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1. Impact of tumour epithelial subtype on circulating microRNAs in breast cancer patients.

Author

Peadar S Waters, Roisin M Dwyer, Cathy Brougham, Claire L Glynn, Deirdre Wall, Peter Hyland, Maria Duignan, Mark McLoughlin, John Newell, and Michael J Kerin

Subjects
Medicine, Science
Abstract

While a range of miRNAs have been shown to be dysregulated in the circulation of patients with breast cancer, little is known about the relationship between circulating levels and tumour characteristics. The aim of this study was to analyse alterations in circulating miRNA expression during tumour progression in a murine model of breast cancer, and to detemine the clinical relevance of identified miRNAs at both tissue and circulating level in patient samples. Athymic nude mice received a subcutaneous or mammary fat pad injection of MDA-MB-231 cells. Blood sampling was performed at weeks 1, 3 and 6 following tumour induction, and microRNA extracted. MicroRNA microArray analysis was performed comparing samples harvested at week 1 to those collected at week 6 from the same animals. Significantly altered miRNAs were validated across all murine samples by RQ-PCR (n = 45). Three miRNAs of interest were then quantified in the circulation(n = 166) and tissue (n = 100) of breast cancer patients and healthy control individuals. MicroArray-based analysis of murine blood samples revealed levels of 77 circulating microRNAs to be changed during disease progression, with 44 demonstrating changes >2-fold. Validation across all samples revealed miR-138 to be significantly elevated in the circulation of animals during disease development, with miR-191 and miR-106a levels significantly decreased. Analysis of patient tissue and blood samples revealed miR-138 to be significantly up-regulated in the circulation of patients with breast cancer, with no change observed in the tissue setting. While not significantly changed overall in breast cancer patients compared to controls, circulating miR-106a and miR-191 were significantly decreased in patients with basal breast cancer. In tissue, both miRNAs were significantly elevated in breast cancer compared to normal breast tissue. The data demonstrates an impact of tumour epithelial subtype on circulating levels of miRNAs, and highlights divergent miRNA profiles between tissue and blood samples from breast cancer patients.

Published
2014
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3. Bridging Disciplines to Form a New One: The Emergence of Forensic Genetic Genealogy

Author

Claire L, Glynn

Subjects
Forensic Genetics, Genetics, Humans, DNA, United States, Genetics (clinical), Pedigree
Abstract

Forensic Genetic Genealogy (FGG) has fast become a popular tool in criminal investigations since it first emerged in 2018. FGG is a novel investigatory tool that has been applied to hundreds of unresolved cold cases in the United States to generate investigative leads and identify unknown individuals. Consumer DNA testing and the public’s increased curiosity about their own DNA and genetic ancestry, have greatly contributed to the availability of human genetic data. Genetic genealogy has been a field of study/interest for many years as both amateur and professional genetic genealogists use consumer DNA data to explore genetic connections in family trees. FGG encompasses this knowledge by applying advanced sequencing technologies to forensic DNA evidence samples and by performing genetic genealogy methods and genealogical research, to produce possible identities of unknown perpetrators of violent crimes and unidentified human remains. This combination of forensic genetics, genetic genealogy, and genealogical research has formed a new subdiscipline within the forensic sciences. This paper will summarize the individual disciplines that led to the emergence of FGG, its practice in forensic investigations, and current/future considerations for its use.

Published
2022

4. Investigating the Potential and Pitfalls of EV-Encapsulated MicroRNAs as Circulating Biomarkers of Breast Cancer

Author

Emma Holian, Adriele Prina-Mello, Emma McDermott, Doireann P. Joyce, Mohamed Elhadi, Erin Naughton, Clodagh P O'Neill, Andrea B. Grealish, Brian M. Moloney, Carmel Malone, Katie E. Gilligan, Ciaran Manus Maguire, Roisin M. Dwyer, Sonja Khan, Claire L. Glynn, Michael J. Kerin, Peter Dockery, Killian P. O’Brien, Ronan Waldron, and Thomas Ritter

