ABSTRACT
Abstract Novel coronavirus (nCoV) namely "SARS-CoV-2" is being found responsible for current PANDEMIC commenced from Wuhan (China) since December 2019 and has been described with epidemiological linkage to China in about 221 countries and territories until now. In this study we have characterized the genetic lineage of SARS-CoV-2 and report the recombination within the genus and subgenus of coronaviruses. Phylogenetic relationship of thirty nine coronaviruses belonging to its four genera and five subgenera was analyzed by using the Neighbor-joining method using MEGA 6.0. Phylogenetic trees of full length genome, various proteins (spike, envelope, membrane and nucleocapsid) nucleotide sequences were constructed separately. Putative recombination was probed via RDP4. Our analysis describes that the "SARS-CoV-2" although shows great similarity to Bat-SARS-CoVs sequences through whole genome (giving sequence similarity 89%), exhibits conflicting grouping with the Bat-SARS-like coronavirus sequences (MG772933 and MG772934). Furthermore, seven recombination events were observed in SARS-CoV-2 (NC_045512) by RDP4. But not a single recombination event fulfills the high level of certainty. Recombination mostly housed in spike protein genes than rest of the genome indicating breakpoint cluster arises beyond the 95% and 99% breakpoint density intervals. Genetic similarity levels observed among "SARS-CoV-2" and Bat-SARS-CoVs advocated that the latter did not exhibit the specific variant that cause outbreak in humans, proposing a suggestion that "SARS-CoV-2" has originated possibly from bats. These genomic features and their probable association with virus characteristics along with virulence in humans require further consideration.
Resumo O novo coronavírus (nCoV), nomeadamente "SARS-CoV-2", foi considerado responsável pela pandemia atual iniciada em Wuhan (China) desde dezembro de 2019 e foi descrito com ligação epidemiológica à China em cerca de 221 países e territórios até agora. Neste estudo, caracterizamos a linhagem genética do SARS-CoV-2 e relatamos a recombinação dentro do gênero e subgênero dos coronavírus. A relação filogenética de 39 coronavírus pertencentes a seus quatro gêneros e cinco subgêneros foi analisada usando o método de Neighbour-joining usando MEGA 6.0. Árvores filogenéticas do genoma de comprimento total, várias proteínas (espícula, envelope, membrana e nucleocapsídeo), sequências de nucleotídeos foram construídas separadamente. A recombinação putativa foi testada via RDP4. Nossa análise descreve que o "SARS-CoV-2", embora mostre grande semelhança com as sequências de Bat-SARS-CoVs em todo o genoma (dando semelhança de sequência de 89%), exibe agrupamento conflitante com as sequências de coronavírus do tipo Bat-SARS (MG772933 e MG772934) Além disso, sete eventos de recombinação foram observados em SARS-CoV-2 (NC045512) por RDP4. Mas nem um único evento de recombinação preenche o alto nível de certeza. A recombinação está alojada mais em genes de proteína de pico, principalmente, do que no resto do genoma, indicando que o cluster de ponto de interrupção surge além dos intervalos de densidade de ponto de interrupção de 95% e 99%. Os níveis de similaridade genética observados entre "SARS-CoV-2" e Bat-SARS-CoVs defendem que o último não exibe a variante específica que causa surto em humanos, sugerindo que "SARS-CoV-2" tenha se originado possivelmente de morcegos. Essas características genômicas e sua provável associação com as características do vírus, juntamente com a virulência em humanos, requerem uma consideração mais aprofundada.
Subject(s)
Humans , Animals , Chiroptera , COVID-19 , Phylogeny , Computer Simulation , Genome, Viral/genetics , SARS-CoV-2ABSTRACT
Abstract INTRODUCTION: We performed an epidemiological surveillance of the Chikungunya (CHIKV) lineages in Bahia after the 2014 East/Central/South African (ECSA) genotype outbreak. METHODS: Reverse-transcription polymerase chain reaction (RT-PCR), viral isolation, and phylogenetic analyses were conducted on serum samples from 605 patients with CHIKV-like symptoms during 2014-2018. RESULTS: Of the 605 samples, 167 were CHIKV-positive. Viral isolation was achieved for 20 samples; their phylogenetic analysis (E2 protein) revealed the presence of ECSA lineage and reinforced the phylogenetic relationship between ECSA and Indian Ocean lineages. CONCLUSIONS: The genomic surveillance of CHIKV showed that only ECSA lineage circulated in Bahia since the 2014 outbreak.
