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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.
151

Genetic variability in a species possessing extensive gene duplication : genetic interpretation of duplicate loci and examination of genetic variation in populations of rainbow trout /

Allendorf, Frederick William. January 1975 (has links)
Thesis (Ph. D.)--University of Washington, 1975. / Bibliography: leaves [90]-98.
152

Influence of physical and biological habitat variables on juvenile salmonid and invertebrate drift abundance in southwest British Columbia streams

Nicol, Sandra Diane 05 1900 (has links)
Determining the physical and biological habitat variables that influence the abundance of juvenile salmonids in British Columbia streams will improve management practices. Habitat models are tools that provide insight into organisms’ habitat needs and provide a more efficient mechanism for estimating population abundance than direct measurement. Models have been developed for salmonids in other jurisdictions, but very few have included invertebrate drift (a primary food source for juvenile salmonids) as a predictive variable. This is because temporal and spatial variation of drift abundance are widely assumed to be so high that drift cannot be reliably estimated without unreasonable effort. This thesis investigates the temporal and spatial variability of invertebrate drift and the impact of its inclusion in habitat models for juvenile salmonid abundance in two chapters. The first objective of the first chapter was to evaluate the temporal variability of invertebrate drift by comparing the seasonal and day-to-day variation in drift abundance to spatial variation within and between sites. The second objective was to develop predictive models for invertebrate drift abundance. Aquatic, terrestrial and total invertebrate drift abundances varied primarily between sites and very little between days or months at the same site, indicating that a single day of sampling is sufficient to assess drift abundance for comparison among sites. The abundance of invertebrate drift was related to productivity- and flow-related habitat variables. The objectives of the second chapter were to develop predictive models for juvenile salmonid abundance in southwestern BC using physical and biological habitat variables, to determine whether habitat variables differ between the Coast and Interior regions of BC, to determine the contribution of invertebrate drift to the relative predictive ability of the models, and to determine cost:benefit ratios for the predictive models and their component variables. The final models for predicting abundance of all young-of-year salmonids combined, and rainbow trout (Oncorhynchus mykiss) and coho salmon (O. kisutch) individually, included variables related to stream structure and productivity, and the models for rainbow and coho showed regional differences. Invertebrate drift did not improve model fit.
153

Cardiac output and respiratory measurements in the rainbow trout and their application to the study of blood and water flow limitations on chemical flux at the gill

Schmieder, Patricia K. (Patricia Kathleen) 19 July 1990 (has links)
A method has been developed for the continuous automated monitoring of cardiac output in adult rainbow trout. Average cardiac output measured under control conditions and varied environmental conditions of hypoxia and post-hypoxia was significantly higher (P≤ 0.05) in male than female trout. The cardiac output of trout in spawning condition was significantly higher (P≤ 0.05) than that of trout not in spawning condition. Measurements of pulsatile cardiac output were made simultaneously with trout ventilation, and revealed ventilatory interactions with blood flow that varied depending on environmental oxygen condition. The method for monitoring gill blood flow was used with methods for automated measurement of gill water flow, oxygen uptake, and chemical flux in vivo. An experimental protocol was developed in which environmental oxygen was varied to obtain maximum increases in water flow over the gills without blood flow changes, and subsequent attainment of maximum increases in blood flow through the gills with decreasing water flow. The protocol was used as a probe to study variations in chemical flux with varied blood or water flow. The changes in gill flux of butanol (Log octanol/water partition coefficient (P) = 0.88) measured during control, hypoxia, and post-hypoxia correlated with observed changes in blood flow. A 70% increase in butanol flux was noted with a 50% increase in cardiac output, but there was no increase in butanol flux with a 100% increase in ventilation volume. Changes observed in the gill flux of decanol (Log P = 4.57) measured under varied environmental oxygen conditions correlated with observed changes in ventilation volume. A 100% increase in decanol flux was noted with a 160% increase in ventilation volume. The observed blood flow limitations to uptake of the low Log P butanol, and the water flow limitations to uptake of the high Log P decanol helped to verify assumptions made in recently proposed flow-limited models for prediction of chemical flux across fish gills. / Graduation date: 1991
154

