PESQUISA VETERINÁRIA BRASILEIRA

Abstract in English:

ABSTRACT.- Groff A.C.M., Kirinus J.K., Sá e Silva M., Machado G., Costa M.M. & Vargas A.P.C. 2010. Polymerase chain reaction for the diagnosis of bovine genital campylobacteriosis. Pesquisa Veterinária Brasileira 30(12):1031-1035. Laboratório de Bacteriologia, Departamento de Medicina Veterinária Preventiva, Centro de Ciências Rurais, Universidade Federal de Santa Maria, Av. Roraima 1000, Santa Maria, RS 97105-900, Brazil. E-mail: agueda.vargas@gmail.com Bovine genital campylobacteriosis is a common venereal disease of cattle; the prevalence of this disease can be underestimated mostly because of the nature of the etiological agent, the microaerobic Campylobacter fetus subspecies venerealis. The purpose of the current study was to evaluate the utilization of polymerase chain reaction (PCR) in the diagnosis of genital campylobacteriosis in samples obtained from bull prepuce aspirate, cow cervical mucus, and abomasum contents of aborted fetuses, collected into enrichment medium. Five different DNA extraction protocols were tested: thermal extraction, lysis with proteinase K, lysis with guanidine isothiocyanate, lysis with DNAzol, and lysis with hexadecyltrimethylammonium bromide (CTAB). The specificity, sensitivity, and technical application of the PCR assay were also evaluated with clinical samples and compared to bacterial isolation by standard culture. DNA extraction by the CTAB protocol provided better results in PCR, and it was able to detect 63 colony-forming units per ml of C. fetus. Out of 277 clinical samples tested, 68 (24%) were positive for Campylobacter fetus using PCR, while only 8 (2.8%) of the samples were positive by bacterial isolation in solid medium, proving the superiority of the PCR technique when compared to the standard isolation method, and providing evidence for its usefulness as a better screening test in cattle for the diagnosis of bovine genital campylobacteriosis.

• Bovine genital campylobacteriosis campylobacteriosis Campylobacter fetus campilobacteriose genital bovina

Abstract in Portuguese:

RESUMO.- Groff A.C.M., Kirinus J.K., Sá e Silva M., Machado G., Costa M.M. & Vargas A.P.C. 2010. Polymerase chain reaction for the diagnosis of bovine genital campylobacteriosis. [Reação em cadeia da polimerase para o diagnóstico de campilobacteriose genital bovina.] Pesquisa Veterinária Brasileira 30(12):1031-1035. Laboratório de Bacteriologia, Departamento de Medicina Veterinária Preventiva, Centro de Ciências Rurais, Universidade Federal de Santa Maria, Av. Roraima 1000, Santa Maria, RS 97105-900, Brazil. E-mail: agueda.vargas@gmail.com RESUMO.- [Reação em cadeia da polimerase para o diagnóstico de campilobacteriose genital bovina.] Campilobacteriose genital bovina é uma doença venérea comum em bovinos. A prevalência desta doença pode ser subestimada na maioria das vezes pela natureza microaeróbica do agente etiológico, Campylobacter fetus subspecies venerealis. O propósito do presente estudo foi avaliar a utilização da reação de polimerase em cadeia (PCR) no diagnóstico de campilobacteriose genital em amostras obtidas de aspirado prepucial de touros, muco cervical de vacas e conteúdo abomasal de fetos abortados, coletados em meio enriquecido. Cinco protocolos diferentes de extração de DNA foram testados: termo extração, lise com proteinase K, lise com guanidine isothiocyanate, lise com DNAzol e lise com hexadeciltrimetilamônio brometo (CTAB). A especificidade, sensibilidade e a aplicação da técnica da PCR foram também avaliadas com amostras clínicas e comparadas com bactérias isoladas por cultura padrão. DNA extraído pelo protocolo de CTAB demonstrou os melhores resultados na PCR, e foi capaz de detectar 63 unidades formadoras de colônias de C. fetus por ml de meio. Das 277 amostras clínicas testadas, 68 (24%) foram positivas para Campylobacter fetus pela PCR, enquanto 8 (2,8%) das amostras foram positivas por isolamento bacteriológico, provando a superioridade da técnica de PCR quando comparada com métodos padrão de isolamento, e fornecendo evidências de sua utilização como um teste de melhor projeção para diagnóstico em campilobacteriose genital bovina.

