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  • About
  • The Global ETD Search service is a free service for researchers to find electronic theses and dissertations. This service is provided by the Networked Digital Library of Theses and Dissertations.
    Our metadata is collected from universities around the world. If you manage a university/consortium/country archive and want to be added, details can be found on the NDLTD website.
11

Effects of Vasoflux on DNA-Histone Complexes in Vitro and on Organ Function and Survival Outcome in a Murine Model of Sepsis

Sharma, Neha January 2018 (has links)
Sepsis is life-threatening organ dysfunction produced by a dysregulated host response to infection in which neutrophils release neutrophil extracellular traps (NETs). NETs consist of DNA, histones, and antimicrobial peptides which kill pathogens. However, DNA and histones also exert damage by activating the intrinsic pathway of coagulation and inducing endothelial cell death, respectively. AADH, a 15kDa non-anticoagulant unfractionated heparin (UFH), prevents histone-mediated cytotoxicity in vitro and improves survival in septic mice. We explored the effectiveness of Vasoflux, a 5.5kDa low-molecular-weight-heparin as an anti-sepsis treatment as compared to enoxaparin and UFH. Vasoflux has reduced anticoagulant functions and hence reduces the risk of bleeding as compared to enoxaparin or UFH. We showed that UFH, enoxaparin, or Vasoflux at concentrations of up to 13.3uM, 40uM, or 40uM, neutralize histone-mediated cytotoxicity. These results suggest that these glycosaminoglycans (GAGs) are able to neutralize histone-mediated cytotoxicity independent of the AT-binding pentasaccharide. To quantitate the binding affinity between GAGs and histones, surface plasmon resonance was conducted. UFH is a more potent inhibitor of histone-mediated cytotoxicity compared to Vasoflux as UFH has a 10-fold greater binding affinity to histones compared to Vasoflux. To translate our in vitro findings to in vivo, Vasoflux, enoxaparin, and UFH were administered in a murine model of sepsis. Vasoflux at 8mg/kg - 50mg/kg reduced survival and exhibited damage in the lung, liver, and kidney in septic mice compared to 10 mg/kg of UFH or 8mg/kg of enoxaparin. This may be due to Vasoflux and UFH disrupting the DNA-histone complex, thereby releasing free procoagulant DNA. This is evident by our gel electrophoresis experiments, where addition of 1uM Vasoflux or 3.3uM UFH to DNA-histone complexes lead to histone dissociation from DNA. UFH bound to histones may be able to inhibit DNA-mediated thrombin generation, as it retains its anticoagulant properties, demonstrated by UFH-histone complexes attenuating DNA and TF-mediated thrombin generation. In contrast, Vasoflux may not neutralize the procoagulant DNA leading to a hypercoagulable state in the mice. Our study may have important clinical implications as there is an ongoing trial, HALO, which will administer intravenous UFH to patients suspected to have septic shock to reduce mortality. Based on our results, future clinical trials should consider the antithrombin-dependent anticoagulant activity of UFH being used as a sepsis treatment. / Thesis / Master of Science (MSc) / Sepsis is a life threatening condition caused by the body’s extreme response to microbial infection of the blood, whereby neutrophils release traps composed of cell-free DNA (cfDNA), histones, and antimicrobial proteins. In addition to fighting off infections, these traps also exert harmful effects like triggering clotting and killing host cells. Currently, no specific anti-septic drugs exist. Studies have shown that DNase1 (a recombinant protein that digests double stranded cfDNA) or a modified form of heparin (neutralizes histones) improves survival in septic mice. Our goal was to explore the protective effects of Vasoflux, (a non-anticoagulant heparin) and DNase1 in a mouse model of sepsis. We hypothesize that the combined therapy of DNase1 and Vasoflux will improve survival. We found that Vasoflux has minimal blood thinning activity and can prevent histones from killing cells. However, Vasoflux administered into septic mice worsened organ damage and decreased survival. We hypothesize that this damage may be due to Vasoflux’s ability to displace histones from histone-DNA complexes, thereby releasing free DNA, which promotes excessive blood clotting in sepsis.
12

Clinical impact of detecting low-frequency variants in cell-free DNA on treatment of castration-resistant prostate cancer / 血中遊離DNAにおける低頻度変異検出が去勢抵抗性前立腺癌の治療に与える影響

Mizuno, Kei 23 March 2022 (has links)
京都大学 / 新制・課程博士 / 博士(医学) / 甲第23772号 / 医博第4818号 / 新制||医||1056(附属図書館) / 京都大学大学院医学研究科医学専攻 / (主査)教授 村川 泰裕, 教授 松田 文彦, 教授 篠原 隆司 / 学位規則第4条第1項該当 / Doctor of Medical Science / Kyoto University / DFAM
13

O fenômeno de lente térmica em amostras de DNA livre circulante de pacientes com malignidade e sãos, investigado por meio da técnica de varredura-Z / The Thermal Lens Phenomenon in Cell Free DNA Samples from Patients with Malignancy and Sane, Investigated by the Z-Scan Technique.

