ABSTRACT
Abstract Background: Bovine leukemia virus (BLV) is the causative agent of enzootic bovine leukosis (EBL). This disease mainly affects cattle, causing severe economic losses to producers. Objective: To establish individual and herd seroprevalence and determine the risk factors associated with BLV seropositivity for dairy and dual-purpose cattle herds in Ecuador. Methods: A total of 2,668 serum samples from 386 herds were collected. A questionnaire, including variables related to cattle health, management and the environment was completed by each herd. A commercial blocking enzyme-linked immunosorbent assay (ELISA) test was used to determine seropositivity. A generalized estimating equation model (GEE) was developed to determine the factors associated with BLV seropositivity. Results: Individual seroprevalence of BLV infection in Ecuador was 17.3% (CI95% = 15.86-18.74%). Herd prevalence was 37.8% (CI95% = 33.0-42.6%), and intra-herd prevalence ranged between 12.5 and 100% (median: 37.5%). The risk factors associated with BLV seropositivity were artificial insemination (OR: 2,215; CI95% =1.402-3.501), concrete floors (OR: 2.178; CI95% = 1.217-3.889), presence of wild ruminants (OR: 2.998; CI95% = 1.788-5.027), and sampling season (wet; OR: 1.996; CI95% = 1.140-3.497). Conclusions: Results indicate that BLV is widespread in cattle herds in Ecuador. In addition, the study suggests that a control program to fight BLV infection should focus on controlling the risk factors identified.
Resumen Antecedentes: El virus de la leucosis bovina (BLV) es el principal agente etiológico causante de la leucosis enzoótica bovina (EBL). Esta enfermedad afecta a los bovinos causando grandes pérdidas económicas a los productores. Objetivo: Establecer la seroprevalencia y dispersión del BLV, así como los factores de riesgo asociados a la seropositividad en explotaciones lecheras y de doble propósito en Ecuador. Métodos: Se recolectó un total de 2.668 muestras de suero de 386 explotaciones. Se aplicó un cuestionario que incluyó variables relacionadas con la salud del hato, medidas de manejo, y características ambientales de cada explotación. Para los análisis serológicos se utilizó un test inmunológico ligado a enzimas (ELISA). Para definir los factores de riesgo asociados a la seropositividad a BLV se desarrolló un modelo utilizando ecuaciones de estimación generalizadas (GEE). Resultados: La seroprevalencia de BLV en Ecuador fue de 17,3% (IC95% = 15,86-18,74%). La dispersión fue de 37,8% (IC95%= 33,0-42,6%), y la prevalencia intra-hato alcanzó rangos entre 12,5-100% (media: 37,5%). Los factores de riesgo asociados a la seropositividad a BLV fueron: inseminación artificial (OR: 2,215; IC95% = 1,402-3,501), piso de concreto (OR: 2,178; IC95% = 1,217-3,889), presencia de rumiantes salvajes (OR: 2,998; IC95% = 1,788-5,027), y temporada de muestreo (húmeda; OR: 1,996; IC95% = 1,140-3,497). Conclusiones: Los resultados indican que el BLV se encuentra disperso en las explotaciones de Ecuador. Adicionalmente, se sugiere la implementación de un programa de control para la lucha contra el BLV, debiéndose considerar medidas que se enfoquen al control de los factores de riesgo identificados en esta investigación.
Resumo Antecedentes: O vírus da leucemia bovina (BLV) é o principal agente causador da leucose enzoótica bovina (EBL). Esta doença afeta o gado causando graves prejuízos econômicos aos produtores. Objetivo: Estabelecer a soroprevalência e dispersão do BLV, assim como os fatores de risco associados à soropositividade nas produções leiteiras e de duplo propósito no Equador. Métodos: Um total de 2.668 amostras de soro de 386 explorações foram coletadas. Foi aplicado um questionário que incluía variáveis relacionadas à saúde do rebanho, medidas de manejo e ambiente para cada exploração. Para a análise sorológica foi utilizado um teste imunológico sobre enzimas (ELISA) para determinação da soropositividade. Para definir os fatores de risco associados à soropositividade a BLV, foi utilizado um modelo de equações estimativas generalizadas (GEE). Resultados: A soroprevalência de BLVno Equador é de 17,3% (IC95% = 15,86-18,74%). La dispersão de 37,8% (IC95% = 33,0-42,6%), e a prevalência intra-rebanho alcançou entre 12,5-100% (media: 37,5%). Os fatores de risco associados à soropositividade a BLV foram inseminação artificial (OR: 2,215; IC95% = 1,402-3,501), chão de concreto (OR: 2,178; IC95% = 1,217-3,889), presença de ruminantes selvagens (OR: 2,998; IC95% = 1,788-5,027) e época da amostragem (úmida; OR: 1,996; IC95% = 1,140-3,497). Conclusões: Os resultados indicam que o BLV se encontra disseminado nas explorações no Equador. Adicionalmente, o estudo pode contribuir para a implementação de um programa de controle para a luta contra o BLV, devendo-se considerar ações de controle dos fatores de risco identificados nesta investigação.
