16 resultados para rhabdoviridae
Resumo:
A raiva é uma das zoonoses mais antigas e temidas pelo homem devido a seu desfecho fatal. Os cães ainda são considerados os principais responsáveis pela manutenção e transmissão da raiva para o homem. Porém, nos últimos anos os morcegos hematófagos têm ganhado destaque como potenciais transmissores de raiva para animais e humanos nas Américas. Recentemente, várias epidemias de raiva humana transmitida por morcegos hematófagos foram relatados no estado do Pará, o que mostra uma grande alteração no ambiente natural destes animais. A amplificação parcial do gene N pela técnica de RT-PCR foi aplicada em 62 amostras positivas para o Vírus da raiva, pela imunofluorescência direta e prova biológica. As seqüências nucleotídicas obtidas foram comparadas entre si e com outras amostras de vírus rábico isoladas no Brasil, utilizando os métodos de análise filogenética máxima verossimilhança e Bayesiano. Estas análises permitiram traçar o perfil epidemiológico molecular das variantes virais circulantes no estado do Pará, observando a emergência da transmissão de casos associados à variante antigênica 3 (VAg3), comumente encontrada em morcegos hematófagos Desmodus rotundus em detrimento dos casos relacionados à variante antigênica 2 (VAg2) associada a cães domésticos, bem como a identificação de três linhagens genéticas relacionadas a VAg3 e uma relacionada a VAg2 e uma possível nova variante isolada de morcego frugívoro Uroderma bilobatum.
Resumo:
The Rhabdoviridae, whose members collectively infect invertebrates, animals, and plants, form a large family that has important consequences for human health, agriculture, and wildlife ecology. Plant rhabdoviruses can be separated into the genera Cytorhabdovirus and Nucleorhabdovirus, based on their sites of replication and morphogenesis. This review presents a general overviewof classical and contemporary findings about rhabdovirus ecology, pathology, vector relations, and taxonomy. The genome organization and structure of several recently sequenced nucleorhabdoviruses and cytorhabdoviruses is integrated with new cell biology findings to provide a model for the replication of the two genera. A prospectus outlines the exciting opportunities for future research that will contribute to a more detailed understanding of the biology, biochemistry, replication and host interactions of the plant rhabdoviruses.
Resumo:
Rhabdoviruses are important pathogens of humans, livestock, and plants that are often vectored by insects. Rhabdovirus particles have a characteristic bullet shape with a lipid envelope and surface-exposed transmembrane glycoproteins. Sigma virus (SIGMAV) is a member of the Rhabdoviridae and is a naturally occurring disease agent of Drosophila melanogaster. The infection is maintained in Drosophila populations through vertical transmission via germ cells. We report here the nature of the Drosophila innate immune response to SIGMAV infection as revealed by quantitative reverse transcription-PCR analysis of differentially expressed genes identified by microarray analysis. We have also compared and contrasted the immune response of the host with respect to two nonenveloped viruses, Drosophila C virus (DCV) and Drosophila X virus (DXV). We determined that SIGMAV infection upregulates expression of the peptidoglycan receptor protein genes PGRP-SB1 and PGRP-SD and the antimicrobial peptide (AMP) genes Diptericin-A, Attacin-A, Attacin-B, Cecropin-A1, and Drosocin. SIGMAV infection did not induce PGRP-SA and the AMP genes Drosomycin-B, Metchnikowin, and Defensin that are upregulated in DCV and/or DXV infections. Expression levels of the Toll and Imd signaling cascade genes are not significantly altered by SIGMAV infection. These results highlight shared and unique aspects of the Drosophila immune response to the three viruses and may shed light on the nature of the interaction with the host and the evolution of these associations.
Resumo:
RNA silencing in plants and insects provides an antiviral defense and as a countermeasure most viruses encode RNA silencing suppressors (RSS). For the family Rhabdoviridae, no detailed functional RSS studies have been reported in plant hosts and insect vectors. In agroinfiltrated Nicotiana benthamiana leaves we show for the first time for a cytorhabdovirus, lettuce necrotic yellows virus (LNYV), that one of the nucleocapsid core proteins, phosphoprotein (P) has relatively weak local RSS activity and delays systemic silencing of a GFP reporter. Analysis of GFP small RNAs indicated that the P protein did not prevent siRNA accumulation. To explore RSS activity in insects, we used a Flock House virus replicon system in Drosophila S2 cells. In contrast to the plant host, LNYV P protein did not exhibit RSS activity in the insect cells. Taken together our results suggest that P protein may target plant-specific components of RNA silencing post siRNA biogenesis.
