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Papillomaviruses (PVs) have been identified in several animal species, including dogs (canine papillomaviruses, CPVs) and cattle (bovine papillomaviruses, BPVs). Although some BPVs may occasionally infect species other than cattle, to the best of our knowledge, BPVs have not been reported in dogs to date. Herein, we carried out a retrospective phylogenetic study of PVs circulating in dogs from southern Brazil between 2017 and 2022, also investigating possible mixed infections and spillover events. For this, we screened 32 canine papilloma samples by PCR using the degenerate primers FAP59/64 and/or MY09/11, which amplify different regions of the L1 gene; the genomic target often used for PV classification/typing. Out these, 23 PV DNA samples were successfully amplified and sequenced. All PVs amplified by FAP59/64 (n = 22) were classified as CPV-1. On the other hand, PVs amplified by MY09/11 (n = 4) were classified as putative BPV-1. Among these, three samples showed mixed infection by CPV-1 and putative BPV-1. One of the putative BPV-1 detected in co-infected samples had the L1 gene full-sequenced, confirming the gene identity. Furthermore, the phylogenetic classifications from the FAP59/64 and/or MY09/11 amplicons were supported by a careful in silico analysis, which demonstrated that the analysis based on them matches to the classification from the complete L1 gene. Overall, we described CPV-1 circulation in southern Brazil over the years and the potencial BPV infection in dogs (potential spillover event), as well as possible CPV/1/BPV-1 co-infections. Finally, we suggest the analysis of the complete genome of the putative BPVs detected in dogs in order to deepen the knowledge about the PV-host interactions.
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Bovine papillomaviruses (BPVs) exhibit a high degree of genetic variability, and several viral types have been identified based on analysis of the L1 gene. The L1 is the main capsid protein and the main target for neutralizing antibodies. We performed a retrospective study on BPVs circulating in Rio Grande do Sul state, Southern Brazil, in 2016-2020. DNA from 43 bovine papilloma samples were amplified using two degenerate primer sets - FAP59/64 and MY09/11 - targeting the L1 region, and analyzed for phylogeny, mixed BPV infections (coinfections) and amino acid (aa) sequences. We also performed an in silico analysis with 114 BPV L1 sequences from the GenBank database to assess the agreement between the phylogeny obtained based on complete L1 sequences versus that based on the region amplified using the FAP59/64 and MY09/11 primer sets. Considering single and coinfections, we identified 31 BPV-1 (31/43; 72.1%), 27 BPV-2 (27/43; 62.8%) and 4 BPV-6 (4/43; 9.3%). Coinfections with BPV-1 and BPV-2 were observed in 61.3% of the samples. Our results are supported by in silico analyses that demonstrate that the classification using FAP59/64 or MY09/11 matches the complete L1 results, except for BPV-17 and -18, which may be mistakenly classified depending on the primers used. Furthermore, we found unique or rare amino acids in at least one L1 sequence of each BPV type identified in our study, some of which have been identified previously in papillomavirus epitopes, suggesting immune-mediated selection. Finally, our study provides an overview of BPVs circulating in Southern Brazil over the last five years and point to the combined use of primers FAP59/64 and MY09/11 for analysis of BPV coinfections and putative epitopes.
Assuntos
Papillomavirus Bovino 1 , Doenças dos Bovinos , Coinfecção , Infecções por Papillomavirus , Animais , Bovinos , Infecções por Papillomavirus/epidemiologia , Infecções por Papillomavirus/veterinária , Filogenia , Brasil/epidemiologia , Aminoácidos/genética , Estudos Retrospectivos , DNA Viral/genética , Papillomaviridae/genética , Doenças dos Bovinos/epidemiologiaRESUMO
The aim of this study was to investigate the presence of adenovirus (AdV), rotavirus (RV), and hepatitis E virus (HEV) in beef, pork, and chicken meat cuts in retail trade in the city of Uruguaiana, RS, Brazil. A total of 131 meat products were collected (beef, n = 55; chicken, n = 47; pork, n = 29) from 18 commercial establishments (supermarkets, n = 7; butchers, n = 7; markets/grocery stores, n = 4). All samples were evaluated for AdV, RV, and HEV. The genomes of RV and AdV were identified in 29% (n = 38) and 5.34% (n = 7) of the samples, respectively. HEV was not identified in any of the samples. Chicken cuts had a higher frequency of AdV and RV isolates compared to beef and pork (P < 0.05). Among the categories of commercial establishments evaluated, all revealed at least one positive sample for AdV and RV; however, supermarkets showed a higher frequency of RV than others (P < 0.05). The genetic material of AdV and RV was identified simultaneously in 2.29% (n = 3) of samples from supermarkets (n = 2) and grocery stores (n = 1). This is the first report on detection of enteric viruses in meat cuts in the western region of the state of Rio Grande do Sul, Brazil, and the presence of AdV and RV in these products may indicate flaws during the process of handling these foods, especially in places where commercialization provides important public health issues.
