Hepatitis B Virus HBx Protein Mediates the Degradation of Host Restriction Factors through the Cullin 4 DDB1 E3 Ubiquitin Ligase Complex.

The hepatitis B virus (HBV) regulatory HBx protein is required for infection, and its binding to cellular damaged DNA binding protein 1 (DDB1) is critical for this function. DDB1 is an adaptor protein for the cullin 4A Really Interesting New Gene (RING) E3 ubiquitin ligase (CRL4) complex and functions by binding cellular DDB1 cullin associated factor (DCAF) receptor proteins that recruit substrates for ubiquitination and degradation. We compared the proteins found in the CRL4 complex immunoprecipitated from uninfected versus HBV-infected hepatocytes from human liver chimeric mice for insight into mechanisms by which HBV and the cell interact within the CRL4 complex. Consistent with its role as a viral DCAF, HBx was found in the HBV CRL4 complexes. In tissue culture transfection experiments, we showed that HBx expression led to decreased levels of known restriction factor structural maintenance of chromosomes protein 6 (SMC6) and putative restriction factors stromal interaction molecule 1 (STIM1, zinc finger E-box binding homeobox 2 (ZEB2), and proteasome activator subunit 4 (PSME4). Moreover, silencing of these proteins led to increased HBV replication in the HepG2-sodium taurocholate cotransporting polypeptide (NTCP) infection model. We also identified cellular DCAF receptors in CRL4 complexes from humanized mice. Increasing amounts of HBx did not reveal competitive DCAF binding to cullin4 (CUL4)-DDB1 in plasmid-transfected cells. Our results suggest a model in which HBx benefits virus replication by directly or indirectly degrading multiple cellular restriction factors.


Introduction
Chronic infection with hepatitis B virus (HBV) affects over 257 million people worldwide [1] and is a leading risk factor for the development of serious liver disease, including cirrhosis and hepatocellular carcinoma (HCC). The currently approved antiviral treatments (pegylated interferon-α; nucleos(t)ide analogs) reduce levels of viral replication (reviewed in Reference [2]). A cure for chronic α; nucleos(t)ide analogs) reduce levels of viral replication (reviewed in Reference [2]). A cure for chronic HBV remains elusive, in part, because of an inability to eliminate HBV covalently closed circular (ccc) DNA, a replicative intermediate that serves as the template for viral transcription. Novel strategies are needed to disrupt chronic HBV replication and will require new insight on how HBV interacts with a host cell to sustain viral replication.
The 3.2-kB HBV genome encodes the polymerase (P), core (C), surface (S), and X genes. The 17-kD HBx protein product of the X gene is of particular interest because it is required for HBV infection in human liver chimeric mice [3] and in HepaRG cells [4] and is required for maximal virus replication in the HBV plasmid DNA model of virus replication [5,6] (reviewed in Reference [7]). However, the functions of HBx in the virus life cycle are not completely understood. As the sole HBV regulatory protein, HBx has multiple functions including transactivation of viral and cellular promoters [8,9], binding to cccDNA and modifying its epigenetic regulation [10,11], and targeting for degradation cellular factors that restrict virus replication [12][13][14]. HBx is reported to interact with over 100 cellular proteins [15], consistent with HBx effects on diverse pathways such as calcium signaling, cell cycle progression, and apoptosis (reviewed in References [7,[16][17][18]).
HBV and many other viruses exploit host cellular ubiquitin machinery for their own benefit (reviewed in References [19][20][21][22][23]). It has been reported that HBx binds to the cullin 4 RING E3 ubiquitin ligase complex (CRL4) via its interaction with the CRL4 adaptor protein damaged DNA binding protein 1 (DDB1) (Figure 1) [24][25][26]. The HBx-DDB1 interaction is conserved among mammalian hepadnaviruses [25] and is required for virus infection and replication in woodchucks [27] and for maximal replication in the HBV plasmid replication assay [28,29]. As a CRL4 adaptor protein, DDB1 mediates its function through interactions with DDB1 cullin-associated factor (DCAF) receptors that recruit specific substrates to the CRL4 for ubiquitination, and this generally, although not always, results in proteasomal degradation [30][31][32] (reviewed in Reference [33]) ( Figure 1). Such substrates include the HBV restriction factors Structural Maintenance of Chromosomes Protein 5 and 6 (SMC5/6), discovered by binding to a DDB1-HBx fusion protein [13] and by tandem affinity purification from HepG2-HBx cells [14]. Existing data support the idea that HBx is a viral DCAF, including that HBx contains a DDB1-binding motif shared among other DCAF proteins [26] (reviewed in Reference [34]); it competes with DCAFs DDB2 and DCAF9 for binding to DDB1 [26,35], and it is stabilized by its interaction with DDB1 rather than being ubiquitinated and degraded [29]. The CRL4 complex has a modular structure consisting of the cullin-4A (CUL4) scaffold, the damaged DNA binding protein 1 (DDB1) adaptor protein, and the DCAF receptor (DCAF) proteins that recruit substrate (S) proteins for ubiquitination and degradation. The crooked S' indicates different substrates recruited by HBx. The regulator of cullins protein 1 (ROC1) contains a Really Interesting New Gene (RING) finger domain, which binds the ubiquitin-charged E2 (ubiquitin conjugating enzyme) [36]. The hepatitis B virus (HBV) HBx protein is a viral DCAF that binds to DDB1 [24,25] via a motif shared with cellular receptors [26,30] (reviewed in Reference [34]). In the present study, the CRL4 complexes from uninfected and HBVinfected human hepatocytes were isolated and the associated proteins were identified and compared to provide insight into the impact of HBV replication on the CRL4 complex. Figure is modified with the publisher's permission [37]. The CRL4 complex has a modular structure consisting of the cullin-4A (CUL4) scaffold, the damaged DNA binding protein 1 (DDB1) adaptor protein, and the DCAF receptor (DCAF) proteins that recruit substrate (S) proteins for ubiquitination and degradation. The crooked S' indicates different substrates recruited by HBx. The regulator of cullins protein 1 (ROC1) contains a Really Interesting New Gene (RING) finger domain, which binds the ubiquitin-charged E2 (ubiquitin conjugating enzyme) [36]. The hepatitis B virus (HBV) HBx protein is a viral DCAF that binds to DDB1 [24,25] via a motif shared with cellular receptors [26,30] (reviewed in Reference [34]). In the present study, the CRL4 complexes from uninfected and HBV-infected human hepatocytes were isolated and the associated proteins were identified and compared to provide insight into the impact of HBV replication on the CRL4 complex. Figure is modified with the publisher's permission [37].
Several viruses encode proteins that specifically interact with the CRL4 complex (Table 1) (reviewed in Reference [38]), one of over 200 distinct CRLs in human cells (reviewed in Reference [39]). These virus-cell interactions result in degradation of critical innate immune response proteins [40,41], disruption of the cell cycle [42,43], and degradation of viral restriction factors [12][13][14] (Table 1). Identifying the critical function(s) provided by the HBx-DDB1 interaction has been difficult, in part due to the lack of convenient and authentic HBV infection models in cell culture. Recent advancements with sodium-taurocholate cotransporting polypeptide (NTCP)-overexpressing HBV culture systems have facilitated viral infection studies. However, the host gene expression profile is significantly altered in cancer cell lines compared to primary human hepatocytes in vivo [44]. Human liver chimeric mice have been used for many years to study hepatitis virus replication [45][46][47][48]. In this study, we utilize human hepatocyte tissue from the same donor in an infectious and normal setting. Table 1. Viral proteins that interact with CUL4-DDB1: Proteins encoded by several viruses interact directly with CUL4-DDB1 and benefit virus replication. For example, several paramyxoviridae express V proteins that target signal transducer and activator of transcription (STAT) proteins for degradation via CUL4-DDB1 to inactivate the innate immune response. Other viral proteins and the cellular functions targeted are also listed. The goal of our study was to investigate the impact of HBV infection on the CRL4 complex in order to gain insight into the contribution of the HBx-DDB1 interaction to virus replication. HBV infection in human liver was studied in the FAH −/− , RAG2 −/− , and IL2RG −/− mouse model in which human liver chimeric mice were infected with HBV subtype ayw. The CRL4 was purified from the livers of uninfected (CRL4 UN ) and HBV-infected (CRL4 HBV ) human liver chimeric mice, and the CRL4-associated proteins were identified by mass spectrometry (MS). We tested two hypotheses generated by these data sets. In the first, we characterized four proteins unique to CRL4 UN as putative HBV restriction factors using in vitro transfection experiments and restriction factor silencing in the HepG2-NTCP HBV infection model. In the second, we identified six DCAF receptor proteins present in both CRL4 UN and CRL4 HBV and tested the ability of HBx to compete with different DCAFs for binding to CUL4-DDB1. Overall, our results suggest that multiple cellular restriction factors are present that limit HBV and that one of the functions of HBx may be to direct these proteins for CRL4-mediated degradation, thereby increasing virus replication.

