Spelling suggestions: "subject:"contagion bovine pleuropneumoniae"" "subject:"contagion bovine bronchopneumonia""
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Contagious bovine pleuropneumonia (CBPP) in the Maasai ecosystem of south-western Kenya : evaluation of seroprevalence, risk factors and vaccine safety and efficacyMtui-Malamsha, Niwael Jesse January 2009 (has links)
Contagious bovine pleuropneumonia (CBPP) is a bovine bacterial disease of major economic importance in sub-Saharan Africa. Vaccination has been recommended to control the disease in endemic areas such as the Maasai ecosystems of Kenya and Tanzania; however, the currently used live attenuated vaccine has been reported to have poor vaccine safety and efficacy. To compare standard (current) and an improved (buffered) version of the live CBPP-vaccine, several epidemiological studies were carried out in Maasai cattle in Kenya between 2006 and 2008. Specifically, the aims were to estimate CBPP seroprevalence at herd and animal level; to identify risk factors for seroprevalence at both levels; to investigate the spatial distribution of seroprevalence; to compare post vaccination adverse events in cattle vaccinated with a standard and a buffered vaccine, and finally to compare efficacy of the two vaccines to induce seroconversion and to prevent development of clinical signs suggestive of CBPP. A cross-sectional study was carried out in 6872 cattle in 175 randomly selected herds from Loita and Mara divisions. A competitive ELISA revealed that 85% of the herds in the area had at least one seropositive animal and that seropositive herds were harbouring 11% seropositive cattle. A complement fixation test revealed that 46% of the herds had at least one seropositive animal and that seropositive herds were harbouring 4% seropositive cattle. A multivariable logistic regression analysis of the seroprevalence indicated that previous vaccination against CBPP, a history of CBPP outbreaks in the herd, animal age and the location of the herd in the division of Mara were positively correlated to seroprevalence. To investigate the observed difference in herd seroprevalence between the two divisions further, a spatial analysis was conducted. A SatScan test revealed clusters in Mara in areas identified by veterinary personnel as CBPP ‘hot spots’. A logistic regression using spatial information identified that location in the midland agro-ecological zone or close to a river and vaccination were positively associated with seroprevalence. To compare safety and efficacy of a standard and a buffered vaccine, two cohorts of approximately 40,000 cattle were used. The study showed that within 100 days post vaccination, 6.2 cattle per 1000 vaccinates developed adverse events, 4.1 of which were specifically attributable to vaccination and ranging from swelling of the tail to the tail sloughing off. This study revealed a slightly higher incidence of adverse events in cattle vaccinated with the buffered vaccine compared to the standard vaccine. A comparison of the efficacy of the two vaccines revealed that cattle vaccinated with the buffered vaccine had higher odds of seroconversion and lower odds of developing symptoms of CBPP, three and twelve months post vaccination respectively. The epidemiological studies conducted clearly show wide spread seroprevalence in the Maasai cattle. Given the (spatial) heterogeneity observed, control measures should probably be targeted in areas of increased risk (clusters). However, positive association of vaccination and seropositivity call for better diagnostics tests that can differentiate vaccinated from infected animals. Vaccination with buffered vaccine resulted in increased seroconversion, decreased clinical signs indicative of CBPP post vaccination and low seroprevalence post ‘outbreak’. Nevertheless, the increase in adverse events related to the buffered vaccine calls for further research into safer CBPP vaccines.
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Economics of contagious bovine pleuropneumonia and its control in pastoral systems in KenyaOnono, Joshua Orungo January 2013 (has links)
No description available.
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Evaluation of lipoprotein Q and L-a-glycerol-3-phosphate oxidase of mycoplasma mycoides subs. mycoides (small colony) as virulence factors in contagious bovine pleuropneumonia (CBPP) infectionsMulongo, Musa Matsanza January 2010 (has links)
No description available.
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The role of Mycoplasma species in bovine respiratory disease complex in feedlot cattle in South AfricaCarrington, Christopher Antony Paul. January 2007 (has links)
Thesis (MMedVet (Production Animal Studies)--University of Pretoria, 2007. / Includes bibliographical references.