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Embryonic lipids are crucial for the formation of cellular membranes and dynamically participate in metabolic pathways. Cells can synthesize simple fatty acids, and the elongation of fatty acids facilitates the formation of complex lipids. The aim of this work was to investigate the involvement of the elongation of very long chain fatty acid enzyme 5 (ELOVL5) in embryonic development and lipid determination. Bovine embryos were produced in vitro using a standard protocol and randomly divided to receive one of three treatments at Day 4: morpholino (Mo) gene expression knockdown assay for ELOVL5 (ELOVL5-Mo), Mo antisense oligonucleotides for the thalassemic ß-globulin human mRNA (technical control Mo), and placebo (biological control). The phenotypes of embryonic development, cell number, ELOVL5 protein abundance, lipid droplet deposits, and lipid fingerprint were investigated. No detrimental effects (p > 0.05) were observed on embryo development in terms of cleavage (59.4 ± 3.5%, 63.6 ± 4.1%, and 65.4 ± 2.2%), blastocyst production (31.3 ± 4.2%, 28.1 ± 4.9%, and 36.1 ± 2.1%), and blastocyst cell number (99.6 ± 7.7, 100.2 ± 6.2, 86.8 ± 5.6), respectively, for biological control, technical control Mo, and ELOVL5-Mo. ELOVL5 protein abundance and cytoplasmic lipid droplet deposition were increased (p < 0.05) in ELOVL5-Mo-derived blastocysts compared with the controls. However, seven lipid species, including phosphatidylcholines, phosphatidylethanolamines, and triacylglycerol, were downregulated in the ELOVL5-Mo-derived blastocysts compared with the biological control. Therefore, ELOVL5 is involved in the determination of embryonic lipid content and composition. Transient translational blockage of ELOVL5 reduced the expression of specific lipid species and promoted increased cytoplasmic lipid droplet deposition, but with no apparent deleterious effect on embryonic development and blastocyst cell number.
Assuntos
Blastocisto/metabolismo , Membrana Celular/química , Citoplasma/química , Elongases de Ácidos Graxos/genética , Elongases de Ácidos Graxos/metabolismo , Animais , Blastocisto/química , Bovinos , Desenvolvimento Embrionário , Elongases de Ácidos Graxos/antagonistas & inibidores , Feminino , Técnicas de Silenciamento de Genes , Humanos , Metabolismo dos Lipídeos , Morfolinos/farmacologia , Gravidez , Globinas beta/antagonistas & inibidores , Globinas beta/genéticaRESUMO
ABSTRACT: This study evaluated the sanitary hygienic quality and the presence of pathogenic microorganisms in raw meats and fresh sausages marketed in the city of Uruguaiana, Rio Grande do Sul (RS), Brazil. We analyzed 238 samples of fresh sausages, beef, pork, and chicken from 18 commercial establishments (butchers, supermarkets, and groceries). Samples were subjected to enumerate hygiene indicator microorganisms (mesophilic aerobes and enterobacteria) and detection of Salmonella spp. and Listeria monocytogenes. The mean counts of mesophilic aerobes and enterobacteria were 5.09 and 3.54 log CFU/g, respectively. Beef samples presented the highest frequency of Salmonella spp. (7.93%) and fresh sausages present the highest frequency of L. monocytogenes (19.04%). Among the analyzed samples, 43.70% did not comply with the microbiological parameters established by the Brazilian Ministry of Health. The presence of Salmonella spp. and L. monocytogenes in different samples and commercial establishments demonstrate the failures of good manufacturing practices in industrial environmental and retails points and the need to train food handlers to reduce the exposure of consumers to potential risks.
RESUMO: Este estudo teve como objetivo avaliar a qualidade higiênica sanitária e a presença de microrganismos patogênicos em carnes in natura e linguiças frescais comercializadas na cidade de Uruguaiana, Rio Grande do Sul (RS), Brasil. Foram analisadas 238 amostras de linguiças, carne bovina, suína e de frango de 18 estabelecimentos comerciais (açougues, supermercados e mercearias). As amostras foram submetidas à enumeração de microrganismos indicadores de higiene (aeróbios mesófilos e enterobactérias) e detecção de Salmonella spp. e Listeria monocytogenes. As contagens médias de aeróbios mesófilos e enterobactérias foram 5,09 e 3,54 log UFC/g, respectivamente. Salmonella spp. esteve presente mais frequentemente em amostras de carne bovina (4,91 %), enquanto L. monocytogenes foi mais frequente em linguiças frescais (19,04 %). Das amostras analisadas, 43,70 % não atenderam aos parâmetros microbiológicos estabelecidos pelo Ministério da Saúde. A presença de Salmonella spp. e L. monocytogenes em diferentes amostras e estabelecimentos comerciais demonstra falhas de boas práticas de fabricação na indústria e pontos de venda, além da necessidade de treinar manipuladores de alimentos para reduzir a exposição dos consumidores à riscos.
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The aim of this study was to investigate hepatitis A virus (HAV), hepatitis E (HEV), and rotavirus (RV) in fresh and processed meat traded on the border of Brazil with Argentina and Uruguay. In total, 159 samples of raw and processed foods of animal origin were collected in Paso de los Libres, Argentina (n = 53 raw meat, n = 24 processed meat) and Rivera, Uruguay (n = 55 raw meat, n = 18 processed meat), or were seized by the Brazilian International Agricultural Surveillance System-VIGIAGRO (Brazil-Argentina border) (n = 8 raw meat, n = 1 bush meat). All samples were tested for the presence of HAV, HEV, and RV genomes. HAV genes were detected in 18.23% of samples and RV genes in 23.89%. No HEV-positive samples were detected. HAV was also detected in two of the VIGIAGRO samples. Processed meats from Argentina and Uruguay had a higher rate of HAV and RV than raw meat (P > 0.05). The median HAV in the Argentinian and Uruguayan samples was 6.9 × 104 and 3.5 × 103 copies/g, respectively. The presence of RV viral genes in raw meats from Argentina was significant, and this was not observed in processed meats. The presence of HAV and RV genes in a significant portion of products from Argentina and Uruguay is a potential source of human infection. This also indicates precarious conditions of acquisition, processing, and manipulation, which could be improved by improved regulation of food across borders.
