Pseudorabies Virus Inhibits Expression of Liver X Receptors to Assist Viral Infection

Pseudorabies virus (PRV) is a contagious herpesvirus that causes Aujeszky’s disease and economic losses worldwide. Liver X receptors (LXRs) belong to the nuclear receptor superfamily and are critical for the control of lipid homeostasis. However, the role of LXR in PRV infection has not been fully established. In this study, we found that PRV infection downregulated the mRNA and protein levels of LXRα and LXRβ in vitro and in vivo. Furthermore, we discovered that LXR activation suppressed PRV proliferation, while LXR inhibition promoted PRV proliferation. We demonstrated that LXR activation-mediated reduction of cellular cholesterol was critical for the dynamics of PRV entry-dependent clathrin-coated pits. Replenishment of cholesterol restored the dynamics of clathrin-coated pits and PRV entry under LXR activation conditions. Interestingly, T0901317, an LXR agonist, prevented PRV infection in mice. Our results support a model that PRV modulates LXR-regulated cholesterol metabolism to facilitate viral proliferation.


Introduction
Pseudorabies (PR), also called Aujeszky's disease, is a highly infectious disease caused by the PR virus (PRV), which is a member of the subfamily Alphaherpesvirinae of the family Herpesviridae. The genome of PRV is approximately 143 kb encoding at least 70 open reading frames [1]. PRV can infect a wide variety of mammals, including pigs, sheep, and cattle, causing severe clinical symptoms and death [2]. Although scientists have been trying to develop diagnostic approaches and vaccines in recent years, PR remains an important infectious disease that is prevalent in many countries. Several recent reports have suggested that PRV can cause human endophthalmitis and encephalitis [3][4][5]. These findings indicate that PRV infection is a potential public health risk and not limited to the swine industry. Therefore, new methods are urgently needed to prevent PRV infection.
The liver X receptors (LXRs), a family of transcription factors in the nuclear receptor superfamily, are ligand-activated transcription factors and pivotal regulators of cholesterol and lipid metabolism [6,7]. Two LXR subtypes, LXRα and LXRβ, have been identified. While LXRβ is expressed ubiquitously, LXRα is expressed highly in the liver, spleen, intestine, heart, and macrophages [8]. Ligand binding to LXR results in the formation of a

Mice
We purchased female 6-8-week-old BALB/c mice from the Center of Experimental Animal of Zhengzhou University (Zhengzhou, China). Mice were housed in a specific pathogen-free animal facility at Henan Agricultural University. Animal experiments were performed in accordance with protocols approved by the Use of National Research Center for Veterinary Medicine (Permit 20180521047).
The virulent PRV isolate QXX (PRV-QXX) was kindly donated by Yong-Tao Li from the College of Veterinary Medicine, Henan Agricultural University [20]. The recombinant PRV strain of PRV-GFP, derived from the PRV Hubei strain with the TK gene replaced by a GFP expression cassette from the pEGFP-N1 plasmid, was kindly donated by Han-Zhong Wang from Wuhan Institute of Virology, Chinese Academy of Sciences [21].
Full-length porcine AP2B1 cDNA was cloned into the mCherry-N1 expression plasmid using the BamHI and KpnI restriction sites.

Cell Viability Assays
PK-15 cells were seeded at 1 × 10 4 per well in 96-well plates. On the next day, the medium was changed to DMEM/10% FBS supplemented with various concentrations of LXR agonists for 24-48 h. CCK-8 (10 µL, DingGuo, Beijing, China) was then added to each well, and the cells were incubated for 3 h at 37 • C. Absorbance was detected at 450 nm with a microplate reader (Varioskan Flash; Thermo Fisher Scientific).

Flow Cytometry Assay
For green fluorescent protein (GFP) reporter assays, PK-15 cells were infected with PRV-GFP [multiplicity of infection (MOI) = 0.01] for 36 h. Cells were digested with trypsin-EDTA (Gibco), collected by centrifugation, and suspended in PBS. The percentage of GFP-positive cells was measured by flow cytometry on a Beckman CytoFLEX instrument (Brea, CA, USA). All data were analyzed with CytExpert software 2.0.