Silva, Luiz Henrique da 03 February 2017 (has links)
No presente estudo investigou-se amostras de plasma com DNA livre circulante (DNA LC) por meio da técnica Varredura Z. Esta é uma técnica eficiente na determinação de parâmetros de diferentes materiais, tais como cristais líquidos, ferrofluidos e compostos biológicos. Esta experiência é realizada através da focalização de um feixe laser de perfil gaussiano numa amostra. Na medida em que a amostra se aproxima do foco da lente, a intensidade do feixe aumenta e alcança seu valor máximo no ponto focal, então diminui para pontos distantes do foco. Na região próxima ao ponto focal se amplificam os fenômenos não-lineares. Recentemente foi demonstrado que níveis elevados de DNA LC no plasma ocorrem com frequência em pacientes com vários tipos de câncer, podendo ser utilizados para discriminar pacientes com malignidade de pessoas saudáveis. As amostras de DNA LC, submetidas ao experimento Varredura Z, forneceram respostas ópticas devido ao fenômeno de lente térmica. Os resultados revelaram que a amplitude de lente térmica das amostras extraídas do plasma de pacientes com malignidade difere daquela de doadores sãos. A técnica Varredura Z se mostrou mais vantajosa em relação a outras biológicas porque revelou uma maior diferença entre os grupos estudados e tem o caráter de detectar mudanças estruturais no DNA LC. / In the present study plasma samples with cell-free DNA were investigated by means of the Z-Scan technique. This is a powerfull technique in determining parameters of different materials, such as liquid crystals, ferrofluids and biological compounds. This experiment is performed by focusing a Gaussian profile laser beam on a sample. As the sample approaches the focus of the lens, the intensity of the beam increases and reaches its maximum value at the focal point, then decreases to points distant from the focus. In the region near the focal point non-linear phenomena are amplified. It has recently been demonstrated that high levels of plasma cell-free DNA occur frequently in patients with various cancers and can be used to discriminate patients with malignancy from healthy donors. The cell-free DNA samples, submitted to the Z-Scan experiment, provided optical responses due to the thermal lens phenomenon. The results revealed that the thermal lens amplitude of samples extracted from the plasma of patients with malignancy differs from that of healthy donors. The Z-Scan technique was more advantageous than other biological ones because it revealed a greater difference between the studied groups and has the character of detecting structural changes in cell-free DNA.
14

Les acides nucléiques circulants : biomarqueurs d'intérêt en Assistance Médicale à la Procréation / Circulating nucleic acids : innovative biomarkers in Assisted Reproductive Technology.

Scalici, Elodie 18 December 2015 (has links)
Au cours de ces dernières années, l’utilisation des acides nucléiques circulants comme outils diagnostiques et/ou pronostiques en cancérologie a largement été documentée. Récemment, le développement du diagnostic prénatal non-invasif a également révélé l’intérêt grandissant de ces biomarqueurs en gynécologie-obstétrique. Les acides nucléiques circulants ou extracellulaires ont la particularité d’être facilement détectables dans les fluides biologiques de l’organisme et sont de deux types: (1) l’ADN libre, courts ou longs fragments d’ADN provenant des processus apoptotiques et/ou nécrotiques cellulaires (2) les microARNs, petites séquences d’ARN non codantes, qui régulent l’expression des gènes en interférant avec leurs ARNm cibles. Sachant qu’il a été démontré que le taux d’ADN libre circulant est anormalement élevé dans certaines conditions pathologiques et que les microARNs sont impliqués dans la régulation de nombreux processus biologiques tels que la folliculogénèse et la stéroïdogénèse, ces deux types d’acides nucléiques pourraient alors constituer des biomarqueurs d’intérêt dans le domaine de l’Assistance Médicale à la Procréation. Dans ce travail de thèse, nous avons à la fois mesuré le taux d’ADN libre et analysé les profils d’expression de plusieurs microARNs d’intérêt par PCR quantitative, dans le liquide folliculaire (LF) de patientes prises en charge en fécondation in vitro (FIV). Nous avons observé des taux d’ADN libre significativement élevés ainsi que des profils d’expression de microARNs spécifiques dans le LF de patientes présentant des anomalies de la réserve ovarienne (telles que le syndrome des ovaires micropolykystiques ou une faible réserve ovarienne). Nous avons ensuite évalué le potentiel des acides nucléiques circulants en tant biomarqueurs prédictifs des résultats en FIV. Nous avons démontré que le taux d’ADN libre intra-folliculaire et l’expression de certains microARNs étaient significativement associés à la qualité des embryons obtenus in vitro ainsi qu’à la survenue d’une grossesse clinique. Les acides nucléiques circulants offrent donc de nouvelles perspectives à la fois d’un point de vue diagnostique et pronostique dans la prise en charge de l’infertilité humaine. / During the last years, the use of circulating nucleic acids as diagnostic and/or prognostic tools in cancerology was widely documented. The recent development of non-invasive prenatal testing also reveals the growing interest of these biomarkers in obstetrics and gynecology. The circulating or extracellular nucleic acids have for particularity to be easily detectable in the biological fluids of the body and there are two types: (1) Cell-free DNA (cfDNA), short or long DNA fragments resulting from cellular apoptosis and/or necrosis (2) microRNAs (miRNAs), small non-coding RNA sequences, which regulate gene expression by interfering with their mRNA targets. Since it was demonstrated that cfDNA level is abnormally increased in some pathological conditions and miRNAs are involved in the regulation of several biological processes such as folliculogenesis and steroidogenesis, these two types of nucleic acids could constitute new biomarkers of interest in Assisted Reproductive Technology. In this thesis work, we quantified the cfDNA level and analysed the expression profiles of some miRNAs by quantitative PCR, in follicular fluid (FF) samples from women undergoing in vitro fertilization (IVF) procedure. We observed significant high cfDNA levels as well as specific miRNA expression profiles in FF from women with ovarian disorders (such as polycystic ovary syndrome or low ovarian reserve). Next, we investigated the potential of circulating nucleic acids as predictive biomarkers of IVF outcomes. We demonstrated that the intra-follicular cfDNA level and some miRNA expressions were significantly associated with in vitro embryo quality and the clinical pregnancy outcome. Therefore, the circulating nucleic acids offer new diagnostic and prognostic perspectives in human infertility management.
15