Slothrop's Sublime: Perversion and Paranoia in Gravity's Rainbow

Simony, Christopher 11 May 2012 (has links)
This paper examines how the protagonist of Gravity’s Rainbow, Tyrone Slothrop, seeks subjective fixity in the historical and postmodern sublime. Using an approach that draws upon the theories of Freud, Lacan, and Zizek, the essay argues that while Slothrop indulges his own paranoia and commits acts of increasing perversion to assert self, these attempts actually blur the lines of identity instead of presenting an autonomous being.
155

Functional Characterization of Rainbow Trout (<em>Oncorhynchus mykiss</em>) Chemokine 2 (CK-2)

Eshaque, Shathi January 2006 (has links)
Chemokines are cytokines with chemoattractant ability, and comprise one of the major groups of molecules in immune system. These are small, secreted proteins cause the migration of leukocytes to the sites of injury. Over 40 mammalian chemokines have been identified to date, and they have been implicated in a number of immune mediated processes, including regulation of inflammation, antigen presentation, blood cell development, metastasis, viral infection and wound healing. In rainbow trout, there have been fewer chemokines reported and only one functional study has been published. Rainbow trout chemokine 2 (CK-2) is the only known CC chemokine with a mucin stalk, which has the potential for extensive <em>O</em>-glycosylation. However, no functional characterization has been performed on this molecule yet. CK-2 shares the presence of a mucin stalk with the mammalian chemokines, fractalkine (CX<sub>3</sub>CL1), lymphotactin (XCL1), and CXCL16. Another related trout CC chemokine sequence, CK-2. 1, has been discovered recently, which has 98% nucleotide sequence identity with CK-2. CK-2. 1 was believed to be a separate gene due to its apparent differential regulation in challenged rainbow trout. The question remained, however, whether or not CK-2. 1 was a separate gene or an allele of CK-2. The goal of this project was to further characterize both CK-2 and CK-2. 1. <br /><br /> Through genomic PCR on several outbred individuals it was shown that CK-2. 1 is an allele of CK-2 but not a separate gene. Reverse transcriptase (RT) PCR analysis revealed an increased level of transcript both CK-2 and CK-2. 1 in response to phytohaemagglutinin (PHA) stimulation of head kidney leukocytes (HKL) and peripheral blood leukocytes (PBL) collected from fish with different allelic distributions. Similar results were also observed in the rainbow trout macrophage/monocyte cell line, RTS11. Moreover, an anti-CK-2 antiserum was developed in rabbits, which cross-reacted with CK-2. 1. This newly produced antibody was used to determine the protein expression levels in PHA stimulated rainbow trout tissues. RT-PCR was also performed on the same tissues in order to examine the transcript expression. Rainbow trout with both CK-2 and CK-2. 1 were used for this experiment. An overall decreasing pattern of transcript (both CK-2 and CK-2. 1) was observed in brain and HK over 24 hours, while protein was still detected at 24 hours post stimulation. However, in spleen the CK-2 transcript showed a slight upregulation at 4 hours post stimulation along with a very little or no CK-2. 1 expression, although no protein was detected in spleen. Liver showed a very low level of CK-2 and CK-2. 1 transcript at 8 hours post stimulation; while protein was again detected at 24 hours post stimulation. In addition, the sizes of the proteins found in different tissues were larger than expected (&le;30 kDa for CK-2 or &le;35 for CK-2. 1), perhaps due to the presence of extensive <em>O</em>-glycosylation at the mucin stalk of the protein. <br /><br /> A chemotaxis assay was carried out, which is the definitive assay for chemokine activity. This assay showed migration of peripheral blood leukocytes across a membrane with 5µm pores toward CK-2 at an optimal concentration of 500ng/ml (17nm). Moreover, by pre-treating the recombinant chemokine with the polyclonal antisera, it was shown that the chemokine was actually causing the chemotactic activity. Pre-treatment of the cells with pertussis toxin, an inhibitor of G-protein signalling inhibited the migration of PBLs, established the fact that CK-2 caused chemotaxis by binding to a 7 transmembrane, G-coupled receptor just like all other known chemokines. Interestingly, CK-2 was also shown to attract RTS-11 cells. <br /><br /> Overall, the above findings indicate that CK-2 is functionally a chemokine with two very different alleles in rainbow trout. It is probably heavily <em>O</em>-glycosylated and different tissues express different sizes of the protein. This is only the second functional study of a fish chemokine.
156