Abstract in English:

ABSTRACT.- Feitosa F.L.F., Camargo D.G., Yanaka R., Mendes L.C.N, Peiró J.R., Bovino F., Lisboa J.A.N., Perri S.H.V. & Gasparelli E.R.F. 2010. [Index of failure of passive transfer (FPT) in Holstein and Nelore calves at 24 and 48 hours of life: suggestion of total protein, gamma globulin, immunoglobulin G and gamma glutamyl transferase serum activity values for diagnosis of FPT.] Índices de falha de transferência de imunidade passiva (FTIP) em bezerros holandeses e nelores, às 24 e 48 horas de vida: valores de proteína total, de gamaglobulina, de imunoglobulina G e da atividade sérica de gamaglutamiltransferase, para o diagnóstico de FTIP. Pesquisa Veterinária Brasileira 30(8):696-704. Curso de Medicina Veterinária, Universidade Estadual Paulista, Campus de Araçatuba, Rua Clóvis Pestana 793, Araçatuba, SP 16050-680, Brazil. E-mail: leydsonf@fmva.unesp.br In an attempt to determine the passive immunity failure in Holstein and Nelore calves, 413 blood samples were drawn from animals from both breeds. Calves born from pluriparous cows, from both breeds, and Holstein calves had greater serum concentrations of total protein, gamma globulin and IgG than Nelore newborns. However, the passive immune failure index was higher in Holstein calves than those found in Nelore calves at 24 and 48 hours. Some values of serum components were established to predict the passive immunity failure in dependency of environmental antigenic challenge.

• IgG passive immunity imunidade passiva

Abstract in Portuguese:

RESUMO.- Feitosa F.L.F., Camargo D.G., Yanaka R., Mendes L.C.N, Peiró J.R., Bovino F., Lisboa J.A.N., Perri S.H.V. & Gasparelli E.R.F. 2010. [Index of failure of passive transfer (FPT) in Holstein and Nelore calves at 24 and 48 hours of life: suggestion of total protein, gamma globulin, immunoglobulin G and gamma glutamyl transferase serum activity values for diagnosis of FPT.] Índices de falha de transferência de imunidade passiva (FTIP) em bezerros holandeses e nelores, às 24 e 48 horas de vida: valores de proteína total, de gamaglobulina, de imunoglobulina G e da atividade sérica de gamaglutamiltransferase, para o diagnóstico de FTIP. Pesquisa Veterinária Brasileira 30(8):696-704. Curso de Medicina Veterinária, Universidade Estadual Paulista, Campus de Araçatuba, Rua Clóvis Pestana 793, Araçatuba, SP 16050-680, Brazil. E-mail: leydsonf@fmva.unesp.br Com o objetivo de determinar os índices de falha de transferência de imunidade em bezerros holandeses e nelores foram selecionadas, aleatoriamente, 413 amostras sanguíneas de animais de ambas as raças. Os filhos de vacas pluríparas e os bezerros holandeses apresentaram maiores níveis séricos de proteína total, da fração gamaglobulina e de IgG, do que bezerros da raça Nelore. Contudo, os índices de falha de transferência de imunidade passiva foram mais elevados nos animais da raça Holandesa, às 24 e 48 horas de idade. Estabeleceram-se valores de alguns componentes séricos para o diagnóstico de falha de transferência de imunidade passiva, de acordo com o desafio antigênico ambiental.Com o objetivo de determinar os índices de falha de transferência de imunidade em bezerros holandeses e nelores foram selecionadas, aleatoriamente, 413 amostras sanguíneas de animais de ambas as raças. Os filhos de vacas pluríparas e os bezerros holandeses apresentaram maiores níveis séricos de proteína total, da fração gamaglobulina e de IgG, do que bezerros da raça Nelore. Contudo, os índices de falha de transferência de imunidade passiva foram mais elevados nos animais da raça Holandesa, às 24 e 48 horas de idade. Estabeleceram-se valores de alguns componentes séricos para o diagnóstico de falha de transferência de imunidade passiva, de acordo com o desafio antigênico ambiental.

Abstract in English:

ABSTRACT.- Ramos C.A.N., Araújo F.R., Souza I.I.F., Guedes Jr D.S., Oliveira R.H.M., Farias T.A., Oliveira J.B., Alves L.C. & Faustino M.A.G. 2010. [Comparison between several antigens for diagnosis of Anaplasma marginale by ELISA.] Comparação entre diversos antígenos para o diagnóstico de Anaplasma marginale por ELISA. Pesquisa Veterinária Brasileira 30(1):37-41. Laboratório de Doenças Parasitárias, Departamento de Medicina Veterinária, Universidade Federal Rural de Pernambuco, Recife, PE 52171-900, Brazil. E-mail: carlosanramos@yahoo.com.br Bovine anaplasmosis is a major disease in tropical and subtropical regions of the world by determine economical loss due mortality and productive reduction. The disease is caused by Anaplasma marginale, an intraerythrocytic rickettsia whose control requires, besides an efficient vaccine, the accurate identification of chronically infected cattle. Although the existence of diverse methods of diagnosis of this rickettsia, the serological methods, in particular the enzyme immunosorbent assays (ELISAs), are the most used due to its versatility and practice. However, due to the high number of antigens currently available, an evaluation becomes necessary to define which antigens present the better performance in the diagnosis of anaplasmosis. Sera from cattle positive or negative to A. marginale by PCR, and sera from cattle proceeding from Brazil and Costa Rica, were tested by ELISAs based in recombinant MSP1a, MSP2, and MSP5, a pool of the three recombinant proteins, and initial body lisate antigen (CI). Using sera from A. marginale positive cattle by PCR, the highest sensitivity was shown by CI ELISA. Nevertheless, the highest specificity, with sera from negative cattle by PCR, was shown by recombinants ELISAs. The percentiles of positive cattle from Brazil and Costa Rica were higher with CI ELISA. Reasons for such differences were discussed.