Subjects
0301 basic medicine, Quantitative proteomics, Cell, Nanoparticle tracking analysis, Mice, Nude, Breast Neoplasms, exosomes, Article, 03 medical and health sciences, Extracellular Vesicles, 0302 clinical medicine, Breast cancer, breast cancer, Cell Line, Tumor, microRNA, medicine, Biomarkers, Tumor, Animals, Humans, lcsh:QH301-705.5, Mice, Inbred BALB C, Chemistry, General Medicine, medicine.disease, Molecular biology, Microvesicles, Blot, EV characterization, Disease Models, Animal, MicroRNAs, 030104 developmental biology, medicine.anatomical_structure, lcsh:Biology (General), 030220 oncology & carcinogenesis, Case-Control Studies, Biomarker (medicine), biomarker, Female
Abstract

Extracellular vesicles (EVs) shuttle microRNA (miRNA) throughout the circulation and are believed to represent a fingerprint of the releasing cell. We isolated and characterized serum EVs of breast tumour-bearing animals, breast cancer (BC) patients, and healthy controls. EVs were characterized using transmission electron microscopy (TEM), protein quantification, western blotting, and nanoparticle tracking analysis (NTA). Absolute quantitative (AQ)-PCR was employed to analyse EV-miR-451a expression. Isolated EVs had the appropriate morphology and size. Patient sera contained significantly more EVs than did healthy controls. In tumour-bearing animals, a correlation between serum EV number and tumour burden was observed. There was no significant relationship between EV protein yield and EV quantity determined by NTA, highlighting the requirement for direct quantification. Using AQ-PCR to relate miRNA copy number to EV yield, a significant increase in miRNA-451a copies/EV was detected in BC patient sera, suggesting potential as a novel biomarker of breast cancer.

Published
2020

5. Potential applications of microRNA profiling to forensic investigations

Author

Claire L. Glynn

Subjects
0303 health sciences, 030302 biochemistry & molecular biology, Forensic Sciences, Review, Biology, Forensic Medicine, Data science, Criminal investigation, Donor age, Forensic science, 03 medical and health sciences, MicroRNAs, Crime scene, Mirna profiling, Forensic Anthropology, Humans, Identification (biology), Microrna profiling, Molecular Biology, 030304 developmental biology
Abstract

Within the forensic science community, there is a continued push to develop novel tools to aid in criminal investigations. microRNA (miRNA) analysis has been the focus of many researcher's attention in the biomedical field since its discovery in 1993; however, the forensic application of miRNA analysis has only been suggested within the last 10 years and has been gaining considerable traction recently. The primary focus of the forensic application of miRNA analysis has been on body fluid identification to provide confirmatory universal analysis of unknown biological stains obtained from crime scenes or evidence items. There are, however, other forensic applications of miRNA profiling that have shown potential, yet are largely understudied, and warrant further investigation such as organ tissue identification, donor age estimation, and more. This review paper aims to evaluate the current literature and future potential of miRNA analysis within the forensic science field.

Published
2020

6. Employing mesenchymal stem cells to support tumor-targeted delivery of extracellular vesicle (EV)-encapsulated microRNA-379

Author

Martin J. Leahy, Sonja Khan, Helen Ingoldsby, J. R. Schweber, Claire L. Glynn, Cathal O'Flatharta, Pierce Lalor, William M. Gallagher, Peter Dockery, Killian P. O’Brien, Katie E. Gilligan, J. M. Murphy, Timothy O'Brien, K. St John, Roisin M. Dwyer, A. De Bhulbh, Haroon Zafar, and Michael J. Kerin

Subjects
0301 basic medicine, MECHANISM, Cancer Research, THERAPY, Metastasis, Mice, Drug Delivery Systems, Neoplasm Metastasis, Cells, Cultured, education.field_of_study, Mice, Inbred BALB C, Therapies, Investigational, Extracellular vesicle, Primary tumor, CYCLOOXYGENASE-2 EXPRESSION, PANCREATIC-CANCER, APOPTOSIS, Gene Expression Regulation, Neoplastic, Adult Stem Cells, Lymphatic Metastasis, Female, Stromal cell, Drug Compounding, Population, Mice, Nude, Breast Neoplasms, Biology, Mesenchymal Stem Cell Transplantation, 03 medical and health sciences, Extracellular Vesicles, In vivo, Genetics, medicine, Animals, Humans, BREAST-CANCER, education, Molecular Biology, EXOSOMES, Mesenchymal stem cell, Mesenchymal Stem Cells, MIR-379, Genetic Therapy, medicine.disease, Xenograft Model Antitumor Assays, Microvesicles, MicroRNAs, 030104 developmental biology, STROMAL CELLS, METASTASIS, Cancer research
Abstract

