Molecular epidemiological tracing of a cattle rabies outbreak lasting less than a month in Rio Grande do Sul in southern Brazil.

BACKGROUND: Vampire bat-transmitted cattle rabies cases are typically encountered in areas where the disease is endemic. However, over the period of a month in 2009, an outbreak of cattle rabies occurred and then ended spontaneously in a small area of the Rio Grande do Sul State in southern Brazil. To investigate the epidemiological characteristics of this rabies outbreak in Rio Grande do Sul, 26 nucleotide sequences of rabies virus (RABV) genomes that were collected in this area were analyzed phylogenetically. RESULTS: Nucleotide sequence identities of the nucleoprotein gene and G-L intergenic region of the 26 RABVs were greater than 99.6 %. Phylogenetic analysis showed that all RABVs clustered with the vampire bat-related cattle RABV strains and that the RABVs were mainly distributed in southern Brazil. CONCLUSIONS: The findings of the present study suggested that a small population of rabid vampire bats carrying a single RABV strain produced a spatiotemporally restricted outbreak of cattle rabies in southern Brazil.

Isolation of a phylogenetically distinct rabies virus from a tufted capuchin monkey (Cebus apella) in Brazil.

A rabies virus isolate (BRmk1358 strain) was discovered from a rabid tufted capuchin monkey in Brazil. The present study determined the nucleotide sequence of the BRmk1358 strain and compared with the rabies viruses isolated from marmosets and other animals in the Americas. Phylogenetic analyses showed that the BRmk1358 strain formed a lineage distant from that of marmoset rabies virus within the Chiroptera-related rabies virus cluster. This result suggests that the source of rabies infection in the tufted capuchin monkey may have been bat, and that they have a risk to act as rabies reservoir in Brazil.

Molecular epidemiology of livestock rabies viruses isolated in the northeastern Brazilian states of Paraíba and Pernambuco from 2003 - 2009.

BACKGROUND: Limited or no epidemiological information has been reported for rabies viruses (RABVs) isolated from livestock in the northeastern Brazilian states of Paraíba (PB) and Pernambuco (PE). The aim of this study was to clarify the molecular epidemiology of RABVs circulating in livestock, especially cattle, in these areas between 2003 and 2009. FINDINGS: Phylogenetic analysis based on 890 nt of the nucleoprotein (N) gene revealed that the 52 livestock-derived RABV isolates characterized here belonged to a single lineage. These isolates clustered with a vampire bat-related RABV lineage previously identified in other states in Brazil; within PB and PE, this lineage was divided between the previously characterized main lineage and a novel sub-lineage. CONCLUSIONS: The occurrences of livestock rabies in PB and PE originated from vampire bat RABVs, and the causative RABV lineage has been circulating in this area of northeastern Brazil for at least 7 years. This distribution pattern may correlate to that of a vampire bat population isolated by geographic barriers.

Determination and molecular analysis of the complete genome sequence of two wild-type rabies viruses isolated from a haematophagous bat and a frugivorous bat in Brazil.

The complete genome sequences of two Brazilian wild-type rabies viruses (RABV), a BR-DR1 isolate from a haematophagous bat (Desmodus rotundus) and a BR-AL1 isolate from a frugivorous bat (Artibeus lituratus), were determined. The genomes of the BR-DR1 and BR-AL1 had 11,923 and 11,922 nt, respectively, and both encoded the five standard genes of rhabdoviruses. The complete nucleotide sequence identity between the BR-DR1 and BR-AL1 isolates was 97%. The BR-DR1 and BR-AL1 isolates had some conserved functional sites revealed by the fixed isolates, whereas both isolates had unique amino acid substitutions in the antigenic region IV of the nucleocapsid gene. Therefore, it is speculated that both isolates were nearly identical in virologic character. According to our phylogenetic analysis based on the complete genomes, both isolates belonged to genotype 1, and to the previously defined "vampire bat-related RABV lineage" which consisted of mainly D. rotundus- and A. lituratus-isolates; however, a branch pattern with high bootstrap values suggested that BR-DR1 was more closely related to the 9001FRA isolate, which was collected from a dog bitten by a bat in French Guiana, than to BR-AL1. This result suggests that the vampire bat-related RABV lineage includes Brazilian vampire bat and Brazilian frugivorous bat RABV and is further divided into Brazilian vampire bat and Brazilian frugivorous bat RABV sub-lineages. The phylogenetic analysis based on the complete genomes was valuable in discriminating among very closely related isolates.

Evolutionary history of dog rabies in Brazil.