• Anaplasma marginale

Abstract in Portuguese:

RESUMO.- Ramos C.A.N., Araújo F.R., Souza I.I.F., Guedes Jr D.S., Oliveira R.H.M., Farias T.A., Oliveira J.B., Alves L.C. & Faustino M.A.G. 2010. [Comparison between several antigens for diagnosis of Anaplasma marginale by ELISA.] Comparação entre diversos antígenos para o diagnóstico de Anaplasma marginale por ELISA. Pesquisa Veterinária Brasileira 30(1):37-41. Laboratório de Doenças Parasitárias, Departamento de Medicina Veterinária, Universidade Federal Rural de Pernambuco, Recife, PE 52171-900, Brazil. E-mail: carlosanramos@yahoo.com.br Anaplasmose bovina é uma doença com grande importância nas regiões tropicais e subtropicais do mundo por determinar perdas econômicas devido à mortalidade e redução da produtividade. É causada por Anaplasma marginale, uma riquétsia intraeritrocítica obrigatória cujo controle requer, além de uma vacina eficiente, uma acurada identificação de bovinos cronicamente infectados. Apesar de existirem atualmente diversos métodos de diagnóstico dessa riquétsia, os métodos sorológicos, em particular o ensaio de imunoadsorção enzimática–ELISAs, são os mais utilizados devido à sua versatilidade e praticidade. No entanto, devido ao grande número de antígenos disponíveis, atualmente torna-se necessária uma avaliação para definir quais antígenos apresentam um melhor desempenho no diagnóstico da anaplasmose. Soros de bovinos positivos e negativos para A. marginale por PCR, e soros de animais provenientes do Brasil e Costa Rica, foram testados em ELISAs baseados em MSP1a, MSP2 e MSP5 recombinantes, um pool das três proteínas recombinantes, e antígeno de lisado de corpúsculos iniciais da riquétsia (CI). Utilizando soro de bovinos positivos para A. marginale por PCR, uma maior sensibilidade foi observada no ELISA CI. No entanto, uma maior especificidade, com soro de bovinos negativos a PCR, foi observada com os ELISAs recombinantes. O porcentual de bovinos positivos do Brasil e Costa Rica foi maior com ELISA CI. Razões para essas diferenças são discutidas.

Abstract in English:

ABSTRACT.- Miyakawa V.I., Reis A.C.F. & Lisbôa J.A.N. 2009. [Epidemiological and clinical features of stephanofilariasis in dairy cows and diagnosis methods confrontation.] Aspectos epidemiológicos e clínicos da estefanofilariose em vacas leiteiras e comparação entre métodos de diagnóstico. Pesquisa Veterinária Brasileira 29(11):887-893. Departamento de Clínicas Veterinárias, Centro de Ciências Agrárias, Universidade Estadual de Londrina, Campus Universitário, Cx. Postal 6001, Londrina, PR 86051-990, Brazil. E-mail: janlisboa@uel.br Stephanofilariasis is a worldwide disease caused by the nematode Stephanofilaria that determines skin lesions. In cattle, the chronic dermatitis is characteristic begining with papules that progress to nodules, alopecia and ulcers with crusts. Despite it’s long time recognition, there are few studies and reports about this disease, specially in Brazil. This work was conducted in order to investigate epidemiological and clinical features of stephanofilariasis in dairy cows and to compare two methods for the diagnosis confirmation. Fifty-eight naturally affected dairy cows from seven herds located in Santana do Itararé, state of Paraná, and Itaberá, state of São Paulo, were studied from January 2006 through August 2008. Two methods for the diagnosis confirmation were compared using biopsied tissues from the border of the skin lesion: the histopathological examination (n=24) and the direct sediment examination of an isotonic saline solution in which the tissue fragment remained soaked (n=20). The prevalence was higher from December to March (57%) and lactating cows were primarily affected (87,9%). The cranial aspect of the fore mammary glands was the main site of the skin lesions (96,7%), chiefly near the ventral midline (55%). The characteristic wound was of circular shape, ulcerated with crusts and serosanguineous exudation. Chronic dermatitis with eosinophilic and mononuclaer cell infiltrates was the histopathologic change pattern present. The parasite was not detected in any histologic section examined. The direct sediment examination otherwise proved to be efficient for the diagnosis confirmation revealing the nematode adult and larval forms in all the specimens.

• Estefanofilariose Stephanofilaria sp.