Adult Mesenchymal Stem Cells (MSCs) have a well-established tumor-homing capacity, highlighting potential as tumor-targeted delivery vehicles. MSCs secrete extracellular vesicle (EV)-encapsulated microRNAs, which play a role in intercellular communication. The aim of this study was to characterize a potential tumor suppressor microRNA, miR-379, and engineer MSCs to secrete EVs enriched with miR-379 for in vivo therapy of breast cancer. miR-379 expression was significantly reduced in lymph node metastases compared to primary tumor tissue from the same patients. A significant reduction in the rate of tumor formation and growth in vivo was observed in T47D breast cancer cells stably expressing miR-379. In more aggressive HER2-amplified HCC-1954 cells, HCC-379 and HCC-NTC tumor growth rate in vivo was similar, but increased tumor necrosis was observed in HCC-379 tumors. In response to elevated miR-379, COX-2 mRNA and protein was also significantly reduced in vitro and in vivo. MSCs were successfully engineered to secrete EVs enriched with miR-379, with the majority found to be of the appropriate size and morphology of exosomal EVs. Administration of MSC-379 or MSC-NTC cells, or EVs derived from either cell population, resulted in no adverse effects in vivo. While MSC-379 cells did not impact tumor growth, systemic administration of cell-free EVs enriched with miR-379 was demonstrated to have a therapeutic effect. The data presented support miR-379 as a potent tumor suppressor in breast cancer, mediated in part through regulation of COX-2. Exploiting the tumor-homing capacity of MSCs while engineering the cells to secrete EVs enriched with miR-379 holds exciting potential as an innovative therapy for metastatic breast cancer. peer-reviewed

Published
2018

8. Abstract P4-07-05: Exosome-mediated trafficking of microRNAs by breast cancer cells

Author

Peter Dockery, Roisin M. Dwyer, Emma Holian, James A. Brown, Claire L. Glynn, Michael J. Kerin, and Doireann P. Joyce

Subjects
Regulation of gene expression, Cancer Research, Messenger RNA, Cell, Cancer, Biology, medicine.disease, Molecular biology, Exosome, Microvesicles, Cell biology, medicine.anatomical_structure, Oncology, Cell culture, microRNA, medicine
Abstract

Introduction Cellular communication in the primary tumour micro-environment is known to play a key role in tumour development and progression. Exosomes are membrane-derived nanovesicles that are actively secreted by cells. Exosomes have been implicated in cell-to-cell communication through the transfer of genetic material including messenger RNA (mRNA), and more recently microRNA (miRNA). miRNAs are small non-coding RNAs approximately 22 nucleotides in length. They play an important role in posttranscriptional regulation of gene expression. Recent reports suggest exosome-mediated trafficking of microRNAs between cells. The aim of this study was to identify the panel of exosome-encapsulated microRNAs secreted by breast cancer cells in vitro. Methods Four breast cancer cell lines, MDA-MB-231, BT-20, Sk-Br-3 and T47D were cultured in exosome-depleted media for 48 hours. Exosomes secreted by the cells were isolated through a process of differential centrifugation, microfiltration and ultracentrifugation. The presence of exosomes was first confirmed by Transmission Electron Microscopy (TEM) and Western Blot analysis. Global miRNA array analysis of RNA extracted from exosomes was performed to identify the panel of miRNAs secreted by these cells. miRNA targets of interest were further validated using relative quantification PCR (RQ-PCR). Transfer of Red fluorescent protein (RFP)-labelled exosomes between cell populations was visualized using Confocal microscopy. Results TEM analysis of secreted exosomes revealed vesicular bodies of 40-100nm in size. Immunoblotting confirmed the presence of the exosome-associated protein CD63. MicroRNA array analysis of exosome fractions targeting 2089 miRNAs, revealed secretion of between 324 and 394 miRNAs by the cell lines. The miRNAs appeared to cluster in a biologically relevant fashion. 282 miRNAs were common to exosomes from all 4 cell lines, while a small selection were specific to individual cell lines. Exosome-mediated trafficking of miRNA targets of interest including miR-451a and miR-744-5p was successfully validated using RQ-PCR. Further validated targets included miR-10b, miR-145, miR-492 and miR-498, all of which have established roles in regulation of proliferation and apoptosis in cancer. Confocal microscopy supported visualization of miRNA-enriched exosome release from donor cells and subsequent uptake of the RFP-labelled exosomes by recipient cells. Conclusions A distinct panel of miRNAs are actively and selectively packaged into exosomes and secreted by breast cancer cells. This transfer of functional miRNAs between cells may play an important role in intercellular communication in the primary tumour microenvironment. The data presented also has potentially important implications in the identification of a circulating miRNA signature for breast cancer detection. Citation Format: Doireann P Joyce, Claire L Glynn, James Brown, Emma Holian, Peter Dockery, Michael J Kerin, Roisin M Dwyer. Exosome-mediated trafficking of microRNAs by breast cancer cells [abstract]. In: Proceedings of the Thirty-Seventh Annual CTRC-AACR San Antonio Breast Cancer Symposium: 2014 Dec 9-13; San Antonio, TX. Philadelphia (PA): AACR; Cancer Res 2015;75(9 Suppl):Abstract nr P4-07-05.

