Colibacilose em carneiros é associada à enterotoxina termo-estável do tipo I em uma propriedade rural do estado de São Paulo, Brasil

Twenty seven (48.2%) culture supernatants of 56 Escherichia coli isolated from diarrheic lamb feces (7 to 10 days old) in São Paulo State, Brazil, presented positive results to suckling mice assay (fluid accumulation) but none caused cytopathic effects on Vero and CHO cells, indicating that these strains did not produced LT or VT toxins. PCR assays showed that these 27 E. coli strains harbored estA, that codifies for STa, but not for stx1, stx2 or cnf genes. The positive STa strains were checked for genes that codify for F41, F17 and K99 fimbriae, wich are considered colonization factors in ETEC. Only F17 was detect in two samples (7.4%). Twelve of 27 STa positive carried hlyA gene and presented hemolytic activity in blood Agar. Presence of rotavirus was not detected among the diarrheic feces. These data suggests that STa must be an important diarrheagenic factor to small ruminants in São Paulo State425854857COORDENAÇÃO DE APERFEIÇOAMENTO DE PESSOAL DE NÍVEL SUPERIOR - CAPESFUNDAÇÃO DE AMPARO À PESQUISA DO ESTADO DE SÃO PAULO - FAPESPsem informaçãoCinquenta e seis Escherichia coli isoladas de fezes diarreicas de carneiros (7 a 10 dias) no Estado de São Paulo, Brasil, foram avaliadas quando ao acúmulo de fluidos no intestino de camundongos recém-nascidos. Vinte e sete (48,2%) das amostras foram positivas para esse ensaio, porém nenhuma das 56 amostras foi capaz de induzir efeitos citopáticos em células Vero e CHO, indicando que não produzem toxinas LT ou VT. Análise por PCR mostrou que estas 27 E. coli foram positivas para estA, que codifica a proteína STa, mas não para os genes stx1, stx2 ou cnf. As amostras positivas para STa foram também analisadas quanto à presença dos genes que codificam as fímbrias F41, F17 e K99, fatores de colonização em ETEC. Somente F17 foi detectada em 2 amostras (7,4%). Doze das 27 E. coli STa positivas também contêm o gene hlyA e apresentaram atividade hemolítica em Agar sangue. Rotavírus não foi detectado nas fezes desses animais. Em conjunto, esses resultados sugerem que STa é um fator diarreiogênico importante para colibacilose de pequenos ruminantes no Estado de São Paul

Colibacilose em carneiros é associada à enterotoxina termo-estável do tipo I em uma propriedade rural do estado de São Paulo, Brasil

Twenty seven (48.2%) culture supernatants of 56 Escherichia coli isolated from diarrheic lamb feces (7 to 10 days old) in São Paulo State, Brazil, presented positive results to suckling mice assay (fluid accumulation) but none caused cytopathic effects on Vero and CHO cells, indicating that these strains did not produced LT or VT toxins. PCR assays showed that these 27 E. coli strains harbored estA, that codifies for STa, but not for stx1, stx2 or cnf genes. The positive STa strains were checked for genes that codify for F41, F17 and K99 fimbriae, wich are considered colonization factors in ETEC. Only F17 was detect in two samples (7.4%). Twelve of 27 STa positive carried hlyA gene and presented hemolytic activity in blood Agar. Presence of rotavirus was not detected among the diarrheic feces. These data suggests that STa must be an important diarrheagenic factor to small ruminants in São Paulo State.Cinquenta e seis Escherichia coli isoladas de fezes diarreicas de carneiros (7 a 10 dias) no Estado de São Paulo, Brasil, foram avaliadas quando ao acúmulo de fluidos no intestino de camundongos recém-nascidos. Vinte e sete (48,2%) das amostras foram positivas para esse ensaio, porém nenhuma das 56 amostras foi capaz de induzir efeitos citopáticos em células Vero e CHO, indicando que não produzem toxinas LT ou VT. Análise por PCR mostrou que estas 27 E. coli foram positivas para estA, que codifica a proteína STa, mas não para os genes stx1, stx2 ou cnf. As amostras positivas para STa foram também analisadas quanto à presença dos genes que codificam as fímbrias F41, F17 e K99, fatores de colonização em ETEC. Somente F17 foi detectada em 2 amostras (7,4%). Doze das 27 E. coli STa positivas também contêm o gene hlyA e apresentaram atividade hemolítica em Agar sangue. Rotavírus não foi detectado nas fezes desses animais. Em conjunto, esses resultados sugerem que STa é um fator diarreiogênico importante para colibacilose de pequenos ruminantes no Estado de São Paulo.854857Fundação de Amparo à Pesquisa do Estado de São Paulo (FAPESP)Coordenação de Aperfeiçoamento de Pessoal de Nível Superior (CAPES

