Tesis sobre el tema "Human dental tissues"
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Abdullah, Ahmed. "In vitro and in situ studies to investigate the erosion of human dental tissues". Thesis, University of Leeds, 2009. http://etheses.whiterose.ac.uk/11292/.
Texto completoSui, Tan. "Thermal-mechanical behaviour of the hierarchical structure of human dental tissue". Thesis, University of Oxford, 2014. http://ora.ox.ac.uk/objects/uuid:2c8e9604-ec4b-4cfa-b6df-fff3e6579492.
Texto completoMontgomery, Janet. "Lead and strontium isotope compositions of human dental tissues as an indicator of ancient exposure and population dynamics". Thesis, University of Bradford, 2002. http://ethos.bl.uk/OrderDetails.do?uin=uk.bl.ethos.527341.
Texto completoAl-Hazaimeh, Nawaf Ismail. "Revascularization of human dental pulp using tissue engineering approaches". Thesis, University of Leeds, 2012. http://ethos.bl.uk/OrderDetails.do?uin=uk.bl.ethos.582741.
Texto completoFeeney, Robin N. M. "MICROTOMOGRAPHIC ANALYSIS OF SEXUAL DIMORPHISM AND DENTAL TISSUE DISTRIBUTION IN HUMAN MOLARS". The Ohio State University, 2009. http://rave.ohiolink.edu/etdc/view?acc_num=osu1250270343.
Texto completoRizk, Ahmed El Sayed Mahmoud. "Human dental pulp stem cells expressing TGF{221}-3 transgene for cartilage-like tissue engineering". Thesis, The University of Hong Kong (Pokfulam, Hong Kong), 2011. http://hub.hku.hk/bib/B47752890.
Texto completopublished_or_final_version
Dentistry
Doctoral
Doctor of Philosophy
Moretti, Rani da Cunha [UNIFESP]. "Medicação pré-operatória dexametasona – os efeitos na cultura primária de células de polpa dental humana". Universidade Federal de São Paulo (UNIFESP), 2015. http://repositorio.unifesp.br/handle/11600/39323.
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Conselho Nacional de Desenvolvimento Científico e Tecnológico (CNPq)
Fundação de Amparo à Pesquisa do Estado de São Paulo (FAPESP)
Rede Ibero-Americana de Biofabricação
Introdução: A aplicação de dexametasona em cultura de células mesenquimais induz diferenciação osteoblástica, consequentemente formação de tecidos mineralizados. A Engenharia Tecidual propõe o desenvolvimento de estratégias terapêuticas direcionadas à regeneração funcional e estrutural de tecidos biológicos. Nesse sentido, a caracterização celular in vitro é fundamental para garantir o desenvolvimento destas técnicas. Objetivo: Avaliar o efeito da dexametasona administrada como medicação pré-operatória na cultura de células primárias de polpa dental humana. Métodos: Foram utilizadas células provenientes da polpa de terceiros molares. Essas foram distribuídas em dois grupos experimentais com dois protocolos de medicação pré-operatória utilizados em rotina odontológica, onde no protocolo B, o paciente ingeria 1 comprimido de dexametasona 1hora antes à cirurgia e no A não. A avaliação da proliferação, viabilidade e diferenciação, foram pelos testes Trypan Blue, MTT, Von Kossa e Alizarin Red respectivamente, e realizadas em intervalos fixados. Análise de variância de Friedman e t test foram aplicados, fixando em 95% de confiança. Resultados: As células pertencentes ao protocolo A atingiram pico de proliferação aos 21 dias de cultura enquanto as células do protocolo B em 14. Células do protocolo A foram estatisticamente mais viáveis aos 7 e 21 dias enquanto as do protocolo B, aos 14. Na análise de Von Kossa e Alizarin Red observou-se que as células pertencentes ao protocolo B formaram nódulos de calcificação desde 7 dias de cultura enquanto no A aos 14. Conclusão: A utilização da dexametasona como medicação pré-operatória em cirurgia de terceiros molares promove diferenciação celular precocemente, quando observada in vitro.