Although dogs are considered to be the principal transmitter of rabies in Brazil, dog rabies had never been recorded in South America before European colonization. In order to investigate the evolutionary history of dog rabies virus (RABV) in Brazil, we performed a phylogenetic analysis of carnivore RABV isolates from around the world and estimated the divergence times for dog RABV in Brazil. Our estimate for the time of introduction of dog RABV into Brazil was the late-19th to early-20th century, which was later than the colonization period but corresponded to a period of increased immigration from Europe to Brazil. In addition, dog RABVs appeared to have spread to indigenous animals in Brazil during the latter half of the 20th century, when the development and urbanization of Brazil occurred. These results suggest that the movement of rabid dogs, along with human activities since the 19th century, promoted the introduction and expansion of dog RABV in Brazil.

Epidemiology of vampire bat-transmitted rabies virus in Goiás, central Brazil: re-evaluation based on G-L intergenic region.

BACKGROUND: Vampire bat related rabies harms both livestock industry and public health sector in central Brazil. The geographical distributions of vampire bat-transmitted rabies virus variants are delimited by mountain chains. These findings were elucidated by analyzing a high conserved nucleoprotein gene. This study aims to elucidate the detailed epidemiological characters of vampire bat-transmitted rabies virus by phylogenetic methods based on 619-nt sequence including unconserved G-L intergenic region. FINDINGS: The vampire bat-transmitted rabies virus isolates divided into 8 phylogenetic lineages in the previous nucleoprotein gene analysis were divided into 10 phylogenetic lineages with significant bootstrap values. The distributions of most variants were reconfirmed to be delimited by mountain chains. Furthermore, variants in undulating areas have narrow distributions and are apparently separated by mountain ridges. CONCLUSIONS: This study demonstrates that the 619-nt sequence including G-L intergenic region is more useful for a state-level phylogenetic analysis of rabies virus than the partial nucleoprotein gene, and simultaneously that the distribution of vampire bat-transmitted RABV variants tends to be separated not only by mountain chains but also by mountain ridges, thus suggesting that the diversity of vampire bat-transmitted RABV variants was delimited by geographical undulations.

Pathogenicity of different rabies virus isolates and protection test in vaccinated mice.

This study was aimed to evaluate and compare the pathogenicity of rabies virus isolated from bats and dogs, and to verify the efficacy of a commercial rabies vaccine against these isolates. For evaluation of pathogenicity, mice were inoculated by the intramuscular route (IM) with 500MICLD50/0.03 mL of the viruses. The cross-protection test was performed by vaccinating groups of mice by the subcutaneous route and challenged through the intracerebral (IC) route. Isolates were fully pathogenic when inoculated by the IC route. When inoculated intramuscularly, the pathogenicity observed showed different death rates: 60.0% for the Desmodus rotundus isolate; 50.0% for dog and Nyctinomops laticaudatus isolates; 40.0% for Artibeus lituratus isolate; 9.5% Molossus molossus isolate; and 5.2% for the Eptesicus furinalis isolate. Mice receiving two doses of the vaccine and challenged by the IC route with the isolates were fully protected. Mice receiving only one dose of vaccine were partially protected against the dog isolate. The isolates from bats were pathogenic by the IC route in mice. However, when inoculated through the intramuscular route, the same isolates were found with different degrees of pathogenicity. The results of this work suggest that a commercial vaccine protects mice from infection with bat rabies virus isolates, in addition to a canine rabies virus isolate.

Pathogenicity of different rabies virus isolates and protection test in vaccinated mice / Patogenicidade de diferentes isolados do vírus da raiva e teste de proteção em camundongos vacinados

This study was aimed to evaluate and compare the pathogenicity of rabies virus isolated from bats and dogs, and to verify the efficacy of a commercial rabies vaccine against these isolates. For evaluation of pathogenicity, mice were inoculated by the intramuscular route (IM) with 500MICLD50/0.03mL of the viruses. The cross-protection test was performed by vaccinating groups of mice by the subcutaneous route and challenged through the intracerebral (IC) route. Isolates were fully pathogenic when inoculated by the IC route. When inoculated intramuscularly, the pathogenicity observed showed different death rates: 60.0 percent for the Desmodus rotundus isolate; 50.0 percent for dog and Nyctinomops laticaudatus isolates; 40.0 percent for Artibeus lituratus isolate; 9.5 percent Molossus molossus isolate; and 5.2 percent for the Eptesicus furinalis isolate. Mice receiving two doses of the vaccine and challenged by the IC route with the isolates were fully protected. Mice receiving only one dose of vaccine were partially protected against the dog isolate. The isolates from bats were pathogenic by the IC route in mice. However, when inoculated through the intramuscular route, the same isolates were found with different degrees of pathogenicity. The results of this work suggest that a commercial vaccine protects mice from infection with bat rabies virus isolates, in addition to a canine rabies virus isolate.