Colibacillosis in lambs is associated to type I heat-stable enterotoxin in a farm in Sao Paulo State, Brazil

Twenty seven (48.2%) culture supernatants of 56 Escherichia coli isolated from diarrheic lamb feces (7 to 10 days old) in Sao Paulo State, Brazil, presented positive results to suckling mice assay (fluid accumulation) but none caused cytopathic effects on Vero and CHO cells, indicating that these strains did not produced LT or VT toxins. PCR assays showed that these 27 E. coli strains harbored estA, that codifies for STa, but not for stx1, stx2 or cnf genes. The positive STa strains were checked for genes that codify for F41, F17 and K99 fimbriae, wich are considered colonization factors in ETEC. Only F17 was detect in two samples (7.4%). Twelve of 27 STa positive carried hlyA gene and presented hemolytic activity in blood Agar. Presence of rotavirus was not detected among the diarrheic feces. These data suggests that STa must be an important diarrheagenic factor to small ruminants in Sao Paulo State.Coordenacao de Aperfeicoamento de Pessoal de Nivel Superior (CAPES)Coordenacao de Aperfeicoamento de Pessoal de Nivel Superior (CAPES)Fundacao de Amparo a Pesquisa do Estado de Sao Paulo (FAPESP)Fundacao de Amparo a Pesquisa do Estado de Sao Paulo (FAPESP

ATLANTIC EPIPHYTES: a data set of vascular and non-vascular epiphyte plants and lichens from the Atlantic Forest

Epiphytes are hyper-diverse and one of the frequently undervalued life forms in plant surveys and biodiversity inventories. Epiphytes of the Atlantic Forest, one of the most endangered ecosystems in the world, have high endemism and radiated recently in the Pliocene. We aimed to (1) compile an extensive Atlantic Forest data set on vascular, non-vascular plants (including hemiepiphytes), and lichen epiphyte species occurrence and abundance; (2) describe the epiphyte distribution in the Atlantic Forest, in order to indicate future sampling efforts. Our work presents the first epiphyte data set with information on abundance and occurrence of epiphyte phorophyte species. All data compiled here come from three main sources provided by the authors: published sources (comprising peer-reviewed articles, books, and theses), unpublished data, and herbarium data. We compiled a data set composed of 2,095 species, from 89,270 holo/hemiepiphyte records, in the Atlantic Forest of Brazil, Argentina, Paraguay, and Uruguay, recorded from 1824 to early 2018. Most of the records were from qualitative data (occurrence only, 88%), well distributed throughout the Atlantic Forest. For quantitative records, the most common sampling method was individual trees (71%), followed by plot sampling (19%), and transect sampling (10%). Angiosperms (81%) were the most frequently registered group, and Bromeliaceae and Orchidaceae were the families with the greatest number of records (27,272 and 21,945, respectively). Ferns and Lycophytes presented fewer records than Angiosperms, and Polypodiaceae were the most recorded family, and more concentrated in the Southern and Southeastern regions. Data on non-vascular plants and lichens were scarce, with a few disjunct records concentrated in the Northeastern region of the Atlantic Forest. For all non-vascular plant records, Lejeuneaceae, a family of liverworts, was the most recorded family. We hope that our effort to organize scattered epiphyte data help advance the knowledge of epiphyte ecology, as well as our understanding of macroecological and biogeographical patterns in the Atlantic Forest. No copyright restrictions are associated with the data set. Please cite this Ecology Data Paper if the data are used in publication and teaching events. © 2019 The Authors. Ecology © 2019 The Ecological Society of Americ

Genetic characterization of picobirnaviruses detected in fecal samples from different hosts