none

Chang, Hung-ming 14 June 2004 (has links)
Adult movie channel business is always a very controversial subject in the society. However, there is not so much serious research on it. The main reason is adult channels¡¦ sensitivity. On the one hand, people are curious, because they provide the basic natural desire of the human beings. On the other hand, due to that same reason, people tend to take aversive attitude toward the existence of these channels in the society. Based on this phenomenon, the focus of the research is about how these adult channels operate under the pressure of the society. This research can be divided into two parts: the structure of the theory and the analysis of the case. Through relevant theories, we can verify whether these theories are suitable for this particular industry. Meanwhile, we can present the overview and background of adult movie channel market through a lot of related secondary data. We regard these materials as the foundation of analyzing the case company. About the case analysis part, with the combination of theories and case description, we try to sketch the contours of the actual operations of adult movie channel. Because the operation of adult movie channels is based on cable TV, this research will talk about adult movie channel market in terms of cable TV and probe into the market of adult movie channel. From the case study, it can be found that the greatest hindrance of adult movie channel is the law. Under the legal regulations, there is not so much freedom for managers to run the business. In order to overcome these predicaments, they need to adopt cooperations in the industry or develop diversification to keep growing. Besides, they will face other invisible pressure such as moral pressure, the negative impression from the society and conflicts in employees' mind. Through this research, we can come out the true appearance of this special industry, and understand the way of their operation on the ecology of adult movie channel.
157

The biology of naturalized rainbow trout, Oncorhynchus mykiss (Walbaum), in Kenya cold water streams and implications for future management /

Ngugi, Charles Chege, January 1999 (has links)
Thesis (Ph.D.), Memorial University of Newfoundland, 2000. / Restricted until June 2001. Bibliography: leaves 153-162.
158

The technical feasibility of using treated mine water to rear rainbow trout, Oncorhynchus mykiss

Tierney, Aislinn E. January 1900 (has links)
Thesis (M.S.)--West Virginia University, 2002. / Title from document title page. Document formatted into pages; contains viii, 84 p. : ill. (some col.), col. map. Includes abstract. Includes bibliographical references (p. 65-69).
159

Cloning and characterization of a novel oocyte-specific gene Fbos encoding an F-Box protein in rainbow trout (Oncorhynchus mykiss)

Wang, Lei, January 2009 (has links)
Thesis (M.S.)--West Virginia University, 2009. / Title from document title page. Document formatted into pages; contains vii, 51 p. : ill. (some col.). Includes abstract. Includes bibliographical references (p. 46-51).
160

Development of methods to determine prevalence of Flavobacterium psychrophilum in farm systems

