ABSTRACT
Free-range chickens may ingest oocysts of T. gondii present in the environment and consequently harbor virulent strains of this parasite in different tissues, without any clinical signs. Isolation of T. gondii through bioassays on mice and cats from naturally infected chicken tissues has been described in several countries, demonstrating the importance of free-range chickens in the transmission of this parasite. The aim of this study was the genotypic characterization of T. gondii isolates obtained from naturally infected free-range chickens in a rural area of the state of Rio Grande do Sul, Brazil. Brain and heart tissue from 12 chickens seropositive for T. gondii were processed using peptic digestion technique for parasite isolation. From 12 samples subjected to mouse bioassay, nine isolates were obtained. RFLP-PCR genotypic characterization was performed using 11 genetic markers: SAG1, 5'-3'SAG2, alt.SAG2, SAG3, BTUB, GRA6, c22-8, c29-2, L358, PK1 and Apico. Genetic characterization of the isolates revealed the presence of five atypical genotypes according to ToxoDB (# 11, # 55, # 64, # 140 and # 163). Our results showed a wide genetic diversity of T. gondii in free-range chickens in this region.(AU)
Galinhas criadas ao ar livre podem ingerir oocistos de T. gondii presentes no ambiente e, com isso, albergar cepas virulentas desse parasita em diferentes tecidos, sem sinais clínicos. O isolamento de T. gondii por meio de bioensaios em camundongos e gatos, a partir de tecidos de galinhas naturalmente infectadas, tem sido descrito em vários países. Isso demonstra a importância das galinhas caipiras na epidemiologia desse parasita. O objetivo deste trabalho foi caracterizar genotipicamente isolados de T. gondii obtidos de galinhas caipiras naturalmente infectadas em uma área rural do município de Santa Maria, estado do Rio Grande do Sul, Brasil. Fragmentos de cérebro e de coração, de 12 galinhas soropositivas para T. gondii, foram processados pela técnica de digestão péptica para isolamento do parasita. Das 12 amostras submetidas a bioensaio com camundongos, nove isolados foram obtidos. A caracterização genotípica por RFLP-PCR foi realizada utilizando-se 11 marcadores genéticos: SAG1, 5'-3'SAG2, alt.SAG2, SAG3, BTUB, GRA6, c22-8, c29-2, L358, PK1 e Apico e revelou a presença de cinco genótipos atípicos de acordo com o ToxoDB (# 11, # 55, # 64, # 140 e # 163). Os resultados mostraram uma ampla diversidade genética de T. gondii em galinhas caipiras nessa região.(AU)
Subject(s)
Animals , Mice , Toxoplasma , Biological Assay/veterinary , Chickens/virology , Toxoplasmosis, Animal , Genotyping Techniques/veterinary , Rural Areas , Polymerase Chain Reaction/veterinaryABSTRACT
Diarrheagenic (DEC) and avian pathogenic Escherichia coli (APEC) are associated with intestinal and extra-intestinal infections (ExPEC), respectively. We aimed to analyze the antimicrobial susceptibility, gene encoding virulence factors associated to DEC and APEC, and phylogenetic classification in E. coli isolated from 320 samples of feed and ingredients. Antimicrobial susceptibility was performed using the disk diffusion method and Multiple Antibiotic Resistance (MAR) Index and Multi-Drug Resistance (MDR) were calculated. Phylogenetic classification was performed on samples harboring DEC and/or APEC virulence-associated genes. A total of 110 E. coli strains were isolated in 15% (49/320) of the evaluated inputs (n=13 vegetable meal; n=33 animal meal, n=3 feed). In general, the isolates showed the highest rates of antimicrobial resistance to sulfonamide and cefazolin and 18% (20/110) were multi-drug resistant. MAR index of feed samples was the highest (0.467). Six and five strains had APEC and DEC virulence-associated genes, respectively, and belonging to phylogenetic groups A and B1. These findings point to the need for strict microbiological control during the production process of these foods.(AU)
Escherichia coli diarreiogênicas (DEC) e patogênicas para aves (APEC) são associadas a infecções intestinais e extraintestinais (ExPEC), respectivamente. O objetivo do presente trabalho foi avaliar a sensibilidade antimicrobiana, a presença de genes que codificam os fatores de virulência relacionados à DEC e APEC, e a classificação filogenética em E. coli isoladas de 320 amostras de ração para frangos e ingredientes. A sensibilidade antimicrobiana foi determinada pelo método disco-difusão e calculou-se o índice de resistência múltipla aos antimicrobianos (IRMA) e a resistência a múltiplas drogas (MDR). Nas amostras que possuíam genes de virulência relacionados à DEC e/ou APEC, foi realizada a classificação filogenética. Foram isoladas 110 amostras de E. coli em 15% (49/320) dos insumos avaliados (n=13 farelos vegetais; n=33 farinhas de origem animal; n=3 rações). De forma geral, os isolados apresentaram as maiores frequências de resistência antimicrobiana à sulfonamida e à cefazolina e 18% (20/110) foram resistentes a múltiplas drogas. O IRMA das rações foi o mais alto (0,467). Os genes que codificam fatores de virulência associados à APEC e DEC foram detectados em seis e cinco isolados, respectivamente, pertencentes aos grupos filogenéticos A e B1. Os resultados demonstram a necessidade de rigoroso controle microbiológico durante o processo de produção desses alimentos.(AU)