O estudo avaliou e comparou as propriedades patogênicas de cinco isolados do vírus da raiva de morcegos e um isolado do vírus da raiva de cão e analisou a eficácia de vacina comercial contra estes isolados, em camundongos. Para o estudo de patogenicidade camundongos foram inoculados pela via IM com 0,1 mL contendo 500MICLD50/0,03mL das amostras de vírus. Quando inoculados pela via IC, os isolados do vírus da raiva provocaram a morte de 100 por cento dos camundongos. No entanto, 500MICLD50/0,03mL das mesmas amostras, inoculadas pela via IM, ocasionaram mortalidade de: 60,0 por cento quando a amostra era de Desmodus rotundus; 50,0 por cento de cão e de Nyctinomops laticaudatus; 40,0 por cento de Artibeus lituratus; 9,5 por cento de Molossus molossus; e 5,2 por cento de Eptesicus furinalis. Camundongos que receberam duas doses de vacina foram protegidos quando desafiados pela via IC, com todas as amostras testadas. Quando os camundongos receberam uma dose da mesma vacina, houve proteção parcial daqueles desafiados com a amostra de cão. Todos os isolados do vírus da raiva testados foram patogênicos para camundongos, inoculados pela IC. No entanto, pela via IM, os mesmos isolados mostraram diferentes graus de patogenicidade. Concluiu-se também que a vacina comercial contra raiva protegeu os camundongos desafiados com amostras de vírus isolados de morcegos e de cão.

A method for simultaneous detection and identification of Brazilian dog- and vampire bat-related rabies virus by reverse transcription loop-mediated isothermal amplification assay.

At present, the sporadic occurrence of human rabies in Brazil can be attributed primarily to dog- and vampire bat-related rabies viruses. Reverse transcription loop-mediated isothermal amplification (RT-LAMP) was employed as a simultaneous detection method for both rabies field variants within 60 min. Vampire bat-related rabies viruses could be distinguished from dog variants by digesting amplicons of the RT-LAMP reaction using the restriction enzyme AlwI. Amplification and digestion could both be completed within 120 min after RNA extraction. In addition, the RT-LAMP assay also detected rabies virus in isolates from Brazilian frugivorous bats and Ugandan dog, bovine and goat samples. In contrast, there were false negative results from several Brazilian insectivorous bats and all of Chinese dog, pig, and bovine samples using the RT-LAMP assay. This study showed that the RT-LAMP assay is effective for the rapid detection of rabies virus isolates from the primary reservoir in Brazil. Further improvements are necessary so that the RT-LAMP assay can be employed for the universal detection of genetic variants of rabies virus in the field.

Low genetic diversities of rabies virus populations within different hosts in Brazil.

The low rates of nonsynonymous evolution observed in natural rabies virus (RABV) isolates are suggested to have arisen in association with the structural and functional constraints operating on the virus protein and the infection strategies employed by RABV within infected hosts to avoid strong selection by the immune response. In order to investigate the relationship between the genetic characteristics of RABV populations within hosts and the virus evolution, the present study examined the genetic heterogeneities of RABV populations within naturally infected dogs and foxes in Brazil, as well as those of bat RABV populations that were passaged once in suckling mice. Sequence analyses of complete RABV glycoprotein (G) genes showed that RABV populations within infected hosts were genetically highly homogeneous whether they were infected naturally or experimentally (nucleotide diversities of 0-0.95x10(-3)). In addition, amino acid mutations were randomly distributed over the entire region of the G protein, and the nonsynonymous/synonymous rate ratios (d(N)/d(S)) for the G protein gene were less than 1. These findings suggest that the low genetic diversities of RABV populations within hosts reflect the stabilizing selection operating on the virus, the infection strategies of the virus, and eventually, the evolutionary patterns of the virus.

Estudo imunológico e genético de 10 isolados do vírus da raiva de morcegos do Rio de Janeiro, Sudeste do Brasil / Immunological and genetic study of 10 bat rabies virus isolates from Rio de Janeiro State, Southeast

