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Molecular epidemiology, clonality and virulence of Dichelobacter nodosus, the agent of ovine footrot /Buller, Nicky. January 2005 (has links)
Thesis (Ph.D.)--Murdoch University, 2005. / Thesis submitted to the Division of Health Sciences.
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The resistance of Pisum to Mycosphaerella pinodes (Berk. and Blox.) VestergrClulow, Stephen A. January 1989 (has links)
No description available.
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Morphologic, molecular and antigenic characteristics of Bacteroides nodosusGradin, Joseph Lloyd 09 November 1989 (has links)
Graduation date: 1990
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Molecular epidemiology, clonality and virulence of Dichelobacter nodosus, the agent of ovine footrotNbuller@agric.wa.gov.au, Nicky Buller January 2005 (has links)
Dichelobacter nodosus, an anaerobic bacterium, is the major transmissible agent of ovine footrot. The disease expresses as a virulent or benign lesion in the hoof. Virulence is related to the production of serine proteases, particularly a thermostable protease. Isolates of D. nodosus are characterised according to the type of protease produced (either heat-stable or heat-labile) and the electrophoretogram (zymogram) of the protease. This study reports on the use of the DNA-based typing techniques Pulsed-Field Gel Electrophoresis (PFGE) and Infrequent-Restriction-Site-PCR (IRS-PCR) to investigate the molecular epidemiology of D. nodosus, including a consideration of the relationship between genetic type, zymogram patterns and whole cell protein profiles.
The aim of the project was to obtain a better understanding of D. nodosus strain diversity and dissemination in Australia and its relationship to virulence within the population. The overall intention was to use this information to assist in the long-term control of virulent footrot.
Field isolates of D. nodosus from Western Australia (n = 735), New South Wales (n = 16), Victoria (n = 24) and South Australia (n = 21) were obtained and analysed. Both typing techniques that were used offered good differentiation between isolates for epidemiological purposes, and the results were in general agreement. PFGE provided slightly better discrimination between isolates, with 214 PFGE types (181 from Western Australia) compared to 94 IrsT types (77 from Western Australia). Within this diverse range of molecular types clonality was observed - with clones being defined as clusters of isolates having closely related PFGE types. The strains were categorised as genetically diverse, genetically similar or identified as the same strain. This diversity of genetic types was found overall, within flocks of sheep on a farm and within a single hoof where, on a number of occasions, multiple molecular types and zymogram types were found colonising a single hoof. One isolate that was experimentally inoculated into a flock of sheep produced six different genetic types when tested 12 months after the initial infection. This indicates that D. nodosus undergoes rapid genetic change, which means that follow-up epidemiological investigation of disease outbreaks and trace-backs need to be done as soon after infection as possible. The genetic differences appeared to be due to large insertions or deletions of DNA.
Amongst sheep on some properties, isolates that had a different protease expression and virulence expression were found to have the same molecular type. Investigation of these isolates by SDS-PAGE showed that they also had the same whole cell protein profiles. Isolates from the same clonal groups also had the same protein profile, whereas genetically diverse isolates had different protein profiles. The lack of protein differences between isolates of the same molecular type, or within a clonal group, suggests that the differences in protease thermostability may be due to conformational changes in the protein, rather than to overall detectable genetic change and/or expression of different proteins. These results demonstrate that PFGE typing can be useful in predicting likely phenotypic expression of whole cell proteins. Further work is required to elucidate differences between virulent and benign strains of D. nodosus.
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The Role of fimbrial antigens of Dichelobacter nodosus in diagnosis and pathogenesis of footrotDhungyel, Om Prakash January 2002 (has links)
Studies presented in this thesis looked at developing new methods for the diagnosis of virulent footrot (VFR) in sheep and identification of serogroups of Dichelobacter nodosus, the principal causative agent of footrot. Earlier studies had shown that immunological memory response in sheep recovered from VFR can be aroused by natural or recurrent infection or by injection of outer membrane protein (OMP) antigens to be used as a retrospective diagnostic test for VFR. But OMP antigen was found to be non-specific in older animals. To overcome this non-specificity of OMP antigen in anamnestic response, pilus antigen was evaluated in a trial at Camden. The results of this trial indicated that antibodies to pilus antigen can be detected over time in a manner similar to OMP antibodies so a retrospective assessment of VFR status can be made by anamnestic test with pilus antigens. The anamnestic response to pilus was similar in character to OMP antigen but unlike OMP was highly specific. The response to anamnestic challenge with pilus was determined by severity of the lesions they had expressed, with severe lesions triggering the greater responses. However, there was variation between individuals, with some (6 of 46 with severe lesions) failing to respond. This individual variation is probably mediated genetically as is response to vaccination. This anamnestic test was tested in flocks of sheep in Nepal that had a history of VFR which had apparently been eradicated. That assessment, based on clinical findings, was confirmed by the uniformly negative results in the pilus anamnestic test applied to a representative sample of the population. This