ABSTRACT
Enzootic bovine leukosis (EBL) is an infectious disease caused by bovine leukemia virus (BLV) that affects cattle worldwide. Agar gel immunodiffusion (AGID) was the reference test for EBL diagnosis for many years, but enzyme-linked immunosorbent assay (ELISA) showed higher sensitivity, was faster to perform, and resulted in an objective reading. However, the importation of ELISA kits is lengthy and expensive, and currently, no AGID kits are available in Brazil. The aim of this work was to standardize an indirect ELISA (iELISA) for EBL diagnosis using BLV antigens produced in Tadarida brasiliensis lung (Tb1Lu) cells, which are Bovine viral diarrhea virus (BVDV) free, unlike fetal lamb kidney (FLK) cells, currently used for this purpose. Following standardization, iELISA results were compared with those obtained by AGID and the commercial Chekit Leucose-Serum ELISA. Compared to AGID, iELISA had 94,44% sensitivity, 75.68% specificity, 79.10% positive predictive value (PPV) and 93.30% negative predictive value (NPV), with 84% concordance and a Kappa index of 0.699. Compared to the Chekit Leucose-Serum ELISA, iELISA showed 92.60% sensitivity, 87.09% specificity, 90.27% PPV and 90,00% NPV, with 90.27% concordance and a Kappa index of 0.801. Taking into account the high agreement with the traditional tests and the absence of non-specific reactions with BVDV, the developed assay could be used as diagnostic method to control EBL in Brazil.(AU)
A leucose enzoótica bovina (LEB) é uma doença infecciosa natural dos bovinos com distribuição mundial causada pelo "bovine leukemia virus" (BLV). A imunodifusão em gel de ágar (IDGA) foi considerada por muitos anos o teste de eleição, porém ensaios imunoenzimáticos (ELISA) apresentam sensibilidade mais elevada e leitura mais rápida e objetiva. No entanto, a importação de kits de ELISA é um processo dispendioso e demorado, e atualmente não há kits de IDGA comercialmente disponíveis no Brasil. Desta forma, o objetivo deste trabalho foi padronizar um ELISA indireto (iELISA) para diagnóstico da LEB utilizando antígenos produzidos a partir do cultivo do BLV em linhagem celular Tadarida brasiliensis "lung" (Tb1Lu) livre de "bovine viral diarrhea virus" (BVDV), diferentemente do que acontece com as linhagens "fetal lamb kidney" (FLK) atualmente utilizadas na produção desses antígenos para uso em ensaios sorológicos. Após a padronização do iELISA, os resultados foram comparados com aqueles obtidos por IDGA e pelo ELISA comercial "Chekit Leucose-Serum". Comparado ao IDGA, o iELISA apresentou 94,44% de sensibilidade, 75,68% de especificidade, valor preditivo positivo (VPP) de 79,1% e valor preditivo negativo (VPN) de 93,3%, com concordância entre os testes de 84% e o índice Kappa 0,699. Quando comparado ao ELISA "Chekit Leucose-Serum", o iELISA apresentou sensibilidade de 92,6%, especificidade de 87,09%, VPP de 90,27% e VPN de 90%, com concordância de 90,27% e o índice Kappa 0,801. Portanto, devido à alta concordância com os testes tradicionais e ausência da ocorrência de reações inespecíficas com BVDV, o ensaio desenvolvido pode ser utilizado como ferramenta diagnóstica para o controle da LEB no Brasil.(AU)
Subject(s)
Animals , Cattle , Cattle/virology , Enzyme-Linked Immunosorbent Assay/methods , Enzootic Bovine Leukosis/diagnosisABSTRACT
ABSTRACT: In this work, we describe an unusual case of fibrinous pleuropneumonia caused by Pasteurella multocida associated with generalized lymphadenomegaly in a bovine. The animal had a one-month history of generalized superficial lymphadenomegaly that progressed to anorexia and submandibular oedema, resulting in spontaneous death. At necropsy, the parenchyma of the lymph nodes and multiple organs was obliterated by a dense proliferation of round neoplastic cells (lymphoma). Additionally, the neoplasm presented multifocal areas of haemorrhage and necrosis, characteristic of lymphoma. The parietal and visceral pleura and parietal pericardium were enlarged and covered diffusely with large amounts of a yellowish fibrillary material. The lungs were mildly enlarged, non-collapsed, and firm and exhibited interlobular septae that were thickened with a gelatinous material. Histopathological examination showed that the parietal and visceral pleura were enlarged due to a diffuse and severe inflammatory infiltrate composed of degenerate neutrophils associated with severe fibrin deposition, characteristic of fibrinous pleuropneumonia. Pleura and parietal pericardium fragments were cultivated in aerobic and microaerobic microbiological conditions. Round greyish colonies of gram-negative coccobacilli that were shiny and non-haemolytic were observed in sheep blood agar. The biochemical profile was indicative of Pasteurella spp. Molecular identification was performed by partial 16S rRNA amplification following sequencing. Pasteurella multocida was confirmed as the primary bacterium associated with the bovine fibrinous pleuropneumonia. We are able to infer that the lymphoma caused immunodepression, which increased the animal's susceptibility to atypical infectious microorganisms such as pathogenic P. multocida.
RESUMO: Nesse trabalho, relatamos um caso de pleuropneumonia fibrinossupurativa causada por Pasteurella multocida associada à linfoadenomegalia em um bovino. O animal apresentava aumento generalizado de linfonodos há um mês progredindo para anorexia e edema submandibular por três dias culminando com óbito. Durante a necropsia, tanto dos linfonodos quanto de diversos órgãos evidenciaram proliferação neoplásica de células arredondadas e arranjadas em mantos (linfoma). Adicionalmente, áreas multifocais de hemorragia e necrose, características de linfoma, foram observadas. As pleuras parietal e visceral e pericárdio parietal apresentavam-se espessas e recobertas por acentuada quantidade de fibrina. Os pulmões estavam aumentados, não colabados, firmes e exibiam espessamento com edema moderado de septos interlobulares. À microscopia, cortes da pleura visceral exibiram acentuado infiltrado inflamatório de neutrófilos degenerados com intensa deposição de fibrina, características da pleuropneumonia fibrinossupurativa, além de neovascularização e proliferação de fibroblastos. Amostras de pulmão e da pleura foram cultivadas em aerobiose e microaerobiose. Evidenciou-se o crescimento puro no ágar sangue ovino de colônias redondas, acinzentadas, brilhantes e não-hemolíticas, sendo caracterizadas como cocobacilos gram-negativos. As características bioquímicas do isolado foram condizentes com Pasteurella spp. Procedeu-se a identificação molecular do isolado através da amplificação parcial do gene rRNA 16S com posterior sequenciamento do produto amplificado. Deste modo foi possível a confirmação do isolado como Pasteurella multocida, sendo o agente primário da pleuropneumonia fibrinosa. Com estes dados, podemos afirmar que o linfoma causou um quadro de imunodepressão, a qual aumenta a susceptibilidade dos animais a agentes infecciosos atípicos, como a P. multocida patogênica.
