Your search keyword '"ddpcr"' showing total 8 results

1. Evaluation of commercial kits for isolation and bisulfite conversion of circulating cell-free tumor DNA from blood.

Author

Kresse, Stine H., Brandt-Winge, Sara, Pharo, Heidi, Flatin, Bjørnar T. B., Jeanmougin, Marine, Vedeld, Hege Marie, and Lind, Guro E.

Subjects

*CIRCULATING tumor DNA, *DNA analysis, *CELL-free DNA, *DNA methylation, *NUCLEIC acids, *COLORECTAL cancer, *IRINOTECAN

Abstract

Background: DNA methylation biomarkers in circulating cell-free DNA (cfDNA) have great clinical potential for cancer management. Most methods for DNA methylation analysis require bisulfite conversion, causing DNA degradation and loss. This is particularly challenging for cfDNA, which is naturally fragmented and normally present in low amounts. The aim of the present study was to identify an optimal combination of cfDNA isolation and bisulfite conversion kits for downstream analysis of DNA methylation biomarkers in plasma. Results: Of the five tested bisulfite conversion kits (EpiJET Bisulfite Conversion Kit, EpiTect Plus DNA Bisulfite Kit (EpiTect), EZ DNA Methylation-Direct Kit, Imprint DNA Modification Kit (Imprint) and Premium Bisulfite Kit), the highest and lowest DNA yield and recovery were achieved using the EpiTect kit and the Imprint kit, respectively, with more than double the amount of DNA for the EpiTect kit. Of the three tested cfDNA isolation kits (Maxwell RSC ccfDNA Plasma Kit, QIAamp Circulating Nucleic Acid Kit (CNA) and QIAamp MinElute ccfDNA Mini Kit), the CNA kit yielded around twice as much cfDNA compared to the two others kits, although with more high molecular weight DNA present. When comparing various combinations of cfDNA isolation kits and bisulfite conversion kits, the CNA kit and the EpiTect kit were identified as the best-performing combination, resulting in the highest yield of bisulfite converted cfDNA from normal plasma, as measured by droplet digital PCR (ddPCR). As a proof of principle, this kit combination was used to process plasma samples from 13 colorectal cancer patients for subsequent ddPCR methylation analysis of BCAT1 and IKZF1. Methylation of BCAT1 and/or IKZF1 was identified in 6/10 (60%) stage IV patients and 1/3 (33%) stage III patients. Conclusions: Based on a thorough evaluation of five bisulfite conversion kits and three cfDNA isolation kits, both individually and in combination, the CNA kit and the EpiTect kit were identified as the best-performing kit combination, with highest DNA yield and recovery across a range of DNA input amounts. The combination was successfully used for detection of clinically relevant DNA methylation biomarkers in plasma from cancer patients. [ABSTRACT FROM AUTHOR]

Published

2023

2. Circulating NPTX2 methylation as a non-invasive biomarker for prognosis and monitoring of metastatic pancreatic cancer.

Author

García-Ortiz, María Victoria, Cano-Ramírez, Pablo, Toledano-Fonseca, Marta, Cano, María Teresa, Inga-Saavedra, Elizabeth, Rodríguez-Alonso, Rosa María, Guil-Luna, Silvia, Gómez-España, María Auxiliadora, Rodríguez-Ariza, Antonio, and Aranda, Enrique

Subjects

*PANCREATIC cancer, *METASTASIS, *METHYLATION, *PROGNOSIS, *PANCREATIC duct, *PROGRESSION-free survival

Abstract

Background: Pancreatic cancer is the most lethal cancer with a dismal prognosis mainly due to diagnosis at advanced stage and ineffective treatments. CA19-9 levels and computed tomography (CT) imaging are the main standard criteria for evaluating disease progression and treatment response. In this study we explored liquid biopsy-based epigenetic biomarkers for prognosis and monitoring disease in patients with metastatic pancreatic ductal adenocarcinoma (mPDAC). Methods: Plasma samples were collected from 44 mPDAC patients at the time of diagnosis, and in 15 of them, additional samples were obtained during follow-up of the disease. After cell-free DNA (cfDNA), isolation circulating levels of methylated NPTX2, SPARC, BMP3, SFRP1 and TFPI2 genes were measured using digital droplet PCR (ddPCR). BEAMing technique was performed for quantitation of RAS mutations in cfDNA, and CA19-9 was measured using standard techniques. Results: NPTX2 was the most highly and frequently methylated gene in cfDNA samples from mPDAC patients. Higher circulating NPTX2 methylation levels at diagnosis were associated with poor prognosis and efficiently stratified patients for prediction of overall survival (6.06% cut-off, p = 0.0067). Dynamics of circulating NPTX2 methylation levels correlated with disease progression and response to therapy and predicted better than CA19-9 the evolution of disease in mPDAC patients. Remarkably, in many cases the disease progression detected by CT scan was anticipated by an increase in circulating NPTX2 methylation levels. Conclusions: Our study supports circulating NPTX2 methylation levels as a promising liquid biopsy-based clinical tool for non-invasive prognosis, monitoring disease evolution and response to treatment in mPDAC patients. [ABSTRACT FROM AUTHOR]

Published

2023

3. Translation of a tissue epigenetic signature to circulating free DNA suggests BCAT1 as a potential noninvasive diagnostic biomarker for lung cancer.