Manji, Farah January 2008 (has links)
Flavobacterium psychrophilum (Fp), the aetiological agent of rainbow trout fry syndrome (RTFS) and bacterial cold-water disease (BCWD), is responsible for significant mortalities and economic losses in the salmonid aquaculture industry worldwide. Currently, there is no effective commercial vaccine against RTFS available, and the treatment of the disease depends on the oral administration of a wide range of anti-microbial compounds, some of which have proven ineffective. With unsuccessful disinfection procedures, possibilities of antibiotic resistance developing and no commercial vaccine available, there is an increased need to rapidly detect Fp and reduce mortalities in the industry by improving control measures in the farm system. The aim of this thesis was to investigate possible sources of Fp in a rainbow trout fry farm system and to use this data to develop strategies to reduce the prevalence of the pathogen with this farming system. Novel assays to detect Fp (loop-mediated isothermal amplification; LAMP), quantify Fp (quantitative PCR; qPCR) and to detect the fishes’ host response to Fp (Luminex™) were developed, and then used alongside bacterial culture and nested PCR to determine the prevalence of Fp on a commercial fish farm. Four batches of eggs from 3 different geographic sources were collected on arrival at the farm and tested for the prevalence of Fp. Fry from these batches were monitored as they grew and were moved to different sites at the farm. Kidney, spleen and blood were collected at 3 different life stages from the fry, until they were sold for ongrowing by the farm. Water samples from the inlet, outlet and fry tanks were collected at each sampling point. PCR analysis and bacteriology were the two main methods selected for screening the eggs and fry tissue for Fp. All sources of eggs were found to be positive for Fp with prevalences ranging from 1.1 % - 1.9 % and there was a significant increase in prevalence over time for all 4 batches of eggs ranging from 19.8 % - 34.6 % by the final life stage sampled. There was also a substantial difference in the numbers of fry samples positive for Fp depending on whether nested PCR or bacterial culture were used, as well as the organ (kidney or spleen) tested. This highlighted the importance of sampling both organs rather than just the one. Nested PCR was more sensitive than culture with 13 % of the fry samples reported as Fp positive, by sampling both the kidney and spleen collectively, while only 5 % were Fp positive by bacteriology. The levels of Fp in all samples could not be quantified by qPCR due to limits in the sensitivity of the assay. For those samples that were quantified at the levels of Fp detected by qPCR ranged from 3.38 x 104 well-1 - 2.07 x 106 well-1 genome copies in egg samples; from 3.38 x 103 well-1 – 3.07 x 107 well-1 genome copies well-1 in tissue samples (spleen or kidney), and from 7.89 x 103 – 7.22 x 104 genome copies well-1 in water samples. The sensitivity of the standard curve was limited to 103 copies well-1 and following optimisation of the assay the annealing temperature was decreased by 1˚C to 62°C to reduce the cross-reactivity to negligible levels, though this reduced the sensitivity of the assay even further to 104 copies well-1. The detection limits by qPCR obtained by spiking samples with known amounts of Fp were 192 CFU mg-1 from egg samples, 184 CFU mg-1 from fry tissue samples, and 220 CFU ml-1 from water samples,. The sensitivity of the LAMP assay determined by spiking egg, kidney, spleen and water samples was 18 CFU mg-1, 22 CFU mg-1, 25 CFU mg-1 and 16 CFU ml-1, respectively. The latter was similar to, though not as sensitive as nested PCR. Nested PCR limits determined by spiking egg, kidney, spleen and water samples were 14 CFU mg-1, 11 CFU mg-1, 13 CFU mg-1 and 11 CFU ml-1. No cross-reactivity was found with any bacteria including other Flavobacterium species with nested PCR but cross-reactivity with other Flavobacterium species were found with both qPCR (1.51 % with Flavobacterium aquatile and 0.30 % with Flavobacterium johnsoniae) and LAMP. The LAMP assay showed slight cross-reactivity with Flavobacterium columnare and Flavobacterium branchiophilum. A novel Luminex™ assay was also developed and optimised, using microspheres coated with Fp, to detect antibodies to Fp in the serum of the fry. The Luminex™ allowed small volumes of serum from individual fry to be used to evaluate antibody response as an indirect method to determine exposure to and infection by Fp. A large number of fry from all 4 batches (88% - 94%) of eggs were found to contain anti-Fp antibodies though it still remains to be determined whether the antibodies were specific to Fp. From the work carried out in this study, it can be concluded that whether eggs are carrying Fp inside and/or on their surface, it should be possible to reduce the prevalence of Fp in farm systems by regularly screening the broodstock, eggs and fry. Supply of Fp-free eggs and milt is essential to reduce the reservoir of Fp on farms. Both the qPCR and LAMP assay require further optimisation but they do offer potential for the future screening of Fp at farm sites and in the laboratory. Future control measures for RFTS should include the screening of broodstock and eggs by sensitive methods so that Fp-free seed can be supplied to farms. This, alongside effective disinfection procedures, rigorous husbandry practices and future vaccine development will all be required to manage this very significant fish disease.

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