Abstract in Portuguese:

RESUMO.- Miyakawa V.I., Reis A.C.F. & Lisbôa J.A.N. 2009. [Epidemiological and clinical features of stephanofilariasis in dairy cows and diagnosis methods confrontation.] Aspectos epidemiológicos e clínicos da estefanofilariose em vacas leiteiras e comparação entre métodos de diagnóstico. Pesquisa Veterinária Brasileira 29(11):887-893. Departamento de Clínicas Veterinárias, Centro de Ciências Agrárias, Universidade Estadual de Londrina, Campus Universitário, Cx. Postal 6001, Londrina, PR 86051-990, Brazil. E-mail: janlisboa@uel.br A estefanofilariose é uma doença mundialmente distribuída e caracteriza-se por lesões na pele causadas por nematódeo do gênero Stephanofilaria. Nos bovinos manifesta-se por uma dermatite crônica associada com erupção papular progredindo para nódulos, alopecia e ulceração crostosa. Apesar de reconhecida há muitos anos, há poucos estudos e relatos sobre a mesma. A literatura é particularmente escassa no Brasil. Esse trabalho teve como objetivos investigar aspectos epidemiológicos e clínicos da estefanofilariose em vacas leiteiras naturalmente acometidas e comparar dois métodos para a confirmação do diagnóstico, o exame histopatológico e o exame direto. Foram investigados aspectos clínicos relacionados à ocorrência natural da estefanofilariose em 58 vacas de leite de sete rebanhos criados nos municípios de Santana do Itararé, PR e de Itaberá, SP durante o período de janeiro de 2006 a agosto de 2008. Dois métodos foram comparados para confirmação do diagnóstico a partir de tecido colhido por biópsia da borda das lesões, o histopatológico (n=24) e o exame direto do sedimento da solução salina isotônica na qual o tecido permaneceu embebido (n=20). A maior prevalência ocorreu de dezembro a março (57%) e a maioria das vacas era lactante (87,9%). As lesões se localizavam nos quartos anteriores do úbere em seu aspecto cranial (96,7%), principalmente próximo à linha média (55%). A lesão típica tinha formato circular era ulcerada com crostas e exibia exsudato sero-sanguinolento. No exame histopatológico evidenciou-se uma dermatite crônica com infiltrado mononuclear e eosinofílico. A presença do parasita não foi detectada em nenhum dos cortes examinados. O exame direto possibilitou a demonstração do agente em todas as amostras examinadas, comprovando-se como um método eficiente para a confirmação do diagnóstico.

Abstract in English:

ABSTRACT.- Oliveira R.R., Mamprim M.J., Rahal S.C. & Bicudo A.L.C. 2009. [Radiography and ultrasonography in the diagnosis of rupture of the cranial cruciate ligament in dogs.] Radiografia e ultrassonografia no diagnóstico da ruptura do ligamento cruzado cranial em cães. Pesquisa Veterinária Brasileira 29(8):661-665. Departamento de Patologia Geral, Universidade Estadual do Paraná, Cx. Postal 261, Bandeirantes, PR 86360-000, Brazil. E-mail: rodrigoreisvet@hotmail.com Radiography and ultrasonography were evaluated as tools for diagnosis of the rupture of cranial cruciate ligament (CrCL) in dogs. Twenty-five dogs were submitted to radiographic and ultrasonographic examinations and their results were compared with those obtained by artrotomy (gold standard). Radiography detected the rupture in 84% (21/25) of the cases, but 16% (4/25) were false-negative. Ultrasonography identified accurately 76% (19/25) of the cases and gave a probable diagnosis for the remaining 24% (6/25) what means that this technique presented 100% of positive results. It was possible to conclude that radiography and ultrasonography are valuable tools for the diagnosis of CrCL rupture in dogs.

• Cruciate ligament

Abstract in Portuguese:

RESUMO.- ABSTRACT.- Oliveira R.R., Mamprim M.J., Rahal S.C. & Bicudo A.L.C. 2009. [Radiography and ultrasonography in the diagnosis of rupture of the cranial cruciate ligament in dogs.] Radiografia e ultrassonografia no diagnóstico da ruptura do ligamento cruzado cranial em cães. Pesquisa Veterinária Brasileira 29(8):661-665. Departamento de Patologia Geral, Universidade Estadual do Paraná, Cx. Postal 261, Bandeirantes, PR 86360-000, Brazil. E-mail: rodrigoreisvet@hotmail.com Radiografia e ultrassonografia foram avaliadas como técnicas no diagnóstico por imagem na ruptura do ligamento cruzado cranial (LCCr) em cães. Vinte e cinco cães foram submetidos à radiografia e ultrassonografia e seus resultados foram comparados aos obtidos por artrotomia (teste padrão ouro). O exame radiográfico diagnosticou corretamente a lesão em 84% (21/25) dos casos, mas 16% (4/25) apresentaram resultado falso-negativo. O exame ultrassonográfico foi capaz de diagnosticar acertadamente 76% (19/25) dos casos, e sugeriu a ruptura do LCCr nos 24% (6/25) restantes, apresentando 100% de resultados positivos. Concluiu-se que a radiografia e a ultrassonografia são ferramentas valiosas para diagnosticar casos de ruptura do LCCr em cães.