O fenômeno de lente térmica em amostras de DNA livre circulante de pacientes com malignidade e sãos, investigado por meio da técnica de varredura-Z / The Thermal Lens Phenomenon in Cell Free DNA Samples from Patients with Malignancy and Sane, Investigated by the Z-Scan Technique.

Luiz Henrique da Silva 03 February 2017 (has links)
No presente estudo investigou-se amostras de plasma com DNA livre circulante (DNA LC) por meio da técnica Varredura Z. Esta é uma técnica eficiente na determinação de parâmetros de diferentes materiais, tais como cristais líquidos, ferrofluidos e compostos biológicos. Esta experiência é realizada através da focalização de um feixe laser de perfil gaussiano numa amostra. Na medida em que a amostra se aproxima do foco da lente, a intensidade do feixe aumenta e alcança seu valor máximo no ponto focal, então diminui para pontos distantes do foco. Na região próxima ao ponto focal se amplificam os fenômenos não-lineares. Recentemente foi demonstrado que níveis elevados de DNA LC no plasma ocorrem com frequência em pacientes com vários tipos de câncer, podendo ser utilizados para discriminar pacientes com malignidade de pessoas saudáveis. As amostras de DNA LC, submetidas ao experimento Varredura Z, forneceram respostas ópticas devido ao fenômeno de lente térmica. Os resultados revelaram que a amplitude de lente térmica das amostras extraídas do plasma de pacientes com malignidade difere daquela de doadores sãos. A técnica Varredura Z se mostrou mais vantajosa em relação a outras biológicas porque revelou uma maior diferença entre os grupos estudados e tem o caráter de detectar mudanças estruturais no DNA LC. / In the present study plasma samples with cell-free DNA were investigated by means of the Z-Scan technique. This is a powerfull technique in determining parameters of different materials, such as liquid crystals, ferrofluids and biological compounds. This experiment is performed by focusing a Gaussian profile laser beam on a sample. As the sample approaches the focus of the lens, the intensity of the beam increases and reaches its maximum value at the focal point, then decreases to points distant from the focus. In the region near the focal point non-linear phenomena are amplified. It has recently been demonstrated that high levels of plasma cell-free DNA occur frequently in patients with various cancers and can be used to discriminate patients with malignancy from healthy donors. The cell-free DNA samples, submitted to the Z-Scan experiment, provided optical responses due to the thermal lens phenomenon. The results revealed that the thermal lens amplitude of samples extracted from the plasma of patients with malignancy differs from that of healthy donors. The Z-Scan technique was more advantageous than other biological ones because it revealed a greater difference between the studied groups and has the character of detecting structural changes in cell-free DNA.
16