Subject(s)
Humans , Male , Female , Adult , Chikungunya virus/genetics , Genome, Viral/genetics , Chikungunya Fever/virology , Phylogeny , Brazil/epidemiology , Disease Outbreaks , Reverse Transcriptase Polymerase Chain Reaction , Epidemiological Monitoring , Chikungunya Fever/epidemiology , GenotypeABSTRACT
BACKGROUND A number of Zika virus (ZIKV) sequences were obtained using Next-generation sequencing (NGS), a methodology widely applied in genetic diversity studies and virome discovery. However Sanger method is still a robust, affordable, rapid and specific tool to obtain valuable sequences. OBJECTIVE The aim of this study was to develop a simple and robust Sanger sequencing protocol targeting ZIKV relevant genetic regions, as envelope protein and nonstructural protein 5 (NS5). In addition, phylogenetic analysis of the ZIKV strains obtained using the present protocol and their comparison with previously published NGS sequences were also carried out. METHODS Six Vero cells isolates from serum and one urine sample were available to develop the procedure. Primer sets were designed in order to conduct a nested RT-PCR and a Sanger sequencing protocols. Bayesian analysis was used to infer phylogenetic relationships. FINDINGS Seven complete ZIKV envelope protein (1,571 kb) and six partial NS5 (0,798 Kb) were obtained using the protocol, with no amplification of NS5 gene from urine sample. Two NS5 sequences presented ambiguities at positions 495 and 196. Nucleotide analysis of a Sanger sequence and consensus sequence of previously NGS study revealed 100% identity. ZIKV strains described here clustered within the Asian lineage. MAIN CONCLUSIONS The present study provided a simple and low-cost Sanger protocol to sequence relevant genes of the ZIKV genome. The identity of Sanger generated sequences with published consensus NGS support the use of Sanger method for ZIKV population studies. The regions evaluated were able to provide robust phylogenetic signals and may be used to conduct molecular epidemiological studies and monitor viral evolution.
Subject(s)
RNA, Viral/genetics , Genome, Viral/genetics , Reverse Transcriptase Polymerase Chain Reaction , Zika Virus/genetics , Phylogeny , Viral Nonstructural Proteins , High-Throughput Nucleotide SequencingABSTRACT
In Brazil, detection of the HIV-1 sub-subtype F1 has decreased with a simultaneous increase in detection of the recombinant FB and FC forms. In previous HIV-1 env molecular epidemiology studies in Rio de Janeiro, 11.4% of the detected sequences were of the F1 sub-subtype. With the goal of re-estimating the prevalence of the HIV-1 F1 sub-subtype, we performed extended analyses of these samples by examining five genomic regions, resulting in 3.3% being confirmed as F1. Moreover, genomic analysis of 11 of the 21 samples identified as F1 confirmed that nine were F1 and two were BF1. Considering the number of samples assayed, the prevalence of F1 was quite low, which supports the use of different genomic regions for the assessment of HIV-1 classification in countries where several subtypes and recombinant forms co-circulate.