Introduction: The use of dexamethasone in mesenchymal cell culture induces osteoblastic differentiation and, consequently, formation of mineralized tissues. Tissue Engineering proposes the development of therapeutic strategies aiming at structural and functional regeneration of biological tissues. In this sense, cell characterization in vitro is critical to ensure the development of such techniques. Objective: To evaluate the effect of dexamethasone administered as preoperative medication in primary cell culture of human dental pulp. Methods: We used cells from the third molar pulp. These cells were divided into two experimental groups, each with two preoperative medication protocols used in dental routine and differentiated by the intake of dexamethasone in one of them. The assessment of proliferation, differentiation, and viability through Trypan Blue, MTT and von Kossa, and Alizarin Red tests, respectively, were held in fixed intervals. Friedman analysis of variance and t test were applied, and confidence interval was set at 95%. Results: Protocol A cells proliferation reached its peak on day 21 while protocol B cells proliferation reached its peak on day 14. Protocol A cells were statistically more viable between days 7 and 21 whereas protocol B cells viability was higher on day 14. Von Kossa and Alizarin Red analyses showed that calcified nodules formation occurred from the seventh day of cell culture in protocol B cells and on day 14 in protocol A cells. Conclusion: The use of dexamethasone as preoperative medication in third molar surgery promotes cell differentiation earlier, when observed in vitro.
FAPESP: 07/51227-4
FAPESP: 08/57860-3
CNPq: 573661/2008-1
Pääkkönen, V. (Virve). "Expression profiling of human pulp tissue and odontoblasts in vivo and in vitro". Doctoral thesis, University of Oulu, 2009. http://urn.fi/urn:isbn:9789514290053.
Texto completoMoharamzadeh, Keyvan. "Development of a tissue engineered human oral mucosal model for the assessment of the biocompatibility of resin-based dental materials". Thesis, University of Sheffield, 2006. http://ethos.bl.uk/OrderDetails.do?uin=uk.bl.ethos.485086.
Texto completoTerada, Andrea Sayuri Silveira Dias. "Utilização do produto Allprotect Tissue Reagent® na estabilização do DNA extraído de tecidos dentais humanos em diferentes condições de armazenamento". Universidade de São Paulo, 2013. http://www.teses.usp.br/teses/disponiveis/58/58137/tde-17052013-110504/.
Texto completoThe genetic-molecular methodology stands out as an accurate technique for human identification process and among the sources of biological evidence, the use of teeth is of great interest in Forensic Dentistry. Maintaining integrity of the material sent to laboratory is essential for success of the analysis, and one of the main difficulties is related to sample storage, which is usually carried out at low temperatures. This study evaluated the effectiveness of the Allprotect Tissue Reagent® (Qiagen, Hilden, Germany) in stabilizing DNA extracted from human dental tissues stored under different conditions. In this study were used 165 teeth, distributed in two groups: intact teeth and isolated pulp tissue. The samples were stored with or without the product and varying the storage time (1, 7, 30 and 180 days) and temperature (room temperature and under refrigeration). In addition to these groups, was formed a positive control group, composed by five teeth, which was stored at -20ºC for 180 days. After storage, DNA extraction, electrophoresis on agarose gel and genomic DNA quantification by Real-Time PCR and fragments of 37 samples were performed. The fragments of 32 samples representing every possible condition and five positive control group samples were analyzed to verify four pre-selected markers. The agarose gel showed evidences of genomic DNA presence. Quantification results were statistically analyzed with the tests Kruscal-Wallis and Mann-Whitney. Quantification results showed values ranging from 0.01 to 10,246.88 ng/L of DNA. There was a decrease in DNA concentration in stored tooth samples at room temperature for 30 and 180 days compared to those stored for 1 and 7 days. Besides the time factor, temperature also influenced the DNA concentration, being higher in teeth that remained for 30 days and in tooth pulp maintained for 180 days, under refrigeration. Regarding the use of Allprotect Tissue Reagent® (Qiagen, Hilden, Germany) it showed a significant difference in stabilization of stored teeth at room temperature for 30 and 180 days. The analysis of fragments was possible in 37 selected samples, regardless of the DNA quantity variation, confirming that amplification reactions and STR analysis using automated methods provides good results. It was concluded that the use of Allprotect Tissue Reagent® (Qiagen, Hilden, Germany) showed a significant difference in stabilizing DNA samples of intact human teeth stored at room temperature for 30 and 180 days, while in the other test conditions the results showed no justification for using this product.
Zimmerman, Heather. "Preliminary Validation of Handheld X-Ray Fluorescence (HHXRF) Spectrometry: Distinguishing Osseous and Dental Tissue from Non-Bone Material of Similar Chemical Composition". Master's thesis, University of Central Florida, 2013. http://digital.library.ucf.edu/cdm/ref/collection/ETD/id/5895.
Texto completoM.A.
Masters
Anthropology
Sciences
Anthropology
Vernon, Lauren Louise. "A Comparison of the Osteogenic Tissue Engineering Potential of Dental-Derived Stem Cell Lines: Stem Cells from Human Exfoliated Deciduous Teeth (SHEDs) vs. Periodontal Ligament Stem Cells (PERIOS)". Scholarly Repository, 2010. http://scholarlyrepository.miami.edu/oa_theses/19.