Ethics Statement
Approval for all experiments involving mice was obtained from the Institutional Animal Care and Use Committee at Baylor College of Medicine (IACUC Protocols AN-346 and AN-6272) and the Cells 2020, 9, 834 4 of 24 recommendations in the Guided for the Care and Use of Laboratory Animals (Institute for Laboratory Animal Research, National Research Council, National Academy of Sciences, 2011). Human hepatocytes used for transplantation into mice were from cadavers and are not considered human subject research.

Human Liver Chimeric Mice and HBV Infection
Human liver chimeric mice (FAH −/− , RAG2 −/− , and IL2RG −/− ) were repopulated with cadaveric hepatocytes as previously described [48,58]. Human hepatocytes were enriched in the murine liver by applying selection pressure against the murine hepatocyte upon withdrawing the small molecule inhibitor NTBC (Nitisinone [47]). Mice were put back on the drug (cycling of NTBC) to avoid graft failure as described earlier [47]. After three months, human albumin (ELISA, Bethyl Laboratories) was measured in the murine blood to determine human chimerism. Six mice with similarly high human chimerism (>1 mg/mL human albumin) were selected for this study so that animal-to-animal variation in repopulation was not a variable. Human liver chimeric mice were injected via tail vein with 1 × 10 8 genome equivalents (GE) of chimpanzee-derived HBV (subtype ayw), using the same conditions (mice, inoculum) that have led to nearly 100% of human hepatocytes infected by HBV in our previous work [48]. Blood samples were obtained by retro-orbital bleed 10 min postinfection and weekly until infected mice reached a plateau in viremia. Based on our experience with nearly 100 similarly HBV-infected mice, the viremia reaches a plateau within a few weeks and maintains a relatively constant level of viremia with usually less than 1 log variation.

Real-Time qPCR Quantification of HBV Capsid-Associated DNA
Capsid-associated HBV DNA was extracted from 25 µL of cell media or from 12.5 µL serum using the Kingfisher Flex purification system and the 5× MagMax Pathogen RNA/DNA kit (Biosystems Thermo Fisher Scientific) following the manufacturer's protocol. Viral DNA was quantified by Taqman qPCR and compared to plasmid standards diluted 10 0 to 10 7 as previously described [59].

Immunoprecipitation (IP)/MS
IP/MS analysis of CRL4 complexes was performed by the Mass Spectrometry-Based Proteome Profiling Core at Baylor College of Medicine. Uninfected and HBV-infected human liver chimeric mice (3 each) were sacrificed at maximal viremia. Livers were perfused with Krebs-Ringer solution and livers were then lysed in sodium choride, ethylenediaminetetraacetic acid (EDTA), Tris, nonyl phenoxypolyethoxylethanol (NP-40) (NETN) buffer (50 mM Tris-HCl pH 7.5, 1 mM EDTA, 150 mM KCL, and 0.5% NP-40) containing a protease inhibitor cocktail (P3100, GenDepot) and sonicated for 3 min on ice. Since the goal of this MS screen was to identify new restriction factors, we separately pooled uninfected and HBV-infected liver lysates to ensure that the pulldown was technically reproducible. Two independent IPs were performed. Following centrifugation, the supernatants were IP'd with rabbit anti-CUL4A (Supplementary Table S1). In some experiments, purified protein complexes captured on protein A beads were alkylated before SDS-PAGE to reduce disulfide bonds. Complexes were incubated in 100 µL of 5 mM dithiothreitol (DTT) in 100 mM ammonium bicarbonate and for 45 min at 56 • C. Iodoacetamide was added to 14 mM final concentration and incubated for 30 min at room temperature in the dark to alkylate cysteines [60]. Excess iodoacetamide was quenched by adding 5 mM DTT and by incubating 15 min at room temperature in the dark. Alkylated samples were loaded onto NuPage 10% Bis-Tris midi-gels (Thermo Fisher WG1201BX10) and electrophoresed at 80 V constant voltage. The SDS-polyacrylamide gel was minimally stained with Coomassie brilliant blue. The lane was then cut into 4 pieces and subjected to in-solution digestion with 100 ng of trypsin in 50 mM ammonium bicarbonate (MS grade GenDepot) overnight. Digested peptides were extracted with 350 µL of 100% acetonitrile and 20 µL of 2% formic acid and dried in a Savant Speed-Vac. Dried peptides were dissolved in 10 µL of loading solution (5% methanol containing 0.1% formic acid) and subjected to a nano-HPLC 1000 system (Thermo Scientific) coupled to an LTQ Orbitrap Elite™ (Elite) mass spectrometer. An in-house 2 cm × 100 cm inner diameter trap column with 3 µM Reprosil-Pur Basic C18 beads (Dr. Maisch HPLC GmbH, Germany) and an in-house 5 cm × 150 µM capillary column packed with 1.9 µM Reprosil-Pur Basic C18 beads were used to enrich and separate injected peptides. A 75 min discontinuous gradient of 2-24% acetonitrile, 0.1% formic acid at a flow rate of 800 nL/min was applied to the column and then electro-sprayed into the mass spectrometer. The instrument was operated under the control of Xcalibur software Version 2.2 (Thermo Fisher Scientific) in data-dependent mode, acquiring fragmentation spectra of the top 25 strongest ions. Parent MS spectrum was acquired in the Orbitrap with full MS range of 375-1300 m/z in the resolution of 240,000. Collision-induced dissociation fragmented MS/MS spectrum was acquired in ion-trap with rapid scan mode. Spectral data were then searched against target-decoy human refseq database (release 2015_06, containing 73,637 entries) [61] in Proteome Discoverer 1.4 interface (Thermo Fisher) with Mascot algorithm (Mascot 2.4, Matrix Science). This method identified human-specific peptides but did not distinguish between human versus mouse peptides from highly conserved proteins. Dynamic modifications of acetylation of N-term, alkylation of cysteine, and oxidation of methionine were allowed. The precursor mass tolerance was confined within 20 ppm with fragment mass tolerance of 0.5 Dalton, and a maximum of two missed cleavages was allowed. Assigned peptides were filtered with 1% false discovery rate (FDR) using Percolator validation based on q-value.