Assuntos
Contaminação de Alimentos , Vírus da Hepatite A/isolamento & purificação , Vírus da Hepatite E/isolamento & purificação , Produtos da Carne/virologia , Carne/virologia , Rotavirus/isolamento & purificação , Animais , Argentina , Brasil , Vírus da Hepatite A/genética , Vírus da Hepatite E/genética , Humanos , Rotavirus/genética , UruguaiRESUMO
ABSTRACT: This study aimed to characterize the outbreaks of equine infectious anemia (EIA) identified, between the years 2009 and 2015, in the western region of the state of Rio Grande do Sul, Brazil. We identified 26 positive horses on 24 properties. Each positive property was considered an outbreak of the disease. The diagnoses were made using the agar gel immunodiffusion (AGID) test as a part of the sanitary checks conducted during animal transportation or certification of the horse´s sanitary status. The positive properties included farms or horse barns, and the infected animals were used for ranch work, sports, or reproduction. One outbreak was identified in animals that were being illegally transported from Argentina to Brazil. Fifteen outbreaks occurred on properties that were not registered with the Official Veterinary Service (OVS). Eleven outbreaks were identified in urban areas and 13 in rural areas. Twelve of the 24 outbreaks were diagnosed in 2015 alone, nine of which occurred in São Borja county. On two properties, a diagnosis could not be confirmed with a retest; therefore, these outbreaks were discharged. During sanitation checks on three properties, 12 additional positive animals were identified among a population of 1,108 susceptible animals. Based on these findings, we concluded that a subclinical form of the infection is present in that area, which is linked to properties that are not registered with the OVS, and that animals which are transported illegally across international borders represent a potential risk.
RESUMO: O objetivo do estudo foi caracterizar os focos de EIA identificados, entre 2009 e 2015, na região oeste do estado do Rio Grande do Sul, Brasil. Inicialmente foram identificados 26 equinos positivos em 24 propriedades, sendo que cada propriedade foi considerada um foco. Os diagnósticos foram realizados por imunodifusão em gel de ágar (AGID) na ocasião do transporte ou como medidas sanitárias, em casos de vínculo com animais infectados ou para fim de certificação do status sanitário. Um foco foi identificado em animais transportados ilegalmente da Argentina para o Brasil. Os estabelecimentos positivos eram fazendas ou estábulos e os animais infectados utilizados para trabalho, esporte ou reprodução. Quinze focos ocorreram em propriedades não cadastradas no SVO. Onze focos localizaram-se na zona urbana e 13 em propriedades rurais. Somente no ano de 2015 foram diagnosticados 12 dos 24 focos, sendo que no munícipio de São Borja ocorreram nove surtos neste período. Em duas propriedades o resultado inicial não foi confirmado no reteste, fazendo com que estes focos fossem encerrados imediatamente. Em três propriedades, durante o saneamento, identificou-se outros 12 animais positivos em três propriedades, de uma população de 1.108 susceptíveis. Assim sendo, pode-se concluir que a infecção que está presente na região, ocorre de maneira subclínica, associada a propriedades não cadastradas no SVO e animais transportados de forma ilegal, inclusive transporte internacional ilegal.
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ABSTRACT This study sought to evaluate the occurrence of lesions suggestive of hydatidosis, cysticercosis, and tuberculosis in animals slaughtered under sanitary inspection of the Divisão de Inspeção de Produtos de Origem Animal (DIPOA), in the state of Rio Grande do Sul. Condemnation data between the years 2009 and 2017 were obtained from Secretaria da Agricultura Pecuária e Irrigação (SEAPI) and presented according to the administrative regions established by SEAPI. In that period, 7,509,544 cattle were slaughtered and condemnations occurred in all regions of the state at varying levels. The mean condemnation values showed the presence of hydatidosis in 523,399 (6.97%), cysticercosis in 92,277 (1.23%), and tuberculosis in 10,595 (0.14%) cattle carcasses. The mean values of hydatidosis diagnoses were higher in the regions of Alegrete (14.19%), Bagé (19.62%), and Pelotas (17.71%). The regions of Osório (1.86%), Santa Maria (2.10%), and São Luiz Gonzaga (1.83%) had highest rates of cysticercosis condemnations. All regions maintained an average bovine tuberculosis diagnosis rate of less than 1% and Estrela region had the highest index (0.70%). Results showed that the three diseases occurred in all regions of the state, the average prevalence rates in each region are variable, and distribution seems to be regionalized. This knowledge contributes to the plans for controlling these diseases, which are zoonoses that cause economic losses to the productive sector.
