Based Next-Generation Sequencing Assay in a Cohort of Patients with Solid tumors: A Proposed Solution for Decentralized Plasma Testing

et al. 2021

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Characterization of circulating tumor DNA (ctDNA) has been integrated into clinical practice. While labs have standardized validation procedures to develop single locus tests, the efficacy of on-site plasma-based next-generation sequencing (NGS) assays still need to be proven. In this retrospective study, we profiled DNA from matched tissue and plasma samples from 75 cancer patients. We applied the NGS test PGDx elio™ plasma resolve-RUO (EPR), which detects clinically relevant alterations in 33 genes and microsatellite instability (MSI), to analyze plasma cell-free DNA (cfDNA). The concordance between alterations detected in both tissue and plasma samples was higher in patients with metastatic disease. EPR detected 77% of sequence alterations, amplifications, and fusions that were found in metastatic samples compared to 45% of those alterations found in the primary tumor samples (P = 0.00005). There was

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“…Furthermore, total ccfDNA concentrations can be influenced dramatically not only by technical factors such as hemolysis, but also by unrelated factors such as exercise and inflammation [32,33]. Finally, post-analytical determinants such as detection methods that differ in, e.g., sensitivity, complexity, and mutation coverage may also affect the clinical outcome [17,27,34,35].…”

Section: Discussionmentioning

confidence: 99%

Comparison of Circulating Cell-Free DNA Extraction Methods for Downstream Analysis in Cancer Patients

Leest

Boonstra

Elst

et al. 2020

Cancers

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Circulating cell-free DNA (ccfDNA) may contain DNA originating from the tumor in plasma of cancer patients (ctDNA) and enables noninvasive cancer diagnosis, treatment predictive testing, and response monitoring. A recent multicenter evaluation of workflows by the CANCER-ID consortium using artificial spiked-in plasma showed significant differences and consequently the importance of carefully selecting ccfDNA extraction methods. Here, the quantity and integrity of extracted ccfDNA from the plasma of cancer patients were assessed. Twenty-one cancer patient-derived cell-free plasma samples were selected to compare the Qiagen CNA, Maxwell RSC ccfDNA plasma, and Zymo manual quick ccfDNA kit. High-volume citrate plasma samples collected by diagnostic leukapheresis from six cancer patients were used to compare the Qiagen CNA (2 mL) and QIAamp MinElute ccfDNA kit (8 mL). This study revealed similar integrity and similar levels of amplified short-sized fragments and tumor-specific mutants comparing the CNA and RSC kits. However, the CNA kit consistently showed the highest yield of ccfDNA and short-sized fragments, while the RSC and ME kits showed higher variant allelic frequencies (VAFs). Our study pinpoints the importance of standardizing preanalytical conditions as well as consensus on defining the input of ccfDNA to accurately detect ctDNA and be able to compare results in a clinical routine practice, within and between clinical studies.

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The potential of combined mutation sequencing of plasma circulating cell‐free DNA and matched white blood cells for treatment response prediction

Cited by 11 publications

References 18 publications

Circulating tumor DNA as a biomarker for monitoring early treatment responses of patients with advanced lung adenocarcinoma receiving immune checkpoint inhibitors

Circulating tumor DNA as a biomarker for monitoring early treatment responses of patients with advanced lung adenocarcinoma receiving immune checkpoint inhibitors

Validation of a Circulating Tumor DNA-Based Next-Generation Sequencing Assay in a Cohort of Patients with Solid tumors: A Proposed Solution for Decentralized Plasma Testing

Comparison of Circulating Cell-Free DNA Extraction Methods for Downstream Analysis in Cancer Patients

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