Chromosome-specific and noisy IFNB1 transcription in individual virus-infected human primary dendritic cells

Hu, Jianzhong; Sealfon, Stuart C.; Hayot, F.; Jayaprakash, C.; Kumar, Manish; Pendleton, Audrey C.; Ganee, Arnaud; Fernández-Sesma, Ana; Moran, Thomas M.; Wetmur, James G.

doi:10.1093/nar/gkm557

Cited by 58 publications

(92 citation statements)

References 39 publications

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“…Therefore, it is possible that in the absence of DIs or other aberrant RNA generation, the RIG-I pathway may only be poorly activated. This phenomenon would fit well with the observation that only a very small portion of infected cells activate their IFN responses, which may represent those cells in which DIs or other abnormal virus replication products are generated [38][39][40][41].…”

Section: Discussionsupporting

confidence: 84%

Loss of Sendai virus C protein leads to accumulation of RIG-I immunostimulatory defective interfering RNA

Sánchez-Aparicio

Garcin

Rice

et al. 2017

Journal of General Virology

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Retinoic acid inducible gene (RIG-I)-mediated innate immunity plays a pivotal role in defence against virus infections. Previously we have shown that Sendai virus (SeV) defective interfering (DI) RNA functions as an exclusive and potent RIG-I ligand in DI-RNA-rich SeV-Cantell infected cells. To further understand how RIG-I is activated during SeV infection, we used a different interferon (IFN)-inducing SeV strain, recombinant SeVDC, which, in contrast to SeV-Cantell is believed to stimulate IFN production due to the lack of the SeV IFN antagonist protein C. Surprisingly, we found that in SevDC-infected cells, DI RNAs also functioned as an exclusive RIG-I ligand. Infections with wild-type SeV failed to generate any RIG-I-associated immunostimulatory RNA and this correlated with the lack of DI genomes in infected cells, as well as with the absence of cellular innate immune responses. Supplementation of the C protein in the context of SeVDC infection led to a reduction in the number of DI RNAs, further supporting the potential role of the C protein as a negative regulator of DI generation and/or accumulation. Our findings indicate that limiting DI genome production is an important function of viral IFN antagonist proteins.

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Section: Discussionsupporting

confidence: 84%

Loss of Sendai virus C protein leads to accumulation of RIG-I immunostimulatory defective interfering RNA

Sánchez-Aparicio

Garcin

Rice

et al. 2017

Journal of General Virology

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“…That mouse BMDCs show a striking lack of infectivity is consonant with recent results using PR8 reporting only 30 to 40% infectivity at an MOI as high as 30 (7). We confirmed these surprising results by two other sensitive techniques, multiprobe single-molecule fluorescence in situ hybridization (FISH) (8) and single-cell PCR assays (9) (Fig. 1D).…”

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confidence: 89%

Mouse Dendritic Cell (DC) Influenza Virus Infectivity Is Much Lower than That for Human DCs and Is Hemagglutinin Subtype Dependent

Hartmann

Jia

et al. 2013

J Virol

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We show that influenza A H1N1 virus infection leads to very low infectivity in mouse dendritic cells (DCs) in vitro compared with that in human DCs. This holds when H3 or H5 replaces H1 in recombinant viruses. Viruslike particles confirm the difference between mouse and human, suggesting that reduced virus entry contributes to lower mouse DC infectivity. Low infectivity of mouse DCs should be considered when they are used to study responses of DCs that are actually infected.

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“…5B). infb1 is upregulated after infection by all strains by 2 h. Single-cell studies of infb1 induction and its response in conjunction with mathematical modeling suggest that very low levels of ifnb1 generated by a few activated cells, which may not be detected in biochemical assays, may nevertheless be adequate to initiate an ISG response (62,63). A similar mechanism may underlie the apparent lack of correspondence of ifnb1 levels and timing with the levels and timing of ISG in 1918 infections, unlike in infections with the other viruses.…”

Section: Discussionmentioning

confidence: 99%

Human Dendritic Cell Response Signatures Distinguish 1918, Pandemic, and Seasonal H1N1 Influenza Viruses

Hartmann

Thakar

Albrecht

et al. 2015

J Virol

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IMPORTANCEContinuously evolving influenza viruses present a global threat to human health; however, these host responses display straindependent differences that are incompletely understood. Thus, we conducted a detailed comparative study assessing the immune responses of human DC to infection with two pandemic and two seasonal H1N1 influenza strains. We identified in the immune response to viral infection both common and strain-specific features. Among the stain-specific elements were a time shift of the interferon-stimulated gene response, selective induction of NF-B signaling by one of the seasonal strains, and massive RNA degradation as early as 4 h postinfection by the seasonal, but not the pandemic, viruses. These findings illuminate new aspects of the distinct differences in the immune responses to pandemic and seasonal influenza viruses.

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Chromosome-specific and noisy IFNB1 transcription in individual virus-infected human primary dendritic cells

Cited by 58 publications

References 39 publications

Loss of Sendai virus C protein leads to accumulation of RIG-I immunostimulatory defective interfering RNA

Loss of Sendai virus C protein leads to accumulation of RIG-I immunostimulatory defective interfering RNA

Mouse Dendritic Cell (DC) Influenza Virus Infectivity Is Much Lower than That for Human DCs and Is Hemagglutinin Subtype Dependent

Human Dendritic Cell Response Signatures Distinguish 1918, Pandemic, and Seasonal H1N1 Influenza Viruses

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