RESUMO O objetivo do estudo foi avaliar a ocorrência de lesões sugestivas de hidatidose, cisticercose e tuberculose em carcaças bovinas oriundas de abatedouros frigoríficos sob inspeção sanitária da Divisão de Inspeção de Produtos de Origem Animal (DIPOA), no Estado do Rio Grande do Sul. Os dados de condenações entre os anos de 2009 e 2016 foram obtidos junto a Secretaria da Agricultura Pecuária e Irrigação (SEAPI) e apresentados conforme as regiões administrativas estabelecidas pela SEAPI. Nesse período foram abatidos 7.509.544 bovinos e as condenações estiveram presentes em todas as regiões do estado, em níveis variáveis. Os valores médios das condenações demonstraram a presença de hidatidose em 523.399 (6,97%), cisticercose em 92.277 (1,23%) e tuberculose em 10.595 (0,14%) das carcaças bovinas. Os valores médios de condenações por hidatidose foram maiores nas regionais de Alegrete (14,19%), Bagé (19,62%) e Pelotas (17,71%). As regionais de Osório (1,86%), Santa Maria (2,10%) e São Luiz Gonzaga (1,83%) apresentaram as maiores médias para a presença de cisticercose. Todas as regiões mantiveram uma média abaixo de 1% para condenações por tuberculose bovina e a região de Estrela obteve o maior índice (0,70%). Os resultados demonstram que as três enfermidades são causas de condenações em todas as regiões do estado, os índices médios de prevalência em cada região são variáveis e a distribuição parece ser regionalizada. Esse conhecimento poderá subsidiar a elaboração de planos de controle dessas enfermidades, as quais, além do aspecto zoonótico, são responsáveis por perdas econômicas ao setor produtivo pelas condenações de carcaças e órgãos dos bovinos.
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ABSTRACT: To study the pathogenicity of the Brazilian bovine viral diarrhea virus (BVDV) type 1a 241.10 isolate, four calves were intranasally inoculated with a viral suspension containing 107.2 TCID50 mL-1. One calf was left uninoculated and kept in contact with the other calves to investigate viral transmissibility. After inoculation, the animals were monitored daily for clinical signs of infection. The presence of the virus in the blood and nasal secretions was confirmed by virus isolation in cell culture. White blood cells were quantified prior to and every 3 days after infection, and the presence of antibodies was checked every 7 days, starting at day 0 until day 42 post-inoculation (pi). After infection, nasal and ocular serous secretions were observed between days 1 and 5 pi, along with a mild cough from days 2 to 4 pi; however, no severe clinical signs were present. Body temperature was slightly elevated between days 4 and 6 pi. The control calf did not develop any of the signs observed in the infected animals. Cell culture-mediated virus isolation confirmed viremia between days 4 and 8 pi and the presence of the virus in the nasal secretions between days 1 and 10 pi. All infected animals showed a decrease in white blood cell count. Antibodies could be detected from day 14 pi, and these levels remained high until day 35 pi. The control calf had no viremia, viral presence in nasal secretions, or positive serology, indicating the absence of viral transmission. Thus, isolate BVDV 1a 241.10 has low pathogenicity and transmissibility but retains immunosuppressive capacity.
RESUMO: Com o objetivo de estudar a patogenicidade de uma amostra brasileira do BVDV-1a (241.10), quatro bovinos foram inoculados pela via intranasal com uma suspensão viral contendo 107,2 TCID50 mL-1. Um bezerro foi mantido em contato com o grupo infectado para avaliar a transmissibilidade. Após a inoculação, os animais foram monitorados diariamente para observação dos sinais clínicos. A presença de vírus no sangue e na secreção nasal foi confirmada pelo isolamento viral em cultivo celular. A contagem total de leucócitos no sangue foi realizada com intervalos de três dias pré- e pós-infecção e a detecção de anticorpos a cada sete dias, iniciando-se no dia 0 até o dia 42 pós-inoculação (pi). Após a inoculação, não foram observados sinais clínicos evidentes, apenas secreção nasal e ocular serosa entre os dias 1 e 5 pi e tosse discreta entre os dias 2 e 4 pi. A temperatura corporal teve leve aumento entre os dias 4 e 6 pi. O animal controle não desenvolveu os sinais observados no grupo infectado. O isolamento viral indicou presença de viremia entre os dias 4 a 8 pi e excreção viral na secreção nasal entre os dias 1 e 10 pi. Os animais inoculados apresentaram redução na contagem total de leucócitos no sangue. A detecção de anticorpos iniciou-se no dia 14 pi e os níveis mantiveram-se elevados até o dia 35 pi. No animal controle, não foi observada viremia, presença de vírus na secreção nasal e sorologia positiva, demonstrando ausência da transmissão. Assim sendo, conclui-se que a amostra de BVDV 1a 241.10 possui baixa patogenicidade, mantém a capacidade imunossupressora e tem baixa transmissibilidade.
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A thymidine kinase (tk)-deleted bovine herpesvirus 5 (BoHV-5tkΔ) was previously shown to establish latent infection and reactivate - even poorly - in a sheep model (Cadore et al. 2013). As TK-negative alphaherpesviruses are unlike to reactivate in neural tissue, this study investigated the sites of latency and reactivation by this recombinant in lambs. For this, groups of lambs were inoculated intranasally with the parental BoHV-5 strain (SV-507/99) or with the recombinant BoHV-5tkΔ. During latent infection (40 days post-inoculation, pi), the distribution of recombinant virus DNA in neural and non-neural tissues was similar to that of the parental virus. Parental and recombinant virus DNA was consistently detected by PCR in trigeminal ganglia (TGs); frequently in palatine and pharyngeal tonsils and, less frequently in the retropharyngeal lymph nodes. In addition, latent DNA of both viruses was detected in several areas of the brain. After dexamethasone (Dx) administration (day 40pi), the recombinant virus was barely detected in nasal secretions contrasting with marked shedding of the parental virus. In tissues of lambs euthanized at day 3 post-Dx treatment (pDx), reverse-transcription-PCR (RT-PCR) for a late viral mRNA (glycoprotein D gene) demonstrated reactivation of parental virus in neural (TGs) and lymphoid tissues (tonsils, lymph node). In contrast, recombinant virus mRNA was detected only in lymphoid tissues. These results demonstrate that BoHV-5 and the recombinant BoHV-5tkΔ do establish latent infection in neural and non-neural sites. Reactivation of the recombinant BoHV-5tkΔ, however, appeared to occur only in non-neural sites. In anyway, the ability of a tk-deleted strain to reactivate latent infection deserves attention in the context of vaccine safety.