Resumo:
The large protein L of negative-sense RNA viruses is a multifunctional protein involved in transcription and replication of genomic RNA. It also possesses enzymatic activities involved in capping and methylation of viral mRNAs. The pathway for mRNA capping followed by the L protein of the viruses in the Morbillivirus genus has not been established, although it has been speculated that these viruses may follow the unconventional capping pathway as has been shown for some viruses of Rhabdoviridae family. We had earlier shown that the large protein L of Rinderpest virus expressed as recombinant L-P complex in insect cells as well as the ribonucleoprotein complex from purified virus possesses RNA triphosphatase (RTPase) and guanylyltransferase activities, in addition to RNA dependent RNA polymerase activity. In the present work, we demonstrate that RTPase as well as nucleoside triphosphatase (NTPase) activities are exhibited by a subdomain of the L protein in the C terminal region (a.a. 1640 1840). The RTPase activity depends absolutely on a divalent cation, either magnesium or manganese. Both the RTPase and NTPase activities of the protein show dual metal specificity. Two mutant proteins having alanine mutations in the glutamic acid residues in motif-A of the RTPase domain did not show RTPase activity, while exhibiting reduced NTPase activity suggesting overlapping active sites for the two enzymatic functions. The RTPase and NTPase activities of the L subdomain resemble those of the Vaccinia capping enzyme D1 and the baculovirus LEF4 proteins. (C) 2015 Elsevier Inc. All rights reserved.
Resumo:
Viral infections remain a serious global health issue. Metagenomic approaches are increasingly used in the detection of novel viral pathogens but also to generate complete genomes of uncultivated viruses. In silico identification of complete viral genomes from sequence data would allow rapid phylogenetic characterization of these new viruses. Often, however, complete viral genomes are not recovered, but rather several distinct contigs derived from a single entity are, some of which have no sequence homology to any known proteins. De novo assembly of single viruses from a metagenome is challenging, not only because of the lack of a reference genome, but also because of intrapopulation variation and uneven or insufficient coverage. Here we explored different assembly algorithms, remote homology searches, genome-specific sequence motifs, k-mer frequency ranking, and coverage profile binning to detect and obtain viral target genomes from metagenomes. All methods were tested on 454-generated sequencing datasets containing three recently described RNA viruses with a relatively large genome which were divergent to previously known viruses from the viral families Rhabdoviridae and Coronaviridae. Depending on specific characteristics of the target virus and the metagenomic community, different assembly and in silico gap closure strategies were successful in obtaining near complete viral genomes.
Resumo:
The complete genome of spring viraemia of carp virus (SVCV) strain A-1 isolated from cultured common carp (Cyprinus carpio) in China was sequenced and characterized. Reverse transcription-polymerase chain reaction (RT-PCR) derived clones were constructed and the DNA was sequenced. It showed that the entire genome of SVCV A-1 consists of 11,100 nucleotide base pairs, the predicted size of the viral RNA of rhabdoviruses. However, the additional insertions in bp 4633-4676 and bp 4684-4724 of SVCV A-1 were different from the other two published SVCV complete genomes. Five open reading frames (ORFs) of SVCV A-1 were identified and further confirmed by RT-PCR and DNA sequencing of their respective RT-PCR products. The 5 structural proteins encoded by the viral RNA were ordered 3'-N-P-M-G-L-5'. This is the first report of a complete genome sequence of SVCV isolated from cultured carp in China. Phylogenetic analysis indicates that SVCV A-1 is closely related to the members of the genus Vesiculovirus, family Rhabdoviridae.
Resumo:
Co-infection of two viruses has been observed in mandarin fish (Siniperca chuatsi), but the two viruses have not been characterized. In this study, a rhabdovirus has been isolated from the co-infected two viruses extracted from the diseased mandarin fish, and its morphological structure and partial biochemical and biophysical characteristics have been observed and analyzed. The isolated rhabdovirus has a typical bullet shape, and is therefore called S. chttatsi rhabdovirus (SCRV). And, the isolated rhabdovirus produced a higher titer (10(8.5) TCID50 ml(-1)) than did the co-infecting viruses (10(6.5) TCID50 ml(-1)). Subsequently, the viral genome RNA was extracted, and used as template to clone the complete nucleoprotein (N) gene by RT-PCR amplification. Cloning and sequencing of the SCRV N protein revealed 42%-31% amino acid identities to that of trout rhabdovirus 903/87 and the rhabdoviruses in genus Vesiculovirus. SDS-PAGE separation of the isolated SCRV and other two rhabdoviruses also revealed obvious polypeptide profile difference. Moreover, the anti-SCRV N protein antibody was prepared, and the anti-SCRV N protein antibody only could recognize the SCRV N protein, whereas no antigenicity was detected in other two rhabdoviruses. The data suggested that the SCRV should be a rhabdovirus member related to the genus Vesiculovirus in the Rhabdoviridae. (c) 2006 Elsevier B.V. All rights reserved.