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In vivo infection biology of contagious bovine pleuropneumoniaGull, Tamara Brownsey 15 May 2009 (has links)
Contagious Bovine Pleuropneumonia (CBPP), caused by Mycoplasma mycoides
mycoides small colony (MmmSC), is a devastating respiratory disease of cattle in Africa,
Asia and the Middle East. Little investigation has been done on molecular disease
pathogenesis and host response beyond soluble cytokine detection. This study developed
and characterized models for three strains of MmmSC of varying severity. Strains used
were Gladysdale, Ondangwa and Shawawa. Samples of bronchoalveolar lavage fluid,
bronchial biopsy, nasal epithelial cells and blood were obtained prior to and at weekly
time points post-infection. Microarray analysis of RNA extracted from samples revealed
host cellular pathways and genes important in the pathogenesis of CBPP, including
multiple immune system and inflammatory response pathways. A number of pathways
whose influence on disease pathogenesis was not immediately clear were also activated,
including pathways involved in amino acid synthesis, fat metabolism, and endocrine
hormone responses. Microarray results were confirmed with real-time polymerase chain
reaction (RT-PCR) of selected genes. Comparative RT-PCR analysis of selected genes between the three strains of MmmSC revealed genes possibly responsible for differential
strain virulence, including interleukins 1B, 6, 8, and 18 and the gene nuclear factor of
kappa light polypeptide gene enhancer in B cells inhibitor, alpha (NFKBIA). A similar
analysis of selected genes between survivors and nonsurvivors of the virulent Gladysdale
strain of MmmSC suggested genes involved in survival, including interleukin 8,
calmodulin 2 (CALM2), and NFKBIA. Avenues of additional study were identified.
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Molecular characterisation of Mycoplasma mycoides subsp. mycoides SC /Persson, Anja M., January 2002 (has links) (PDF)
Diss. (sammanfattning) Uppsala : Sveriges lantbruksuniv., 2002. / Härtill 4 uppsatser.
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Novel diagnostic microarray assay formats towards comprehensive on-site analysisGantelius, Jesper January 2009 (has links)
Advances in molecular methods for analyzing DNA, RNA and proteins in humans as well as in other animals, plants, fungi, bacteria or viruses have greatly increased the resolution with which we can study life’s complexity and dynamics on earth. While genomic, transcriptomic and proteomic laboratory tools for molecular diagnosis of disease are rapidly becoming more comprehensive, the access to such advanced yet often expensive and centralized procedures is limited. There is a great need for rapid and comprehensive diagnostic methods in low-resource settings or contexts where a person can not or will not go to a hospital or medical laboratory, yet where a clinical analysis is urgent. In this thesis, results from development and characterization of novel technologies for DNA and protein microarray analysis are presented. Emphasis is on methods that could provide rapid, cost-effective and portable analysis with convenient readout and retained diagnostic accuracy. The first study presents a magnetic bead-based approach for DNA microarray analysis for a rapid visual detection of single nucleotide polymorphisms. In the second work, magnetic beads were used as detection reagents for rapid differential detection of presence of pestiviral family members using a DNA oligonucleotide microarray with read-out by means of a tabletop scanner or a digital camera. In paper three, autoimmune responses from human sera were detected on a protein autoantigen microarray, again by means of magnetic bead analysis. Here, special emphasis was made in comprehensively comparing the performance of the magnetic bead detection to common fluorescence-based detection. In the fourth study, an immunochromatographic lateral flow protein microarray assay is presented for application in the classification of contagious pleuropneumonia from bovine serum samples. The analysis could be performed within 10 minutes using a table top scanner, and the performance of the assay was shown to be comparable to that of a cocktail ELISA. In the fifth paper, the lateral flow microarray framework is investigated in further detail by means of experiments and numerical simulation. It was found that downstream effects play an important role, and the results further suggest that the downstream binding profiles may find use in simple affinity evaluation. / QC 20100713
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