Texto completoMaluf, Paulo Sérgio Zaidan [UNIFESP]. "Torque na instalação de implantes dentais pós-transplante de fíbula microvascularizado". Universidade Federal de São Paulo (UNIFESP), 2011. http://repositorio.unifesp.br/handle/11600/10118.
Texto completoINTRODUÇÃO: A reabilitação mastigatória com implantes dentais tornou-se, atualmente, uma terapêutica comum e necessária para pacientes edêntulos. Técnicas em implantodontia são aperfeiçoadas constantemente, dentre as quais o torque, para fixação dos cilindros de titânio em osso, considerado fundamental no prognóstico de sucesso da osteointegração. A reconstrução com retalhos microcirúrgicos, em ossos da face, tem sido cada vez mais realizadas em pacientes para reparação de sequelas pós-cirúrgicas. Para a completa reabilitação funcional desses pacientes é necessária a instalação de implantes osseointegráveis para o suporte de próteses dentais, mas inexistem pesquisas que determinem o torque necessário para estabilização inicial, desses implantes, em transplantes ósseos revascularizados. OBJETIVO: Mensurar o torque na instalação de implantes de titânio, em transplante de fíbula microrrevascularizado e consolidado, para reconstrução de maxila e mandíbula. MÉTODOS: Foram instalados 28 implantes dentais, em sete pacientes, com reconstrução cirúrgica em maxila e mandíbula por retalhos microcirúrgicos. No momento da instalação dos implantes mensurou-se o torque para estabilização final, cujos dados foram tabulados e analisados. RESULTADOS: O torque mínimo para instalação dos implantes foi de 20Ncm em 39,3% dos implantes, e o máximo de 45Ncm em 28,5%. CONCLUSÃO: A medida do torque no implante de titânio em transplante de fíbula microrrevascularizado, para reconstrução maxilomandibular, variou de 20 a 45Ncm, não tendo sido observada nenhuma influência relativamente ao gênero, à faixa etária e ao tempo de transplante.
INTRODUCTION: The masticatory rehabilitation with dental implants has become, a therapeutic technique for edentulous patients. Techniques in dental implant are constantly perfected, as the torque to fix the cylinders in a bone, considered fundamental in the prognosis of success in bone integration. The reconstruction with microsurgical flaps, in facial bones, has been increasingly performed in patients to repair the post-surgical sequelae. For the complete functional rehabilitation of these patients, the installation of bone integrable implants is necessary. With the objective of supporting the dental prosthesis, but there are no studies that determine the necessary torque to the initial stabilization of these dental implants in bone revascularized transplants. OBJECTIVE: To measure torque in installation of titanium implants, fibula microrevascularized and consolidated, in reconstruction of maxilla and mandibula. METHODS: Twenty eight dental implants were installed in seven patients with surgical reconstructions in the maxila and mandibular by microsurgical flaps. At the time of the installation of the implants, torque for final stabilization was measured, whose data were tabulated and analyzed. RESULTS: The minimum torque for installation of the implants was of 20Ncm in 39,3% of the implants, and the maximum, of 45Ncm in 28,5%. CONCLUSION: The measure of torque in implants of titanium of fibula microrevascularized transplants, for maxilomandibular reconstruction, varied from 20 to 45Ncm, and no influence related to gender, to age group or to time of transplant has been observed.
TEDE
Palosaari, H. (Heidi). "Matrix metalloproteinases (MMPs) and their specific tissue inhibitors (TIMPs) in mature human odontoblasts and pulp tissue:the regulation of expressions of fibrillar collagens, MMPs and TIMPs by growth factors, transforming growth factor-β1 (TGF-β1) and bone morphogenetic protein-2 (BMP-2)". Doctoral thesis, University of Oulu, 2003. http://urn.fi/urn:isbn:9514270789.
Texto completoCasagrande, Luciano. "Aplicação de princípios de engenharia tecidual no estudo da diferenciação de células-tronco pulpares". reponame:Biblioteca Digital de Teses e Dissertações da UFRGS, 2008. http://hdl.handle.net/10183/13251.