Published
2015

9. Investigating the Isolation and Amplification of microRNAs for Forensic Body Fluid Identification

Author

Claire L. Glynn and Kelsie R O Leary

Subjects
Adult, Forensic Genetics, Male, Adolescent, Computational biology, Biology, Real-Time Polymerase Chain Reaction, Forensic dna, Young Adult, Semen, microRNA, Humans, Orthopedics and Sports Medicine, Saliva, Menstrual blood, Molecular identification, Body fluid, General Medicine, Middle Aged, Isolation (microbiology), Body Fluids, Menstruation, MicroRNAs, Potential biomarkers, Vagina, Emergency Medicine, Identification (biology), Female, Biomarkers
Abstract

Background The discovery of forensic DNA typing evolved molecular biology far beyond what could have been expected in terms of its forensic application, and now there exists other developments in molecular biology which are ready for application to forensic challenges. One such challenge is the identification of the body fluid source of stains recovered from evidence items and crime scenes. Currently, there are significant efforts in the research field to develop novel methods for the molecular identification of body fluids, with microRNAs (miRNAs) revealing great potential. MiRNAs have been shown to have high tissue specificity and are less susceptible to degradation as a result of their small size, which infers great advantages to their potential role for identifying forensically relevant body fluids. Objective This study investigated the isolation and amplification of miRNAs from forensically relevant body fluids. Method Venous blood, menstrual blood, semen, saliva, and vaginal material samples were extracted using; miRNeasy® mini kit (Qiagen), mirVana™ miRNA isolation kit (Ambion), and a modified mir- Vana™ method, and the quality/quantity of isolated miRNA was determined. miRNAs previously identified to show specificity for particular forensically relevant body fluids were examined. Real Time-Quantitative PCR (RT-qPCR) was performed targeting 5 miRNAs of interest, miR-451, miR- 412, miR-891a, miR-205 and miR-124a. Results This study identified the miRNeasy® mini kit as the optimal method of the three methods investigated for the extraction of miRNAs from body fluids and further validates a selection of miRNAs previously suggested as potential biomarkers. Conclusion This research highlights the potential of miRNAs as novel markers for the identification of forensically relevant body fluids.

Published
2017

11. Impact of Tumour Epithelial Subtype on Circulating microRNAs in Breast Cancer Patients

Author

Deirdre Wall, Peadar S. Waters, Claire L. Glynn, Cathy Brougham, Maria Duignan, Roisin M. Dwyer, John Newell, Michael J. Kerin, Mark McLoughlin, and Peter Hyland

Subjects
Pathology, Microarray, diagnosis, Tumor Physiology, markers, lcsh:Medicine, Polymerase Chain Reaction, Mice, Basal (phylogenetics), Basic Cancer Research, Breast Tumors, lcsh:Science, skin and connective tissue diseases, Oligonucleotide Array Sequence Analysis, Multidisciplinary, Middle Aged, Gene Expression Regulation, Neoplastic, Surgical Oncology, Oncology, Disease Progression, Medicine, Female, Research Article, medicine.medical_specialty, Clinical Research Design, Mice, Nude, Breast Neoplasms, Breast cancer, down-regulation, Diagnostic Medicine, Cell Line, Tumor, expression, microRNA, Biomarkers, Tumor, Cancer Detection and Diagnosis, medicine, Animals, Humans, Clinical significance, Animal Models of Disease, therapy, business.industry, Carcinoma, lcsh:R, Cancers and Neoplasms, biomarkers, medicine.disease, MicroRNAs, Circulating MicroRNA, cell-lines, Cell culture, recommendations, Surgery, lcsh:Q, prognosis, business, serum, General Pathology, Blood sampling
Abstract