ABSTRACT
The genomic diversity of Avian leukosis virus subgroup J (ALV-J) was investigated in an experimentally infected chicken. ALV-J variants in tissues from four different organs of the same bird were re-isolated in DF-1 cells, and their gp85 gene was amplified and cloned. Ten clones from each organ were sequenced and compared with the original inoculum strain, NX0101. The minimum homology of each organ ranged from 96.7 to 97.6%, and the lowest homology between organs was only 94.9%, which was much lower than the 99.1% homology of inoculum NX0101, indicating high diversity of ALV-J, even within the same bird. The gp85 mutations from the left kidney, which contained tumors, and the right kidney, which was tumor-free, had higher non-synonymous to synonymous mutation ratios than those in the tumor-bearing liver and lungs. Additionally, the mutational sites of gp85 gene in the kidney were similar, and they differed from those in the liver and lung, implying that organ- or tissue-specific selective pressure had a greater influence on the evolution of ALV-J diversity. These results suggest that more ALV-J clones from different organs and tissues should be sequenced and compared to better understand viral evolution and molecular epidemiology in the field.
Subject(s)
Animals , Avian Leukosis Virus , Avian Leukosis , Birds , Chickens , Clone Cells , Kidney , Liver , Lung , Molecular Epidemiology , Silent MutationABSTRACT
A infecção pelo vírus da leucemia bovina (VLB) leva ao desenvolvimento de linfocitose persistente (LP) ou linfossarcomas, principalmente em rebanhos bovinos leiteiros. Entretanto, os eventos que induzem tais manifestações ou o efeito da infecção na função das diferentes populações de leucócitos são pouco conhecidos. Avaliou-se o efeito da infecção pelo VLB na produção intracelular de peróxido de hidrogênio (H2O2) em leucócitos circulantes, mensurada pela fluorescência produzida pela diclorodihidrofluoresceína, utilizando-se de citometria de fluxo. As células foram obtidas de cinco vacas soronegativas; cinco vacas infectadas pelo VLB, alinfocitóticas; e cinco vacas infectadas, manifestando LP. Verificou-se que a infecção pelo VLB não altera a porcentagem de leucócitos circulantes produzindo H2O2, com ou sem prévio estímulo por adição in vitro: de 12-miristato 13-acetato de forbol (PMA); de lipopolissacarídeos de Escherichia coli (LPS); ou Staphylococcus aureus. Todavia, a produção de H2O2 em leucócitos de animais apresentando LP, com ou sem estímulo, foi menor que aquela verificada em leucócitos de animais soronegativos e de animais soropositivos alinfocitóticos. Os estímulos aumentaram a porcentagem de leucócitos produzindo H2O2 e a produção intracelular média em animais soronegativos ou naqueles infectados alinfocitóticos. Contudo, em leucócitos de vacas soropositivas manifestando LP, a fagocitose de S. aureus não elevou a porcentagem de leucócitos produzindo H2O2. Também, apenas a adição de PMA elevou a produção intracelular de H2O2 em leucócitos de fêmeas soropositivas manifestando LP. Concluiu-se que bovinos infectados pelo VLB, manifestando LP, apresentam menor produção intracelular de H2O2, demonstrando vulnerabilidade funcional refletida por imunossupressão.
Widespread Bovine Leukemia Virus (BLV) infection leads to persistent lymphocytosis (PL) or lymphosarcoma, mainly in dairy herds. Nevertheless, neither the sequence of events that conducts to these symptoms, nor the effect of infection on function of different leukocyte populations, is well known. We evaluated the effect of BLV infection on immune response of cows through the analysis of hydrogen peroxide (H2O2) intracellular production of circulating leukocytes after in vitro stimuli with phorbol-12-myristate-13-acetate (PMA), Escherichia coli lipopolysaccharides (LPS), or Staphylococcus aureus. Cells were obtained from five BLV-non infected cows, five BLV-infected, non-lymphocytotic cows, and five BLV-infected cows with PL, and analyzed by flow cytometry. Intracellular production of H2O2 was measured by dichlorodihydrofluorescein diacetate dependent fluorescence. Results showed that BLV infection does not alter the percentage of H2O2-producing circulating leukocytes (H2O2-PCL), with or without previous stimuli. However, the average of H2O2 intracellular production, with or without previous stimuli, in leukocytes obtained from cows with PL was smaller than those from cells obtained from BLV-negative cows and from BLV-infected, non-lymphocytotic cows. Moreover, stimuli increased H2O2 intracellular production and the percentage of H2O2-PCL obtained from BLVnegative cows and from BLV-infected, non-lymphocytotic cows. Conversely, neither phagocytosis of S. aureus and stimulus with LPS increases H2O2 intracellular production, nor phagocytosis increases the percentage of H2O2-PCL, when leukocytes were obtained from cows with PL. Thus, results show that BLV-infected cattle, with PL, have an impaired H2O2 intracellular production, demonstrating functional vulnerability reflected by immunosuppression.