Quantitation of MS Data
The intensity-based absolute quantification (iBAQ) number provides a measure of the relative abundance of each protein identified in an IP/MS sample and was calculated as the sum of the intensities of all tryptic peptides for a given protein divided by the number of theoretically observable peptides for that protein [62]. All protein iBAQ numbers were normalized to the CUL4 iBAQ number from the same IP reaction to permit comparison of relative protein levels in the absence versus presence of HBV. The function VLOOKUP (Microsoft Excel) was used to detect overlap between proteins from CRL4 UN vs. CRL4 HBV .

Plasmid DNAs
Two human influenza hemagglutinin (HA) epitope tags (YPYDVPDYA) were added to the N-terminus of HBx by PCR cloning to create pSI-2HA-X [59]. Similarly, two N-terminal HA tags were added to codon-optimized DCAF11 (NCBI NM_001163484.1), DCAF8 (NCBI NM_015726.2), and cereblon (CRBN) (NCBI NM_016302.3), which were then cloned into the NotI and EcoRI sites of the pSI vector. The myc-tagged CUL4A was obtained from Dr. Yong Cang and was described previously [26]. Codon-optimized NTCP (NCBI 003049.3) was PCR-cloned into the BamHI and XhoI sites of the pLVX-IRES-Hyg lentivirus vector to create pLVX-IRES-Hyg-NTCP. 2HA-X WT was cloned into the EcoRI and BamHI sites of the doxycycline (dox)-inducible pLV-TetOne-Puro vector to create pLV-2HA-X. Two N-terminal HA epitope tags were added to the N-terminus of point mutant HBx proteins HBx 69 , HBx 90/91 , or HBx R96E [63,64] and then cloned into the EcoRI and BamHI sites of the pLV-TetOne-Puro vector.

Lentivirus Production and Transduction of Cells
Lentiviruses encoding NTCP, shPSME4, and shZEB2 were prepared by co-transfecting HEK293T cells in 100-mm plates with a plasmid encoding Vesicular stomatitis virus G protein (pVSVG) (Addgene #8454), a plasmid encoding the HIV-1 gag, pol, tat, and rev genes (psPAX2) (Addgene #12260), and the appropriate lentivirus plasmid. Lentivirus was harvested 48 hrs posttransfection and qualitatively analyzed using Lenti-X GoStix (Takara Bio USA). Lentiviruses encoding shSTIM1 and shluciferase (LUC) were purchased from the Cell-Based Assay Screening (C-BASS) core facility at Baylor College of Medicine. Stable HepG2-NTCP cells were established by transduction of HepG2 cells with lentivirus encoding NTCP with a final concentration of 8 µg/mL polybrene to facilitate transduction. Lentivirus-containing supernatant was removed after 24 h and fresh media containing 500 µg/mL hygromycin B was added to select for transduced cells. Knockdown cells were established by transduction of HepG2-NTCP cells with the appropriate lentiviruses encoding shRNAs for LUC, ZEB2, PSME4, SMC6, or STIM1, followed by selection with 2 µg/mL puromycin.

Antibodies
The antibodies used for IP, immunofluorescence (IF) staining, immunohistochemistry (IHC) staining, and western blotting are listed in Supplementary Table S1.

IP and Western Blot
Following transfection, cell lysates were prepared in IP lysis buffer (25 mM Tris-HCl pH 7.4, 150 mM NaCl, 1% NP-40, 1 mM EDTA, and 5% glycerol) and were incubated with the IP antibody at a 1:250 dilution for 1 h at 4 • C and then incubated with staphylococcus Protein A (SPA) or Protein A/G agarose beads (Santa Cruz) for 1 h at 4 • C. The lysates were clarified by centrifugation, and the pelleted SPA/beads were washed three times with cold Phosphate Buffered Saline (PBS). The myc-CUL4A complex was detected in plasmid-transfected cells by IP with mouse anti-C-myc using Protein A/G agarose beads (Santa Cruz). Laemmli buffer was added and the SPA/beads were boiled at 95 • C for 5 min, centrifuged, and loaded onto 4-20% gradient (for detection of HBx) or 10% (for all other proteins) mini-Protean Tris-Glycine-Extended (TGX) polyacrylamide gels (Bio-Rad). After separation by SDS-PAGE, proteins were transferred to nitrocellulose membranes. Membranes were blocked with Odyssey Blocking Buffer-Tris Buffered Saline (TBS) (LI-COR) for 1 h at room temperature and incubated with primary antibody with TBS containing 0.1% Tween-20 (TBS-T) overnight at 4 • C. Membranes were washed with TBS-T and incubated with secondary antibody for 1 h at room temperature. TBS was used to wash the membranes three times before imaging on a LI-COR Odyssey CLx.