Um recombinante do herpesvírus bovino tipo 5 com deleção no gene da timidina quinase (BoHV-5tkΔ) foi capaz de estabelecer latência e reativar - embora ineficientemente - em modelo experimental em ovinos (Cadore et al. 2013). Como a reativação de alfaherpesvírus defectivos na TK em tecido neural é improvável, o presente estudo investigou os sítios de latência e reativação por esse recombinante em ovinos. Para isso, grupos de ovinos foram inoculados com a cepa de BoHV-5 parental (SV-507/99) ou com o recombinante BoHV-5tkΔ. Durante a infecção latente (dia 40 pós-infecção, pi) a distribuição do DNA do vírus recombinante no encéfalo de ovinos infectados experimentalmente foi similar ao do vírus parental (SV-507/99). O DNA de ambos os vírus foi detectado consistentemente por PCR nos gânglios trigêmeos (TGs), frequentemente nas tonsilas faríngeas e palatinas e, com menos frequência, nos linfonodos retrofaríngeos. Após administração de dexametasona (Dx), o vírus recombinante foi raramente detectado nas secreções nasais, contrastando com excreção abundante do vírus parental. RT-PCR para mRNA de um gene tardio (glicoproteína D) realizado em tecidos de animais eutanasiados 3 dias pós-Dx demonstrou reativação do vírus parental em tecido neural (TGs) e não-neural (tonsilas, linfonodo). Em contraste, a reativação do vírus recombinante ficou restrita ao tecido linfoide. Esses resultados demonstram que tanto o BoHV-5 parental quanto o recombinante estabelecem latência em sítios neurais e não-neurais. No entanto, o recombinante BoHV-5tkΔ parece reativar apenas nos tecidos não-neurais (linfoide). De qualquer forma, a capacidade do recombinante reativar a infecção latente deve ser considerada no contexto de segurança vacinal.
Assuntos
Animais , /genética , /isolamento & purificação , Ovinos/microbiologia , Timidina Quinase/isolamento & purificação , Ativação Viral , Latência ViralRESUMO
A thymidine kinase (tk)-deleted bovine herpesvirus 5 (BoHV-5tkΔ) was previously shown to establish latent infection and reactivate - even poorly - in a sheep model (Cadore et al. 2013). As TK-negative alphaherpesviruses are unlike to reactivate in neural tissue, this study investigated the sites of latency and reactivation by this recombinant in lambs. For this, groups of lambs were inoculated intranasally with the parental BoHV-5 strain (SV-507/99) or with the recombinant BoHV-5tkΔ. During latent infection (40 days post-inoculation, pi), the distribution of recombinant virus DNA in neural and non-neural tissues was similar to that of the parental virus. Parental and recombinant virus DNA was consistently detected by PCR in trigeminal ganglia (TGs); frequently in palatine and pharyngeal tonsils and, less frequently in the retropharyngeal lymph nodes. In addition, latent DNA of both viruses was detected in several areas of the brain. After dexamethasone (Dx) administration (day 40pi), the recombinant virus was barely detected in nasal secretions contrasting with marked shedding of the parental virus. In tissues of lambs euthanized at day 3 post-Dx treatment (pDx), reverse-transcription-PCR (RT-PCR) for a late viral mRNA (glycoprotein D gene) demonstrated reactivation of parental virus in neural (TGs) and lymphoid tissues (tonsils, lymph node). In contrast, recombinant virus mRNA was detected only in lymphoid tissues. These results demonstrate that BoHV-5 and the recombinant BoHV-5tkΔ do establish latent infection in neural and non-neural sites. Reactivation of the recombinant BoHV-5tkΔ, however, appeared to occur only in non-neural sites. In anyway, the ability of a tk-deleted strain to reactivate latent infection deserves attention in the context of vaccine safety.
Um recombinante do herpesvírus bovino tipo 5 com deleção no gene da timidina quinase (BoHV-5tkΔ) foi capaz de estabelecer latência e reativar - embora ineficientemente - em modelo experimental em ovinos (Cadore et al. 2013). Como a reativação de alfaherpesvírus defectivos na TK em tecido neural é improvável, o presente estudo investigou os sítios de latência e reativação por esse recombinante em ovinos. Para isso, grupos de ovinos foram inoculados com a cepa de BoHV-5 parental (SV-507/99) ou com o recombinante BoHV-5tkΔ. Durante a infecção latente (dia 40 pós-infecção, pi) a distribuição do DNA do vírus recombinante no encéfalo de ovinos infectados experimentalmente foi similar ao do vírus parental (SV-507/99). O DNA de ambos os vírus foi detectado consistentemente por PCR nos gânglios trigêmeos (TGs), frequentemente nas tonsilas faríngeas e palatinas e, com menos frequência, nos linfonodos retrofaríngeos. Após administração de dexametasona (Dx), o vírus recombinante foi raramente detectado nas secreções nasais, contrastando com excreção abundante do vírus parental. RT-PCR para mRNA de um gene tardio (glicoproteína D) realizado em tecidos de animais eutanasiados 3 dias pós-Dx demonstrou reativação do vírus parental em tecido neural (TGs) e não-neural (tonsilas, linfonodo). Em contraste, a reativação do vírus recombinante ficou restrita ao tecido linfoide. Esses resultados demonstram que tanto o BoHV-5 parental quanto o recombinante estabelecem latência em sítios neurais e não-neurais. No entanto, o recombinante BoHV-5tkΔ parece reativar apenas nos tecidos não-neurais (linfoide). De qualquer forma, a capacidade do recombinante reativar a infecção latente deve ser considerada no contexto de segurança vacinal.