The Relationship Between Cell-Free DNA and Resistance Training

Lang, Henry 01 August 2020 (has links)
The primary purposes of this dissertation were to explore relationship between cell free DNA (cf-DNA), creatine kinase (CK), C-reactive protein (CRP), vertical jump testing delayed onset muscle soreness (DOMS) in response to a high-volume resistance training protocol, and to assess the sensitivity of cf-DNA to different resistance training volume loads. The secondary purpose was to examine the relationship between cf-DNA and relative strength. Study 1 was an exploratory attempt to discover relationships between cf-DNA, CK, CRP, delayed onset muscle soreness, and performance variables. Seventeen resistance trained males were recruited, 9 were randomly assigned to receive BCAAs while 8 received a placebo. Participants performed a high-volume resistance training session consisting of the back squat and bench press. Blood was drawn to measure serum cf-DNA, CK, and CRP levels prior to the training session, with cf-DNA collected immediately post, and CK and CRP at 24hr and 48hrs post. Self-reported DOMS on a scale of 1 to 10 was collected prior to training on day 2, day 3, and day 4. SJH, CMJH, and BOSCO were collected on day 1, day 3, and day 4. Fifty-seven correlations were run to explore the relationships between variables. Only the correlation between %Δ DOMS 48hr and %Δ CRP 48hr in the non-supplement group was significant (p = 0.02). The second study, designed to assess the sensitivity of cf-DNA to different resistance training volume loads, consisted of a high-volume resistance training protocol. Blood was drawn immediately before the resistance training session (T1), immediately after the third lifting set (T2), and immediately after the sixth lifting set (T3). cf-DNA increased significantly from T1 to T2 (p < 0.01) and T1 to T3 (p < 0.01). The linear regression model used to examine the capabilities of relative strength to predict %Δ cf-DNA from T1 to T3 was significant (p = 0.04). The results of this study demonstrate the short response time of cf-DNA in relation to variations in resistance training volume-load, suggesting it may be a valuable marker in monitoring the immune response to volume-load. Results also demonstrated the positive relationship between relative strength and %Δ cf-DNA.
17

Applications of ctDNA Genomic Profiling to Metastatic Triple Negative Breast Cancer