Western Blot Normalization and Quantitation
Proteins within a lane were normalized to either total protein (REVERT Total Protein Stain, LI-COR) or to a housekeeping protein (LI-COR Western Blot Normalization Handbook). Western blots were quantitated using Image Studio Software (LI-COR). All westerns were reproduced in at least three independent experiments.

HBV Infection of HepG2-NTCP Cells
Cells were seeded in 96-well plates to be 90% confluent the following day. polyethylene glycol (PEG)-concentrated HBV derived from HepG2.2.15 cells was used as inoculum. Cells were infected with 1000 GE/cell in media containing final concentrations of PEG (4%), DMSO (2.5%), and DMEM/F12 (3% FBS). The cells were spinoculated at room temperature for 1 h at 1000× g to enhance virus infection [65]. The following day, the inoculum was removed and the cells were washed three times with PBS. Replication media containing DMEM/F12 media with 3% FBS and 2.5% DMSO was added back to the cells, and the media changed every 2-3 days until the cells were fixed at seven days postinfection. In some experiments, cells were treated with HBV entry inhibitor Myrcludex B (MyrB; 500 nM) for 30 min prior to and during infection, as described [66,67].

Detection and Quantitation of HBV Core Protein by IF
Uninfected or HBV-infected HepG2-NTCP cells were fixed with 4% formaldehyde for 30 min, permeabilized with TBS containing 0.5% Triton X-100 for 10 min and blocked with 5% FBS in PBS for 1 h at room temperature. Cells were incubated with primary antibody overnight at 4 • C. Cells were then washed with PBS and incubated with secondary antibody for 1 h at room temp. Nuclei were stained with 4 ,6-diamidino-2-phenylindole (DAPI) for 5 min at room temperature. Images were captured with a wide field epifluorescence Nikon TiE inverted microscope using a SPECTRAX LED light source (Lumencor) and a phase contrast or a 20× Plan Apo (NA 0.75) differential interference contrast (DIC) objective. Fluorescence and transmitted light images were recorded using an ORCA-Flash 4.0 sCMOS camera (Hamamatsu), and Nikon Elements Advanced Research v4.5 software was used for multipoint position selection, data acquisition, and image analysis. Two methods were used to quantitate the number of core-positive hepatocytes per well. In the first, a 5.8 mm × 5.8 mm stitched image array was acquired using the Nikon Elements Software and then transferred into ImageJ. The number of core-positive cells for the entire area were counted by two individuals (M.M.M. and B.L.S.). In the second method, ten fields (500 µm × 500 µm each) were selected randomly throughout the plate and core positive cells were counted. Following calculations of the number of core-positive cells per well, similar results were obtained from both methods, and subsequent experiments used the second method. The GE value from each well (determined by real-time PCR analysis of the infected cell media) was divided by the total number of core positive cells from the corresponding well to determine GE per infected cell.

Inhibition of CRLs by MLN4924 (Pevonedistat)
HEK293T cells were plated in 60-mm dishes and, the following day, were treated with 0, 0.1, 1, 5, or 10 µM of MLN4924 (MedChemExpress), an inhibitor of the neural precursor cell expressed developmentally down-regulated protein 8 (NEDD8) activating enzyme required for CRL activity [68]. After 24 h of treatment, the cells were rinsed with cold PBS and lysed with 250 µL IP lysis buffer (see above). The lysates were centrifuged at 4 • C at 14,000 rpm for five minutes to pellet cell debris, and the supernatant was analyzed by electrophoresis on 10% SDS-PAGE and western immunoblot, followed by densitometer quantitation.

Isolation and Characterization of the CRL4 Complex
The interaction of HBx with DDB1 is critical for HBV infection, but the mechanism(s) of action is not completely understood. To investigate the impact of HBV replication on the CRL4, we isolated the CRL4 complex by IP from CRL4 UN and CRL4 HBV lysates from hepatocytes grown in human liver chimeric mice [48,58]. CRL4-associated proteins were identified by MS (see the Materials and Methods section). This authentic HBV infection model was used to establish the biologic relevance of the identified proteins linked to the HBV infection. The chimeric mice used in this experiment were Cells 2020, 9, 834 8 of 24 approximately 80% repopulated with human hepatocytes that were identified within the chimeric liver by anti-FAH IHC staining (Supplementary Figure S1a). Mice were sacrificed when viremia plateaued (Supplementary Figure S1b). Since the anti-CUL4A antibody used for IP reacted with a region of the protein homologous to the highly related CUL4B protein (reviewed in Reference [69]), the CRL complex is referred to hereafter as CRL4.
The number of unique proteins identified in the CRL4 UN (n = 1373) was similar to that found in the CRL4 HBV (n = 1331), and over 92% of the proteins were present in both complexes ( Figure 2 and Supplementary Table S3). With nearly 100% of the human hepatocytes infected with HBV [48], we observed that infection did not dramatically alter the overall binding capacity of the CRL4. The presence of the expected CRL4 structural components that includes cullin4A, DDB1, and ROC1 (reviewed in Reference [39]) and of DCAF receptors (described in Figure 1) indicated that the complexes were purified intact. We identified 118 proteins unique to the CRL4 UN and 76 proteins unique to the CRL4 HBV (Supplementary Table S4). Importantly, the HBx protein was identified in CRL4 HBV (Supplementary Figure S2), consistent with its role as a viral DCAF. A cysteine alkylation step was required for the detection of HBx [60]. The relative abundance of each protein in the CRL4 complex was determined by the iBAQ method (see the Materials and Methods section), and all recovered proteins were normalized to the amount of CUL4A in that IP. Proteins were then rank-ordered for their relative abundance within the complex (Supplementary Table S3). Comparison by iBAQ numbers of all proteins in the CRL4 allowed us to identify proteins that were enriched ≥3-fold in CRL4 UN versus CRL4 HBV , and vice versa (Supplementary Table S5).
Cells 2020, 9,834 8 of 23 Methods section). This authentic HBV infection model was used to establish the biologic relevance of the identified proteins linked to the HBV infection. The chimeric mice used in this experiment were approximately 80% repopulated with human hepatocytes that were identified within the chimeric liver by anti-FAH IHC staining (Supplementary Figure S1a). Mice were sacrificed when viremia plateaued (Supplementary Figure S1b). Since the anti-CUL4A antibody used for IP reacted with a region of the protein homologous to the highly related CUL4B protein (reviewed in Reference [69]), the CRL complex is referred to hereafter as CRL4.
The number of unique proteins identified in the CRL4 UN (n = 1373) was similar to that found in the CRL4 HBV (n =1331), and over 92% of the proteins were present in both complexes (Figure 2 and Supplementary Table S3). With nearly 100% of the human hepatocytes infected with HBV [48], we observed that infection did not dramatically alter the overall binding capacity of the CRL4. The presence of the expected CRL4 structural components that includes cullin4A, DDB1, and ROC1 (reviewed in Reference [39]) and of DCAF receptors (described in Figure 1) indicated that the complexes were purified intact. We identified 118 proteins unique to the CRL4 UN and 76 proteins unique to the CRL4 HBV (Supplementary Table S4). Importantly, the HBx protein was identified in CRL4 HBV (Supplementary Figure S2), consistent with its role as a viral DCAF. A cysteine alkylation step was required for the detection of HBx [60]. The relative abundance of each protein in the CRL4 complex was determined by the iBAQ method (see the Materials and Methods section), and all recovered proteins were normalized to the amount of CUL4A in that IP. Proteins were then rankordered for their relative abundance within the complex (Supplementary Table S3). Comparison by iBAQ numbers of all proteins in the CRL4 allowed us to identify proteins that were enriched ≥3-fold in CRL4 UN versus CRL4 HBV , and vice versa (Supplementary Table S5).  Table S4). Proteins identified in each IP were assigned an intensity-based absolute quantification (iBAQ) value (described in the Materials and Methods section) and then normalized to CUL4 levels to determine their relative abundance in the complex. Other proteins were enriched in CRL4 UN (n = 36) or the CRL4 HBV (n = 65) (Supplementary Table S5a and S5b). Among the 118 proteins unique to CRL4 UN was SMC6, previously described as an HBV restriction factor [13,14].
We initially predicted that proteins unique to CRL4 HBV (Supplementary Table S4) or enriched in CRL4 HBV (Supplementary Table S5) would include proteins recruited by the virus to the CRL4 complex for ubiquitination and degradation. An additional interpretation was considered after we found the previously described HBV restriction factor SMC6 [13,14] among a subset of 118 proteins that are unique to the CRL4 UN . Proteins normally processed by the CRL4 UN might undergo a more rapid degradation upon HBV infection and might be absent (or reduced) in the CRL4 HBV . We hypothesized that the group of 118 proteins in the CRL4 UN would include additional HBV restriction factors.  Table S4). Proteins identified in each IP were assigned an intensity-based absolute quantification (iBAQ) value (described in the Materials and Methods section) and then normalized to CUL4 levels to determine their relative abundance in the complex. Other proteins were enriched in CRL4 UN (n = 36) or the CRL4 HBV (n = 65) (Supplementary Table S5a,b). Among the 118 proteins unique to CRL4 UN was SMC6, previously described as an HBV restriction factor [13,14].
We initially predicted that proteins unique to CRL4 HBV (Supplementary Table S4) or enriched in CRL4 HBV (Supplementary Table S5) would include proteins recruited by the virus to the CRL4 complex for ubiquitination and degradation. An additional interpretation was considered after we found the previously described HBV restriction factor SMC6 [13,14] among a subset of 118 proteins that are unique to the CRL4 UN . Proteins normally processed by the CRL4 UN might undergo a more rapid degradation upon HBV infection and might be absent (or reduced) in the CRL4 HBV . We hypothesized that the group of 118 proteins in the CRL4 UN would include additional HBV restriction factors.

