Detecção de possíveis agentes virais associados à circovirose suína. / Detection of possible viral agents associated with postweaning multisystemic wasting syndrome

Teixeira, Thais Fumaco

January 2008

O Circovirus suíno tipo 2 (PCV2) é um vírus ubíquo que tem sido associado a um número de síndromes em suínos. Entre elas, a Síndrome Multissistêmica do Definhamento dos Suínos (SMDS) tornou-se uma das principais causas de perdas econômicas na suinocultura nacional. No entanto, existe incerteza se o PCV2 é, de fato, o único agente responsável por esse quadro, essencialmente porque a administração isolada do vírus a animais suscetíveis não tem sido capaz de reproduzir experimentalmente a síndrome. Em vista disso, um número de outros agentes infecciosos (e não infecciosos) tem sido examinados e sua potencial participação no desenvolvimento da SMDS tem sido pesquisada. No presente estudo foram realizados experimentos visando determinar se outro(s) agente(s) com genoma de DNA circular poderia(m) desempenhar algum papel no desenvolvimento da SMDS. Para tanto, a técnica denominada “amplificação por círculo rolante com múltiplos primers” (ACRMP) foi empregada. A ACRMP é baseada na atividade da DNA polimerase do fago phi29, uma enzima capaz de sintetizar novas moléculas de DNA a partir de um molde de DNA circular. Numa segunda etapa, o DNA amplificado é clivado com enzimas de restrição, ocasionando a linearização de grande quantidade de cópias do DNA alvo original. Como a ACRMP é realizada com primers aleatórios, nenhum conhecimento prévio da seqüência de nucleotídeos alvo é necessário. Portanto, pode-se teoricamente amplificar DNA circular de qualquer microorganismo, o que a torna ideal para o propósito do presente estudo. O DNA extraído de soros de 67 suínos com sinais clínicos de SMDS, assim como de 63 suínos saudáveis, foram submetidos à ACRMP. O principal achado deste estudo foi que o genoma de um (ou mais) anelovírus foi(ram) detectado(s) em 88,9% (56/63) dos suínos saudáveis, ao passo que o(s) mesmo(s) agente(s) somente foi(ram) detectado(s) em 16,4% (11/67) dos soros de suínos com sinais clínicos da SMDS. Alguns fragmentos de DNA potencialmente correspondentes a fragmentos de genomas virais foram seqüenciados, revelando que pelo menos um deles corresponde a uma seqüência de anelovírus suíno ainda não descrita. No entanto, outro genoma correspondente a um anelovírus foi encontrado na mesma amostra, sugerindo que mais de um vírus pode estar presente em amostras de soro. Estes resultados demonstraram que os anelovírus, de grande variabilidade genética, são significativamente mais prevalentes em suínos clinicamente saudáveis do que em suínos com SMDS. / Porcine circovirus type 2 (PCV2) is an ubiquitous virus that has been associated to a number of syndromes in swine. Among these, Postweaning Multisystemic Wasting Syndrome (PMWS) has become a major cause of economic losses in swine worldwide. However, there is uncertainty as to whether PCV2 is in fact the sole agent responsible for the disease, essentially because the disease has not been experimentally reproduced when PCV2 is inoculated onto susceptible animals. In view of that, a number of other infectious (and non infectious) agents have been examined and their potential role in PMWS searched for. This study was carried out to determine whether any other agent(s) with circular DNA genome might be playing some role in PMWS. In order to achieve that, a technique called “randomly primed rolling circle amplification” (RPRCA) was employed. RPRCA is based on the activity of bacteriophage phi29 DNA polymerase, an enzyme that synthesizes new DNA molecules starting from a circularized DNA template. In a second phase, the amplified DNA is cleaved with restriction enzymes, so giving rise to large amounts of linearized copies of the original target DNA. As RPRCA is performed with random priming, no previous knowledge of the target nucleotide sequence is necessary. Therefore, it is theoretically possible to amplify circular DNA of any microorganism, thus making it ideal for the purpose of the present study. DNA extracted from sera of 67 pigs with clinical signs of PMWS as well as from 63 healthy pigs was submitted to RPRCA. The major finding of this study was that the genome of one (or more) anelloviruses was detected in 88,9% (56/63) of the healthy pigs, whereas the same agent was only detected in 16,4% (11/67) of pigs with clinical signs of PMWS. Some of the DNA fragments corresponding to the putative virus genomes were sequenced and revealed at least one non-previously described anellovirus sequence. However, other anellovirus could be found on the same sample, suggesting that more than one genome are present in samples of serum. These results demonstrate that anelovírus, of great genetic variability, were significantly more prevalent in healthy pigs than in pigs with PMWS.