O presente trabalho visou estudar 10 isolados de vírus da raiva de morcegos hematófagos e não-hematófagos do Estado do Rio de Janeiro em suas características genéticas quanto aos genes N e G, além da resposta de camundongos vacinados com a vacina anti-rábica produzida pela replicação da amostra Pitman-Moore em cultivo celular, frente ao desafio com estes isolados virais, utilizando-se um ensaio imunológico baseado no teste de potência NIH. A vacina anti-rábica utilizada na imunização dos camundongos ofereceu proteção em mais de 80% dos camundongos vacinados com a diluição 1:5 da vacina, frente à maioria dos isolados. A análise filogenética do gene da proteína N apresentou um padrão de agregação dividido em variante de morcego hematófago e variante de morcego insetívoro, com todos os isolados de morcegos frugívoros Artibeus sp. tendo sido segregados com a variante característica de morcegos Desmodus rotundus. Foram observadas diferenças filogenéticas entre as variantes do vírus da raiva de morcego hematófago isoladas na Região Noroeste do Estado do Rio de Janeiro e aquelas isoladas nas Regiões Metropolitana e Sul do Estado. A substituição do resíduo ácido aspártico por ácido glutâmico na posição 118, encontradas na caracterização genética da proteína G dos isolados 704/97BR-DR e 151/98BR-DR, permite inferir que esta posição esteja relacionada à antigenicidade viral. Não foram observadas diferenças genéticas temporais entre os isolados estudados. A vacina anti-rabica utilizada ofereceu proteção satisfatória contra a maioria dos isolados estudados. (AU)

In the present study we analyzed 10 bats rabies viruses isolated from Rio de Janeiro State, focusing on its genetic characteristics from genes N and G, and also in the response of mice vaccinated with cell-culture rabies vaccine, produced with the Pitman-Moore strain, after viral challenge with bat rabies isolates, using an immunologic essay based on NIH vaccine potency test. The vaccine used conferred protection in more than 80% of the mice vaccinated with 1:15 vaccine dilution, after viral challenge. N gene genetic analysis divided the rabies virus isolates into haematophagous and insectivorous bat variants, with all isolates from Artibeus sp. frugivorous bats being clustered with the variant characteristic of the Desmodus rotundus vampire bat. Phylogenetic differences between isolates from Northeast Region and those from the Metropolitan and South Regions of Rio de Janeiro State were observed. The substitution of an aspartic acid to a glutamic acid found in the position 118 of G gene genetic characterization from samples 704/97BR-DR and 151/98BR-DR seems to be related to viral antigenicity. There were no time-related genetic differences between the studied samples. The vaccine employed was found with satisfactory protection against the majority of the isolates used.(AU)

Estudo imunológico e genético de 10 isolados do vírus da raiva de morcegos do Rio de Janeiro, Sudeste do Brasil / Immunological and genetic study of 10 bat rabies virus isolates from Rio de Janeiro State, Southeast

O presente trabalho visou estudar 10 isolados de vírus da raiva de morcegos hematófagos e não-hematófagos do Estado do Rio de Janeiro em suas características genéticas quanto aos genes N e G, além da resposta de camundongos vacinados com a vacina anti-rábica produzida pela replicação da amostra Pitman-Moore em cultivo celular, frente ao desafio com estes isolados virais, utilizando-se um ensaio imunológico baseado no teste de potência NIH. A vacina anti-rábica utilizada na imunização dos camundongos ofereceu proteção em mais de 80% dos camundongos vacinados com a diluição 1:5 da vacina, frente à maioria dos isolados. A análise filogenética do gene da proteína N apresentou um padrão de agregação dividido em variante de morcego hematófago e variante de morcego insetívoro, com todos os isolados de morcegos frugívoros Artibeus sp. tendo sido segregados com a variante característica de morcegos Desmodus rotundus. Foram observadas diferenças filogenéticas entre as variantes do vírus da raiva de morcego hematófago isoladas na Região Noroeste do Estado do Rio de Janeiro e aquelas isoladas nas Regiões Metropolitana e Sul do Estado. A substituição do resíduo ácido aspártico por ácido glutâmico na posição 118, encontradas na caracterização genética da proteína G dos isolados 704/97BR-DR e 151/98BR-DR, permite inferir que esta posição esteja relacionada à antigenicidade viral. Não foram observadas diferenças genéticas temporais entre os isolados estudados. A vacina anti-rábica utilizada ofereceu proteção satisfatória contra a maioria dos isolados estudados.

In the present study we analyzed 10 bats rabies viruses isolated from Rio de Janeiro State, focusing on its genetic characteristics from genes N and G, and also in the response of mice vaccinated with cell-culture rabies vaccine, produced with the Pitman-Moore strain, after viral challenge with bat rabies isolates, using an immunologic essay based on NIH vaccine potency test. The vaccine used conferred protection in more than 80% of the mice vaccinated with 1:15 vaccine dilution, after viral challenge. N gene genetic analysis divided the rabies virus isolates into haematophagous and insectivorous bat variants, with all isolates from Artibeus sp. frugivorous bats being clustered with the variant characteristic of the Desmodus rotundus vampire bat. Phylogenetic differences between isolates from Northeast Region and those from the Metropolitan and South Regions of Rio de Janeiro State were observed. The substitution of an aspartic acid to a glutamic acid found in the position 118 of G gene genetic characterization from samples 704/97BR-DR and 151/98BR-DR seems to be related to viral antigenicity. There were no time-related genetic differences between the studied samples. The vaccine employed was found with satisfactory protection against the majority of the isolates used.