Texto completoThe effect of dentin pre-treatments and dentin-derived BMPs on SHED differentiation was tested using the Tooth-Slice Scaffold model (TSS). Dentin slices (1mm thickness) were prepared from extracted human third molars. Biodegradable PLLA scaffolds were prepared inside the pulp chamber of the tooth-slices, treated alternatively with a 5.25% NaOCl or 10% EDTA solution, or remaining untreated (WO-T). PLLA sponge scaffolds with no tooth-slice (PSS) were used as control. SHED (5x104) were seeded in TSS and PSS and after 7, 14, 21 and 28 days in culture, RT-PCR (DSPP, DMP1 and MEPE) and WST-1 proliferation assay were performed. Additionally, cells (5x105) were seeded in TSS and PSS and transplanted into SCID mice (14 and 28 days). To verify the dentinderived BMPs bioactivity, SHED (5x104) were cultured in TSS in the presence of antihuman BMP-2, -4, and -7 antibodies for 14 days. Besides, cells in culture were treated with rhBMP-2; -4; or -7 for 24 hours. After in vitro and in vivo time course, SHED altered their genetic expression. The cells cultured in vitro in the TSS (EDTA or WO-T) expressed the differentiation markers after 14 days and maintained expression thereafter. Cell proliferation rate was reduced following the differentiation (p<0.05). Cells transplanted in vivo expressed DSPP, DMP-1 and MEPE after 28 days (EDTA). No transcripts were found in tooth-slices treated with NaOCl or in PSS groups. BMP-2/4Ab prevented the differentiation process and no inhibitory effect was detected for BMP-7Ab. After 24 hours, expression of DSPP, DMP-1 and MEPE was found for rhBMP-2, and DSPP and DMP-1 for rhBMP-4 and rhBMP-7 treated SHED, but not for untreated cells. The tooth slice scaffold model suggests that dentin can provide the environment for SHED differentiation and dentin-derived morphogenic signals BMP-2 and BMP-4 play an important role in this process.
Le, Luyer Mona. "Évolution dentaire dans les populations humaines de la fin du Pléistocène et du début de l’Holocène (19000 – 5500 cal. BP) : une approche intégrée des structures externe et interne des couronnes pour le Bassin aquitain et ses marges". Thesis, Bordeaux, 2016. http://www.theses.fr/2016BORD0003/document.
Texto completoSince the Late Pleistocene, a reduction in size and a morphological simplification of human teeth have been observed and arguably linked to cultural and environmental changes. Following new discoveries along with the revision of key archaeological contexts, a re-assessment of the nature of crown variations on more than 1900 teeth is proposed for 176 Late Paleolithic, Mesolithic and Early Neolithic individuals from the Aquitaine Basin and its margins. In particular, a non-invasive assessment of internal tooth structure variability (enamel thickness, dental tissue proportions, enamel-dentine junction morphology) has been performed using 3D imaging methods (microtomography) and geometric morphometrics in order to characterize and interpret dental evolution from a whole crown perspective. Results from the morphometric analyses show a discontinuity between Late Pleistocene and Early Holocene populations. External dimensions, enamel thicknesses and tissue proportions are reduced in Mesolithic individuals compared to those of the Late Paleolithic, while major differences are observed in occlusal wear patterns and enamel distribution between Mesolithic and Early Neolithic samples. These data suggest that environmentally-driven modifications during the Early Holocene had a major impact on dental reduction in human populations and that Neolithic cultural changes had mostly affected enamel distribution. Finally, a correlation between occlusal wear pattern and enamel thickness distribution is observed and associated with dietary changes. In particular, enamel thickness may have rapidly evolved as a selective response to functional changes in masticatory biomechanics
Pedroni, Ana Clara Fagundes. "Efeito da Laserfototerapia associada ou não à Vitamina C na indução de membranas celulares (cell sheets) de células-tronco da polpa dentária humana". Universidade de São Paulo, 2016. http://www.teses.usp.br/teses/disponiveis/23/23134/tde-03082016-112215/.