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Animais , /genética , /isolamento & purificação , Ovinos/microbiologia , Timidina Quinase/isolamento & purificação , Ativação Viral , Latência ViralRESUMO
Feline calicivirus (FCV) and feline herpesvirus type 1 (FHV-1) are the two primary causes of upper respiratory tract disease in cats. The aim of this study was to demonstrate the distribution of FCV and FHV-1 among the feline population of several counties in Rio Grande do Sul State, Brazil. To this end, conjunctival and nasal swabs were collected from 302 cats from different locations, including households, breeding catteries, veterinary clinics, animal hospitals and experimental research facilities. The samples were collected between July 2006 to June 2009. The virus isolation was performed in CRFK cells and, subsequently, the identification was confirmed by PCR. FCV, FHV-1, or both were isolated from 55 cats from 28 different locations. FCV alone was isolated from 52.7% (29/55) of the animals that tested positively, FHV-1 alone was isolated from 38.2% (21/55) of the animals that tested positively, and co-infection were detected in 9.1% (5/55) of the animals that tested positively. Virus detection was more prevalent in cats that were less than 1 year old, among animals that shared a living space with other cats, and females. FCV and FHV-1 were isolated from vaccinated cats. In addition, both viruses were isolated from cats that showed no signs of disease. The results suggest that a carrier state is common for both viruses in the evaluated population. A search for other causes of respiratory disease in that population is necessary; and further studies relating to the molecular characterization of viruses and vaccine efficacy are also necessary.
Assuntos
Animais , Gatos , Calicivirus Felino/genética , Calicivirus Felino/isolamento & purificação , Infecções por Herpesviridae , Herpesviridae/genética , Herpesviridae/isolamento & purificação , Técnicas In Vitro , Doenças Respiratórias , Reação em Cadeia da Polimerase/métodos , Gatos , Técnicas de Diagnóstico do Sistema Respiratório , Métodos Epidemiológicos , PrevalênciaRESUMO
Feline calicivirus (FCV) and feline herpesvirus type 1 (FHV-1) are the two primary causes of upper respiratory tract disease in cats. The aim of this study was to demonstrate the distribution of FCV and FHV-1 among the feline population of several counties in Rio Grande do Sul State, Brazil. To this end, conjunctival and nasal swabs were collected from 302 cats from different locations, including households, breeding catteries, veterinary clinics, animal hospitals and experimental research facilities. The samples were collected between July 2006 to June 2009. The virus isolation was performed in CRFK cells and, subsequently, the identification was confirmed by PCR. FCV, FHV-1, or both were isolated from 55 cats from 28 different locations. FCV alone was isolated from 52.7% (29/55) of the animals that tested positively, FHV-1 alone was isolated from 38.2% (21/55) of the animals that tested positively, and co-infection were detected in 9.1% (5/55) of the animals that tested positively. Virus detection was more prevalent in cats that were less than 1 year old, among animals that shared a living space with other cats, and females. FCV and FHV-1 were isolated from vaccinated cats. In addition, both viruses were isolated from cats that showed no signs of disease. The results suggest that a carrier state is common for both viruses in the evaluated population. A search for other causes of respiratory disease in that population is necessary; and further studies relating to the molecular characterization of viruses and vaccine efficacy are also necessary.
RESUMO
West Nile virus (WNV) envelope glycoproteins preM/E were stably expressed in baby hamster kidney cells and tested as antigen in a fluorescent antibody assay for WNV antibodies. Sera from horses, mice and chicken immunized with an inactivated WNV vaccine and, less consistently, sera from horses acutely infected with WNV, reacted specifically with viral antigens present in preM/E-expressing cells.
Assuntos
Humanos , Animais , Técnicas e Procedimentos Diagnósticos , Glicoproteínas/análise , Viroses , Febre do Nilo Ocidental , Vírus do Nilo Ocidental , Métodos , MétodosRESUMO
West Nile virus (WNV) envelope glycoproteins preM/E were stably expressed in baby hamster kidney cells and tested as antigen in a fluorescent antibody assay for WNV antibodies. Sera from horses, mice and chicken immunized with an inactivated WNV vaccine and, less consistently, sera from horses acutely infected with WNV, reacted specifically with viral antigens present in preM/E-expressing cells.