Complete genome analysis of a rabies virus isolate from Brazilian wild fox.

The complete genome sequence of wild-type rabies virus (RABV) isolated from a wild Brazilian hoary fox (Dusicyon sp.), the BR-Pfx1 isolate, was determined and compared with fixed RABV strains. The genome structure and organization of the BR-Pfx1 isolate were composed of 11,924 nt and included the five standard genes of rhabdoviruses. Sequences of mRNA start and stop signals for transcription were highly conserved among all structural protein genes of the BR-Pfx1 isolate. All amino acid residues in the glycoprotein (G) gene associated with pathogenicity were retained in the BR-Pfx1 isolate, while unique amino acid substitutions were found in antigenic region I of the nucleoprotein gene and III of G. These results suggest that although the standard genome structure and organization of the RABV isolate are common between the BR-Pfx1 isolate and fixed RABV strains, the unique amino acid substitutions in functional sites of the BR-Pfx1 isolate may result in different biological characteristics from fixed RABV strains.

Experimental infection of vampire bats Desmodus rotundus (E. Geoffroy) maintained in captivity by feeding defibrinated blood added with rabies vírus / Infecção experimental de morcegos hematófagos Desmodus rotundus(E. Geoffroy) mantidos em cativeiro e alimentados com sangue desfibrinado adicionado de vírus da raiva

In vampire bats, food sharing behavior would contribute for the oral transmission of rabies virus among the roostmates. To test this hypothesis, 10 captive Desmodus rotundus bats were fed defibrinateds wine blood containing mice brain suspension of PV-strain of rabies virus. Other 10 bats were fed blood mixed with a mice brain suspension of T-9/95 vampire-bat-field isolate of rabies virus. Another group of 10 bats was inoculated intramuscularly with a mice brain suspension of the T-9/95 isolate. Other 20 bats were maintained without treatment and fed defibrinated swine blood for 158 days. All animals found dead during the observation period or those sacrificed at the end of the experiment were necropsied and specimens such as the brain and non-nervous tissues were collected for rabies examination. Four bats inoculated intramuscularly developed clinical rabies, with signs lasting 1-2 days, and the survival periods ranged from 11-14 days. The initial rabies diagnosis was based on direct fluorescent antibody (dFA) and mouse inoculation test (MIT) performed only on brain specimens, and subsequently, brains andthe non-nervous materials were further reexamined by means of dFA, MIT and heminested-polymerase chain reaction (ht-PCR)technique. The intake of the PV-strain caused rabies in 2 bats, with survival period of 25 and 32 days, while the three bats ingesting theT-9/95 isolate presented periods of 26-31 days. Although discrepant results were found among the diagnostic tests, viruses have disseminated to the central nervous system and other organs, as seenin bats inoculated intramuscularly.(AU)

Em morcegos hematófagos, o hábito de compartilhar alimentopoderia contribuir na transmissão oral do vírus da raiva. Para verificar esta hipótese, 10 morcegos Desmodus rotundus em cativeiro foram alimentados com sangue suíno desfibrinado, contendo suspensão de cérebros de camundongos infectados com vírus rábico PV. Outros 10 camundongos receberam sangue contendo suspensão cerebral de camundongos infectados com vírus de morcego hematófago (T-9/95). Um grupo de 10 camundongos foi inoculado intramuscularmente com suspensão de vírus T-9/95. Outros 20 morcegos foram mantidossem tratamento e alimentados com sangue desfibrinado por 158 dias. Todos os animais encontrados mortos durante o período de observação ou sacrificados no final do experimento foram necropsiados e os cérebros e órgãos não-nervosos foram colhidos para a confirmação da raiva. Quatro morcegos inoculados intramuscularmente apresentaram raiva clínica, com sinais persistind opor 1-2 dias e os períodos de sobrevivência variaram de 11-14 dias. O diagnóstico da raiva inicialmente foi realizado somente com os fragmentos do cérebro, submetendo-os às provas de imunoflurescência direta (IFD) e inoculação em camundongos (IC).Subseqüentemente, os cérebros e os órgãos não-nervosos foram reexaminados com as técnicas de IFD, IC e heminested-polymerase chain reaction (ht-PCR). A ingestão do vírus PV causou raiva em dois morcegos, com período de sobrevivência de 25 e 32 dias, enquanto que os três morcegos que ingeriram o isolado T-9/95 apresentaram períodos de 26-31 dias. Embora encontrando resultados discrepantes entre as técnicas diagnósticas utilizadas, os vírus ingeridos pelos morcegos foram detectados no sistema nervoso central e outros órgãos não-nervosos, como nos morcegos inoculados intramuscularmente.(AU)

