Activation of liver X receptor plays a central role in antiviral actions of 25-hydroxycholesterol

Production of 25-hydroxycholesterol (25HC), a potent inhibitor of viral infection, is catalyzed by cholesterol 25-hydroxylase (CH25H). We previously reported that 25HC induced CH25H expression in a liver X receptor (LXR)-dependent manner, implying that LXR can play an important role in antiviral infection. In this study, we determined that activation of LXR by 25HC or synthetic ligands [T0901317 (T317) or GW3965] inhibited infection of herpes simplex virus type 1 (HSV-1) or MLV-(VSV)-GFP in HepG2 cells or RAW 264.7 macrophages. Genetic deletion of LXRα, LXRβ, or CH25H expression in HepG2 cells by CRISPR/Cas9 method increased cell susceptibility to HSV-1 infection and attenuated the inhibition of LXR on viral infection. Lack of interferon (IFN)-γ expression also increased cell susceptibility to viral infection. However, it attenuated, but did not block, the inhibition of LXR on HSV-1 infection. In addition, expression of CH25H, but not IFN-γ, was inversely correlated to cell susceptibility to viral infection and the antiviral actions of LXR. Metabolism of 25HC into 25HC-3-sulfate (25HC3S) by cholesterol sulfotransferase-2B1b moderately reduced the antiviral actions of 25HC because 25HC3S is a weaker inhibitor of HSV-1 infection than 25HC. Furthermore, administration of T317 to BALB/c mice reduced HSV-1 growth in mouse tissues. Taken together, we demonstrate an antiviral system of 25HC with involvement of LXR activation, interaction between CH25H and IFN-γ, and 25HC metabolism.

25-Hydroxycholesterol (25HC) is produced in cells by an enzymatic reaction catalyzed by cholesterol 25-hydroxylase (CH25H). 25HC can function as an inhibitor of viral infection and an endogenous agonist of liver X receptor (LXR), a ligand-activated transcription factor. The previous studies have demonstrated the multiple biological functions of 25HC. For instance, CH25H expression and 25HC production are involved in immunological processes (1). Stimulation of macrophage Toll-like receptors can induce CH25H expression and consequently enhance 25HC production/ secretion and suppress immunoglobulin A production (2).
CH25H expression in bone marrow-derived dendritic cells and macrophages can be upregulated by interferons (IFNs) (3). This finding results in the identification of CH25H as one of the IFN-stimulated genes and 25HC as a potent inhibitor of viral infection (4,5). In vitro, 25HC can inhibit growth of multiple viruses in cells by blocking viral entry. The inhibition of viral infection by IFNs is also related to induction of CH25H expression and 25HC production (4,5). In vivo, CH25H-deficient mice are more susceptible to viral infection than wild-type mice (4). 25HC also functions as an amplifier of inflammatory signaling via the activator protein 1 signaling pathway (6) and mediates the negative-feedback pathway of IFN signaling on interleukin 1 family cytokine production and inflammasome activity (7).
Besides antiviral infection (4,5,(8)(9)(10)(11), 25HC can regulate lipid/cholesterol metabolism by interacting with sterol regulatory element-binding proteins or LXR (12). LXR plays various biological roles, particularly in lipid metabolism (13). Binding of a ligand to LXR results in formation of a heterodimer between LXR and retinoid X receptor (RXR), the LXR/RXR complex. The LXR/RXR complex then binds to the LXR response elements in the promoter and initiates transcription of the target genes (14). Previously, we identified several LXR response elements in the CH25H promoter, and found that both 25HC and synthetic LXR ligand [T0901317 (T317) or GW3965] induced CH25H expression in different cell types. Furthermore, treatment of mice with GW3965 increased CH25H expression in liver and peritoneal macrophages (15).
Expression of CH25H can be activated by IFNs (4). Interestingly, we have reported that LXR activation induced IFN- expression, particularly in macrophages (16). Administration of LXR ligand to mice inhibited xenograft-or carcinogen-induced tumor growth in an IFN--dependent manner (16)(17)(18). 25HC can be further metabolized into 25HC-3-sulfate (25HC3S) in a reaction catalyzed by cholesterol sulfotransferase-2B1b (SULT2B1b) (19). Taken together, these studies suggest that LXR activation, interaction between CH25H and IFN-, and 25HC metabolism may form an antiviral system that can regulate 25HC production and its antiviral actions, with the central role played by LXR.