allowed a conclusion that the virulent strains of D. nodosus involved had been eliminated from these flocks. As mentioned in the preceding study pilus antigen was found to be very specific and ideal for retrospective diagnosis of virulent footrot with an anamnestic challenge ELISA test. However, serogroup specificity was seen as a disadvantage of using pilus antigen for the anamnestic test. The possibility of using multivalent pilus antigens was tested in another trial. These animals had been involved in a clinical expression experiment conducted by another research group and had a clinical and bacteriological history extending over more than 12 months. After these initial trials all these animals were treated for footrot and managed for 5 months as a single flock at Camden. These were then challenged with multivalent pilus antigen (serogroup A - I) as a single injection. The results obtained indicate that multivalent pilus anamnestic ELISA is equally effective as monovalent pilus. This has the added advantage that prior knowledge of the serogroups present in the flock is not required. It has the possibility of being used as an indirect test to check the presence of serogroups in a flock without doing the bacterial cultures. This test can identify most animals with pre-existing underrunning lesions (Scores of 3 or higher). However, the sensitivity and specificity of this test need to be tested extensively in flocks of known clinical history before it could be adopted as a routine test. As a key component of a larger study to determine the role of fimbrial genes (fimA and fimB) of D. nodosus in the pathogenesis of footrot using allelic exchange to disrupt these genes of a strain (serogroup G), the study presented in this thesis contributed a detailed characterisation of the resultant mutant and the wild strains and tested these strains for virulence in sheep. The results presented provided the first definitive evidence that the fimA gene is essential for virulence of D.nodosus in sheep. In vivo virulence testing of two fimA mutants showed that they were not able to establish any footrot whereas the wild type of the same strain produced virulent footrot in the same trial conducted under similar conditions. These mutant bacteria were not re-isolated from interdigital skin after in vivo challenge. This indicated that fimA mutant strains could not colonise the ovine foot, and the simplest and most likely explanation for these results was that colonisation of the interdigital skin and subsequent penetration of the stratum corneum requires the adhesive activity of type IV fimbriae. However, since these mutants also had altered ability to secrete extracellular proteases, and perhaps other as yet unknown extracellular proteins, the possibility of the involvement of these factors as major determinants of host colonisation or invasion cannot be excluded. Current methods for the identification of the serogroup of D. nodosus present in the bacterial population requires isolation of the organism and after purification by subculture, antigenic analysis with agglutination tests. This usually takes at least 3 to 4 weeks. With the objective of developing a rapid serogroup specific PCR assay, the basis of serogroup variation in D. nodosus localised in the fimbrial gene region was exploited. A common forward primer and 9 serogroup specific reverse primers were selected from the fimbrial gene sequences of the prototype strains. Analytical sensitivity of the serogroup specific primers on chromosomal DNA was similar to PCR tests in other bacterial species reported before. Immuno-magnetic bead capture PCR method was able to detect 5 to 10 cells in cell lysates. Specificity within and between the serogroups of D. nodosus was tested with all the prototype strains. They were found to be very specific to each serogroup and specific only to D. nodosus when tested with 84 commonly found bacterial strains or strains related to D. nodosus. To overcome the time delay in conducting 9 different amplifications to find out the prevalence of all possible serogroups in a flock multiplex PCR reactions with common forward primer and groups of 3, 4 and 5 reverse primers were successful in reducing the number of reactions to 2 (with groups of 4 and 5) or 3 (with groups of 3) primers. A drawback of the multiplex reaction was that if a template was 1000 times less concentrated that the others in the mixture it was not amplified but the margin for difference is very high. The main aim of developing rapid serogroup specific PCR was to apply these tests directly on footrot lesion samples to make it a rapid diagnostic test for field samples. The sensitivity of the test on lesion samples was found to be very low. To try and improve the sensitivity an overnight or four days old pre-enrichment culture in broth was tested but was found to be no better than direct PCR. The immuno-magnetic capture method which improved the sensitivity of pure culture samples by 10 -100 fold also had very low sensitivity with lesion samples. However, this drawback can be overcome by picking up colonies from 4 days old lesion cultures on hoof agar (HA) plates for serogroup specific multiplex PCR. If the colonies are too small/ too few on the lesion cultures these can be sub cultured onto a quarter of 4 percent HA plates and then used for the PCR test which also reduces the time taken for serogrouping at least by 2 weeks. The other advantage is that individual colonies do not need to be isolated. A PCR test can be done on pooled colonies just as well and can be used to identify all serogroups present in the sample. Serogroup specific PCR is much faster and is more sensitive and accurate than slide agglutination tests which take 3 to 4 weeks to complete. Multiplex PCR makes it easier to detect different serogroups in a sample with a maximum of 3 PCR tests. Serogroup specific multiplex PCR will be a useful tool for footrot control based on specific vaccination. The difficulty in using the test on direct lesion swabs needs to be further looked into. There may be future advances in the application of PCR tests to clinical samples.
