Primary Human Macrophages Serve as Vehicles for Vaccinia Virus Replication and Dissemination

Byrd, Daniel; Shepherd, Nicole; Lan, Jie; Hu, Ningjie; Amet, Tohti; Yang, Kai; Desai, Mona; Yu, Qigui

doi:10.1128/jvi.03726-13

Cited by 27 publications

(24 citation statements)

References 86 publications

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“…In primary human macrophages in vitro , the cells are permissive to VACV infection and can be a vehicle for VACV replication and dissemination. These macrophages can produce extracellular enveloped virions for long-range VACV dissemination and form virion-associated structures contributing to cell-cell spread (36). Although the co-expression of CD11b and F4/80 has been often been used to identify macrophage-lineage cells, macrophages cannot be accurately distinguished from conventional DCs (CD11b + DC) and mo-DCs in skin.…”

Section: Discussionmentioning

confidence: 99%

IL-1R Type 1–Deficient Mice Demonstrate an Impaired Host Immune Response against Cutaneous Vaccinia Virus Infection

Tian

Jin

Dubin

et al. 2017

The Journal of Immunology

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The IL-1 superfamily of cytokines and receptors has been studied extensively. However, the specific roles of IL-1 elements in host immunity to cutaneous viral infection remain elusive. In this study, we applied vaccinia virus (VACV) by scarification to IL-1 receptor type 1 knockout mice (IL-1R1−/−) and found that these mice developed markedly larger lesions with higher viral genome copies in skin than wild-type (WT) mice. The phenotype of infected IL-1R1−/− mice was similar to eczema vaccinatum (EV), a severe side effect of VACV vaccination that may develop in humans with atopic dermatitis (AD). Interestingly, the impaired cutaneous response of IL-1R1−/− mice did not reflect a systemic immune deficiency, since immunized IL-1R1−/− mice survived subsequent lethal VACV intranasal challenge, or defects of T cell activation or T cell homing to the site of inoculation. Histologic evaluation revealed that VACV infection and replication after scarification were limited to the epidermal layer of WT mice, whereas lack of IL-1R1 permitted extension of VACV infection into dermal layers of the skin. We explored the etiology of this discrepancy and determined that IL-1R1−/− mice contained significantly more macrophages and monocyte-derived dendritic cells (mo-DC) in the dermis after VACV scarification. These cells were vulnerable to VACV infection and may augment the transmission of virus to adjacent skin, thus leading to larger skin lesions and satellite lesions in IL-1R1−/− mice. These results suggest new therapeutic strategies for treatment of EV and inform assessment of risks in patients receiving IL-1 blocking antibodies for treatment of chronic inflammatory disorders.

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Section: Discussionmentioning

confidence: 99%

IL-1R Type 1–Deficient Mice Demonstrate an Impaired Host Immune Response against Cutaneous Vaccinia Virus Infection

Tian

Jin

Dubin

et al. 2017

The Journal of Immunology

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“…Viruses VACV (strain WR) was grown and titrated using 143B TK 2 cells, screened regularly for the presence of adventitious pathogens, as previously described (36). Recombinant VACV (rVACV) expressing GFP driven by the early/late p7.5 promoter (VACV-p7.5 GFP) or the late p11 promoter (VACV-p11 GFP) were described previously (31). For titrations of VACV from infected BMDC, cells were lysed at the time points indicated and titrated on 142B TK 2 cells as above.…”

Section: Cellsmentioning

confidence: 99%

“…The inability of late VACV promoter-driven Ag to stimulate T CD8+ responses has been correlated to an abortive in vitro infection of pAPC, in which late Ags are not produced and so direct presentation cannot occur (27)(28)(29)(30). However, some publications have indicated that VACV can replicate and spread following infection of APC (31), indicating either that all late genes required for productive replication can be produced within infected APC populations or that some APC populations may allow late VACV gene transcription. Therefore, the possibility exists that immunogenic late VACV Ags are primed by VACV-infected DC that directly present Ag.…”