Circovirose suína

Vírus

Porcine circovirus

PCV2

PMWS

Co-infections

TTV

Detecção de possíveis agentes virais associados à circovirose suína. / Detection of possible viral agents associated with postweaning multisystemic wasting syndrome

Teixeira, Thais Fumaco

January 2008

O Circovirus suíno tipo 2 (PCV2) é um vírus ubíquo que tem sido associado a um número de síndromes em suínos. Entre elas, a Síndrome Multissistêmica do Definhamento dos Suínos (SMDS) tornou-se uma das principais causas de perdas econômicas na suinocultura nacional. No entanto, existe incerteza se o PCV2 é, de fato, o único agente responsável por esse quadro, essencialmente porque a administração isolada do vírus a animais suscetíveis não tem sido capaz de reproduzir experimentalmente a síndrome. Em vista disso, um número de outros agentes infecciosos (e não infecciosos) tem sido examinados e sua potencial participação no desenvolvimento da SMDS tem sido pesquisada. No presente estudo foram realizados experimentos visando determinar se outro(s) agente(s) com genoma de DNA circular poderia(m) desempenhar algum papel no desenvolvimento da SMDS. Para tanto, a técnica denominada “amplificação por círculo rolante com múltiplos primers” (ACRMP) foi empregada. A ACRMP é baseada na atividade da DNA polimerase do fago phi29, uma enzima capaz de sintetizar novas moléculas de DNA a partir de um molde de DNA circular. Numa segunda etapa, o DNA amplificado é clivado com enzimas de restrição, ocasionando a linearização de grande quantidade de cópias do DNA alvo original. Como a ACRMP é realizada com primers aleatórios, nenhum conhecimento prévio da seqüência de nucleotídeos alvo é necessário. Portanto, pode-se teoricamente amplificar DNA circular de qualquer microorganismo, o que a torna ideal para o propósito do presente estudo. O DNA extraído de soros de 67 suínos com sinais clínicos de SMDS, assim como de 63 suínos saudáveis, foram submetidos à ACRMP. O principal achado deste estudo foi que o genoma de um (ou mais) anelovírus foi(ram) detectado(s) em 88,9% (56/63) dos suínos saudáveis, ao passo que o(s) mesmo(s) agente(s) somente foi(ram) detectado(s) em 16,4% (11/67) dos soros de suínos com sinais clínicos da SMDS. Alguns fragmentos de DNA potencialmente correspondentes a fragmentos de genomas virais foram seqüenciados, revelando que pelo menos um deles corresponde a uma seqüência de anelovírus suíno ainda não descrita. No entanto, outro genoma correspondente a um anelovírus foi encontrado na mesma amostra, sugerindo que mais de um vírus pode estar presente em amostras de soro. Estes resultados demonstraram que os anelovírus, de grande variabilidade genética, são significativamente mais prevalentes em suínos clinicamente saudáveis do que em suínos com SMDS. / Porcine circovirus type 2 (PCV2) is an ubiquitous virus that has been associated to a number of syndromes in swine. Among these, Postweaning Multisystemic Wasting Syndrome (PMWS) has become a major cause of economic losses in swine worldwide. However, there is uncertainty as to whether PCV2 is in fact the sole agent responsible for the disease, essentially because the disease has not been experimentally reproduced when PCV2 is inoculated onto susceptible animals. In view of that, a number of other infectious (and non infectious) agents have been examined and their potential role in PMWS searched for. This study was carried out to determine whether any other agent(s) with circular DNA genome might be playing some role in PMWS. In order to achieve that, a technique called “randomly primed rolling circle amplification” (RPRCA) was employed. RPRCA is based on the activity of bacteriophage phi29 DNA polymerase, an enzyme that synthesizes new DNA molecules starting from a circularized DNA template. In a second phase, the amplified DNA is cleaved with restriction enzymes, so giving rise to large amounts of linearized copies of the original target DNA. As RPRCA is performed with random priming, no previous knowledge of the target nucleotide sequence is necessary. Therefore, it is theoretically possible to amplify circular DNA of any microorganism, thus making it ideal for the purpose of the present study. DNA extracted from sera of 67 pigs with clinical signs of PMWS as well as from 63 healthy pigs was submitted to RPRCA. The major finding of this study was that the genome of one (or more) anelloviruses was detected in 88,9% (56/63) of the healthy pigs, whereas the same agent was only detected in 16,4% (11/67) of pigs with clinical signs of PMWS. Some of the DNA fragments corresponding to the putative virus genomes were sequenced and revealed at least one non-previously described anellovirus sequence. However, other anellovirus could be found on the same sample, suggesting that more than one genome are present in samples of serum. These results demonstrate that anelovírus, of great genetic variability, were significantly more prevalent in healthy pigs than in pigs with PMWS.

