Canine Neural Angiostrongyliasis

Lunn, Julian Alexander

January 2007

Master of Veterinary Clinical Studies / Summary Canine Neural Angiostrongyliasis (CNA) is caused by the obligatory neural migration of Angiostrongylus cantonensis larvae in dogs. Characteristically, cases are juvenile dogs with progressive CNS dysfunction characterised by hyperaesthesia and often associated with eosinophilic pleocytosis of the CSF. In Australia, most cases occur between March and June. The rat lungworm, A cantonensis was first described by Chen in 1935 in Canton, China. While initially called Pulmonema cantonensis the parasite was later reclassified as A cantonensis. A disease diagnosed as eosinophilic meningoencephalitis was first described in 1944 in Taiwan. The same disease was reported in 1948 in the East Caroline Islands but it was not until 1961 that A cantonensis was confirmed as the aetiological agent when a patient in a Hawaiian mental institution, who had died of eosinophilic meningoencephalitis, had A cantonensis larvae recovered from the brain and spinal cord. The first reports of animals infected with A cantonensis were made by Mason in 1976 when he described a syndrome occurring in puppies in the Brisbane area, characterised by urinary incontinence, hind limb paresis and hyperaesthesia, often associated with eosinophilic pleocytosis of the CSF. Reports of infection in other species followed including macropods, bats, horses, primates and birds. Twenty-two cases of suspected CNA were collected prospectively to compare with those previously described, including 37 cases published by Mason in 1983, and to examine the accuracy of an ELISA used to diagnose human neural angiostrongyliasis in Australia. Samples were collected from two control populations in an attempt to validate the ELISA results. In the prospective series of cases, there was a significantly older subpopulation of dogs in addition to “classical” young dogs, suggesting that this syndrome can occur at any age and should be considered a differential in any dog with progressive neurological disease. The mortality rate in the prospective group was lower than in the published group, which is a reflection of the severity of the disease in younger animals as is the case with human patients. Definitive diagnosis of neural angiostrongyliasis in human patients has been achieved by identifying A cantonensis larvae within the CSF or aqueous humour. In dogs, the only definitive way to diagnose CNA has been via necropsy. While many cases of CNA are characteristic and presumptive diagnosis can be made based on typical history, signalment, clinical signs, CSF analysis and response to glucocorticoids, there appear to be an increasing number of cases occurring in older dogs, that displaying focal, atypical clinical signs or that develop permanent sequelae. Serology has been a useful tool in diagnosing neural angiostrongyliasis in humans. In its current form the ELISA is not sensitive or specific enough to allow a definitive diagnosis of CNA to be made using serum but is useful when applied to CSF specimens. Further refinement of the antigen or using monoclonal rather than polyclonal antibodies may improve the accuracy of the serology. Alternatively, methods such as Western Blot, Immuno-PCR or dot-blot ELISA, which have been successfully used to diagnoses angiostrongyliasis in humans, may be worthy of investigation The major differential diagnosis for CNA is neosporosis. Other differential diagnoses include idiopathic eosinophilic meningoencephalitis, parasitic infections including Toxoplasma gondii, Taenia solium, Gnathostoma spinigerum, visceral larval migrans (Toxocara canis) and schistosomiasis, fungal, bacterial, viral and rickettsial infections as well as neoplasia, trauma, drug reactions and toxicities. Treatment of CNA has been limited to glucocorticoids, however there may be adjunct therapies including anthelmintices, cyclosporine, and matrix metalloproteinase inhibitors. In Mason’s series of cases the use of anthelmintics significantly worsened the clinical outcome for patients. It does not appear, however, that the use of these agents in species other than the dog exacerbates clinical signs. Acquired immunity is short lived in rats and mice, which would suggest the same is true in dogs. Routine heartworm and intestinal parasite prophylaxis appears to have no influence on the occurrence of CNA.