HBV Restriction Factors
A screening strategy was developed to determine whether cellular HBV restriction factors, in addition to SMC6, were present in the group of 118 proteins recovered in the CRL4 UN . Steps in this strategy included first establishing that the protein is normally processed through a CRL and then demonstrating that HBx expression lowers the steady-state levels of the protein. Finally, we determined whether silencing of the putative restriction factor led to elevated HBV replication. Five proteins that were unique to CRL4 UN were selected for initial studies as potential restriction factors based on their potential to restrict the HBV life cycle. For example, Proteasome Activator Subunit 4 (PSME4) is reported to mediate the degradation of acetylated histones [70,71], and acetylated histones play a role in the transcriptionally active form of viral cccDNA [72]. Zinc Finger E-Box Binding Homeobox 2 (ZEB2) overexpression inhibits HBV replication in HepG2.2.15 cells through an interaction with the core promoter [73], but its interactions with HBx or the CRL4 are unknown. Stromal Interaction Molecule 1 (STIM1) is an endoplasmic reticulum calcium sensor that regulates extracellular calcium entry into the cytoplasm [74]. Elevated calcium benefits HBV replication [75,76], but the mechanisms exploited by HBV to modulate this increased cytosolic calcium to prevent calcium overload and subsequent apoptosis are unknown. Proteasome Activator Subunit 1 (PSME1) is a subunit of the immunoproteasome (reviewed in Reference [77]) that generates antigenic peptides for presentation on MHC class I molecules and may be important in the host response to HBV. SMC6 was included in the screening analysis because its interaction with CRL4 in the presence of HBx has been previously studied [13,14].
To confirm that the putative restriction factors were processed through a CRL, HEK293T cells were cultured in the presence of increasing concentrations of MLN4924 (Pevonedistat), a small molecule inhibitor of the NEDD8-activating enzyme that is required for CRL function [68]. If the candidate restriction factor was normally processed through a CRL, its steady-state level should increase in the presence of increasing concentrations of MLN4924. Indeed, increased steady-state levels of PSME4, SMC6, and ZEB2 were reproducibly detected with increasing amounts of MLN4924 (Figure 3). STIM1 protein levels increased only when cells were treated with the highest dose (10 µM) of MLN4924 (Figure 3b). Since MLN4924 had little effect on PSME1 levels (Figure 3), this protein was not included in further experiments. These results confirm that PSME4, SMC6, ZEB2, and STIM1 are normally processed through a CRL.
We next examined the impact of HBx expression on the steady-state levels of the putative restriction factors in HEK293T cells, which are easily transfected and are a standard model for protein interaction studies, including a recent study on HBx and SMC5/6 [14]. Cells were transfected with plasmid DNA encoding a dox-inducible HBx and cultured in the presence of dox to induce HBx expression or left uninduced (no dox) to serve as the negative control. HBx expression was associated with a measurable decrease in the steady-state levels of putative restriction factors PSME4, ZEB2, and STIM1 and of SMC6 ( Figure 4). The 40% reduction was similar to that previously reported for SMC6 [13,14] and ZEB2 [73] and extends those results to include new candidate restriction factors that may be targeted directly or indirectly by HBx for degradation.
increase in the presence of increasing concentrations of MLN4924. Indeed, increased steady-state levels of PSME4, SMC6, and ZEB2 were reproducibly detected with increasing amounts of MLN4924 ( Figure 3). STIM1 protein levels increased only when cells were treated with the highest dose (10 μM) of MLN4924 (Figure 3b). Since MLN4924 had little effect on PSME1 levels (Figure 3), this protein was not included in further experiments. These results confirm that PSME4, SMC6, ZEB2, and STIM1 are normally processed through a CRL. Protein levels for putative restriction factors PSME4, Zinc Finger E-Box Binding Homeobox 2 (ZEB2), STIM1, and PSME1 and for SMC6 [13,14] in the absence and presence of MLN4924 were determined by western blot assays and normalized either to total protein (indicated by asterisks) or to actin  Protein levels for putative restriction factors PSME4, Zinc Finger E-Box Binding Homeobox 2 (ZEB2), STIM1, and PSME1 and for SMC6 [13,14] in the absence and presence of MLN4924 were determined by western blot assays and normalized either to total protein (indicated by asterisks) or to actin (described in the Materials and Methods section). We next examined the impact of HBx expression on the steady-state levels of the putative restriction factors in HEK293T cells, which are easily transfected and are a standard model for protein interaction studies, including a recent study on HBx and SMC5/6 [14]. Cells were transfected with plasmid DNA encoding a dox-inducible HBx and cultured in the presence of dox to induce HBx expression or left uninduced (no dox) to serve as the negative control. HBx expression was associated with a measurable decrease in the steady-state levels of putative restriction factors PSME4, ZEB2, and STIM1 and of SMC6 (Figure 4). The 40% reduction was similar to that previously reported for SMC6 [13,14] and ZEB2 [73] and extends those results to include new candidate restriction factors that may be targeted directly or indirectly by HBx for degradation.  Table S1). Protein levels were normalized to actin levels (bottom panel). Comparison of treated cells with untreated cells revealed the impact of HBx expression. (b) Graphical representation of western blot results from three independent experiments: The level of each restriction factor in the absence of HBx was set to 100% and compared to the level of that same protein in the presence HBx. Significance was determined by student t test using GraphPad Prism Version 8.1.2. Asterisks indicate p < 0.05.
A previous study reported that HBx expression led to the degradation of SMC5/6 [13,14]. To determine whether an HBx-DDB1 interaction was required for the degradation of the putative restriction factors described above, we next investigated a panel of HBx mutant proteins that do not bind DDB1. SMC6 was included for comparison. Cells were transfected with plasmid DNA encoding dox-inducible wildtype HBx (HBx WT ) that binds DDB1 or with plasmids encoding point mutant HBx  Table S1). Protein levels were normalized to actin levels (bottom panel). Comparison of treated cells with untreated cells revealed the impact of HBx expression. (b) Graphical representation of western blot results from three independent experiments: The level of each restriction factor in the absence of HBx was set to 100% and compared to the level of that same protein in the presence HBx. Significance was determined by student t test using GraphPad Prism Version 8.1.2. Asterisks indicate p < 0.05.
