PESQUISA VETERINÁRIA BRASILEIRA

Abstract in English:

ABSTRACT.- Fonteque J.H., Kohayagawa A., Takahira R.K., Bianchi E.H., Cherubini A.L., Piccinin A., Bruder E.M. & Ramos P.R.R. 2009. [Serum protein electrophoresis profile of the rattlesnake Crotalus durissus terrificus kept in captivity.] Perfil eletroforético das proteínas séricas de serpentes Crotalus durissus terrificus (cascavel) criadas em cativeiro. Pesquisa Veterinária Brasileira 29(6):457-460. Departamento de Medicina Veterinária, Hospital de Clínica Veterinária, Centro de Ciências Agroveterinárias, Universidade do Estado de Santa Catarina, Av. Luiz de Camões 2090, Lages, SC 88520-000, Brazil. E-mail: fonteque@cav.udesc.br The poisonous snakes of the genera Crotalus and Bothrops have been kept in captivity with the purpose of extracting poison for the production of immunobiological. Knowledge of the physiology of these animals and serum proteins concentration changes are important for early identification of major diseases which lead to states of hypoproteinemia and hyperproteinemia. The objective was to determine the concentration of total protein and serum protein electrophoresis profile of Crotalus durissus terrificus (rattlesnake) in captivity. Blood samples were taken from the ventral coccygeal vein of 21 adult and healthy snakes divided into groups: Group 1 with 12 males, weighing in average 588.89±193.55g, and Group 2 with nine females, weighing in average 708.33±194.04g. The total serum concentration of protein was determined by the method of refractometry and agarose gel electrophoresis. The total protein values in the serum for females was 4.82±0.72, for males 4.51±0.50 and males and females 4.64±0.61, identified by four fractions (g/dL): albumin, a, b and g-globulin. Additionally the albumin/globulin ratio was calculated. The female snakes showed higher values for the variables, albumin and the albumin/globulin (AG) differed significantly (P<0.05) from the group of male snakes, but there was no clinical significance.

• Protein fractions albumin alpha beta and gamma-globulin sex agarose gel

Abstract in Portuguese:

ABSTRACT.- Fonteque J.H., Kohayagawa A., Takahira R.K., Bianchi E.H., Cherubini A.L., Piccinin A., Bruder E.M. & Ramos P.R.R. 2009. [Serum protein electrophoresis profile of the rattlesnake Crotalus durissus terrificus kept in captivity.] Perfil eletroforético das proteínas séricas de serpentes Crotalus durissus terrificus (cascavel) criadas em cativeiro. Pesquisa Veterinária Brasileira 29(6):457-460. Departamento de Medicina Veterinária, Hospital de Clínica Veterinária, Centro de Ciências Agroveterinárias, Universidade do Estado de Santa Catarina, Av. Luiz de Camões 2090, Lages, SC 88520-000, Brazil. E-mail: fonteque@cav.udesc.br The poisonous snakes of the genera Crotalus and Bothrops have been kept in captivity with the purpose of extracting poison for the production of immunobiological. Knowledge of the physiology of these animals and serum proteins concentration changes are important for early identification of major diseases which lead to states of hypoproteinemia and hyperproteinemia. The objective was to determine the concentration of total protein and serum protein electrophoresis profile of Crotalus durissus terrificus (rattlesnake) in captivity. Blood samples were taken from the ventral coccygeal vein of 21 adult and healthy snakes divided into groups: Group 1 with 12 males, weighing in average 588.89±193.55g, and Group 2 with nine females, weighing in average 708.33±194.04g. The total serum concentration of protein was determined by the method of refractometry and agarose gel electrophoresis. The total protein values in the serum for females was 4.82±0.72, for males 4.51±0.50 and males and females 4.64±0.61, identified by four fractions (g/dL): albumin, a, b and g-globulin. Additionally the albumin/globulin ratio was calculated. The female snakes showed higher values for the variables, albumin and the albumin/globulin (AG) differed significantly (P<0.05) from the group of male snakes, but there was no clinical significance.

Abstract in English:

ABSTRACT.- Cavallini Sanches E.M., Pacheco S.M., Cericatto A.S., Melo R.M., Colodel E.M., Hummel J., Bianchi S.P., Spanamberg A., Santurio J.M. & Ferreiro L. 2009. Detection of Pneumocystis in lungs of bats from Brazil by PCR amplification. Pesquisa Veterinária Brasileira 29(6):469-473. Setor de Micologia Veterinária, Faculdade de Veterinária, Universidade Federal do Rio Grande do Sul, Av. Bento Gonçalves 9090, Porto Alegre, RS 90540-000, Brazil. E-mail: cavallini.sanches@ufrgs.br Pneumocystis has been isolated from a wide range of unrelated mammalian hosts, including humans, domestic and wild animals. It has been demonstrated that the genome of Pneumocystis of one host differs markedly from that of other hosts. Also, variation in the chromosome and DNA sequence of Pneumocystis within a single host species has been observed. Since information about the occurrence and nature of infections in wild animals is still limited, the objective of this work was to detect the presence of Pneumocystis sp. in lungs of bats from two states from Brazil by Nested-PCR amplification. The bats, captured in caves and in urban areas, were obtained from the Program of Rabies Control of two States in Brazil, Mato Grosso and Rio Grande do Sul, located in the Mid-Western and Southern regions of the country, respectively. DNAs were extracted from 102 lung tissues and screened for Pneumocystis by nested PCR at the mtLSU rRNA gene and small subunit of mitochondrial ribosomal RNA (mtSSU rRNA). Gene amplification was performed using the mtLSU rRNA, the primer set pAZ102H - pAZ102E and pAZ102X - pAZY, and the mtSSU rRNA primer set pAZ102 10FRI - pAZ102 10R-RI and pAZ102 13RI - pAZ102 14RI. The most frequent bats were Tadarida brasiliensis (25), Desmodus rotundus (20), and Nyctinomops laticaudatus (19). Pneumocystis was more prevalent in the species Nyctinomops laticaudatus (26.3% = 5/19), Tadarida brasiliensis (24% = 6/25), and Desmodus rotundus (20% = 4/20). Besides these species, Pneumocystis also was detected in lungs from Molossus molossus (1/11, 9.1%), Artibeus fimbriatus (1/1, 100%), Sturnira lilium (1/3, 33.3%), Myotis levis (2/3, 66.7%) and Diphylla ecaudata (1/2, 50%). PCR products which could indicate the presence of Pneumocystis (21.56%) were identified in DNA samples obtained from 8 out of 16 classified species from both states (5 bats were not identified). This is the first report of detection of Pneumocystis in bats from Brazil.

• Pneumocystis sp. bats Nested-PCR

Abstract in Portuguese:

ABSTRACT.- Cavallini Sanches E.M., Pacheco S.M., Cericatto A.S., Melo R.M., Colodel E.M., Hummel J., Bianchi S.P., Spanamberg A., Santurio J.M. & Ferreiro L. 2009. Detection of Pneumocystis in lungs of bats from Brazil by PCR amplification. Pesquisa Veterinária Brasileira 29(6):469-473. Setor de Micologia Veterinária, Faculdade de Veterinária, Universidade Federal do Rio Grande do Sul, Av. Bento Gonçalves 9090, Porto Alegre, RS 90540-000, Brazil. E-mail: cavallini.sanches@ufrgs.br Pneumocystis has been isolated from a wide range of unrelated mammalian hosts, including humans, domestic and wild animals. It has been demonstrated that the genome of Pneumocystis of one host differs markedly from that of other hosts. Also, variation in the chromosome and DNA sequence of Pneumocystis within a single host species has been observed. Since information about the occurrence and nature of infections in wild animals is still limited, the objective of this work was to detect the presence of Pneumocystis sp. in lungs of bats from two states from Brazil by Nested-PCR amplification. The bats, captured in caves and in urban areas, were obtained from the Program of Rabies Control of two States in Brazil, Mato Grosso and Rio Grande do Sul, located in the Mid-Western and Southern regions of the country, respectively. DNAs were extracted from 102 lung tissues and screened for Pneumocystis by nested PCR at the mtLSU rRNA gene and small subunit of mitochondrial ribosomal RNA (mtSSU rRNA). Gene amplification was performed using the mtLSU rRNA, the primer set pAZ102H - pAZ102E and pAZ102X - pAZY, and the mtSSU rRNA primer set pAZ102 10FRI - pAZ102 10R-RI and pAZ102 13RI - pAZ102 14RI. The most frequent bats were Tadarida brasiliensis (25), Desmodus rotundus (20), and Nyctinomops laticaudatus (19). Pneumocystis was more prevalent in the species Nyctinomops laticaudatus (26.3% = 5/19), Tadarida brasiliensis (24% = 6/25), and Desmodus rotundus (20% = 4/20). Besides these species, Pneumocystis also was detected in lungs from Molossus molossus (1/11, 9.1%), Artibeus fimbriatus (1/1, 100%), Sturnira lilium (1/3, 33.3%), Myotis levis (2/3, 66.7%) and Diphylla ecaudata (1/2, 50%). PCR products which could indicate the presence of Pneumocystis (21.56%) were identified in DNA samples obtained from 8 out of 16 classified species from both states (5 bats were not identified). This is the first report of detection of Pneumocystis in bats from Brazil.

