Global ETD Search

101	UGA-mediated selenium incorporation into glutathione peroxidase 1 and green fluorescent protein Wen, Wu, January 1998 (has links) Thesis (Ph. D.)--University of Missouri-Columbia, 1998. / Typescript. Vita. Includes bibliographical references (leaves 141-152). Also available on the Internet.
102	Role of DksA and Hfq in Shigella flexneri virulence Sharma, Ashima Krishankumar 28 August 2008 (has links) Not available / text RNA-protein interactions Genetic transcription--Regulation Shigella flexneri Virulence (Microbiology) Proteins Non-coding RNA Messenger RNA
103	Role of DksA and Hfq in Shigella flexneri virulence Sharma, Ashima Krishankumar, 1979- 18 August 2011 (has links) Not available / text RNA-protein interactions Genetic transcription--Regulation Shigella flexneri Virulence (Microbiology) Proteins Non-coding RNA Messenger RNA
104	Quantitative analysis of hTERT mRNA expression in gestational trophoblastic disease by real-time PCR 張綺雲, Cheung, Yee-wan. January 2002 (has links) published_or_final_version / Medical Sciences / Master / Master of Medical Sciences Trophoblastic tumors - Genetic aspects. Telomerase. Messenger RNA. Polymerase chain reaction. Gene expression.
105	Mathematical modeling of eukaryotic gene expression Tang, Terry, University of Lethbridge. Faculty of Arts and Science January 2010 (has links) Using the Gillespie algorithm, the export of the mRNA molecules from their transcription site to the nuclear pore complex is simulated. The effect of various structures in the nu- cleus on the efficiency of export is discussed. The results show that having some of the space filled by chromatin near the mRNA synthesis site shortens the transport time. Next, the complete eukaryotic gene expression including transcription, splicing, mRNA export, translation, and mRNA degradation is modeled using delay stochastic simulation. This allows for the study of stochastic effects during the process and on the protein production rate patterns. Various protein production patterns can be produced by adjusting the poly-A tail length of the mRNA and the promoter efficiency of the gene. After that, the opposing effects of the chromatin density on the seeking time of the transcription factors for the promoter and the exit time of the mRNA product are discussed. / xi, 102 leaves ; 28 cm Messenger RNA -- Research Proteins -- Synthesis Eukaryotic cells -- Research Gene expression Chromatin Cytology -- Mathematical models Dissertations, Academic
106	Real-time RNA-based amplification allows for sensitive forensic blood evidence analysis / Real time ribonucleic acid based amplification allows for sensitive forensic blood evidence analysis Counsil, Tyler I. January 2008 (has links) The purpose of this experiment was to determine if nucleic acid sequence based amplification (NASBA) is a suitable application for the differentiation of body fluids that might comprise a forensic evidence sample. NASBA is a sensitive RNA transcription based amplification system. NASBA could theorhetically be used for bodily fluid identification based upon amplification of tissue-specific mRNA transcripts present in a given forensic sample.Amplification of both Glyceraldehyde 3-phosphate dehydrogenase (GAPDH) and Matrix Metalloproteinase 1 1 (MMPmRNA transcripts were used to determine that NASBA could amplify body fluid transcripts and whether it could distinguish between menstrual and non-menstrual blood, respectively. GAPDH is a housekeeping gene that is constituently expressed and its mRNA transcripts could therefore be used to determine whether non-menstrual blood could be amplified using the NASBA procedure. MMP 11 is a menstrual cycle-specific gene associated with endometrial breakdown. Using the mRNA transcripts from MMP 11, NASBA could be utilized for menstrual blood identification. In this study, non-menstrual and menstrual blood samples were analyzed with NASBA both in the presence and absence of chemical contamination. Contaminants utilized ranged from commercial automotive wax, transmission fluid, brake fluid, artificial tears, hand soap, 10% bleach, and the luminol blood detecting reagent. Non-menstrual blood was aliquoted onto a 1 cm x 1 cm cotton cloth for contamination, while menstrual blood was provided on a 1 cm x 1 cm area of sterile menstrual pad. All samples underwent Tri reagent extraction to obtain RNA samples for NASBA amplification.With respect to NASBA amplification data, non-menstrual blood data (from extracted RNA and unextracted blood samples) revealed the highest levels of amplification as shown in relative fluorescence units (RFU). Uncontaminated menstrual blood revealed the second highest amplification data. In the presence of chemical contamination, high levels of amplification were observed when samples were contaminated with brake fluid and commercial hand soap. Moderately low amplification was observed with samples contaminated with transmission fluid, 10% bleach, and artificial tears. NASBA amplification was completely inhibited in the presence of automotive wax and luminol. Cycle threshold (CO values for each amplification result were also obtained from each reaction. Smaller Ct values correspond to a higher NASBAreaction efficiency and therefore larger amplification values. The Ct values obtained for each amplified sample correlate strongly with the amount of amplification observed from reaction. Based upon the results of this experiment, NASBA should be considered as a novel tool for forensic evidence analysis. / Department of Biology Polymerase chain reaction. Messenger RNA -- Analysis. Forensic genetics -- Technique. Blood -- Analysis.