Western blot analysis
After treatment, cellular proteins were extracted. Expression of CH25H, LXR, LXR, IFN-, SULT2B1b protein, and total HSV-1 proteins in cellular lysate was determined by Western blot as described (15). Expression of GAPDH or -tubulin was determined as loading control.

Immunofluorescent staining
After treatment, levels of HSV-1 proteins in intact HepG2 cells were determined by immunofluorescent staining as described (23). Briefly, cells were fixed with 4% paraformaldehyde for 30 min, washed with PBS for 10 min, and permeabilized in 0.5% Triton X-100/PBS for 10 min. Cells were then blocked with 2% BSA for 2 h at room temperature. After incubation with rabbit anti-HSV-1 protein antibody overnight at 4°C, cells were incubated with FITC-conjugated secondary antibody for 2 h. Cells were then stained with DAPI solution to detect the nucleus followed by observation and photographs with a fluorescence microscope (Leica, Wetzlar, Germany).

Determination of virus growth
Cells were pretreated with LXR ligand for 24 h followed by infection with HSV-1 for 2 h. After washing with PBS, cells were cultured in fresh complete medium or medium containing LXR ligand for 16 h. Cells were then lysed, followed by determination of HSV-1 proteins in cellular lysate by Western blot. The HSV-1infected HepG2 cells were also used to determine infecting viruses by immunofluorescent staining with anti-HSV-1 protein antibody and the protocol as described above.
The inhibition of LXR ligand on HSV-1 infection in HepG2 cells was also determined by viral plaque formation assay. HepG2 cells were pretreated with 25HC or T317 for 24 h followed by HSV-1 infection for 2 h. After removal of viruses, HepG2 cells were treated with 25HC or T317 for the indicated times. The infected HepG2 cells were harvested and the infecting viruses in HepG2 cells were released by repeated freezing and thawing. The cellular lysate was collected as the source of viruses. The collected viruses were diluted with 199v medium and then added to the monolayer of Vero cells. After viral growth for more than 24 h, Vero cells were observed under a microscope and the plaques formed were counted. The virus titers were calculated and normalized by the dilution factor.
The infecting MLV-(VSV)-GFP pseudotyped viruses in HepG2 cells were determined by two methods, image assay and fluorescence-activated cell sorting (FACS) assay, based on the fact that the viruses were labeled with GFP. In an image assay, after infection, the virus-infected cells are observed under a fluorescence microscope and the cells' images are photographed. In a FACS assay, the infected cells are applied to an FACS machine to quantify infected cells, using the negative control cells (uninfected HepG2) as the set for gating. In this study, after infection and treatment, HepG2 cells were collected and then observed under a fluorescence microscope. Images of cells with fluorescence or phase contrast were photographed. For FACS assay, cells were harvested and subjected to the FACS machine directly to quantify cells containing GFP. Based on the gate with negative control cells, the percentage of MLV-(VSV)-GFP pseudotyped virusinfected cells out of total cells was determined.