Subject(s)
Humans , HIV Infections/epidemiology , HIV Infections/virology , HIV-1/genetics , Genome, Viral/genetics , Phylogeny , Brazil/epidemiology , DNA Mutational Analysis , Base Sequence , Molecular Epidemiology , GenotypeABSTRACT
The current yellow fever outbreak in Brazil is the most severe one in the country in recent times. It has rapidly spread to areas where YF virus (YFV) activity has not been observed for more than 70 years and vaccine coverage is almost null. Here, we sequenced the whole YFV genome of two naturally infected howler-monkeys (Alouatta clamitans) obtained from the Municipality of Domingos Martins, state of Espírito Santo, Brazil. These two ongoing-outbreak genome sequences are identical. They clustered in the 1E sub-clade (South America genotype I) along with the Brazilian and Venezuelan strains recently characterised from infections in humans and non-human primates that have been described in the last 20 years. However, we detected eight unique amino acid changes in the viral proteins, including the structural capsid protein (one change), and the components of the viral replicase complex, the NS3 (two changes) and NS5 (five changes) proteins, that could impact the capacity of viral infection in vertebrate and/or invertebrate hosts and spreading of the ongoing outbreak.
Subject(s)
Animals , Polymorphism, Genetic/genetics , Yellow Fever/veterinary , Yellow fever virus/genetics , Genome, Viral/genetics , Alouatta/virology , Monkey Diseases/virology , Phylogeny , Yellow Fever/epidemiology , Yellow Fever/virology , Brazil/epidemiology , Disease Outbreaks , Sequence Alignment , Amino Acid Sequence , Genotype , Monkey Diseases/epidemiologyABSTRACT
Recombinant gene expression using adeno-associated viruses (AAVs) has become a valuable tool in animal studies, as they mediate safe expression of transduced genes for several months. The liver is a major organ of metabolism, and liver-specific expression of a gene can be an invaluable tool for metabolic studies. AAV-DJ is a recombinant AAV generated by the gene shuffling of various AAV serotypes and shares characteristics of AAV2 and AAV8. AAV-DJ contains a heparin-binding domain in its capsid, which suggests that a heparin column could be used for the purification of the AAV. Given that AAV-DJ has been only recently available, relatively little is known about the optimal preparation/purification and application of AAV-DJ. Here, we present a simple large-scale preparation method that can generate 3×10(13) viral particles for in vivo experiments and demonstrate liver-specific gene expression via systemic injection in mice.
Subject(s)
Animals , Humans , Mice , Capsid , Capsid Proteins/genetics , Dependovirus/genetics , Gene Expression , Genetic Vectors , Genome, Viral/genetics , Hep G2 Cells , Liver/metabolism , Mice, Inbred C57BLABSTRACT
Parvovirus B19 (B19V) infects individuals worldwide and is associated with an ample range of pathologies and clinical manifestations. B19V is classified into three distinct genotypes, all identified in Brazil. Here, we report a complete sequence of a B19V genotype 1A that was obtained by high-throughput metagenomic sequencing. This genome provides information that will contribute to the studies on B19V epidemiology and evolution.
Subject(s)
Child , Humans , Male , Genome, Viral/genetics , /genetics , Brazil , Fatal Outcome , High-Throughput Nucleotide Sequencing , /classification , Sequence Analysis, DNAABSTRACT
To assess the correlation between serum HBsAg titers and hepatitis B virus [HBV] DNA levels in patients with hepatitis B envelop antigen-negative [HBeAg -ve] HBV genotype-D [HBV/D] infection. A total of 106 treatment- nave, HBeAg -ve HBV/D patients were included; 78 in the inactive carrier [IC] state and 28 in the active hepatitis [AH] stage. HBV DNA load and HBsAg titers were tested using TaqMan real-time polymerase chain reaction [PCR] and automated chemiluminescent microparticle immunoassay, respectively. The median [range] log10 HbsAg titer was significantly lower in the IC group compared with AH group, 3.09 [-1 to -4.4] versus 3.68 [-0.77 to 5.09] IU/mL, respectively; P < 0.001. The suggested cutoff value of HBsAg titer to differentiate between the two groups was 3.79 log10 IU/mL. In addition, there was a significant positive correlation between HBsAg and HBV DNA levels in the whole cohort, AH, and IC groups [r = 0.6, P < 0.0001; r = 0.591, P = 0.001; and r = 0.243, P = 0.032, respectively]. Serum HBsAg titers may correlate with HBV DNA in treatment-nave HBeAg -ve HBV/D patients, and supports the use of HBsAg levels in clinical practice as a predictor of serum HBV DNA levels.