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The Role of fimbrial antigens of Dichelobacter nodosus in diagnosis and pathogenesis of footrotDhungyel, Om Prakash January 2002 (has links)
Studies presented in this thesis looked at developing new methods for the diagnosis of virulent footrot (VFR) in sheep and identification of serogroups of Dichelobacter nodosus, the principal causative agent of footrot. Earlier studies had shown that immunological memory response in sheep recovered from VFR can be aroused by natural or recurrent infection or by injection of outer membrane protein (OMP) antigens to be used as a retrospective diagnostic test for VFR. But OMP antigen was found to be non-specific in older animals. To overcome this non-specificity of OMP antigen in anamnestic response, pilus antigen was evaluated in a trial at Camden. The results of this trial indicated that antibodies to pilus antigen can be detected over time in a manner similar to OMP antibodies so a retrospective assessment of VFR status can be made by anamnestic test with pilus antigens. The anamnestic response to pilus was similar in character to OMP antigen but unlike OMP was highly specific. The response to anamnestic challenge with pilus was determined by severity of the lesions they had expressed, with severe lesions triggering the greater responses. However, there was variation between individuals, with some (6 of 46 with severe lesions) failing to respond. This individual variation is probably mediated genetically as is response to vaccination. This anamnestic test was tested in flocks of sheep in Nepal that had a history of VFR which had apparently been eradicated. That assessment, based on clinical findings, was confirmed by the uniformly negative results in the pilus anamnestic test applied to a representative sample of the population. This allowed a conclusion that the virulent strains of D. nodosus involved had been eliminated from these flocks. As mentioned in the preceding study pilus antigen was found to be very specific and ideal for retrospective diagnosis of virulent footrot with an anamnestic challenge ELISA test. However, serogroup specificity was seen as a disadvantage of using pilus antigen for the anamnestic test. The possibility of using multivalent pilus antigens was tested in another trial. These animals had been involved in a clinical expression experiment conducted by another research group and had a clinical and bacteriological history extending over more than 12 months. After these initial trials all these animals were treated for footrot and managed for 5 months as a single flock at Camden. These were then challenged with multivalent pilus antigen (serogroup A - I) as a single injection. The results obtained indicate that multivalent pilus anamnestic ELISA is equally effective as monovalent pilus. This has the added advantage that prior knowledge of the serogroups present in the flock is not required. It has the possibility of being used as an indirect test to check the presence of serogroups in a flock without doing the bacterial cultures. This test can identify most animals with pre-existing underrunning lesions (Scores of 3 or higher). However, the sensitivity and specificity of this test need to be tested extensively in flocks of known clinical history before it could be adopted as a routine test. As a key component of a larger study to determine the role of fimbrial genes (fimA and fimB) of D. nodosus in the pathogenesis of footrot using allelic exchange to disrupt these genes of a strain (serogroup G), the study presented in this thesis contributed a detailed characterisation of the resultant mutant and the wild strains and tested these strains for virulence in sheep. The results presented provided the first definitive evidence that the fimA gene is essential for virulence of D.nodosus in sheep. In vivo virulence testing of two fimA mutants showed that they were not able to establish any footrot whereas the wild type of the same strain produced virulent footrot in the same trial conducted under similar conditions. These mutant bacteria were not re-isolated from interdigital skin after in vivo challenge. This indicated that fimA mutant strains could not colonise the ovine foot, and the simplest and most likely explanation for these results was that colonisation of the interdigital skin and subsequent penetration of the stratum corneum requires the adhesive activity of type IV fimbriae. However, since these mutants also had altered ability to secrete extracellular proteases, and perhaps other as yet unknown extracellular proteins, the possibility of the involvement of these factors as major determinants of host colonisation or invasion cannot be excluded. Current methods for the identification of the serogroup of D. nodosus present in the bacterial population requires isolation of the organism and after purification by subculture, antigenic analysis with agglutination tests. This usually takes at least 3 to 4 weeks. With the objective of developing a rapid serogroup specific PCR assay, the basis of serogroup variation in D. nodosus localised in the fimbrial gene region was exploited. A common forward primer and 9 serogroup specific reverse primers were selected from the fimbrial gene sequences of the prototype strains. Analytical sensitivity of the serogroup specific primers on chromosomal DNA was similar to PCR tests in other bacterial species reported before. Immuno-magnetic bead capture PCR method was able to detect 5 to 10 cells in cell lysates. Specificity within and between the serogroups of D. nodosus was tested with all the prototype strains. They were found to be very specific to each serogroup and specific only to D. nodosus when tested with 84 commonly found bacterial strains or strains related to D. nodosus. To overcome the time delay in conducting 9 different amplifications to find out the prevalence of all possible serogroups in a flock multiplex PCR reactions with common forward primer and groups of 3, 4 and 5 reverse primers were successful in reducing the number of reactions to 2 (with groups of 4 and 5) or 3 (with groups of 3) primers. A drawback of the multiplex reaction was that if a template was 1000 times less concentrated that the others in the mixture it was not amplified but the margin for difference is very high. The main aim of developing rapid serogroup specific PCR was to apply these tests directly on footrot lesion samples to make it a rapid diagnostic test for field samples. The sensitivity of the test on lesion samples was found to be very low. To try and improve the sensitivity an overnight or four days old pre-enrichment culture in broth was tested but was found to be no better than direct PCR. The immuno-magnetic capture method which improved the sensitivity of pure culture samples by 10 -100 fold also had very low sensitivity with lesion samples. However, this drawback can be overcome by picking up colonies from 4 days old lesion cultures on hoof agar (HA) plates for serogroup specific multiplex PCR. If the colonies are too small/ too few on the lesion cultures these can be sub cultured onto a quarter of 4 percent HA plates and then used for the PCR test which also reduces the time taken for serogrouping at least by 2 weeks. The other advantage is that individual colonies do not need to be isolated. A PCR test can be done on pooled colonies just as well and can be used to identify all serogroups present in the sample. Serogroup specific PCR is much faster and is more sensitive and accurate than slide agglutination tests which take 3 to 4 weeks to complete. Multiplex PCR makes it easier to detect different serogroups in a sample with a maximum of 3 PCR tests. Serogroup specific multiplex PCR will be a useful tool for footrot control based on specific vaccination. The difficulty in using the test on direct lesion swabs needs to be further looked into. There may be future advances in the application of PCR tests to clinical samples.
