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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.
41

Mammalian Cell Surface Display of Functional Alpha 1-Protease Inhibitor: Building "Designer" Serpins

Gierczak, Richard Frank January 2015 (has links)
Human serpins belong to a superfamily of serine protease inhibitors involved in the regulation of essential physiological processes, including coagulation via thrombin inhibition by AT. Inhibitory serpins undergo a remarkable folding mechanism to a thermodynamically unstable (i.e. metastable) conformation, highlighted by a long and flexible RCL, prior to secretion as soluble proteins into circulation. The serpin alpha-1-proteinase inhibitor (API) normally protects tissues from proteases released from inflammatory cells (e.g., neutrophil elastase). Importantly, a variant of API (i.e. API-Pittsburgh or API-M358R) was reported to be the cause of a fatal bleeding disorder in a young patient in the late 1970`s; the point mutation M358R at P1 of the RCL resulted in a dramatic shift in function toward thrombin inhibition. This dissertation summarizes the results from experiments performed with serpins expressed as membrane proteins tethered to the surface of mammalian cells. Serpins API-M358R, AT, HCII, and the non-inhibitory double mutant API-M358R/T345R were anchored to 293 and COS cell plasma membranes with N-terminal non-cleavable protein sequences derived from either the human asialoglycoprotein (AR) or transferrin (TF) receptors. Sub-cellular fractionation (with or without monolayer exposure to thrombin) immunoblots confirmed serpin localization to the integral membrane fraction using either anchoring approach or cell type. The blots also revealed that tethered API-Pittsburgh in particular, and AT to a lesser extent formed serpin-enzyme complex (SEC) with thrombin, while HCII and API-M358R/T345R (as expected) did not. While tethered API-M358R maintained inhibitory function, kinetic studies revealed that the rate of SEC formation was less rapid compared to its soluble counterpart. Additional testing by immunofluorescence microscopy, and flow cytometry confirmed the status of tethered API-M358R as a robust inhibitor of thrombin. That tethered serpins maintained the ability to inhibit thrombin provided the underlying rationale for the thesis hypotheses: surface displayed serpins can be used in gene therapy to temper thrombogenicity associated with certain diseased tissues (i.e. cancer), and tethered serpins can be used as a platform for screening RCL mutant libraries to identify “better” protease (i.e. thrombin) inhibitors. The potential gene therapy scheme was tested by expressing tethered API-Pittsburgh on the surface of T24/83 cancer cells constitutively co-expressing tissue factor (TF), and then measuring endogenous thrombin generation in the presence of re-calcified, and defibrinated human plasma by either discontinuous or continuous fluorescence-based thrombin generation assays (TGA). Unexpectedly, the displayed API-Pittsburgh did not appear to reduce discontinuous TGA thrombin suggesting that the difference may have been too low for accurate measurement by this method. Moreover, the results were identical when the same reaction was continuously monitored by fluorescence-based TGA, indicating that the levels of API-Pittsburgh expression were simply insufficient to effectively counter thrombin generation. The high levels were confirmed when up to 1 µM of hirudin variant 3, or soluble API-M358R, were required to completely abolish the thrombin profile. With this in mind, a measureable reduction in TGA was achieved when 293 cells were co-transfected with DNA ratios of API-M358R: TF adjusted to 9:1. Mammalian cell display, in combination with FACS/flow cytometry, has previously been employed to successfully develop improved monoclonal antibodies. However, there was never any certainty that the technique was applicable to the screening of displayed serpin mutant RCL libraries. The method was tested with a modest library degenerate only at P1; the rationale was that successful sorting would generate the expected wild-type (WT) P1 Arg (i.e. API-Pittsburgh). Unfortunately, repeated attempts did not result in enrichment, and flow cytometry was abandoned. An alternate protocol based on bacterial expression, and previously developed in our lab, was implemented in order to perform the library screens. This technique involved incubating lysates, containing soluble serpin RCL mutant candidates, with immobilized thrombin. Encouragingly, the P1 library screen identified the WT candidate at the expected frequency (5 in 150 lysates) as well as the more rare P1 mutant Lys (1 in 150 lysates). A kinetic comparison between mutant proteins containing the three basic residues revealed that P1 Arg (k2 ~ 105 M-1sec-1) was approximately two orders of magnitude more efficient than either Lys or His (both with k2 ~ 103 M-1sec-1) at inhibiting thrombin. The bacterial expression technique was then enhanced through kinetic optimization in order to facilitate the screening of more complex libraries. Analysis of the P7 to P1 (always Arg) library returned a selection of anticipated non-polar residues (5 in 100 lysates; 2 x Pro, 2 x Leu and Met) at P2. Extensive screening (~ 1300 colonies) of a second expanded library with the repeated VNN nucleotide sequence (i.e. no stop codons to eliminate truncated proteins) at P7 to P2 and P1 Arg, identified 7 x Pro mutants at P2 further confirming the results from the original library screen. Importantly, the assay also identified the novel mutant TLSATPR which registered the largest kinetic response (k2 ~ 5 x 105 M-1sec-1), and even exceeding API- M358R by a factor of ~ 3 (k2 ~ 1.5 x 105 M-1 sec-1). / Dissertation / Doctor of Philosophy (PhD)
42