Subject(s)
Humans , Male , Female , Hepatitis B Surface Antigens/genetics , DNA, Viral/blood , Hepatitis B virus/immunology , Hepatitis B, Chronic/blood , Hepatitis B, Chronic/immunology , Genome, Viral/genetics , Viral Envelope ProteinsABSTRACT
The viral genome-linked protein (VPg) of Potyviruses is covalently attached to the 5’ end of the genomic RNA. Towards biophysical characterization, the VPg coding region of Cardamom mosaic virus (CdMV) was amplified from the cDNA and expressed in E. coli. Most of the expressed VPg aggregated as inclusion bodies that were solubilized with urea and refolded with L-arginine hydrochloride. The various forms of CdMV VPg (native, denatured and refolded) were purified and the conformational variations between these forms were observed with fluorescence spectroscopy. Native and refolded CdMV VPg showed unordered secondary structure in the circular dichroism (CD) spectrum. The model of CdMV VPg was built based on the crystal structure of phosphotriesterase (from Pseudomonas diminuta), which had the maximum sequence homology with VPg to identify the arrangement of conserved amino acids in the protein to study the functional diversity of VPg. This is the first report on the VPg of CdMV, which is classified as a new member of the Macluravirus genus of the Potyviridae family.
Subject(s)
Circular Dichroism , Elettaria/metabolism , Genome, Viral/genetics , Inclusion Bodies/genetics , Inclusion Bodies/metabolism , Models, Molecular , Mosaic Viruses/genetics , Mosaic Viruses/metabolism , Plant Viruses/genetics , Plant Viruses/metabolism , Potyvirus/genetics , Potyvirus/metabolism , Protein Refolding , Protein Structure, Secondary , RNA-Binding Proteins/chemistry , RNA-Binding Proteins/genetics , RNA-Binding Proteins/isolation & purification , RNA-Binding Proteins/metabolism , Viral Proteins/chemistry , Viral Proteins/genetics , Viral Proteins/metabolismABSTRACT
INTRODUCTION: Human cytomegalovirus is an opportunistic betaherpesvirus that causes persistent and serious infections in immunodeficient patients. Recurrent infections occur due to the presence of the virus in a latent state in some cell types. It is possible to examine the virus using molecular methods to aid in the immunological diagnosis and to generate a molecular viral profile in immunodeficient patients. The objective of this study was to characterize cytomegalovirus genotypes and to generate the epidemiological and molecular viral profile in immunodeficient patients. METHODS: A total of 105 samples were collected from immunodeficient patients from the City of Belém, including newborns, hemodialysis patients, transplant recipients and HIV+ patients. An IgG and IgM antibody study was completed using ELISA, and enzymatic analysis by restriction fragment length polymorphism (RFLP) was performed to characterize viral genotypes. RESULTS: It was observed that 100 percent of the patients had IgG antibodies, 87 percent of which were IgG+/IgM-, consistent with a prior infection profile, 13 percent were IgG+/IgM+, suggestive of recent infection. The newborn group had the highest frequency (27 percent) of the IgG+/IgM+ profile. By RFLP analysis, only one genotype was observed, gB2, which corresponded to the standard AD169 strain. CONCLUSIONS: The presence of IgM antibodies in new borns indicates that HCMV continues to be an important cause of congenital infection. The low observed genotypic diversity could be attributed to the small sample size because newborns were excluded from the RFLP analysis. This study will be continued including samples from newborns to extend the knowledge of the general and molecular epidemiology of HCMV in immunodeficient patients.