CRISPR/Cas9-mediated mutations
HepG2 cells lacking LXR, LXR, CH25H, or SULT2B1 expression were established using the clustered regulatory interspaced short palindromic repeat (CRISPR)/CRISPR-associated protein 9 (Cas9) technology, respectively (24). The guide sequence was designed based on the online CRISPR Design Tool (http://tools. genome-engineering.org), and the sequences of the guide oligos are listed in Table 1. After ligation, HepG2 cells were transfected with plasmid of pSpCas9 (BB)-2A-Puro vector or vector ligated with guide oligos, respectively. The selection of mutated clonal cell lines was completed using the standard protocol (24), and the knockout of target genes was confirmed by Western blot. The cells lacking LXR, LXR, CH25H, or SULT2B1b expression were defined as CRISPR-LXR, CRISPR-LXR, CRISPR-CH25H, or CRISPR-SULT2B1b cells, while the corresponding control cells were defined as CRISPR-Ctrl cells.

In vivo study
The protocols for in vivo study with mice were approved by the Ethics Committee of Nankai University (Tianjin, China) and conform to the Guide for the Care and Use of Laboratory Animals published by the National Institutes of Health. BALB/c mice (6 weeks old) were purchased from Beijing Vital River Laboratory Animal Technology Co., Ltd. (Beijing, China) and maintained at the Animal Center of Nankai University with free access to water and food. The mice were randomly divided into three groups and received the following treatment: mice in groups 1 and 2 were fed normal chow, and the mice in group 3 were fed normal chow containing T317 (5 mg/day/kg bodyweight) for 4 days. Mice in group 1 were then intraperitoneally injected with PBS (as a mock); mice in groups 2 and 3 were intraperitoneally injected with HSV-1 (5 × 10 5 PFU/mouse). Mice in groups 1 and 2 continued to be fed normal chow, while the mice in group 3 were fed normal chow containing T317. Seven days after viral injection, all the mice were euthanized. Mouse peritoneal fluid was first collected by lavage with PBS (2 ml/mouse), and it was named "peritoneal washing fluid (PWF)". Liver and brain samples were then collected individually. A piece of liver or brain stem was weighed and then homogenized in PBS (0.1 g/ml). HSV-1 in PWF or homogenates of liver or brain stem were released by repeated freezing and thawing, the viral titers in mouse tissues were determined by the plaque formation assay as described above.

Data analysis
All experiments were repeated at least three times, and the representative results are presented. Data are presented as mean ± SEM and were analyzed by two-tailed unpaired Student's t-test or post hoc test of one-way ANOVA analysis. The difference was considered significant if P < 0.05.

LXR activation inhibits infection of HSV-1 or MLV-(VSV)-GFP in HepG2 cells
CH25H has been identified as an antiviral molecule because it catalyzes the production of 25HC, a potent antiviral small chemical. In addition, CH25H is an IFN-inducible molecule (4,5). Interestingly, we have reported that expression of hepatic CH25H or macrophage IFN- can be activated by LXR (15,16). Based on the above studies, we hypothesized that LXR activation may play an important role in antiviral infection by activating CH25H expression.
To test this, we initially infected HepG2 cells with HSV-1 and determined CH25H expression in response to viral infection. In contrast to the previous report that indicates viral infection can activate macrophage CH25H mRNA expression (5), we found that HSV-1 infection had little effect on hepatic CH25H protein expression (Fig. 1A). This difference may be due to the fact that macrophages are a major cell type expressing IFNs, and viral infection to macrophages can induce IFN production, which, in turn, induces CH25H mRNA expression (5). Meanwhile, HSV-1 infection had little effect on 25HC-or T317-induced CH25H expression in HepG2 cells (Fig. 1B).
Next, we determined that pretreatment of HepG2 cells with 25HC or T317 reduced cellular HSV-1 protein levels in a dose-dependent manner with the greater effect by 25HC indicating either of them inhibits HSV-1 infection (Fig. 1C). The greater inhibition by 25HC than T317 should be partially attributed to the action of exogenously added 25HC. The results of immunofluorescent staining of cellular HSV-1 proteins show that the fluorescent intensity was substantially reduced by 25HC or T317 (Fig. 1D), which directly demonstrates that LXR activation inhibits viral infection.
To further determine inhibition of HSV-1 growth by 25HC or T317, the 25HC-or T317-pretreated HepG2 cells were infected with HSV-1, and then continually exposed to 25HC or T317 for different times. The viruses collected from the above HepG2 cells were added to Vero cells for 36 h and the formed plaques were counted. The results of the virus titer assay shown in Fig. 1E confirm that 25HC and T317 inhibited viral growth in HepG2 cells dose dependently.
To determine the effect of LXR on infection of other viruses in HepG2 cells, the pretreated HepG2 cells with LXR ligand were infected with MLV-(VSV)-GFP pseudotyped viruses. Because MLV-(VSV)-GFP pseudotyped viruses are labeled with GFP, we are able to determine viral infection using either image assay or FACS assay. As shown in Fig. 2A, B, LXR ligands (25HC, T317, or GW3965) inhibited growth of MLV-(VSV)-GFP pseudotyped viruses in a dose-dependent manner. To determine the role of LXR or CH25H expression in antiviral infection, we selectively inhibited LXR or CH25H expression by transfecting cells with the corresponding siRNA. Indeed, inhibition of LXR or CH25H expression by siRNA increased the cells' susceptibility to MLV-(VSV)-GFP pseudotyped virus infection, while the inhibition of viral infection by T317 or 25HC was attenuated (Fig. 2C, D).