Subject(s)
Animals , Chickens/virology , Virulence Factors , Diarrhea/veterinary , Escherichia coli/isolation & purification , Animal Feed/microbiology , Drug Resistance, MicrobialABSTRACT
The aim was to determine the spread of genetically similar profiles of Campylobacter in chicken carcasses and evaluate their ability to produce transcripts for ciaB, dnaJ, p19 and sodB genes, before and after cultivation in Caco-2 cells. The strains used were isolated from 420 samples of chicken carcasses chilled and frozen ready for marketing. The species were identified by PCR-multiplex, the phylogeny was determined by RAPD-PCR and the presence of transcripts was performed by RT-PCR. We identified 74 (17.6%) of Campylobacter strains, being 55 (74.3%) C. jejuni and 19 (25.7%) C. coli. The phylogenetic relationship demonstrated heterogeneity between isolates of the same species, with absence of clones, indicating the high level of diversity of circulating genotypes. The gene transcription showed conflicting results before and after the culture in Caco-2 cell, so that before cultivation isolates showed greater capacity to transcribe genes related to survival and after the interaction with human cells, the strains showed higher potential to transcribe genes associated with virulence. The result of this study contributes to the understanding of how these seemingly fragile microorganisms are the most prevalent bacterial agents in human gastroenteritis.(AU)
O objetivo foi determinar a disseminação de perfis geneticamente semelhantes de Campylobacter em carcaças de frango e avaliar sua capacidade de produzir transcritos para os genes ciaB, dnaJ, p19 e sodB, antes e após o cultivo em células Caco-2. As cepas utilizadas foram isoladas de 420 amostras de carcaças de frango resfriadas e congeladas prontas para comercialização. As espécies foram identificadas por PCR-multiplex, a filogenia foi determinada por RAPD-PCR e a presença de transcritos foi realizada por RT-PCR. Identificamos 74 (17,6%) das cepas de Campylobacter, sendo 55 (74,3%) C. jejuni e 19 (25,7%) C. coli. A relação filogenética demonstrou heterogeneidade entre isolados da mesma espécie, com ausência de clones, indicando o alto nível de diversidade dos genótipos circulantes. A transcrição gênica mostrou resultados conflitantes antes e após a cultura em células Caco-2, de modo que, antes do cultivo, os isolados apresentaram maior capacidade de transcrever genes relacionados à sobrevivência e após a interação com células humanas, as linhagens apresentaram maior potencial para transcrever genes associados à virulência. O resultado deste estudo contribui para a compreensão de como esses microrganismos aparentemente frágeis são os agentes bacterianos mais prevalentes na gastroenterite humana.(AU)
Subject(s)
Humans , Animals , Zoonoses/etiology , Campylobacter jejuni/isolation & purification , Campylobacter coli/isolation & purification , Chickens/virology , Virulence Factors , Real-Time Polymerase Chain Reaction/veterinary , TranscriptomeABSTRACT
Chickens are considered to be potential reservoirs of Newcastle disease virus (NDV). In this study, six Newcastle disease virus strains were isolated and characterized in Tibetan chickens. The HN gene was sequenced, and phylogenetic relationship to reference strains was studied. The phylogenetic analysis demonstrated that these six isolated strains were closely related to NDV isolates of the reference strains GQ245823, KT002186, KU527561, KJ563939, AY225110, EU305607, KM056357, Y18898, GQ245832, AF077761 and lasota strain. Among them, EU305607, KJ563939 and KM056357 were isolated from India, while lasota strain came from attenuated vaccine widely used in China. Then, mean death time (MDT) and intracerebral pathogenicity index (ICPI) were used to estimate the pathogenicity of the isolates. Pathogenicity experiment showed HNH1 and HN17 to be virulent. Our results indicated that genetically diverse viruses circulate in Tibetan chickens, and based upon the phlogeographic analysis, we estimated the origin of ancestral viruses of the isolates and its sister strains located in India and China (lasota strain). It indicates the importance of continuous surveillance to enhance current understanding of the genetic evolution of the NDV strains.(AU)
Subject(s)
Animals , Female , Newcastle disease virus/genetics , Newcastle disease virus/pathogenicity , Chickens/virology , Phylogeny , TibetABSTRACT
Antimicrobial sensitivity and pathogenicity level of 90 strains of Escherichia coli isolated from livers and intestines from commercial layer hens presenting diarrhea were analyzed. To evaluate the antimicrobial susceptibility, all samples were subjected to antimicrobial susceptibility testing using 11 commercial drugs. The results have showed none of the strains was susceptible to all antibiotics tested. All samples showed resistance to two or more drugs. According to the mortality rate of the birds, the in-vivo pathogenicity test classifies the strains into four classes: high, intermediate, low and nonpathogenic. The test has showed 23 (25.5%) of the samples were highly pathogenic, 21 (23.3%) of intermediate pathogenicity, 23 (25.5%) low pathogenic, and 23 (25.5%) nonpathogenic. When the results of the classes of pathogenicity from isolates have been associated with antimicrobial susceptibility, nonpathogenic strains were less sensitive to the antibiotic ampicillin and increased sensitive to streptomycin antimicrobial compared to the others classes of pathogenic. Nonpathogenic strains showed resistance to many antimicrobials, an alert for poultry, since these bacteria might acquire the virulence genes and infect birds, others animals and even human beings.(AU)