Orientador: Maria Silvia Viccari GattiTese (doutorado) - Universidade Estadual de Campinas, Instituto de BiologiaResumo: Picobirnavírus (PBV) pertencem à família Picobirnaviridae, gênero Picobirnavirus e têm como espécie tipo Human picobirnavirus e Rabbit picobirnavirus. Estes pequenos vírus não envelopados, de dois segmentos genômicos de RNA dupla fita, são encontrados em amostras de fezes diarreicas ou não de diferentes hospedeiros mamíferos, incluindo o homem, aves e répteis. Os mecanismos da infecção por PBV e sua associação a gastroenterites ainda não estão esclarecidos, mas são colocados como agentes emergentes e oportunistas e seu potencial zoonótico foi sugerido. As técnicas utilizadas para a identificação desses vírus são: eletroforese em gel de poliacrilamida (EGPA) e RT-PCR. A primeira permite diferenciar os PBV pelas diferenças de migração dos seus segmentos genômicos. Já na RT-PCR são sete os pares de iniciadores descritos, incluindo aqueles que permitem sua diferenciação em genogrupo I ou II. Este projeto objetivou caracterizar genética e filogeneticamente PBV de diferentes hospedeiros naturais e as estratégias utilizadas foram o sequenciamento total e parcial dos segmentos genômicos de PBV e a definição de uma região conservada para o desenho de iniciadores capazes de diagnosticar todos os PBV por RT-PCR. Foram analisadas para a presença de PBV amostras de fezes de suínos, coelhos, ratos, cães, cobras, ratos silvestres, capivaras, cavalos e bovinos. Utilizando a EGPA, PBV foram identificados em todos os hospedeiros estudados e pela RT-PCR identificou-se genogrupo I de PBV em quase todos, com exceção de capivaras e bovinos. O genogrupo II não foi identificado. A circulação do genogrupo I em diferentes hospedeiros sugere que não existe especificidade genogrupo-espécie de hospedeiro. O sequenciamento parcial do segmento menor dos PBV identificados em cães, cobra e ratos mostrou uma relativa homologia principalmente com sequências de PBV identificados em humanos. A coexistência de duas ou mais populações de PBV em um mesmo hospedeiro foi identificada em cavalos, suínos, rato, rato silvestre e coelho a partir do sequenciamento parcial do segmento menor após clonagem, sugerindo um possível mecanismo de reassortment, o que pode levar a salto entre espécies. Esses resultados suportam o potencial emergente e zoonótico dos PBV. A heterogeneidade nas sequências de nucleotídeos verificada por esse sequenciamento sugere a presença de quasiespécies de PBV nesses hospedeiros. A menor variação observada nas sequências de nucleotídeos de PBV identificados em animais não confinados pode ser justificada pela tendência ao menor contato entre esses animais do que entre os de cativeiro, fazendo com que a transmissão viral também seja menor. Foi proposta uma padronização para a nomenclatura dos PBV, baseada em seu hospedeiro, país e ano de identificação. O atual sistema de classificação para os PBV não é apropriado, devido à identificação de PBV não pertencentes a nenhum dos genogrupos já descritos e à presença de heterogeneidade nas sequências de PBV do genogrupo I. Infelizmente, não foi possível sequenciar o genoma completo dos PBV estudados, não sendo identificada nenhuma sequência conservada que permitisse o desenho de iniciadores capazes de unificar o diagnóstico dos PBV. Estudos tentativos estão em andamento para que, a partir do sequenciamento completo e análise do genoma de diferentes PBV, seja possível definir as porcentagens de identidade mínimas para sua classificação em genogrupos e/ou genotiposAbstract: Picobirnaviruses (PBV) belong to the Picobirnaviridae family, genus Picobirnavirus, and Human picobirnavirus and Rabbit picobirnavirus are the type species. These small non-enveloped viruses, with two genetic segments of double-stranded RNA, can be found in diarrheic or nondiarrheic fecal samples from different hosts like mammals, including humans, birds and reptiles. PBV infection and its association with gastroenteritis are still unknown, but they are considered opportunistic and emergent pathogens, and their zoonotic potential has also been suggested. Techniques for PBV identification include: polyacrylamide gel electrophoresis (PAGE) and RTPCR. The first one allows characterization of PBV according to the migration pattern of their genomic segments. In the RT-PCR, seven primers' pairs have been designed, including one that allows classification of PBV into genogroups I or II. The aim of this project was the genetic and phylogenetic characterization of PBV identified in fecal samples from different natural hosts by complete and partial sequencing of PBV genomic segments and set up of a conserved region for designing primers able to detect all PBV by RT-PCR. Fecal samples from pigs, rabbits, rats, dogs, snakes, wild rats, capybaras, horses and cattle were analyzed for PBV occurrence. PBV were identified in all studied hosts by PAGE and genogroup I was identified in the majority of them by RT-PCR, except in capybaras and cattle. Genogroup II was not identified. Genogroup I circulation in different hosts suggests that there is no genogroup-host species' specificity. Partial sequencing of small PBV's genomic segment identified in fecal samples from dogs, snake and rats showed homology mainly to human PBV sequences. Coexistence of two or more PBV population in the same host could be determined in fecal samples from horses, pigs, rat, wild rat and rabbit by partial sequencing of small PBV's genomic segment after cloning, suggesting that reassortment may occur in nature, allowing host species jump. These results support the emergent and zoonotic potential of PBV. The heterogeneity found in PBV's nucleotide sequences after cloning suggests the existence of PBV quasispecies in these hosts. The little variation in nucleotide sequences of PBV identified in hosts living in an open environment could be justified by a tendency of less contact among these animals, allowing less viral spread. The classification system used nowadays is cannot be considered appropriated as it doesn't consider the heterogeneity found in PBV's genogroup I sequences. Also, PBV that don't belong to any of the described genogroups, remain with no classification. Therefore, a new standard nomenclature for PBV, based on its host, country and year of identification was proposed. Unfortunately, it was not possible to sequence the complete genome of PBV found in this study. Also, no conserved sequence could be identified for primers' design, which would be capable of standardized PBV detection. Additional studies are ongoing to try to define nucleotide sequences identity percentages for genogroups and/or genotypes classificationDoutoradoMicrobiologiaDoutor em Genetica e Biologia Molecula

Nomenclature Proposal For Picobirnavirus.