Abstract in English:

ABSTRACT.- Silva K.P.C., Mota R.A., Cunha A.P., Silva L.B.G., Leal N.C., Cavalcante Y.V.N., Teles J.A.A., Pereira M.C.C. & Freitas N.S. 2009. [Phenotypic and molecular characterization of Burkholderia mallei isolated in northeastern Brazil.] Caracterização fenotípica e molecular de amostras de Burkholderia mallei isoladas na Região Nordeste do Brasil. Pesquisa Veterinária Brasileira 29(5):439-444. Departamento de Medicina Veterinária, Universidade Federal Rural de Pernambuco, Dois Irmãos, Recife, PE 52171-900, Brazil. E-mail: rinaldo.mota@hotmail.com The objective of this paper was to study the molecular performance and phenotypic characterization of Burkholderia mallei isolated from horses with clinical and serological diagnosis of glanders, originating from the Metropolitan District of Recife and Zona da Mata of Pernambuco and Alagoas. The isolation and biochemical identification of B. mallei was carried out by microbiological and molecular techniques of PCR-fingerprinting and RAPD-PCR. From the eight samples studied, four showed little phenotype variations. In the molecular tests, the samples formed 4 groups of different ribotype profiles and 4 genotype profiles. There was some association of PCR-fingerprinting with RAPD-PCR results. It was concluded that the slight biochemical variations were not associated with different molecular profiles. They also indicated that these differences show heterogeneity associated with the origin of the sample, indicating that the infection was caused by clones of different strains and that the polymorphism of DNA observed could make it

• Burkholderia mallei glanders mormo doenças de eqüdeos

Abstract in Portuguese:

ABSTRACT.- Silva K.P.C., Mota R.A., Cunha A.P., Silva L.B.G., Leal N.C., Cavalcante Y.V.N., Teles J.A.A., Pereira M.C.C. & Freitas N.S. 2009. [Phenotypic and molecular characterization of Burkholderia mallei isolated in northeastern Brazil.] Caracterização fenotípica e molecular de amostras de Burkholderia mallei isoladas na Região Nordeste do Brasil. Pesquisa Veterinária Brasileira 29(5):439-444. Departamento de Medicina Veterinária, Universidade Federal Rural de Pernambuco, Dois Irmãos, Recife, PE 52171-900, Brazil. E-mail: rinaldo.mota@hotmail.com The objective of this paper was to study the molecular performance and phenotypic characterization of Burkholderia mallei isolated from horses with clinical and serological diagnosis of glanders, originating from the Metropolitan District of Recife and Zona da Mata of Pernambuco and Alagoas. The isolation and biochemical identification of B. mallei was carried out by microbiological and molecular techniques of PCR-fingerprinting and RAPD-PCR. From the eight samples studied, four showed little phenotype variations. In the molecular tests, the samples formed 4 groups of different ribotype profiles and 4 genotype profiles. There was some association of PCR-fingerprinting with RAPD-PCR results. It was concluded that the slight biochemical variations were not associated with different molecular profiles. They also indicated that these differences show heterogeneity associated with the origin of the sample, indicating that the infection was caused by clones of different strains and that the polymorphism of DNA observed could make it

Abstract in English:

ABSTRACT.- Néspoli P.B, Gheller V.A., Mahecha G.A.B., Godoy de Araújo D.K., Gilberto L. Macedo G.L.J. & Bordin A.I. 2009. [Morphologic aspects of hepatic ultrasonography in sheep.] Aspectos morfológicos da ultra-sonografia hepática de ovinos. Pesquisa Veterinária Brasileira 29(4):333-338. Departamento de Clínica Médica Veterinária, Faculdade Agronomia e Medicina Veterinária, Universidade Federal de Mato Grosso, Av. Fernando Corrêa da Costa s/n, Coxipó, Cuiabá, MT 78060-900, Brazil. E-mail: nespoli@ufmt.br The ultrasonography (US) is a complementary technique of choice for the diagnostic of hepatic diseases in many domestics’ species. In sheep however there are few reports about ultrasonography in hepatic diseases and there is not precise definition about the anatomic standards of normal liver limits in ultrasonographic examination. In this study 58 Santa Inês sheep breed were used and divided in 3 groups: n1=8 males, n2=10 not pregnant females and n3=40 pregnant females. The animals were scanned from the 12º to 8º intercostal spaces (EI) to observe the localization of the vena cava caudal (VC), gallbladder (VB) and to measure the liver thickness above the VC and vena portae VP under the 11º and 10º EI. The liver was examined on satisfactory way from the 12º till the 8º EI. Both the VC and the VP where observed from the 12º to 9º EI, however the VC could not be observed in 11 animals, 10 of them were over 50 kg. Between the two female groups the VC and VP where observed most frequently from the 11º to 10º EI and in all males examined from the 12º to 10º EI. The location of the gallbladder varies between the 10º to the 8º EI, with bigger incidence between the 9º and the 8º EI in pregnant and no pregnant females groups and underneath the 9º EI on the male group. Comparatively, the ecogenicity of the liver parenchyma was more intense than kidney cortex. There was a significant correlation between liver’s weight and hepatic thikness above the vena portae on the 11º and 10º EI on the pregnant females group. The US supplied to important information about the topography and echogenicity of the liver and showed to be a useful tool to esteem the liver’s weight.