Resumo:
The complete nucleotide sequence of the genomic RNA 1 (8745 nt) and RNA 2 (4986 nt) of Citrus leprosis virus cytoplasmic type (CiLV-C) was determined using cloned cDNA. RNA 1 contains two open reading frames (ORFs), which correspond to 286 and 29 kDa proteins. The 286 kDa protein is a polyprotein putatively involved in virus replication, which contains four conserved domains: methyltransferase, protease, helicase and polymerase. RNA 2 contains four ORFs corresponding to 15, 61, 32 and 24 kDa proteins, respectively. The 32 kDa protein is apparently involved in cell-to-cell movement of the virus, but none of the other putative proteins exhibit any conserved domain. The 5' regions of the two genomic RNAs contain a 'cap' structure and poly(A) tails were identified in the 3'-terminals. Sequence analyses and searches for structural and non-structural protein similarities revealed conserved domains with members of the genera Furovirus, Bromovirus, Tobravirus and Tobamovirus, although phylogenetic analyses strongly suggest that CiLV-C is a member of a distinct, novel virus genus and family, and definitely demonstrate that it does not belong to the family Rhabdoviridae, as previously proposed. Based on these results it was proposed that Citrus leprosis virus be considered as the type member of a new genus of viruses, Cilevirus.
Resumo:
O vírus Marabá (Be AR 411459) é um Vesiculovírus (VSV), membro da família Rhabdoviridae, isolado em 1983, de um pool de flebotomíneos capturado em Marabá-PA pela Seção de Arbovírus do Instituto Evandro Chagas. Na literatura pouco se tem sobre neuropatologia experimental induzida pelo vírus Marabá, apesar dos 30 anos de isolamento. Um único estudo, porém, revelou que a infecção viral em camundongos recém-nascidos provoca necrose e picnose em neurônios em várias regiões do sistema nervoso central (SNC) O objetivo do presente trabalho foi investigar a distribuição do vírus Marabá no SNC, a ativação microglial e astrocitária, aspectos histopatológicos; e a expressão de citocinas e óxido nítrico (NO), na encefalite induzida pelo vírus Marabá em camundongo BALB/c adultos. Para tanto, foram realizados processamentos de amostras para análise histopatologica; immunohistoquímica para marcação de microglia, astrócitos e antígeno viral; testes de quantificação de citocinas e NO; e análises estatísticas. Os resultados demonstraram que os animais infectados (Ai) 3 dias após a inoculação (d.p.i.) apresentam discreta marcação do antígeno viral, bem como quanto a ativação de microglia e astrócitos no SNC. Por outro lado, nos Ai 6 d.p.i. a marcação do antígeno viral foi observada em quase todas regiões encefálicas, observando-se intensa ativação microglial nestes locais, embora a astrogliose tenha sido menor. Edema, necrose e apoptose de neurônios foram observados principalmente no bulbo olfatório, septo interventrícular e córtex frontal dos Ai 6 d.p.i. A quantificação dos níveis de IL-12p40, IL-10, IL-6, TNF- α, INF-ү, MCP-1 e de NO mostrou aumentos significativos nos Ai 6 d.p.i., quando comparados aos animais controles e Ai 3 d.p.i.. Por outro lado, os níveis de TGF-β, importante imunossupressor, não foi significativo em todos os grupos e tempos avaliados (3 e 6 d.p.i.). Estes resultados indicam que o vírus Marabá pode infectar diversas regiões do SNC de camundongo BALB/c adulto 6 d.p.i., produzindo alterações anátomo-patológicas e uma forte resposta imune inflamatória que pode ser letal para o animal.
