Wild-type (WT) female 6-8-week-old C57BL/6 mice were purchased from Liaoning Changsheng Experimental Animal Centre. Nlrp3^-/- mice with C57BL/6 genetic background were obtained from the Jackson Laboratory (4). WT or Nlrp3^-/- mice were intraperitoneally injected with 2 ml of 5% thioglycolate medium (BD Biosciences, CA, USA) per mouse, and 3 days later peritoneal macrophages (PMs) from the peritoneal cavity were collected by flushing twice with 6 ml ice sterile PBS. PMs were counted and plated into 6-well-plate at 2.5×10⁶ cells per well with RPMI-1640 medium supplemented with 10% fetal bovine serum (FBS). The supernatant was discarded the next day, and adherent cells were further cultures as PMs (27).

N. caninum used in the present study was Nc-1 strain and was maintained in Vero cells with RPMI-1640 medium supplemented with 2% FBS (BI, Israel) in a 5% CO₂ atmosphere at 37°C. N. caninum tachyzoites were harvested by gradient density centrifugation with 40% Percoll solution (Sigma, Shanghai, China) at 1500×g for 30 min. The precipitate was collected and washed twice with RPMI-1640 medium, while the supernatant was discarded. The numbers of tachyzoites were determined using a hemocytometer. Excretory secretory products (ESPs) of N. caninum were prepared and stored as previously reported (28). And the concentration of ESPs was determined using the BCA Protein Assay Kit (Thermo Fisher Scientific, Waltham, MA).

Mouse anti-Tim23 was from Santa Cruz Biotechnology (CA, USA). Rabbit anti-Hsp60 antibody, FITC-conjugated anti-rabbit IgG antibody, and HRP-conjugated anti-mouse, rabbit, or goat IgG antibodies were purchased from Proteintech (Wuhan, China). Rabbit anti-β-actin, anti-LC3, anti-ERK, anti-p38, anti-p65, anti-phospho-ERK (Thr202/Tyr204), anti-phospho-p38 (Thr180/Tyr182), and anti-phospho-p65 (Ser536) antibodies were obtained from Cell Signaling Technology (Danvers, MA, USA). Goat anti-IL-1β antibody was from R&D (Minneapolis, USA). Mouse anti-caspase-1 (p20) and mouse anti-Nlrp3 antibodies were purchased from Adipogen (Liestal, Switzerland).

The mice were randomly divided into seven groups, including Mdivi1+N. caninum group (10 mice), CCCP+N. caninum group (10 mice), solvent+N. caninum group (10 mice), and N. caninum group (10 mice). The mice were infected intraperitoneally with 2.5×10⁷ N. caninum tachyzoites diluted in 100 µl PBS. After 24 h, Mdivi1 (MCE, Shanghai, China) and CCCP was diluted in PBS, and mice were then immediately injected intraperitoneally with Mdivi-1 (50 mg/kg body weight/per day) or with CCCP at a dose of 5 mg/kg body weight/per day (20). The mice were monitored and weighed each day. Then the mice were euthanized at 5 d p.i. and the brain, heart, liver, spleen, kidney, and lung tissues were collected to measure parasite burden. The serum was collected to detect cytokines at 5 d p.i. Mdivi1 group (3 mice as inhibitor control), CCCP group (3 mice as inhibitor control) and PBS group (3 mice as negative control).

PMs were pretreated with Mdivi1 (20 µM), CCCP (10 µM) (20), and ROS inhibitor (NAC; 2 mM, Selleck, Shanghai, China) for 2 h (29) before being stimulated by N. caninum for 30 min to detect the phosphorylation of p38, ERK, and NF-κB p65. PMs were also stimulated by N. caninum for 24 h to measure Nlrp3, Caspase1, and IL-1β by Western blot as previously described (30). PMs were pretreated with Mdivi1 (20 µM), CCCP (10 µM), NAC (2 mM), p38 inhibitor (SB203580; 5 μM, Sigma-Aldrich, MO, USA), and ERK inhibitor (PD98059; 5 μM, Sigma-Aldrich, MO, USA) for 2 h, followed by stimulation with N. caninum for 24 h to detect parasite burden by qPCR and the production of cytokines by ELISA.