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Lesões podais em ovinos na mesorregião sudoeste rio-grandense / Foot lesions in sheep from southwest mesoregion of rio grande do sul stateSilveira, Caroline da Silva 23 February 2016 (has links)
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Previous issue date: 2016-02-23 / Doenças podais são uma das principais injúrias em rebanhos de pequenos ruminantes em diversos países e a pododermatite infecciosa (Footrot) é relatada como a mais frequente em ovinos no Brasil. No Rio Grande do Sul, as doenças podais ainda são um grave problema para os criadores de ovinos e pouco tem sido feito para saná-las. O Footrot, mesmo se tratando de uma doença de notificação obrigatória e frequente na região, os registros oficiais sobre a situação da doença nos rebanhos são escassos. Esse trabalho teve como objetivo descrever as principais características das lesões podais observadas em ovinos da Mesorregião Sudoeste do Rio Grande do Sul, com ênfase nos aspectos epidemiológicos, macroscópicos, microscópicos e radiográficos das lesões de Footrot. O estudo foi realizado em duas etapas. Inicialmente foram avaliados ovinos em 27 propriedades rurais, das quais 21 registraram a ocorrência de lesões podais em ovinos com perdas econômicas significativas. Aproximadamente 1.700 ovinos, em média 10% dos animais do rebanho, apresentavam diferentes graus de claudicação decorrente de lesões podais que, macroscopicamente, variavam de brandas a severas. Posteriormente, foram avaliados os variados graus de lesões de Footrot nos ovinos. Em casos de abate e necropsia, os cascos dos ovinos com as lesões foram submetidos à avaliação macroscópica, radiográfica e microscópica. Dessa forma a doença foi classificada em cinco graus de severidade que variaram de 1 (lesões leves) a 5 (lesões graves). Verificou-se que diversos fatores como clima e manejo foram favoráveis para o desenvolvimento das lesões podais e essas estão associadas, na maioria dos casos, a Footrot em diferentes estágios de evolução. A partir dessa classificação em graus foi possível classificá-los macroscopicamente em duas síndromes clínicas propostas, a saber Footrot benigno e maligno. Essa classificação facilita o estabelecimento das medidas de controle com intuito de limitar a propagação da doença e evitar a evolução das lesões nos cascos acometidos. / Foot diseases are one of the main disorders in small ruminant flocks in several countries and infectious pododermatite (Footrot) is reported as the most frequent podal lesions in sheep in Brazil. In Rio Grande do Sul state, foot diseases still a serious problem for sheep farmers and little has been done to remedy them. Footrot is a notifiable disease and frequent in the region, the official records on the disease situation in herds are scarce. This study aimed to describe the main features of foot lesions observed in sheep from Mesoregion Southwest of Rio Grande do Sul, with emphasis on epidemiology, macroscopic, microscopic and radiographic changes of Footrot injuries. The study was conducted in two steps. Initially, sheep were evaluated on 27 farms, of which 21 showed records of the occurrence of foot lesions in sheep and significant economic losses. Approximately 1,700 sheep, about 10% of the flocks, showed varying degrees of lameness due to foot lesions, macroscopically characterized as mild to severe. Subsequently, they assessed the varying degrees of injuries Footrot in sheep. Hooves with injuries were submitted to macroscopic, radiographic and microscopic evaluation. Thus the disease was classified into five grades of severity ranging from 1 (mild injury) to 5 (severe damage). It has been found that several factors such as weather and handling were favorable for the development of foot injuries and these are associated in most Footrot cases in different stages of evolution. Based on the classification in degrees of infectious pododermatitis it was possible to classify them macroscopically in clinical syndromes proposed as benign and malignant Footrot. This classification facilitates the establishment of control measures with the intention of reduce spread of disease and prevent the development of lesions in affected hooves.