• Sheep ultrasonography liver Vena cava caudalis Vena portae gall bladder

Abstract in Portuguese:

ABSTRACT.- Néspoli P.B, Gheller V.A., Mahecha G.A.B., Godoy de Araújo D.K., Gilberto L. Macedo G.L.J. & Bordin A.I. 2009. [Morphologic aspects of hepatic ultrasonography in sheep.] Aspectos morfológicos da ultra-sonografia hepática de ovinos. Pesquisa Veterinária Brasileira 29(4):333-338. Departamento de Clínica Médica Veterinária, Faculdade Agronomia e Medicina Veterinária, Universidade Federal de Mato Grosso, Av. Fernando Corrêa da Costa s/n, Coxipó, Cuiabá, MT 78060-900, Brazil. E-mail: nespoli@ufmt.br The ultrasonography (US) is a complementary technique of choice for the diagnostic of hepatic diseases in many domestics’ species. In sheep however there are few reports about ultrasonography in hepatic diseases and there is not precise definition about the anatomic standards of normal liver limits in ultrasonographic examination. In this study 58 Santa Inês sheep breed were used and divided in 3 groups: n1=8 males, n2=10 not pregnant females and n3=40 pregnant females. The animals were scanned from the 12º to 8º intercostal spaces (EI) to observe the localization of the vena cava caudal (VC), gallbladder (VB) and to measure the liver thickness above the VC and vena portae VP under the 11º and 10º EI. The liver was examined on satisfactory way from the 12º till the 8º EI. Both the VC and the VP where observed from the 12º to 9º EI, however the VC could not be observed in 11 animals, 10 of them were over 50 kg. Between the two female groups the VC and VP where observed most frequently from the 11º to 10º EI and in all males examined from the 12º to 10º EI. The location of the gallbladder varies between the 10º to the 8º EI, with bigger incidence between the 9º and the 8º EI in pregnant and no pregnant females groups and underneath the 9º EI on the male group. Comparatively, the ecogenicity of the liver parenchyma was more intense than kidney cortex. There was a significant correlation between liver’s weight and hepatic thikness above the vena portae on the 11º and 10º EI on the pregnant females group. The US supplied to important information about the topography and echogenicity of the liver and showed to be a useful tool to esteem the liver’s weight.

Abstract in English:

ABSTRACT.- Alves F.R., Feitosa M.L.T., Gatti A., Fadel L., Unruh S.M., Ambrósio C.E., Sterman F.A., Pinto A.C.B.C.F. & Miglino M.A. 2009. [Radiologic images of the thoracic cavity of Golden Retriever dogs affected by muscular dystrophy.] Imagem radiográfica da cavidade torácica de cães Golden Retriever acometidos pela Distrofia Muscular. Pesquisa Veterinária Brasileira 29(2):99-104. Departamento de Cirurgia, Faculdade de Medicina Veterinária e Zootecnia, Universidade de São Paulo, Av. Prof. Dr. Orlando Marques de Paiva 87, São Paulo, SP 05508-270, Brazil. E-mail: flaviovet@usp.br Duchenne Muscular Dystrophy (DMD) is a genetic disorder with clinical signs of muscular weaknesses and progressive atrophy. Golden Retriever dogs show similar genotypic and phenotypic characteristics to Human Muscular Dystrophy and are considered a proper animal model for DMD studies. Latero-lateral and dorso-ventral thoracic radiographies were obtained from 10 Golden Retriever dogs affected by muscular dystrophy, to investigate possible radiographic alterations. Thorax radiographic examination revealed (a) interstitial and alveolar pattern, (b) initial phases of pneumonia and pulmonary edema, (c) cardiomegaly as a principal alteration in the thoracic cavity, (d) megaesophagus displacing the trachea and heart silhouette, and (e) cranial protrusion of the diaphragm lining into the thorax with development of a hiatus hernia displacing the stomach to the caudal mediastinum. Postmortem examination showed pleural effusion, pulmonary emphysema, degenerative and metaplasic processes in the diaphragm and intercostal muscles. Radiographic examination was considered essential for the diagnosis of cardiac and respiratory disease in Golden Retriever dogs affected by muscular dystrophy, and to identify the primary pulmonary process and to provide the establishment of suitable therapeutic treatment, with a reserved prognosis in advanced stage of the disease.

• Muscular dystrophy Duchenne Golden Retriever dog radiology

Abstract in Portuguese:

ABSTRACT.- Alves F.R., Feitosa M.L.T., Gatti A., Fadel L., Unruh S.M., Ambrósio C.E., Sterman F.A., Pinto A.C.B.C.F. & Miglino M.A. 2009. [Radiologic images of the thoracic cavity of Golden Retriever dogs affected by muscular dystrophy.] Imagem radiográfica da cavidade torácica de cães Golden Retriever acometidos pela Distrofia Muscular. Pesquisa Veterinária Brasileira 29(2):99-104. Departamento de Cirurgia, Faculdade de Medicina Veterinária e Zootecnia, Universidade de São Paulo, Av. Prof. Dr. Orlando Marques de Paiva 87, São Paulo, SP 05508-270, Brazil. E-mail: flaviovet@usp.br Duchenne Muscular Dystrophy (DMD) is a genetic disorder with clinical signs of muscular weaknesses and progressive atrophy. Golden Retriever dogs show similar genotypic and phenotypic characteristics to Human Muscular Dystrophy and are considered a proper animal model for DMD studies. Latero-lateral and dorso-ventral thoracic radiographies were obtained from 10 Golden Retriever dogs affected by muscular dystrophy, to investigate possible radiographic alterations. Thorax radiographic examination revealed (a) interstitial and alveolar pattern, (b) initial phases of pneumonia and pulmonary edema, (c) cardiomegaly as a principal alteration in the thoracic cavity, (d) megaesophagus displacing the trachea and heart silhouette, and (e) cranial protrusion of the diaphragm lining into the thorax with development of a hiatus hernia displacing the stomach to the caudal mediastinum. Postmortem examination showed pleural effusion, pulmonary emphysema, degenerative and metaplasic processes in the diaphragm and intercostal muscles. Radiographic examination was considered essential for the diagnosis of cardiac and respiratory disease in Golden Retriever dogs affected by muscular dystrophy, and to identify the primary pulmonary process and to provide the establishment of suitable therapeutic treatment, with a reserved prognosis in advanced stage of the disease.

Abstract in English:

ABSTRACT.- Aguiar D.M, Gennari S.M., Cavalcante G.T., Labruna M.B., Vasconcellos S.A., Rodrigues A.A.R., Moraes Z.M. & Camargo L.M.A. 2006. Seroprevalence of Leptospira spp in cattle from Monte Negro municipality, western Amazon. Pesquisa Veterinária Brasileira 26(2):102-104. Department of Preventive Veterinary Medicine and Animal Health, Faculty of Veterinary Medicine and Animal Production, University of São Paulo, Av. Prof. Orlando Marques de Paiva 87, São Paulo, SP 05508-900, Brazil. E-mail: danmoura@aptaregional.sp.gov.br The prevalence of anti-Leptospira spp antibodies was investigated in 2,109 female cattle from 86 herds of Monte Negro municipality, Rondônia, Brazil. Sera samples were evaluated by Microscopic Agglutination Test against 24 leptospira serovars. Titers =100 for at least one of 24 leptospira serovars were detected in 1,114 cows (52.8%) from 82 (95.3%) herds. The adjusted overall prevalence for Monte Negro municipality was 53.9% (49-58.7%; CI: 95%). The most prevalent serovars were Hardjo (14.5%), Wolffi (12.3%), Shermani (10.8%), Patoc (7.9%), and Hebdomadis (6.1%). Other serovars worldwidely reported like Bratislava, Pomona and Grippotyphosa were detected in low levels.

• Leptospira spp cattle epidemiology Amazon.

Abstract in Portuguese:

ABSTRACT.- Aguiar D.M, Gennari S.M., Cavalcante G.T., Labruna M.B., Vasconcellos S.A., Rodrigues A.A.R., Moraes Z.M. & Camargo L.M.A. 2006. Seroprevalence of Leptospira spp in cattle from Monte Negro municipality, western Amazon. Pesquisa Veterinária Brasileira 26(2):102-104. Department of Preventive Veterinary Medicine and Animal Health, Faculty of Veterinary Medicine and Animal Production, University of São Paulo, Av. Prof. Orlando Marques de Paiva 87, São Paulo, SP 05508-900, Brazil. E-mail: danmoura@aptaregional.sp.gov.br The prevalence of anti-Leptospira spp antibodies was investigated in 2,109 female cattle from 86 herds of Monte Negro municipality, Rondônia, Brazil. Sera samples were evaluated by Microscopic Agglutination Test against 24 leptospira serovars. Titers =100 for at least one of 24 leptospira serovars were detected in 1,114 cows (52.8%) from 82 (95.3%) herds. The adjusted overall prevalence for Monte Negro municipality was 53.9% (49-58.7%; CI: 95%). The most prevalent serovars were Hardjo (14.5%), Wolffi (12.3%), Shermani (10.8%), Patoc (7.9%), and Hebdomadis (6.1%). Other serovars worldwidely reported like Bratislava, Pomona and Grippotyphosa were detected in low levels.