Foram verificados a sensibilidade antimicrobiana e o índice de patogenicidade de 90 amostras de Escherichia coli isoladas do fígado e do intestino de pintainhas de postura comercial com diarreia. Para avaliar a sensibilidade antimicrobiana, todas as amostras foram submetidas ao teste de susceptibilidade antimicrobiana por meio de 11 drogas comerciais. Os resultados demonstraram que nenhuma das estirpes foi sensível a todos os antimicrobianos testados. Todas as amostras apontaram resistência a duas ou mais drogas. De acordo com o índice de mortalidade das aves, o teste de patogenicidade in vivo classificou as estirpes em quatro classes: alta, intermediária, baixa e não patogênica. O teste revelou que 23 (25,5%) das amostras foram de alta patogenicidade, 21 (23,3%) de patogenicidade intermediária, 23 (25,5%) de baixa patogenicidade e 23 (25,5%) não patogênicas. Quando os resultados das classes de patogenicidade dos isolados foram associados à sensibilidade antimicrobiana, estirpes não patogênicas apresentaram menor sensibilidade ao antimicrobiano ampicilina e maior sensibilidade ao antimicrobiano estreptomicina, quando comparadas com as estirpes das demais classes de patogenicidade. Estirpes não patogênicas exibiram resistência a vários antimicrobianos, representando um alerta para a avicultura, uma vez que essas bactérias podem adquirir genes de virulência e, assim, infectar aves, outros animais e até mesmo o seres humanos.(AU)
Subject(s)
Animals , Microbial Sensitivity Tests , Chickens/virology , Escherichia coli/pathogenicity , Anti-Infective Agents , Poultry , BirdsABSTRACT
In order to investigate the immune enhancement effects of Ophiopogon japonicus polysaccharide Ophiopogon japonicus (OJPS) on Newcastle disease (ND) live vaccine, chickens vaccinated against ND live vaccine was orally administered with the OJPS at high, medium and low concentrations respectively. In negative control group, chickens were given orally equal volume of physiological saline. On day 14, 21 and 28, the serum antibody titer, erythrocyte-C3b receptor rosette rate (E-C3bRR), erythrocyte-C3b immune complex rosette rate (E-ICRR) and peripheral lymphocyte proliferation were measured. The results showed that at most time points, the antibody titer, peripheral lymphocyte proliferation, E-C3bRR and elimination rate of immune complex of three OJPS administrating groups were significantly higher (P<0.05) than those in negative control group. It indicated that OJPS could significantly improve the immune efficacy of Newcastle disease live vaccine, Ophiopogon japonicus polysaccharide possessed synergistical immunoenhancement.(AU)
Subject(s)
Animals , Chickens/virology , Newcastle Disease/immunology , Ophiopogon/chemistry , Viral Vaccines/analysis , Adjuvants, Immunologic , Antibodies/blood , Erythrocytes/immunology , Lymphocytes/immunologyABSTRACT
Enteric disease is a multifactorial problem in chickens, which causes gastrointestinal alterations, elevated feed conversions and impairment. In the last years, several enteric viruses were implicated in enteric disease; case reports have shown their presence alone or in concomitant infections during outbreaks and have suggested that they might be determining factors in the aetiology of enteric disease. This study shows high detection rates of enteric viruses in the pancreas and spleen in samples from an outbreak of enteritis and malabsorption in 16 chicken flocks (n=80 broilers). Avian nephritis virus (ANV) was the most ubiquitous virus, present in 75% of the flocks followed by avian rotavirus group A (ART-A) with 68.75%, and by chicken astrovirus (CAstV) and chicken parvovirus (ChPV) in 43.75% of samples. Viruses were present in the pancreas of positive flocks at extremely high rates: 100% for ART-A, 91.7% for ANV, 100% for CAstV and 57.14% for ChPV. By contrast, only 16.7% and 57.14% of intestine samples were positive for ANV and CAstV, respectively. Avian reovirus (AReo) and avian adenovirus group 1 (FAdV-1) were not detected. These results suggest that high viral detection rates in pancreas samples may be a result of viremia during enteric disease, with subsequent damage of the exocrine pancreas, leading to runting-stunting syndrome (RSS).(AU)