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Controle de Footrot em rebanho ovino no Estado do Rio Grande do Sul: uso de vacina autógena e resposta sorológica. uso de vacina autógena e resposta sorológicaRodrigues, Paulo Ricardo Centeno January 2010 (has links)
O objetivo desta dissertação de mestrado foi avaliar a eficácia de uma vacina autógena no controle do footrot (FR) dos ovinos, para tanto foram desenvolvidos dois experimentos em duas propriedades rurais distintas, no Estado do Rio Grande do Sul (RS). O primeiro experimento foi conduzido em uma propriedade rural do município de Santiago, com um extenso histórico de surtos de footrot no rebanho ovino. Inicialmente foi colhido material infeccioso presente no rebanho para a produção de uma vacina autógena, posteriormente 347 ovelhas foram vacinadas (grupo V) com duas doses da vacina com 30 dias de intervalo, a dose foi 2 ml por via subcutânea. Desse grupo, 150 animais receberam a vacina na região axilar (grupo Va) e 197 animais receberam a vacina na região inguinal (grupo Vb). Um grupo de 75 ovelhas formou o grupo controle (grupo C) sem vacinação. Os dados mostraram que a prevalência do FR no grupo V que inicialmente era de 4%, sofreu uma redução para 2% na semana 23, chegando à zero na semana 30. No grupo C a prevalência de animais infectados foi de 6,7% no início do experimento, teve uma redução para 5,3% na semana 23 e ao final estava em 3,7%. Observou-se uma redução gradativa no número de ovinos infectados nos dois grupos, entretanto a eliminação seletiva ocorrida no grupo controle prejudicou a análise estatística dos dados. Amostras de sangue foram colhidas da jugular dos animais para verificar títulos de anticorpos aglutinantes contra o antígeno presente na propriedade em cinco ocasiões durante o experimento. Os resultados mostraram diferenças significativas (p<0,001) entre os títulos de anticorpos aglutinantes contra Dichelobacter nodosus no soro de ovinos vacinados e não vacinados durante o experimento. A análise das reações vacinais locais apontou a região inguinal como o melhor local para a aplicação da vacina com adjuvante oleoso por via subcutânea e também demonstrou uma relação direta entre a idade dos ovinos e o percentual de reações vacinais locais e a severidade dessas reações. Os resultados sugerem que a vacina autógena com adjuvante oleoso obteve sucesso no controle da doença. O segundo experimento foi conduzido em uma propriedade rural do município de Glorinha, com o objetivo de avaliar a resposta imunológica provocada por uma vacina monovalente e por uma vacina polivalente (7 sorogrupos) contra o FR. Trinta fêmeas ovinas, com idades variadas, foram divididas aleatoriamente em 3 grupos de 10 animais: grupo controle (C) que não foi vacinado, grupo vacinado com vacina monovalente (Vm) e grupo vacinado com vacina polivalente (Vp). Os ovinos vacinados receberam duas doses com quatro semanas de intervalo, a dose foi de 2 ml por via subcutânea na região inguinal. Amostras de sangue foram colhidas da jugular dos animais para verificar títulos de anticorpos aglutinantes contra o D. nodosus em quatro ocasiões durante o experimento. Os resultados mostraram diferenças significativas (p<0,001) entre os títulos médios geométricos (GMT) de anticorpos aglutinantes contra D. nodosus no soro de ovinos dos grupos Vm, Vp e C na quarta, sétima e 12ª semanas do experimento. Em relação aos títulos médios geométricos (GMT) entre os grupos Vm e Vp houve diferenças estatisticamente significativas na quarta e sétima semanas. A vacina monovalente induziu títulos de aglutininas superiores contra o D.nodosus em comparação com a vacina polivalente. / The objective of this work was to evaluate the efficacy of an autogenous vaccine in the control of footrot (FR) in sheep. Two field experimental works were carried on two different farms located in the State of Rio Grande do Sul (RS), Brazil. The first experiment was conducted on a farm in the municipality of Santiago, with a long history of FR outbreaks in their sheep flock. At beginning of the trail samples from FR infected sheep were collected for the production of an autogenous vaccine. Following 347 sheep were vaccinated (group V) with two doses of 2 ml subcutaneously vaccine 30 days apart. Of this group, 150 animals received the vaccine in the axillary region (group Va) and 197 animals received the vaccine in the inguinal region (group Vb). A group of 75 sheep formed the control group (group C) without vaccination. The data showed that the prevalence of FR in the group V initially 4%, was reduced to 2% at 23 weeks, reaching to zero at week 30. In the group C the prevalence of infected animals of 6.7% at the beginning of the experiment, was reduced to 5.3% at week 23, decreasing to 3.7%, at the end. There was a gradual reduction in the number of infected sheep in both groups, however the selective elimination occurred in the group C affected the statistical analysis. Blood samples were collected from the jugular vein of the animals to see evidence of agglutinating antibodies against the antigen present on the property on five occasions during the experiment. The results showed significant differences (p<0,001) between antibody titers against