Picobirnaviruses have been identified in the feces of a broad range of hosts by several international research groups. Because there is no standard nomenclature for these viruses, we propose a clear and unique name for each strain.1541953-

Molecular Characterization Of Picobirnaviruses From New Hosts.

Picobirnaviruses (PBVs) have recently been classified into the Picobirnaviridae family. They are small, non-enveloped viruses with bisegmented, double-stranded (ds) RNA genomes. Although they are found in the feces of a broad range of hosts, information regarding their genomes is limited to viruses detected from humans, rabbits, and porcine. Identification of PBVs has been done using PAGE and reverse transcription PCR (RT-PCR). In this study, we present a phylogenetic analysis of PBVs detected in the feces of dogs, snakes, and rats. In addition, we compare these strains to those from human and porcine hosts. To do so, 487 fecal specimens from dogs, snakes and rats were analyzed by PAGE. The positive specimens for PBV were tested by RT-PCR using primers for genogroup I of the PBVs. From the 11 genogroup I PBV samples, at least one from each host was sequenced and submitted for phylogenetic analysis. All of the sequences showed high homology with the human and porcine genogroup I PBV sequences. In this study we report the first detection of PBVs in snakes (8.5%). We also report a phylogenetic analysis that goes beyond humans and pigs to include dogs, rats, and snakes. However, more hosts must be included in the analysis so that we may reach better conclusions regarding the spread of these viruses.143134-

Molecular Characterisation Of The Nsp4 Gene Of Group A Human Rotavirus G2p[4] Strains Circulating In São Paulo, Brazil, From 1994 And 2006 To 2010.

Group A human rotaviruses (HuRVA) are causative agents of acute gastroenteritis. Six viral structural proteins (VPs) and six nonstructural proteins (NSPs) are produced in RV-infected cells. NSP4 is a diarrhoea-inducing viral enterotoxin and NSP4 gene analysis revealed at least 15 (E1-E15) genotypes. This study analysed the NSP4 genetic diversity of HuRVA G2P[4] strains collected in the state of São Paulo (SP) from 1994 and 2006-2010 using reverse transcription-polymerase chain reaction, sequencing and phylogenetic analysis. Forty (97.6%) G2P[4] strains displayed genotype E2; one strain (2.4%) displayed genotype E1. These results are consistent with the proposed linkage between VP4/VP7 (G2P[4]) and the NSP4 (E2) genotype of HuRVA. NSP4 phylogenetic analysis showed distinct clusters, with grouping of most strains by their genotype and collection year, and most strains from SP were clustered together with strains from other Brazilian states. A deduced amino acid sequence alignment for E2 showed many variations in the C-terminal region, including the VP4-binding domain. Considering the ability of NSP4 to generate host immunity, monitoring NSP4 variations, along with those in the VP4 or VP7 protein, is important for evaluating the circulation and pathogenesis of RV. Finally, the presence of one G2P[4]E1 strain reinforces the idea that new genotype combinations emerge through reassortment and independent segregation.110786-79

Prevalence of enteropathogens in normal feces from healthy children at an infant day care in Brazil

Introduction: The diarrhea associated with gastroenteritis is a major cause of morbidity and mortality worldwide, affecting mainly infants. The characterization of both viral and bacterial agents associated with gastroenteritis can establish policies for surveillance, prevention and treatment of infections. Group A rotaviruses are the major infectious agent associated with dehydration in children, followed by pathotypes of Escherichia coli. There are three main types of clinical infections caused by E. coli strains that have acquired virulence genes: (i) enteric and diarrheal diseases, (ii) urinary tract infections, and (iii) sepsis and meningitis. Methodology: In this study, the objective was to identify the presence of rotavirus and diarrhogenic E. coli in the feces of children 4 to 14 months of age who displayed no gastroenteritis symptoms and stayed all day in a day-care center. We analyzed 188 samples using PAGE and PCR to identify rotaviruses and E. coli virulence genes, respectively. Results: Thirty-six samples (19.1%) were positive for at least one pathotype of E. coli. Nineteen were identified to be of the EPEC group and fifteen of the EAEC group. Rotaviruses were not identified. Conclusions: As EPEC and EAEC are potential pathogens for children less than one year of age or immunocompromised individuals, our results show the importance of appropriate monitoring by public health agencies. In the situation that we have studied, children can be considered asymptomatic carriers of these pathogens and can transmit them to other susceptible children.6217618