A doença entérica é um problema multifatorial em galinhas que causa alterações gastrointestinais, conversão alimentar elevada e deficiência de crescimento. Nos últimos anos, os vírus entéricos foram associados à doença entérica; casos reportados mostraram a infecção de um único vírus e também infecções concomitantes durante os surtos sugerindo a presença de múltiplos fatores etiológicos nas doenças entéricas. Este estudo mostra uma alta taxa de detecção dos vírus entéricos em amostras de pâncreas e baço de um surto de enterite e má-absorção em 16 lotes de frangos (n=80 frangos). O vírus de nefrite aviária (ANV) foi o vírus mais detectado, estando presente em 75% dos lotes seguido pelo rotavírus aviário grupo A (ART-A) em 68,75% dos casos, e pelo astrovirus (CAstV) e parvovírus aviários (ChPV), ambos em 43,75% das amostras. Os vírus estavam presentes no pâncreas dos lotes positivos em percentuais elevados: 100% para ART-A e CAstV; 91,7% para ANV, e em 57,14% para ChPV. Em contraste, somente 16,7% e 57,14%, em amostras de intestino, foram positivos para ANV e CAstV, respectivamente. Reovírus aviário (AReo) e o adenovírus do grupo 1 (FAdV-1) não foram detectados. Estes resultados sugerem que os elevados percentuais de vírus detectados em amostras de pâncreas podem estar associados à viremia durante a doença entérica, com subsequente lesão no pâncreas exócrino das aves levando ao desenvolvimento da síndrome de nanismo e raquitismo.(AU)
Subject(s)
Animals , Avastrovirus/isolation & purification , Chickens/virology , Malabsorption Syndromes/diagnosis , Malabsorption Syndromes/veterinary , Parvovirus/isolation & purification , Dwarfism/diagnosis , Dwarfism/veterinary , Gastrointestinal Diseases/veterinary , Pancreas/physiopathology , Real-Time Polymerase Chain Reaction/veterinary , Rickets/diagnosis , Rickets/veterinary , Spleen/virologyABSTRACT
Newcastle disease vaccines
Subject(s)
Animals , Chick Embryo , Chickens/virology , Newcastle disease virus/pathogenicity , Poultry Diseases/prevention & control , Vaccines, Attenuated/therapeutic use , Viral Vaccines/therapeutic use , Cell Culture Techniques , Cells, Cultured , Chickens/immunology , Newcastle disease virus/classification , Newcastle disease virus/growth & development , Primary Cell Culture , Poultry Diseases/immunology , Poultry Diseases/virology , Vaccination , Vaccines, Attenuated/adverse effects , Vaccines, Attenuated/immunology , Viral Vaccines/adverse effects , Viral Vaccines/immunologyABSTRACT
A Brazilian field isolate (IBV/Brazil/PR05) of avian infectious bronchitis virus (IBV), associated with development of nephritis in chickens, was previously genotyped as IBV variant after S1 gene sequencing. The aim of this study was to evaluate the levels of IL-6 in kidneys and trachea of birds vaccinated and challenged with IBV/Brazil/PR05 strain, correlating these results with scores of microscopic lesions, specific IBV antigen detection and viral load. The up-regulation of IL-6 and the increased levels of viral load on renal and tracheal samples were significantly correlated with scores of microscopic lesions. Reduced levels of viral load were detected in kidneys of birds previously vaccinated and challenged, compared to non-vaccinated challenged group, although markedly microscopic lesions were observed for both groups. The expression of IL-6, present both in the kidney and in the tracheas, was dependent on the load of the virus present in the tissue, and the development of lesions was related with IL-6 present in the tissues. These data suggest that variant IBV/Brazil/PR05 can induce the expression of proinflammatory cytokines in a manner correlated with viral load and increased IL-6 is involved in the tissue with the influx of inflammatory cells and subsequent nephritis. This may contribute with a model to the development of immunosuppressive agents of IL-6 to prevent acute inflammatory processes against infection with IBV and perhaps other coronaviruses, as well as contribute to the understanding of the immunopathogenesis of IBV nephropatogenic strains.
Uma estirpe variante do vírus da bronquite infecciosa (VBI) associada com o desenvolvimento de nefrite em galinhas, foi isolado e identificado como variante por análise do gene S1. A estirpe IBV/Brazil/PR05 foi testada quanto à sua capacidade de induzir a expressão de interleucina-6 (IL-6) nos tecidos renais e traqueais. Galinhas vacinadas com a estirpe Massachusetts H120 e não vacinadas foram desafiadas com a estirpe IBV/Brazil/PR05. Cinco dias após a infecção, traquéias e rins foram coletados para análise por RT-qPCR, imunohistoquímica e histopatologia. Foi determinada a expressão relativa de IL-6 e da carga viral. A expressão de IL-6 e carga viral foram correlacionadas com o desenvolvimento de nefrite e lesão traqueal. A expressão de IL-6 foi maior quando houve aumento da carga viral na traqueia e nos rins. A carga viral presente nos rins foi inferior quando as aves foram vacinadas, entretanto foi observada nefrite acentuada. Houve alta correlação entre o desenvolvimento de nefrite e o nível de expressão de IL-6, bem como a expressão de IL-6 e a carga viral. A expressão de IL-6, presente tanto nos rins e nas traqueias, foi relacionada a carga viral presente nestes tecidos, e o desenvolvimento das lesões foi relacionado com a expressão de IL-6. Estes dados sugerem que a variante IBV/Brazil/PR05 pode induzir a expressão de citocinas pró-inflamatórias de forma correlacionada com a carga viral, e o aumento de IL-6 está envolvido com o influxo de células inflamatórias no tecido, o que evolui para o desenvolvimento de nefrite. Isto pode contribuir como um modelo para o desenvolvimento de agentes imunossupressores da IL-6 para evitar processos inflamatórios agudos contra infecção com o VBI e talvez outros coronavírus, bem como contribuir para o entendimento da imunopatogênese das estirpes nefropatogênicas deste vírus.