Dichelobacter nodosus in the serum of sheep vaccinated and not vaccinated during the experiment. The analysis of local vaccine reactions showed the inguinal region as the best place for the application subcutaneously oil-adjuvant vaccine and also demonstrated a direct relationship between the age of the sheep and the percentage of local vaccine reactions and the severity of these reactions. The results suggest that autogenous oil-adjuvant vaccine succeeded in controlling the disease. The second experiment was conducted on a farm in the municipality of Glorinha, in order to evaluate the immune response elicited by a monovalent and a polyvalent vaccine against FR, containing seven serogroups. Thirty ewes, of various ages were randomly divided into 3 groups of 10 animals each: control group (C) was not vaccinated, group vaccinated with monovalent vaccine (Vm) and the group vaccinated with polyvalent vaccine (Vp). The sheep were vaccinated with two doses of 2 ml subcutaneously in the inguinal region, four weeks apart. Blood samples were collected from the jugular vein of the animals to determine agglutination titers against D. nodosus in the beginning of the experiment (day zero) and in other three occasions, weeks 4, 7 and 12. The results showed significant differences (p<0,001) between the geometric mean titers (GMT) of antibodies against D. nodosus in the serum of sheep of groups Vm, Vp and group C in the fourth, seventh and 12th weeks of the experiment. For the geometric mean titers (GMT) between the groups Vm and Vp there was statistically significant differences in the fourth and the seventh weeks. The monovalent vaccine induced titers of higher against D. nodosus compared with the polyvalent vaccine.
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Controle de Footrot em rebanho ovino no Estado do Rio Grande do Sul: uso de vacina autógena e resposta sorológica. uso de vacina autógena e resposta sorológicaRodrigues, Paulo Ricardo Centeno January 2010 (has links)
O objetivo desta dissertação de mestrado foi avaliar a eficácia de uma vacina autógena no controle do footrot (FR) dos ovinos, para tanto foram desenvolvidos dois experimentos em duas propriedades rurais distintas, no Estado do Rio Grande do Sul (RS). O primeiro experimento foi conduzido em uma propriedade rural do município de Santiago, com um extenso histórico de surtos de footrot no rebanho ovino. Inicialmente foi colhido material infeccioso presente no rebanho para a produção de uma vacina autógena, posteriormente 347 ovelhas foram vacinadas (grupo V) com duas doses da vacina com 30 dias de intervalo, a dose foi 2 ml por via subcutânea. Desse grupo, 150 animais receberam a vacina na região axilar (grupo Va) e 197 animais receberam a vacina na região inguinal (grupo Vb). Um grupo de 75 ovelhas formou o grupo controle (grupo C) sem vacinação. Os dados mostraram que a prevalência do FR no grupo V que inicialmente era de 4%, sofreu uma redução para 2% na semana 23, chegando à zero na semana 30. No grupo C a prevalência de animais infectados foi de 6,7% no início do experimento, teve uma redução para 5,3% na semana 23 e ao final estava em 3,7%. Observou-se uma redução gradativa no número de ovinos infectados nos dois grupos, entretanto a eliminação seletiva ocorrida no grupo controle prejudicou a análise estatística dos dados. Amostras de sangue foram colhidas da jugular dos animais para verificar títulos de anticorpos aglutinantes contra o antígeno presente na propriedade em cinco ocasiões durante o experimento. Os resultados mostraram diferenças significativas (p<0,001) entre os títulos de anticorpos aglutinantes contra Dichelobacter nodosus no soro de ovinos vacinados e não vacinados durante o experimento. A análise das reações vacinais locais apontou a região inguinal como o melhor local para a aplicação da vacina com adjuvante oleoso por via subcutânea e também demonstrou uma relação direta entre a idade dos ovinos e o percentual de reações vacinais locais e a severidade dessas reações. Os resultados sugerem que a vacina autógena com adjuvante oleoso obteve sucesso no controle da doença. O segundo experimento foi conduzido em uma propriedade rural do município de Glorinha, com o objetivo de avaliar a resposta imunológica provocada por uma vacina monovalente e por uma vacina polivalente (7 sorogrupos) contra o FR. Trinta fêmeas ovinas, com idades variadas, foram divididas aleatoriamente em 3 grupos de 10 animais: grupo controle (C) que não foi vacinado, grupo vacinado com vacina monovalente (Vm) e grupo vacinado com vacina polivalente (Vp). Os ovinos vacinados receberam duas doses com quatro semanas de intervalo, a dose foi de 2 ml por via subcutânea na região inguinal. Amostras de sangue foram colhidas da jugular dos animais para verificar títulos de anticorpos aglutinantes contra o D. nodosus em quatro ocasiões durante o experimento. Os resultados mostraram diferenças significativas (p<0,001) entre os títulos médios geométricos (GMT) de anticorpos aglutinantes contra D. nodosus no soro de ovinos dos grupos Vm, Vp e C na quarta, sétima e 12ª semanas do experimento. Em relação aos títulos médios geométricos (GMT) entre os grupos Vm e Vp houve diferenças estatisticamente significativas