Immunoblotting Analysis
Cells were collected by centrifugation and lysed in RIPA buffer (Beyotime, Shanghai, China) in the presence of protease and phosphatase inhibitor cocktail (MedChemExpress). The protein concentration was determined by a BCA Protein Assay Kit (DingGuo). Equivalent amounts of total protein (30 µg) were subjected to SDS-PAGE for immunoblotting. The target proteins were detected with specific primary antibodies and appropriate horseradish peroxidase (HRP)-conjugated secondary antibodies. Visualization was performed with Luminata Crescendo Western HRP Substrate (Millipore, Billerica, MA, USA) on a GE AI600 imaging system.

Cell Surface Biotinylation Assay
Cells were incubated in ice-cold PBS-CM (0.1 mM CaCl 2 , 1 mM MgCl 2 ) in the presence of 1 mg/mLEZ-Link NHS-biotin (Thermo Fisher Scientific) for 30 min at 4 • C. After two washes with ice-cold PBS-CM, cells were cultured in medium containing 10 mM glycine for 30 min at 37 • C. Cytosolic and membrane fractions were prepared as previously described [22]. Briefly, the cells were homogenized by passing through a #7 needle 30 times in 0.5 mL of homogenization buffer (10 mM HEPES [pH 7.4], 10 mM KCl, 1.5 mM MgCl 2 , 5 mM sodium EDTA, 5 mM sodium EGTA, 250 mM sucrose) supplemented with protease and phosphatase inhibitors (MedChemExpress) and centrifuged at 1000× g at 4 • C for 7 min. The pellet, containing the crude nuclear fraction, was discarded, and the supernatant was centrifuged at 12,000× g at 4 • C for 15 min. The resulting supernatant was the cytosol, and the pellet containing the membrane fraction was dissolved in lysis buffer (10 mM Tris-HCl [pH 6.8], 100 mM NaCl, 1% SDS, 1 mM EDTA, 1 mM EGTA) supplemented with protease and phosphatase inhibitors (MedChemExpress). Each fraction was incubated with NeutrAvidin-agarose (Thermo Fisher Scientific) and rotated for 2 h at 4 • C. After three washes with homogenization buffer (10 mM HEPES pH 7.4, 10 mM KCl, 1.5 mM MgCl 2 , 5 mM EDTA, 5 mM EGTA, 250 mM sucrose), biotinylated proteins on NeutrAvidin-agarose were eluted with SDS-PAGE sample buffer and subjected to immunoblotting analysis.

Fluorescence Recovery after Photobleaching (FRAP)
HeLa cells were transfected with the AP2B1-mCherry plasmid for 24 h. After 8 h of pre-treatment with the indicated compound, the cells were bleached at maximum laser intensity for 30 s in a region of 7 × 7 µm 2 and then imaged for 5 min at 37 • C. CCP dynamics was defined by the fluorescence recovery of AP2B1-mCherry, which was performed on a Zeiss LSM 800 confocal microscope.

Histological Analysis
Animal tissues were fixed in 4% paraformaldehyde and embedded in paraffin. The paraffin blocks were sectioned (7 µm) for hematoxylin-eosin staining.

Statistical Analysis
All data were obtained from three independent experiments for quantitative analyses and expressed as the mean ± standard error. All statistical analyses were performed with a two-tailed Student's t test. Significant differences relative to the corresponding controls were accepted at * p < 0.05. For mouse survival studies, Kaplan-Meier survival curves were generated and analyzed for statistical significance.