Subject(s)
Animals , Chickens/virology , /isolation & purification , Nephritis/veterinary , Infectious bronchitis virus/isolation & purification , Real-Time Polymerase Chain Reaction/veterinary , Kidney/pathology , Trachea/pathologyABSTRACT
Although the infection of different animals and non-human primates with other members of Anelloviridae have already been reported there is no report about infection of animals with Torque teno midi virus/Small anellovirs [TTMDV/SAV]. The aim of this study was to detect the virus in domestic village chickens. Blood samples were collected from 79 domestic village chickens in Isfahan. Blood samples of five adult laying hens and one cockerel were collected in three consecutive weeks [days 1, 8 and 14] as experimental chickens. Ten eggs were randomly collected from the eggs laid during days 12 to 17 and thin and thick egg whites and yolk samples were collected aseptically. After DNA extraction Nested-PCR was performed using SMAs/SMAr primers. In PCR, 431 bp and 441 bp products were detected. The detected bands were extracted and sequenced. Totally 26 out of 79 [32.9%] of the blood samples were positive for the virus. The frequency of the infection of the different parts of the eggs tested was 76%. For the first time TTMDV/SAV was detected in domestic village chickens which also vertically transmitted to eggs
Subject(s)
Animals , Anelloviridae , Chickens/virology , Infectious Disease Transmission, Vertical , EggsABSTRACT
Commercial broiler flocks from a farm located in the State of São Paulo, Brazil, presented diarrhea, depression, increased mortality and poor weight gain. Upon post-mortem examination, classical signs of Inclusion Body Hepatitis/Hydropericardium Syndrome (IBH/HPS) were observed, including enlarged pale yellow-colored livers and straw-colored liquid in the pericardial sac. In addition, gross lesions were also observed in the kidneys, pancreas, thymus, intestines and gallbladder. Samples of these organs were analyzed by PCR for the detection of the hexon gene of the Fowl Adenovirus (FAdVs) Group I. The results were positive for both flocks (A and B) assayed by PCR. The macroscopic lesions associated with the detection of FAdV Group I by PCR in several of these affected organs allowed for the identification of IBH/HPS. In fact, this is the first report in Brazil of IBH/HPS in broilers, which identifies FAdVs group I as a causal agent of the disease. These findings may contribute to the worldwide epidemiology of the adenovirus-mediated hepatitis/hydropericardium syndrome...
Lotes comerciais de frangos de uma granja localizada no Estado de São Paulo, Brasil, apresentavam diarreia, depressão, aumento de mortalidade e baixo ganho de peso. Após o exame post-mortem, sinais clássicos da síndrome de hepatite por corpúsculo de inclusão/hidropericárdio (IBH/HPS) foram observados incluindo hepatomegalia com aspecto amarelado pálido e líquido de coloração amarelo palha no saco pericárdio. Além disso, as alterações macroscópicas foram também observadas nos rins, pâncreas, timo, intestinos e vesícula biliar. Amostras destes órgãos foram analisadas pela técnica de PCR para detectar o adenovírus aviário do grupo I através do gene Hexon. Os resultados foram positivos para ambos os lotes (A e B) utilizando-se a técnica de PCR. As lesões macroscópicas associadas à detecção do adenovírus aviário do grupo I pela técnica de PCR em vários destes órgãos acometidos permitiu a identificação da síndrome de hepatite/hidropericárdio em frangos no Brasil. Ao nosso conhecimento, este é a primeira descrição da síndrome de hepatite/hidropericárdio causado por adenovírus aviário do grupo I, no Brasil. Estes achados podem contribuir com a epidemiologia mundial do adenovírus mediando a síndrome de hepatite/hidropericárdio...
Subject(s)
Animals , Aviadenovirus/isolation & purification , Chickens/virology , Hepatitis, Viral, Animal/diagnosis , Autopsy/veterinary , Polymerase Chain Reaction/veterinaryABSTRACT
Canarypox viruses (CNPV) carrying the coding sequence of VP2 protein from infectious bursal disease virus (IBDV) were obtained. These viruses were able to express VP2 protein in vitro and to induce IBDV-neutralizing antibodies when inoculated in specific pathogen-free chickens demonstrating that CNPV platform is usefulness to develop immunogens for chickens.
Subject(s)
Animals , Chickens/virology , Viral Proteins , Infectious bursal disease virus , Canarypox virusABSTRACT
A recent (November 2010) outbreak of infectious laryngotracheitis (ILT) in a multi-age laying hen facility in Minas Gerais state, Brazil, is described. Previous ILT outbreak in laying hens was only notified in São Paulo state, Brazil, in 2002. In the outbreak described here, the affected population was approximately eight million hens, with flock sizes ranging from 100,000 to 2,900,000 chickens. The average mortality ranged from 1 to 6%, and morbidity was around 90% (most of the twenty seven farms of the area were positive for ILT virus). Three multi-age laying farms from one company were selected for this report. Clinical signs included prostration, dyspnea, conjunctivitis, occasional swelling of the paranasal sinuses and bloody mucous nasal discharge. Severely affected chickens presented with dyspnea, gasping and became cyanotic before death. At necropsy, these chickens had fibrinous exudate blocking the larynx and the lumen of cranial part of the trachea. In addition, conjunctivitis with intense hyperemia, edema and sinuses with caseous exudate were present. On histopathology, there were marked necrosis and desquamation of respiratory ephitelium and conjunctiva with numerous syncytial cells formation and fibrinous exudate. Moderate to marked non suppurative (especially lymphocytes and plasma cells) infiltration in the lamina propria also was observed. Sixteen out of 20 examined chickens, eosinophilic intranuclear inclusion bodies were observed in the syncytial cells. The DNA extracted from larynx and trachea produced positive PCR results for ILT virus (ILTV) DNA using formalin-fixed, paraffin embedded (FFPE) samples. Amplicons from a small region of ICP4 gene were submitted to sequencing and showed 100% identity with ILTV EU104910.1 (USA strain), 99% with ILTV JN596963.1 (Australian strain) and 91% with ILTV JN580316.1 (Gallid herpesvirus 1 CEO vaccine strain) and JN580315.1 (Gallid herpesvirus 1 TCO vaccine strain).