Subject(s)
Animals , Immunosuppression Therapy/methods , Leukocytes/cytology , Enzootic Bovine Leukosis/pathology , Hydrogen Peroxide/chemistry , Virology/trendsABSTRACT
Para a avaliação funcional de monócitos de bovinos infectados pelo vírus da leucose enzoótica bovina (LEB), foram coletadas amostras de sangue de 10 vacas com sorodiagnóstico negativo (SN), 10 com sorodiagnóstico positivo e que manifestavam linfocitose persistente (LP), e 10 com sorodiagnóstico positivo alinfocitóticas (AL). Os monócitos foram separados por gradiente de densidade e aderência em placa, submetidos aos testes de viabilidade por exclusão do azul de tripan, fagocitose de partículas de Zymosan, espraiamento em lamínula de vidro e quantificação da liberação de peróxido de hidrogênio (H2O2) e de óxido nítrico (ON). Monócitos de animais com LP apresentaram os menores índices de viabilidade (P<0,001), de fagocitose (P<0,001) e de espraiamento (P=0,006). Também apresentaram maior produção de H2O2 sem prévio estímulo (P=0,001) e após estímulo in vitro com 12-miristato 13-acetato de forbol (P=0,006) do que monócitos de animais SN e AL. O aumento da produção de H2O2 proporcionado pelo estímulo foi menor (P=0,015) nos monócitos de fêmeas que manifestaram LP. Não houve diferença na produção de ON pelos monócitos segundo os grupos. Os resultados indicam que o vírus da LEB, apesar de infectar linfócitos B, altera funcionalmente os monócitos circulantes em bovinos que manifestam LP.
Assuming that the bovine leukosis virus (BLV) alters quantitatively and qualitatively bovine circulating leukocyte subpopulations, thus influencing the innate immune response, monocytes function in BLV-infected cattle was assessed. Peripheral blood was obtained from 10 BLV-negative cows (SN), 10 naturally BLV-infected, non-lymphocytotic cows (AL), and 10 BLV-infected cows with persistent lymphocytosis (PL). Monocytes were isolated by density gradient and adherence to plates. Cells were submitted to Trypan Blue dye exclusion viability assay, phagocytosis of Zymosan and cell-spreading assays, and quantification of hydrogen peroxide (H2O2) and nitric oxide (NO) production. Monocytes from cattle with PL had the lowest viability (P<0.001), phagocytosis of Zymosan particles (P<0.001), and spreading (P=0.006) rates. Additionally, monocytes from cows with PL had the highest production of H2O2 , with no prior stimulus (P=0.001), and after in vitro stimulus with phorbol 12-myristate 13-acetate (P=0.006). Nonetheless, the boost in H 2 O 2 production, provided by in vitro stimulus, observed in monocytes from cows with PL was lower (P=0.015) than that observed in monocytes from SN and AL cattle. There was no difference in NO production among groups. Results show that BLV, despite infecting B lymphocytes, alters innate immune functions of monocytes isolated from BLV-infected cows expressing PL.
Subject(s)
Cattle , Cattle , Lymphocytes , Lymphocytosis/veterinary , Monocytes , Retroviridae , Disease Transmission, Infectious , Equipment ContaminationABSTRACT
Neste trabalho são descritos os sinais clínicos, patologia clínica e patologia de 24 bovinos com leucose bovina enzoótica atendidos na Clínica de Bovinos de Garanhuns da Universidade Federal Rural de Pernambuco. Esses casos representaram 0,5 por cento de 4.758 bovinos atendidos entre os anos de 2000 e 2010. A doença afetou 22 (91,7 por cento) fêmeas e dois machos. Vinte e um animais (87,5 por cento) eram de raças leiteras (seis Holandês, 13 Girolando, um Jersey e um Pardo Suíça) e três (12,5 por cento) eram da raça Nelore. Vinte e três animais (95,8 por cento) tinham idade entre 3 e 8 anos e um era mais jovem. Todos eram criados em regime de confinamento ou semi-confinamento. Clinicamente todos os animais apresentaram aumento dos linfonodos superficias. Outros sinais frequentes foram hiporexia, diminuição da produção de leite, emagrecimento progressivo, escore corporal baixo, desidratação, hipomotilidade dos pré-estômagos e fezes alteradas e em pouca quantidade. Com menor frequência foram observados exoftalmia, dispneia e aumento de volume do útero. No leucograma foi constatada leucocitose média de 34.082/µL, com linfocitose de 21.814/µL e neutrofilia de 10.906/µL. Treze animais foram necropsiados e os demais foram enviados pelos proprietários para o abate. Dos treze animais abatidos todos apresentaram lesões nos linfonodos superficiais, seis nos linfonodos mesentéricos, seis no intestino, três no abomaso, um no coração, um no fígado, um no rúmen, um no útero e um no rim. Diante da importância desta enfermidade e dos prejuízos causados pela mesma é necessário alertar produtores sobre os cuidados a serem tomados durante a aquisição de animais, assim como da necessidade de implantar medidas que evitem a difusão da doença entre as fazendas.
The article reports epidemiological data, clinical signs, and laboratory and pathological findings in 24 cattle with enzootic bovine leukosis observed in the Clinic of Garanhuns, at the Federal Rural University of Pernambuco. The 24 cases represented 0.5 percent of 4,758 cattle examined from 2000 to 2010. The disease affected 22 (91.7 percent) females and two males. Twenty one of the animals were dairy (six Holstein, 13 girolando, one Brown Swiss and one Jersey), and three were for meat production (Nelore). Twenty three animals were 3-8 years of age and one was younger. All were raised in confinement or semi-confinement. All animals showed enlarged superficial lymph nodes. Other frequent clinical signs were hyporexia, decreased milk production, progressive weight loss, dehydration, hypomotility of the fore stomachs, and altered scant feces. Exophthalmia, dyspnea, and enlarged uterus were observed with less frequency. Leukocytosis (mean of 34,082 leukocytes/µL) with lymphocytosis (21,814 lymphocytes/µL) and neutrophilia (10,906lymphocytes/µL) was observed in the white blood count. Thirteen bovines were necropsied and 11 were slaughtered. Gross lesions were observed on the superficial lymph nodes of all animals necropsied. Six had lesions in the mesenteric lymph nodes, six in the gut, three in the abomasum, two in the uterus, one in the heart, one in the rumen, one in heart, and one in the liver. Due to the importance of enzootic bovine leukosis it is necessary for the farmers to introduce animals free of the disease and to establish a strict health policy for its control.