Texto completoCell Sheets, consisting of stem cells (SCs) are self detachable from the cultivation plate, and with no subcultivation can generate large amount of cells. The cell sheets can be transplanted closer to cell physiology environment by keeping the cell connections and the extracellular matrix produced in culture. Ascorbic acid or Vitamin C (VC) has inductive effect on cell sheet formation, increasing the longevity and the stemness of the cell for long period of time. The similarity between biological responses of VC in cell sheets and those of Laserphototherapy (LPT, Laser) on cells and tissues led us to hypothesize that these therapies could improve the prognosis of future clinical application of these cell sheets in regeneration of dental tissues. To test this hypothesis, LPT and VC were applied, associated or not, to induce human dental pulp stem cells (hDPSCs). Therefore, hDPSCs, which expressed typical levels of mesenchymal stem cell surface markers, were plated in 6-well plates (5x104 cells per well). Twenty-four hours later they were subjected to the treatment of experimental groups: Control: hDPSCs in P3 cultured with regular medium; Senescent: hDPSCs in P27 cultured with regular medium; VC: P3 cultured with regular medium supplemented with VC (20 ?g/ml); Laser: P3 cultures with regular medium and submitted to LPT (punctual and contact mode-5 points / well, 660 nm, 20 mW, 0.028 cm², 0.71 W/cm², 7 sec, 5 J/cm², 0.14 J per point, 48 hours-intervals) and Laser+VC: P3 cultured with regular medium supplemented with VC and submitted to LPT Within 24 hours, 7 and 13 days the hDPSCs of the different experimental groups were observed macroscopically and microscopically, and the telomerase enzyme activity was assessed by PCR-TRAP, complemented by ELISA. To evaluate the expression of genes related to the nature and differentiation (Mitofilina and Oct 4), longevity (catalytic phase of telomerase-hTERT enzyme), and the senescence of the senescent group cells (?-galactosidase), the hDPSCs of all experimental groups were subjected to RT-qPCR. The RT-qPCR data were compared by ANOVA complemented by the Tukey\'s test (p <= 0.05). The hDPSCs were able to form cell sheets only in the VC and Laser+VC groups (100%). Additionally, the cell sheets of the Laser+VC group presented easier handling. Telomerase activity in hDPSCs was observed only in 24 hours (Control and Laser) and seven days (VC and Laser + VC). The undifferentiating marker (Oct 4) and mesenchymal marker (mitofilin), as well as hTERT were expressed in hDPSCs of all experimental groups. Oct4 and hTERT presented expressions significantly higher at 7 days in VC and Laser+VC groups than in all other groups (p < 0.0001, p = 0.0009, respectively). The expression of mitofilin was significantly higher in the Laser+VC group, in 7 days (p = 0.0338). The technique of obtaining cell sheets of hDPSCs by the methodology here presented was considered appropriate to be further tested in regenerative procedures. The LPT when combined with VC did not interfere with the formation of the cell sheets, neither in the maintenance of longevity and undifferentiating status of hDPSCs. Moreover, LPT improved the handling of the cell sheets. Thus, the association of VC and LPT in the induction of cell sheets seems promising for future use in regenerative dentistry.
Neto, Eduardo Felippe Duailibi. "Desenvolvimento de metodologia radiográfica e volumétrica dos diferentes estágios de desenvolvimento dentário para qualificação de material biológico em Engenharia Tecidual". Universidade de São Paulo, 2013. http://www.teses.usp.br/teses/disponiveis/23/23139/tde-28052013-194243/.
Texto completoThe usage of human dental stem cells and tissue engineering technics represents a huge tecnological development and it may benefits many patients in a promissing future. The discovery of suitable source of human dental stem cells were made using tooth buds. Duailibi et al. 2011 indicated a new tooth classification on a stem cell harvesting based research, sugesting new methods for diagnosis these stages. Several method were developed for dental age assesement. The presente study aims to evaluate some of these dental age technics and make adaptations for estimating Duailibi et al. 2011 tooth stages. A 67 tooth sample previoulsy classificated by Duailbi et al. 2011 were submited through periapical parallel long cone X-rays and CBCT analysis. Age estimation ratio methods were applied by measuring tooth/root lenth, crown/root lenth, tooth/pulp lenth, crown/pulp lenth, tooth/poulp área and tooth/pulp volume. Results indicated by linear regression analisys a R2 value of tooth/pulp lenth 0,14050; crown/pulp lenth 0,65369; crown/root lenth 0,5408; tooth/root lenth 0,54074; pulp/tooth volume 0,23925; e tooth/pulp volume de 0,08553, with p value of 0,005. In conclusion , the best method for estimating Duailibi et al. 2011 tooth classification techinic is made by using periapical long cone X-rays using crown/pulp lenth ratio.
Nicola, Fabrício do Couto. "Efeito neuroprotetor do transplante de células-tronco mesenquimais derivadas de dente decíduo humano em ratos Wistar submetidos à lesão medular". reponame:Biblioteca Digital de Teses e Dissertações da UFRGS, 2017. http://hdl.handle.net/10183/170284.
Texto completoSpinal cord injury (SCI) is a disabling condition that results in sensory and motor deficits. The estimated annual incidence in Brazil is of 30 new cases of spinal cord injury per 1 million of individuals; unfortunately SCI remains without an effective treatment. Stem cells from human exfoliated deciduous teeth (SHED) are one among potential sources of stem cells for transplantation after spinal cord injury in order to promote protection or tissue and functional recovery after spinal cord injury. The aim of this Thesis was to evaluate the effects of stem cells from human exfoliated deciduous teeth (SHED) transplantation, one hour after lesion, in the acute, subacute and chronic phases on neuroprotection, tissue protection and functional recovery in Wistar rats submitted to spinal cord injury by contusion The main goals were: a) to investigate the effects of SHED transplantation on functional recovery, lesion volume, and neuronal death; b) to verify the effects of the transplantation on the progenitor cells number, glial scar formation and astrocytic modifications after spinal cord contusion. Improvement of functional recovery, reduction of lesion volume and neuronal death were observed in the spinal cord of animals submitted to spinal cord injury and SHED transplantation. SHEDs increased the number of precursor cells in the spinal cord in the subacute period, reduced the expression of glial fibrillary acidic protein (GFAP) and increased the expression of the potassium influx rectifier channel 4.1, both astrocyte proteins. We conclude that transplantation of stem cells from human exfoliated deciduous teeth after spinal cord injury promotes functional recovery from the neuroprotection effect, which starts in the acute phase and is confirmed six weeks after the contusion with a higher number of motor neurons in the ventral horn of spinal cord. SHEDs are able to increase the number of precursor cells and produce astrocyte modifications in the spinal cord of injured rats in the subacute phase, reducing glial scar formation.