Um surto recente (Novembro de 2010) de laringotraqueite infecciosa (LTI) em granjas de postura de múltiplas idades em Minas Gerais, Brasil, é descrito. Um surto de LTI em galinhas de postura havia sido previamente relatado apenas no Estado de São Paulo em 2002. No surto aqui descrito, a população afetada foi de aproximadamente oito milhões de galinhas, com lotes variando de 100.000 a 2.900.000 galinhas. A mortalidade média variou de 1 a 6% e a morbidade atingiu cerca de 90% (a maioria das 27 granjas foram positivas para o virus da LTI). Três granjas com aves de múltiplas idades pertencentes a uma empresa foram selecionadas para o presente relato. Os sinais clinicos incluíram prostração, dispneia, conjuntivite, edema ocasional dos seios paranasais e secreção nasal mucosa e/ou sanguinolenta. As aves severamente afetadas apresentaram acentuada dispneia, aparente engasgo e tornaram-se cianóticas antes da morte. Nestas aves, exsudato fibrinoso denso obstruindo o lúmen da laringe e parte cranial da traqueia foi observado na necropsia. Havia também, conjuntivite com hiperemia intensa e edema, além de sinusite com exsudato caseoso. Na histopatologia, observaram-se necrose e descamação acentuada do epitélio respiratório e da conjuntiva com formação de numerosos sincícios e exsudato fibrinoso. Além disso, infiltrado inflamatório mononuclear (especialmente linfócitos e plasmócitos) moderado a acentuado na lâmina própria foi observado. Corpúsculos de inclusão intranucleares nas células sinciciais foram observados em 16 das 20 aves examinadas. Resultados positivos pela PCR para o virus da LTI foram obtidos de DNA extraído das laringes e traqueias utilizando amostras fixadas em formol e incluidas na parafina. O produto amplificado de uma região pequena do gen ICP4 foi submetido ao sequenciamento e quando comparado com outras sequências depositadas no Genbank mostrou os seguintes resultados: 100% de identidade com uma estirpe do virus de LTI dos Estados Unidos (JN596963.1), 99% de identidade com uma estirpe Australiana e 91% com a estirpe vacinal CEO (JN580316.1) e TCO (JN580315.1).
Subject(s)
Animals , Chickens/virology , Herpesvirus 1, Gallid/isolation & purification , Polymerase Chain Reaction/veterinary , Dyspnea/veterinaryABSTRACT
Infectious bursal disease [IBD] is one of the most important viral poultry diseases. To prevent the disease it is required that there be maternal and active immunity prior to and after three weeks of age. Live vaccines are usually used to immunize the broiler flocks. In addition to the type of vaccine, the route of vaccination, also, has effects on mounting an immune response. In this study, we administered a single dose vaccination of an intermediate IBD vaccine strain at 21 days of age via five routes including subcutaneous [SC], intramuscular [IM], drinking water, eye drop, and course spray. The impact of the vaccination route on mounting antibody response was evaluated by a commercial ELISA kit [IDEXX]. Antibody response was mounted by all routes. The highest antibody titer in the last two sampling turns belonged to birds in the group vaccinated by the SC route, but this difference was not statistically significant [p>0.05] when compared to those of other vaccinated groups. In addition to the highest antibody titer, the highest bursal/body weight ratio and body weight were observed in birds of the SC-vaccinated group. It was found that the groups vaccinated by injection, SC or IM, were the only groups that achieved to a protective level of antibody titer in the last turn of sampling. It was concluded that a single dose injection of an intermediate IBD vaccine, via SC route, is able to induce higher antibody response, and improve bursal health and performance of chickens as compared with those vaccinated via drinking water
Subject(s)
Animals , Vaccines, Attenuated , Drug Administration Routes , Birnaviridae Infections/prevention & control , Enzyme-Linked Immunosorbent Assay , Chickens/virologyABSTRACT
The current study was conducted to investigate the incidence of IBV in commercial chicken farms suspected of having IBV infection, as well as other available avian species [turkeys, pigeons, parrots and canaries] revealed respiratory manifestations. Reverse-transcriptase polymerase chain reactions [RT-PCRs] were used to examine RNA extracted from tracheal swabs as well as corresponding harvested inoculated allantoic fluids. The universal oligonucleotide primers used were based on conserved sequences of IBV nucleocapsid [N] protein to ensure a very wide detection range. The overall RT-PCRs detection rates were 24/65 [37%] for the swab samples and 18/65 [28%] for allantoic harvests, while the revealing rates varied between 12/15 [80%], 10/15 [66.7%] in chickens, 5/15 [33.3%], 3/15 [20%] in turkeys, 3/15 [20%], 3/15 [20%] in pigeons and 4/15 [26.7%]. 2/15 [13.3%] in parrots for the swab samples and allantoic harvests respectively. It could be concluded that: RT-PCR using this universal oligonucleotide primer can be used to screen field samples suspected of containing IBVs. Once positive samples are identified, they are inoculated into embryonating chicken eggs for traditional virus isolation, serotyping and gene sequences. In addition; there is a real threat of IB spreading among chickens and other avian species[indeed, present in Turkeys, Pigeons and parrots]. However, it remains unclear how this virus emerged in that birds so further studies are recommended. For the author knowledge no previous statement of IBV infection in other avian species in Egypt were recorded