Weber, Zachary Thomas 01 October 2020 (has links)
No description available.
18

IN VIVO STUDIES OF CELL-FREE DNA AND DNASE IN A MURINE MODEL OF POLYMICROBIAL SEPSIS

Mai, Safiah Hwai Chuen January 2016 (has links)
Sepsis is a clinical syndrome characterized by the systemic activation of inflammatory and coagulation pathways in response to microbial infection of normally sterile parts of the body. Despite considerable advances in our understanding of sepsis pathophysiology, sepsis remains the leading cause of death in non-coronary intensive care units (ICU) with a global disease burden between 15 and 19 million cases per year (Dellinger et al., 2008). Severe sepsis, defined as sepsis associated with organ dysfunction is associated with mortality rates of 33% to 45%. The incidence of severe sepsis continues to increase by 1.5% per annum due to the aging population, a rise in the prevalence of comorbidities, and the wider use of immunosuppressive agents and invasive procedures (Angus et al., 2001). Over the past several decades, many potential treatments for sepsis have shown early promise, yet have failed to improve survival in over 100 Phase II and Phase III clinical trials (Marshall, 2014) suggesting that some fundamental knowledge is lacking in our understanding of sepsis pathophysiology. Emerging studies on cell-free DNA (cfDNA), DNA released extracellularly into the circulation, demonstrate that cfDNA is a crucial link between inflammation and coagulation . In various conditions characterized by excessive inflammatory responses or aberrant prothrombotic responses, cfDNA has been implicated in exacerbating disease pathology (Atamaniuk, Kopecky, Skoupy, Säemann, & Weichhart, 2012; Fuchs, Brill, & Wagner, 2012; Swystun, Mukherjee, & Liaw, 2011). In clinical sepsis, levels of cfDNA upon admission into the ICU have strong prognostic value in predicting mortality (Dwivedi et al., 2012; Saukkonen et al., 2008). However, it is unclear whether these increases in cfDNA are an epiphenomenon during sepsis progression, or whether cfDNA actively plays a role in sepsis pathophysiology. In this work, in vivo studies were conducted to characterize the role of cfDNA in sepsis, the effects of DNase administration, and the potential mechanism by which cfDNA is released during experimental sepsis. In addition, mortality studies were conducted to identify surrogate markers of death to promote the design of humane and ethical animal studies in conducting sepsis research. Polymicrobial sepsis was induced via a surgical procedure whereby the cecum is exteriorized, ligated and punctured twice to introduce a continuous source of microorganisms, a model termed cecal ligation and puncture (CLP). In our CLP sepsis model, levels of cfDNA increased in a time-dependent manner. These increases accompanied an early pro-inflammatory response marked by increased pro-inflammatory IL-6, a transient increase in anti-inflammatory IL-10, and elevated lung myeloperoxidase (MPO) activity. Septic mice with elevated cfDNA levels also had high bacterial loads in the lungs, blood, and peritoneal cavity fluid. Organ damage was also observed in mice following CLP surgery versus mice subjected to the non-septic sham control surgery marked by increased levels of creatinine and alanine aminotransferase (ALT) indicative of kidney and liver injury, respectively. Histological analyses further confirmed lung and kidney damage following CLP surgery. Changes in coagulation were also observed in septic mice as mice subjected to CLP had sustained increases in thrombin-antithrombin (TAT) complexes. In addition, plasma from CLP-operated mice had increased thrombin generation (i.e. increased endogenous thromin potential, increased peak thrombin, decreased time to peak, and decreased lag time) mediated by FXIIa and enhanced by platelets. Following CLP-induced sepsis, elevations in cfDNA levels accompanied pro-inflammatory and pro-coagulant responses. The effects of in vivo DNase treatment in septic mice were time-dependent. Early DNase treatment when cfDNA levels were low resulted in an exaggerated pro-inflammatory response marked by increased plasma IL-6 levels and increased lung damage. In contrast, delayed DNase treatment at time-points when cfDNA levels were elevated suppressed inflammation characterized by an increase in anti-inflammatory IL-10 and reductions in cfDNA, IL-6, lung MPO, and ALT activity. Furthermore, delayed DNase administration resulted in decreased bacterial load in the lungs, blood, and peritoneal cavity fluid. Delayed DNase treatment also resulted in blunted pro-coagulant responses as levels of TAT complexes were suppressed and thrombin generation from septic mouse plasma was normalized. Moreover, DNase treatment when cfDNA levels were elevated increased survival in CLP-operated mice by 80% and reduced lung and liver damage. These findings suggest that administration of DNase when cfDNA levels are elevated may reduce pro-inflammatory and pro-coagulant responses and that delayed DNase treatment may infer protection in the CLP model of sepsis. One mechanism by which cfDNA is released is via the formation of neutrophil extracellular traps (NETs). Upon inflammatory stimulation, some neutrophils release chromatin material and antimicrobial proteins (i.e. neutrophil elastase, MPO, and histones) in an active process termed NETosis. Although NETs ensnare bacteria and exert antimicrobial properties, NETs may also exert harmful effects on the host by activating inflammation and coagulation. While some in vitro evidence suggest that neutrophils are the main source of cfDNA released following inflammatory stimulation, others have reported that neutrophils are not the main source of circulating cfDNA following septic challenge. To determine whether NETs contribute to cfDNA released during CLP sepsis, genetically modified mice that are incapable of forming NETs, PAD4-/- mice, were used. Levels of cfDNA in PAD-/- mice were significantly lower than cfDNA levels in C57Bl/6 mice following CLP surgery, suggesting that NETs were a source of cfDNA in our model. Levels of IL-6, MPO, and bacterial load in the lungs, blood, and peritoneal cavity were significantly reduced, indicating that NETs exert pro-inflammatory effects in CLP sepsis. Thrombin generation was also suppressed in PAD4-/- mice which suggests that NETs contribute to thrombin generation following CLP sepsis. NETs contribute to increases in circulating cfDNA and may exacerbate pathology by driving pro-inflammatory and pro-coagulant responses in CLP-induced sepsis. Appreciating the implications of conducting research using animals, it is pertinent that researchers ensure the highest ethical standards and design animal studies in the most humane, yet scientifically rigorous manner. Using mortality studies, we validated the utility of physiological and phenotypic markers to assess disease severity and predict death in murine sepsis. Temperature via a rectal probe monitor and sepsis scoring systems which assess components such as orbital tightening, level of consciousness, and activity were effective surrogate markers of death. These tools offer a non-invasive assessment of disease progression which do not artificially exacerbate sepsis pathology and immediate information regarding any changes in the health status. Surrogate markers of death also provide reliable monitoring to meet increasing standards of ethical, humane animal research and a feasible and cost-efficient means to obtain vital signs in small rodents. We have proposed a scoring system which can be used for assessing disease severity, endpoint monitoring, and predicting death to obviate inhumane methods of using death as an endpoint in sepsis studies. In summary, cfDNA levels are elevated in CLP-induced sepsis and these elevations accompany pro-inflammatory and pro-coagulant responses. NETosis may be a mechanism by which cfDNA is released and NETs may drive inflammation and coagulation in CLP sepsis. Delayed DNase administration may suppress inflammation and coagulation and may be protective in polymicrobial sepsis. In future animal sepsis studies, surrogate markers of death and a sepsis scoring system can be used in place of death as an endpoint to raise the standards in conducting ethical, humane sepsis research. / Thesis / Doctor of Philosophy (PhD)
19

Targeted Sequencing of Plasma-Derived vs. Urinary cfDNA from Patients with Triple-Negative Breast Cancer

Herzog, Henrike, Dogan, Senol, Aktas, Bahriye, Nel, Ivonne 05 December 2023 (has links)
In breast cancer, the genetic profiling of circulating cell-free DNA (cfDNA) from blood plasma was shown to have good potential for clinical use. In contrast, only a few studies were performed investigating urinary cfDNA. In this pilot study, we analyzed plasma-derived and matching urinary cfDNA samples obtained from 15 presurgical triple-negative breast cancer patients. We used a targeted next-generation sequencing approach to identify and compare genetic alterations in both body fluids. The cfDNA concentration was higher in urine compared to plasma, but there was no significant correlation between matched samples. Bioinformatical analysis revealed a total of 3339 somatic breast-cancer-related variants (VAF ≥ 3%), whereof 1222 vs. 2117 variants were found in plasma-derived vs. urinary cfDNA, respectively. Further, 431 shared variants were found in both body fluids. Throughout the cohort, the recovery rate of plasma-derived mutations in matching urinary cfDNA was 47% and even 63% for pathogenic variants only. The most frequently occurring pathogenic and likely pathogenic mutated genes were NF1, CHEK2, KMT2C and PTEN in both body fluids. Notably, a pathogenic CHEK2 (T519M) variant was found in all 30 samples. Taken together, our results indicated that body fluids appear to be valuable sources bearing complementary information regarding the genetic tumor profile.
20