The cell lysates and supernatants of PMs were collected and assessed by Western blot as described previously (28). The rabbit monoclonal anti-β-actin, anti-ERK, anti-p38, anti-p65, anti-phospho-ERK (Thr202/Tyr204), anti-phospho-p38 (Thr180/Tyr182), anti-phospho-IκBα (Ser32), anti-phospho-p65 (Ser536), mouse monoclonal anti-Caspase1 and anti-NLRP3, and goat monoclonal anti-IL-1β diluted at 1:1000 with 5% BSA were used to incubate the membranes overnight at 4°C. Then the membranes were incubated with anti-rabbit/mouse/goat secondary HRP-conjugated antibodies (Proteintech, Wuhan, China) diluted at 1:5000 with 5% skim milk. Western blot bands were detected using the enhanced chemiluminescence reagent (Vigorous, Beijing, China). The membranes were visualized using the ECL Western blot Detection System.

Parasite replication in the infected cells and mouse homogenized tissues was monitored as previously described by performing qPCR analysis of the parasite DNA (4). Genomic DNA from 1×10⁷ tachyzoites of N. caninum and total DNA from infected cells and mouse tissues were extracted using a Genomic DNA Extraction Kit (TIANGEN, Beijing, China) following the manufacturer’s protocol. The total DNA from infected cells (200 ng) and tissues (500 ng) was analyzed by qPCR with FastStart Universal SYBR Green Master reagent (Roche Diagnostics, Mannheim, Germany), and a 76-bp fragment of N. caninum DNA was amplified using the following primers: forward (5′-ACTGGAGGCACGCTGAACAC-3′); reverse (5′-AACAATGCTTCGCAAGAG GAA-3′). The number of parasites was determined based on a standard curve obtained using DNA from serial dilutions of N. caninum tachyzoites (from 1×10⁷ to 1×10⁰ parasite).

Supernatants from cell culture and serum from mice were measured by mouse IL-1β, IL-18, IFN-γ, IL-12p40, IL-6, or TNF-α Ready-Set-Go Kits (eBioscience, San Diego, CA, USA) according to the manufacturer’s instructions.

PMs were pretreated with Mdivi1 (20 µM), CCCP (10 µM), NAC (2 mM) for 2 h, followed by stimulation with N. caninum (MOI 1:3) for 3 h or with Rosup (Beyotime Biotechnology, Shanghai, China) according to the instructions as the positive control. Then the supernatant was removed, and the PMs were incubated with the DCFH-DA (Beyotime Biotechnology, Shanghai, China) for 20–30 min at 37°C, followed by 3 washes with FBS-free RPMI in the dark as the manufacturer’s instructions. Intracellular ROS were analyzed using a FACS Aria flow cytometer (BD Biosciences, CA, USA).

The data were expressed as mean ± SD. Data sets with only two independent groups were analyzed for statistical significance using unpaired, two-tailed Student’s T-test. Data sets with more than two groups were analyzed using one-way ANOVA with Tukey-Kramer post hoc test. All graphs were generated using GraphPad Prism 5 (GraphPad Software, Inc., San Diego, CA, USA). All p values less than 0.05 were considered significant (*p<0.05, **p<0.01, ***p<0.001). P values equal to or more than 0.05 were considered no significant (p>0.05, ns). All data of this study were obtained from 3 independent experiments.

TEM and Immunofluorescence experiments were performed to determine whether mitophagy occurred in mouse macrophages during N. caninum infection. Results showed that mitochondria were enclosed by autophagosome in N. caninum-stimulated or CCCP treated (mitophagy inducer) PMs by TEM ( Figure 1A ). Immunofluorescence results demonstrated that N. caninum induced co-localization of mitochondria with endogenous LC3 in PMs and with GFP-LC3 in 293T cells ( Figures 1B, C ). And N. caninum induced mitophagy occurrence in 32.6% PMs and 31.0% 293T cells ( Figures S1A, B ). To evaluate whether N. caninum-induced mitophagy was dependent on infecting numbers of N. caninum or infection time, the levels of mtDNA and the amount of mitochondrial inner membrane protein Tim23 and matrix protein Hsp60 in mouse PMs were measured. With the increase of the numbers of N. caninum- or infection time, the mtDNA/nDNA ratios and the levels of Hsp60 and Tim23 protein decreased gradually, which was similar to that of CCCP treatment ( Figures 2A–C ). In addition, Western blot results were further analyzed by grayscale analysis ( Figures 2D, E ). However, N. caninum ESPs had no impact on the expression levels of Hsp60 and Tim23 in PMs ( Figures 2C–E ). Altogether, our data demonstrated that N. caninum induced mitophagy in mouse macrophages.