PRV Infection Inhibits LXRα and LXRβ Expression In Vitro and In Vivo
To determine the role of LXR in PRV infection, we evaluated the expression of LXR under PRV challenge in vitro. Cells were infected with PRV-QXX for 0-24 h, and cells were processed to measure the mRNA and protein levels of LXRα and LXRβ. PRV infection caused a reduction in Lxra and Lxrb mRNA in PK-15 and 3D421 cells ( Figure 1A,B). Consistent with the mRNA levels, LXRα and LXRβ protein levels in PK-15 and 3D421 cells were all downregulated in response to PRV infection ( Figure 1C,D). These results suggested that PRV inhibited LXRα and LXRβ expression in vitro.
under PRV challenge in vitro. Cells were infected with PRV-QXX for 0-24 h, and cell were processed to measure the mRNA and protein levels of LXRα and LXRβ. PRV infec tion caused a reduction in Lxra and Lxrb mRNA in PK-15 and 3D421 cells ( Figure 1A,B) Consistent with the mRNA levels, LXRα and LXRβ protein levels in PK-15 and 3D421 cells were all downregulated in response to PRV infection ( Figure 1C,D). These result suggested that PRV inhibited LXRα and LXRβ expression in vitro. We verified whether PRV reduced LXR expression in vivo. Mice were mock infected or intranasally infected with PRV-QXX for 3 days, and the lungs were assessed fo mRNA and protein levels of LXRα and LXRβ by qRT-PCR and immunoblotting analysis PRV infection resulted in a >two-fold decrease in Lxra and Lxrb mRNAs as compared to that in mock-infected lungs, as well as the protein levels of LXRα and LXRβ ( Figure 1E,F) These data indicated that PRV infection suppressed LXR expression both in vitro and in vivo.

Inhibition of LXR Increases PRV Infection
We aimed to determine whether LXR was involved in PRV infection. SR9243 is an inverse agonist of LXR that induces LXR-co-repressor interaction and downregulate LXR-mediated gene expression [24]. As expected, treatment of PK-15 cells with SR9243 inhibited the transcription of LXR target genes, such as Abca1 and Abcg1 (Figure 2A) The mRNA levels of PRV gB in SR9243-treated cells were significantly higher than those in control cells ( Figure 2B). This indicated that SR9243 promoted transcription of PRV genes. PRV gE expression was enhanced in an SR9243 dose-dependent manner ( Figure  2C). We next detected the multiplication of PRV progeny virus in response to SR9243 using a viral titer assay. PK-15 cells were infected with PRV-QXX (MOI = 0.1 and 1.0) and treated with SR9243 (0-10 μM) for 24 h. SR9243 significantly promoted the production o PRV progeny virus ( Figure 2D). To gain further insight into the effect of SR9243 on PRV We verified whether PRV reduced LXR expression in vivo. Mice were mock infected or intranasally infected with PRV-QXX for 3 days, and the lungs were assessed for mRNA and protein levels of LXRα and LXRβ by qRT-PCR and immunoblotting analysis. PRV infection resulted in a >two-fold decrease in Lxra and Lxrb mRNAs as compared to that in mock-infected lungs, as well as the protein levels of LXRα and LXRβ ( Figure 1E,F). These data indicated that PRV infection suppressed LXR expression both in vitro and in vivo.