Entwicklung neuer Messverfahren zum Nachweis frei zirkulierender Tumor-DNA in Blutproben von Patienten mit malignen Erkrankungen

Gutewort, Katharina 03 June 2024 (has links)
Das Prostatakarzinom (PCa) ist die häufigste Krebsneuerkrankung und die zweithäufigste Krebstodesursache des Mannes in Deutschland. Die etablierten Tumormarker führen aufgrund ihrer unzureichenden diagnostischen Sensitivität und Spezifität zu Überdiagnosen mit folglich unnötigen Prostatabiopsien und den damit verbundenen klinischen Komplikationen. Darüber hinaus kann die derzeitige PSA-basierte Screeningpraxis nicht zuverlässig zwischen indolenter Erkrankung und therapienotwendigem Krebs unterscheiden. Auf DNA-Methylierung basierende Biomarker haben ein erhebliches Potenzial für die klinisch-chemische Labordiagnostik sowohl als tumorspezifische Biomarker für die Früherkennung oder posttherapeutische Überwachung von Krebs als auch als prognostische und prädiktive Biomarker für die therapeutische Stratifizierung. In dieser Arbeit erfolgte die Entwicklung neuer krebsspezifischer Methylierungs-Biomarker unter Anwendung OBBPA-ddPCR-basierter Assays. Diese neue Methode ermöglicht die Identifizierung geringster Mengen methylierter zellfreier-Tumor-DNA vor einem hohen Hintergrund von unmethylierter Wildtyp-DNA in Form einer minimal invasiven Blutprobenentnahme (liquid biopsy). Die Methylierungs-Biomarker beruhen auf Gensequenzen, welche zwischen gesunden Probanden und Patienten mit benigner Prostatahyperplasie (BPH) und PCa signifikante Methylierungsunterschiede aufweisen. Die Methylierungs-Biomarker RASSF1, SOX8, GSTP1, mir129-2, CCDC181, PAI1 und NRIP3, welche eine hohe diagnostische Sensitivität bei hoher diagnostischer Spezifität aufweisen, wurden zu einem Marker-Panel kombiniert. Anschließend wurde die Eignung dieses Panels als diagnostische Tumormarker in einer weiteren Probenserie validiert. Die Proben der Optimierungs- und Validierungsprobenserie beruhten auf Serumproben von 52 gesunden Probanden, sechs BPH-Patienten und 43 PCa-Patienten. Dabei erreichte das Biomarker-Panel eine diagnostische Sensitivität von 81,40 % bei einer diagnostischen Spezifität von 100 %. Die Methylierungsanalyse der cfDNA könnte deshalb als sinnvolles Hilfsmittel, ergänzend zur PSA-Bestimmung im Serum, bei der PCa-Frühdiagnose eingesetzt werden. Außerdem legen die Ergebnisse dieser Arbeit nahe, dass die Anzahl der methyliert vorliegenden epigenetischen Biomarker des Panels als prognostischer Parameter sowie zur Verlaufskontrolle und Risiko-Stratifizierung der Tumorerkrankung dienen könnte. Um diese Daten zu bestätigen und das Potenzial der cfDNA-Methylierungsanalyse weiter einschätzen zu können, bedarf es jedoch weiterer Untersuchungen mit größerer Stichprobenanzahl, verbesserter Präanalytik und größeren Probenvolumen.:Abbildungsverzeichnis Tabellenverzeichnis Abkürzungsverzeichnis 1 Einleitung 1.1 Prostatakarzinom 1.2 Benigne Prostatahyperplasie 1.3 Tumor-/Biomarker 1.3.1 Flüssigbiopsie „Liquid biopsy“ 1.3.2 Zirkulierende zellfreie (Tumor-)DNA 1.3.3 Methylierung der cfDNA 1.3.4 Etablierte Tumor-Biomarker – Das Prostataspezifisches Antigen 1.4 Verfahren zu DNA-Methylierungsanalyse 1.4.1 Experimentelle Tumor-Biomaker 1.4.2 State-of-the-Art Methylierungsanalyse-Methoden 1.4.3 OBBPA-ddPCR 1.5 Motivation und Hintergrund 2 Material 2.1 Biologisches Material 2.2 Primer und Sonden 2.3 Chemikalien und Reagenzien 2.4 Puffer und Lösungen 2.5 Kitsysteme 2.6 Laborgeräte 2.7 Software 2.8 Verbrauchsmaterial 3 Methoden 3.1 Biomarker-Recherche 3.2 Primer- und Sondendesign 3.3 Whole genome amplification (WGA) des 0%-DNA-Standards (0%-SD) 3.4 Methyltransferase-Behandlung des 100%-SD 3.5 Aufreinigung der Standards 3.6 Quantitative real-time PCR (qPCR) und Methylation-sensitive