na quarta e sétima semanas. A vacina monovalente induziu títulos de aglutininas superiores contra o D.nodosus em comparação com a vacina polivalente. / The objective of this work was to evaluate the efficacy of an autogenous vaccine in the control of footrot (FR) in sheep. Two field experimental works were carried on two different farms located in the State of Rio Grande do Sul (RS), Brazil. The first experiment was conducted on a farm in the municipality of Santiago, with a long history of FR outbreaks in their sheep flock. At beginning of the trail samples from FR infected sheep were collected for the production of an autogenous vaccine. Following 347 sheep were vaccinated (group V) with two doses of 2 ml subcutaneously vaccine 30 days apart. Of this group, 150 animals received the vaccine in the axillary region (group Va) and 197 animals received the vaccine in the inguinal region (group Vb). A group of 75 sheep formed the control group (group C) without vaccination. The data showed that the prevalence of FR in the group V initially 4%, was reduced to 2% at 23 weeks, reaching to zero at week 30. In the group C the prevalence of infected animals of 6.7% at the beginning of the experiment, was reduced to 5.3% at week 23, decreasing to 3.7%, at the end. There was a gradual reduction in the number of infected sheep in both groups, however the selective elimination occurred in the group C affected the statistical analysis. Blood samples were collected from the jugular vein of the animals to see evidence of agglutinating antibodies against the antigen present on the property on five occasions during the experiment. The results showed significant differences (p<0,001) between antibody titers against Dichelobacter nodosus in the serum of sheep vaccinated and not vaccinated during the experiment. The analysis of local vaccine reactions showed the inguinal region as the best place for the application subcutaneously oil-adjuvant vaccine and also demonstrated a direct relationship between the age of the sheep and the percentage of local vaccine reactions and the severity of these reactions. The results suggest that autogenous oil-adjuvant vaccine succeeded in controlling the disease. The second experiment was conducted on a farm in the municipality of Glorinha, in order to evaluate the immune response elicited by a monovalent and a polyvalent vaccine against FR, containing seven serogroups. Thirty ewes, of various ages were randomly divided into 3 groups of 10 animals each: control group (C) was not vaccinated, group vaccinated with monovalent vaccine (Vm) and the group vaccinated with polyvalent vaccine (Vp). The sheep were vaccinated with two doses of 2 ml subcutaneously in the inguinal region, four weeks apart. Blood samples were collected from the jugular vein of the animals to determine agglutination titers against D. nodosus in the beginning of the experiment (day zero) and in other three occasions, weeks 4, 7 and 12. The results showed significant differences (p<0,001) between the geometric mean titers (GMT) of antibodies against D. nodosus in the serum of sheep of groups Vm, Vp and group C in the fourth, seventh and 12th weeks of the experiment. For the geometric mean titers (GMT) between the groups Vm and Vp there was statistically significant differences in the fourth and the seventh weeks. The monovalent vaccine induced titers of higher against D. nodosus compared with the polyvalent vaccine.
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Controle de Footrot em rebanho ovino no Estado do Rio Grande do Sul: uso de vacina autógena e resposta sorológica. uso de vacina autógena e resposta sorológicaRodrigues, Paulo Ricardo Centeno January 2010 (has links)
O objetivo desta dissertação de mestrado foi avaliar a eficácia de uma vacina autógena no controle do footrot (FR) dos ovinos, para tanto foram desenvolvidos dois experimentos em duas propriedades rurais distintas, no Estado do Rio Grande do Sul (RS). O primeiro experimento foi conduzido em uma propriedade rural do município de Santiago, com um extenso histórico de surtos de footrot no rebanho ovino. Inicialmente foi colhido material infeccioso presente no rebanho para a produção de uma vacina autógena, posteriormente 347 ovelhas foram vacinadas (grupo V) com duas doses da vacina com 30 dias de intervalo, a dose foi 2 ml por via subcutânea. Desse grupo, 150 animais receberam a vacina na região axilar (grupo Va) e 197 animais receberam a vacina na região inguinal (grupo Vb). Um grupo de 75 ovelhas formou o grupo controle (grupo C) sem vacinação. Os dados mostraram que a prevalência do FR no grupo V que inicialmente era de 4%, sofreu uma redução para 2% na semana 23, chegando à zero na semana 30. No grupo C a prevalência de animais infectados foi de 6,7% no início do experimento, teve uma redução para 5,3% na semana 23 e ao final estava em 3,7%. Observou-se uma redução gradativa no número de ovinos infectados nos dois grupos, entretanto a eliminação seletiva ocorrida no grupo controle prejudicou a análise estatística dos dados. Amostras de sangue foram colhidas da jugular dos animais para verificar títulos de anticorpos aglutinantes contra o antígeno presente na propriedade em cinco ocasiões