Abstract in English:

ABSTRACT.- Carvalho D., Oliveira T.M.F.S., Baldani C.D. & Machado R.Z. 2009. An enzyme-linked immunosorbent assay (ELISA) for the detection of IgM antibodies against Leishmania chagasi in dogs. Pesquisa Veterinária Brasileira 29(2):120-124. Departamento de Patologia Veterinária, Universidade Estadual Paulista, Faculdade de Ciências Agrárias e Veterinárias, Via de Acesso Prof. Paulo Donato Castellane s/n, Jaboticabal, SP 14870-000, Brazil. E-mail: zacarias@fcav.unesp.br Visceral leishmaniasis is an emergent zoonosis with an increasing number of new cases in Brazil where the domestic dog is an important parasite reservoir in the infectious cycle of Leishmania chagasi. An enzyme-linked immunosorbent assay (ELISA), based upon the use of a total soluble antigenic preparation of L. chagasi, was adapted for the detection of IgM antibodies in the serum of infected dogs. Optimal dilutions of the antigen, using positive and negative reference sera, were determined by checkboard titrations. The specificity and sensitivity of the ELISA were 100 %. A total of 110 serum samples were taken from dogs in Belo Horizonte, Minas Gerais, Brazil, and examined for anti-L. chagasi IgM antibody by ELISA and indirect fluorescent antibody test (IFAT). About 25% (n=27) of all the dogs tested were found serologically positive for L. chagasi by IFAT, while 89.09% (n=98) were seropositive by ELISA. The results obtained by ELISA and IFAT were significantly different (P<0.01). The combined use of ELISA and IFAT is recommended in order to enable veterinary services to more efficiently detect canine visceral leishmaniasis.

• Leishmania chagasi diagnosis dogs IgM enzyme-linked immunosorbent assay

Abstract in Portuguese:

ABSTRACT.- Carvalho D., Oliveira T.M.F.S., Baldani C.D. & Machado R.Z. 2009. An enzyme-linked immunosorbent assay (ELISA) for the detection of IgM antibodies against Leishmania chagasi in dogs. Pesquisa Veterinária Brasileira 29(2):120-124. Departamento de Patologia Veterinária, Universidade Estadual Paulista, Faculdade de Ciências Agrárias e Veterinárias, Via de Acesso Prof. Paulo Donato Castellane s/n, Jaboticabal, SP 14870-000, Brazil. E-mail: zacarias@fcav.unesp.br Visceral leishmaniasis is an emergent zoonosis with an increasing number of new cases in Brazil where the domestic dog is an important parasite reservoir in the infectious cycle of Leishmania chagasi. An enzyme-linked immunosorbent assay (ELISA), based upon the use of a total soluble antigenic preparation of L. chagasi, was adapted for the detection of IgM antibodies in the serum of infected dogs. Optimal dilutions of the antigen, using positive and negative reference sera, were determined by checkboard titrations. The specificity and sensitivity of the ELISA were 100 %. A total of 110 serum samples were taken from dogs in Belo Horizonte, Minas Gerais, Brazil, and examined for anti-L. chagasi IgM antibody by ELISA and indirect fluorescent antibody test (IFAT). About 25% (n=27) of all the dogs tested were found serologically positive for L. chagasi by IFAT, while 89.09% (n=98) were seropositive by ELISA. The results obtained by ELISA and IFAT were significantly different (P<0.01). The combined use of ELISA and IFAT is recommended in order to enable veterinary services to more efficiently detect canine visceral leishmaniasis.

Abstract in English:

ABSTRACT.- Teixeira T.F., Holz C.L., Caixeta S.P.M.B., Dezen D., Cibulski S.P., Silva J.R., Rosa J.C.A., Schmidt E., Ferreira J.C., Batista H.B.C.R., Caldas E., Franco A.C. & Roehe P.M. 2008. [Rabies diagnosis in the state of Rio Grande do Sul, Brazil, from 1985 to 2007.] Diagnóstico de raiva no Rio Grande do Sul, Brasil, de 1985 a 2007. Pesquisa Veterinária Brasileira 28(10):515-520. Instituto de Pesquisas Veterinárias Desidério Finamor, Fepagro-Saúde Animal, Cx. Postal 2076, Porto Alegre, RS 90001-970, Brazil. E-mail: proehe@ufrgs.br The results of 23 years of rabies diagnosis carried out at the Veterinary Research Institute Desidério Finamor, in the state of Rio Grande do Sul, RS, Brazil, are reported. From 1985 to 2007, a total of 23.460 specimens were examined, corresponding to 95% of the total number of samples submitted to rabies laboratory diagnosis notified within the state. Diagnostic methods included standard techniques such as the fluorescent antibody test (FAT) and mouse inoculation test (MIT). No cases of human rabies occurred in the period. Rabies virus (RV) was detected in 739 specimens (3.1%), from which 656 (88.7%) were from cattle. The virus was also identified in specimens from 23 dogs (3.1%), 21 horses (2.9%), 29 bats (4.0%), 4 cats (0.5%), 3 sheep (0.4%), 2 pigs (0.27%) and a wild animal of undetermined species (0.13%). The last case of rabies associated with a canine variant was diagnosed in 1988. Two cases of rabies associated with bat variant viruses were reported, in a domestic cat (2001) and in a dog (2007). In cattle, a marked tendency to a decrease in the number of cases was detected in the examined period. In contrast, an increase in the number of cases in haematophagous as well as in non haematophagous bats is noticed. However, as the number of bat specimens submitted for diagnosis has increased, this finding most likely reflects a higher degree of awareness on the possible role for bats in the rabies transmission cycle, rather than any particular changes on the virus or its hosts.