Domínguez, Santamaría Juan Mario. "Importancia de la relación de ayuda en la entrevista familiar de donación de órganos de fallecidos: una perspectiva de los profesionales sanitarios". Doctoral thesis, Universidad de Alicante, 2011. http://hdl.handle.net/10045/23521.
Texto completoOxilia, Gregorio. "Human dental tissues: Advancement in virtual dental analysis". Doctoral thesis, 2018. http://hdl.handle.net/2158/1119840.
Texto completoBeaumont, Julia, Andrew R. Gledhill, Julia A. Lee-Thorp y Janet Montgomery. "Childhood diet: a closer examination of the evidence from dental tissues using stable isotope analysis of incremental human dentine". 2013. http://hdl.handle.net/10454/5636.
Texto completoIncremental dentine analysis utilizes tissue that does not remodel and that permits comparison, at the same age, of those who survived infancy with those who did not at high temporal resolution. Here, we present a pilot study of teeth from a 19th-century cemetery in London, comparing the merits of two methods of obtaining dentine increments for subsequent isotope determination. Covariation in ¿13C and ¿15N values suggests that even small variations have a physiological basis. We show that high-resolution intra-dentine isotope profiles can pinpoint short-duration events such as dietary change or nutritional deprivation in the juvenile years of life.
Cardona, Dayana Elisa Jacinto Baptista de. "Análise macroscópica e radiográfica de tecidos e materiais dentários sujeitos a altas temperaturas". Master's thesis, 2018. http://hdl.handle.net/10400.14/26080.
Texto completoIn forensic situations involving exposure to high temperatures, in particular by the action of fire, a significant destruction of the cadaver occurs. The characterization of the mineralized tissues and dental restoration materials becomes particularly important in these cases, as it correlates with the temperature to which the corpse was exposed. In extreme situations of high temperature dental identification may be impossible, especially when a complete destruction of the tooth occurs or when ante mortem clinical records are nonexistent. Preferentially, we should proceed with the analysis of the teeth, taking into account their excellence in terms of preservation. Objectives: To observe the macro-structural and radiographic changes of the dental tissues and dental restoration materials used at present, when subjected to different temperatures. Checked the capacity of the observed alterations being used at the level of forensic identification, jointly in cases of cadavers burned, cribbed or incinerated. Materials and methods: An in vitro experimental study was carried out to observe the macroscopic and radiographic physical changes of the dental tissues and some dental materials. The protocol involved wrapped 36 human teeth divided into 3 groups, of 12 teeth restored with amalgam, composite resin and glass ionomer, these teeth were subjected to 3 temperature ranges (600 ° C, 900 ° C and 1100 ° C) which correspond to teeth for each propustate temperature. Results: The tissues and dentinal materials studied in this research present great resistance at high temperatures without significantly varying their macrostructure, so that physical changes (dimensional stability, cracks, cracks, fractures, texture, color, carbonization and incineration) can get to identify and associate with each specific temperature range. Conclusion: The tissues and dental materials present great resistance in action of high temperatures. In the same way, they present specific changes (color, texture, fissures, cracks, fractures and fragmentation) that can contribute to the process of identifying a corpse or human remains burned, incinerated or charred.
Baker, Ryan William. "Effects of DynaMatrix® Membrane on Angiogenic Cytokine Expression From Human Dental Pulp Stem Cells". Thesis, 2013. http://hdl.handle.net/1805/3718.
Texto completoThe aim of this current study was to determine if the exposure of human dental pulp stem cells (HDPSC) to the DynaMatrix membrane will result in an increased production of angiogenic cytokines that are critical for pulp/root regeneration. Angiogenesis cytokine arrays have been established as a viable method for assessing expression of cytokines.20 HDPSC were chosen as they are expected to be found in the apical papilla and the infected immature root canal system of teeth that current regenerative endodontic techniques are designed to treat.
Al-Mosawi, M., G. R. Davis, A. Bushby, J. Montgomery, Julia Beaumont y M. Al-Jawad. "Crystallographic texture and mineral concentration quantification of developing and mature human incisal enamel". 2018. http://hdl.handle.net/10454/16576.