While a range of miRNAs have been shown to be dysregulated in the circulation of patients with breast cancer, little is known about the relationship between circulating levels and tumour characteristics. The aim of this study was to analyse alterations in circulating miRNA expression during tumour progression in a murine model of breast cancer, and to detemine the clinical relevance of identified miRNAs at both tissue and circulating level in patient samples. Athymic nude mice received a subcutaneous or mammary fat pad injection of MDA-MB-231 cells. Blood sampling was performed at weeks 1, 3 and 6 following tumour induction, and microRNA extracted. MicroRNA microArray analysis was performed comparing samples harvested at week 1 to those collected at week 6 from the same animals. Significantly altered miRNAs were validated across all murine samples by RQ-PCR (n = 45). Three miRNAs of interest were then quantified in the circulation(n = 166) and tissue (n = 100) of breast cancer patients and healthy control individuals. MicroArray-based analysis of murine blood samples revealed levels of 77 circulating microRNAs to be changed during disease progression, with 44 demonstrating changes >2-fold. Validation across all samples revealed miR-138 to be significantly elevated in the circulation of animals during disease development, with miR-191 and miR-106a levels significantly decreased. Analysis of patient tissue and blood samples revealed miR-138 to be significantly up-regulated in the circulation of patients with breast cancer, with no change observed in the tissue setting. While not significantly changed overall in breast cancer patients compared to controls, circulating miR-106a and miR-191 were significantly decreased in patients with basal breast cancer. In tissue, both miRNAs were significantly elevated in breast cancer compared to normal breast tissue. The data demonstrates an impact of tumour epithelial subtype on circulating levels of miRNAs, and highlights divergent miRNA profiles between tissue and blood samples from breast cancer patients.

Published
2014

12. Isolation of secreted microRNAs (miRNAs) from cell-conditioned media

Author

Roisin M. Dwyer, Claire L. Glynn, Sonja Khan, Michael J. Kerin, and ~

Subjects
Pathology, medicine.medical_specialty, Stromal cell, Cell, Extraction, Breast Neoplasms, Biology, Real-Time Polymerase Chain Reaction, Cell culture media, Breast cancer, Fresh Tissue, microRNA, Biomarkers, Tumor, Tumor Cells, Cultured, medicine, Humans, Orthopedics and Sports Medicine, Lymph node, Secretion, Biomarker, General Medicine, Molecular biology, Gene Expression Regulation, Neoplastic, Circulation, MicroRNAs, medicine.anatomical_structure, Real-time polymerase chain reaction, Cell culture, Culture Media, Conditioned, Emergency Medicine, Female, Explant culture
Abstract

MicroRNAs (miRNAs) have been found to be stable in the circulation of cancer patients raising their potential as circulating biomarkers of disease. The specific source and role, however, of miRNAs in the circulation is unknown and requires elucidation to determine their true potential. In this study, along with primary tissue explants and primary stromal cells, three breast cancer cell lines were employed, including T47D, MDA-MB-231 and SK-BR-3. Tissue explants were harvested in theatre, with informed patient consent, and included tumour, tumour associated normal, and diseased lymph node samples. Cell-conditioned media containing all factors secreted by the cells were harvested. MiRNAs were extracted from samples using 5 different extraction techniques including the blood protocol, RNeasy® (Qiagen), miRNeasy® mini kit (Qiagen), mirVana(tm) isolation kit (Ambion) and RNAqueous® kit (Ambion). MiRNAs were successfully isolated from all media samples collected from cell lines, primary cells and fresh tissue explants. However, there was remarkable variation in yield depending on the extraction method used. Aliquots of the same samples were extracted, revealing the two column extraction protocol of the mirVana® miRNA isolation kit to be the most suitable approach. A range of miRNAs, including miR-16, miR-195, miR-497 and miR-10b, were successfully amplified. While miR-16 and miR-195 were detected in media from both cell lines and tissue explants, miR-497 and miR-10b were only detected in secretions from whole tissue explants. The ability to achieve reliable and reproducible miRNA yields from cell-conditioned media is vital for the successful amplification of miRNAs by RQ-PCR. NBCRI peer-reviewed