• Rabies epidemiology diagnosis incidence

Abstract in Portuguese:

ABSTRACT.- Teixeira T.F., Holz C.L., Caixeta S.P.M.B., Dezen D., Cibulski S.P., Silva J.R., Rosa J.C.A., Schmidt E., Ferreira J.C., Batista H.B.C.R., Caldas E., Franco A.C. & Roehe P.M. 2008. [Rabies diagnosis in the state of Rio Grande do Sul, Brazil, from 1985 to 2007.] Diagnóstico de raiva no Rio Grande do Sul, Brasil, de 1985 a 2007. Pesquisa Veterinária Brasileira 28(10):515-520. Instituto de Pesquisas Veterinárias Desidério Finamor, Fepagro-Saúde Animal, Cx. Postal 2076, Porto Alegre, RS 90001-970, Brazil. E-mail: proehe@ufrgs.br The results of 23 years of rabies diagnosis carried out at the Veterinary Research Institute Desidério Finamor, in the state of Rio Grande do Sul, RS, Brazil, are reported. From 1985 to 2007, a total of 23.460 specimens were examined, corresponding to 95% of the total number of samples submitted to rabies laboratory diagnosis notified within the state. Diagnostic methods included standard techniques such as the fluorescent antibody test (FAT) and mouse inoculation test (MIT). No cases of human rabies occurred in the period. Rabies virus (RV) was detected in 739 specimens (3.1%), from which 656 (88.7%) were from cattle. The virus was also identified in specimens from 23 dogs (3.1%), 21 horses (2.9%), 29 bats (4.0%), 4 cats (0.5%), 3 sheep (0.4%), 2 pigs (0.27%) and a wild animal of undetermined species (0.13%). The last case of rabies associated with a canine variant was diagnosed in 1988. Two cases of rabies associated with bat variant viruses were reported, in a domestic cat (2001) and in a dog (2007). In cattle, a marked tendency to a decrease in the number of cases was detected in the examined period. In contrast, an increase in the number of cases in haematophagous as well as in non haematophagous bats is noticed. However, as the number of bat specimens submitted for diagnosis has increased, this finding most likely reflects a higher degree of awareness on the possible role for bats in the rabies transmission cycle, rather than any particular changes on the virus or its hosts.

Abstract in English:

ABSTRACT.- Silva M.S., Brum M.C.S., Weiblen R. & Flores E.F. 2007. [Identification and differentiation of herpesvirus types 1 and 5 isolated from clinical samples in central-southern Brazil, Argentina and Uruguay (1987-2006).] Identificação e diferenciação de herpesvírus bovino tipos 1 e 5 isolados de amostras clínicas no Centro-Sul do Brasil, Argentina e Uruguai (1987-2006). Pesquisa Veterinária Brasileira 27(10):403-408. Departamento de Medicina Veterinária Preventiva, Universidade Federal de Santa Maria, 97105-900 Santa Maria, RS, Brazil. E-mail: flores@ccr.ufsm.br Bovine herpesviruses types 1 and 5 (BoHV-1; BoHV-5) are genetically and antigenically closely related such they can not be distinguished by routine diagnostic tests. As BoHV-1 has been historically associated with respiratory and genital disease, herpesviruses isolated from these clinical syndromes have been tentatively – and sometimes definitively - diagnosed as BoHV-1. Likewise, cases of herpetic neurological infection in cattle have been generally attributed to BoHV-5. This study reports the identification of 40 herpesvirus isolates from different clinical specimens and syndromes in central-southern Brazil, Argentina and Uruguay (1987-2006) by the use of a PCR able to differentiate between BoHV-1 and BoHV-5. BoHV-1 isolates (n=16) were identified in cases of respiratory disease (n=3), vulvovaginitis and/or balanoposthitis (n=3), in semen of healthy bulls (n=5) and in cases of neurological disease (n=5). Viruses identified as BoHV-5 (n=24) were isolated predominantly from cases of neurological disease (n=21), but also from semen of healthy bulls (n=2) and from a spleen of a calf with systemic disease (n=1). These results show that both BoHV-1 and BoHV-5 are not strictly associated with their respective diseases; yet are frequently involved in clinical conditions otherwise attributed to the other virus. These findings also reinforce the need of correctly identifying the herpesvirus isolates as to better understand their pathogenesis and epidemiology.