ABSTRACT
Se realizó un estudio sobre la seroprevalencia de la leucosis enzoótica bovina (LEB) en 360 bovinos lecheros, representativos de los municipios Pedraza y Barinas del estado Barinas, Venezuela, durante el periodo comprendido entre julio y noviembre 2007. En todos ellos se evaluó la presencia de signos clínicos compatibles con LEB (caquexia, decaimiento, y tumefacciones en los ganglios linfáticos supraescapulares e inguinales superficiales). Se recolectaron muestras de sangre, para la detección de anticuerpos y la proporción de linfocitos, lo cual se hizo mediante la prueba de ELISA y por contaje de linfocitos, respectivamente, relacionándose el porcentaje de animales seropositivos con el hallazgo de signos, tumefacciones en los ganglios y valores linfocíticos. Adicionalmente, se evaluó la seropositividad entre sexos, grupos etarios y número de partos, como factores de riesgo, mediante la prueba de Chi cuadrado (X²). Se detectaron 219 de 360 (60,83%) bovinos con anticuerpos específicos contra el virus de la LEB (VLEB), indicando una prevalencia elevada de distribución uniforme, en ambos municipios. La proporción de animales seropositivos con signos clínicos resultó ligeramente superior (33,79%) a la de los seronegativos (19,86%), aunque estos valores no fueron estadísticamente significativos. De igual manera, no se encontraron diferencias entre los seropositivos y seronegativos, en cuanto a las tumefacciones detectadas en los ganglios detectados, indicando que la ausencia de ellas no implica ausencia de infección. Las elevadas proporciones de linfocitos en los bovinos seropositivos y seronegativos resultaron similares, revelando no estar relacionadas con la infección por el VLEB. Con respecto a los factores de riesgo, la edad y el número de partos, mostraron estar asociados con la presencia de anticuerpos (P=0,0030 y P=0,0001, respectivamente), mientras que para el sexo no se detectaron. Estos resultados representan una contribución al conocimiento del comportamiento de la LEB en Venezuela.
An investigation was conducted to study the seroprevalence of enzootic bovine leukosis (EBL) in dairy cattle from the municipalities of Pedroza and Barinas, located at the State of Barinas, Venezuela, from July to November 2007. A total of 360 dairy cows were used. In all animals, the presence of clinical signs compatible with EBL, such as emaciation, weakness, tumefaction in suprascapular and superficial inguinal lymph nodes, were assessed. Blood samples positive to antibodies against EBLV were collected, specific antibodies to EBLV and lymphocyte proportion in samples were determined through the ELISA test and lymphocyte count, respectively. The percentage of positive animals was related to clinical findings, tumors, and lymphocytes values. Additionally, seropositivity among sex, age groups, and calving number, considered as risk factors, were also analyzed using the Chi square (X²) test. Of a total of 360 animals, 219 (60.83%) were positive to EBLV antibodies, indicating an elevated prevalence of uniform distribution in both municipalities. The proportion of seropositive animals with clinical signs was slightly higher (33.79%), when compared to seronegative animals (19.86%), although these values were not statistically significant. Likewise, no differences were found between serpositives and seronegatives regarding tumefaction detected, indicating that absence of such tumefaction does not imply lack of infection. The elevated amount of lymphocytes in both seropositive and seronegative animals was similar, reflecting no relationship with the infection through the EBLV. Concerning risk factors, age and calving number showed to be associated with the presence of antibodies (P=0.0030 and P=0.0001, respectively). In contrast, such association was not found for the variable sex. These results represent a contribution to the comprehension of EBL behaviour in Venezuela.
ABSTRACT
The critical time of avian leukosis virus subgroup J (ALV-J)-mediated immunosuppression was determined by body weight, relative immune organ weight, histopathology, and presence of group specific antigen and antibodies in specific pathogen-free (SPF) chickens. CD4+ and CD8+ cell activity in the spleen, total and differential leukocyte counts in blood, and viral RNA levels in spleen were measured. Significant growth suppression was observed in the two ALV-J-infected groups. A strong immune response by infected groups was present in spleen at 2-weeks-of-age, but after 4-weeks-of-age, the response decreased quickly. The thymus and bursa showed persistent immunosuppression until 4-weeks-of-age. Proliferation of fibroblasts and dendritic cells were observed in immune organs at 4- and 5-weeks-of-age. However, the granulocyte cell number was markedly lower in the infected groups than in the control group. In group 1 (day 1 infection) CD4+ cells increased during the second week but significantly decreased during the fourth week, while group 2 (day 7 infection) showed the opposite effect. Viral RNA increased significantly by the fourth week. These data identify 3~4 weeks post-infection as the key time at which the ALV-J virus exerts its immunosuppressive effects on the host.
Subject(s)
Animals , Antibodies, Viral/blood , CD4 Antigens/blood , CD8 Antigens/blood , Avian Leukosis/immunology , Avian Leukosis Virus/classification , Body Weight , Chickens , China , Enzyme-Linked Immunosorbent Assay/veterinary , Immune Tolerance , Leukocyte Count/veterinary , Poultry Diseases/immunology , RNA, Viral/genetics , Real-Time Polymerase Chain Reaction/veterinary , Reverse Transcriptase Polymerase Chain Reaction/veterinary , Specific Pathogen-Free Organisms , Spleen/immunologyABSTRACT
Avian leukosis virus subgroup J (ALV-J) is a new type of virus that mainly induces myeloid leukosis (ML) in chickens. To further elucidate the pathogenesis of ALV-J infection and tumor development, expression profiles from the bone marrow tissue of 15 infected and 18 non-infected birds from a local-breed poultry-farm under naturally infected conditions, were analyzed by suppression-subtractive hybridization. The birds were diagnosed as ML+ (or ML-) by specific ALV-J detection methods, involving serological tests for antigens and antibodies, and RT-PCR to detect viral RNA. A total of 59 partial gene sequences were revealed by differential screening of 496 forward and 384 reverse subtracted cDNA clones. Of these, 22 identified genes, including 8 up-regulated and 14 down-regulated, were related to immune functions, these genes being, MHC B-G antigen, translationally-controlled tumor protein (TPT1/TPTC), transferrin and ferritin, hemoglobin and Carbonic anhydrase. Four of the down-regulated genes were selected for further analysis, in view of their predicted roles in infection and immunity by real-time qRT-PCR, using RNA collected from the same birds as those used for SSH. The four genes were expressed at significantly lower levels (p < 0.001) in ALV-J infected birds than in non-infected ones.