Circovirose suína

Vírus

Porcine circovirus

PCV2

PMWS

Co-infections

TTV

Genetic Stability of a Genetically-Engineered Chimeric Porcine Circovirus (PCV) Vaccine, PCV1-2

Gillespie, Jennifer Ann

04 June 2009

Porcine circovirus type 2 (PCV2) is the primary causative agent of porcine circovirus associated disease (PCVAD), an economically important swine disease that causes wasting in pigs 5-18 weeks of age. There exist two different types of porcine circoviruses: porcine circovirus type 1 (PCV1) was discovered as a contaminant of porcine kidney (PK-15) cells and was determined to be nonpathogenic in swine; whereas porcine circovirus type 2 (PCV2) is pathogenic. A recently released vaccine for PCVAD was generated by inserting the gene encoding the immunogenic capsid protein of PCV2 into the genetic backbone of the non-pathogenic PCV1. This chimeric PCV vaccine, called PCV1-2, was shown to induce protective immunity against PCV2 infection in pigs. The vaccine is currently on the market in a killed form. In order to develop a live version of the vaccine, the genetic stability of the chimeric PCV1-2 vaccine virus was investigated by in vitro and in vivo passaging of the vaccine virus. In vitro passaging of the PCV1-2 vaccine virus was done in a porcine kidney PK-15 cell line. Cells were infected with the PCV1-2 vaccine virus and then serially passaged 11 times. The passaged vaccine viruses recovered from passages 5 and 11 were sequenced, and the sequences were compared to that of the original PCV1-2 vaccine virus. The in vitro serial passage result showed that no mutation occurred during the 11 in vitro passages. The in vivo passaging was done using specific-pathogen-free (SPF) pigs. In in vivo "passage 1", nine piglets were divided into 3 groups of 3 each: group 1 each inoculated with 200ug of PCV1-2 plasmid, group 2 each with 1Ã 103 TCID50 live PCV1-2 vaccine virus, and group 3 each with 3ml phosphate buffered saline (PBS) buffer as a control. One pig from each group was necropsied at 14, 21, and 28 days post-inoculation (DPI), respectively. A panel of tissue samples including lymph nodes and thymus were collected from each pig. Tissue homogenates from DPI 28 that were positive by PCR for PCV1-2 DNA were used to inoculate new piglets in the in vivo passage 2 experiment. Viruses recovered from passage 2 pigs were subsequently used for inoculation in the in vivo passage 3 experiment. The PCV1-2 vaccine virus DNA from pigs in each passage was amplified and sequenced. The results of the in vivo serial passage experiment showed that, after 3 passages of the PCV1-2 vaccine virus in pigs, there were no new mutations in the viruses recovered from pigs. The PCV1-2 vaccine contained an introduced marker mutation at amino acid position number 79, which is in the capsid region. During the in vivo passaging of the vaccine virus in pigs, this marker mutation quickly reverted back to its original nucleotide. This marker back mutation occurred between DPI 21 and DPI 28 of passage 1 in the PCV1-2 live vaccine virus group, and between DPI 28 of passage 1 and DPI 14 of passage 2 in the PCV1-2 vaccine plasmid group, and remained stable throughout the reminder of the in vivo study. Based upon the results from this study, we conclude that the PCV1-2 chimeric vaccine virus is genetically stable in vitro and in pigs, and thus should serve as a good candidate for a live vaccine against PCV2. / Master of Science

vaccine

swine

Porcine Circovirus

PCV2

Effect of vaccination against porcine circovirus type 2 (PCV2) on ejaculate characteristics and the shedding of virus in boar semen