• Bovine herpesvirus BoHV-1 BoHV-5 differential diagnosis epidemiology

Abstract in Portuguese:

ABSTRACT.- Silva M.S., Brum M.C.S., Weiblen R. & Flores E.F. 2007. [Identification and differentiation of herpesvirus types 1 and 5 isolated from clinical samples in central-southern Brazil, Argentina and Uruguay (1987-2006).] Identificação e diferenciação de herpesvírus bovino tipos 1 e 5 isolados de amostras clínicas no Centro-Sul do Brasil, Argentina e Uruguai (1987-2006). Pesquisa Veterinária Brasileira 27(10):403-408. Departamento de Medicina Veterinária Preventiva, Universidade Federal de Santa Maria, 97105-900 Santa Maria, RS, Brazil. E-mail: flores@ccr.ufsm.br Bovine herpesviruses types 1 and 5 (BoHV-1; BoHV-5) are genetically and antigenically closely related such they can not be distinguished by routine diagnostic tests. As BoHV-1 has been historically associated with respiratory and genital disease, herpesviruses isolated from these clinical syndromes have been tentatively – and sometimes definitively - diagnosed as BoHV-1. Likewise, cases of herpetic neurological infection in cattle have been generally attributed to BoHV-5. This study reports the identification of 40 herpesvirus isolates from different clinical specimens and syndromes in central-southern Brazil, Argentina and Uruguay (1987-2006) by the use of a PCR able to differentiate between BoHV-1 and BoHV-5. BoHV-1 isolates (n=16) were identified in cases of respiratory disease (n=3), vulvovaginitis and/or balanoposthitis (n=3), in semen of healthy bulls (n=5) and in cases of neurological disease (n=5). Viruses identified as BoHV-5 (n=24) were isolated predominantly from cases of neurological disease (n=21), but also from semen of healthy bulls (n=2) and from a spleen of a calf with systemic disease (n=1). These results show that both BoHV-1 and BoHV-5 are not strictly associated with their respective diseases; yet are frequently involved in clinical conditions otherwise attributed to the other virus. These findings also reinforce the need of correctly identifying the herpesvirus isolates as to better understand their pathogenesis and epidemiology.

Abstract in English:

ABSTRACT.- Baldani C.D., Machado R.Z., Raso T.F. & Pinto A.A. 2007. Serodiagnosis of Babesia equi in horses submitted to exercise stress. Pesquisa Veterinária Brasileira27(4):179-183. Departamento de Patologia Veterinária, Universidade Estadual Paulista, Faculdade de Ciências Agrárias e Veterinárias, Via de Acesso Prof. Paulo Donato Castellane s/n, Jaboticabal, SP 14870-000, Brazil. E-mail: zacarias@fcav.unesp.br A complement fixation test (CFT), performed in microtitre plates, based upon the use of crude antigenic preparation of Babesia equi was adapted for the detection of antibodies in serum of infected horses. The indirect fluorescent antibody test (IFAT) and enzyme-linked immunosorbent assay (ELISA) were also used for the immunodiagnosis of B. equi. Serum samples from 15 apparently healthy horses, previously conditioned to a high-speed equine treadmill, were taken before and after exercise. All the samples analyzed were positive for B. equi infection. There were no significant differences (P<0.01) between these 3 tests, or the condition of rest or stress. The combined use of CFT and IFAT or ELISA should be recommended in order to enable veterinary services to more efficiently prevent introduction of infected horses into disease-free areas.

• Babesia equi diagnosis complement fixation indirect fluorescent antibody test enzyme-linked immunosorbent assay

Abstract in Portuguese:

ABSTRACT.- Baldani C.D., Machado R.Z., Raso T.F. & Pinto A.A. 2007. Serodiagnosis of Babesia equi in horses submitted to exercise stress. Pesquisa Veterinária Brasileira27(4):179-183. Departamento de Patologia Veterinária, Universidade Estadual Paulista, Faculdade de Ciências Agrárias e Veterinárias, Via de Acesso Prof. Paulo Donato Castellane s/n, Jaboticabal, SP 14870-000, Brazil. E-mail: zacarias@fcav.unesp.br A complement fixation test (CFT), performed in microtitre plates, based upon the use of crude antigenic preparation of Babesia equi was adapted for the detection of antibodies in serum of infected horses. The indirect fluorescent antibody test (IFAT) and enzyme-linked immunosorbent assay (ELISA) were also used for the immunodiagnosis of B. equi. Serum samples from 15 apparently healthy horses, previously conditioned to a high-speed equine treadmill, were taken before and after exercise. All the samples analyzed were positive for B. equi infection. There were no significant differences (P<0.01) between these 3 tests, or the condition of rest or stress. The combined use of CFT and IFAT or ELISA should be recommended in order to enable veterinary services to more efficiently prevent introduction of infected horses into disease-free areas.