ABSTRACT
An exogenous avian leukosis virus (ALV) strain SDAU09C1 was isolated in DF-1 cells from one of 240 imported 1-day-old white meat-type grand parent breeder chicks. Inoculation of SDAU09C1 in ALV-free chickens induced antibody reactions specific to subgroup A or B. But gp85 amino acid sequence comparisons indicated that SDAU09C1 fell into subgroup A; it had homology of 88.8% - 90.3% to 6 reference strains of subgroup A, much higher compared to other subgroups including subgroup B. This is the first report for ALV of subgroup A isolated from imported breeders.
ABSTRACT
La leucosis enzoótica bovina (LEB), también conocida como leucosis viral bovina (LVB), es una enfermedad neoplásica de origen viral, producida por un oncornavirus tipo C (retroviridae) que ocurre con o sin formación de nódulos neoplásicos. La leucosis bovina (LB) en Venezuela ha sido diagnosticada clínicamente en base a las manifestaciones y evidencias clínico patológicas, así como sobre los cambios anatomopatológicos que han sido descritos en algunos casos, pero ninguno publicado. Se han hecho reportes de esta enfermedad en bovinos de leche, evidenciando la presencia de casos sin formación de nódulos neoplásicos, los cuales han sido considerados sospechosos, en razón de no haber realizado pruebas serológicas en el laboratorio. De igual forma, se han descrito casos de leucosis con formación de nódulos neoplásicos en diferentes órganos y han sido reportados como casos sospechosos de LB. La literatura refiere la existencia de cuatro (4) formas de leucosis: multicéntrica adulta, juvenil poco común, tímica y cutánea. Esta clasificación, es referida a los casos con presencia de nódulos neoplásicos constituidos por tejido linfoide anaplástico, sobre el cual se fundamenta el diagnóstico anatomopatológico. En el presente trabajo se reporta un caso de linfoma o linfosarcoma multicéntrico que se describe como sospechoso de LB en una búfala de agua de 10 años de edad en el estado Mérida, Venezuela, fundamentado en el diagnóstico anatomopatológico, con descripción de los cambios macro y microscópicos observados. Adicionalmente se reporta una ocurrencia de 2 por ciento de positividad a LB mediante las técnicas ELISA y AGID en el rebaño (300 búfalos) de la misma procedencia del caso descrito.
Bovine Enzootic Leukosis (BEL), also known as Viral Bovine Leukosis (VBL), is a viral, oncornavirus type C (retroviridae), neoplasic disease which occurs with or without neoplasic nodules. The disease has been clinically and morphologically diagnosed as suspicious cases in Venezuela since lab serological tests were not performed. Macroscopic and microscopic changes have been described in a few cases with neoplastic nodules and referred as a Bovine leukosis (BL), but none has been published. Bovine leucosis has also been referred in milking cows with or without neoplasic nodules, most cases have not been diagnosed by blood serum analysis and considered to be only suspicious cases. There are four distinct forms of BL (adult mullticentric, juvenile uncommon, thymic and cutaneous) have been reported in the literature around the world, this classification is based upon the presence of neoplasic nodules composed of anaplastic lymphoid tissue. This work reports a case of multicentric form of bovine lymphoma which could be suspicious of BL, in a 10 years old female water buffaloe in Mérida State, Venezuela. This report of one case of lymphosarcoma is supported by macroscopic and microscopic changes described. Aditionally, a frequency of 2 percent of positive cases diagnosed by ELISA and AGID tests is reported in the herd (300 buffaloes) of similar procedence of the described case.
Subject(s)
Cattle , Animals , Buffaloes/abnormalities , Enzootic Bovine Leukosis/diagnosis , Lymph Nodes/pathology , Enzyme-Linked Immunosorbent Assay/methods , Enzyme-Linked Immunosorbent Assay/veterinary , Veterinary MedicineABSTRACT
This paper evaluated the epidemiological situation of the enzootic bovine leucosis from 1995 to 2005, in Portugal. With exception of the South region, Algarve, the disease was distributed throughout the country, being more prevalent in the north, between Douro and Minho and Trás-os-Montes, than in the centre. A decrease in prevalence and incidence of the infection throughout the studied period was also observed.
Subject(s)
Communicable Disease Control/methods , Immunodiffusion/methods , Enzootic Bovine Leukosis/epidemiologyABSTRACT
Avaliou-se, por citometria de fluxo, a fagocitose de Staphylococcus aureus conjugados com iodeto de propídio (IP), por leucócitos circulantes obtidos de cinco fêmeas bovinas negativas no sorodiagnóstico para a Leucose Enzoótica Bovina (LEB); de cinco fêmeas infectadas, manifestando linfocitose persistente (LP); e de cinco fêmeas infectadas, porém alinfocitóticas. Observou-se que, entre as amostras dos animais soronegativos, a porcentagem média de células realizando fagocitose (12,90%) não diferiu da observada entre as células dos animais alinfocitóticos (14,70%). Contudo, ambas foram maiores (p=0,047) que aquela verificada entre as células obtidas de animais manifestando LP (7,20%). Além disso, a intensidade média de fagocitose (caracterizada pela intensidade de fluorescência do IP, em valores arbitrários), verificada em leucócitos de animais manifestando LP (17,43) foi menor (p<0,001) que a observada em leucócitos de animais alinfocitóticos (29,50), e que a observada em leucócitos de animais soronegativos (25,18), que não diferiram entre si. Assim, os resultados permitem-nos alvitrar que há alteração na função fagocítica de leucócitos circulantes em animais infectados pelo vírus da LEB, manifestando LP.