Alberti, Kyle Anthony

24 June 2010

Research has demonstrated that porcine circovirus type 2 (PCV2) can be shed into boar semen, raising the possibility that artificial insemination may be an important route by which disease associated with PCV2 is transmitted. The objective of this experiment was to determine the effect of vaccination against PCV2 on ejaculate characteristics and PCV2-specific antibody titers in serum of PCV2-positive boars viremia and viral shedding in semen. Semen and blood samples were collected weekly from week 0 to week 8. After collections at week 0, boars were vaccinated with a commercial vaccine against PCV2 (n = 5) (Suvaxyn PCV2 One dose; Fort Dodge Animal Health, Fort Dodge, IA) or served as controls and received 2 ml 0.9% saline (n = 5). Sperm concentrations and characteristics of sperm motility were assessed using a computer-assisted sperm analysis system (Hamilton Thorne Research, Beverly, MA) and sperm morphology was evaluated after staining using light microscopy. The PCV2 antibody titers were determined in serum using an ELISA (Iowa State Veterinary Diagnostic Laboratory; Ames, IA). The genomic copy number of PCV2 DNA in serum and semen was determined by PCR (Iowa State Veterinary Diagnostic Laboratory; Ames, IA). There were no effects of treatment or treatment by week on semen characteristics (P > 0.05). An effect of treatment by week was detected for serum antibody titers (P < 0.01). Compared with controls, antibody titers in vaccinated boars tended to be greater at week 0 (1.13 ± 0.05 titer/ml vs 1.01 ± 0.05 titer/ml; P = 0.09) and were greater at week 2 (1.15 ± 0.05 titer/ml vs 1.01 ± 0.05 titer/ml; P < 0.05) but lesser at week 7 (1.01 ± 0.05 titer/ml vs 1.23 ± 0.05 titer/ml; P < 0.01) and tended to be lesser at week 8 (1.05 ± 0.05 titer/ml vs 1.17 ± 0.05 titer/ml; P = 0.07). There were no effects of treatment, week, or treatment by week for serum genomic copy number of PCV2 DNA (P > 0.1). An effect of week was detected for semen genomic copy number of PCV2 DNA (P < 0.04). During week 3, PCV2 genomic copy number was at its greatest numerical value, however, semen PCV2 genomic copy number was at its lowest point. This was followed by an increase in semen PCV2 genomic copy number during week 7. This increase could be related to the increase in viral shedding in the serum. In summary, vaccination against PCV2 can lower antibody titers when given post-infection and has no effect on indicators of semen fertility. Vaccination also can decrease the length of reoccurring infection by decreasing the length of viral shedding in serum. / Master of Science

Antibody

Semen

Vaccine

Porcine circovirus type 2 (PCV2)

In vitro and in vivo virulence evaluation of the new genotype of porcine circovirus type 2 and identification of a new cell line permissive to virus replication

Music, Nedzad

January 2008

Mémoire numérisé par la Division de la gestion de documents et des archives de l'Université de Montréal.

SDPS

PMWS

Cellules NPTr

NPTr cells

Réplication virale

Virus replication

Génotypes de PCV-2

PCV-2 genotypes

Circovirus porcin

Porcine circovirus

In vitro and in vivo virulence evaluation of the new genotype of porcine circovirus type 2 and identification of a new cell line permissive to virus replication

Music, Nedzad

January 2008

Mémoire numérisé par la Division de la gestion de documents et des archives de l'Université de Montréal