Abstract in English:

ABSTRACT.- Mathias L.A., Meirelles R.B. & Buchala F.G. 2007. [Stability of Brucella abortus whole cell antigen for use in the serological diagnosis of bovine brucellosis by the complement fixation test.] Estabilidade do antígeno de célula total de Brucella abortus para uso no diagnóstico sorológico da brucelose bovina pela reação de fixação de complemento. Pesquisa Veterinária Brasileira 27(1):18-22. Departamento de Medicina Veterinária Preventiva e Reprodução Animal, Faculdade de Ciências Agrárias e Veterinárias (FCAV), Universidade Estadual Paulista (Unesp), Jaboticabal, SP 14884-900, Brazil. E-mail: lmathias@fcav.unesp.br The complement fixation test is used worldwide in the confirmatory diagnosis of bovine brucellosis. For this technique the antigen is the same as the one used in the tube agglutination test. However, literature is poor in information about the stability of the whole cell Brucella antigen for use in the complement fixation test to establish a time of validity of the antigen. Hence the aim of this investigation was to evaluate the stability of this antigen under refrigeration for use in the complement fixation test. Fourteen batches of antigen prepared with Brucella abortus strain 1119/3, produced from 9 months to 23 years and 11 months before, were analysed. One hundred and sixty-seven cattle sera with varying titres of antibodies to Brucella were tested through the warm complement fixation microtechnique with five 50% haemolytic units of complement. Sera with at least 25% of complement fixation in dilution 1:4 were considered positive. The results with 13 of the antigen batches were compared with the results obtained with the batch produced 9 months before by the McNemar c2 test and kappa statistic. The oldest antigen batch gave a higher proportion of sera titres which were exactly the same observed with the 9-month-batch (90.4%), and the antigen produced 4 years and 3 months before the test gave de lowest proportion of sera with the same titre of the 9-month-antigen (73.7%). The comparison of the results after being classified as positive and negative showed that the highest proportion of agreed results was observed with the antigen produced 21 years and 4 months before (98.8%, kappa 0.98). The antigen with the lowest proportion of agreed results was the one produced 3 years and 2 months before (91.6%, kappa 0.84). The results of the study show that most sera gave very similar results with all antigen batches evaluated, and that there was no relationship between the period of antigen production and the difference in test results.

• Bovine brucellosis serological diagnosis complement fixation test

Abstract in Portuguese:

ABSTRACT.- Mathias L.A., Meirelles R.B. & Buchala F.G. 2007. [Stability of Brucella abortus whole cell antigen for use in the serological diagnosis of bovine brucellosis by the complement fixation test.] Estabilidade do antígeno de célula total de Brucella abortus para uso no diagnóstico sorológico da brucelose bovina pela reação de fixação de complemento. Pesquisa Veterinária Brasileira 27(1):18-22. Departamento de Medicina Veterinária Preventiva e Reprodução Animal, Faculdade de Ciências Agrárias e Veterinárias (FCAV), Universidade Estadual Paulista (Unesp), Jaboticabal, SP 14884-900, Brazil. E-mail: lmathias@fcav.unesp.br The complement fixation test is used worldwide in the confirmatory diagnosis of bovine brucellosis. For this technique the antigen is the same as the one used in the tube agglutination test. However, literature is poor in information about the stability of the whole cell Brucella antigen for use in the complement fixation test to establish a time of validity of the antigen. Hence the aim of this investigation was to evaluate the stability of this antigen under refrigeration for use in the complement fixation test. Fourteen batches of antigen prepared with Brucella abortus strain 1119/3, produced from 9 months to 23 years and 11 months before, were analysed. One hundred and sixty-seven cattle sera with varying titres of antibodies to Brucella were tested through the warm complement fixation microtechnique with five 50% haemolytic units of complement. Sera with at least 25% of complement fixation in dilution 1:4 were considered positive. The results with 13 of the antigen batches were compared with the results obtained with the batch produced 9 months before by the McNemar c2 test and kappa statistic. The oldest antigen batch gave a higher proportion of sera titres which were exactly the same observed with the 9-month-batch (90.4%), and the antigen produced 4 years and 3 months before the test gave de lowest proportion of sera with the same titre of the 9-month-antigen (73.7%). The comparison of the results after being classified as positive and negative showed that the highest proportion of agreed results was observed with the antigen produced 21 years and 4 months before (98.8%, kappa 0.98). The antigen with the lowest proportion of agreed results was the one produced 3 years and 2 months before (91.6%, kappa 0.84). The results of the study show that most sera gave very similar results with all antigen batches evaluated, and that there was no relationship between the period of antigen production and the difference in test results.