Analysis of cell-associated DENV RNA by oligo(dT) primed 5’ capture scRNAseq

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作者
Mark A. Sanborn
Tao Li
Kaitlin Victor
Hayden Siegfried
Christian Fung
Alan L. Rothman
Anon Srikiatkhachorn
Stefan Fernandez
Damon Ellison
Richard G. Jarman
Heather Friberg
Irina Maljkovic Berry
Jeffrey R. Currier
Adam T. Waickman
机构
[1] Viral Diseases Branch,
[2] Walter Reed Army Institute of Research,undefined
[3] Department of Cell and Molecular Biology,undefined
[4] Institute for Immunology and Informatics,undefined
[5] University of Rhode Island,undefined
[6] Faculty of Medicine,undefined
[7] King Mongkut’s Institute of Technology Ladkrabang,undefined
[8] Department of Virology,undefined
[9] Armed Forces Research Institute of Medical Sciences,undefined
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Scientific Reports | / 10卷
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摘要
Dengue is one of the most widespread vector-borne viral diseases in the world. However, the size, heterogeneity, and temporal dynamics of the cell-associated viral reservoir during acute dengue virus (DENV) infection remains unclear. In this study, we analyzed cells infected in vitro with DENV and PBMC from an individual experiencing a natural DENV infection utilizing 5’ capture single cell RNA sequencing (scRNAseq). Both positive- and negative-sense DENV RNA was detected in reactions containing either an oligo(dT) primer alone, or in reactions supplemented with a DENV-specific primer. The addition of a DENV-specific primer did not increase the total amount of DENV RNA captured or the fraction of cells identified as containing DENV RNA. However, inclusion of a DENV-specific cDNA primer did increase the viral genome coverage immediately 5’ to the primer binding site. Furthermore, while the majority of intracellular DENV sequence captured in this analysis mapped to the 5’ end of the viral genome, distinct patterns of enhanced coverage within the DENV polyprotein coding region were observed. The 5’ capture scRNAseq analysis of PBMC not only recapitulated previously published reports by detecting virally infected memory and naïve B cells, but also identified cell-associated genomic variants not observed in contemporaneous serum samples. These results demonstrate that oligo(dT) primed 5’ capture scRNAseq can detect DENV RNA and quantify virus-infected cells in physiologically relevant conditions, and provides insight into viral sequence variability within infected cells.
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