Furthermore, mitophagy was identified in mice during N. caninum infection. No significant difference in total cells counts was observed in peritoneal lavage fluids ( Figure 3A ). With the decrease of N. caninum number, the levels of mtDNA/nDNA ratios gradually increased from the third to seventh days post-infection in peritoneal lavage cells during N. caninum infection ( Figures 3B, C ). However, with the increase of parasite load in the brain, the levels of mtDNA and the protein expression levels of Hsp60 and Tim23 showed a downward trend ( Figures 3D–F ). Western blot results were further analyzed by grayscale analysis ( Figure 3G ). Taken together, these results indicated that mitophagy occurred in in vitro and in vivo during N. caninum infection.

To further determine the effects of mitophagy on N. caninum infection, mitophagy inducer (CCCP) and inhibitor (Mdivi1) were used both in vivo and in vitro. We found that Mdivi1 treatment increased the survival rate of mice while CCCP treatment accelerated the time to death of mice during N. caninum infection ( Figure 4A ). The CCCP-treated mice exhibited a significant loss in body weight compared with untreated mice during N. caninum infection. On the contrary, Mdivi1 alleviated the weight loss in mice ( Figure 4B ). Subsequently, we examined the parasite burden of different tissues by qPCR, and the parasite loads in the brain (2.46-fold), heart (1.89-fold), lung (1.41-fold), spleen (3.51-fold), and kidney (1.73-fold) in mice treated by CCCP were significantly increased compared to that in the solvent+N. caninum mice ( Figures 4C–E, G, H ). There was no difference in the parasite load in the liver ( Figure 4F ). Moreover, Mdivi1 treatment inhibited N. caninum burden in the brain (20%), heart (38%), lung (25%), spleen (44%), and kidney (74%) but not in the liver ( Figures 4C–H ). In addition, the number of N. caninum in mouse PMs treated with Mdivi1 (30%) was reduced, while the number was increased with CCCP treatment (1.60-fold) during N. caninum infection ( Figure 5A ). Taken together, these results indicated that N. caninum–induced mitophagy played a critical role in parasite survival in mice.

It is noted that the secretions of IL-1β, IL-6, IL-12p40, IFN-γ, IL-18, and TNF-α played essential roles against N. caninum infection (4–6). Thus, we examined whether the role of mitophagy in parasite survival was through inhibiting cytokines production. We found that Mdivi1 treatment enhanced the production of IL-6 (1035.54 ± 165.21 pg/ml), IL-12p40 (1654.33 ± 39.62 pg/ml), IFN-γ (1981.31 ± 49.41 pg/ml), and IL-18 (765.21 ± 59.81 pg/ml), while CCCP treatment suppressed the production of IL-6 (222.67 ± 64.78 pg/ml), IL-12p40 (435.21 ± 87.52 pg/ml), IFN-γ (1046.76 ± 128.61 pg/ml), and IL-18 (213.65 ± 68.35 pg/ml) in mice during N. caninum infection compared to the solvent+N. caninum group (580.57 ± 29.60 pg/ml, 1338.57 ± 31.59 pg/ml, 1633.27 ± 62.69 pg/ml, 542.12 ± 60.68 pg/ml) ( Figures 4I, J, K, M ). Moreover, the production of IL-1β, IL-6, IL-12p40, IFN-γ were increased in Mdivi1-treated PMs (42.85 ± 4.39 pg/ml, 438.03 ± 41.80 pg/ml, 1674.33 ± 66.86 pg/ml, and 1755.52 ± 170.31 pg/ml), while were inhibited in CCCP-treated PMs (10.07 ± 2.76 pg/ml, 39.78 ± 4.78 pg/ml, 982.21 ± 90.11 pg/ml, and 763.62 ± 47.06 pg/ml) compared with solvent-treated PMs (291.35 ± 33.16 pg/ml, 1413.22 ± 43.48 pg/ml, 1365.22 ± 83.60 pg/ml) infected by N. caninum ( Figures 5B–D, F ). However, there were no significant differences in TNF-α production both in vivo and in vitro ( Figures 4L , 5E ). These data suggested that N. caninum-induced mitophagy could inhibit the production of proinflammatory cytokines in PMs and mice during N. caninum infection.