Subject(s)
Chickens/virology , Polymerase Chain Reaction/methods , Incidence , Serotyping , Bird Diseases/virologyABSTRACT
Variações genética e antigênica são observadas com frequência elevada entre estirpes do VBIG e envolvem principalmente a glicoproteína S1. Com o objetivo de contribuir com a disponibilidade de ferramentas para o imunodiagnóstico e a imunoprofilaxia da bronquite infecciosa das galinhas foi desenvolvida uma metodologia para expressão recombinante da glicoproteína S1 na levedura Picchia pastoris. O cDNA do gene codificador dessa proteína foi obtido a partir de RNA viral de ovos embrionados infectados com a estirpe M41 do VBIG submetido à transcrição reversa (RT) e reação em cadeia da polimerase (PCR), amplificando-se a sequência codificadora de S1 acrescida de extremidades compatíveis com a clonagem no vetor usado na transformação de leveduras. A indução com metanol resultou na produção de uma proteína detectada como banda única do tamanho previsto, em western-blot, no lisado celular das leveduras transformadas. A expressão em P. pastoris mostrou ser um método eficaz para a produção recombinante da proteína S1 do VBIG, com potencial para utilização em técnicas de imunodiagnóstico da bronquite infecciosa das galinhas.
Genetic and antigenic variation are very frequently observed among IBV strains and affect mainly the S1 glycoprotein. In order to contribute to the availability of tools for immunodiagnosis and immunoprophylaxis of chicken infectious bronchitis we developed an expression system for production of recombinant S1 glycoprotein in Pichia pastoris. We obtained the cDNA from viral RNA on embryonated eggs infected with the M41 strain of IBV, by reverse transcription (RT) and polymerase chain reaction (PCR), amplifying the S1 coding sequence with extremities compatible with the vector used to transform yeast. Induction with methanol led to the production of a protein with the predicted molecular weight that was detected by Western blot in the cell lysate of transformed yeast. Expression in P. pastoris proved to be an effective method for recombinant production of S1 protein from IBV, with potential for use in immuno-diagnosis of chicken infectious bronchitis virus.
Subject(s)
Animals , Pichia/ultrastructure , Glycoproteins/analysis , Chickens/virology , Viral Fusion Proteins/analysis , Infectious bronchitis virus/geneticsABSTRACT
Newcastle disease is one of the most important causes of economic losses in the poultry production and can he resulted in high mortality. Antibody detection is also an important tool for assessment of the immunity against the disease. In the present study a trial was conducted to evaluate the effect of an immune stimulator[Echinacea purpurea] on antibody production against Newcastle disease vaccine. 450 one day old broiler chicks were divide into five groups of three repeat each. For three weeks from day one various doses of Echinacea purpurea extract was prescribed to four treatment groups and to the fifth group placebo in water was prescribed. All groups were vaccinated on days:11, 19, 38. Subsequently. serum samples were collected at days 10. 25, 34.52 of post vaccination from 21 chicks of each group [4 samples of each repeat] and were tested for Newcastle antibody titers by HI test. This experiment showed that the use of Echinacea purpurea extract with the rate of 29, 75Mg per kilo body weight per day had better effects on antibody titers and significantly increased between control group arid treatment groups [p<0.01]. It is also revealed that the use of Echinacea purpurea induces FCR improvement and mortality rate was decreased significantly [p<0.01]
Subject(s)
Animals , Newcastle Disease/prevention & control , Newcastle Disease/immunology , Plant Extracts/pharmacology , Antibody-Producing Cells/drug effects , Adjuvants, Immunologic , Hemagglutination , Chickens/virologyABSTRACT
Epidemiological studies on AI virus in different governorates in Egypt [Alexandria, Bohera, Gharbia, Kafr El Sheikh, Fayoum and Menofia] during 2007 to 2009 were carried out. These studies included broiler, layer and breeder flocks in addition to duck flocks and pigeon samples. Using the RT-PCR and Chromatography test, the data revealed the following: A total of 29 out of 59, 5 out of 11 and 2 out of 5 broiler, layer and breeder examined flocks were positive with a percentage of 49.2%, 45.5% and 40% respectively. Regard to duck flocks, 10 examined flocks were negative but 2 birds out of 82 pigeon samples were positive with a percentage of 2.4%. The data clearly indicated that the highest outbreaks with AI virus were recorded in broiler flocks followed by layer and breeder flocks, then pigeon samples. The data also, indicated that the chromatography test is a highly sensitive test used for detection of the avian influenza virus. The phylogenetic analysis of the full length genome sequences of the eight viral segments from virus isolates from chicken revealed that the clustering of our samples was within clade 2.2. The isolates had the multiple basic sequences in the heamagglutinin gene at cleavage site indicating a highly pathogenic phenotype. Sequence analysis of the eight gene segments showed nucleotide as well as amino acid substitutions