canine neural angiostrongyliasis

angiostrongylus cantonensis

spinal cord disease

ELISA

dog

central nervous system

eosinophilic meningoencephalitis

EME

rat lung worm

A Novel ELISA to Detect Methionine Sulfoxide−Containing Apolipoprotein A−I

Wang, Xiao suo

January 2009

Doctor of Philosophy(PhD) / Atherosclerosis manifests a state of increased oxidative stress characterized by comparable lipid and protein oxidation in the affected arterial wall. While oxidative modification of low density lipoprotein (LDL) has been extensively studied, increasing attention has been focused recently on oxidation of high-density lipoproteins (HDL) and its functional consequences in relation to atherosclerosis. Oxidative modification is thought to generate “dysfunctional” HDL that has lost anti-atherosclerotic activities, including the ability to remove cholesterol from lipid-laden cells. Therefore, there has been much interest in the detection of oxidized HDL. Unfortunately, available methods to detect oxidized HDL are limited at present, in part because oxidative modification of HDL is a complex process and ‘oxidized HDL’ is not a chemically defined entity. What is known however is that conversion of methionine (Met) residues of apolipoprotein (apo) A-I to methionine sulfoxide (MetO) is a process that occurs commonly as HDL undergoes oxidative modification. For example, human apoA-I+16 (containing MetO86 or MetO112) and apoA-I+32 (MetO86 plus MetO112) are generated when apoA-I reacts with lipid hydroperoxides formed as a consequence of the lipoprotein being exposed to 1e−oxidants. The formation of MetO in apoA−I induced by 2e−oxidants (i.e., hydrogen peroxide, hypochlorous acid or myeloperoxidase/hydrogen peroxide/chloride system) is associated with an impaired ability of the apolipoprotein to facilitate reactions relevant to reverse cholesterol transport. In addition, a previous study has suggested the plasma content of apoA-I+32 to be increased in certain subjects that have an increased risk to develop cardiovascular disease (CVD). Moreover, the MetO content in circulating, HDL−associated apoA−I is elevated in type 1 diabetes, a disorder commonly associated with increased oxidative stress and a risk factor for atherosclerosis. Therefore, in the present study, an existing HPLC method was applied to HDL samples from the Fletcher−Challenge study, a nested case control study, to test the potential usefulness of MetO-containing apoA-I as a marker of oxidative stress and/or CVD in a general population. Plasma samples whose HDL contained detectable apoA-I+16 and/or apoA-I+32 had significantly elevated levels of F2-isoprostanes, a marker of in vivo lipid oxidation, consistent with MetO-containing apoA-I being a useful marker of in vivo protein oxidation. Despite this however, there was no significant difference between controls and cases in their concentrations of HDL apoA-I+16 and apoA-I+32 or F2-isoprostanes, suggesting that markers of protein and lipid oxidation are not associated with the risk of coronary heart disease (CHD) in this general population. A limitation of the Fletcher−Challenge study was that only 22% of the 534 HDL samples analyzed contained apoA-I+16 and/or apoA-I+32. In addition, the HPLC−based method used is expensive and time−consuming and may lack the sensitivity needed for apolipoproteins to clinical studies. Thus, a mouse monoclonal anti-human apoA-I+32 antibody (MOA−1) was raised using HPLC−purified apoA-I+32 as immunogen. A sensitive ELISA was then developed using a commercial anti-human apoA-I monoclonal antibody as capture and biotinylated MOA−1 as detection antibody, respectively. The assay detected lipid−free HPLC−purified human apoA-I+32 in a concentration-dependent manner and with a significantly lower limit of detection (i.e., 3 ng/mL) than the HPLC method (1 μg/mL). The ELISA also detected lipid-free apoA-I modified by 2e-oxidants (hydrogen peroxide, hypochlorous acid, peroxynitrite), and HDL oxidized by 1e- or 2e-oxidants and present in buffer or human plasma. Moreover, the extent of recognition of MetO by MOA−1 increased with increasing numbers of MetO in apoA−I, as assessed by the experiments with H2O2−oxidized forms of apoA−I mutants, in which one, two or three Met residues were replaced with Leu. Their detection was concentration-dependent, reproducible, and exhibited a linear response over a physiologically plausible range of concentrations of oxidized HDL. In contrast, MOA-I failed to recognize native apoA-I, native apoA-II, apoA-I modified by hydroxyl radicals or metal ions, or LDL modified by 2e-oxidants. Furthermore, MOA−1 did not detect other Met−containing proteins oxidized by either hypochlorous acid or hydrogen peroxide. Taken together, the results showed that recognition of oxidized proteins by MOA−1 is limited to MetO contained in apoA−I. Finally, in a pilot study, plasma samples obtained from subjects with coronary artery disease (CAD) proven by angiography, and samples from CAD patients undergoing percutaneous coronary intervention (PCI) were analyzed by the ELISA. The preliminary data obtained showed elevated levels of MetO-containing apoA-I in plasma samples of CAD patients compared to those of corresponding control subjects. Unexpectedly, levels of MetOcontaining apoA-I decreased PCI compared to before PCI. A possible explanation for these results is that HDL−associated apoA−I become displaced by acute phase proteins, such as serum amyloid A, in response to PCI. In summary, the ELISA developed here specifically detects apoA-I containing MetO in HDL and human plasma. As such it may provide a useful tool for investigating the relationship between oxidized HDL and CAD.