Section: Introductionmentioning

confidence: 99%

Analysis of MHC Class I Processing Pathways That Generate a Response to Vaccinia Virus Late Proteins

et al. 2019

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Use of recombinant viral vectors encoding nonnative Ags is an attractive mechanism for the generation of protective Ab, CD4 + T cell (T CD4+ ), and CD8 + T cell (T CD8+ ) responses in vivo following immunization. However, the life cycle and tropism of the viral vector, and its interactions with various components of the immune system, must be fully understood to maximize the efficacy of any vaccination strategies. Ab and T CD4+ responses typically target native Ags driven by late promoters in vaccinia virus (VACV)-based vectors. However, it has been demonstrated that model Ags driven by late promoters in recombinant VACV vectors do not stimulate T CD8+ responses, whereas identical Ags driven by early promoters stimulate strong responses. Conversely, T CD8+ can be generated against some natural late VACV Ags. We explored this dichotomy by investigating the Ag presentation pathways responsible for presentation of natural late VACV Ags in mice. We found that all of the late VACV Ags we examined could be cross-primed (i.e., presented by uninfected professional APC), as well as directly presented by infected dendritic cell populations. However, one Ag was only presented by professional APC populations and was not the target of a protective T CD8+ response. Therefore, there is no generalized blockade in Ag presentation of late VACV Ags, and expression of nonnative Ags driven by a late promoter allows production of large quantities of Ag that may allow simultaneous targeting of both T CD4+ and Ab responses, as well as T CD8+ responses, in the future. ImmunoHorizons, 2019, 3: 559-572.

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“…Signals were sequentially collected using single fluorescence excitation and acquisition settings to avoid crossover. [45][46][47] Images were processed and analyzed using FV10-ASW 3.0 Viewer software (Olympus America, Center Valley, PA) or ImageJ 1.44p (NIH, Bethesda, MD).…”

Section: Confocal Microscopymentioning

confidence: 99%

Glycosylphosphatidylinositol Anchor Deficiency Attenuates the Production of Infectious HIV-1 and Renders Virions Sensitive to Complement Attack

Amet

Lan

Shepherd

et al. 2016

AIDS Research and Human Retroviruses

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Human immunodeficiency virus type 1 (HIV-1) escapes complement-mediated lysis (CML) by incorporating host regulators of complement activation (RCA) into its envelope. CD59, a key member of RCA, is incorporated into HIV-1 virions at levels that protect against CML. Since CD59 is a glycosylphosphatidylinositol-anchored protein (GPI-AP), we used GPI anchor-deficient Jurkat cells (Jurkat-7) that express intracellular CD59, but not surface CD59, to study the molecular mechanisms underlying CD59 incorporation into HIV-1 virions and the role of host proteins in virus replication. Compared to Jurkat cells, Jurkat-7 cells were less supportive to HIV-1 replication and more sensitive to CML. Jurkat-7 cells exhibited similar capacities of HIV-1 binding and entry to Jurkat cells, but were less supportive to viral RNA and DNA biosynthesis as infected Jurkat-7 cells produced reduced amounts of HIV-1 RNA and DNA. HIV-1 virions produced from Jurkat-7 cells were CD59 negative, suggesting that viral particles acquire CD59, and probably other host proteins, from the cell membrane rather than intracellular compartments. As a result, CD59-negative virions were sensitive to CML. Strikingly, these virions exhibited reduced activity of virus binding and were less infectious, implicating that GPI-APs may be also important in ensuring the integrity of HIV-1 particles. Transient expression of the PIG-A gene restored CD59 expression on the surface of Jurkat-7 cells. After HIV-1 infection, the restored CD59 was colocalized with viral envelope glycoprotein gp120/gp41 within lipid rafts, which is identical to that on infected Jurkat cells. Thus, HIV-1 virions acquire RCA from the cell surface, likely lipid rafts, to escape CML and ensure viral infectivity.

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Primary Human Macrophages Serve as Vehicles for Vaccinia Virus Replication and Dissemination

Cited by 27 publications

References 86 publications

IL-1R Type 1–Deficient Mice Demonstrate an Impaired Host Immune Response against Cutaneous Vaccinia Virus Infection

IL-1R Type 1–Deficient Mice Demonstrate an Impaired Host Immune Response against Cutaneous Vaccinia Virus Infection

Analysis of MHC Class I Processing Pathways That Generate a Response to Vaccinia Virus Late Proteins

Glycosylphosphatidylinositol Anchor Deficiency Attenuates the Production of Infectious HIV-1 and Renders Virions Sensitive to Complement Attack

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