2017
DOI: 10.1186/s12885-017-3424-0
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Droplet digital PCR for detection and quantification of circulating tumor DNA in plasma of head and neck cancer patients

Abstract: BackgroundDuring posttreatment surveillance of head and neck cancer patients, imaging is insufficiently accurate for the early detection of relapsing disease. Free circulating tumor DNA (ctDNA) may serve as a novel biomarker for monitoring tumor burden during posttreatment surveillance of these patients. In this exploratory study, we investigated whether low level ctDNA in plasma of head and neck cancer patients can be detected using Droplet Digital PCR (ddPCR).Methods TP53 mutations were determined in surgica… Show more

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Cited by 99 publications
(89 citation statements)
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References 48 publications
(38 reference statements)
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“…Here, sampling error may play a role since mutated cfDNA molecules might not be present in each replicate . Therefore, samples should always be analyzed in triplicates if low allele frequencies are expected …”
Section: Different Methods For Mutation Detection In Routine Diagnosticsmentioning
confidence: 99%
“…Here, sampling error may play a role since mutated cfDNA molecules might not be present in each replicate . Therefore, samples should always be analyzed in triplicates if low allele frequencies are expected …”
Section: Different Methods For Mutation Detection In Routine Diagnosticsmentioning
confidence: 99%
“…Analysis of ctDNA consists of quantitative and qualitative studies. Quantitative analysis of ctDNA using ddPCR assays is performed on the basis of the correlation between disease stage and ctDNA:cfDNA concentration ratio . On the other hand, qualitative studies use NGS to examine ctDNA for variations in cancer hotspots or the entire genome to examine early‐stage disease, response to treatment and prognosis .…”
Section: Liquid Biopsy Componentsmentioning
confidence: 99%
“…Recently, the ddPCR assay has been widely used to detect genetic and epigenetic alterations . ddPCR can detect very rare sequences with high precision and sensitivity by partitioning individual target molecules within distinct compartments and, therefore, reduces the limitations of conventional methods such as classic real‐time quantitative PCR (qPCR) or the amplification refractory mutation system qPCR (ARMS qPCR) .…”
Section: Discussionmentioning
confidence: 99%
“…Although the sensitivity of NGS is superior to that of direct Recently, the ddPCR assay has been widely used to detect genetic and epigenetic alterations. [18][19][20][21] ddPCR can detect very rare sequences with high precision and sensitivity by partitioning individual target molecules within distinct compartments and, therefore, reduces the limitations of conventional methods such as classic real-time quantitative PCR (qPCR) or the amplification refractory mutation system qPCR (ARMS qPCR). [22][23][24] However, the PNA-LNA clamp method is a molecular probe-based PCR method; its unique design and allele-specific approach allow exceptionally high specificity and sensitivity.…”
Section: Discussionmentioning
confidence: 99%