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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

The Development of a Human Operator Informatic Model (HOIM) incorporating the Effects of Non-Invasive Brain Stimulation on Information Processing while performing Multi-Attribute Task Battery (MATB)

Nelson, Justin 02 May 2016 (has links)
No description available.
12

The Role of Interleukin-2 in Directing Vascular Smooth Muscle Cell Function and its Implications for Understanding the Progression of Atherosclerosis

Arumugam, Prakash 30 August 2016 (has links)
No description available.
13

MULTICEULLULAR TUMOR HEMI-SPHEROID: A NOVEL IN VITRO 3D MODEL PLATFORM FOR ACCELERATED DRUG DEVELOPMENT

Kim, Kihwan 08 February 2017 (has links)
No description available.
14

Development of Cell-based Therapies for Ischemic Stroke and Type I Diabetes using Nanotechnology-based Cell Reprogramming

Lemmerman, Luke Roger 05 October 2022 (has links)
No description available.
15

IN-PIXEL TIME DIGITAL CONVERTER FOR TIME-OF-FLIGHT PET IMAGING

Nemati, Hosseinabadi Ebrahim 10 1900 (has links)
<p>In the past decades, great advances in biomedical imaging towards using less invasive and more sensitive imaging modalities have enabled early detection of diseases through timely diagnosis of patients. Positron emission tomography (PET) imaging, as one of the recent imaging technologies, provides imaging from cellular-level metabolic changes in tissues. This gives PET imaging a substantial lead in detecting disease in their very early stages. PET imaging provides high sensitivity and chemical specificity. However, it suffers from low resolution compared to other imaging methods. Time of Flight (ToF) PET imaging, one of the derivations of the PET, improves the imaging by exactly determining the position of the annihilation event using a time digital converter (TDC). By achieving the timing information of the incident anti-parallel photons coming from an event in ToF PET scanner, the TDC helps to determine the exact location of the event. So, it increases the resolution of the PET scanner.</p> <p>A ToF PET custom-designed TDC has been proposed in this work. The designed TDC offers relatively high resolution and dynamic range (DR) to satisfy some PET imaging specifications. To increase the sensitivity and reduce the noise and latency, in-pixel design of TDC is desired. Therefore, a time digital converter that is specifically designed for ToF PET should follow a strict set of criteria in its design procedure. A three-staged hierarchical TDC was designed and implemented in 0.13μm standard CMOS technology to reduce the total number of delay elements for this area limitation issue. Also, a novel half-CLK period interpolation idea was proposed to reduce the total size of the TDC even more. A counter and half-CLK counter construct the coarse stage of the TDC. A delay locked loop (DLL) works as the first fine interpolator, while, the Vernier delay line (VDL) acts as the second fine interpolation stage.</p> <p>A high resolution of 39ps was achieved with a relatively high DR of 1.28μs and the measured DNL and INL of 0.2T<sub>LSB</sub> and 0.4T<sub>LSB</sub>. Due to all area reduction techniques used, the final designed TDC measures for 0.11 mm<sup>2</sup>, which is much smaller than other similar TDCs with the same resolution and DR. As the amount of delay in the delay elements in the TDC are susceptible to any change in the environmental changes, a delay locking method was used to compensate for process, voltage and temperature (PVT) variations. <strong><br /> </strong></p>
16

The Tissue Response to Infectious Burden and Implantable Devices in Healthy and Diabetic Animal Models