SDPS

PMWS

Cellules NPTr

NPTr cells

Réplication virale

Virus replication

Génotypes de PCV-2

PCV-2 genotypes

Circovirus porcin

Porcine circovirus

Circovirus Infection in Cattle / Circovirus-Infektion beim Rind

Halami, Mohammad Yahya

20 November 2014

Circoviren sind kleine, unbehüllte Viren mit einem einzelsträngigen zirkulären DNA Genom mit eine Größe von 1,7 bis 2,4 kb. Das Porcine Circovirus Typ 2 (PCV2), welches zum Genus Circovirus gehört, ist mit einer Anzahl von Krankheitsmanifestationen verbunden worden, die heute als Porcine Circovirus Assoziierte Krankheiten (PCVAD) zusammengefasst sind. Die PCV2-Infektion bei Rindern ist bis zum jetzigen Zeitpunkt marginal erforscht worden. Serologische Untersuchungen auf Circovirus spezifische Antikörperführten zu widersprüchlichen Ergebnissen. Im Jahr 2007 wurde von der Bovinen Neonatalen Panzytopenie (BNP) in Europa mit unklarer Genese berichtet. Das klinisch - pathologische Bild der Hämorrhagien ähnelte dem Krankheitsbild der Infektiösen Anämie, welche durch ein Circovirus bei Hühnern verursacht wird. Deshalb wurde in dieser Studie eine Breitspektrum PCR zum Nachweis von Cirocvirus-Genomen durchgeführt. In 5 von 25 BNP betroffenen Kälbern konnte circovirale DNA nachgewiesen werden. Das komplette Genom wurde nachfolgend amplifiziert, kloniert und sequenziert. Das nachgewiesene Genom (PCV2-Ha08) hat eine Länge von 1768 Nukleotiden und zeigte eine hohe Homologie (bis zu 99%) mit PCV2-Genotyp b (siehe Publikation 1). Als Ursache der BNP ist vor kurzen die Übertragung von Alloantikörpern über das Kolostrum beschrieben wurden, welche die Zerstörungen von Leukozyten und Thrombozyten sowie deren Vorläuferzellen bewirken. Ungeachtet dessen war es wichtig, die Empfänglichkeit und Immunantwort von Kälbern nach experimenteller Infektion mit PCV2 zu studieren. Für diesen Zweck wurden weitere 181 Proben von BNP-Kälbern aus Deutschland mit Hilfe einer Breitspektrum-PCR getestet. In zwei von 181 Proben wurde PCV2 DNA nachgewiesen. Die vollständigen Sequenzen konnten amplifiziert werden. Während das erste Genom aus einer Blutprobe eines Kalbs in Bayern stammte (PCV2-Ha09), stammte das zweite nachgewiesene Genom aus Lunge und Gehirn von einem Kalb in Sachsen (PCV2-Ha10). Das Genom (PCV2-Ha09) besteht aus 1768 nt, währenddessen das Genom (PCV2-Ha10) aus 1767 nt aufgebaut ist (siehe Publikation 2). Weiterhin wurden die PCV2 Empfänglichkeit und die Immunantwort von Kälbern durch experimentellen PCV2 Inokulation sowie die Möglichkeit, eine Serokonversion nach Impfung mit einer kommerziellen PCV2 Vakzin zu entwickeln, untersucht. PCV2-spezifische Antikörper wurden in den PCV2-infizierten Tieren und in den PCV2-immunisierten Tieren im Tag 11 und 7 nach Inokulation (p.i.) nachgewiesen. PCV2-Genome wurden durch quantitative Realtime-PCR zwischen Tag 4 und Tag 46 p.i. nur in den Blutproben sowie in verschiedenen Geweben (z.B. Milz, Lymphknoten, Thymus) der PCV2-infizierten Tiere nachgewiesen. Das Genom, welches von den Lymphknoten der PCV2-infizierten Kälber erneut isoliert wurde, zeigt eine Identität von 99,9% gegenüber dem Inokulum. Dies weist möglicherweise auf adaptierte Mutationen im PCV2 Genom hin. Die Mutationen C1708T und G365C sind während der Infektionen aufgetreten. Die Sequenzanalyse zeigt eine mögliche adaptierte Mutation an der Aminosäure Nr. 105 in Replikationsgen (Met zu Ile) (siehe Publikation 3). Zusammenfassend kann geschlussfolgert werden, dass der Nachweis der PCV2 Genomen und eine experimentell induzierte Serokonversion möglich war. Es konnte gezeigt werden, dass die Empfänglichkeit von PCV2 nicht allein auf Schweine begrenzt ist und eine Übertragung von PCV2 auf Rinder möglich ist.

Porcine Circovirus Type 2

Bovine Neonatale Panzytopenie

Serokonversion

qPCR

porcine circovirus type 2

Bovine neonatal pancytopenia

serconversion

qPCR

ddc:636.089

Investigação do potencial de roedores peridomésticos como reservatório do porcine circovirus 2 (PCV2) / Investigação do potencial de roedores peridomésticos como reservatório do porcine circovirus 2 (PCV2) / Investigation of the potencial of peridomestic rodents as reservoir of the Porcine circovirus 2 (PCV2) / Investigation of the potencial of peridomestic rodents as reservoir of the Porcine circovirus 2 (PCV2)

