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Optimizing PCR Detection of West Nile Virus from Body Fluid Specimens to Delineate Natural History in an Infected Human Cohort

West Nile virus (WNV), a mosquito-borne arbovirus, remains a major global health concern. In this study, we optimized PCR methods then assessed serially-collected whole blood (WB), urine (UR), saliva, and semen specimens from a large cohort of WNV-positive participants to evaluate the natural histor...

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Autores principales: Gorchakov, Rodion, Gulas-Wroblewski, Bonnie E., Ronca, Shannon E., Ruff, Jeanne C., Nolan, Melissa S., Berry, Rebecca, Alvarado, R. Elias, Gunter, Sarah M., Murray, Kristy O.
Formato: Online Artículo Texto
Lenguaje:English
Publicado: MDPI 2019
Materias:
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC6514913/
https://www.ncbi.nlm.nih.gov/pubmed/31010160
http://dx.doi.org/10.3390/ijms20081934
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author Gorchakov, Rodion
Gulas-Wroblewski, Bonnie E.
Ronca, Shannon E.
Ruff, Jeanne C.
Nolan, Melissa S.
Berry, Rebecca
Alvarado, R. Elias
Gunter, Sarah M.
Murray, Kristy O.
author_facet Gorchakov, Rodion
Gulas-Wroblewski, Bonnie E.
Ronca, Shannon E.
Ruff, Jeanne C.
Nolan, Melissa S.
Berry, Rebecca
Alvarado, R. Elias
Gunter, Sarah M.
Murray, Kristy O.
author_sort Gorchakov, Rodion
collection PubMed
description West Nile virus (WNV), a mosquito-borne arbovirus, remains a major global health concern. In this study, we optimized PCR methods then assessed serially-collected whole blood (WB), urine (UR), saliva, and semen specimens from a large cohort of WNV-positive participants to evaluate the natural history of infection and persistent shedding of WNV RNA. Viral RNA extraction protocols for frozen WB and UR specimens were optimized and validated through spiking experiments to maximize recovery of viral RNA from archived specimens and to assess the degradation of WNV RNA in stored UR specimens. The resultant procedures were used in conjunction with PCR detection to identify WNV-positive specimens and to quantify their viral loads. A total of 59 of 352 WB, 10 of 38 UR, and 2 of 34 saliva specimens tested positive for WNV RNA. Although a single semen specimen was positive 22 days post onset, we could not definitively confirm the presence of WNV RNA in the remaining specimens. WNV RNA-positive UR specimens exhibited profound loss of viral RNA during storage, highlighting the need for optimal preservation pre-storage. This study provides optimized methods for WNV RNA detection among different fluid types and offers alternative options for diagnostic testing during the acute stages of WNV.
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spelling pubmed-65149132019-05-30 Optimizing PCR Detection of West Nile Virus from Body Fluid Specimens to Delineate Natural History in an Infected Human Cohort Gorchakov, Rodion Gulas-Wroblewski, Bonnie E. Ronca, Shannon E. Ruff, Jeanne C. Nolan, Melissa S. Berry, Rebecca Alvarado, R. Elias Gunter, Sarah M. Murray, Kristy O. Int J Mol Sci Article West Nile virus (WNV), a mosquito-borne arbovirus, remains a major global health concern. In this study, we optimized PCR methods then assessed serially-collected whole blood (WB), urine (UR), saliva, and semen specimens from a large cohort of WNV-positive participants to evaluate the natural history of infection and persistent shedding of WNV RNA. Viral RNA extraction protocols for frozen WB and UR specimens were optimized and validated through spiking experiments to maximize recovery of viral RNA from archived specimens and to assess the degradation of WNV RNA in stored UR specimens. The resultant procedures were used in conjunction with PCR detection to identify WNV-positive specimens and to quantify their viral loads. A total of 59 of 352 WB, 10 of 38 UR, and 2 of 34 saliva specimens tested positive for WNV RNA. Although a single semen specimen was positive 22 days post onset, we could not definitively confirm the presence of WNV RNA in the remaining specimens. WNV RNA-positive UR specimens exhibited profound loss of viral RNA during storage, highlighting the need for optimal preservation pre-storage. This study provides optimized methods for WNV RNA detection among different fluid types and offers alternative options for diagnostic testing during the acute stages of WNV. MDPI 2019-04-19 /pmc/articles/PMC6514913/ /pubmed/31010160 http://dx.doi.org/10.3390/ijms20081934 Text en © 2019 by the authors. Licensee MDPI, Basel, Switzerland. This article is an open access article distributed under the terms and conditions of the Creative Commons Attribution (CC BY) license (http://creativecommons.org/licenses/by/4.0/).
spellingShingle Article
Gorchakov, Rodion
Gulas-Wroblewski, Bonnie E.
Ronca, Shannon E.
Ruff, Jeanne C.
Nolan, Melissa S.
Berry, Rebecca
Alvarado, R. Elias
Gunter, Sarah M.
Murray, Kristy O.
Optimizing PCR Detection of West Nile Virus from Body Fluid Specimens to Delineate Natural History in an Infected Human Cohort
title Optimizing PCR Detection of West Nile Virus from Body Fluid Specimens to Delineate Natural History in an Infected Human Cohort
title_full Optimizing PCR Detection of West Nile Virus from Body Fluid Specimens to Delineate Natural History in an Infected Human Cohort
title_fullStr Optimizing PCR Detection of West Nile Virus from Body Fluid Specimens to Delineate Natural History in an Infected Human Cohort
title_full_unstemmed Optimizing PCR Detection of West Nile Virus from Body Fluid Specimens to Delineate Natural History in an Infected Human Cohort
title_short Optimizing PCR Detection of West Nile Virus from Body Fluid Specimens to Delineate Natural History in an Infected Human Cohort
title_sort optimizing pcr detection of west nile virus from body fluid specimens to delineate natural history in an infected human cohort
topic Article
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC6514913/
https://www.ncbi.nlm.nih.gov/pubmed/31010160
http://dx.doi.org/10.3390/ijms20081934
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