Pathogens affecting the reproductive system of camels in the United Arab Emirates : with emphasis on Brucella abortus, Bovine Viral Diarrhoea Virus and Bovine Herpes Virus-1: a serological survey in the Al-Ain region /

Hassan Taha, Tariq,

January 2007

Thesis (M. Sc.) Uppsala : Sveriges lantbruksuniv., 2007.

Diagnosis of root-infecting Phytophthora spp. /

Olsson, Christer H. B.,

January 1900

Diss. (sammanfattning) Uppsala : Sveriges lantbruksuniv. / Härtill 4 uppsatser.

Epidemiology of bovine viral diarrhoea virus and bovine herpesvirus type1 infections in dairy cattle herds : evidence of self-clearance and detection of infection with a new atypical pestivirus /

Kampa, Jaruwan,

January 2006

Diss. (sammanfattning) Uppsala : Sveriges lantbruksuniv., 2006. / Härtill 5 uppsatser.

Antígenos naturais, recombinantes e sintéticos do Mycobacterium leprae e implicações diagnósticas na hanseníase

Lobato, Janaina

25 July 2011

CHAPTER II: Objective: Our aim was to compare the performance of three serological assays in leprosy patients and their household contacts utilizing two quantitative ELISA tests using native PGL-I (PGL-1 ELISA), synthetic ND-O-HSA (ND-O-HSA ELISA), and the semi-quantitative lateral flow test (ML-Flow). Methods: Compare the performance of three immunological assays, PGL-I ELISA, ND-O-HSA ELISA, and ML-Flow were evaluated in 156 leprosy patients and 191 household contacts. Results: The sensitivity results of the PGL-1, ND-O-HSA, and ML-Flow were 68.83%, 63.65%, and 60.65%, respectively. The native and synthetic PGL-I ELISA assays detected antibodies in 22.73%, 31.82% of the paucibacillary (PB) patients, and the ML Flow test did not detect antibodies in this group. The ML-Flow test was able to discriminate patients into PB and multibacillary (MB) forms, while the native PGL-I and ND-O-HSA correlated with the bacillary load and the Ridley-Jopling clinical forms. In household contacts, the native PGL-I, ND-O-HSA, and ML-Flow assays detected seropositivity of 25%, 17%, and 10%, respectively. Conclusions: The use of ELISA and ML-Flow tests are thus recommended as additional tools in the diagnosis and classification of the clinical forms, aiding in prescribing the correct treatment regimen to prevent subsequent nerve damage and disability. CHAPTER III: Host pathogen interactions are mainly mediated by specialized molecules of the cell envelope. One of these essential mycobacterial cell wall components is the lipoarabinomannan (LAM). LAM has immunomodulatory roles, but its heterogeneity may be responsible for the differential immune response in leprosy patients and contacts. The research to structural motifs that could contribute as virulence factors and/or protective epitopes, and thereby derive effective biomarkers for diagnosis, drugs and/ or vaccines against leprosy has been very developed. Therefore, our aim was to develop specific mimetic peptides to this lipoglycan by using Phage Display of a random heptamer peptide library that may recognize a differential response in patients and contacts. We have used the anti-LAM CS-35 monoclonal antibody as a target for three rounds of selection. After sequencing and translation, peptides were pre-validated by ELISA and compared to the synthetic LAM-BSA antigen. The most reactive and repetitive peptide motif (A9) was subsequently tested against serum from 54 leprosy patients and 27 endemic controls by ELISA. The A9 phage-displayed peptide clone presented high levels of IgG antibodies in paucibacillary patients, from which 50% of them presented highly reactive sera. This reactivity has also been detected in tuberculoid, borderline-borderline and lepromatous patients. High levels of IgG1 were most frequent in endemic controls and reactional patients. On the other hand, the IgG profile and its subclasses in patients presented high levels of IgG and IgG2 and low levels of IgG1. The A9 clone presented a significant correlation with the synthetic LAM-BSA, for the IgG1 response. The highly reactive IgG response against the A9 clone was associated with the tuberculoid clinical form diagnosis, and detection of both IgG1 and IgG3 against this clone was associated with protection in endemic controls. CHAPTER IV: Heat Shock Proteins (HSPs), GroES and GroEL, are targets of strong human T-cell response, and a third of the cells responsive to M. leprae, recognize these proteins. Monoclonal antibodies mAbs CS-01 and CS-44 selected mimetic peptides that are ligands of their Fab portions, by phage display technique. Sera from 54 patients, 48 household contacts and 27 endemic controls were submitted to ELISA with B2 and A1 mimetic clones of the GroES and GroEL proteins, respectively, for detection of IgG and its subclasses. Using the mimetic clone of B2 GroES, the ELISA detected IgG antibodies present in sera of patients, contacts and endemic controls. The IgG antibodies were abundant in sera from multibacillary patients, especially in lepromatous (LL). A decline of IgG1 was found in patients and household contacts that became sick with leprosy and a raise of this subclass was present in sera of household contacts that did not develop the disease. With the mimetic clone of GroEL A1, the reactive antibodies were abundant in multibacillary patients, with a correlation with the bacillary load. In this study we observed that IgG antibodies against GroEL and GroES can be detected in the diagnosis of leprosy in serological tests produced with clones mimetics of these proteins. And the subclasses of IgG antibodies