durante o experimento. Os resultados mostraram diferenças significativas (p<0,001) entre os títulos de anticorpos aglutinantes contra Dichelobacter nodosus no soro de ovinos vacinados e não vacinados durante o experimento. A análise das reações vacinais locais apontou a região inguinal como o melhor local para a aplicação da vacina com adjuvante oleoso por via subcutânea e também demonstrou uma relação direta entre a idade dos ovinos e o percentual de reações vacinais locais e a severidade dessas reações. Os resultados sugerem que a vacina autógena com adjuvante oleoso obteve sucesso no controle da doença. O segundo experimento foi conduzido em uma propriedade rural do município de Glorinha, com o objetivo de avaliar a resposta imunológica provocada por uma vacina monovalente e por uma vacina polivalente (7 sorogrupos) contra o FR. Trinta fêmeas ovinas, com idades variadas, foram divididas aleatoriamente em 3 grupos de 10 animais: grupo controle (C) que não foi vacinado, grupo vacinado com vacina monovalente (Vm) e grupo vacinado com vacina polivalente (Vp). Os ovinos vacinados receberam duas doses com quatro semanas de intervalo, a dose foi de 2 ml por via subcutânea na região inguinal. Amostras de sangue foram colhidas da jugular dos animais para verificar títulos de anticorpos aglutinantes contra o D. nodosus em quatro ocasiões durante o experimento. Os resultados mostraram diferenças significativas (p<0,001) entre os títulos médios geométricos (GMT) de anticorpos aglutinantes contra D. nodosus no soro de ovinos dos grupos Vm, Vp e C na quarta, sétima e 12ª semanas do experimento. Em relação aos títulos médios geométricos (GMT) entre os grupos Vm e Vp houve diferenças estatisticamente significativas na quarta e sétima semanas. A vacina monovalente induziu títulos de aglutininas superiores contra o D.nodosus em comparação com a vacina polivalente. / The objective of this work was to evaluate the efficacy of an autogenous vaccine in the control of footrot (FR) in sheep. Two field experimental works were carried on two different farms located in the State of Rio Grande do Sul (RS), Brazil. The first experiment was conducted on a farm in the municipality of Santiago, with a long history of FR outbreaks in their sheep flock. At beginning of the trail samples from FR infected sheep were collected for the production of an autogenous vaccine. Following 347 sheep were vaccinated (group V) with two doses of 2 ml subcutaneously vaccine 30 days apart. Of this group, 150 animals received the vaccine in the axillary region (group Va) and 197 animals received the vaccine in the inguinal region (group Vb). A group of 75 sheep formed the control group (group C) without vaccination. The data showed that the prevalence of FR in the group V initially 4%, was reduced to 2% at 23 weeks, reaching to zero at week 30. In the group C the prevalence of infected animals of 6.7% at the beginning of the experiment, was reduced to 5.3% at week 23, decreasing to 3.7%, at the end. There was a gradual reduction in the number of infected sheep in both groups, however the selective elimination occurred in the group C affected the statistical analysis. Blood samples were collected from the jugular vein of the animals to see evidence of agglutinating antibodies against the antigen present on the property on five occasions during the experiment. The results showed significant differences (p<0,001) between antibody titers against Dichelobacter nodosus in the serum of sheep vaccinated and not vaccinated during the experiment. The analysis of local vaccine reactions showed the inguinal region as the best place for the application subcutaneously oil-adjuvant vaccine and also demonstrated a direct relationship between the age of the sheep and the percentage of local vaccine reactions and the severity of these reactions. The results suggest that autogenous oil-adjuvant vaccine succeeded in controlling the disease. The second experiment was conducted on a farm in the municipality of Glorinha, in order to evaluate the immune response elicited by a monovalent and a polyvalent vaccine against FR, containing seven serogroups. Thirty ewes, of various ages were randomly divided into 3 groups of 10 animals each: control group (C) was not vaccinated, group vaccinated with monovalent vaccine (Vm) and the group vaccinated with polyvalent vaccine (Vp). The sheep were vaccinated with two doses of 2 ml subcutaneously in the inguinal region, four weeks apart. Blood samples were collected from the jugular vein of the animals to determine agglutination titers against D. nodosus in the beginning of the experiment (day zero) and in other three occasions, weeks 4, 7 and 12. The results showed significant differences (p<0,001) between the geometric mean titers (GMT) of antibodies against D. nodosus in the serum of sheep of groups Vm, Vp and group C in the fourth, seventh and 12th weeks of the experiment. For the geometric mean titers (GMT) between the groups Vm and Vp there was statistically significant differences in the fourth and the seventh weeks. The monovalent vaccine induced titers of higher against D. nodosus compared with the polyvalent vaccine.
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