Yellow Fever 17DD Vaccine Virus Infection Causes Detectable Changes in Chicken Embryos

Manso, Pedro Paulo de Abreu; Oliveira, Barbara Cristina Euzébio Pereira Dias de; Sequeira, Patrícia Carvalho de; Souza, Yuli Rodrigues Maia de; Ferro, Jessica Maria dos Santos; Silva, Igor José da; Caputo, Luzia Fátima Gonçalves; Guedes, Priscila Tavares; Santos, Alexandre Araújo Cunha dos; Freire, Marcos da Silva; Bonaldo, Myrna C.; Pelajo-Machado, Marcelo

doi:10.1371/journal.pntd.0004064

Cited by 4 publications

(10 citation statements)

References 49 publications

(71 reference statements)

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“…Specific pathogen-free (SPF) fertilized White Leghorn chicken eggs ( Gallus gallus domesticus ; Linnaeus, 1758) were obtained from the YF vaccine production unit (Fiocruz). There, eggs were infected in the yolk sac with 17DD EPlow virus seed lot (1–5 x 10 3 PFU per inoculum) on the ninth day of development [ 4 , 8 – 10 ]. Eggs were kept in an IP70 brooder (Premium Ecologica, Brazil) with controlled temperature at 37.5°C, and 55% relative humidity.…”

Section: Methodsmentioning

confidence: 99%

“…Sections of all paraffin blocks from three infected animals and three control embryo specimens per point of infection were submitted to immunofluorescence assay, as previously described [ 8 ], with a mouse polyclonal anti-yellow fever virus antibody (Evandro Chagas Institute). Double staining was performed in some samples with an anti-desmin antibody (cat.…”

Section: Methodsmentioning

confidence: 99%

“…RNA samples were extracted from formalin-fixed, paraffin-embedded tissue (FFPE). RNA was extracted from the same blocks in the immunofluorescence analysis, which were either positive or negative to the YF 17DD virus, as previously described [ 8 ]. Samples eluted after the procedure were amplified by reverse transcription-PCR (Thermoscript RT-PCR kit—cat.…”

Section: Methodsmentioning

confidence: 99%

“…11146016, Life Technologies, USA) with universal Flavivirus Yellow Fever primers (YF1–5`GGTCTCCTCTAACCTCTAG 3`and YF3- 5`GAGTGGATGACCACGGAAGACATGC 3`) [ 13 ]. Afterwards, a second amplification was carried out with yellow fever internal primers previously designed by our group [ 8 ] (YF2–5`CGAGTTTTGCCACTGCTAAGCT 3`and YF4–5`TAGACCCCGTCTTTCTACCACC 3`). Two different protocols were adopted with specific primers in RT-PCR using forward and reverse YF-1 and YF-3 primers to detect the genomic and replicative intermediate RNA.…”

Section: Methodsmentioning

confidence: 99%

“…Recently, our group [ 8 ] demonstrated by molecular techniques and immunofluorescence assays that the YFV 17DD replicates mainly in skeletal muscle tissue, and also in the nervous system, fibroblast cells and cardiomyocytes of White Legorn SPF chicken embryos at 72 hours post infection, representing a similar condition employed in yellow fever vaccine manufacture. It was possible to observe for the first time the histopathological alterations in this model and to determinate that muscle tissue could be the major site of virus replication.…”

Section: Introductionmentioning

confidence: 99%

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Kinetic Study of Yellow Fever 17DD Viral Infection in Gallus gallus domesticus Embryos

et al. 2016

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Yellow fever continues to be an important epidemiological problem in Africa and South America even though the disease can be controlled by vaccination. The vaccine has been produced since 1937 and is based on YFV 17DD chicken embryo infection. However, little is known about the histopathological background of virus infection and replication in this model. Here we show by morphological and molecular methods (brightfield and confocal microscopies, immunofluorescence, nested-PCR and sequencing) the kinetics of YFV 17DD infection in chicken embryos with 9 days of development, encompassing 24 to 96 hours post infection. Our principal findings indicate that the main cells involved in virus production are myoblasts with a mesenchymal shape, which also are the first cells to express virus proteins in Gallus gallus embryos at 48 hours after infection. At 72 hours post infection, we observed an increase of infected cells in embryos. Many sites are thus affected in the infection sequence, especially the skeletal muscle. We were also able to confirm an increase of nervous system infection at 96 hours post infection. Our data contribute to the comprehension of the pathogenesis of YF 17DD virus infection in Gallus gallus embryos.

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Section: Methodsmentioning

confidence: 99%

Section: Methodsmentioning

confidence: 99%

Section: Methodsmentioning

confidence: 99%

Section: Methodsmentioning

confidence: 99%

Section: Introductionmentioning

confidence: 99%

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Kinetic Study of Yellow Fever 17DD Viral Infection in Gallus gallus domesticus Embryos

et al. 2016

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Sonic Hedgehog signaling and Gli-1 during embryonic chick myogenesis

Teixeira

Rosa

Brito

et al. 2018

Biochemical and Biophysical Research Communications

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Generation of Yellow Fever virus vaccine in skeletal muscle cells of chicken embryos

Souza

Manso

Oliveira

et al. 2019

Mem. Inst. Oswaldo Cruz

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BACKGROUND The Yellow Fever (YF) vaccine is produced by the inoculation of embryonated chicken eggs with YF17DD virus on the ninth day of development. Full embryos are collected on the twelfth day of development for vaccine formulation. Skeletal muscle tissue is the main site where biosynthesis of viral particles occurs.OBJECTIVES This study aimed to analyse the experimental infection of skeletal muscle cells of chicken embryos by the 17DD Yellow Fever virus (YFV) in vivo and in vitro.METHODS Chicken embryos infected with YF17DD virus were analysed by immunofluorescence using confocal and super-resolution microscopes. Primary cultures of skeletal muscle cells of non-infected chicken embryos were evaluated for susceptibility and permissiveness to YF17DD virus using different protocols. This evaluation was performed based on morphological, viral titration, molecular biology, and colorimetric techniques.FINDINGS The present work phenotypically characterises embryonic chicken skeletal muscle cells as myogenic precursors expressing the Pax7 transcription factor in some cases. We demonstrated that these cells are susceptible to in vitro infection at different multiplicities of infection (MOIs), reproducing the same infection pattern observed in vivo. Furthermore, myogenic precursors and myoblasts are preferred infection targets, but establishment of infection does not depend on the presence of these cells. The peak of viral production occurred at 48 hpi, with decay occurring 72 hpi, when the cytopathic effect can be observed.MAIN CONCLUSIONS In conclusion, the primary culture of chicken skeletal muscle cells is a good model for studying muscle cells infected with YF17DD virus. This culture system displays satisfactory emulation of the in vitro phenomenon observed, contributing to our understanding of virus infection dynamics and leading to the development of alternative methods of vaccine production.

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Yellow Fever 17DD Vaccine Virus Infection Causes Detectable Changes in Chicken Embryos

Cited by 4 publications

References 49 publications

Kinetic Study of Yellow Fever 17DD Viral Infection in Gallus gallus domesticus Embryos

Kinetic Study of Yellow Fever 17DD Viral Infection in Gallus gallus domesticus Embryos

Sonic Hedgehog signaling and Gli-1 during embryonic chick myogenesis

Generation of Yellow Fever virus vaccine in skeletal muscle cells of chicken embryos

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