to GroES can demonstrate a targeting of antigenic molecules that induce the production of protective antibodies. / CAPÍTULO III: Objetivo: O objetivo do trabalho foi comparar a performance de três testes sorológicos em pacientes e seus contatos domiciliares utilizando dois testes quantitativos ELISA, um com o antígeno PGL-1 nativo (ELISA PGL-1), com o antígeno ND-O-HSA sintético (ELISA ND-O-HSA), e o teste semi-quantitativo do fluxo lateral (ML-FLow). Métodos: Os três testes imunológicos ELISA PGL-I, ELISA ND-O-HSA, e ML-Flow foram realizados utilizando soros de 156 pacientes com hanseníase e 191 contatos domiciliares. Resultados: Os resultados da sensibilidade dos testes ELISA PGL-1, ND-O-HSA e ML-FLow foram de 68.83%, 63.65%, e 60.65%, respectivamente. Os testes ELISA PGL-1 nativo e sintético detectaram anticorpos em 22,73% e 31,82% dos soros de pacientes paucibacilares (PB),e o teste ML-FLow não apresentou reatividade em nenhum soro. O ML-Flow foi capaz de discriminar entre os pacientes com as formas PB e multibacilares (MB), enquanto que o ELISA PGL-1 e ND-O-HSA correlacionaram com a carga bacilar e as formas clínicas de Ridley-Jopling. Em contatos domiciliares, os testes ELISA PGL-1 nativo, ND-O-HSA e Ml-FLow detectaram soropositividade de 25%, 17%, e 10%, respectivamente. Conclusões: O uso do teste ELISA e ML-Flow são recomendados no diagnóstico e classificação das formas clínicas, auxiliando na prescrição do tratamento correto e na prevenção do dano neural e da incapacidade. CAPÍTULO IV: Interação patógeno-hospedeiro é mediada principalmente por moléculas especializadas do envelope celular. Um dos componentes essenciais da parede celular das micobactérias é a lipoarabinomanana (LAM). A LAM tem um papel imunomodulador, mas a sua heterogeneidade pode ser responsável pela resposta imune diferenciada em pacientes com hanseníase e contatos. Espera-se que a pesquisa por motivos estruturais de M. leprae possam contribuir, como fatores de virulência ou epítopos de proteção, e assim, derivar biomarcadores eficazes para o diagnóstico, drogas e vacinas contra a hanseníase. Portanto, nosso objetivo foi desenvolver peptídeos miméticos específicos à LAM utilizando Phage Display de uma biblioteca aleatória de peptídeos heptameros que possam reconhecer uma resposta diferencial em pacientes com hanseníase e contatos. Nós utilizamos o anticorpo monoclonal anti-LAM, CS-35, como um alvo de três rodadas de seleção. Após seqüenciamento e tradução, os peptídeos foram pré-validados por ELISA e comparados com o antígeno sintético LAM-BSA. O motivo peptídeo mais reativo e repetitivo (A9) foi posteriormente testado contra o soro de 54 pacientes com hanseníase e 27 controles endêmicos por ELISA. O clone mimético A9 apresentou altos níveis de anticorpos IgG em pacientes paucibacibacilares (PB), sendo que 50% destes soros foram altamente reativos. Esta reação também ocorreu em pacientes tuberculóides, dimorfo-dimorfo e virchowiano. Controles endêmicos e pacientes reacionais apresentaram altos níveis de IgG1 no soro. Por outro lado, o perfil de IgG e suas subclasses em pacientes apresentou altos níveis de IgG e IgG2 e baixos níveis de IgG1. O clone A9 apresentou uma correlação positiva significativa com o antígeno LAM-BSA sintético para a resposta IgG1. A resposta de IgG altamente reativa contra o clone A9 foi associada com o diagnóstico da forma clínica tuberculóide, e a detecção de ambos, IgG1 e IgG3, contra esse clone foi associado à proteção nos controles endêmicos. CAPÍTULO V: Interação patógeno-hospedeiro é mediada principalmente por moléculas especializadas do envelope celular. Um dos componentes essenciais da parede celular das micobactérias é a lipoarabinomanana (LAM). A LAM tem um papel imunomodulador, mas a sua heterogeneidade pode ser responsável pela resposta imune diferenciada em pacientes com hanseníase e contatos. Espera-se que a pesquisa por motivos estruturais de M. leprae possam contribuir, como fatores de virulência ou epítopos de proteção, e assim, derivar biomarcadores eficazes para o diagnóstico, drogas e vacinas contra a hanseníase. Portanto, nosso objetivo foi desenvolver peptídeos miméticos específicos à LAM utilizando Phage Display de uma biblioteca aleatória de peptídeos heptameros que possam reconhecer uma resposta diferencial em pacientes com hanseníase e contatos. Nós utilizamos o anticorpo monoclonal anti-LAM, CS-35, como um alvo de três rodadas de seleção. Após seqüenciamento e tradução, os peptídeos foram pré-validados por ELISA e comparados com o antígeno sintético LAM-BSA. O motivo peptídeo mais reativo e repetitivo (A9) foi posteriormente testado contra o soro de 54 pacientes com hanseníase e 27 controles endêmicos por ELISA. O clone mimético A9 apresentou altos níveis de anticorpos IgG em pacientes paucibacibacilares (PB), sendo que 50% destes soros foram altamente reativos. Esta reação também ocorreu em pacientes tuberculóides, dimorfo-dimorfo e virchowiano. Controles endêmicos e pacientes reacionais apresentaram altos níveis de IgG1 no soro. Por outro lado, o perfil de IgG e suas subclasses em pacientes apresentou altos níveis de IgG e IgG2 e baixos níveis de IgG1. O clone A9 apresentou uma correlação positiva significativa com o antígeno LAM-BSA sintético para a resposta IgG1. A resposta de IgG altamente reativa contra o clone A9 foi associada com o diagnóstico da forma clínica tuberculóide, e a detecção de ambos, IgG1 e IgG3, contra esse clone foi associado à proteção nos controles endêmicos. / Doutor em Genética e Bioquímica