107	Mapping the structure of the "e;on"e; and "e;off"e; states of the yykkCD putative riboswitch in Bacillus subtilis / Title on signature form: Mapping the "e;on"e; and "e;off"e; states of the ykkCD putative riboswitch in Bacillus subtilis Roark, Krystal A. January 2009 (has links) Access to abstract permanently restricted to Ball State community only / Access to thesis permanently restricted to Ball State community only / Department of Chemistry Genetic regulation Messenger RNA Bacillus subtilis--Genetics
108	Microbial forensics and the use of RT-PCR and NASBA for human saliva evidence analysis Counsil, Tyler I. 05 August 2011 (has links) Access to abstract permanently restricted to Ball State community only / Access to thesis permanently restricted to Ball State community only / Department of Biology Polymerase chain reaction Nucleotide sequence Messenger RNA Forensic genetics--Technique Saliva--Analysis
109	Development of androgen receptor messenger RNA targeted molecular beacons for use in the study of prostate cancer progression Glick, Cindy Jennifer 31 July 2008 (has links) Messenger RNA (mRNA) posttranscriptional regulation has been implicated in the development and/or progression of several diseases including many types of cancer, rheumatoid arthritis, vascular disease, and Alzheimer's disease. Differential regulation of Androgen Receptor (AR) mRNA has been associated specifically with prostate cancer progression. In this thesis, molecular beacons were developed to allow for the detection of the expression and localization of AR mRNA in live prostate cancer cells. These beacons were then applied as a tool for studying how AR mRNA regulation is involved in prostate cancer growth and advancement. Two AR mRNA targeted beacons were designed and tested in solution and in live cells to determine their functionality. The beacon-based approach for AR mRNA detection was then optimized through the use of the two beacons in tandem and alteration of their backbone chemistry. A series of validation tests were performed on these beacons, including testing their abilities to: 1) produce a feasible localization pattern, 2) discriminate between AR positive (AR+) and AR negative (AR-) prostate cancer cell lines and 3) follow stimulus-induced changes in AR mRNA expression. Based on these results, a dual chimeric beacon approach was selected to determine the role of AR mRNA regulation in two systems that represent important stages in prostate cancer growth and progression: 1) hormone stimulation of androgen-dependent prostate cancer cells and 2) progression of androgen-dependent prostate cancer cells to the androgen-independent state. Our results suggest that changes in AR mRNA expression, organization, and localization may be indicative of molecular mechanisms involved in these critical transitions associated with prostate cancer progression. Taken together, this work provides a feasibility study for visualizing changes in AR mRNA state as a diagnostic measure for evaluating the aggressiveness of the disease and demonstrates the possible utility of therapeutically targeting AR mRNA regulation in order to prevent prostate cancer advancement. Prostate cancer Molecular beacons Androgen receptor MRNA Prostate Cancer Messenger RNA Molecular probes
110	Transcriptional analysis of the role of CD8+ T lymphocytes in acute neural herpes simplex virus infection / David C. Tscharke. Tscharke, David C. January 1997 (has links) Bibliography: leaves 141-182. / xi, 182, [36] leaves, [12] leaves of plates : ill. ; 30 cm. / Title page, contents and abstract only. The complete thesis in print form is available from the University Library. / The aim of this thesis is to analyse the molecular events associated with CD8+ T lymphocyte activity in HSV infected sensory ganglia. The role of CD8+ T cells in cytokine responses to ganglionic HSV infection is investigated, with particular reference to the Th1/Th2 paradigm and a known anti-viral mediator, IFN-[gamma]. A non-directed method of mRNA analysis is applied to HSV infected ganglia with the specific aim of identifying transcripts that may be associated with CD8+ T cell activity in the nervous system. / Thesis (Ph.D.)--University of Adelaide, Dept. of Microbiology and Immunology, 1997 Herpes simplex virus. Lymphocytes. T cells. Messenger RNA. Cytokines. Ganglia, Sensory. Mice as laboratory animals.

Search results