Resumo:
The causative agents of rabies are single-stranded, negative-sense RNA viruses in the genus Lyssavirus of Rhabdoviridae, consisting of twelve classified and three as yet unclassified species including classical rabies virus (RABV). Highly neurotropic RABV causes rapidly progressive encephalomyelitis with nearly invariable fatal outcome. Rapid and reliable diagnosis of rabies is highly relevant for public and veterinary health. Due to growing variety of the genus Lyssavirus observed, the development of suitable molecular assays for diagnosis and differentiation is challenging. This work focused on the establishment of a suitable real-time RT-PCR technique for rabies diagnosis as a complement to fluorescent antibody test and rabies tissue culture infection test as gold standard for diagnosis and confirmation. The real-time RT-PCR was adapted with the goal to detect the whole spectrum of lyssavirus species, for nine of which synthesized DNA fragments were used. For the detection of species, seven probes were developed. Serial dilutions of the rabies virus strain CVS-11 showed a 100-fold higher sensitivity of real-time PCR compared to heminested RT-PCR. Using a panel of thirty-one lyssaviruses representing four species, the suitability of the protocol could be shown. Phylogenetic analysis of the sequences obtained by heminested PCR allowed correct classification of all viruses used.
Resumo:
A reverse genetics approach was applied to generate a chimeric nonsegmented negative strand RNA virus, rabies virus (RV) of the Rhabdoviridae family, that expresses a foreign protein. DNA constructs containing the entire open reading frame of the bacterial chloramphenicol acetyltransferase (CAT) gene and an upstream RV cistron border sequence were inserted either into the nontranslated pseudogene region of a full-length cDNA copy of the RV genome or exchanged with the pseudogene region. After intracellular T7 RNA polymerase-driven expression of full-length antigenome RNA transcripts and RV nucleoprotein, phosphoprotein and polymerase from transfected plasmids, RVs transcribing novel monocistronic mRNAs and expressing CAT at high levels, were recovered. The chimeric viruses possessed the growth characteristics of standard RV and were genetically stable upon serial cell culture passages. CAT activity was still observed in cell cultures infected with viruses passaged for more than 25 times. Based on the unprecedented stability of the chimeric RNA genomes, which is most likely due to the structure of the rhabdoviral ribonucleoprotein complex, we predict the successful future use of recombinant rhabdovirus vectors for displaying foreign antigens or delivering therapeutic genes.
Resumo:
El maíz es uno de los principales cereales, ubicándose tercero en el ranking de producción mundial. Las enfermedades virales en el cultivo de maíz son factores importantes de pérdidas en la producción, en el mundo. Se ha citado mundialmente la presencia de varios rhabdovirus en maíz, aunque ninguno en Argentina. Maize mosaic virus (MMV) es el más importante debido a las pérdidas que ocasiona. Durante 2006/07 se detectó en trigo Argentina, un Cytorhabdovirus denominado Cereal Rhabdovirus caracterizado serológicamente como Barley yellow striate mosaic virus (BYSMV). Desde 2000/01 hasta la actualidad, se observan plantas de maíz con achaparramiento, esterilidad y estriado amarillo en hojas, en localidades de Córdoba y Santa Fe. Se observaron al microscopio electrónico partículas de rhabdovirus en el citoplasma de las células. Pruebas serológicas para MMV resultaron negativas. Esta virosis fue transmitida a plantas de maíz sanas por el delfácido Peregrinus maidis. Se amplificó un segmento del gen de la polimerasa L de rhabdovirus, mediante RT-PCR con iniciadores degenerados y se obtuvieron las relaciones filogenéticas con otros rhabdovirus, confirmando que se trata de un miembro del género Cytorhabdovirus. Se trataría de un virus nuevo, de la familia Rhabdoviridae presente en diversas localidades del área maicera argentina. El objetivo de este proyecto es estudiar la epidemiología de este virus, mediante la reconstrucción de su historia demográfica y patrones espacio-temporales, utilizando análisis de coalescencia y filogeografía. Se busca: Determinar la secuencia genómica completa del virus en estudio; Obtener iniciadores específicos para el gen de la nucleocápside; Obtener las secuencias nucleotídicas del gen de la nucleocápside viral de aislamientos de diferentes localidades del área maicera argentina; Analizar los patrones filogeográficos de dichos aislamientos. Materiales y métodos. Recolección de material enfermo. Se colectarán plantas de maíz con sintomatología de estriado amarillo, en distintas localidades de Córdoba y Santa Fe. Secuenciación del genoma completo viral. Se purificará el virus en estudio a partir de tejido enfermo (Creamer, 