Mycobacterium leprae

Hanseníase

PGL-I

ND-O-HSA

ML-Flow

ELISA

Bioquímica

Hanseníase - Diagnóstico

Leprosy

CNPQ::CIENCIAS BIOLOGICAS::GENETICA

Clonagem e expressão do gene da nucleoproteína do vírus da bronquite infecciosa em sistemas hospedeiros eucarioto (Pichia pastoris) e procarioto (Escherichia coli)

Gibertoni, Aliandra Maura [UNESP]

20 February 2009

Made available in DSpace on 2014-06-11T19:32:54Z (GMT). No. of bitstreams: 0 Previous issue date: 2009-02-20Bitstream added on 2014-06-13T18:44:31Z : No. of bitstreams: 1 gibertoni_am_dr_jabo.pdf: 1047291 bytes, checksum: 9be7492afd065b969b043d3a6d16e4be (MD5) / Fundação de Amparo à Pesquisa do Estado de São Paulo (FAPESP) / Foram realizadas a clonagem e expressão do gene da nucleoproteína (N) de uma estirpe vacinal de referência M41 do vírus da bronquite infecciosa (VBI), como proteína recombinante de fusão, contendo uma cauda de poli-histidina na extremidade carboxi-terminal, em 2 sistemas hospedeiros; na levedura metilotrófica, Pichia pastoris e na bactéria Escherichia coli. A proteína N derivada de um isolado variante do VBI de surtos a campo no Brasil, também foi expressa em E. coli. As características bioquímicas e imunoquímicas de tais proteínas recombinantes, foram determinadas, tendo sido evidenciado maior eficiência de produção no sistema hospedeiro constituído por E. coli, comparativamente ao sistema composto por P. pastoris. Uma vez obtidas, caracterizadas e purificadas, através da técnica de cromatografia de afinidade em resina de níquel-sepharose, as preparações de proteína N recombinante expressas em E. coli e derivadas ou da estirpe de referência M41 ou do novo isolado de campo no Brasil, foram utilizadas de forma bem sucedida, como antígenos alvo de ensaios indiretos de ELISA, que foram aplicados na detecção e mensuração de anticorpos dos isótipos IgG e IgM em aves infectadas com estirpes homóloga ou variantes do VBI. Foi, também, investigada a atividade imunogênica da proteína N recombinante em aves, que depois de imunizadas e re-imunizadas com essas proteínas recombinantes, produziram no soro sanguíneo e na secreção lacrimal quantidades elevadas de anticorpos anti-VBI específicos, mas não desenvolveram proteção efetiva contra o desafio com a estirpe homóloga desse vírus. Concluindo, a proteína N recombinante do VBI expressa pela E. coli possui elevada imunogenicidade, no sentido de induzir altos níveis de anticorpos específicos, e reatividade cruzada com proteínas N de outras variantes desse vírus, tendo um grande potencial de ser aplicada em... / Two host systems, represented by Escherichia coli and Pichia pastoris were used for cloning and protein expression of the nucleoprotein (N) gene of M41 strain of infectious bronchitis virus (IBV) as a fusion recombinant protein containing a poli-histidine tag. The N protein from a new variant Brazilian field isolate was also cloned and expressed by E. coli system. The biochemical and immunochemical properties of these recombinant N proteins were determined and higher efficiency on protein production was achieved by using the E. coli expression system. Both recombinant N proteins expressed by E. coli were purified in nickel-sepharose resin and used as antigen in indirect ELISA methods for the detection of IgG and IgM antibodies in birds infected with homologous and variant IBVs. The immunogenicity of N recombinant protein was also evaluated by immunizing and re-immunizing birds and high antibody levels were generated in lachrymal secretion and serum, but no effective protection against challenge with homologous virulent stain of IBV was induced. Concluding, the recombinant N IBV protein expressed by E. coli is highly immunogenic for inducing specific and crossreactive antibodies, and can be applied in the immuno-diagnosis of IB