INTRODUÇÃO: O citomegalovírus é um betaherpesvírus oportunista, causador de infecções persistentes e graves em pacientes imunodeficientes. As infecções recorrentes ocorrem devido à presença do vírus em estado de latência, em alguns tipos celulares, o que possibilita a pesquisa viral por métodos moleculares para auxiliar nos diagnósticos imunológicos, assim como traçar o perfil epidemiológico e molecular viral em pacientes imunodeficientes. O objetivo deste estudo foi caracterizar os genótipos de citomegalovírus e traçar o perfil epidemiológico e molecular viral em pacientes imunodeficientes. MÉTODOS: Um total de 105 amostras foi coletado de pacientes imunodeficientes da Cidade de Belém, incluindo recém-nascidos, hemodialisados, transplantados e pacientes HIV+. Foi realizada a pesquisa de anticorpos IgG e IgM pelo método ELISA e análise enzimática pelo método restriction fragment length polymorphism (RFLP) para caracterização dos genótipos virais. RESULTADOS: Foi observado que 100 por cento dos pacientes apresentavam anticorpos IgG, 87 por cento eram IgG+/IgM-perfil de infecção pregressa; e 13 por cento IgG+/ IgM+ sugestivo de infecção recente. O grupo dos recém-nascidos apresentou maior frequência (27 por cento) do perfil IgG+/IgM+. Na análise por RFLP, foi observado um único genótipo, o gB2, que corresponde ao padrão genotípico da cepa AD169. CONCLUSÕES: A presença de anticorpos IgM nos recém-nascidos indica que o vírus CMV continua sendo causa importante de infecção congênita; a baixa diversidade genotípica pode ser atribuída ao tamanho amostral devido a exclusão dos recém-nascidos na análise por RFLP. Esse estudo será continuado incluindo amostras de recém-nascidos a fim de contribuir para um amplo conhecimento da epidemiologia geral e molecular do citomegalovírus em pacientes imunodeficientes da Cidade de Belém.
Subject(s)
Adult , Humans , Infant, Newborn , Cytomegalovirus Infections/virology , Cytomegalovirus/genetics , Genome, Viral/genetics , HIV Infections/immunology , Immunocompromised Host/immunology , Kidney Transplantation/immunology , Brazil , Dialysis , Immunoglobulin G/blood , Immunoglobulin M/blood , Restriction Mapping/methodsABSTRACT
INTRODUÇÃO: Os métodos de genotipagem do vírus da hepatite C têm sido muito discutidos. O objetivo deste trabalho foi comparar as metodologias de hibridização reversa e sequenciamento direto para a genotipagem do vírus da hepatite C. MÉTODOS: Noventa e uma amostras de plasma de pacientes assistidos na Faculdade de Medicina de Botucatu da Universidade Estadual Paulista foram utilizadas. A genotipagem por hibridização reversa foi realizada utilizando o kit comercial INNO-LiPA® v.1.0. O sequenciamento direto foi efetuado em sequenciador automático utilizando protocolos in house. RESULTADOS: A genotipagem por sequenciamento direto mostrou-se eficiente na resolução dos resultados inconclusivos pelo kit comercial. O kit mostrou resultados errôneos em relação à subtipagem viral. Além disso, a genotipagem por sequenciamento direto revelou um erro do kit com relação à determinação genotípica questionando a eficiência do método também para a identificação do genótipo viral. CONCLUSÕES: A genotipagem realizada por meio de sequenciamento direto permite uma maior acurácia na classificação viral quando comparada à hibridização reversa.
INTRODUCTION: The methods for genotyping the hepatitis C virus have been much discussed. The aim of this study was to compare the methodologies of reverse hybridization and direct sequencing for genotyping the hepatitis C virus. METHODS: Ninety-one plasma samples from patients attended at the Botucatu Medical School, São Paulo State University, were used. Genotyping by reverse hybridization was performed using the INNO-LiPA® v.1.0 commercial kit. Direct sequencing was performed in an automated sequencer using in-house protocols. RESULTS: Genotyping by direct sequencing was shown to be efficient for resolving cases that had remained inconclusive after using the commercial kit. The kit showed erroneous results in relation to virus subtyping. Moreover, direct sequencing revealed an error of the kit regarding the genotypic determination, thereby raising doubts about the efficiency of reverse hybridization for identifying the virus genotype. CONCLUSIONS: Genotyping by direct sequencing allowed greater accuracy of virus classification than did reverse hybridization.