Subject(s)
Animals , Reverse Transcriptase Polymerase Chain Reaction/methods , Chromatography/methods , Chickens/virologyABSTRACT
In this study, 8000 Hubbared 1-day old broiler chicks having maternal antibodies to infectious bursal disease [IBD] were reared on deep litter in a poultry farm. The chicks were received IBD [Bursine-2] intermediate vaccine at the 12[th] day of life via drinking water to investigate its immunogenicity and its effect on broiler performance. No IBD related clinical signs or mortalities or lesions were observed after vaccination till the end of the breeding period [7 weeks]. The result of serological response to IBDV vaccines using ELISA test showed that the maternal antibody titer to IBD antigen in 1 day old chicks was 5571.1 +/- 1761.8 and waned to1237.7 +/- 915.8 at 2 weeks [2 days after vaccination. At the 3[rd] and 4[th] weeks after vaccination IBD ELISA titres were increased to 2662.1 +/- 186.3 and 3394.1 +/- 768.8; respectively. This result revealed that the used live IBD vaccine was able to induce antibody levels in chickens with maternal IBD antibodies. The best weekly feed conversion rate [FCR] was recorded at the 4[th] week [1.31] and the 6[th] week [1.71] with total FCR of 1.89. Mortality rate in the susceptible age [2-6 week] was the lowest [0.4-.73%] with total mortality of 3.27 at the end of the 7[th]. These fining pointed out that live IBD intermediate Burcin-2 vaccine was save, immunogenic to maternally immune chicks and has no adverse effect on performance of vaccinate chickens
Subject(s)
Chickens/virology , Vaccines, Attenuated/immunologyABSTRACT
Infectious bursal disease (IBD) is an acute, contagious, viral disease of young chickens characterized by diarrhea, ventpicking, trembling, incoordination, inflammation followed by atrophy of the bursa of Fabricius and by variable degrees of immunosuppression. The diseases is caused by the infectious bursal disease virus (IBDV) which upon its antigenic characteristics and pathogenicity has been classified as classic (mild, intermediate and intermediate plus) strains, very virulent IBDV (vvIBDV) and variant strains. With the widespread presence of vvIBDV, the poultry industry has resorted to the use of less attenuated vaccines raising the concern about bursal integrity after vaccination. IBD vaccination using intermediate plus vaccine strains can temporarily deplete the bursal follicles and interrupt the normal B-cell development; if the damage is reversible this process can be followed by B-cell repopulation and histological regeneration. In order to assess this bursal restoration process, specific pathogen free birds were vaccinated with intermediate and intermediate plus IBDV vaccine and bursas were evaluated by histopathology and immunohistochemistry. Both B and T cells were detected in the recovering bursas. At the end of the trial, signs of bursal regeneration and B cell repopulation were observed in the intermediate IBDV vaccinated birds. The bursal restoration process was impaired or delayed in the intermediate plus vaccine group. Relevance of B and T cell repopulation is discussed.
La enfermedad infecciosa de la bolsa (por sus siglas en Inglés IBD) es una enfermedad viral aguda y contagiosa que afecta a los pollos jóvenes, caracterizada por diarrea, picado de la cloaca, temblores, incoordinación, inflamación seguida de atrofia de la bolsa de Fabricious y por grados variables de inmunosupresión. La enfermedad es causada por el virus de la enfermedad infecciosa de la bolsa (por sus siglas en Inglés IBDV) que basado en sus características antigénicas y de patogenicidad ha sido clasificado en cepas clásicas (virus suaves, intermedios e intermedios plus), IBDV muy virulento y cepas variantes. Debido a la amplia presencia de IBDV muy virulento, la industria avícola ha implementado la utilización de vacunas menos atenuadas, lo que genera preocupación por la integridad de la bolsa posterior a la vacunación. La vacunación contra IBD utilizando vacunas intermedias plus puede despoblar los folículos de la bolsa e interrumpir el desarrollo normal de las células B, si el daño es reversible este proceso puede ser seguido de la repoblación de la bolsa con células B y de regeneración histológica. Con la finalidad de evaluar este proceso de restauración, se vacunaron aves libres de patógenos específicos con vacunas intermedia e intermedia plus contra IBDV y se evaluaron las bolsas mediante histopatología e inmunohistoquímica. En las bolsas en recuperación se detectaron tanto células B como células T. Al final del experimento, en las aves vacunadas con la cepa intermedia se observaron signos de regeneración de la bolsa y repoblación de células B. El proceso de restauración de la bolsa se vio comprometido o retrasado en el grupo vacunado con la cepa intermedia plus. Se discute la relevancia de la repoblación de la bolsa con células T y B.