RESUMO
Bovine papillomaviruses (BPVs) are widespread pathogens mainly associated with benign, self-limiting, cutaneous lesions (warts). At least 8 viral types, defined by serology or nucleotide sequences of the L1 gene, have been identified to date. Different serotypes are associated with the specific type and morphology of the lesion and with particular geographical regions. This article describes the molecular identification of papillomaviruses from Brazilian cattle (n = 48) and horses (n = 1) through partial amplification and sequencing of the L1 gene. Bovine papillomavirus-1 (BPV-1) was identified in warts from 29 cattle (59%), BPV-6 from 9 cattle (18%), and BPV-2 in 8 lesions (16%). Warts of 2 cattle harbored L1 sequences of a new BPV type (BAA5), otherwise identified almost exclusively in healthy skin. The newly proposed BPV type "BR-UEL-4" was identified in a sarcoid tumor of a horse. Thus, the present report provides information on the main types of BPV involved in bovine papillomatosis in Brazil and reveals a new viral type associated with equine sarcoid, which to date has been attributed exclusively to BPV-1 and BPV-2.
Assuntos
Doenças dos Bovinos/virologia , Deltapapillomavirus/isolamento & purificação , Infecções por Papillomavirus/veterinária , Xipapillomavirus/isolamento & purificação , Animais , Brasil/epidemiologia , Bovinos , Doenças dos Bovinos/diagnóstico , Doenças dos Bovinos/epidemiologia , Infecções por Papillomavirus/diagnóstico , Infecções por Papillomavirus/epidemiologia , Infecções por Papillomavirus/virologia , FilogeniaRESUMO
Um equino, sem raça definida, macho com três anos de idade apresentou múltiplos nódulos na pele, em diversas regiões do corpo. As lesões localizavam-se predominantemente nos lábios, nas bochechas, na região submandibular e na região inguinal direita. Os tumores caracterizavam-se como sarcoides dos tipos misto, fibroblástico, verrucoso e oculto. Histologicamente apresentaram proliferação de fibroblastos dérmicos, muitas vezes ulcerado, com ou sem hiperplasia pseudoepiteliomatosa da epiderme e formação de pequenos grupos isolados de fibroblastos neoplásicos na derme superficial. Três amostras de tecido foram submetidas à extração de DNA e amplificação por PCR com oligonucleotídeos iniciadores genéricos direcionados para uma região interna do gene L1 dos papilomavírus. Os produtos resultantes da amplificação de duas amostras foram sequenciados e demonstraram identidade de 99 por cento com o papilomavírus bovino (BPV) BR-UEL-4. Essa é a primeira descrição da infecção de equinos, bem como de sua associação com sarcoide pelo BPV BR-UEL-4, um suposto novo tipo de BPV identificado recentemente no Brasil a partir de papilomas cutâneos em bovinos.
A 3-year-old, mixed breed, male horse showed multiple nodules in different areas of the skin. Lesions occurred predominantly on the lips, cheeks, and submandibular and right inguinal regions. The nodules were characterized as mixed, fibroblastic, verrucous and occult types of sarcoid. Histologically there was proliferation of dermal fibroblasts, with or without pseudoepitheliomatous hyperplasia of the epidermis (frequently ulcerated), and formation of small isolated groups of neoplastic fibroblasts in the superficial dermis. Three tissue samples were submitted to DNA extraction and PCR amplification with generic primers for the internal region of the papillomavirus L1 gene. The amplified products from two samples were sequenced and showed 99 percent identity with the bovine papillomavirus (BPV) BR-UEL-4. This is the first description of BPV BR-UEL-4 infecting a horse and causing sarcoid in this species. BPV BR-UEL-4 is a putative new BPV type recently identified in skin papillomas in a Brazilian cattle herd.
RESUMO
Os herpesvírus bovino tipos 1 (BoHV-1) e 5 (BoHV-5) são agentes virais genética e antigenicamente relacionados, associados com diversas manifestações clínicas em bovinos, incluindo doença respiratória, genital, neurológica e abortos. Estudos epidemiológicos indicam que esses vírus estão amplamente disseminados no rebanho bovino brasileiro. O diagnóstico sorológico, que permite identificar animais portadores da infecção latente, se constitui em importante ferramenta para monitoramento individual e de rebanho. O presente artigo relata a padronização de um teste imunoenzimático do tipo ELISA, com base em anticorpo monoclonal (AcM), para a detecção de anticorpos séricos que reagem contra BoHV-1 e/ou BoHV-5. Inicialmente, determinou-se o AcM mais adequado para a sensibilização das placas, as diluições apropriadas do antígeno e dos soros-teste e o ponto de corte do ensaio. Após a padronização, o ensaio foi validado testando-se 506 amostras de soro bovino, previamente testadas para anticorpos neutralizantes contra BoHV-1 e/ou BoHV-5 pela técnica de soroneutralização (SN). Comparando-se com os resultados da SN frente a BoHV-1, o teste de ELISA apresentou sensibilidade e especificidade de 96,6 por cento e 98,3 por cento, respectivamente. Os valores preditivos positivo e negativo foram de 97,6 por cento, a concordância foi de 97,6 por cento e o índice de correlação kappa entre os testes foi de 0,95, o que indica uma excelente concordância. Comparando-se com os resultados da SN frente o BoHV-5, o ELISA apresentou 94,3 por cento de sensibilidade; 97,9 por cento de especificidade; 97,1 por cento de valor preditivo positivo e 95,9 por cento de valor preditivo negativo. Para BoHV-5, a concordância entre os testes foi de 96,4 por cento e o índice de correlação foi de 0,92, também excelente. Esses resultados demonstram que o teste padronizado apresenta sensibilidade e especificidade adequados para o diagnóstico sorológico das infecções por BoHV-1 e BoHV-5...