Bronquite

Clonagem

Teste imunoenzimático

Vírus da bronquite infecciosa

Proteína recombinante

Infectious bronchitis virus

Cloning

Protein expression

Recombinant protein

ELISA

Vírus da diarréia viral bovina: detecção e aspectos epidemiológicos

Almeida, Laura Lopes de

January 2010

O vírus da diarreia viral bovina (BVDV) é um dos principais patógenos virais dos bovinos e sua infecção causa importantes perdas na produção dos rebanhos afetados. O presente trabalho contém os estudos realizados para esclarecer determinados aspectos da epidemiologia e da detecção da infecção causada pelo BVDV no Estado do Rio Grande do Sul, Brasil. O primeiro artigo consistiu de um estudo transversal onde os níveis de anticorpos contra o BVDV em amostras de tanque de leite que foram correlacionados com os aspectos produtivos dos rebanhos. As amostras e as informações foram coletadas de 300 criações escolhidas aleatoriamente entre 1.656 associados de uma cooperativa de leite na região central do Estado do Rio Grande do Sul e que não utilizaram vacina contra BVDV nos últimos 12 meses anteriores ao experimento. Dessas, 80 foram consideradas positivas para BVDV pela detecção de anticorpos contra vírus em níveis superiores ao ponto de corte do teste de ELISA comercial utilizado. A prevalência aparente estimada foi de 26,7% e, usando um intervalo de confiança de 95%, apresentou uma variação entre 22 e 31%. Os parâmetros de produção mensal de leite, densidade de bovinos (relação vacas/hectare), tipo de armazenamento do leite e origem do sêmen não apresentaram associação com a infecção pelo BVDV, mas o aumento do número total de animais por rebanho foi correlacionado positivamente com a infecção. A prevalência estimada foi considerada baixa para uma população de rebanhos, criados em sistema semi-intensivo de produção de leite, que não usava medidas específicas de controle contra a infecção. A hipótese proposta no presente artigo é que o pequeno número de animais por rebanho está favorecendo a uma provável limpeza ou erradicação da infecção nas criações e que a prevalência encontrada deve corresponder ao ponto de equilíbrio entre a pressão de infecção e a limpeza da infecção destes rebanhos. A baixa prevalência estimada pode ser uma condição favorável para iniciar um programa de controle para BVDV na população estudada. No segundo artigo, um teste da transcrição reversa seguida da reação em cadeia da polimerase (RT-PCR) foi estabelecido para detecção do vírus nas amostras de tanque de leite dos rebanhos suspeitos de infecção ativa pelo BVDV identificados no primeiro artigo. O teste foi capaz de detectar até 0,001 TCID50 de BVDV por mL de leite. Esses resultados demonstraram uma sensibilidade analítica 100 ou 1000 vezes superior aos testes de RTPCR convencionais descritos anteriormente para leite e são semelhantes aos resultados obtidos em testes de RT-PCR em tempo real para BVDV. Na análise das amostras de campo, o teste detectou RNA viral em dois rebanhos entre os 59 analisados. Esses resultados comprovaram a capacidade do teste para identificar amostras naturalmente infectadas e a presença de vacas adultas produtivas e virêmicas em 3% dos rebanhos suspeitos de infecção. Este teste é uma alternativa rápida e sensível para monitorar a infecção pelo vírus em rebanhos leiteiros, a partir de amostras coletivas. O terceiro artigo tratou da detecção do BVDV em carrapatos Rhipicephalus (Boophilus) microplus alimentados em bovino persistentemente infectado (PI). Seu objetivo foi investigar o papel do carrapato bovino R. microplus na transmissão do BVDV. O RNA viral foi detectado nas teleóginas alimentadas no bovino PI, mas não pode ser identificado em sua progênie (ovos e larvas). Esses resultados sugeriram não haver transmissão transovariana do BVDV nos carrapatos. Por outro lado, a infestação experimental de um segundo bovino com as larvas oriundas das teleóginas contaminadas com BVDV não resultou em manifestação clínica e o animal foi negativo no teste de RT-PCR. O experimento demonstrou que o carrapato