Subject(s)
Humans , Genotype , Hepacivirus/genetics , Nucleic Acid Hybridization/genetics , Oligonucleotide Array Sequence Analysis/methods , /genetics , Genome, Viral/genetics , Hepacivirus/classification , Viral Nonstructural Proteins/geneticsABSTRACT
El virus de Epstein-Barr se encuentra en relación directa con algunas neoplasias como los linfomas y el carcinoma indiferenciado de nasofaringe. Más recientemente se han reportado la presencia del genoma viral en tumores similares a linfoepiteliomas de otras localizaciones como estómago, hígado, mama y pulmón. Fueron tomadas muestras en fresco de pacientes con tumores localizados en tracto aerodigestivo superior entre enero y junio de 2006. Se determinó el genoma viral. Dieciocho de 41 muestras eran positivas para virus, 23 negativas. Trece de los tumores malignos resultaron positivos para el genoma del virus mientras que el 48,1 por ciento restante resultaron negativos. La presencia del genoma viral fue encontrada en 8 muestras de laringe, 4 de nasofaringe, 2 de senos piriformes y en 1 de cada una de los siguientes sitios: fosas nasales, mucosa yugal, amígdala, y antro maxilar. A pesar del número limitado de muestras tomadas en algunas de las localizaciones mencionadas en este trabajo, pudimos encontrar el genoma viral en sitios como laringe, fosas nasales y cavidad oral. La mayor parte de los tumores malignos eran carcinomas escamosos, sólo 2 muestras correspondían a linfoepiteliomas. El genoma del virus puede ser identificado en muestras tomadas en fresco de tumores del tracto aerodigestivo superior tales como en carcinomas escamosos de laringe, fosas nasales, cavidad oral y faringe. Es necesario realizar más estudios para poder identificar la posible relación que existe entre este virus y dichos tumores.
The Epstein-Barr virus is been related with many malignancies as lymphoma and nasopharyngeal undifferentiated carcinoma. More recently, the presence of viral genome had been reported in some similar tumors how the lymphoepithelioma in other localizations for example the stomach, the liver, the breast and lung. From January to June 2006, we had taken fresh from the patients superior aero digestive tumors samples. The Epstein-Barr viral genome was determined by the Polymerasa Chain Reaction. From 41 samples of tumors, 18 were viruses positive and 23 of them were viruses negative. Thirteen malignant tumors were positive for the viruses genome and the rest ant other 48.1 % were negative. In eight larynxes, 4 nasopharyngeal, 2 piriform sinuses and some of this localization: nasal cavity, oral yugal mucosa, tonsil and maxillary sinus, and samples the viral genome of Epstein Barr was present. Although, we had a limited number of sample in some regions mentioned in these work, we could determine the viral genome of Epstein Barr in some sites how larynx, nasal and oral cavity. The majority of malignant tumors were squamous cell carcinoma, only two of them were correspondent to lymphoepithelioma. The Epstein-Barr viral genome may be identified in fresh superior aero digestive tumors samples, like in squamous cell carcinoma of the larynx, the oral cavity, nasal cavity and in the pharynx. Further studies are necessary to identify the probability relation between this virus and these tumors.
Subject(s)
Humans , Male , Female , Middle Aged , Genome, Viral/genetics , /immunology , Nasopharynx/injuries , Head and Neck Neoplasms/surgery , Head and Neck Neoplasms/pathology , Alcoholism/etiology , Carcinoma/diagnosis , Lymphoma/diagnosis , Medical Oncology , Tobacco Use Disorder/adverse effectsABSTRACT
INTRODUCTION: Prolonged survival of patients under HAART has resulted in new demands for assisted reproductive technologies. HIV serodiscordant couples wish to make use of assisted reproduction techniques in order to avoid viral transmission to the partner or to the newborn. It is therefore essential to test the effectiveness of techniques aimed at reducing HIV and HCV loads in infected semen using molecular biology tests. METHODS: After seminal analysis, semen samples from 20 coinfected patients were submitted to cell fractioning and isolation of motile spermatozoa by density gradient centrifugation and swim-up. HIV and HCV RNA detection tests were performed with RNA obtained from sperm, seminal plasma and total semen. RESULTS: In pre-washing semen, HIV RNA was detected in 100 percent of total semen samples, whereas HCV RNA was concomitantly amplified in only one specimen. Neither HIV nor HCV were detected either in the swim-up or in the post-washing semen fractions. CONCLUSIONS: Reduction of HIV and/or HCV shedding in semen by density gradient centrifugation followed by swim-up is an efficient method. These findings lead us to believe that, although semen is rarely found to contain HCV, semen processing is highly beneficial for HIV/HCV coinfected individuals.