The antiviral action of 25HC mainly depends on LXR-induced CH25H expression
We created HepG2 cells lacking either LXR or LXR expression by CRISPR-Cas9 method (right half of Fig. 3A, D) and infected control HepG2 cells or LXR or LXR  (Fig. 3B, C, E, F) (15). The direct evidence demonstrating the importance of LXR-induced CH25H expression in 25HC-inhibited viral infection was obtained by the following experiment. HepG2 cells lacking CH25H expression (CRISPR-CH25H cells, Fig. 3G) were cultured in fresh medium for 24 h.   The conditioned media were collected from CRISPR-Ctrl and CRISPR-CH25H cells, respectively, and then used to culture HSV-1 pre-infected HepG2 cells for 16 h. Compared with cells cultured in nonconditioned medium, reduced HSV-1 growth was determined in cells cultured in the conditioned medium collected from CRISPR-Ctrl cells. However, little reduction of HSV-1 growth was determined in the cells cultured in the conditioned medium collected from CRISPR-CH25H cells (Fig. 3H). The reduced viral growth in cells cultured in the conditioned medium collected from CRISPR-Ctrl cells should be attributed to the secreted 25HC. Similar to CRISPR-LXR or CRISPR-LXR cells, inhibition of HSV-1 infection by 25HC or T317 was substantially reduced in CRISPR-CH25H cells (Fig. 3I, J).
To compare the effects of LXR, LXR, and CH25H expression on cell susceptibility to HSV-1 infection, CRISPR-Ctrl, CRISPR-LXR, CRISPR-LXR, or CRISPR-CH25H cells were infected with HSV-1 at the same titers for 24 h followed by determination of viral growth. Compared with CRISPR-Ctrl cells, Fig. 3K and L demonstrate that lack of LXR, LXR, or CH25H expression increased cell susceptibility to HSV-1 infection in an order of CH25H /  LXR / ≈ LXR / , confirming the importance of LXR and CH25H expression in antiviral infection.