RARE EARTH-DOPED GALLIUM NITRIDE FLAT PANEL DISPLAY DEVICES

HEIKENFELD, JASON CHARLES January 2003 (has links)
No description available.
43

Novel Electrowetting Display Devices

Zhou, Kaichang January 2008 (has links)
No description available.
44

The design of computer based integrated information displays /

Mitchell, Christine Marie January 1980 (has links)
No description available.
45

Look Ma, No Hardware!

Guadiana, Juan M. 10 1900 (has links)
ITC/USA 2009 Conference Proceedings / The Forty-Fifth Annual International Telemetering Conference and Technical Exhibition / October 26-29, 2009 / Riviera Hotel & Convention Center, Las Vegas, Nevada / Google Soft Decom and the number of hits will be tenfold over the same search last year. The migration of hardware functionality toward software is relentless. On the telemetry front, Data Bridges that take Pulse Code Modulated (PCM) signals and transform them to ubiquitous network packets make it all too easy. The need for expensive hardware such as the Decommutator (Decom), Frame Synchronizer, Digital Recorder, and Oscillograph Recorder (StripChart) will diminish sharply. Software Decom packages will feel the squeeze too, from homegrown Soft Decom software that is easier to maintain and has no licensing issues. This paper airs the dirty laundry associated with this hardware and software. Latencies and ugly temporal aberration that really plague an analyst. Also discussed is how a few packet/file formats eliminate the need for most of the hardware in a traditional telemetry data processing facility.
46

An investigation of new methods of creating three-dimensional multiplanar displays

Sucharov, Leon January 1998 (has links)
No description available.
47

The interference of human immunodeficiency virus assembly and maturation by ankyrin repeat proteins / Interférences avec l'assemblage et la maturation du Virus de l'Immunodeficience Humaine (VIH) par des protéines à motifs répétés Ankyrines