Abstract in English:

Simionatto S., Lima-Rosa C.A.V., Rubin L.L. & Canal C.W. 2005. [A nested-PCR protocol for detection of the chicken anemia virus.] Um protocolo de “nested-PCR” para detecção do virus da anemia das galinhas. Pesquisa Veterinária Brasileira 25(2):106-110. Laboratório de Virologia, Faculdade de Veterinária, Universidade Federal do Rio Grande do Sul, Av. Bento Gonçalves 9090, Porto Alegre, RS 91540-000, Brazil. E-mail: claudio.canal@ufrgs.br This paper reports a nested polymerase chain reaction (nested-PCR) protocol for detection of chicken anemia virus (CAV), the causal agent of infectious chicken anemia. For DNA extraction from clinical samples, a method based on guanidine thiocyanate was found more sensitive and practical than other extraction protocols tested. The pair of primers used in the initial PCR targeted a 664 bp fragment on the VP1 gene. The primers for the internal PCR targeted a fragment of 520 bp. The specificity of the primers was evaluated on samples of CAV controlled flocks. Thirty different viruses and bacteria isolated from chickens did not give rise to any amplification product in the assay. The sensitivity of the nested-PCR was determined on serial dilutions of a CAV vaccine. The nested-PCR was more sensitive than a one step PCR and was able to detect at least 0.16 TCID50 of the vaccine strain. In addition, the protocol employed here detected viral DNA from tissues, sera and litter from flocks with or without clinical signs of disease. It is concluded that the nested-PCR protocol described here is more sensitive, faster and less cumbersome than virus isolation in cell culture as a diagnostic technique for detection of CAV.

• Chicken anemia virus CAV molecular diagnosis nested-PCR.

Abstract in Portuguese:

Simionatto S., Lima-Rosa C.A.V., Rubin L.L. & Canal C.W. 2005. [A nested-PCR protocol for detection of the chicken anemia virus.] Um protocolo de “nested-PCR” para detecção do virus da anemia das galinhas. Pesquisa Veterinária Brasileira 25(2):106-110. Laboratório de Virologia, Faculdade de Veterinária, Universidade Federal do Rio Grande do Sul, Av. Bento Gonçalves 9090, Porto Alegre, RS 91540-000, Brazil. E-mail: claudio.canal@ufrgs.br This paper reports a nested polymerase chain reaction (nested-PCR) protocol for detection of chicken anemia virus (CAV), the causal agent of infectious chicken anemia. For DNA extraction from clinical samples, a method based on guanidine thiocyanate was found more sensitive and practical than other extraction protocols tested. The pair of primers used in the initial PCR targeted a 664 bp fragment on the VP1 gene. The primers for the internal PCR targeted a fragment of 520 bp. The specificity of the primers was evaluated on samples of CAV controlled flocks. Thirty different viruses and bacteria isolated from chickens did not give rise to any amplification product in the assay. The sensitivity of the nested-PCR was determined on serial dilutions of a CAV vaccine. The nested-PCR was more sensitive than a one step PCR and was able to detect at least 0.16 TCID50 of the vaccine strain. In addition, the protocol employed here detected viral DNA from tissues, sera and litter from flocks with or without clinical signs of disease. It is concluded that the nested-PCR protocol described here is more sensitive, faster and less cumbersome than virus isolation in cell culture as a diagnostic technique for detection of CAV.

Abstract in English:

Lemos E.R.S., D'Andrea P.S., Bonvicino C. R., Famadas K. M., Padula P., Cavalcanti A.A. & Schatzmayr H.G. 2004. Evidence of hantavirus infection in wild rodents captured in a rural area of the state of São Paulo, Brazil. Pesquisa Veterinária Brasileira 24(2):71-73. Depto Virologia, Instituto Oswaldo Cruz, Av. Brasil 4365, Pavilhão Rocha Lima, 5º andar, Manguinhos, Rio de Janeiro, RJ, 21045-900, Brazil. E-mail: elemos@ioc.fiocruz.br Hantaviruses are the etiological agents of the Hantavirus Cardio-Pulmonary Syndrome, a serious rodent-borne disease in Brazil. In order to investigate the occurrence of hantavirus infection in wild rodents, a survey was conducted in three different suburban areas of the municipality of Pedreira, State of São Paulo, Brazil. Of the 145 wild animals captured belonging to 12 different species identified by morphology and karyological analysis, 107 were rodents of the following species: Akodon montensis, Bolomys lasiurus, Calomys tener, Oligoryzomys nigripes, Oligoryzomys flavescens, and Myocastor coypus. Blood samples from these rodents were assayed for the presence of antibodies against hantavirus by IgG ELISA using Andes recombinant nucleocapsid antigen. Antibody reactive to Andes virus was found in two different species, O. nigripes and O. flavescens. These results indicate a potential risk for hantavirus transmission to humans in this area, where reservoir rodents are present in peridomestic settings.

• Hantavirus rodent survey Pedreira São Paulo Brazil.