O aumento da sobrevida dos pacientes que utilizam terapêutica antiretroviral altamente eficaz (HAART- Highly Active Antiretroviral Therapy) trouxe uma nova demanda de casais sorodiscordantes que desejam filhos. Como esses casais não podem abandonar o uso de preservativos, torna-se indispensável tratar o sêmen infectado com técnicas laboratoriais eficazes que além de isolar os melhores espermatozóides, reduzam a carga viral do HIV e HCV a níveis indetectáveis. Para isso, são utilizadas técnicas de semen washing, associadas a testes ultra sensíveis de biologia molecular. Após análise seminal, sêmen de 20 pacientes co-infectados HIV-HCV foram submetidos a fracionamento celular e isolamento de espermatozóides móveis através de método de densidade de gradiente descontínuo e swim-up. Posteriormente, testes para detecção do RNA do HIV e HCV foram aplicados nos sêmens totais e frações seminais obtidas. Em fase pré semen washing, o HIV foi detectado em 100 por cento dos semens totais. Contrariamente, o HCV foi detectado em apenas uma amostra. Em fase pós semen washing, o HIV e HCV não foram detectados em nenhuma das frações seminais. A redução do HIV e do HCV através de semen washing mostra-se um método eficaz a indivíduos co-infectados HIV-HCV, apesar do encontro do HCV no sêmen ser raro.
Subject(s)
Humans , Male , Adult , Middle Aged , HIV , Hepacivirus/isolation & purification , RNA, Viral/analysis , Semen/virology , Spermatozoa/virology , Cell Separation , Centrifugation, Density Gradient , Genome, Viral/genetics , HIV , HIV Infections/prevention & control , HIV Infections/virology , Hepacivirus/genetics , Hepatitis C/prevention & control , Hepatitis C/virology , Reproductive Techniques, Assisted , Reverse Transcriptase Polymerase Chain Reaction , Viral LoadABSTRACT
Calves born persistently infected with non-cytopathic bovine viral diarrhea virus (ncpBVDV) frequently develop a fatal gastroenteric illness called mucosal disease. Both the original virus (ncpBVDV) and an antigenically identical but cytopathic virus (cpBVDV) can be isolated from animals affected by mucosal disease. Cytopathic BVDVs originate from their ncp counterparts by diverse genetic mechanisms, all leading to the expression of the non-structural polypeptide NS3 as a discrete protein. In contrast, ncpBVDVs express only the large precursor polypeptide, NS2-3, which contains the NS3 sequence within its carboxy-terminal half. We report here the investigation of the mechanism leading to NS3 expression in 41 cpBVDV isolates. An RT-PCR strategy was employed to detect RNA insertions within the NS2-3 gene and/or duplication of the NS3 gene, two common mechanisms of NS3 expression. RT-PCR amplification revealed insertions in the NS2-3 gene of three cp isolates, with the inserts being similar in size to that present in the cpBVDV NADL strain. Sequencing of one such insert revealed a 296-nucleotide sequence with a central core of 270 nucleotides coding for an amino acid sequence highly homologous (98 percent) to the NADL insert, a sequence corresponding to part of the cellular J-Domain gene. One cpBVDV isolate contained a duplication of the NS3 gene downstream from the original locus. In contrast, no detectable NS2-3 insertions or NS3 gene duplications were observed in the genome of 37 cp isolates. These results demonstrate that processing of NS2-3 without bulk mRNA insertions or NS3 gene duplications seems to be a frequent mechanism leading to NS3 expression and BVDV cytopathology.