Texto completoFor dental human enamel, what is the precise mineralization progression spatially and the precise timings of mineralization? This is an important question in the fundamental understanding of matrix-mediated biomineralization events, but in particular because we can use our understanding of this natural tissue growth in humans to develop biomimetic approaches to repair and replace lost enamel tissue. It is important to understand human tissues in particular since different species have quite distinct spatial and temporal progression of mineralization. In this study, five human central incisors at different stages of enamel maturation/mineralization were spatially mapped using synchrotron X-ray diffraction and X-ray microtomography techniques. From the earliest developmental stage, two crystallite-orientation populations coexist with angular separations between the crystallite populations averaging approximately 40o and varying as a function of position with the tooth crown. In general, population one had significantly lower texture magnitude and contributed a higher percentage to the overall crystalline structure, compared to population two which only contributed 20-30% but had significantly higher texture magnitude. This quantitative analysis allows us to understand the complex and co-operative structure-function relationship between two populations of crystallites within human enamel. There was an increase in the mineral concentration from the enamel-dentin junction peripherally and from the incisal tip cervically as a function of maturation time. Quantitative backscattered-electron analyses revealed that mineralization of prism cores precedes that of prism boundaries. These results provide new insights into the precise understanding of the natural growth of human enamel.
Partly funded by NERC grant ”Timelines in Teeth” NE/F018096/2.
Masumbuko, Kahamba Nyota. "Isolation, culture and neurogenic differentiation of human dental stem cells". Thesis, 2016. http://hdl.handle.net/10539/21593.
Texto completoDental stem cells (DSCs) have been identified in teeth and their supporting tissues. They represent an exclusive source of adult stem cells, easily isolated and manipulated for tissue repair and regeneration. This research project evaluated the neurogenic potential of the dental pulp stem cells (DPSCs) and stem cells from the pulp of human exfoliated deciduous teeth (SHEDs) in a South African cohort. Sixty non-carious permanent and deciduous teeth were extracted from healthy patients aged between 18 and 30 years and 5 and 10 years, at the University of the Witwatersrand's Oral Health Clinic in Johannesburg Charlotte Maxeke Academic Hospital, South Africa. The cells, isolated from the extracted pulp tissue were cultured, counted and then phenotyped by flow cytometry analysis. The cells were further expanded in a neural induction medium and immunocytochemistry analysis for Ki-67, doublecortin (DCX) and nestin were performed. Large colonies of both DPSCs and SHEDS were harvested from the extracted pulp tissues and positively cultured. Flow cytometry analysis confirmed the presence of CD44+ and CD29+ cells as well as the known mesenchymal stem cell markers CD90 and CD105. Both DPSCs and SHEDs demonstrated successful proliferation and neural differentiation. This study confirmed that DPSCs and SHEDs are highly proliferative human adult stem cells that exhibit a neurogenic potential that may contribute in the treatment of neurological disorders.
AC2017
Adams, Joseph Benjamin. "Effects of DynaMatrix® on angiogenic cytokine expression from human dental pulp fibroblasts : an in vitro study". Thesis, 2015. http://hdl.handle.net/1805/6494.
Texto completoEFFECTS OF DYNAMATRIX® ON ANGIOGENIC CYTOKINE EXPRESSION FROM HUMAN DENTAL PULP FIBROBLASTS: AN IN VITRO STUDY by Joseph Benjamin Adams Indiana University School of Dentistry Indianapolis, IN Introduction: An exogenous scaffold may lead to more predictable pulp tissue regeneration and continued root formation in a regenerative endodontic procedure. DynaMatrix® is a natural membrane scaffold made of porcine small intestine, currently used in periodontal regenerative surgeries. Objective: The purpose of this study was to investigate if human dental pulp fibroblasts (HDPFs) seeded on DynaMatrix® membrane would result in an increase in the expression of angiogenic cytokines. Materials and Methods: HDPFs (75,000 per well) were seeded in 6-well plates. Three groups were tested: Group 1 (C): HDPFs in 70 media only; Group 2 (M): DynaMatrix® (Cook Biotech, Indianapolis, IN) alone in media; and Group 3 (C+M): HDPFs seeded on DynaMatrix® membranes. After 72 hours of incubation in serum positive, the conditioned media were collected and analyzed for the expression of 20 angiogenic cytokines utilizing RayBiotech Inc., arrays per the manufacturer’s instruction. The data were analyzed by ANOVA. Results: Group M was significantly higher than C for bFGF (p = 0.0023). C+M was significantly higher than M for ANG (p = 0.0104); GRO (p = 0.0003); IFN-γ (p = 0.0023); IL-6 (p = 0.0003); IL-8 (p = 0.0003); Leptin (p = 0.0003); MCP-1 (p = 0.0104); TIMP-1 (p = 0.0190); TIMP-2 (0.0123). C was significantly higher than C+M for ANG (p = 0.0104); MCP-1 (p = 0.0104); and THPO (p = 0.0308). Cytokines such as b-FGF, ANG, and leptin promote angiogenesis, and stimulate migration and proliferation of cells. Conclusion: The cytokine expression profile from the cells seeded on DynaMatrix® suggests that it might be a suitable scaffold for regenerative endodontic procedures. It could improve vascularization by increasing angiogenic cytokines in the microenvironment of the treated root canal and supporting tissue regeneration.
