2017
DOI: 10.1128/jvi.00767-17
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Differential Innate Immune Signaling in Macrophages by Wild-Type Vaccinia Mature Virus and a Mutant Virus with a Deletion of the A26 Protein

Abstract: The Western Reserve (WR) strain of mature vaccinia virus contains an A26 envelope protein that mediates virus binding to cell surface laminin and subsequent endocytic entry into HeLa cells. Removal of the A26 protein from the WR strain mature virus generates a mutant, WRΔA26, that enters HeLa cells through plasma membrane fusion. Here, we infected murine bone marrow-derived macrophages (BMDM) with wild-type strain WR and the WRΔA26 mutant and analyzed viral gene expression and cellular innate immune signaling.… Show more

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Cited by 10 publications
(9 citation statements)
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“…Recombinant viruses expressing WR-A26(76–500) or WR-A26(321–500) were isolated and plaque-purified. A recombinant vaccinia virus expressing full-length flag-tagged A26 protein, named WR-A26, was also included [36]. HeLa cells were infected with individual virus at a multiplicity of infection (MOI) of 5 plaque-forming units (PFU) per cell and harvested at 24 hours post infection (hpi) to determine MV growth (Fig 1C).…”
Section: Resultsmentioning
confidence: 99%
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“…Recombinant viruses expressing WR-A26(76–500) or WR-A26(321–500) were isolated and plaque-purified. A recombinant vaccinia virus expressing full-length flag-tagged A26 protein, named WR-A26, was also included [36]. HeLa cells were infected with individual virus at a multiplicity of infection (MOI) of 5 plaque-forming units (PFU) per cell and harvested at 24 hours post infection (hpi) to determine MV growth (Fig 1C).…”
Section: Resultsmentioning
confidence: 99%
“…Schematics of recombinant viruses showing the WR-A26-H2R and WR-A26-H3R mutant genome arrangements. WR-A26 and WR-ΔA26 were described previously [32, 36], and the latter was used as the parental virus to generate the WR-A26-H2R and WR-A26-H3R recombinant viruses. The A26-H2R and A26-H3R gene cassettes were inserted into the A26L native locus and recombinant virus was selected as blue plaques in agar plates containing X-gal.…”
Section: Resultsmentioning
confidence: 99%
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“…Viral genomic DNA containing an early Venus expression cassette flanked by J4L and J5R sequences was obtained from John H. Connor (54,55) and used as the template to obtain a PCR fragment, which was subsequently cloned into a TOPO plasmid, resulting in pTopo-J4R-Venus-J5L, in which Venus is expressed from a viral early promoter of the C11R gene (54). The plasmid was sequenced to ensure accuracy and subsequently transfected into CV-1 cells that had been infected with WRΔA26-A4mCherry (50). The lysates were harvested at 24 h postinfection (hpi), and virus titration was performed on BSC40 cells to isolate the WRΔA26-Venus-A4-mCherry virus through multiple rounds of plaque purification by fluorescence microscopy until 100% purity was reached.…”
Section: Methodsmentioning
confidence: 99%
“…Many other VACV proteins, either immunomodulators or proteins with other functions, affect virulence and/or the host immune response. These include I4 (ribonucleotide reductase large subunit) [ 271 , 272 ], J2 (thymidine kinase) [ 273 ], A26 (virion attachment/entry) [ 274 ], B5 (virion envelope glycoprotein related to complement control factor) [ 275 , 276 ], B13 and B22 (serine protease inhibitors SPI-2 and SPI-1, respectively) [ 163 , 277 , 278 , 279 ], F12 (IEV transport protein) [ 280 ], A36 (IEV transport protein and actin tail inducer) [ 163 , 281 ], A40 (cell surface glycoprotein) [ 163 , 282 ], A50 (DNA ligase) [ 283 ], C2, F3 and A55 (intracellular kelch protein immunomodulators) [ 284 , 285 , 286 ] and A33 (virion envelope glycoprotein) [ 276 ], However, the protective capacity of viruses lacking these proteins requires further study.…”
Section: Vaccine Engineering By Targeting Vaccinia Virus Proteins mentioning
confidence: 99%