Inhibition of viral infection by LXR is correlated to activation of CH25H expression in a cell type-dependent manner
IFN- is an LXR target (16) while it can induce CH25H expression (4). Therefore, LXR-induced CH25H expression can be further enhanced in cells expressing IFN-. Reciprocally, lack of IFN- expression reduced, but did not block, LXR-induced CH25H expression (15). Therefore, the lack of IFN- expression may result in increased cell susceptibility to viral infection and reduced antiviral actions of LXR. Similar to HepG2 cells, primary hepatocytes isolated from wild-type mice can also be infected by HSV-1 (Fig.  4A). Compared with wild-type hepatocytes, deficiency of IFN- expression moderately increased cell susceptibility to HSV-1 infection (lane 5 vs. lane 1, Fig. 4B). In addition, the antiviral actions of 25HC and T317 (lanes 2-4 vs. lane 1, Fig. 4B) were reduced in IFN- / hepatocytes (lanes 6-8 vs. lanes 2-4, Fig. 4B), which should be related to the induction of CH25H expression by IFN- having not occurred in IFN--deficient cells.
Activation of CH25H expression by IFNs is believed to be an important antiviral mechanism of IFNs in macrophages (4,5). LXR also induces macrophage CH25H expression (15), indicating that either T317 or 25HC can inhibit HSV-1 infection in macrophages. Initially, we compared expression patterns of CH25H and IFN- between HepG2 cells and RAW 264.7 macrophages, which can be used to correlate the inhibitory effect of LXR on viral infection with the levels of CH25H or IFN- expression. Figure 5A (upper panel) shows that little CH25H protein was presented in macrophages, while abundant CH25H protein was expressed by HepG2 cells. In contrast, IFN- was mainly expressed by macrophages, but not hepatocytes. However, 25HC treatment induced IFN- expression in RAW 264.7 macrophages, not HepG2 cells (lower panel, Fig. 5A). In contrast, T317 substantially induced CH25H expression in HepG2 cells, while slightly affecting it in RAW 264.7 cells. Thus, CH25H protein levels in HepG2 cells are much higher than in RAW 264.7 macrophages, at both the basal level and induction by LXR (top row, Fig. 5B). The higher expression of CH25H in HepG2 cells should be related to the higher expression of LXR/ in HepG2 cells (middle rows, Fig. 5B).
A previous study indicates that 25HC inhibits viral infection to mouse embryo fibroblasts in an LXR-independent pathway (5). We propose that the reason why T317 failed to inhibit viral growth in mouse embryo fibroblasts is due to a low basal level of CH25H or a poor response to LXR activation in the cells. Compared with HepG2 cells, when T317 concentration was increased up to 10 M (50-fold of that used in HepG2 cells), it clearly inhibited HSV-1 infection to RAW 264.7 macrophages (Fig. 5C).
The lower levels of CH25H in RAW 264.7 cells than in HepG2 cells suggest that macrophages might be more susceptible to viral infection, while T317 or 25HC may have reduced inhibitory effect on viral infection in macrophages. Indeed, in control cells, Fig. 5D or E demonstrates that more HSV-1 viruses were presented in RAW 264.7 cells than in HepG2 cells (lane 1 vs. lane 4). Meanwhile, T317 at low concentrations moderately inhibited HSV-1 infections in HepG2 cells (lane 2 or 3 vs. lane 1, Fig. 5D), but had no effect on viral infection in RAW 264.7 cells (lane 5 or 6 vs. lane 4). Similarly, 25HC had a more potent inhibitory effect on viral infection in HepG2 cells than in RAW 264.7 macrophages (Fig. 5E). Thus, the results in Fig. 5 suggest that the antiviral actions of LXR can be correlated to the basal levels of cellular CH25H protein and its response to LXR activation, and are unrelated to cellular IFN- protein.
The results above also indicate that SUL2B1b expression can impact the antiviral actions of 25HC by enhancing conversion of 25HC into 25HC3S. Indeed, when HepG2 cells were transfected with SULT2B1b expression vector, the high expressing SULT2B1b increased cell susceptibility to HSV-1 infection (left half, Fig. 6F). It also reduced the inhibitory effect of 25HC on HSV-1 infection (right half, Fig. 6F). In contrast, lack of SULT2B1b expression had little effect on CH25H expression, although it moderately activated LXR expression (Fig. 6G). Interestingly, deficiency of SULT2B1b expression did not reduce cell susceptibility to HSV-1 infection or influence the antiviral effects of 25HC (Fig. 6H), indicating that the endogenous SULT2B1b activity is not high enough to regulate cellular 25HC homeostasis or the antiviral actions of 25HC. Similar to CRISPR-Ctrl cells, treatment of CRISPR-CH25H cells with 25HC3S inhibited HSV-1 infection in a concentration-dependent manner (Fig. 6I), suggesting that 25HC3S inhibits viral infection directly. However, a greater inhibitory effect of 25HC3S on HSV-1 infection in CRISPR-Ctrl cells than in CRISPR-CH25H cells was determined, which should be attributed to activation of CH25H expression by 25HC3S in CRISPR-Ctrl cells (Fig. 6A, B).