This study evaluated the phagocytosis of propidium iodide-labeled Staphylococcus aureus (PI-Sa) by circulating leukocytes obtained from five Enzootic Bovine Leukosis (EBL)-negative cows, five naturally EBL-infected, non-lymphocytotic cows, and five EBL-positive cows with persistent lymphocytosis (PL), analyzed by flow cytometry. Among cells obtained from EBL-infected cows, presenting PL, the percentage of leukocytes carrying out phagocytosis (7.20%), was smaller (p=0.047) than that verified among cells obtained from non-infected (12.90%), and from BLV-infected, non-lymphocytotic cows (14.70%). Furthermore, leukocytes obtained from EBL-infected cows, presenting PL, showed smaller phagocytosis intensity (characterized by the intensity of propidium iodide fluorescence) than leukocytes obtained from non-infected and from EBL-infected, non-lymphocytotic, cows (p<0.001). Therefore, results show a decreased phagocytic function among circulating leukocytes obtained from BLV-infected, lymphocytotic cows.
Subject(s)
Animals , Cattle , Flow Cytometry/methods , Enzootic Bovine Leukosis/diagnosis , Phagocytosis , Staphylococcus aureus/isolation & purification , Leukocyte Disorders/metabolismABSTRACT
We examined lymphocyte subpopulations of peripheral blood from BLV infected and noninfected Holstein-Friesian dairy cattle reared in Korea by flow cytometry using monoclonal antibodies specifically reactive with bovine leukocyte differentiation marker. Lymphocyte subpopulations expressing BoCD11b, B-B2, CD5, B, MHC II-DP, MHC II-DQ, and MHC II-DR antigens were significantly abundant in the BLV(+) group than the BLV(-) group (p<0.01). On double staining, subpopulation of B-1a(BoCD5+ BoCD11b+) lymphocytes was significantly increased in leukemic group. However, T-lymphocyte lineage expressing BoCD2, BoCD4, BoCD8, and WC1 antigens was significantly lower than in the BLV(+) group (p<0.01). However the absolute number of T-lymphocytes expressing BoCD2, BoCD4, BoCD8, and WC1 antigens in BLV(+) group remained with in the normal range. Furthermore mean ratio of BoCD4/BoCD8 in the BLV(+) groups was higher than that in the BLV(-) group. Taken together, cellular immune responses did not seem to significantly be decreased in the leukemic cattle.
Subject(s)
Animals , Cattle , Antibodies, Monoclonal , Enzootic Bovine Leukosis , Flow Cytometry , Immunity, Cellular , Korea , Leukemia Virus, Bovine , Leukocytes , Lymphocyte Subsets , Lymphocytes , Reference Values , T-LymphocytesABSTRACT
Studies were performed to determine the effects of Bcell suppression on the pathogenesis of Subgroup J avian leukosis virus (ALV-J) in broiler chickens. Neonatal chickens were treated with cyclophosphamide (CY) or PBS, and then infected with ALV-J (ADOL-7501) at 2 weeks of age. CY treatment induced B cell specific immunosuppression throughout the experiment confirmed by decreased bursal weight, intact lymphocyte mitogenetic activity stimulated by Con A and increased relative subpopulation of CD3-positive cells as measured by flow cytometry. Chickens in this experiment had Mareks disease virus exposure prior to three weeks of age as determined by the presence of lymphocytic infiltration and antibody. Virus neutralizing antibody against ALV-J was first observed at 6 weeks post-infection in some of the infected chickens in the PBS group. As expected, none of the chickens from the CY group and uninfected chickens developed virus-neutralizing antibody. The viremic status was measured by real time RT-PCR using SYBR green I dye. The percentage of viremic chickens was significantly higher, and more chickens had high titered viremia, in the CY treated group. No neoplastic foci consistent with ALVJ infection were observed in any of the experimental chickens. The frequency and intensity of viral antigen expression determined by immunohistochemistry was significantly higher in tissues from CY treated birds than those of PBS treated chickens at 3 weeks post-infection. This study showed that B cell specific immunosuppression with CY treatment in chickens resulted in increase in viremia and viral antigen load in tissues.
Subject(s)
Animals , Avian Leukosis/immunology , Avian Leukosis Virus/genetics , Body Weight/physiology , Bursa of Fabricius/immunology , Chickens , Concanavalin A/immunology , Cyclophosphamide/pharmacology , Flow Cytometry/veterinary , Immunocompromised Host , Immunohistochemistry/veterinary , Immunophenotyping/veterinary , Immunosuppressive Agents/pharmacology , Lymphocyte Activation/drug effects , Organic Chemicals/chemistry , Poultry Diseases/immunology , RNA, Viral/chemistry , Random Allocation , Reverse Transcriptase Polymerase Chain Reaction/veterinary , Spleen/immunology , Statistics, Nonparametric , Viremia/veterinaryABSTRACT
In this study, we investigated the effects of T-cell suppression on the pathogenesis of subgroup J avian leukosis virus (ALV-J). Chickens were treated with cyclosporin A (CSP) 50 mg/Kg body weight or a corresponding volume of olive oil per every three days after hatching until the end of experiment. Some of the chickens from each treatment group were infected with an isolate of ALV-J, ADOL-7501, at 2 weeks of age. The effects of viral infection were compared to uninfected birds in same treatment group. Intramuscular injection of CSP induced significant T-cell specific immunosuppression determined by decreased cutaneous basophilic hypersensitivity response and decreased lymphocyte mitogenic activity using concanavalin A. Most of the chickens examined had Marek's disease virus infection prior to 3 weeks of age. The percentage of antibody-positive birds and antibody titers were similar in infected chickens between both treatment groups. The ratio of viremic chickens was significantly higher in CSP treated group than that of the Oil treated group. Microscopically, one CSP treated chicken had a nephroblastoma at 10 weeks post infection. At 7 and 10 weeks post-infection, more chickens had myeloid cell infiltrations in multiple organs including heart, liver and occasionally lung. Expression of ALV-J viral antigen determined by immunohistochemical staining was significantly higher in CSP treated chickens than Oil treated chickens at 10 weeks post-infection. This study indicated that chemically-induced T-cell suppression may enhance pathogenicity of the AVL-J virus in broilers.
