PARP-1 controls NK cell recruitment to the site of viral infection
Qiyang Shou, Huiying Fu, Xiaopei Huang, Yiping Yang
Qiyang Shou, Huiying Fu, Xiaopei Huang, Yiping Yang
View: Text | PDF
Research Article Immunology Virology

PARP-1 controls NK cell recruitment to the site of viral infection

Abstract

The activation and recruitment of NK cells to the site of viral infection are crucial for virus control. However, it remains largely unknown what controls the recruitment of the activated NK cells to the infection site. In a model of intraperitoneal infection with vaccinia virus (VV), we showed that poly(ADP-ribose) polymerase-1 (PARP-1), a sensor of DNA damage, is critical for NK cell recruitment to the site of infection and viral control in vivo. We further demonstrated that PARP-1 promotes the production of CCL2 and that the CCL2-CCR2 axis is essential for NK cell recruitment to the infection site. In addition, we demonstrated that peritoneal macrophages are the main producer of PARP-1–dependent CCL2 secretion. Mechanistically, PARP-1 functions as a regulator of NF-κB by promoting its nuclear translocation and binding to its response sequences in macrophages upon VV infection. Taken together, our results reveal a potentially previously unknown role for PARP-1–dependent CCL2 production in NK cell migration and viral control and may provide important insights into the design of effective NK cell–based therapies for viral infections and cancer.

Authors

Qiyang Shou, Huiying Fu, Xiaopei Huang, Yiping Yang

×

Figure 3

The production of CCL2 in response to VV infection is diminished in Parp-1–/– mice.

Options: View larger image (or click on image) Download as PowerPoint
The production of CCL2 in response to VV infection is diminished in Parp...
WT or Parp-1–/– mice were infected with VV (5 × 106 PFU, i.p.) and some mice were left uninfected as controls (Naive). (A) 12 hours after infection, intraperitoneal cells were collected and assayed for CCL2, CCL3, CCL4, CCL5, CCL7, and CCL8 mRNA levels by real-time quantitative PCR. Relative mRNA levels were normalized to β-actin RNA within each sample. Data represent mean relative mRNA levels ± SD (n = 3). Folds (F) of change in samples from VV-infected WT (WT VV) over Parp1–/– (Parp1–/– VV) mice are shown. (B) 24 hours after infection, peritoneal fluid was harvested and measured for CCL2 production by the colorimetric beads assay. Data represent mean CCL2 concentrations (pg/ml) ± SD (n = 3). *P < 0.05, **P < 0.01, 2-tailed Student’s t test.