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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.
21

Contested rationality : early regulation of GMO releases in Britain

Levidow, Les January 1994 (has links)
This thesis analyses the development of safety regulation for the intentional release of genetically modified organisms (GMOs) between 19 89-92, especially in Britain in its European context, and by contrast to the USA. The thesis emphasizes the practical dilemmas of GMO regulation in accommodating uncertainties about public unease and environmental harm. It serves as a case study of safety regulation as a constructed rationality, of national regulatory styles, and of environmental precaution. In anticipating hazards prior to evidence of harm, GMO regulation had a contested 'rational' basis. Regulators encountered disputes in defining the risk problem, in establishing risk-management institutions, and in reducing scientific uncertainty about potential harm. Insofar as GMO regulation had a precautionary content, it undermined the 'rational' stereotype of risk-assessment steps. Both the precautionary potential and its limits derived from the project of overcoming obstacles to a biotechnology market. This meant symbolically normalizing GMOs as benign products, while specifying testable ecological uncertainties rooted in some naturalistic analogy. Technical 'risk' abstracted potential harm from issues of socioagronomic control which underlay the earlier environmental controversy. The thesis argues for recasting theoretical models of safety regulation as a 'technical' or 'procedural' rationality. GMO regulation contained poles of tension which such theoretical models attribute to antagonistic rationalities. Broadly speaking, the regulatory system was managing an internal contradiction between social legitimacy and commercialization. The difficulties of GMO regulation arose from its implicit role in legitimizing biotechnology, by default of any democratic procedure for adjudicating a contentious technoscientific development.
22

Science, internationalization, and policy networks : regulating genetically-engineered food crops in Canada and the United States, 1973-1998 /

Moore, Elizabeth Louise, January 1900 (has links) (PDF)
Thesis (Ph. D.)--University of Toronto, 2000. / Includes bibliographical references (p. 413-445). Also available on the World Wide Web.
23

Agricultural extension management strategies in Cameroon : a comparative study

Tata, Thomas Fofung January 1998 (has links)
No description available.
24

Development of a durable polymer-modified cement matrix for ferrocement

Ramli, Mahyuddin January 1997 (has links)
No description available.
25

Elastomer modified epoxies : Toughening of tetraglycidyl diamino diphenyl methane epoxy

Lee, W. H. January 1986 (has links)
No description available.
26

An evaluation of attitudes and behaviours towards food-related risks

McDonald, Anne-Lise Nadia Marina January 2001 (has links)
No description available.
27

The Effects of Three Methods of Practice on Improving the Performance of a Modified Free-Throw by Sixth Grade Girls

Pruner, Sherry W. 08 1900 (has links)
This investigation is concerned with the problem of determining the effects of three kinds of practice (mental-physical, distributive, and physical) on improving the performance of the Modified Free-Throw. In addition, this study investigates whether or not any one of the practice methods used was superior to the others.
28

Luminescence based monitoring of genetically modified microbial inoculants in the soil

Meikle, Audrey January 1992 (has links)
A luminescence based marker system was developed for detection of genetically modified Pseudomonas fluorescens and E. coli. During batch growth in liquid culture, luminescence measured by luminometry was directly proportional to biomass concentration and enabled detection of 104 - 106 cells ml-1 of P. fluorescens and 101 cells ml-1 of E. coli, in actively growing cultures. Following inoculation into soil, detection levels were reduced ten-fold. After the subsequent utilisation of available nutrients, activity and luminescence decreased and luminometry then provided a direct, non-extractive means of measuring population activity of lux-marked inocula. Potential luminescence, measured as luminescence following amendment with nutrients, enabled assessment of the rate of reactivation of the lux-marked inocula and quantification of the size of the activatable population. Both these techniques, and traditional techniques, were used to investigate the survival of P. fluorescens and E. coli in soil microcosms. The effect of matric potential and indigenous organisms on luminescence and on survival of P. fluorescens was assessed. Matric potential significantly decreased the activity of both introduced and indigenous populations, but the indigenous population also significantly decreased the activity and biomass concentration of the introduced P. fluorescens population. Use of luminometry as a non-extractive measure of biomass concentration provided qualitative correlation with viable cell concentration, suggesting its potential for rapid enumeration of marked inocula. Reactivation of cells at increased matric stress was decreased, but use of high substrate:cell ratios at -30 kPa produced higher levels of luminescence and may, therefore, improve the use of luminometry as an estimate of biomass.
29

Luminescence based detection of genetically modified Pseudomonas fluorescens in soil

Amin-Hanjani, Soheila January 1992 (has links)
Methods currently available for the detection and enumeration of genetically modified micro-organisms in the environment include culturing methods, direct microscopic detection and nucleic hybridization techniques. The aim of this project was to develop luminescence as a molecular based-marker system in Pseudomonas fluorescens. The lux genes, originally isolated from Vibrio fischeri, were introduced into Ps. fluorescens on plasmid vectors and on the chromosome. The efficiency of these two strategies for the detection of Ps. fluorescens in soil was assessed. Luminometry was used to estimate biomass concentration during growth. The sensitivity of luminescence detection was greater for the plasmid marked Ps. fluorescens in both liquid culture and soil, however, cellular light output was less closely linked to biomass concentration. Enumeration of cells by luminometry was only possible for growing cells as light output is correlated with microbial activity. The lux chromosomal marker was stable in liquid culture for at least 200 generations and in soil for up to 135 days. The plasmid borne lux genes had a half-life of 20 generations in liquid culture. After inoculation in sterile soil, plasmid loss was only observed during cellular growth. The frequency of transfer of the lux genes from Ps. fluorescens, by conjugation and transformation, was assessed in liquid culture. Mobilisation of these genes by three self transmissible plasmids was negligible due to the instability of these vectors in this host. Transformation of Ps. stutzeri with lux genes, by cell contact, was at frequencies below levels of detection. Luminescence provided a valuable marker for tracking pseudomonads in soil. Detection of marked strains by luminometry provided a sensitive, rapid and non-extractive technique for enumeration of growing cells and measurement of microbial activity. As the chromosomally encoded lux genes were stable, regardless of growth conditions, and emitted sufficient levels of light to enable visual enumeration of colonies by eye, this was considered the best system for long term risk assessment studies.
30

Diabetes: a gene therapy approach using genetically modified skin cells

Facey, Sandra Lee, University of Western Sydney, College of Science, Technology and Environment, School of Science, Food and Horticulture January 2004 (has links)
The long-term implications of deregulation of glucose metabolism, manifesting itself as diabetes is significant. Whilst treatments for the disease are progressing, often they require multiple daily insulin injections. This may be difficult for diabetics in poorer nations. This thesis examines the possibility of utilising keratinocytes and melanocytes transfected with either normal or furin-modified proinsulin constructs, to process and secrete mature insulin via secreted protein pathways. The advantage of this approach is that it may allow normalisation of basal glucose levels, which in turn may prevent or delay the onset of many of the complications associated with diabetes. The results confirmed that keratinocytes and melanocytes are able to process and secrete mature insulin from a furin-modified proinsulin construct, thus validating this approach and paving the way for skin grafts of genetically modified cells to be used as a possible treatment for diabetes. Whilst the results regarding the ability of these cells to process a normal proinsulin construct are inconclusive, they highlight areas of interest that could help to resolve this issue / Master of Science (Hons.)

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