Macho, Gabriele A., D. Shimizu y I. R. Spears. "The effect of prism orientation and loading direction on contact stresses in prismatic enamel: implications for interpreting wear patterns". 2005. http://hdl.handle.net/10454/3551.
Texto completoThe ability of prisms to effectively dissipate contact stress at the surface will influence wear rates in teeth. The aim of this investigation was to begin to quantify the effect of prism orientation on surface stresses. Seven finite element models of enamel microstructure were created, each model differing in the angulation of prism orientation with regard to the wear surface. For validation purposes, the mechanical behavior of the model was compared with published experimental data. In order to test the enamel under lateral loads, a compressed food particle was dragged across the surface from the dentino-enamel junction (DEJ) towards the outer enamel surface (OES). Under these conditions, tensile stresses in the enamel model increased with increases in the coefficient of friction. More importantly, stresses were found to be lowest in models in which the prisms approach the surface at lower angles (i.e., more obliquely cut prisms), and highest when the prisms approached the surface at 60° (i.e., less obliquely cut). Finally, the direction of travel of the simulated food particle was reversed, allowing comparison of the difference in behavior between trailing and leading edge enamels (i.e., when the food particle was dragged either towards or away from the DEJ). Stresses at the trailing edge were usually lower than stresses at the leading edge. Taken together with what is known about prism orientation in primate teeth, such findings imply greater wear resistance at the intercuspal region and less wear resistance at the lateral enamel at midcrown. Such findings appear to be supported by archeological evidence.
Nirmalasari, Putu Risti y 李思媞. "The Effects of Natural Teeth with Different Interface Tissue around Implant towards Significant Direction of Resonance Frequency Vibration of Dental Implant on Human Mandible by Resonance Frequency Analysis". Thesis, 2017. http://ndltd.ncl.edu.tw/handle/qfg5k7.
Texto completo國立中央大學
機械工程學系
105
Abstract The work within this thesis investigates the significant direction of resonance frequency for osseointegration assessment. The significant directions of resonance frequencies give information to support the resonance frequency analysis. This study discusses about the influence of natural teeth and interface tissue as the structures around dental implantation to the resonance frequencies. The analysis performed in numerical by using modal analysis and harmonic response analysis from ANSYS Workbench Software Inc. Modal analysis determine the natural frequencies and mode shapes of a structure, whereas harmonic response analysis determine the resonance frequencies spectrum. After the highest resonance frequency obtained on the spectrum, it plotted into the radar graph and see the direction trend line in certain mandible models. The analysis based on the theories of dynamic structure by using finite element method. The analysis of cantilever beam and artificial bone block were performed as an initial analysis to explain phenomena that occur in the main case (mandible models). Cantilever beam used two different types of cross-sections, circular and rectangular. The resonance frequency results of circular cross-section were all the same in different excitation directions, vice versa for rectangular cross-section. Artificial bone block was modeled with cortical thickness without-interface tissue, 2mm. The resonance frequency value in buccal-lingual (BL) direction is higher than mesial-distal (MD) direction. The other artificial bone blocks were modeled in two different conditions of interface tissue with cortical thickness, 1mm. The result showed that the behavior of a physical structure without-interface tissue is stiffer than with-interface tissue but the mode shapes remain the same. In this thesis, the mandible was varied into three different models, based on position of teeth beside implant structure with different interface tissue stiffness. Model-1 was mandible with teeth beside implant structure; Model-2 was mandible without teeth beside implant structure; Model-3 was the mandible with teeth only on one side of implant structure. Interface tissue was varied into three different values of Young’s modulus (2, 25, 137 MPa) and it applied on each mandible models. The result showed the lower stiffness (2MPa) had almost the same resonance frequency in every direction, vice versa for higher stiffness (25, 137MPa) which had a significant direction in different excitation load directions. Keywords: significant direction, resonance frequencies (RFs), mode shape, resonance frequency analysis (RFA), finite element analysis (FEA).