Subject(s)
Animals , Antibodies, Viral/blood , Avian Leukosis/immunology , Avian Leukosis Virus/genetics , Body Weight , Chickens , Cyclosporine/pharmacology , Dermatitis, Contact/immunology , Flow Cytometry , Immunocompromised Host , Immunohistochemistry/veterinary , Immunophenotyping , Immunosuppressive Agents/pharmacology , Lymphocyte Activation/immunology , Marek Disease/immunology , RNA, Viral/chemistry , Reverse Transcriptase Polymerase Chain Reaction/veterinary , T-Lymphocytes/immunology , Viremia/veterinaryABSTRACT
The prevalence of bovine leukaemia virus (BLV) was determined, through the anti-BLV serum antibody test, in 661 samples collected in 16 dairy herds from four municipalities in the micro region of Manaus, at the Amazonas state. The agar gel immunodiffusion test with an envelop glycoprotein virus-antigen (gp-51) was used as a method of diagnosis the infection or the presence of anti-BLV antibodies transferred passively by the colostrum to calves up to six- month-old.. ll herds were positive for the BLV test. The overall prevalence was 8.9%. When the calves less than six-month-old were excluded a rate of 9.6% (58/604) infection prevalence was found. The influence of the age and sex factors on the prevalence of BLV were analysed by the two-proportion test. Higher prevalence rate was found in cattle older than 12-month-old as compared to the younger calves. No sexual effect was found.
Determinou-se a prevalência de anticorpos séricos anti-Vírus da Leucose dos Bovinos (anti-VLB) em 661 amostras de soro sangüíneo, colhidas em 16 rebanhos leiteiros criados em quatro municípios da Microrregião de Manaus, no Estado do Amazonas (Manaus, Iranduba, Autazes e Careiro da Várzea). Para detecção de anticorpos anti-VLB utilizou-se o teste de Imunodifusão Radial Dupla de Ouchterlony em gel de ágar, com uso do antígeno glicoprotéico (gp-51) da cápsula do vírus. Os resultados demonstraram a ocorrência da Leucose Enzoótica dos Bovinos nos rebanhos estudados, sendo a taxa de prevalência de anticorpos séricos anti-VLB na população examinada igual a 8,9% (59/661), com a exclusão dos animais com menos de seis meses de idade, nos quais a sororeação positiva poderia representar transferência passiva de anticorpos colostrais, verificou-se uma taxa de prevalência da infecção igual a 9,6% (58/604). Os animais avaliados, foram estratificados em grupos de acordo com a faixa etária e sexo. A análise dos resultados obtidos, pelo teste de duas proporções, permitiu concluir que a prevalência de bovinos portadores de anticorpos anti-VLB foi significativamente maior nos animais com mais de 12 meses de idade, não havendo diferenças significativas nos resultados obtidos entre machos e fêmeas.
ABSTRACT
Two subgroup J avian leukosis viurses (ALVs) were isolated from broiler breeder flocks, in which myeloid leukosis had occurred. The isolates could be classified as subgroup J ALV. by the positive reaction in polymerase chain reaction (PCR) with primers specific for subgroup J ALV. Two isolates replicated in chicken embryo fibroblast (CEF) cells from the alv6 chicken line in which cells are resistant to subgroup A and E ALVs. In in vitro serum neutralization tests with other subgroup ALVs including ADOL-Hc1, the prototype of subgroup J ALVs isolated in the United States of America, two isolates were partially neutralized by antibody to ADOL-Hc1, indicating that Korean isolates and ADOL-Hc1 may be antigenically related, but not identical. When the PCR was done with a primer pair designed to amplify genes of E element and long terminal repeat of proviral DNA, the PCR product size of one isolate (KOAL-PET) was smaller than that of ADOL-Hc1, suggesting that some sequences in these regions are deleted.
Subject(s)
Animals , Chick Embryo , Antibodies, Viral/immunology , Antigens, Viral/immunology , Avian Leukosis/virology , Avian Leukosis Virus/classification , Cell Line , Chickens/virology , Korea , Neutralization Tests , Polymerase Chain Reaction , Poultry Diseases/virologyABSTRACT
The occurrence of the infection with Bovine Leukosis Virus (BLV) was examined in agar-gel immunodiffusion (AGID) test and with indirect enzyme-linked immunosorbent assay (ELISA), in the State of Pará, Brazil. The blood sera were collected from different breeds including Nelore, Piemontes, Simental, Holstein Frisian, Indubrasil, Girolanda, Simbrasil and their cross-breedings. The majority of the animals were adults. The overall occurrence of infections was 49.8% (359/721) and 26.0% (174/668) for ELISA and AGID test, respectively. All animal groups examined showed infection in ELISA, however in the AGID test two groups were sera negative.(AU)
A ocorrência da infecção pelo Vírus da Leucose Enzoótica dos Bovinos (BLV) no Estado do Pará, foi estudada através do método de imunodifusão em ágar-gel (AGID) e por um ensaio imunoenzimatico (ELISA) indireto, paralelamente. Os exames foram realizados com amostras de soros sanguíneos oriundos de bovinos de diferentes raças sendo a maioria deles adultos. A prevalência observada foi de 49,8% (359/721) no ELISA e 26,0% (174/668) no AGID. Todos os 14 grupos dos animais estudados pelo ELISA indireto, mostraram a existência da infeção, enquanto que pelo método da AGID, dois grupos de animais foram negativos.(AU)