Inhibition of LXR Increases PRV Infection
We aimed to determine whether LXR was involved in PRV infection. SR9243 is an inverse agonist of LXR that induces LXR-co-repressor interaction and downregulates LXRmediated gene expression [24]. As expected, treatment of PK-15 cells with SR9243 inhibited the transcription of LXR target genes, such as Abca1 and Abcg1 (Figure 2A). The mRNA levels of PRV gB in SR9243-treated cells were significantly higher than those in control cells ( Figure 2B). This indicated that SR9243 promoted transcription of PRV genes. PRV gE expression was enhanced in an SR9243 dose-dependent manner ( Figure 2C). We next detected the multiplication of PRV progeny virus in response to SR9243 using a viral titer assay. PK-15 cells were infected with PRV-QXX (MOI = 0.1 and 1.0) and treated with SR9243 (0-10 µM) for 24 h. SR9243 significantly promoted the production of PRV progeny virus ( Figure 2D). To gain further insight into the effect of SR9243 on PRV infection, we assessed the growth kinetics of PRV under SR9243 treatment. TCID 50 assay of viral titer indicated that SR9243 enhanced the production of the PRV progeny virus at 8 h post-treatment ( Figure 2E). We also determined whether knockdown of LXRα and LXRβ improved PRV infection. Simultaneous interference LXRα and LXRβ expressions increased the production of PRV progeny virus ( Figure 2F,G). These data demonstrated that inhibition of LXR benefited PRV infection. infection, we assessed the growth kinetics of PRV under SR9243 treatment. TCID50 assay of viral titer indicated that SR9243 enhanced the production of the PRV progeny virus at 8 h post-treatment ( Figure 2E). We also determined whether knockdown of LXRα and LXRβ improved PRV infection. Simultaneous interference LXRα and LXRβ expressions increased the production of PRV progeny virus ( Figure 2F,G). These data demonstrated that inhibition of LXR benefited PRV infection. simultaneously treated with SR9243 (0-10 μM) for 24 h. Viral titers were assessed by a TCID50 assay. * p < 0.05, ** p < 0.01, *** p < 0.001. (E) PK-15 cells were infected with PRV-QXX (MOI = 0.1) and simultaneously treated with SR9243 (10 μM) for 2-24 h. One-step growth curves of PRV-QXX were assessed using a TCID50 assay of viral titers. * p < 0.05, ** p < 0.01. ns, no significance. (F) PK-15 cells were transfected with NC and siLXRα/β for 48 h. LXRα and LXRβ were assessed by immunoblotting analysis. (G) PK-15 cells were transfected with NC and siLXRα/β. At 24 h post-transfection, cells were infected with PRV-QXX (MOI = 1) for another 24 h. Viral titers were assessed by a TCID50 assay. ** p < 0.01.
inhibitory effect of LXR agonists on PRV infection by a viral titer assay. PK-15 cells wer infected with PRV-QXX (MOI = 0.1 and 1) and treated with LXR-623 (0-6 μM), T090131 (0-6 μM), 22R-HC (0-6 μM), and GW3965 (0-3 μM) for 24 h. Multiplication of the PRV progeny virus decreased with an increased concentration of LXR agonists ( Figure 3C PRV gB and gE expression was inhibited by LXR agonists ( Figure 3D). The growth ki netics of PRV assessed by TCID50 assay of viral titer indicated that LXR agonists de creased the production of PRV progeny virus at 8 h post-treatment ( Figure 3E). Thes data suggested that LXR played a negative role in PRV infection.

Activation of LXR Inhibits PRV Entry
Next, we sought to determine which stage of viral life cycle was influenced by LXR agonists and inverse agonists in a time-of-addition assay. We examined whether activation of LXR could influence PRV attachment to cells. We pretreated PK-15 cells with LXR agonists for 8 h, and infected cells with PRV-QXX combined with LXR agonists for 1 h at 4 • C. After three washes with ice-cold PBS, we analyzed viral attachment by quantification of the PRV genome copy number by qRT-PCR analysis. LXR-623, T0901317, 22R-HC, and GW3965 did not affect PRV attachment to cells ( Figure 4A). We next performed a viral entry assay by quantification of the PRV genome copy number in cells. qRT-PCR analysis indicated that LXR agonists inhibited PRV entry ( Figure 4B). We also assessed PRV entry by immunoblotting analysis of PRV gE. PRV gE was decreased in cells treated with LXR agonists, which further indicated that LXR agonists inhibited PRV entry ( Figure 4C).

Activation of LXR Inhibits PRV Entry
Next, we sought to determine which stage of viral life cycle was influenced by LXR agonists and inverse agonists in a time-of-addition assay. We examined whether activation of LXR could influence PRV attachment to cells. We pretreated PK-15 cells with LXR agonists for 8 h, and infected cells with PRV-QXX combined with LXR agonists for 1 h at 4 °C. After three washes with ice-cold PBS, we analyzed viral attachment by quantification of the PRV genome copy number by qRT-PCR analysis. LXR-623, T0901317, 22R-HC, and GW3965 did not affect PRV attachment to cells ( Figure 4A). We next performed a viral entry assay by quantification of the PRV genome copy number in cells. qRT-PCR analysis indicated that LXR agonists inhibited PRV entry ( Figure 4B). We also assessed PRV entry by immunoblotting analysis of PRV gE. PRV gE was decreased in cells treated with LXR agonists, which further indicated that LXR agonists inhibited PRV entry (Figure 4C).  In addition, we used LXR inverse agonists to examine whether SR9243 could promote PRV attachment and entry. qRT-PCR analysis indicated that SR9243 had no inhibitory effect on PRV attachment to cells, but it could promote PRV entry ( Figure 4D,E). Immunoblotting analysis of PRV gE indicated that SR9243 increased gE in SR9243-treated cells, suggesting that SR9243 boosted PRV entry ( Figure 4F). These results demonstrated that LXR was related to PRV entry.