Pinheiro, Albanno Leonard Braz Campos

22 November 2011

Made available in DSpace on 2015-03-26T13:47:03Z (GMT). No. of bitstreams: 1 texto completo.pdf: 914989 bytes, checksum: 6324bfc7a5398520ac5042a3539b706e (MD5) Previous issue date: 2011-11-22 / Porcine circovirus-2 (PCV2) has been related as the causative agent of the Postweaning Multissystemic Wasting Syndrome (PMWS) and other diseases called porcine circovirus associated diseases (PCVAD). They are responsible for economic losses in pork production worldwide. There is only a few scientific studies describing the infection in other species but swine and their hole at the epidemiologic dynamics of the diseases related to the PCV2. The aim of this study is to investigate the occurrence of infection by the PCV2 in wild mice (Mus musculus and Rattus rattus) captured in hog farms. The capture of the 40 sorted mice was made at 5 pig wean tofinish farms in Minas Gerais, an important state of pork production in Brazil. Samples of tissues (lymph nodes, spleen, kidney, heart and lungs) and blood were collected from the mice. The tissue fragments collected were submitted to immunohistochemistry and Nested PCR. Additionally, samples from spleen and lungs were analyzed by histology assays. Presence of antibodies anti-PCV2 was tested by ELISA assays. Immunohistochemical analysis showed positive prints in 12 animals, mostly on spleen (sub scapular area), lungs (alveolar macrophages) and kidney (inside the tubules). The 12 serum analyzed by ELISA hasn t detected antibodies anti-PCV2. Histopathological analyses revealed in some samples, a multifocal and lympho-neutrophilic interstitial bronchopneumonia, with some node formations. Moreover, spleen samples showed a mild to moderate lymphocyte depletion related to the PCVAD. The Nested PCR assays showed the presence of viral DNA at different tissues from 6 tested rodents. Thus, the results found in this work, indicate that mice from the species Mus musculus and Rattus rattus can be naturally infected by the PCV2 and they would play a hole in the epidemiology of PCVAD. However, more studies are necessary to confirm the transmission of the PCV2 from wild rodents to pigs. / O porcine circovirus-2 (PCV2) é atribuído como um dos agentes relacionados a doenças associadas ao circovírus (PCVAD), ocasionando perdas econômicas significativas na produção mundial de suínos. Poucos trabalhos são realizados a respeito da infecção em outras espécies pelo PCV2 e sua participação na epidemiologia das doenças associadas ao vírus. O propósito desse estudo foi investigar a ocorrência de infecção em roedores peridomésticos das espécies Mus musculus e Rattus rattus pelo PCV2 em granjas comerciais de suínos. Animais dessas espécies foram capturados em importantes centros de produção no estado de Minas Gerais. Amostras de órgãos (linfonodos, baço, rins, fígado, pulmão) e sangue foram coletadas. Os fragmentos de tecidos coletados foram submetidos ao teste de imunohistoquímica e Nested PCR. Adicionalmente, foram realizadas avaliações histológicas em amostras de baço, rim e pulmão. Presença de anticorpos anti-PCV2 foram avaliados pela técnica de ELISA. O teste de imunohistoquímica demonstrou marcações encontradas em 12 animais, principalmente no baço (região subcapsular), no pulmão (macrófagos alveolares) e nos rins (interior dos túbulos). A análise do soro pela técnica de ELISA não detectou anticorpos contra o PCV-2 nas 12 amostras avaliadas.. A histopatologia demonstrou em algumas amostras, uma pneumonia bronco-intersticial neutrofílica e linfocítica, multifocal e moderada, com formação de nódulos linfóides associados a vasos e bronquíolos. No ensaio de nested-PCR foi detectado DNA viral em diferentes tecidos avaliados de seis animais. Os resultados citados demonstram que os roedores domésticos das espécies estudadas podem exercer importante papel na epidemiologia das doenças relacionadas ao PCV2. No entanto, mais estudos são necessários para comprovar a transmissão do PCV2 dos roedores para os suínos.

Porcine circovirus 2

Epidemiologia

Roedores

Porcine circovirus 2

Epidemiology

Rodents

Uso do plasma spray dried na dieta de suínos para prevenção da circovirose suína e doenças associadas / The use of plasma spray dried in the prevention of porcine circovirus and associated diseases