1992). Se extraerá ARN total y se lo enviará al servicio de pirosecuenciación (INDEAR, Argentina). Las secuencias obtenidas serán analizadas utilizando software específico (Lasergene 10, DNASTAR, entre otros). Diseño de iniciadores específicos para el gen de la proteína N viral. Serán diseñados a partir de la secuencia del genoma completo del virus. Determinación de patrones filogeográficos. Se extraerá ARN total de plantas sintomáticas de distintas localidades argentinas. Se amplificará el gen N de cada uno de los aislamientos, se clonarán y secuenciarán estos fragmentos y se alinearán las secuencias obtenidas. Se reconstruirá la filogenia mediante metodología Bayesiana y se realizará un análisis de coalescencia. Finalmente se analizará el patrón filogeográfico del rhabdovirus en estudio. Con el presente trabajo se espera avanzar en el conocimiento de este nuevo virus que afecta cultivos de maíz en Argentina. Se pretende obtener la secuencia genómica completa viral, lo que significará un avance en la caracterización e identificación del mismo. Se busca conocer sus patrones de dispersión espacio-temporales, para comprender los orígenes y posible evolución hacia otras regiones del país. El análisis de secuencias genómicas, brinda una herramienta rápida y de menor esfuerzo de muestreo en el estudio epidemiológico de las poblaciones. El conocimiento de la distribución actual e histórica de este nuevo virus sería crucial para futuros planes de manejo de la enfermedad. El tema de investigación se lleva a cabo en el marco de una tesis doctoral con el apoyo de una beca de formación de CONICET. La transferencia es constante a traves del contacto con productores y asesores agrícolas y mediante la realización de jornadas, charlas, cursos y publicaciones periódicas en medios de difusión.
Resumo:
Flying foxes have been the focus of research into three newly described viruses from the order Mononegavirales, namely Hendra virus (HeV), Menangle virus and Australian Bat Lyssavirus (ABL). Early investigations indicate that flying foxes are the reservoir host for these viruses. In 1994, two outbreaks of a new zoonotic disease affecting horses and humans occurred in Queensland. The virus which was found to be responsible was called equine morbillivirus (EMV) and has since been renamed HeV. Investigation into the reservoir of HeV has produced evidence that antibodies capable of neutralising HeV have only been detected in flying foxes. Over 20% of flying foxes in eastern Australia have been identified as being seropositive. Additionally six species of flying foxes in Papua New Guinea have tested positive for antibodies to HeV. In 1996 a virus from the family Paramyxoviridae was isolated from the uterine fluid of a female flying fox. Sequencing of 10 000 of the 18 000 base pairs (bp) has shown that the sequence is identical to the HeV sequence. As part of investigations into HeV, a virus was isolated from a juvenile flying fox which presented with neurological signs in 1996. This virus was characterised as belonging to the family Rhabdoviridae, and was named ABL. Since then four flying fox species and one insectivorous species have tested positive for ABL. The third virus to be detected in flying foxes is Menangle virus, belonging to the family Paramyxoviridae. This virus was responsible for a zoonotic disease affecting pigs and humans in New South Wales in 1997. Antibodies capable of neutralising Menangle virus, were detected in flying foxes. (C) 1999 Elsevier Science B.V. All rights reserved.
Resumo:
Resumen Según la OMS la forma más eficaz para reducir los casos de rabia anuales en humanos es a través de vacunaciones en perros y gatos, dado que el 90 % de los mismos son debido a mordeduras de estos animales, mayoritariamente caninos, infectados con el virus. En países de la región, donde se ha evaluado el nivel de protección de perros vacunados contra el virus de la rabia, se han encontrado variaciones importantes. El objetivo de este trabajo fue evaluar la respuesta inmune humoral contra la rabia en perros con algún tipo de modulación inmunológica inducida experimentalmente. Para esto se inmunizaron cinco grupos de perros con vacunas polivalentes (Grupo 1), monovalentes (Grupo 2), inmunizados durante la castración quirúrgica (Grupo 3), que estaban en tratamiento con Triamcinolona acetonido (corticoides) durante la inmunización (Grupo 4) o que fueron vacunados simultáneamente con un inmunoestimulante comercial (Grupo 5). En términos generales los resultados obtenidos indican que en todos los casos, la mayoría de los animales pudieron superar el límite mínimo de anticuerpos para estar protegidos según la OMS (0.5UI/ml). Sin embargo, se encontraron diferencias significativas (p<0.05) en el uso de vacunas mono o polivalente, el uso de corticoides al momento de la inmunización y en la vacunación durante la castración quirúrgica