PRV Infection Increases Cellular Cholesterol Content That Is Inhibited by LXR Activation
Cholesterol is critical for PRV entry [26], so we examined cellular cholesterol content by filipin staining in PRV-infected and T0901317-treated cells. PRV infection significantly increased cellular cholesterol content ( Figure 5A). However, activation of LXR by T0901317 abrogated PRV-induced enhancement of cellular cholesterol, which was restored by cholesterol replenishment ( Figure 5A). This phenomenon was verified by quantification of cellular cholesterol ( Figure 5B). We examined whether cholesterol replenishment rescued PRV entry during LXR activation. qRT-PCR indicated that PRV genome copy number in T0901317treated PK-15 cells was gradually increased with the concentration of cholesterol ( Figure 5C). Exogenous supplementation of cholesterol in T0901317-treated PK-15 cells restored the internalization of PRV gE, as indicated by immunoblotting analysis ( Figure 5D). These data suggested that LXR influenced cellular cholesterol to inhibit PRV entry.

T0901317 Inhibit CCP Dynamics through Reducing Cellular Cholesterol
Our previous study suggested that Niemann-Pick C1 deficiency attenuates PRV entry by decreasing cholesterol abundance and by inhibiting CCP dynamics [26]. Therefore, we examined whether LXR agonists acted via a similar mechanism. To corroborate the role of T0901317 in CCP dynamics, FRAP analysis was carried out with live-cell confocal microscopy imaging. Following the 20-s bleaching laser pulse, AP2B1-mCherry fluorescence rapidly recovered to about 50% of its initial value at approximately 180 s in control cells, while T0901317-treated cells did not show recovery of AP2B1-mCherry fluorescence ( Figure 6A,B). Exogenous cholesterol was able to complement the inhibitory effect of T0901317 on the recovery of AP2B1-mCherry fluorescence ( Figure 6A,B). Additionally, using a cell surface biotinylation assay, we confirmed that T0901317 had no effect on the interaction between PRV virions and AP2B1, but inhibited viral entry, which could be restored by the addition of cholesterol ( Figure 6C). These data demonstrated that activation of LXR blocked PRV entry by interfering with cholesterol-dependent CCP dynamics.
Viruses 2022, 14, x FOR PEER REVIEW 10 of 1 the role of T0901317 in CCP dynamics, FRAP analysis was carried out with live-ce confocal microscopy imaging. Following the 20-s bleaching laser pulse, AP2B1-mCherr fluorescence rapidly recovered to about 50% of its initial value at approximately 180 s i control cells, while T0901317-treated cells did not show recovery of AP2B1-mCherr fluorescence ( Figure 6A,B). Exogenous cholesterol was able to complement the inhibitor effect of T0901317 on the recovery of AP2B1-mCherry fluorescence ( Figure 6A,B). Add tionally, using a cell surface biotinylation assay, we confirmed that T0901317 had no ef fect on the interaction between PRV virions and AP2B1, but inhibited viral entry, whic could be restored by the addition of cholesterol ( Figure 6C). These data demonstrate that activation of LXR blocked PRV entry by interfering with cholesterol-dependent CC dynamics.

T0901317 Prevents PRV Infection In Vivo
To determine whether LXR agonists can be used as antivirals in vivo, we examine the protective effect of T0901317 against PRV infection. Mice were intraperitoneally in jected with T0901317 twice every 2 days before the PRV challenge. Mice were intranasall infected with PRV-QXX for 10 days. We observed that all mice died at 4 day post-infection in the vehicle-treated group ( Figure 7A). However, 92% of mice (10/12

T0901317 Prevents PRV Infection In Vivo
To determine whether LXR agonists can be used as antivirals in vivo, we examined the protective effect of T0901317 against PRV infection. Mice were intraperitoneally in-jected with T0901317 twice every 2 days before the PRV challenge. Mice were intranasally infected with PRV-QXX for 10 days. We observed that all mice died at 4 days post-infection in the vehicle-treated group ( Figure 7A). However, 92% of mice (10/12) survived in the T0901317-treated group ( Figure 7A). Analysis of PRV gE by immunoblotting and immunohistochemistry showed that T0901317 decreased PRV gE expression in lungs, suggesting that T0901317 inhibited PRV proliferation in vivo ( Figure 7B,C). Less infiltration of inflammatory cells was observed in the lungs in T0901317-treated mice than in vehicle-treated mice ( Figure 7D). All the results indicated that activation of LXR prevented PRV infection in vivo.
Viruses 2022, 14, x FOR PEER REVIEW 11 of 1 infiltration of inflammatory cells was observed in the lungs in T0901317-treated mic than in vehicle-treated mice ( Figure 7D). All the results indicated that activation of LXR prevented PRV infection in vivo.