Subject(s)
Animals , Cattle , Cytopathogenic Effect, Viral/genetics , Diarrhea Viruses, Bovine Viral/genetics , Gene Duplication , Genome, Viral/genetics , Viral Nonstructural Proteins/genetics , Amino Acid Sequence , Diarrhea Viruses, Bovine Viral/isolation & purification , Gene Rearrangement , Molecular Sequence Data , Reverse Transcriptase Polymerase Chain Reaction , RNA, Viral/geneticsABSTRACT
Rotaviruses are the major cause of acute gastroenteritis in infants world-wide. The genome consists of eleven double stranded RNA segments. The major segment encodes the structural protein VP1, the viral RNA-dependent RNA polymerase (RdRp), which is a minor component of the viral inner core. This study is a detailed bioinformatic assessment of the VP1 sequence. Using various methods we have identified canonical motifs within the VP1 sequence which correspond to motifs previously identified within RdRps of other positive strand, double-strand RNA viruses. The study also predicts an overall structural conservation in the middle region that may correspond to the palm subdomain and part of the fingers and thumb subdomains, which comprise the polymerase core of the protein. Based on this analysis, we suggest that the rotavirus replicase has the minimal elements to function as an RNA-dependent RNA polymerase. VP1, besides having common RdRp features, also contains large unique regions that might be responsible for characteristic features observed in the Reoviridae family.
Subject(s)
Animals , Genome, Viral/genetics , RNA-Dependent RNA Polymerase/genetics , Rotavirus/genetics , Viral Core Proteins/genetics , Cell Line , Computational Biology/methods , Macaca mulatta , Predictive Value of TestsABSTRACT
A partir das primeiras sequências genômicas do Cil V-C (Citrus leprosis virus tipo citoplasmático) através de bibliotecas de cDNA provenientes do produto da replicação viral (dsRNA) (locali, 2002), foi possível concluir o seqüenciamento completo do seu genoma. As informações obtidas possibilitaram caracterizá-lo como um vírus de genoma constituído por ssRNA (mais), bipartido (menos 14 Kb), contendo no RNA 1 duas ORFs, uma delas codificadora de uma poliproteína com três domínios envolvidos com replicase viral e um relacionado com protease. No RNA 2, foram detectadas quatro ORFs, uma delas codificadora da proteína de movimento. Foram identificadas caudas poli A nas extremidades 3 dos dois RNAs, bem como a presença de uma sequência conservada de nucleotídeos (GAUAAAUCU) nas extremidades 5 dos dois RNAs, sugerindo a presença de uma estrutura Cap. As informações até então conhecidas sobre o vírus associado à leprose dos citros e aos ácaros do gênero Brevipalpus os relacionavam à família Rhabdoviridae. Entretanto, através de análises estruturais e organizacionais do genoma do CilV-C ficou evidente que o vírus apresenta alguns (poucos) domínios conservados com membros de vários gêneros e famílias de fitovírus, mas não com rhabdovírus. Através de análises filogenéticas e associando estas informações às características morfológicas do virion, além dos efeitos citopáticos e sintomas induzidos por esses vírus em seus hospedeiros, sugerimos que o CilV-C seja considerado o membro-tipo de um novo gênero de vírus, denominado Cilevirus. Foi possível também determinar com segurança que ele não pertence a família Rhabdoviridae, como proposto anteriormente. Essas informações permitiram uma análise comparativa entre regiões genômicas do CilV-C com as de outros vírus transmitidos por Brevipa/pus (VTBs), entre eles, Orchid fleck virus - OFV, Coffee ringspot virus - CoRSV, e Ligustrum ringspot virus - LigRSV.
Subject(s)
Citrus/genetics , Genes/physiology , Genome, Viral/physiology , Genome, Viral/geneticsABSTRACT
Una sonda específica para la detección de genomas del VHD fue desarrollada a partir del plásmido recombinante pa-1. La sonda fue marcada mediante un método no isotópico, lo cual permite el almacenaje prolongado de la misma