R. microplus pode ser contaminado com BVDV durante o repasto sanguíneo, reforçando a idéia de que vetores hematófagos possam estar envolvidos na disseminação da doença e merecem mais investigações. / Bovine viral diarrhea virus (BVDV) is one of the main pathogenic agents in cattle and the infection with the agent causes important production losses in the affected herds. The present work contains studies carried out to clarify some aspects of the epidemiology and detection of the infection caused by BVDV in the State of Rio Grande do Sul, Brazil. The first paper consisted of a transversal study, where antibody levels against BVDV in samples of bulk milk tank were correlated with some aspects of milk production in the herds. Samples and information were collected from 300 herds randomly chosen between 1656 associates of a dairy cooperative in the region of the central area of the state of Rio Grande do Sul, Brazil, that were not using routine vaccination against BVDV in the last 12 months previous to the experiment. Among them, 80 were considered positive to BVDV by detection of antibodies against the virus in levels above the cut off point of the commercial ELISA test used. The apparent estimated prevalence was 26.7% and, using a confidence interval of 95%, showed a range between 22 and 31%. The parameters of average milk production, bovine density (relationship cattle/hectare), milk storing process and origin of the semen were not significantly associated with BVDV infection, but the increase in the total number of cows in the herds was positively correlated with the infection. The prevalence was considered low for a population of herds raised in a semi-intensive milk production system that was not using specific measures to control the viral infection. The hypothesis proposed in the present study is that the small number of animals present in the analyzed herds would favors a likely virus clearance in the herd and that the prevalence found would correspond to a point of balance between the pressure of infection and the virus clearance. The low prevalence detected can be a favorable condition to launch a control program for BVDV in the studied population. In the second paper, a reverse transcription polymerase chain reaction (RT-PCR) was established for BVDV detection in bulk tank milk samples of the herds suspected of active infection with BVDV in the first paper. The test detected up to 0.001 TCID50 of BVDV per mL of milk. These results demonstrated an analytical sensitivity 100 to 1000 times higher than conventional RT-PCR tests described previously for milk and are similar to results obtained by the use of real time RT-PCR already published. In the analysis of field samples, the test detected viral RNA in 2 out of 59 analyzed herds. These results demonstrated the relationship between the ability of the test to identify samples naturally infected and the presence of viremic adult cows in 3% of the herds suspected of the infection. This test represents a fast and sensitive alternative for monitoring virus infection in dairy herds, through the analysis of collective samples. The third article dealt with the detection of BVDV in the tick Rhipicephalus (Boophilus) microplus fed in a bovine persistently infected (PI). The objective was to investigate the role of the cattle tick R. microplus in the transmission of BVDV. Viral RNA was detected in adult females fed on the PI bovine, but could not be identified in its progeny (eggs and larvae). These results suggest that there is no transovarial transmission of BVDV in ticks. On the other side, experimental infestation of a second bovine with larvae derived from adult cattle contaminated with BVDV did not result in clinical manifestations and the animal was negative in the RT-PCR test. The study demonstrated that the tick R. microplus can be contaminated with BVDV during blood feeding, strengthening the idea that haematophagous vectors could be involved in the dissemination of the disease and would deserve further consideration.