Author

Palanca-Ballester, Cora, Hervas, David, Villalba, Maria, Valdes-Sanchez, Teresa, Garcia, Diana, Alcoriza-Balaguer, Maria Isabel, Benet, Marta, Martinez-Tomas, Raquel, Briones-Gomez, Andres, Galbis-Caravajal, Jose, Calvo, Alfonso, Juan, Oscar, Lahoz, Agustin, Cases, Enrique, and Sandoval, Juan

Subjects

*CIRCULATING tumor DNA, *CELL-free DNA, *LUNG cancer, *DNA methylation, *EPIGENETICS, *CONFOUNDING variables

Abstract

Lung cancer patients are diagnosed at late stages when curative treatments are no longer possible; thus, molecular biomarkers for noninvasive detection are urgently needed. In this sense, we previously identified and validated an epigenetic 4-gene signature that yielded a high diagnostic performance in tissue and invasive pulmonary fluids. We analyzed DNA methylation levels using the ultrasensitive digital droplet PCR in noninvasive samples in a cohort of 83 patients. We demonstrated that BCAT1 is the candidate that achieves high diagnostic efficacy in circulating DNA derived from plasma (area under the curve: 0.85). Impact of potentially confounding variables was also explored. [ABSTRACT FROM AUTHOR]

Published

2022

4. An epigenetic classifier for early stage lung cancer

Author

Yun Su, Hong Bin Fang, and Feng Jiang

Subjects

ddPCR, DNA methylation, Sputum, Diagnosis, Lung cancer, Medicine, Genetics, QH426-470

Abstract

Abstract Background Methylated genes detected in sputum are promise biomarkers for lung cancer. Yet the current PCR technologies for quantification of DNA methylation and diagnostic value of the sputum biomarkers are not sufficient to be used for lung cancer early detection. The emerging droplet digital PCR (ddPCR) is a straightforward means for precise, direct, and absolute quantification of nucleic acids. Here, we investigate whether ddPCR can sensitively and robustly quantify DNA methylation in sputum for more precise diagnosis of lung cancer. Results First, the analytic performance of methylation-specific ddPCR (ddMSP) and quantitative methylation-specific PCR (qMSP) is determined in methylated and unmethylated DNA samples. Second, 29 genes, previously proposed as potential sputum biomarkers for lung cancer, are analyzed by using ddMSP in a training set of 127 lung cancer patients and 159 controls. ddMSP has higher sensitivity, precision, and reproducibility for quantification of methylation compared with qMSP (all p 0.05). The classifier has higher accuracy compared with sputum cytology (88.8 vs. 70.6%, p

Published

2018

5. Refinement of cg05575921 demethylation response in nascent smoking.

Author

Dawes, Kelsey, Andersen, Allan, Papworth, Emma, Hundley, Brandon, Hutchens, Natasha, El Manawy, Heba, Becker, Ashley, Sampson, Luke, Philibert, Willem, Gibbons, Frederick X., Gerrard, Meg, and Philibert, Robert

Subjects

*DEMETHYLATION, *ADOLESCENT smoking, *SMOKING, *COTININE, *HIGH school students, *CARBON monoxide

Abstract

The initiation of adolescent smoking is difficult to detect using carbon monoxide or cotinine assays. Previously, we and others have shown that the methylation of cg05575921 is an accurate predictor of adult smoking status. But the dose and time dependency of the demethylation response to smoking initiation in adolescents is not yet well understood. To this end, we conducted three consecutive annual in-person interviews and biological samplings of 448 high school students (wave 1 (W1)-wave 3 (W3)). At W1 (n = 448), 62 subjects reported using tobacco and 72 subjects reported using cannabis at least once in their life-time with 38 and 20 subjects having a positive cotinine and cannabinoid levels, respectively, at W1 intake. At W3 (n = 383), 67 subjects reported using tobacco and 60 subjects reported using cannabis at least once with 75 and 60 subjects having positive cotinine and cannabinoid levels, respectively, at W3. Subjects with undetectable cotinine levels at all three-time waves had stable levels of cg05575921 methylation throughout the study (88.7% at W1 and 88.8% at W3, n = 149), while subjects with positive cotinine levels at all 3 time points manifested a steady decrease in cg05575921 methylation (81.8% at W1 and 71.3% at the W3, n = 12). In those subjects with an affirmative smoking self-report at W3 (n = 17), the amount of demethylation at cg05575921 was correlated with time and intensity of smoking. We conclude that cg05575921 methylation is a sensitive, dose-dependent indicator of early stages of smoking, and may help to identify smokers in the early stages of smoking. [ABSTRACT FROM AUTHOR]