Brown, Nga Le January 2015 (has links)
<p>Performance of biomedical implants has been hindered by fibrosis, infection, and deficient tissue integration due in part to the body's foreign body response. In addition, diabetes mellitus is affecting a greater number of people worldwide and in the United States. As the percentage of the population affected by diabetes increases, a larger fraction of these implanted devices will be placed in diabetic patients. Unfortunately, diabetes is often complicated by poor wound healing and a greater risk of infection, issues that could adversely affect proper acceptance of an implant. Diabetic animal models are useful in studying the response to infection as well as the tissue response to an implanted device. Therapies such as nitric oxide release have been applied to indwelling devices to mediate the foreign body response and improve the wound healing response around implants. Particularly relevant to diabetic patients are implantable glucose sensors, and so determining the diabetic tissue response to these devices is crucial to improving their lifetime and performance. </p><p>A novel outcome-based streptozotocin dosing regimen was developed to induce Type 1 diabetes in a rodent model. Male CD (Sprague-Dawley type) rats weighing 150-200 g were given three consecutive daily doses of 40 mg/kg streptozotocin (STZ) on Days 1, 2, and 3. On Day 5, tail vein blood glucose was checked. If blood glucose was not within the target diabetic range of 350-600 mg/dl, rats received an additional dose of STZ. This procedure was repeated every 48 hours until all rats achieved target hyperglycemia. Control rats were given similar doses of vehicle (saline/citrate), which had no effect on blood glucose. After the last injection of streptozotocin, two weeks were allowed to ensure the full effects of the diabetic state would be present at device implantation. Blood glucose was measured every 2 days for diabetics and 4 days for controls for the duration of the experiment. The developed diabetic model resulted in a stable hyperglycemia for the duration of the experiment (in some cases, up to 2 months). Animals also exhibited typical symptoms of diabetes, such as minimal changes in weight, excessive thirst, and polyuria.</p><p>Infection response in the presence of implanted devices was investigated in healthy and diabetic animal models. In the healthy animal model, control stainless steel compression plates and plates coated with a nitric-oxide releasing xerogel (20% AHAP) were attached to the femurs of 12 adult rabbits. Both femurs were inoculated with 3x106 CFU MSSA (methicillin-sensitive Staph aureus) for a period of 20 minutes before the surgical sites were sutured. After 7 days, the wound, device, and a portion of bone were cultured. A muscle biopsy was removed and homogenized to quantify bacterial infection. Since the microbiologic data were not normally distributed, they were compared using an unpaired Wilcoxon Rank Sum Test. No significant differences in bacterial burden were observed between the control and NO-eluting devices, however the study did find a high correlation of temperature of the adjacent muscle at implantation with the ensuing bacterial content. In the diabetic animal model, a novel dosing regimen of streptozotocin based on a target blood glucose of 350-600 mg/dl was used to induce type-1 diabetes. Stable hyperglycemia was maintained for 21 days. Two weeks after achieving the target hyperglycemia, stainless steel fracture plates were secured to each femur with stainless steel screws approximately 3 mm in length. The implant site on the right side of the animal was inoculated with 3 x 107 CFU of methicillin-sensitive S. aureus while the left side served as a control. After seven days, quantitative bacterial count was performed at explantation and no cross-over of bacteria was detected from the inoculated side to the non-inoculated side. Infection after S aureus inoculation in the presence of an implanted device was significantly higher in diabetic animals when compared to that of control animals (p = 0.0003, Wilcoxin Rank-Sum Test) supporting the hypothesis that diabetes adversely affects the ability to fight infection in the presence of an indwelling device in an animal model. There was not a significant difference detected in the infectious burden for the non-inoculated limb (left) between the diabetic and non-diabetic groups when compared using a Wilcoxon Rank-Sum Test (p = 0.0682), however this near-significance suggests that even in the absence of an introduced inoculum, diabetes increases infection susceptibility in the presence of an implant.</p><p>Nitric oxide (NO) release can be used to mediate the foreign body response around implanted devices. NO also has antibacterial properties that may enhance the body's immune response to implant-associated infection. Additionally, diabetic wounds are characterized by nitric oxide deficiency, and thus NO supplementation may promote better wound healing and implant acceptance in diabetics. The use of nitric oxide to modulate the tissue response to indwelling implants was explored in two studies. In vivo glucose recovery of subcutaneously implanted NO-releasing microdialysis probes was evaluated in a healthy rat model using saturated NO solutions that provided a steady release of NO. A constant NO flux of 162 pmol cm-2 s-1 was perfused through the probe membrane for 8 hours daily. The in vivo effects of increased localized NO were evaluated by monitoring glucose recovery over a 14-day period. Beginning at 7 days, significant differences in glucose recovery between the control and NO-releasing probes were observed. At the 14-day time point, histological analysis revealed decreased inflammatory cell density at the probe surface and a thinner collagen capsule. In the second study, polyurethane-coated wires with varying NO release properties were implanted subcutaneously in 17 Yorkshire piglets with time points of 3, 7, 21, and 42 days. To create the NO-releasing coating, the NO-releasing vehicle (i.e., PROLI/NO, AEAP3 or MPTMS nanoparticles) was dispersed into EtOH (2.5 mL) at concentrations of 36 or 72 mg/mL. This solution was then mixed with an equal volume of 50:50 wt% HPU/TPU (160 mg/mL total PU). Effects of NO release were analyzed using histological data. These data were analyzed using a non-parametric Wilcoxon rank-sum test. Coatings with short NO release durations (i.e., 24 h) failed to reduce collagen capsule thickness at 3 and 6 weeks. Longer release durations (3 and 14d) however significantly reduced collagen capsule thickness at longer timepoints. The acute inflammatory response was significantly affected by coatings with the longest duration and greatest dose of NO release. However these benefits were not realized at later timepoints, suggesting that NO must be actively released in order to influence inflammatory response.</p><p>The tissue response to percutaneously implanted glucose sensors was investigated in healthy and diabetic rats. A multi-dose regimen of streptozotocin was used to induce diabetes in experimental rats. Three types of functional, implantable glucose sensors, supplied by Medtronic® were used: SofTM sensor, EnliteTM sensor, and Enlite 2TM sensor. The sensors were percutaneously implanted in the rat dorsum subcutaneous space. MiniLinkTM transmitters were attached to the rats, permitting continuous glucose monitoring. At 3 days, 1 week, and 4 weeks, tissue directly adjacent to the sensors was evaluated for collagen encapsulation, density of any collagen encapsulation, inflammatory response as measured via inflammatory cell density, and microvessel density. These endpoints were evaluated histologically via Masson's trichrome, Hoechst, H&E, and CD31 staining. Additionally, continuous functional sensor data was evaluated for sensor accuracy, attenuation, and lag time. Histological analyses revealed few significant differences in collagen thickness among different sensors, in different tissue types, or over time. In general, Masson's trichrome-stained images seem to suggest a balance between collagen capsule formation and inflammatory cell density. As inflammation increased adjacent to sensors over time, collagen capsule thickness decreased somewhat and stabilized. Collagen capsule formation was most evident adjacent to the plastic tubing portion of the sensor whereas inflammation was greatest adjacent to the sensing electrode. Likewise, few significant differences in collagen density index (CDI) were observed among sensor types, tissue types, or over time. CDI remained relatively constant over time for all sensors. Analysis of inflammatory cell density in general revealed a greater inflammatory response adjacent to percutaneous Enlite sensors, though these results were not significant. Additionally, inflammatory cell density was generally greater adjacent to non-diabetic sensors, however this result was also not significant. Inflammatory cell density increased or remained stable over time for all sensor types, suggesting that the presence of percutaneously-implanted sensors produces a chronic inflammatory response that does not resolve. Vascularity adjacent to implanted sensors remained generally stable over time, sometimes decreasing but not significantly. At the 1-month timepoint, no significant differences in vasculature were seen among sensor types. A balance also appears to exist for microvessel and inflammatory cell densities. The non-diabetic percutaneous Enlite sensor had the greatest microvessel density at earlier timepoints, while also having the greatest inflammatory cell density. However, at later timepoints, microvessel density decreased somewhat as inflammation increased somewhat. Finally, analysis of sensor performance showed significant sensor failure at longer timepoints. Sensitivity decreased somewhat for all sensors except for the non-diabetic Enlite sensor, which in general had greater overall sensitivity in comparison to the non-diabetic Sof sensor. Lag time was relatively similar among all sensor types, tissue types, and over time. MARD values were considerably lower for diabetic sensors for the Day 1 bolus, but were generally similar for all sensors at the 1-week bolus. These results suggest that the diabetic foreign body response, while somewhat decreased, is not significantly different than that in non-diabetic tissue. In addition, the design of the EnliteTM and Enlite 2TM sensors promoted a more aggressive inflammatory response despite being smaller and more flexible in design. Most evident from the results was the presence of a chronic inflammatory response adjacent to the percutaneously-implanted sensors, which likely contributed to the high rate of sensor failure over time.</p> / Dissertation
17