A previous study reported that HBx expression led to the degradation of SMC5/6 [13,14]. To determine whether an HBx-DDB1 interaction was required for the degradation of the putative restriction factors described above, we next investigated a panel of HBx mutant proteins that do not bind DDB1. SMC6 was included for comparison. Cells were transfected with plasmid DNA encoding dox-inducible wildtype HBx (HBx WT ) that binds DDB1 or with plasmids encoding point mutant HBx proteins HBx 69 , HBx 90/91 , or HBx R96E that neither bind DDB1 [63,64] nor rescue HBx-deficient replication in a plasmid replication assay [28,29]. While HBx WT was successful at reducing the levels of the putative restriction factors, the point mutant HBx proteins did not (Figure 5a,b). The steady-state levels of the mutant HBx proteins were lower than that of HBx WT (Figure 5a, lower panel), consistent with previous reports that an interaction with DDB1 stabilizes HBx [29,35,78]. To rule out that the lower levels of mutant HBx protein expression was responsible for the failure to decrease the restriction factor levels, cells were transfected with decreasing amounts of plasmid encoding HBx WT (Figure 5c). HBx WT was still able to reduce steady state levels of SMC6 even when present at levels similar to that of HBx mutant proteins (Figure 5c). This result suggests that mutant HBx proteins were present at sufficient levels to reduce the restriction factors if the HBx mutants were functionally capable of this. We note that, while SMC6 completely disappeared from the CRL4 HBV (Supplementary Table S3), there was incomplete SMC6 degradation in the whole cell lysates of cells expressing inducible HBx (Figure 5a,c). The different results may be explained by the characteristic protein amounts present in these two methods.
Finally, we used the HepG2-NTCP HBV infection model to determine if shRNA targeting of the putative restriction factors would lead to increased HBV replication. HepG2 cells were transduced with lentivirus encoding the HBV receptor NTCP [79] (Figure 6a) to allow permissivity to HBV infection that was lacking in HepG2 cells without NTCP overexpression (Figure 6b). HepG2 cells overexpressing NTCP had significantly elevated levels of HBV replication in comparison to infection of normal HepG2 cells that lacked overexpressed NTCP. Treatment with the HBV inhibitor MyrB significantly reduced the level of HBV replication (Figure 6b,c). Lentiviruses encoding shZEB2, shPSME4, shSTIM1, or shSMC6 were transduced into HepG2-NTCP cells to create stable knockdown cell lines that were used for HBV infection experiments. A lentivirus encoding shLUC was used to create a negative control cell line. Transduction of cells with lentivirus encoding shRNA targeting SMC6 led to cell growth arrest, and so, this cell line could not be included in subsequent analyses. The reason for the growth arrest is unknown but suggests the SMC6 knockdown is not tolerated by these HepG2-NTCP cells. Consistent with this idea, SMC6 knockout is embryonically lethal in mice [80].
We first validated that the shRNA cell lines exhibited lower steady-state levels of their targeted restriction factor (Figure 6d). Next, the cell lines were infected with HBV derived from HepG2.2.15 cells (Figure 6e), and HBV replication was assessed on day 7 by quantifying HBV capsid-associated DNA in the media of infected cells. Relative to HBV replication in the HepG2-NTCP shLuc control cell line, virus replication was reproducibly elevated in all shRNA restriction factor cell lines (Figure 6f). These results are consistent with previous findings that knockdown of ZEB2 in HepG2.2.15 cells leads to increased virus replication [73] and extends those findings into the HepG2-NTCP HBV infection model. The increased virus replication measured in the HepG2-NTCP shPSME4 and HepG2-NTCP shSTIM1 cells (Figure 6f) reached statistical significance in most experiments. Our results indicate that the knockdown of an individual restriction factor is associated with a reproducible two-to three-fold increase in virus replication. An affect may be due to the proportional silencing of the restriction factor in this cell culture model. It also may indicate that there are additional restriction factors that must be overcome to robustly increase HBV replication. similar to that of HBx mutant proteins (Figure 5c). This result suggests that mutant HBx proteins were present at sufficient levels to reduce the restriction factors if the HBx mutants were functionally capable of this. We note that, while SMC6 completely disappeared from the CRL4 HBV (Supplementary  Table S3), there was incomplete SMC6 degradation in the whole cell lysates of cells expressing inducible HBx (Figure 5a,c). The different results may be explained by the characteristic protein amounts present in these two methods. Finally, we used the HepG2-NTCP HBV infection model to determine if shRNA targeting of the putative restriction factors would lead to increased HBV replication. HepG2 cells were transduced with lentivirus encoding the HBV receptor NTCP [79] (Figure 6a) to allow permissivity to HBV infection that was lacking in HepG2 cells without NTCP overexpression (Figure 6b). HepG2 cells overexpressing NTCP had significantly elevated levels of HBV replication in comparison to infection of normal HepG2 cells that lacked overexpressed NTCP. Treatment with the HBV inhibitor MyrB significantly reduced the level of HBV replication (Figure 6b,c). Lentiviruses encoding shZEB2, shPSME4, shSTIM1, or shSMC6 were transduced into HepG2-NTCP cells to create stable knockdown cell lines that were used for HBV infection experiments. A lentivirus encoding shLUC was used to create a negative control cell line. Transduction of cells with lentivirus encoding shRNA targeting SMC6 led to cell growth arrest, and so, this cell line could not be included in subsequent analyses. The reason for the growth arrest is unknown but suggests the SMC6 knockdown is not tolerated by these HepG2-NTCP cells. Consistent with this idea, SMC6 knockout is embryonically lethal in mice [80].