Virologia veterinaria : Bovinos

Epidemiologia veterinaria

Virologia veterinaria

Diarreia viral : Bovinos

BVDV

Milk

ELISA

Prevalence

RT-PCR

R. microplus

Transmission

Purifikace viru mozaiky jetele bílého (white clover mosaic virus) s následnou přípravou antiséra a izolací IgG pro sérologickou detekci viru pomocí ELISA / Purification of white clover mosaic virus, antiserum production and IgG isolation for serological detection of virus by ELISA

KOLÁŘOVÁ, Klára

January 2011

White clover mosaic virus (WClMV) virions were purified using a modified method of Wetter (1960). Antisera were produced by rabbit immunisation and virus-specific polyclonal antibodies were obtained. Suitable conditions were optimised for serological detection of virus by DAS-ELISA and compared with a commercial kit.

Development of an immunoassay panel to predict aseptic implant loosening

Ramchandra Desai, Suchita

January 2018

During our lifetime, our bones constantly go through remodelling to maintain the skeletal system. This is done by osteoblasts that deposit new bone tissue, osteoclasts that remove the bone matrix and mechanosensing osteocytes. In case of bone implants, increased resorption by osteoclasts due to inflammation (inflammatory osteolysis) leads to aseptic implant loosening. This study focuses on how to detect these inflammatory resorbing cells at an early stage and prevent their activity with appropriate medication. To achieve this, we differentiated classical monocytes into macrophage-like cells, osteoclasts(OCs) and foreign body giant cells (FBGC) and their secretome was studied to identify specific biomarkers. Previously, tartrate resistant acid phosphatase (TRAP) was studied as an important biomarker for OCs and macrophages. An ELISA to separate and quantitate the two TRAP isoforms was used to distinguish the resorbing OCs from inflammatory FBGCs on the basis of the isoform ratio. This assay gave high levels of 5b isoform for osteoclastic stimulation and high 5a levels for the inflammatory stimulation. Also, different aminothiazole inhibitors were tested which were shown to be efficient drugs in inhibiting inflammatory osteolysis by reducing osteoclast formation and resorption in sub-micromolar concentration. Further to apply this study to patient samples, an immunoassay panel can be developed which will help detect TRAP and multiple biomarkers like CTX specific to aseptic loosening simultaneously. This will help in early, efficient and accurate diagnosis of inflammatory osteolytic bone loss and provide us with an accurate diagnosis and sufficient time for appropriate treatment.

Osteoclasts

M1 macrophage

M2 macrophage

Parathyroid hormone

RANKL

Calcium

TRAP

monocytes

FBGCs

ELISA

Biological Sciences

Biologiska vetenskaper