All-Optical Quantification of Ciliary Physiology

Huang, Brendan 17 March 2016 (has links)
<p> Cilia are cellular organelles that generate microfluidic flow at multiple sites in the body. They are important for health due to their critical roles in mucus clearance in the respiratory tract, circulation of cerebrospinal fluid in the ventricles of the brain, transport of ova in the Fallopian tubes, and left-right patterning of the body. Nonetheless, standards for basic mechanical phenotyping of cilia are still relatively undefined. The aim of this thesis is to develop an experimental and conceptual framework for comprehensive ciliary phenotyping. Towards that aim, we pursue three major lines of investigation involving ciliary physiology, pathophysiology, and measurement.</p><p> Our investigation into pathophysiology looks at the possibility of quantifying intermediate ciliary flow defects. Specifically, we investigate subtle changes to ciliary flow generated by genetic knockdown of ciliary proteins, alterations in chemical signaling, and changes to the viscous environment of ciliated surfaces. We additionally quantify the onset of ciliary flow in the context of normal development.</p><p> Secondly, we demonstrate the use of optical coherence tomography (OCT)-based velocimetry techniques for the measurement of cilia-driven fluid flow. In particular, we focus on a class of correlation-based techniques that utilizes the complex OCT signal to recover the total speed of fluid flow. We analyze and extend these techniques towards directional velocity measurements, and eventually towards quantification of the full three-dimensional, three vector component velocity flow field.</p><p> Finally, our investigation into ciliary physiology involves the development of a simplified model of ciliary function. Building on previous models of ciliated surfaces as shearing elements, we develop our "treamdill-in-a-pool" model of ciliated surface that also incorporates the dynamics of functional reserve and failure. These efforts motivate the measurement of three important physical parameters, flow rate, force, and mechanical power output, under conditions of increased viscous loading.</p><p> Building on these themes, we propose a comprehensive, optical-imaging based approach towards quantifying flow, force, and power in the context of ciliary performance and failure. We present a method of quantifying these mechanical properties not by direct measurement, but rather by inference from the fluid flow field that is generated by ciliary action. In all, we propose a new theoretical and experimental framework for biomechanical phenotyping of ciliated surfaces.</p>
18