Nangola, Sawitree 28 January 2011 (has links)
Le but de ce travail est de découvrir des nouvelles protéines suceptibles d'interférer avec le cycle vital du virus HIV. De par leur repliement, les protéines à motifs ankyrines peuvent constituer une ossature protéique trés bien adaptée à cet objectif. Plusieurs interacteurs spécifiques de la protéine MA-CA du HIV ont été sélectionnées par exposition sur phage à partir d'une bibliothèque de variants d'ankyrines. Trois protéines isolées ont été produites à partir de clones ayant une forte activité de liaison. Le meilleur interacteur protéique (1D4) interagit avec un épitope situié sur le domaine CA. La constante de dissociation entre 1D4 et la protéine HACA a été déterminée par Calorimétrie de Titrage Isotherme (ou ITC) et est égale à 0,45M. La protéine 1D4 n'a pas d'effet détectable sur la maturation virale suivie par une technique ELISA de dosage de la Protease du HIV. En revanche, cette protéine interfere avec l'assemblage viral dans des cellules supT1 qui exprime de façon stable la protéine 1D4 sous forme myristoylée. Ce resultat ouvre une perspective d'appoche pour interferer avec le cycle vital du HIV. / Presently, the standard regimen for antiretroviral treatment is highly active antiretroviral therapy (HAART). However, this strategy inherits the well-known side effects and is prone to promote the HIV drug-resistant strains. As a consequence, gene therapy has been introduced as an alternative approach. In this study, we aimed to discover the novel protein-based agents for intervening viral replication by gene targeting procedure. Regarding the efficient folding dynamic in cytoplasm, ankyrin repeat protein was considered to be a candidate scaffold. Several engineered ankyrin binders specific to HIV MA-CA domain were successfully retrieved from the ankyrin-displayed phage library. Three positive clones with high binding activity by ELISA were selected for further analyzing their binding property in soluble form. The best binder, 1D4, recognized its epitope located on CA domain as shown by Western immunobloting and ELISA. The affinity of 1D4 against H6MA-CA was 0.45 μM with one to two moles of target molecule determined by isothermal titration calorimetry (ITC). Although 1D4 exhibited no effect on viral maturation as verified by an ELISA based HIV protease assay technique, it disturbed the viral assembly process in Sup-T1 cells which stably expressed the myristoylated 1D4. This finding has provided a concrete prospect for HIV life cycle interruption by stem cell gene therapy in the future.
48

Readability of electronic displays

Winkler, Robert E January 2010 (has links)
Photocopy of typescript. / Digitized by Kansas Correctional Industries
49

The effectiveness of library displays

Stephenson, Judy Anne, n/a January 1989 (has links)
This present study sought to evaluate the effectiveness of two types of school library displays: a display with books only, called Display, and a display with books, posters, models, copy, and realia, called Display +. The effectiveness of these displays was to be measured in two ways: a) through the observation of the attaction power, holding power and viewer participation in a display and b) through measuring the circulation of displayed books. Before commencing the study a literature search was conducted. The result of the literature search yielded four authors, Goldhor (1972; 1981), Aguilar (1983), Watson (1985), and Baker (1986), who had researched the relationship between circulation and displays. Each of these studies used the measurable effect of circulation increasing, decreasing or remaining constant to determine the effect of the display. This present study used a similar methodology and monitored the circulation of books on both types of displays. However, this study sought to go beyond the effect of circulation in determining the effectiveness of displays because the previous studies had not taken into account the library user who is affected by the display but is unable to borrow a book from the display. The literature search turned towards the area of museum exhibits and displays and the methodology employed to evaluate these exhibits and displays. Shettel (1968), Warren (1972), Screven (1976), Linn (1976), Clowes and Wolfe (1980), and Miles (1982) used attraction and holding power as measures of museum exhibit and display effectiveness. Similarly, library users can be attracted and their attention held by library displays. To the variables of attraction and holding power this study added the variable of participation, picking up books or other items in the display not necessarily with the intent of borrowing the books. In order to construct a Display + and control as far as possible the elements in the display a literature search of books and articles relating to the design elements of displays was conducted, and findings applied in the construction of the display. Shettel's (1968) methodology of unobtrusive observation was employed in this study with the added benefit of videotaping the observations. The hypotheses were set out in three groups, those relating to a single display, those comparing the effectiveness of Display and Display +, and those relating to circulation. The results of this study found in general that the attraction power of Display + exceeded the attraction power of Display but the holding power and participation in Display was greater than that of Display + indicating that the designer of library displays should pay particular attention to the purpose of displays in their libraries. The results of the circulation hypothesis confirmed the results of Goldhor (1972;1981), Aguilar (1983), Watson (1985), and Baker (1986) that more books circulated when they were displayed than when they were on the library shelves.
50

Multi-user retinal displays with two components. New degrees of freedom.

Biverot, Hans January 2001 (has links)
No description available.

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