Experimental infection of vampire bats Desmodus rotundus (E. Geoffroy) maintained in captivity byfeeding defibrinated blood added with rabies vírus / Infecção experimental de morcegos hematófagos Desmodus rotundus(E. Geoffroy) mantidos em cativeiro e alimentados com sangue desfibrinado adicionado de vírus da raiva

In vampire bats, food sharing behavior would contribute for the oral transmission of rabies virus among the roostmates. To test this hypothesis, 10 captive Desmodus rotundus bats were fed defibrinateds wine blood containing mice brain suspension of PV-strain of rabies virus. Other 10 bats were fed blood mixed with a mice brain suspension of T-9/95 vampire-bat-field isolate of rabies virus. Another group of 10 bats was inoculated intramuscularly with a mice brain suspension of the T-9/95 isolate. Other 20 bats were maintained without treatment and fed defibrinated swine blood for 158 days. All animals found dead during the observation period or those sacrificed at the end of the experiment were necropsied and specimens such as the brain and non-nervous tissues were collected for rabies examination. Four bats inoculated intramuscularly developed clinical rabies, with signs lasting 1-2 days, and the survival periods ranged from 11-14 days. The initial rabies diagnosis was based on direct fluorescent antibody (dFA) and mouse inoculation test (MIT) performed only on brain specimens, and subsequently, brains andthe non-nervous materials were further reexamined by means of dFA, MIT and heminested-polymerase chain reaction (ht-PCR)technique. The intake of the PV-strain caused rabies in 2 bats, with survival period of 25 and 32 days, while the three bats ingesting theT-9/95 isolate presented periods of 26-31 days. Although discrepant results were found among the diagnostic tests, viruses have disseminated to the central nervous system and other organs, as seenin bats inoculated intramuscularly

Em morcegos hematófagos, o hábito de compartilhar alimentopoderia contribuir na transmissão oral do vírus da raiva. Para verificar esta hipótese, 10 morcegos Desmodus rotundus em cativeiro foram alimentados com sangue suíno desfibrinado, contendo suspensão de cérebros de camundongos infectados com vírus rábico PV. Outros 10 camundongos receberam sangue contendo suspensão cerebral de camundongos infectados com vírus de morcego hematófago (T-9/95). Um grupo de 10 camundongos foi inoculado intramuscularmente com suspensão de vírus T-9/95. Outros 20 morcegos foram mantidossem tratamento e alimentados com sangue desfibrinado por 158 dias. Todos os animais encontrados mortos durante o período de observação ou sacrificados no final do experimento foram necropsiados e os cérebros e órgãos não-nervosos foram colhidos para a confirmação da raiva. Quatro morcegos inoculados intramuscularmente apresentaram raiva clínica, com sinais persistind opor 1-2 dias e os períodos de sobrevivência variaram de 11-14 dias. O diagnóstico da raiva inicialmente foi realizado somente com os fragmentos do cérebro, submetendo-os às provas de imunoflurescência direta (IFD) e inoculação em camundongos (IC).Subseqüentemente, os cérebros e os órgãos não-nervosos foram reexaminados com as técnicas de IFD, IC e heminested-polymerase chain reaction (ht-PCR). A ingestão do vírus PV causou raiva em dois morcegos, com período de sobrevivência de 25 e 32 dias, enquanto que os três morcegos que ingeriram o isolado T-9/95 apresentaram períodos de 26-31 dias. Embora encontrando resultados discrepantes entre as técnicas diagnósticas utilizadas, os vírus ingeridos pelos morcegos foram detectados no sistema nervoso central e outros órgãos não-nervosos, como nos morcegos inoculados intramuscularmente

Molecular and geographic analyses of vampire bat-transmitted cattle rabies in central Brazil.

BACKGROUND: Vampire bats are important rabies virus vectors, causing critical problems in both the livestock industry and public health sector in Latin America. In order to assess the epidemiological characteristics of vampire bat-transmitted rabies, the authors conducted phylogenetic and geographical analyses using sequence data of a large number of cattle rabies isolates collected from a wide geographical area in Brazil. METHODS: Partial nucleoprotein genes of rabies viruses isolated from 666 cattle and 18 vampire bats between 1987 and 2006 were sequenced and used for phylogenetic analysis. The genetic variants were plotted on topographical maps of Brazil. RESULTS: In this study, 593 samples consisting of 24 genetic variants were analyzed. Regional localization of variants was observed, with the distribution of several variants found to be delimited by mountain ranges which served as geographic boundaries. The geographical distributions of vampire-bat and cattle isolates that were classified as the identical phylogenetic group were found to overlap with high certainty. Most of the samples analyzed in this study were isolated from adjacent areas linked by rivers. CONCLUSION: This study revealed the existence of several dozen regional variants associated with vampire bats in Brazil, with the distribution patterns of these variants found to be affected by mountain ranges and rivers. These results suggest that epidemiological characteristics of vampire bat-related rabies appear to be associated with the topographical and geographical characteristics of areas where cattle are maintained, and the factors affecting vampire bat ecology.