Bovine herpesviruses 1 (BoHV-1) and 5 (BoHV-5) are antigenic and genetically related viruses associated with different clinical syndromes in cattle, including respiratory, reproductive, neurological disease and abortion. Epidemiological studies indicate the widespread distribution of both viruses among Brazilian cattle. Serological diagnosis, that allows the identification of latently infected animals, represents an important tool for individual and herd monitoring. The present article describes the standardization of a monoclonal antibody (MAb)-based immunoenzymatic test (ELISA) for detection of antibodies to BoHV-1 and/or BoHV-5. The initial steps involved the determination of the most suitable MAb, the appropriate dilutions of viral antigen and serum samples, and the cut-off value of the assay. After standardization, the ELISA was validated by testing 506 cattle serum samples previously tested for neutralizing antibodies to BoHV-1 and BoHV-5 by virus neutralizing assay (VN). Comparing to the VN for BoHV-1 antibodies, the ELISA presented sensitivity and specificity of 96.6 percent and 98.3 percent, respectively. Positive and negative predictive values were 97.6 percent, the concordance between the tests was 97.6 percent and the coefficient of correlation k (kappa) was 0.95, demonstrating an excellent correlation. Comparing to the VN for BoHV-5 antibodies, the ELISA presented 94.3 percent of sensitivity, 97.9 percent of specificity, 97.1 percent of positive predictive value, 95.9 percent negative predictive value, concordance of 96.4 percent and kappa coefficient of 0.92. These results demonstrate that the ELISA presents suitable specificity and sensitivity to be used for individual and herd serological diagnosis of BoHV-1 and BoHV-5, thus, representing an alternative for VN assays and imported ELISA kits.
Assuntos
Herpesvirus Bovino 1 , Técnicas Imunoenzimáticas/métodos , Testes Sorológicos/métodos , Testes de Neutralização/métodos , Anticorpos Monoclonais , Diagnóstico/métodos , Testes Sorológicos/veterináriaRESUMO
Bovine herpesvirus type 5 (BoHV-5) is the agent of meningoencephalitis, an important disease of cattle in South America. The neuropathogenesis of BoHV-5 infection is poorly understood and most previous research focused on the role of envelope glicoproteins in neurovirulence. Thymidine kinase (TK) is a viral enzyme necessary for virus replication in neurons and, therefore, represents a potential target for virus attenuation. The selection and characterization of BoHV-5 variants resistant to the nucleoside analog brivudin (BVDU), which selects TK-defective viruses is here described. Several BVDU-resistant clones were obtained after multiple passages in tissue culture in the presence of BVDU and one clone (BoHV-5/R-27) was further characterized. The selected clone replicated to similar titers and produced plaques with similar size and morphology to those of wild-type virus (SV507/99). The genetic stability of the resistant virus was demonstrated after ten passages in cell culture in the absence of the drug. Moreover, the drug-resistant virus showed reduced virulence in a rabbit model: virus inoculation in four rabbits did not result in disease, in contrast with 75 percent morbidity (3/4) and 50 percent mortality (2/2) among rabbits inoculated with the parental virus. These results demonstrate that BoHV-5 is sensitive to BVDU and that drug-resistant mutants can be readily selected upon BVDU treatment. BVDU-resistant mutants, likely defective in TK, retained their ability to replicate in tissue culture yet were attenuated for rabbits. This strategy to obtain TK-defective BoHV-5 may be useful to study the role of TK in BoHV-5 neuropathogenesis and for vaccine development.
Assuntos
Animais , Bovinos , Resistência Microbiana a Medicamentos , /genética , Meningoencefalite , Nucleosídeos , Patogenesia Homeopática , Timidina Quinase/análise , Timidina Quinase/isolamento & purificação , Vacinas , Bovinos , Células Clonais , Técnicas e Procedimentos Diagnósticos , Métodos , VirulênciaRESUMO
Bovine herpesvirus type 5 (BoHV-5) is the agent of meningoencephalitis, an important disease of cattle in South America. The neuropathogenesis of BoHV-5 infection is poorly understood and most previous research focused on the role of envelope glicoproteins in neurovirulence. Thymidine kinase (TK) is a viral enzyme necessary for virus replication in neurons and, therefore, represents a potential target for virus attenuation. The selection and characterization of BoHV-5 variants resistant to the nucleoside analog brivudin (BVDU), which selects TK-defective viruses is here described. Several BVDU-resistant clones were obtained after multiple passages in tissue culture in the presence of BVDU and one clone (BoHV-5/R-27) was further characterized. The selected clone replicated to similar titers and produced plaques with similar size and morphology to those of wild-type virus (SV507/99). The genetic stability of the resistant virus was demonstrated after ten passages in cell culture in the absence of the drug. Moreover, the drug-resistant virus showed reduced virulence in a rabbit model: virus inoculation in four rabbits did not result in disease, in contrast with 75% morbidity (3/4) and 50% mortality (2/2) among rabbits inoculated with the parental virus. These results demonstrate that BoHV-5 is sensitive to BVDU and that drug-resistant mutants can be readily selected upon BVDU treatment. BVDU-resistant mutants, likely defective in TK, retained their ability to replicate in tissue culture yet were attenuated for rabbits. This strategy to obtain TK-defective BoHV-5 may be useful to study the role of TK in BoHV-5 neuropathogenesis and for vaccine development.