T317 reduces viral growth in mouse tissues
Our results above demonstrate that LXR activation inhibits viral infection in HepG2 cells or RAW 264.7 macrophages. To determine the physiological relevance of LXR activation, we prefed BALB/c mice with normal chow or normal chow containing T317 (5 mg/day/kg bodyweight) for 4 days. Mice were then intraperitoneally injected with HSV-1 at the same titers. Meanwhile, a group of mice fed normal chow were injected with PBS as a mock treatment. After HSV-1 injection, the feeding of normal chow or normal chow containing T317 was continued for 7 days.
After HSV-1 injection, we checked food intake, water drinking, and the external appearance of the animals daily. Although we did not observe differences of food intake/ water drinking among the groups with mock, HSV-1, or HSV-1 plus T317 treatment, compared with mice receiving mock treatment, mice injected with HSV-1 alone had fur with a hunched posture, piloerection, and a slight dark color. However, mice that received HSV-1 and T317 treatment had little difference of external appearance from that of mice with mock treatment (Fig. 7A).
The effect of T317 treatment on viral growth in vivo was determined by the plaque formation assay. At the end of the experiment, mouse peritoneal fluid was first collected by lavage with PBS followed by liver and brain samples. A piece of liver or brain stem was homogenized in PBS. HSV-1 in PWF or homogenates of liver or brain stem were released and used to determine viral titers. As shown in Fig. 7B, after injection, viral growth can occur to the liver. Treatment of mice with T317 reduced viral growth substantially in liver and peritoneal fluid, but only moderately in brain stem (Fig. 7B). Thus, the results in Fig. 7 suggest the protection of LXR against viral infection in vivo.