high resolution melting (MS-HRM)-PCR 3.7 Agarose-Gelelektrophorese 3.8 Isolierung zellfreier DNA aus Blutproben 3.9 DNA-Konzentrationsbestimmung 3.10 Bisulfitkonversion 3.11 Optimierte Bias-basierte Prä-Amplifikation mit anschließender ddPCR (OBBPA-ddPCR) 3.11.1 Präamplifikation 3.11.2 Droplet Digital PCR (ddPCR) 3.12 Datenanalyse 3.13 Statistische Analyse 4 Ergebnisse 4.1 Ergebnisse der Biomarker-Recherche 4.2 Ergebnisse der qPCR und MS-HRM-PCR 4.2.1 Ermittlung der qPCR TA, TM und Cq-Werte der neuen Marker 4.2.2 Testung der neuen Marker in der MS-HRM-PCR an Serumproben von gesunden Probanden und PCa-Patienten 4.3 Ergebnisse der Primer- und Sondenbedingungen der OBBPA-ddPCR 45 4.3.1 ddPCR-Bedingungen 4.3.2 Präamplifikationsbedingungen 4.4 Ergebnisse der Datenanalyse und Auswertungsoptimierung 4.4.1 Datenanalyse 4.4.2 OBBPA-ddPCR-Bedingungen des Marker-Panels 4.5 Ergebnisse der Blutuntersuchungen 4.5.1 Vergleich der PCa-, BPH- und GM-Kohorten hinsichtlich ihres DNA-Methylierungsanteils 4.5.2 Vergleich der PCa-Subkohorten unterschiedlicher PSA-Wertbereiche hinsichtlich ihres Methylierungsanteils 4.5.3 Vergleich der Marker hinsichtlich ihrer diagnostischen Sensitivität bei 100 %iger diagnostischer Spezifität 4.5.4 Vergleich der diagnostischen Sensitivität der einzelnen Marker und des Marker-Panels hinsichtlich PCa-Proben unterschiedlicher PSA-Konzentrationsbereiche 4.5.5 Vergleich der Optimierungs- und Validierungsprobenserie hinsichtlich ihrer diagnostischen Sensitivität bei einer diagnostischen Spezifität von 100 % 5 Diskussion 5.1 Limitierungen etablierter PCa-Tumormarker 5.2 Suche und Etablierung eines neuen Biomarker-Panels 5.3 Ergebnisse des neu entwickelten Biomarker-Panels 5.3.1 GSTP1 5.3.2 RASSF1A 5.3.3 SOX8 5.3.4 CCDC181 5.3.5 MIR129-2 5.3.6 PAI-1 5.3.7 NRIP3 5.4 Gesamt-Performance des Biomarker-Panels 5.5 Ausblick 6 Zusammenfassung 7 Summary 8 Referenzen 9 Anhang Danksagung Anlage 1: Erklärungen zur Eröffnung des Promotionsverfahrens Anlage 2: Bestätigung über Einhaltung der aktuellen gesetzlichen Vorgaben / Prostate cancer (PCa) is the most common newly diagnosed cancer and the second leading cause of cancer-related deaths among men in Germany. The insufficient diagnostic sensitivity and specificity of established tumor markers, lead to overdiagnosis, resulting in unnecessary prostate biopsies and associated clinical complications. Furthermore, the current PSA-based screening practice cannot reliably distinguish between indolent disease and clinically significant cancer. DNA methylation-based biomarkers have significant potential for clinical laboratory diagnostics, both as tumor-specific biomarkers for early detection or post-therapeutic monitoring of cancer, and as prognostic and predictive biomarkers for therapeutic stratification. This study aimed to develop novel cancer-specific methylation biomarkers using OBBPA-ddPCR-based assays. This new method enables the identification of minute amounts of methylated cell-free tumor DNA amidst a high background of unmethylated wild-type DNA, using a minimally invasive blood sample collection (liquid biopsy). The methylation biomarkers are based on gene sequences that exhibit significant methylation differences between healthy individuals and patients with benign prostatic hyperplasia (BPH) and PCa. The methylation biomarkers RASSF1, SOX8, GSTP1, mir129-2, CCDC181, PAI1, and NRIP3, which demonstrate high diagnostic sensitivity with high diagnostic specificity, were combined into a marker panel. Subsequently, the suitability of this panel as diagnostic tumor marker was validated in an additional series of samples. The optimization and validation sample series consisted of serum samples from 52 healthy individuals, six BPH patients, and 43 