Genetic analysis of phosphoprotein and matrix protein of rabies viruses isolated in Brazil.

To investigate the genetic characteristics of phosphoprotein (P) and matrix protein (M) genes of variable rabies virus (RV) prevalent in Brazil, the authors genetically characterized the P and M genes from 30 Brazilian RV field isolates. Phylogenetic analysis based on the P and M genes revealed the presence of six RV variants that consisted primarily of three insectivorous bats, the vampire bat, dog and fox in Brazil. Specific amino acid substitutions corresponding to these phylogenetic lineages were observed, with Asp(42) and Glu(62) in the P protein found to be characteristic of Brazilian chiroptera- and carnivora-related RVs, respectively. Amino acid sequence motifs predicted to associate with a viral function in the P and M proteins were conserved among Brazilian RV variants.

Phylogenetic characterization of rabies virus isolates from Carnivora in Brazil.

The incidence of canine rabies has been widely reported in Brazil, and new rabies virus (RV) variants, genetically similar to canine RV, have recently been isolated from foxes. In order to derive the epidemiological characteristics of Brazilian Carnivora RV, Brazilian RVs isolated from dogs, cats, and foxes were genetically analyzed. Brazilian Carnivora RV isolates were divided into 2 main lineages. The predominant lineage was found in dogs and cats, which included the Argentinean and Bolivian Carnivora RV isolates, and was extensively distributed throughout Brazil and surrounding countries. The other lineage consisted of three sublineages containing Brazilian dog and fox RV isolates, with the dog sublineages located on an internal branch of 2 fox sublineages, suggesting that RV transmission events might have occurred between foxes and dogs in the past. These results suggest that contact between dogs and wildlife has the potential to generate new rabies variants and that it is important to control RV infection cycles in both dogs and wildlife to prevent spread of rabies infection.

Experiments on intramuscular inoculation and feeding domestic cats (Felis catus) with brains of mice previously infected by rabies viruses / Ensaios sobre inoculação intramuscular e alimentação de gatos domésticos (Felis catus) com cérebros de camundongos préviamente inoculados com vírus da raiva

Nineteen kittens divided into four groups were fed with brains of mice infected with rabies viruses. Each four kittens (group I) received four brains infected with the PV fixed strain; nine kittens (group II) ingested 4-5 brains infected with the field isolate T-9/95, isolated from the Desmodus rotundus vampire bat; two kittens (group III) fedten T-9/95-infected brains, and four cats consumed 32-37 PV strain infected brains. One adult male, inoculated into masseter muscle with a 20% T-9/95-infected brain suspension, presented rabies after an incubation period of six days, followed with 8 days of clinical evolution, and died there after and this cat was considered as the rabies “positive standard”. After observing for 20-230 days, all the cats feeding the rabid brains were submitted to euthanasia, by using Acepran®, Zoletil®,and T-61®. At necropsy, samples of brain, heart, lung, kidney, submaxillary salivary gland, and cervical medulla were collected from all the cats and further submitted to the direct fluorescence anti bodytest (dFA), mouse inoculation test (MIT) and to the reverse transcriptase-polymerase chain reaction (RT-PCR) technique. Brain, cervical medulla, and the submaxillary salivary gland of the positive standard cat were dFA-positive, and brain and cervical medulla were positive for MIT. All specimens of this cat tested by the RT-PCR were found positive. No animals ingesting PV or T-9/95 virus-infected brains developed clinical signs and all materials tested were negative by dFA and MIT. Several specimens, however, showed positive reactions by the RT-PCR technique, but cats were resistant to rabies through the viruses administered orally.(AU)