DISCUSSION
25HC has been well-documented as a potent antiviral molecule (4,5,(8)(9)(10)(11), indicating the importance of cellular 25HC homeostasis in antiviral actions. Cellular 25HC levels are determined by both CH25H activity and activity of the enzyme catalyzing 25HC metabolism, such as SULT2B1b (27,30). Our previous study demonstrates that CH25H can be activated by LXR ligands, implying that LXR can inhibit viral infection (15). In the current study, we observed that T317 or GW3965 inhibited viral infection in different cell types in vitro and mouse tissues in vivo (Figs. 1, 2, 5, 7). In contrast, lack of LXR and CH25H expression increased cell susceptibility to viral infection (Figs. 2, 3), in the order of CH25H /  LXR / ≈ LXR / (Fig. 3K, L). Meanwhile, the antiviral activity of LXR in these cell types was attenuated (Fig. 3C, F, J), which is attributed to either reduced induction or no induction of CH25H expression in LXR/ / or CH25H / HepG2 cells.
CH25H is an IFN-inducible gene (3)(4)(5), while IFN- can be activated by LXR (16)(17)(18), indicating that IFN- can facilitate LXR-activated CH25H expression/25HC production and antiviral actions of 25HC. Indeed, lack of IFN- expression reduces basal levels of CH25H and attenuates, but does not block, LXR-activated CH25H expression (15). Consequently, lack of IFN- expression increased cell susceptibility to viral infection and reduced LXR-inhibited viral infection (Fig. 4). Furthermore, the expression/ induction of CH25H, but not of IFN-, can be inversely correlated to cell susceptibility to viral infection and the antiviral effect of LXR (Fig. 5).
25HC can be metabolized into 25HC3S by SULT2B1b. Therefore, both SULT2B1b and 25HC3S may influence the antiviral actions of 25HC. Indeed, compared with 25HC, 25HC3S is a weaker activator for CH25H expression (Fig. 6C) and a weaker inhibitor of viral growth (Fig. 6E), although 25HC3S can directly inhibit viral infection (Fig. 6I). Therefore, high expression of SULT2B1b increased cell susceptibility to HSV-1 infection and attenuated 25HC-inhibited viral infection (Fig. 6F). Intriguingly, SULT2B1b expression can be activated by LXR ligands, including 25HC (31). Although LXR may induce 25HC production and IFN- expression in a positive loop, activation of SULT2B1b expression by LXR can enhance the conversion of 25HC into 25HC3S, which should be an important mechanism regulating 25HC/ IFN- homeostasis to protect cells against the cytotoxicity of 25HC or IFN- at high concentrations.
Although 25HC/CH25H demonstrates potent antiviral functions, regulation of CH25H expression and 25HC homeostasis has not been fully understood. In this study, we found several signaling pathways that may play important roles in the antiviral actions of 25HC. Briefly, 25HC functions as an LXR ligand to induce its own production by activating CH25H expression. Meanwhile, 25HC enhances IFN- expression and, consequently, the activated IFN- feedback enhances CH25H expression/ 25HC production, indicating that the interaction between CH25H and IFN- is involved in 25HC-inhibited viral infection. Finally, SULT2B1b expression can keep 25HC-activated CH25H and IFN- expression under control, an important mechanism regulating 25HC homeostasis/functions. These pathways form an important antiviral infection system in which LXR plays a central role (Fig. 8). Fig. 7. Administration of T317 to mice reduces viral growth in tissues. BALB/c mice were randomly divided into three groups. Mice in the mock or control groups were fed normal chow, while mice in T317 group were fed normal chow containing T317 (5 mg/day/kg bodyweight) for 4 days. Mice in the mock group were then injected with PBS intraperitoneally and the rest mice were intraperitoneally injected with HSV-1 (5 × 10 5 PFU). Feeding of normal chow or normal chow plus T317 was continued for all mice. A: Mice were photographed at day 4 of viral injection. B: Seven days after viral injection, all mice were euthanized, followed by collection of PWF and liver and brain stem samples. The viral titers in mouse tissues were determined by plaque formation assay. *P < 0.05 (n = 5). Fig. 8. The model depicts the antiviral system of LXR with involvement of activation of CH25H expression, interaction between IFN- and CH25H, and 25HC metabolism. Based on the results in this study and our previous report (15), we obtained the following findings: 1 (circled), 25HC functions as an LXR ligand and induces CH25H expression; 2 (circled), 25HC activates IFN- expression and, in turn, activated IFN- induces CH25H expression; 3 (circled), 25HC induces SULT2B1b expression to enhance the conversion of 25HC into 25HC3S. These three pathways work cooperatively and result in: 1) 25HC efficiently and continuously inhibits viral infection; 2) IFN- can enhance, but not determine, the antiviral actions of 25HC; and 3) 25HC homeostasis and antiviral actions are further regulated through its metabolism by action of SULT2B1b. Furthermore, in the cells with high CH25H expression, such as hepatocytes, the auto-induction of CH25H expression/25HC production substantially increases the resistance of cells to viral infection. In contrast, in cells with low CH25H expression and high IFN- expression, such as macrophages, the cell susceptibility to viral infection is increased while the inhibitory effects of 25HC or LXR are reduced. Taken together, our study demonstrates an antiviral system formed by activation of CH25H expression, interaction between CH25H and IFN-, and 25-HC metabolism in which LXR plays a central role.