HBx Does Not Compete with Cellular DCAFs for Binding to DDB1 in the CRL4
A subset of CRL4-associated proteins of great interest to studies of HBV infection is the DCAF receptors that bind DDB1 and recruit substrate proteins to the CRL4 for ubiquitination and degradation ( Figure 1). The HBV regulatory HBx protein is a viral DCAF [26,29,35] (reviewed in Reference [34]), but its impact on cellular DCAFs that reside in the CRL4 of human liver is unknown. However, the ability of HBx to bind to the DCAF receptor binding site on DDB1 [26] (reviewed in Reference [34]) raises the possibility that the HBx expressed from the HBV genome during replication may interfere with CRL4-DDB1-DCAF interactions and potentially alter the spectrum of substrates recruited to the CRL4. The human genome encodes approximately 60 DCAF receptors (reviewed in Reference [33]), and 32 of these are detectable by IHC staining in human liver [81,82]. In our study, six of these DCAFs were found in the CRL4 UN and in CRL4 HBV ( Table 2). Three of the six recovered DCAF receptors (CRBN, DCAF11, and DCAF8) were selected for follow-up analysis based on their potential involvement in the HBV life cycle. Their interaction with DDB1 was validated in HepG2 cells by IP of the individual DCAFs, followed by MS detection of DDB1 and CUL4A (Supplementary Table S6). Table 2. DCAF receptor proteins identified in the CRL4 of human liver: Six DCAF receptor proteins were identified in the CRL4 complex from both uninfected and HBV-infected human hepatocytes. HBx, a viral DCAF receptor [26,29,83] (reviewed in Reference [34]), was also identified in the CRL4 from HBV-infected human hepatocytes.
We next determined whether these three DCAFs could compete with HBx for binding to DDB1 within the CRL4, since two previous studies suggested that HBx might compete with DCAF receptors for binding to DDB1. In the first, HBx expressed as a GFP-HBx fusion protein competed with DCAF DDB2 in transfected HeLa cells [35]. In the second, peptides spanning the DDB1 binding domain of woodchuck WHx protein competed with DCAF9 for binding to DDB1 in an in vitro pulldown assay [26]. Neither DDB2 nor DCAF9 were found in the CRL4 complexes in our experiments, but we hypothesized that other DCAFs (CRBN, DCAF11, and DCAF8) in the CRL4 from human liver ( Table 2) would compete with HBx for binding to DDB1 within CRL4. Current known functions of these DCAFs possibly relevant to the liver are provided ( Table 2). Plasmids encoding 2HA-tagged DCAFs were created and tested in transfection experiments to demonstrate that the HA tags did not prevent the DCAFs from entering the CRL4 complex (Supplementary Figure S3). Next, plasmids encoding myc-tagged CUL4A and 2HA-tagged DCAFs were co-transfected into cells in the absence or presence of increasing amounts of plasmid encoding HBx (pSI-2HA-X or control pSI). Transfected cells were detergent-lysed, and the lysates IP'd with an anti-myc antibody to pull down the CRL4 complex, followed by western blot analysis for the presence of DDB1 and the DCAF receptor of interest (Supplementary Figure S4a). In these experimental conditions, increasing amounts of HBx did not alter the ratio of DDB1-CRBN within the CRL4 complex and remained the same as in cells lacking HBx expression. Similar results were obtained with DDB1-DCAF8 and DDB1-DCAF11 (not shown). In summary, we have no evidence that HBx can compete with these DCAFs for binding to DDB1 within the CRL4 and under these experimental conditions.