PCa patients. The biomarker panel achieved a diagnostic sensitivity of 81.40% with a diagnostic specificity of 100%. Therefore, the methylation analysis of cfDNA could serve as a valuable addition to serum PSA determination in the early diagnosis of prostate cancer. Additionally, the results of this study suggest that the number of hypermethylated epigenetic biomarkers of the selected panel could serve as a prognostic parameter, as well as for disease monitoring and risk stratification. However, further investigation with larger sample sizes, improved pre-analytical procedures, and larger sample volumes is needed to confirm these findings and assess the potential of cfDNA methylation analysis.:Abbildungsverzeichnis Tabellenverzeichnis Abkürzungsverzeichnis 1 Einleitung 1.1 Prostatakarzinom 1.2 Benigne Prostatahyperplasie 1.3 Tumor-/Biomarker 1.3.1 Flüssigbiopsie „Liquid biopsy“ 1.3.2 Zirkulierende zellfreie (Tumor-)DNA 1.3.3 Methylierung der cfDNA 1.3.4 Etablierte Tumor-Biomarker – Das Prostataspezifisches Antigen 1.4 Verfahren zu DNA-Methylierungsanalyse 1.4.1 Experimentelle Tumor-Biomaker 1.4.2 State-of-the-Art Methylierungsanalyse-Methoden 1.4.3 OBBPA-ddPCR 1.5 Motivation und Hintergrund 2 Material 2.1 Biologisches Material 2.2 Primer und Sonden 2.3 Chemikalien und Reagenzien 2.4 Puffer und Lösungen 2.5 Kitsysteme 2.6 Laborgeräte 2.7 Software 2.8 Verbrauchsmaterial 3 Methoden 3.1 Biomarker-Recherche 3.2 Primer- und Sondendesign 3.3 Whole genome amplification (WGA) des 0%-DNA-Standards (0%-SD) 3.4 Methyltransferase-Behandlung des 100%-SD 3.5 Aufreinigung der Standards 3.6 Quantitative real-time PCR (qPCR) und Methylation-sensitive high resolution melting (MS-HRM)-PCR 3.7 Agarose-Gelelektrophorese 3.8 Isolierung zellfreier DNA aus Blutproben 3.9 DNA-Konzentrationsbestimmung 3.10 Bisulfitkonversion 3.11 Optimierte Bias-basierte Prä-Amplifikation mit anschließender ddPCR (OBBPA-ddPCR) 3.11.1 Präamplifikation 3.11.2 Droplet Digital PCR (ddPCR) 3.12 Datenanalyse 3.13 Statistische Analyse 4 Ergebnisse 4.1 Ergebnisse der Biomarker-Recherche 4.2 Ergebnisse der qPCR und MS-HRM-PCR 4.2.1 Ermittlung der qPCR TA, TM und Cq-Werte der neuen Marker 4.2.2 Testung der neuen Marker in der MS-HRM-PCR an Serumproben von gesunden Probanden und PCa-Patienten 4.3 Ergebnisse der Primer- und Sondenbedingungen der OBBPA-ddPCR 45 4.3.1 ddPCR-Bedingungen 4.3.2 Präamplifikationsbedingungen 4.4 Ergebnisse der Datenanalyse und Auswertungsoptimierung 4.4.1 Datenanalyse 4.4.2 OBBPA-ddPCR-Bedingungen des Marker-Panels 4.5 Ergebnisse der Blutuntersuchungen 4.5.1 Vergleich der PCa-, BPH- und GM-Kohorten hinsichtlich ihres DNA-Methylierungsanteils 4.5.2 Vergleich der PCa-Subkohorten unterschiedlicher PSA-Wertbereiche hinsichtlich ihres Methylierungsanteils 4.5.3 Vergleich der Marker hinsichtlich ihrer diagnostischen Sensitivität bei 100 %iger diagnostischer Spezifität 4.5.4 Vergleich der diagnostischen Sensitivität der einzelnen Marker und des Marker-Panels hinsichtlich PCa-Proben unterschiedlicher PSA-Konzentrationsbereiche 4.5.5 Vergleich der Optimierungs- und Validierungsprobenserie hinsichtlich ihrer diagnostischen Sensitivität bei einer diagnostischen Spezifität von 100 % 5 Diskussion 5.1 Limitierungen etablierter PCa-Tumormarker 5.2 Suche und Etablierung eines neuen Biomarker-Panels 5.3 Ergebnisse des neu entwickelten Biomarker-Panels 5.3.1 GSTP1 5.3.2 RASSF1A 5.3.3 SOX8 5.3.4 CCDC181 5.3.5 MIR129-2 5.3.6 PAI-1 5.3.7 NRIP3 5.4 Gesamt-Performance des Biomarker-Panels 5.5 Ausblick 6 Zusammenfassung 7 Summary 8 Referenzen 9 Anhang Danksagung Anlage 1: Erklärungen zur Eröffnung des Promotionsverfahrens Anlage 2: Bestätigung über Einhaltung der aktuellen gesetzlichen Vorgaben

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