Discussion
Viruses can manipulate lipid metabolism to facilitate their replication [27]. During infection, some viruses induce changes in cell membrane structures or utilize lipid syn thetic enzymes to build a suitable microenvironment for different stages of the infection [12]. LXR controls cellular lipid homeostasis [28]. Oxysterols are endogenous ligands o LXR [29], and they promote HBV gene expression through activation of LXR [30]. Murin gammaherpesvirus 68 infection increases LXR expression, and there is not a corre sponding increase in LXR target genes [17]. NDV infection activates LXR and its down stream lipogenic gene expression [13]. In this study, we found that PRV infection down regulated LXR expression both in vitro and in vivo, and LXR activation inhibited PRV infection. Our data indicated that different viruses used LXR for optimal replication through diverse mechanisms throughout their entire life cycle. Other physiological func tions of LXR may be required for virus replication, as well as their roles in lipid metabo lism.

Discussion
Viruses can manipulate lipid metabolism to facilitate their replication [27]. During infection, some viruses induce changes in cell membrane structures or utilize lipid synthetic enzymes to build a suitable microenvironment for different stages of the infection [12]. LXR controls cellular lipid homeostasis [28]. Oxysterols are endogenous ligands of LXR [29], and they promote HBV gene expression through activation of LXR [30]. Murine gammaherpesvirus 68 infection increases LXR expression, and there is not a corresponding increase in LXR target genes [17]. NDV infection activates LXR and its downstream lipogenic gene expression [13]. In this study, we found that PRV infection downregulated LXR expression both in vitro and in vivo, and LXR activation inhibited PRV infection. Our data indicated that different viruses used LXR for optimal replication through diverse mechanisms throughout their entire life cycle. Other physiological functions of LXR may be required for virus replication, as well as their roles in lipid metabolism.
Cholesterol is a critical component that determines membrane fluidity and architecture. For some viruses, cholesterol plays an essential role in the process of virus entry into cells, such as PRV [33], foot-and-mouth disease virus [35], and human rhinovirus type 2 [36], and depletion of cholesterol significantly inhibits viral entry and infection. Our data indicated that PRV enhanced cellular cholesterol levels, which were abrogated by LXR agonists. We further demonstrated that LXR activation decreased cellular cholesterol levels to inhibit PRV entry-dependent CCP dynamics, which could be rescued by cholesterol replenishment. Our study demonstrated a mechanism by which PRV disturbed LXR expression to promote viral entry through modulation of cholesterol homeostasis. This is in accordance with our previous report that cholesterol is critical for CCP dynamics in PRV entry [26]. These data provide novel insights into the prevention and control of diverse viruses that require cholesterol-regulated CCP dynamics for viral entry.

Conclusions
Viruses hijack cellular metabolism for their optimal replication. A better understanding of the interaction between virus and cellular metabolism will provide insights into an antiviral strategy. Lipids are the key component of cellular membrane compartments that participate in viral replication. We previously reported that Niemann-Pick C1-mediated intracellular cholesterol transport is essential for CCP dynamics and for viral entry. Here, we reported that PRV modulated cholesterol metabolism by downregulating the expression of LXR to assist viral entry through clathrin-mediated endocytosis. Therefore, our data further validated that cholesterol-regulated CCP dynamics are pivotal for PRV infection, suggesting that pharmacological reduction of cellular cholesterol levels has the potential to prevent PRV infection. Funding: This work was supported by grants from the National Natural Science Foundation of China (32072858), the Ten Thousand Talents Program for Young Talents (W03070106), and Outstanding Talents of Henan Agricultural University (30600773).