Rangel, Luís Fernando Sarmento

02 March 2009

O trabalho foi realizado em granja com histórico de ocorrência de Circovirose Suína e Doenças Associadas - PCVAD maior que 5%. Foram utilizados 560 leitões na fase de creche (25 - 66 dias de idade) e 468 no início de crescimento (66 - 94 dias de idade), em experimento delineado em blocos ao acaso, com dois tratamentos e 9 repetições por tratamento na creche e 18 repetições no crescimento. Os tratamentos: Plasma - os leitões foram alimentados com rações contendo plasma (AP 920®) conforme segue: 6,0% na ração pré-inicial I (15 dias); 3,0% na ração pré-inicial II (13 dias); 1,5% de na ração inicial (14 dias); e 1,0% na ração de crescimento I (14 dias), seguindo-se por mais 14 dias com a mesma ração sem plasma. Controle: os leitões foram alimentados com as mesmas rações, porém sem plasma. As rações utilizadas foram formuladas para satisfazer as necessidades nutricionais dos leitões. As variáveis avaliadas: ganho de peso, consumo de ração, conversão alimentar, ocorrência da PCVAD, taxa de mortalidade pela PCVAD e anticorpos anti-PCV2. Houve diferença significativa (P<0,05) no peso dos leitões e no ganho de peso diário em todas as medidas realizadas na fase de creche. A diferença de peso no final da creche foi de 1,92 kg/leitão a mais para o Plasma. Não houve diferença estatística (P>0,05) no coeficiente de variação do peso dos leitões em todas as medidas realizadas. O consumo médio de ração com plasma foi superior (P<0,05) em todas as fases de creche. A conversão alimentar foi melhor (P=0,087) no Plasma. As idades calculadas dos leitões, para o peso ideal para venda (22 e 24 kg), indicaram que os leitões do Plasma atingiriam tais pesos 2,3 e 2,2 dias antes que os controles, respectivamente. Na fase inicial de crescimento, houve diferença significativa (P<0,05) no consumo de ração e no peso final (94 dias de idade) com uma diferença final de 2,28 kg/suíno a mais no grupo Plasma. Isso tem conseqüências importantes no manejo das granjas, permitindo um período maior de vazio sanitário. Aos 39, 52 e 66 dias de idade, houve menor freqüência (P<0,05) de leitões com sinais da PCVAD no Plasma. Verificou-se que a infecção pelo PCV2 estava disseminada nos leitões de ambos os tratamentos. Houve efeito de bloco e idade no título de anticorpos para o PCV2. No período total, o aumento nesse título foi parcial (P=0,0856) para o Plasma. Porém, aos 52 dias de idade, os leitões alimentados com plasma apresentaram aumento nesse título (P<0,05). Isso sugere que os leitões que receberam plasma apresentavam melhor capacidade de resposta imunológica ao PCV2. Os leitões tratados com plasma apresentaram: melhor ganho de peso na creche, que foi ampliado no início do crescimento, reduzindo em 2,3 dias a idade para atingir 22,0 kg; melhor capacidade de resposta imunológica ao PCV2 aos 52 dias de idade e menor manifestação de PCVAD. O aumento no ganho de peso nos leitões foi atribuído ao aumento no consumo de ração e à menor ocorrência de leitões com sinais de PCVAD. / The work was conducted in a farm with historical data, recording pigs with clinical Porcine Circovirus and Associated Diseases - PCVAD higher than 5%. In the nursery 560 pigs (25-66 days of age) and early in growing phase 468 piglets (66-94 days of age) were used in random blocks design with two treatments and 9 replicates in the nursery and 18 replicates in growing phase per treatment. Treatments: Plasma - pigs were fed plasma (AP 920®) containing diets as follows: 6% in the pre-starter I (15 days); 3% in the pre-starter II (13 days); 1.5% in the starter phase (14 days); and 1% in the growing phase (14 days), followed by 14 days with the same feed without plasma. Control: pigs were fed with the same feeds from the Plasma treatment but without plasma. Both feeds were formulated to meet the nutritional requirements of the pigs in different stages. Evaluated variables: weight gain, feed intake, feed conversion, clinical presence of PCVAD, mortality rate related with PCVAD and antibodies against PCV2. There was a significant difference (P<0.05) in the pigs weight and in the weight gain the nursery. The weight difference at the end of the nursery phase was 1.92 kg/pig grater to the plasma group. There was no statistical difference (P>0.05) in the coefficient of variation of weight in all measurements performed. The average feed intake was higher (P<0.05) on Plasma in all nursery phases. A better feed conversion was observed on Plasma (P=0.087). The calculated age of pigs to reach the ideal sale weight (22-24 kg) indicated that Plasma achieved those weights 2.3-2.2 days prior than the Control respectively. In the growing phase there was a significant difference (P<0.05) in the feed intake and final weight (94 days of age) with a final weight 2.28 kg/pig heavier for Plasma. This has important consequences in the management of a farm, allowing a longer downtime period between groups. At 39, 52 and 66 days of age, there was less frequency (P<0.05) of pigs with sings of PCVAD in the plasma fed group. It was observed that the infection by PCV2 was widely spread in both treatments pigs. There was block and age effect in the PCV2 antibody titers. There was a partial treatment effect (P=0.0856) over the PCV2 antibodies when the data was evaluated at different sampling ages. However, at 52 days of age, there was an increase in the PCV2 antibody titers (P<0.05) of pigs that received plasma. This observation suggests that plasma fed pigs had a better immune response to PCV2. The plasma fed pigs showed better weight gain in the nursery. That effect was amplified in the beginning of the growing phase, leading to a reduction in 2.3 days the age to reach 22.0 kg of body weight, better immune response to PCV2 at 52 days of age and less presence of sings of PCVAD. The increase in the weight gain was due to an increase in feed intake and lower incidence of pigs with sings of PCVAD.

Animal Diet

Circovirus Prevenção e controle

Circovirus Prevention and Control

Dieta animal

Feed

Leitões - Desempenho

Patologia veterinária

Piglets Performance

Plasma

Plasma

Rações

Suínos.

Swine I.