Dezenove gatos, divididos em quatro grupos, foram alimentados com cérebros de camundongos infectados com vírus de raiva. Cada um dos quatro gatos (grupo I) receberam quatro cérebros infectados com vírus fixo PV; nove gatos (grupo II) ingeriram 4-5 cérebros infectados com uma amostra de campo T-9/95, isolada do morcego Desmodus rotundus; dois gatos (grupo III) ingeriram 10 cérebros infectados com T-9/95 e quatro gatos (grupo IV) ingeriram 32-37 cérebros infectados com vírus PV. Um macho adulto, inoculado no músculo masséter, com uma suspensão cerebral a 20% da amostra T-9/95, desenvolveu raiva após período de incubação de seis dias,seguidos por oito dias de evolução clínica, morrendo em seguida. Este gato foi denominado de “padrão positivo”. Após observação por um período de 20-230 dias, todos os gatos que receberam cérebros foram submetidos à eutanásia, utilizando Acepran®, Zoletil® e T-61®. À necropsia, foram colhidas amostras do cérebro, coração, pulmão, rim, glândula salivar submaxilar e medula cervical e submetidas à prova de imunofluorescência direta (IFD), inoculação em camundongos (IC), e reação em cadeia pela polimerase-transcriptase reversa (RT-PCR). No “padrão positivo”, cérebro, medula cervical e glândula salivar foram positivos à IFD e à IC, cérebro e medula cervical foram os positivos. Todos os espécimes do “padrão positivo” foram positivos à RT-PCR. Nenhum animal que ingeriu cérebros contendo amostras de vírus PV ou T-9/95 apresentou sinais clínicos e todos os espécimes testados foram negativos à IFD e IC, no entanto, alguns espécimes reagiram positivamente à RT-PCR, porém, os gatos foram resistentes à raiva com vírus administrados oralmente.(AU)

Experiments on intramuscular inoculation and feeding domestic cats (Felis catus) with brains of mice previously infected by rabies viruses

Nineteen kittens divided into four groups were fed with brains of mice infected with rabies viruses. Each four kittens (group I) received four brains infected with the PV fixed strain; nine kittens (group II) ingested 4-5 brains infected with the field isolate T-9/95, isolated from the Desmodus rotundus vampire bat; two kittens (group III) fedten T-9/95-infected brains, and four cats consumed 32-37 PV strain infected brains. One adult male, inoculated into masseter muscle with a 20% T-9/95-infected brain suspension, presented rabies after an incubation period of six days, followed with 8 days of clinical evolution, and died there after and this cat was considered as the rabies “positive standard”. After observing for 20-230 days, all the cats feeding the rabid brains were submitted to euthanasia, by using Acepran®, Zoletil®,and T-61®. At necropsy, samples of brain, heart, lung, kidney, submaxillary salivary gland, and cervical medulla were collected from all the cats and further submitted to the direct fluorescence antibodytest (dFA), mouse inoculation test (MIT) and to the reverse transcriptase-polymerase chain reaction (RT-PCR) technique. Brain, cervical medulla, and the submaxillary salivary gland of the positive standard cat were dFA-positive, and brain and cervical medulla were positive for MIT. All specimens of this cat tested by the RT-PCR were found positive. No animals ingesting PV or T-9/95 virus-infectedbrains developed clinical signs and all materials tested were negativeby dFA and MIT. Several specimens, however, showed positive reactions by the RT-PCR technique, but cats were resistant to rabies through the viruses administered orally.

Dezenove gatos, divididos em quatro grupos, foram alimentadoscom cérebros de camundongos infectados com vírus de raiva. Cada um dos quatro gatos (grupo I) receberam quatro cérebros infectados com vírus fixo PV; nove gatos (grupo II) ingeriram 4-5 cérebros infectados com uma amostra de campo T-9/95, isolada do morcego Desmodus rotundus; dois gatos (grupo III) ingeriram 10 cérebros infectados com T-9/95 e quatro gatos (grupo IV) ingeriram 32-37 cérebros infectados com vírus PV. Um macho adulto, inoculado no músculo masséter, com uma suspensão cerebral a 20% da amostra T-9/95, desenvolveu raiva após período de incubação de seis dias,seguidos por oito dias de evolução clínica, morrendo em seguida. Este gato foi denominado de “padrão positivo”. Após observação por um período de 20-230 dias, todos os gatos que receberam cérebros foram submetidos à eutanásia, utilizando Acepran®, Zoletil® e T-61®. À necropsia, foram colhidas amostras do cérebro, coração, pulmão,rim, glândula salivar submaxilar e medula cervical e submetidas à prova de imunofluorescência direta (IFD), inoculação em camundongos (IC), e reação em cadeia pela polimerase-transcriptase reversa (RT-PCR). No “padrão positivo”, cérebro, medula cervical eglândula salivar foram positivos à IFD e à IC, cérebro e medula cervical foram os positivos. Todos os espécimes do “padrão positivo” foram positivos à RT-PCR. Nenhum animal que ingeriu cérebros contendo amostras de vírus PV ou T-9/95 apresentou sinais clínicos e todos osespécimes testados foram negativos à IFD e IC, no entanto, alguns espécimes reagiram positivamente à RT-PCR, porém, os gatos foram resistentes à raiva com vírus administrados oralmente. Master thesis submitted to the Faculty of Veterinary Medicine and Zootechny of the University of São Paulo, on June 24th, 2003. Fellowship from the Fundação de Amparo à Pesquisa do Estado de São Paulo-FAPESP, process No. 01/07188-8.