Published

2020

6. Refinement of cg05575921 demethylation response in nascent smoking

Author

Luke Sampson, Willem Philibert, Brandon Hundley, Frederick X. Gibbons, Meg Gerrard, Allan M. Andersen, Robert A. Philibert, Natasha Hutchens, Ashley Becker, Heba El Manawy, Emma Papworth, and Kelsey Dawes

Subjects

0301 basic medicine, Epigenomics, Male, Adolescent, medicine.medical_treatment, Physiology, ddPCR, Interviews as Topic, 03 medical and health sciences, chemistry.chemical_compound, 0302 clinical medicine, Genetics, medicine, Basic Helix-Loop-Helix Transcription Factors, Humans, 030212 general & internal medicine, Longitudinal Studies, Cotinine, Molecular Biology, Genetics (clinical), Demethylation, Carbon Monoxide, DNA methylation, biology, business.industry, Cannabinoids, Research, Smoking, cg05575921, Methylation, biology.organism_classification, Repressor Proteins, Smoking initiation, 030104 developmental biology, chemistry, Case-Control Studies, Smoking status, Female, Cannabinoid, Cannabis, Self Report, business, Developmental Biology

Abstract

The initiation of adolescent smoking is difficult to detect using carbon monoxide or cotinine assays. Previously, we and others have shown that the methylation of cg05575921 is an accurate predictor of adult smoking status. But the dose and time dependency of the demethylation response to smoking initiation in adolescents is not yet well understood. To this end, we conducted three consecutive annual in-person interviews and biological samplings of 448 high school students (wave 1 (W1)-wave 3 (W3)). At W1 (n = 448), 62 subjects reported using tobacco and 72 subjects reported using cannabis at least once in their life-time with 38 and 20 subjects having a positive cotinine and cannabinoid levels, respectively, at W1 intake. At W3 (n = 383), 67 subjects reported using tobacco and 60 subjects reported using cannabis at least once with 75 and 60 subjects having positive cotinine and cannabinoid levels, respectively, at W3. Subjects with undetectable cotinine levels at all three-time waves had stable levels of cg05575921 methylation throughout the study (88.7% at W1 and 88.8% at W3, n = 149), while subjects with positive cotinine levels at all 3 time points manifested a steady decrease in cg05575921 methylation (81.8% at W1 and 71.3% at the W3, n = 12). In those subjects with an affirmative smoking self-report at W3 (n = 17), the amount of demethylation at cg05575921 was correlated with time and intensity of smoking. We conclude that cg05575921 methylation is a sensitive, dose-dependent indicator of early stages of smoking, and may help to identify smokers in the early stages of smoking.

Published

2020

7. An epigenetic classifier for early stage lung cancer

Author

Su, Yun, Fang, Hong Bin, and Jiang, Feng

Published

2018

8. An epigenetic classifier for early stage lung cancer

Author

Feng Jiang, Yun Su, and Hong-Bin Fang

Subjects

0301 basic medicine, Oncology, Male, medicine.medical_specialty, Sputum Cytology, Lung Neoplasms, lcsh:QH426-470, lcsh:Medicine, ddPCR, Polymerase Chain Reaction, Sensitivity and Specificity, Epigenesis, Genetic, 03 medical and health sciences, 0302 clinical medicine, Internal medicine, Diagnosis, Genetics, medicine, Biomarkers, Tumor, Humans, Digital polymerase chain reaction, Epigenetics, Lung cancer, Molecular Biology, Genetics (clinical), Early Detection of Cancer, Aged, Neoplasm Staging, DNA methylation, business.industry, Research, lcsh:R, Sputum, Methylation, Middle Aged, medicine.disease, Human genetics, respiratory tract diseases, lcsh:Genetics, 030104 developmental biology, 030220 oncology & carcinogenesis, Female, medicine.symptom, business, Developmental Biology

Abstract

Background Methylated genes detected in sputum are promise biomarkers for lung cancer. Yet the current PCR technologies for quantification of DNA methylation and diagnostic value of the sputum biomarkers are not sufficient to be used for lung cancer early detection. The emerging droplet digital PCR (ddPCR) is a straightforward means for precise, direct, and absolute quantification of nucleic acids. Here, we investigate whether ddPCR can sensitively and robustly quantify DNA methylation in sputum for more precise diagnosis of lung cancer. Results First, the analytic performance of methylation-specific ddPCR (ddMSP) and quantitative methylation-specific PCR (qMSP) is determined in methylated and unmethylated DNA samples. Second, 29 genes, previously proposed as potential sputum biomarkers for lung cancer, are analyzed by using ddMSP in a training set of 127 lung cancer patients and 159 controls. ddMSP has higher sensitivity, precision, and reproducibility for quantification of methylation compared with qMSP (all p 0.05). The classifier has higher accuracy compared with sputum cytology (88.8 vs. 70.6%, p

Published

2018