Veterinary Pathology

Avaliação da co-infecção do circovirus suíno 2 com Mycoplasma hyopneumoniae em amostras de pulmões coletadas em abatedouro / Evaluation of co-infection of porcine circovirus 2 with Mycoplasma hyopneumoniae in lung samples collected from slaughterhouse

Bezerril, Juliana Evangelista

27 February 2009

Made available in DSpace on 2015-03-26T13:46:46Z (GMT). No. of bitstreams: 1 texto completo.pdf: 618598 bytes, checksum: 78e08690fd4db366e1e37fe332d558bc (MD5) Previous issue date: 2009-02-27 / The porcine circovirus, caused by the porcine circuvirus type 2 (PCV 2), and the porcine enzootic pneumonia, caused by the Mycoplasma hyopneumoniae, are infectious contagious diseases of great importance for worldwide swine production, both causes pneumonias with different presentation patterns. They have cosmopolite distribution and are among the major causes in economic losses. This work was made aiming the evaluation of the co-infection between porcine circovirus 2 (PCV2) and Mycoplasma hyopneumoniae using real time polymerase chain reaction (qPCR), immunohistochemistry and histopathological analyses. 120 lungs fragments, 45 being from fragments with macroscopic lesions (CLM) and 75 being from fragments without macroscopic lesions (SLM) were analyzed by histopathology procedures. Among these, 32 samples were randomly selected (being 16 without macroscopic lesions and 16 with macroscopic lesions) for the immunohistochemistry analyses (for Mycoplasma hyopneumoniae detection) and qPCR (for PCV 2 detection). No significant difference was observed between the groups (SLM and CLM) on the tests, indicating that the absence of macroscopic lesions doesn t reject the possible presence of agents neither the presence of microscopic lesions. The histopatological technique showed itself as an important tool for diagnosis approach. Although the lesion are not patognomonic for the agents in the analyses, they are quite suggestive about the viral and bacterium scene, and these findings, together with the presence of clinical signs and agent detection (more frequently made by qPCR and immunohistochemistry), confirm the diagnosis of each agent isolated or co-infection. Although the samples analyzed by RT-PCR had shown higher number of negative results and low viral quantity, many authors related that lungs are among the organs with the lowest viral quantities of PCV2, being, for that reason, the liver linfonodes, the main target of the PCV2, more indicated for viral quantification. It was verified a positive correlation between the immunohistochemistry analysis and the histopathology analysis using the Pearson statistical test, which confirms the presence of the agent in the histopathology observations. Forward studies using linfonodes samples (target of the PCV2) and samples collected from different lung anatomic regions must be realized for evaluation of a co-infection for more accurate results. / A circovirose suína, causada pelo circovirus suíno tipo 2 (PCV2), e a pneumonia enzoótica suína, causada pelo Mycoplasma hyopneumoniae, são doenças infecto-contagiosas de grande importância na suinocultura mundial, ambas causam pneumonias com diferentes formas de apresentação. Têm distribuição cosmopolita e estão entre as principais causas de perdas econômicas. O presente trabalho foi realizado com o objeto de avaliar a coinfecção entre Circovírus suíno 2 e o Mycoplasma hyopneumoniae, por meio da reação da polimerase em cadeia em tempo real (qPCR), técnica de imunoistoquímica e exames histopatológicos. Cento e vinte fragmentos de pulmões, sendo 45 com lesões macroscópicas (CLM) e 75 sem lesões macroscópicas (SLM) foram analisados pela histopatologia. Destes, foram selecionadas aleatoriamente 32 amostras (sendo 16 sem lesões macroscópicas e 16 com lesões macroscópicas) para a realização dos testes de imunoistoquímica (para a detecção do Mycoplasma hyopneumoniae) e qPCR (para detecção do PCV2). Não foi observada diferença significativa entre os grupos (SLM e CLM) em nenhum dos testes, o que indica que a ausência de lesões macroscópicas não descarta a possibilidade da presença dos agentes nem de lesões microscópicas. A técnica de histopatologia representou uma importante ferramenta para se aproximar ao diagnóstico. Embora as lesões não sejam patognomônicas para os agentes avaliados, elas são bastante sugestivas dos quadros viral e bacteriano, e esses achados, aliados a presença de sinais clínicos e detecção do agente (que são mais frequentemente realizados por qPCR e imunoistoquímica), confirmam o diagnóstico de cada agente isoladamente ou da coinfecção. Apesar das amostras analisadas pelo qPCR terem apresentado grande número de resultados negativos e baixa carga viral, diversos autores relatam que o pulmão é um dos órgãos com menor carga viral de PCV2, sendo desta forma os órgãos linfóides, principais alvos do PCV2, mais indicados para a quantificação viral. Foi verificada uma correlação positiva do teste de imunoistoquímica com o teste histopatológico de acordo com o teste estatístico de Pearson, o que confirma a presença do agente nas lesões observadas na histopatologia. Estudos futuros utilizando a coleta de linfonodos (órgão alvo do PCV2) e amostras coletadas de diferentes regiões anatômicas pulmonares devem ser realizados para avaliar a co-infecção de uma forma mais acurada.

Circovirus suíno 2

Mycoplasma hyopneumoniae

Co-infecção

Porcine circovirus 2

Mycoplasma hyopneumoniae

Co-infection