Abstract in Portuguese:

Lemos E.R.S., D'Andrea P.S., Bonvicino C. R., Famadas K. M., Padula P., Cavalcanti A.A. & Schatzmayr H.G. 2004. Evidence of hantavirus infection in wild rodents captured in a rural area of the state of São Paulo, Brazil. Pesquisa Veterinária Brasileira 24(2):71-73. Depto Virologia, Instituto Oswaldo Cruz, Av. Brasil 4365, Pavilhão Rocha Lima, 5º andar, Manguinhos, Rio de Janeiro, RJ, 21045-900, Brazil. E-mail: elemos@ioc.fiocruz.br Hantaviruses are the etiological agents of the Hantavirus Cardio-Pulmonary Syndrome, a serious rodent-borne disease in Brazil. In order to investigate the occurrence of hantavirus infection in wild rodents, a survey was conducted in three different suburban areas of the municipality of Pedreira, State of São Paulo, Brazil. Of the 145 wild animals captured belonging to 12 different species identified by morphology and karyological analysis, 107 were rodents of the following species: Akodon montensis, Bolomys lasiurus, Calomys tener, Oligoryzomys nigripes, Oligoryzomys flavescens, and Myocastor coypus. Blood samples from these rodents were assayed for the presence of antibodies against hantavirus by IgG ELISA using Andes recombinant nucleocapsid antigen. Antibody reactive to Andes virus was found in two different species, O. nigripes and O. flavescens. These results indicate a potential risk for hantavirus transmission to humans in this area, where reservoir rodents are present in peridomestic settings.

Abstract in English:

Canal C.W., Ferreira D.J., Macagnan M., Fallavena L.C.B., Moraes H.L.S. & Wald V.B. 2004. Prevalence of antibodies against chicken anaemia virus (CAV) in broiler breeders in Southern Brazil. Pesquisa Veterinária Brasileira 24(2):89-92. Centro de Diagnóstico e Pesquisa em Patologia Aviária (CDPA), Faculdade de Veterinária da Universidade Federal do Rio Grande do Sul, Porto Alegre, RS 91540-000, Brazil. E-mail: claudio.canal@ufrgs.br Chicks infected during the first two weeks of life with chicken anaemia virus (CAV) manifest clinical disease that can be avoided if the breeder hens transfer enough antibodies to their progeny. The objective of the present work was to establish the prevalence and titer of anti-CAV antibodies in some Brazilian broiler hen breeder flocks and verify in which phase of life the birds were infected. A total of 1,709 serum samples from 12 broiler hen flocks vaccinated against CAV and 64 unvaccinated flocks were analyzed for CAV antibodies with an enzyme-linked immunosorbent assay (ELISA). All non-vaccinated breeder flocks were found to be infected with CAV, with 89% of the hens tested presenting antibodies, 52% of these with titers considered high enough to protect their progeny against CAV infection. Likewise, all vaccinated hens had antibody titer to CAV capable of conferring protection to their progeny. Thus, vaccination of hens seems capable of conferring protection to chicks against clinically apparent CAV-associated disease.

• Antibodies avian pathology chicken anemia virus CAV epidemiology prevalence.

Abstract in Portuguese:

Canal C.W., Ferreira D.J., Macagnan M., Fallavena L.C.B., Moraes H.L.S. & Wald V.B. 2004. Prevalence of antibodies against chicken anaemia virus (CAV) in broiler breeders in Southern Brazil. Pesquisa Veterinária Brasileira 24(2):89-92. Centro de Diagnóstico e Pesquisa em Patologia Aviária (CDPA), Faculdade de Veterinária da Universidade Federal do Rio Grande do Sul, Porto Alegre, RS 91540-000, Brazil. E-mail: claudio.canal@ufrgs.br Chicks infected during the first two weeks of life with chicken anaemia virus (CAV) manifest clinical disease that can be avoided if the breeder hens transfer enough antibodies to their progeny. The objective of the present work was to establish the prevalence and titer of anti-CAV antibodies in some Brazilian broiler hen breeder flocks and verify in which phase of life the birds were infected. A total of 1,709 serum samples from 12 broiler hen flocks vaccinated against CAV and 64 unvaccinated flocks were analyzed for CAV antibodies with an enzyme-linked immunosorbent assay (ELISA). All non-vaccinated breeder flocks were found to be infected with CAV, with 89% of the hens tested presenting antibodies, 52% of these with titers considered high enough to protect their progeny against CAV infection. Likewise, all vaccinated hens had antibody titer to CAV capable of conferring protection to their progeny. Thus, vaccination of hens seems capable of conferring protection to chicks against clinically apparent CAV-associated disease.

Abstract in English:

RESUMO.- Colodel E.M., Driemeier D. & Pilati C. 2000. [Experimental poisoning by the burs of Xanthium cavanillesii (Asteraceae) in cattle.] Intoxicação experimental pelos frutos de Xanthium cavanillesii em bovinos. Pesquisa Veterinária Brasileira 20(1):31-38. Depto Clínica Médica Veterinária; Faculdade de Agronomia e Medicina Veterinária, UFMT, Av. Fernando Correa da Costa, Cuiabá, MT 78010-900, Brazil. Os frutos moídos de Xanthium cavanillesii Schouw, foram administrados por via oral, em doses única ou repetidas, com intérvalo semanal, a onze bovinos. Desses, quatro morreram. Doses únicas a partir de 5 g/kg foram letais para bovinos. Dose de 3 g/kg produziu sinais clínicos e recuperação em um bovino. Repetições de 4 doses de 3 g/kg para um bovino e 2 doses de 5 g/kg para outro bovino não foram tóxicas. Foram constatadas hipoglicemia e elevação dos níveis séricos de aspartato aminotransferase (AST) nos bovinos que apresentaram sinais clínicos da intoxicação. Os primeiros sinais clínicos nos animais que morreram foram observados entre 6 e 12 horas após a administração dos frutos. A evolução do quadro clínico variou entre 5h30min e 8 horas. O quadro clínico foi semelhante nestes animais sendo que os principais sinais clínicos foram anorexia, apatia, salivação profusa e tremores musculares. Ocorreram também hipomotilidade e atonia ruminal, cólicas abdominais, gemidos freqüentes, ranger de dentes, sudorese generalizada e endoftalmia. As alterações de locomoção observadas foram incoordenação motora, instabilidade do trem posterior, decúbito permanente com movimentos de pedalagem, espasmos musculares e opistótono. As alterações respiratórias foram aumento da freqüência respiratória, respiração laboriosa com ruídos e momentos de apnéia. Finalmente ocorria perda do reflexo palpebral, ausência de reflexo pupilar e morte. No bovino que se recuperou, os primeiros sinais clínicos foram observados 18 horas após a administração e evoluíram num período de aproximadamente 72 horas. Neste bovino, através de biópsias hepáticas, observou-se necrose hepática coagulativa associada a congestão e hemorragias. Necrose hepática coagulativa massiva foi observado por biópsias hepáticas em um bovino que morreu, a partir de 12 horas após a administração dos frutos, associada com alterações nos níveis séricos de glicose e AST. As principais lesões encontradas na necropsia foram no fígado e consistiam de aumento do padrão lobular na superfície capsular e de corte, distensão da vesícula biliar e edema moderado da parede da vesícula biliar. A principal alteração microscópica era caracterizada por necrose coagulativa centrolobular ou massiva associada a congestão e hemorragia e alterações degenerativas nos hepatócitos circunjacentes.

• Plant poisoning Xanthium cavanillesii cattle hepatocellular necrosis Plantas tóxicas bovinos necrose hepatocelular.

Abstract in Portuguese:

RESUMO.- Colodel E.M., Driemeier D. & Pilati C. 2000. [Experimental poisoning by the burs of Xanthium cavanillesii (Asteraceae) in cattle.] Intoxicação experimental pelos frutos de Xanthium cavanillesii em bovinos. Pesquisa Veterinária Brasileira 20(1):31-38. Depto Clínica Médica Veterinária; Faculdade de Agronomia e Medicina Veterinária, UFMT, Av. Fernando Correa da Costa, Cuiabá, MT 78010-900, Brazil. Os frutos moídos de Xanthium cavanillesii Schouw, foram administrados por via oral, em doses única ou repetidas, com intérvalo semanal, a onze bovinos. Desses, quatro morreram. Doses únicas a partir de 5 g/kg foram letais para bovinos. Dose de 3 g/kg produziu sinais clínicos e recuperação em um bovino. Repetições de 4 doses de 3 g/kg para um bovino e 2 doses de 5 g/kg para outro bovino não foram tóxicas. Foram constatadas hipoglicemia e elevação dos níveis séricos de aspartato aminotransferase (AST) nos bovinos que apresentaram sinais clínicos da intoxicação. Os primeiros sinais clínicos nos animais que morreram foram observados entre 6 e 12 horas após a administração dos frutos. A evolução do quadro clínico variou entre 5h30min e 8 horas. O quadro clínico foi semelhante nestes animais sendo que os principais sinais clínicos foram anorexia, apatia, salivação profusa e tremores musculares. Ocorreram também hipomotilidade e atonia ruminal, cólicas abdominais, gemidos freqüentes, ranger de dentes, sudorese generalizada e endoftalmia. As alterações de locomoção observadas foram incoordenação motora, instabilidade do trem posterior, decúbito permanente com movimentos de pedalagem, espasmos musculares e opistótono. As alterações respiratórias foram aumento da freqüência respiratória, respiração laboriosa com ruídos e momentos de apnéia. Finalmente ocorria perda do reflexo palpebral, ausência de reflexo pupilar e morte. No bovino que se recuperou, os primeiros sinais clínicos foram observados 18 horas após a administração e evoluíram num período de aproximadamente 72 horas. Neste bovino, através de biópsias hepáticas, observou-se necrose hepática coagulativa associada a congestão e hemorragias. Necrose hepática coagulativa massiva foi observado por biópsias hepáticas em um bovino que morreu, a partir de 12 horas após a administração dos frutos, associada com alterações nos níveis séricos de glicose e AST. As principais lesões encontradas na necropsia foram no fígado e consistiam de aumento do padrão lobular na superfície capsular e de corte, distensão da vesícula biliar e edema moderado da parede da vesícula biliar. A principal alteração microscópica era caracterizada por necrose coagulativa centrolobular ou massiva associada a congestão e hemorragia e alterações degenerativas nos hepatócitos circunjacentes.