BCL::SAS- Small Angle X-Ray / Neutron Scattering Profiles to Assist Protein Structure Prediction

Putnam, Daniel Kent 28 March 2016 (has links)
The Biochemical Library (BCL) is a protein structure prediction algorithm developed in the Meiler Lab at Vanderbilt University based on the placement of secondary structure elements (SSEs). This algorithm incorporates sparse experimental data constraints from nuclear magnetic resonance (NMR), Cryo- electron microscopy (CryoEM), and electron paramagnetic resonance (EPR), to restrict the conformational sampling space but does not have the capability to use Small Angle X-Ray / Neutron data. This dissertation delineates my work to add this capability to BCL::Fold. Specifically I show and show for what type of structures SAXS/SANS experimental data improves the accuracy BCL:: Fold and importantly where it does not. Furthermore, in collaboration with Oak Ridge National Labs, I present my work on structural determination of the Cellulose Synthase Complex in Arabidopsis Thaliana.
19

Predicting the Spatio-Temporal Evolution of Tumor Growth and Treatment Response in a Murine Model of Glioma

Hormuth, David Andrew II 30 March 2016 (has links)
Glioblastoma is a highly invasive and aggressive brain tumor which accounts for nearly 82% of all gliomas. Patients with glioblastoma typically have a poor prognosis, suffering recurrence 7 to 10 months from the conclusion of adjuvant therapy. One promising direction for improving the clinical care of cancer, in general, and glioblastomas, in particular, is the development of accurate and precise predictive mathematical models of tumor growth. Through the use of non-invasive imaging data, mathematical models can be parameterized by the unique characteristics of an individualâs tumor to provide a âforecastâ of future tumor growth and treatment response. However, there is currently a paucity of mathematical models that have been evaluated in a controlled setting where model predictions can be validated directly to experimental results. In this work, an experimental and modeling framework is developed in which imaging measurements acquired before and after treatment are used to inform individualized biophysical models of glioma growth and response to radiotherapy. For untreated tumor growth, this work demonstrated that the commonly used reaction-diffusion model poorly predicts in vivo glioma growth. Secondly, this work demonstrated that mechanobiological effects are a necessary component to brain tumor modeling. Thirdly, this work showed that a variable carrying capacity is needed to capture the intra-tumoral spatial heterogeneity. Finally, a model was developed incorporating rapid cell death and reduced cellular proliferation and was shown to accurately predict future tumor growth following whole brain radiotherapy. Together, these studies show the potential power that image driven individualized tumor âforecastsâ could have on improving the clinical care of cancer.
20

Dopamine Regulation of Insulin Secretion Investigated by Fluorescence Fluctuation Spectroscopy

Caldwell, Brittany Catherine 04 April 2016 (has links)
Insulin resistance together with insufficient insulin secretion leads to the development of type II diabetes mellitus. Glucose-stimulation of insulin secretion has been extensively studied, but other pathways that regulate insulin secretion are not as well understood. I investigated the signaling mechanisms involved in the inhibition of insulin secretion by dopamine, which is synthesized by pancreatic ?-cells and co-secreted with insulin. Previous research has shown that dopamine-inhibition of insulin secretion is mediated primarily by the D3 dopamine receptor (DRD3) even though the DRD2 receptor has been reported to be expressed in ?-cells. To further understand this dichotomy, I investigated the dynamic protein-protein interactions between the dopamine receptor subtypes and their heterotrimeric G-proteins using two-color fluorescence fluctuation spectroscopy (FFS). I characterized the use of two fluorescent proteins, mApple and EGFP, to measure dynamic heteromerization changes with FFS. Furthermore, I showed that to detect proper GPCR signaling, both the G? and G? subunits of the G?? complex must be overexpressed in the cell. Triple transfections of a dopamine receptor and G? and G? subunits each labeled with a different fluorescent protein resulted in plasma membrane localization of all three fluorescent proteins and permitted FFS evaluation of interactions between the dopamine receptor and G?? complex. Upon dopamine stimulation, I measured a decrease in protein-protein interactions between the D3 receptor and G?? complex, indicating activation of the D3 receptor. In contrast, no significant changes in protein interactions were measured between the D2 receptor and G?? complex after dopamine treatment. These results demonstrate that two-color FFS is a powerful tool to measure dynamic protein interactions in living cells, and show that preferential DRD3 signaling in ?-cells occurs at the level of G-protein release.

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