13. Screening of exosomal microRNAs from colorectal cancer cells

Author

Claire L. Glynn, Peter Dockery, Pierce Lalor, Michael J. Kerin, Myles R. Joyce, James A. Brown, Sonja Khan, Roisin M. Dwyer, Cillian Clancy, Emma Holian, Breast Cancer Research, and Irish Cancer Society

Subjects
EXPRESSION, 0301 basic medicine, Cancer Research, INVASION, Cell, colorectal cancer, Biology, Exosomes, Exosome, 03 medical and health sciences, 0302 clinical medicine, Cell Line, Tumor, microRNA, Genetics, medicine, Humans, BREAST-CANCER, Secretion, MESSENGER-RNAS, Cell Proliferation, CD63, Cell growth, MIR-378, General Medicine, HCT116 Cells, Molecular biology, Microvesicles, microRNAs, Cell biology, 030104 developmental biology, medicine.anatomical_structure, MEDIATED TRANSFER, Oncology, Cell culture, 030220 oncology & carcinogenesis, Colorectal Neoplasms, HT29 Cells
Abstract

BACKGROUND:Cells release extracellular membrane vesicles including microvesicles known as exosomes. Exosomes contain microRNAs (miRNAs) however the full range within colorectal cancer cell secreted exosomes is unknown. OBJECTIVE: To identify the full range of exosome encapsulated miRNAs secreted from 2 colorectal cancer cell lines and to investigate engineering of exosomes over-expressing miRNAs. METHODS: Exosomes were isolated from HCT-116 and HT-29 cell lines. RNA was extracted from exosomes and microRNA array performed. Cells were engineered to express miR-379 (HCT-116-379) or a non-targeting control (HCT-116-NTC) and functional effects were determined. Exosomes secreted by engineered cells were transferred to recipient cells and the impact examined. RESULTS: Microvesicles 40–100 nm in size secreted by cell lines were visualised and confirmed to express exosomal protein CD63. HT-29 exosomes contained 409 miRNAs, HCT-116 exosomes contained 393, and 338 were common to exosomes from both cell lines. Selected targets were validated. HCT-116-379 cells showed decreased proliferation (12–15% decrease, p< 0.001) and decreased migration (32–86% decrease, p< 0.001) compared to controls. HCT-116-379 exosomes were enriched for miR-379. Confocal microscopy visualised transfer of HCT-116-379 exosomes to recipient cells. CONCLUSIONS: Colorectal cancer cells secrete a large number of miRNAs within exosomes. miR-379 decreases cell proliferation and migration, and miR-379 enriched exosomes can be engineered.

14. Investigating the Potential and Pitfalls of EV-Encapsulated MicroRNAs as Circulating Biomarkers of Breast Cancer

Author

Brian M. Moloney, Katie E. Gilligan, Doireann P. Joyce, Clodagh P. O’Neill, Killian P. O’Brien, Sonja Khan, Claire L. Glynn, Ronan M. Waldron, Ciarán M. Maguire, Emma Holian, Erin Naughton, Mohamed Elhadi, Andrea B. Grealish, Carmel Malone, Emma McDermott, Peter Dockery, Thomas Ritter, Adriele Prina-Mello, Michael J. Kerin, and Róisín M. Dwyer

Subjects
breast cancer, extracellular vesicles, exosomes, microrna, biomarker, ev characterization, Cytology, QH573-671
Abstract

Extracellular vesicles (EVs) shuttle microRNA (miRNA) throughout the circulation and are believed to represent a fingerprint of the releasing cell. We isolated and characterized serum EVs of breast tumour-bearing animals, breast cancer (BC) patients, and healthy controls. EVs were characterized using transmission electron microscopy (TEM), protein quantification, western blotting, and nanoparticle tracking analysis (NTA). Absolute quantitative (AQ)-PCR was employed to analyse EV-miR-451a expression. Isolated EVs had the appropriate morphology and size. Patient sera contained significantly more EVs than did healthy controls. In tumour-bearing animals, a correlation between serum EV number and tumour burden was observed. There was no significant relationship between EV protein yield and EV quantity determined by NTA, highlighting the requirement for direct quantification. Using AQ-PCR to relate miRNA copy number to EV yield, a significant increase in miRNA-451a copies/EV was detected in BC patient sera, suggesting potential as a novel biomarker of breast cancer.

Published
2020
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