ROS contributed to the production of proinflammatory cytokines (23) and mitophagy played an important role in ROS scavenging (16, 24). To examine whether N. caninum-induced mitophagy inhibited the production of proinflammatory cytokines through scavenging ROS in PMs, we detected the level of N. caninum-induced ROS in PMs treated with Mdivi1 and CCCP. Mdivi1 treatment enhanced the ROS generation in PMs infected by N. caninum (1.12-fold compared to DMSO-Nc group), while CCCP treatment suppressed it (78% compared to DMSO-Nc group) ( Figures 6A, B ). And the production of IL-1β, IL-6, IL-12p40, and IFN-γ were significantly reduced in N. caninum-infected PMs treated by NAC ( Figures 6C–F ). These data suggested that ROS, which could be controlled by N. caninum-induced mitophagy, down-regulated the production of IL-1β, IL-6, IL-12p40, and IFN-γ in PMs.

It is noted that Nlrp3, NF-κB, p38, and ERK signal pathways participated in modulating the production of inflammatory cytokines (4, 31–33). Therefore, we examined whether Nlrp3 inflammasome, NF-κB, p38, and ERK signal pathways in N. caninum-infected PMs were modulated by the mitophagy-ROS axis. The data revealed the phosphorylation of ERK was reduced in N. caninum-infected PMs treated with CCCP and NAC, while that was up-regulated in Mdivi1-treatment group ( Figures 7A, B ). On the contrary, the phosphorylation of p38 was promoted by NAC or CCCP, but was inhibited in PMs treated by Mdivi1 during N. caninum infection ( Figures 7A, B ). However, there were no significant differences in the phosphorylation of NF-κB p65 in PMs treated by CCCP and Mdivi1 during N. caninum infection ( Figure 7A ). The Western blot results showed that NLRP3, pro-caspase1, pro-IL-1β, cleavage of caspase-1, and active IL-1β were significantly increased after Mdivi1 treatment while decreased after CCCP or NAC treatment in N. caninum-infected PMs for 24 h ( Figures 7C, D ). To further investigate the roles of the p38, ERK, and Nlrp3 inflammasome in cytokine production and parasite proliferation, p38 (SB203580) and ERK (PD98059) inhibitors and Nlrp3^-/- mice PMs were used. SB203580 treatment promoted N. caninum-induced production of IL-1β (42.29 ± 2.51 pg/ml), IL-6 (391.81 ± 9.71 pg/ml), IL-12p40 (1626.45 ± 30.74 pg/ml), and IFN-γ (1630.32 ± 65.91 pg/ml) in PMs compared to solvent-N. caninum group (30.31 ± 6.74 pg/ml, 311.89 ± 11.34 pg/ml, 1414.56 ± 30.33 pg/ml, 1387.21 ± 74.32 pg/ml). While PD98059 treatment inhibited N. caninum-induced production of IL-1β (25.71 ± 3.59 pg/ml), IL-6 (209.72 ± 10.15 pg/ml), IL-12p40 (931.17 ± 41.12 pg/ml), and IFN-γ (935.82 ± 71.74 pg/ml) in PMs ( Figures 7E–H ). The production of IL-1β (15.29 ± 2.12 pg/ml) was inhibited in Nlrp3^-/- PMs infected by N. caninum ( Figure 7E ). Correspondingly, the number of parasites was increased in PD98059-treated PMs (1.17-fold) and Nlrp3^-/- PMs (1.39-fold), while the number of parasites was decreased in SB203580-treated PMs (75%) ( Figure 7I ). Taken together, N. caninum-induced mitophagy-ROS axis could regulate the production of cytokines through p38, ERK, and Nlrp3 inflammasome pathways.