Discussion
Viruses have evolved different mechanisms to usurp host cell pathways to benefit virus replication, and the targeting of cellular E3 ligases is a common mechanism used to modify host gene expression (reviewed in References [19,20,38,100]). The HBV HBx protein binding to CRL4 adaptor protein DDB1 is critical for HBV replication [28,29]. However, the mechanism(s) by which this interaction benefits HBV replication is not completely understood. The goal of the present study was to investigate the impact of HBV replication on the CRL4 complex in the authentic and well-established human liver chimeric mouse HBV infection model [48]. Most importantly, we combine in this study the sophisticated animal model with an unbiased MS approach to identify a list of cellular proteins differentially bound to the CRL4 complex. Our studies suggest the existence of multiple cellular restriction factors targeted for inactivation by HBV and indicate that one mechanism by which HBx dampens the expression of these restriction factors is through an interaction between HBx and DDB1.
Interestingly, this study also provides a large database of CRL4-related proteins from normal human liver that can be used by other investigators for hypothesis-driven research. Our initial comparison of CRL4-associated proteins from uninfected versus HBV-infected human liver revealed 118 proteins unique to CRL4 UN that were absent in CRL4 HBV . Since the previously studied HBV restriction factor SMC6 [13,14] was among the 118 proteins, we reasoned that additional restriction factors might also be present in that population of proteins. Indeed, of four additional candidate restriction factors tested in our study, three (PSME4, STIM1, and ZEB2) met the criteria of being processed by a CRL (and stabilized by MLN4924 treatment). They were also present at lower steady-state levels in the presence of HBx. Finally, their silencing led to a reproducible increase in HBV replication in the HepG2-NTCP HBV infection model. Together, these results confirm previous observations that HBx targets SMC5/6 for degradation [13,14] and extends those results to include additional cellular restriction factors that may act to inhibit HBV replication. While previous studies have concluded that a major function of HBx is to direct SMC5/6 for degradation, we now propose an expanded role for HBx in virus replication that involves targeting additional cellular restriction factors.
Previous studies demonstrated that HBx-mediated degradation of SMC5/6 requires CUL4 [14] and a form of DDB1 that interacts with CUL4 [13]. It was proposed that HBx serves as a "bridge" to link SMC5/6 to the CRL4 where it is ubiquitinated and degraded [14]. Importantly, we detected SMC6 and other restriction factors in the CRL4 from uninfected liver, indicating that HBx was not needed for their recruitment to the CRL4. Their presence in the CRL4 was supported by demonstrating increased levels of these factors following the addition of MLN4924, a chemical that renders CRLs inactive. Our data supports a model in which there are at least two groups of HBV restriction factors. First, the factors are present and processed by CRL4 UN (Figure 7a, green triangles). Upon HBV infection, these factors would be degraded via polyubiquitination as described for SMC5/6 [14]. Alternatively, HBx might mediate a more global effect on restriction factor turnover, perhaps by modulating CRL4 regulatory proteins such as cullin-associated NEDD8-dissociated protein 1 (CAND1) or NEDD8 (reviewed in Reference [101]). In support of this idea, the inhibition of NEDD8 (and of CRL4 activity) by Pevonedistat (MLN4924) also inhibited HBV transcription and restored SMC5/6 levels [102]. The model predicts that a second group of restriction factors are either absent or at low level in CRL4 UN but, upon HBV infection, are recruited to the CRL4 HBV and present at increased levels ( Figure 7a, green squares). Examples of this second group are provided in Supplementary Table S5b and discussed below. Further work is needed to firmly establish these proposed models.
The specific step in virus replication targeted by a cellular restriction factor is expected to vary, depending on the normal function of that cellular protein. For example, SMC6 is part of the highly conserved SMC5/6 complex that binds DNA (reviewed in Reference [103]) and, in HBV-infected cells, is proposed to restrict virus replication by binding to cccDNA to prevent viral transcription [13,14]. In primary human hepatocytes, SMC5/6 localizes to the Nuclear Domain 10 ((also known as promyelocytic leukaemia (PML) body)) where it prevents HBV transcription without initiating an innate immune response [104]. The degradation of SMC5/6 by HBx that ultimately occurs is an evolutionarily conserved function [105]. The results of our study suggest two additional HBV restriction factor models. The first involves ZEB2, a negative regulator of transcription that inhibits HBV through specific binding to the HBV core promoter in the HepG2.2.15 cell model of HBV replication [73] (Figure 7b, left). Relief of this transcriptional repression is mediated through microRNA 146a (miR-146a) [106], and in turn, miR-146a is positively regulated by HBx (Figure 7b, right) [107]. Our finding that HBx mediates the degradation of ZEB2 extends those findings (1) by demonstrating that downregulation of ZEB2 enhances virus replication in the HepG2-NTCP HBV infection model and (2) by suggesting a second mechanism for relief from ZEB2 transcriptional repression, namely through HBx-DDB1-mediated degradation of ZEB2.
A second new HBV restriction factor model arising from our results predicts targeting of HBV cccDNA, which exists in either a transcriptionally active or inactive state, depending upon the associated proteins and the presence of acetylated histones [10,72,[108][109][110] (Figure 7c). Cellular PSME4 is a proteasome component that recognizes acetylated histones and targets them for ATP-and ubiquitin-independent degradation during spermatogenesis and the DNA damage response [70,71]. Our model proposes that PSME4 normally cooperates with other cellular factors to return the transcriptionally active cccDNA to the silenced form (Figure 7c). The degradation of PSME4 would allow cccDNA to remain transcriptionally active, thus favoring virus transcription. More research is needed to confirm that STIM1, ZEB2, and PSME4 are indeed restriction factors. For example, they will need to be tested for their ability to rescue HBx-deficient HBV replication in an infection model, as described for the SMC6 restriction factor [13,14]. If confirmed as restriction factors, our results then support the idea that the host cell may restrict HBV replication in multiple processes in virus replication only to be nullified by the HBx-CRL4 interaction. Our initial studies focused on only five of the 118 proteins unique to the CRL4 UN , and it is likely that additional restriction factors are present in this group of host cell proteins.
A similar CUL4 IP/MS study performed on a transfected human BT474 breast cancer line recovered two DCAF receptors: DCAF11 and human immunodeficiency virus type 1 Viral Protein R (Vpr)-binding protein (VPRBP) [30], of the approximately 60 DCAFs encoded in the human genome (reviewed in Reference [33]). Our finding of six DCAF receptors is a similarly small number. Our results showed that HBx does not compete with CRBN for binding to DDB1 in the CRL4 complex, which contrasts with two previous studies that concluded that HBx competed with the binding of DCAFs DDB2 [35] and DCAF9 [26] to DDB1. However, important differences in experimental design may account for the differing observations. Competition of DDB2-DDB1 with GFP-HBx was demonstrated in HeLa cells transfected with HA-DDB1 and myc-DDB2, followed by IP [35]. In the second study, increasing amounts of woodchuck hepatitis X (WHx) peptide were shown to prevent GST-DCAF9 from copurifying with DDB1 [26]. Neither DDB2 nor DCAF9 were identified in the CRL4 complexes in our study. Importantly, the previous studies did not examine the impact of HBx on CUL4-bound DDB1-DCAF, as was done in the current study. Left, ZEB2 is a DNA binding transcriptional repressor previously shown to bind to the HBV core promoter and significantly decrease HBV transcription [73]. Right, HBx relieves ZEB2-mediated transcriptional suppression by upregulating miR146a [107], which promotes HBV replication by targeting ZEB2 [106]. In the current study, we propose that HBx utilizes the CRL4 complex to target ZEB2 for degradation. (c) Proposed mechanism for restriction factor PSME4. Left, Transcriptionally inactive cccDNA has a preponderance of hypoacetylated histones (empty circles) and associates with specific factors ((histone deacetylases (HDACs), transcriptional repressors, and methyltransferases)] such as HDAC1 and Nicotinamide adenine dinucleotide (NAD)-dependent protein deacetylase sirtuin 1 (Hsirt1) [10], yin yang 1 (YY1) and enhancer of zeste homolog 2 (Ezh2) [111], protein arginine methyltransferase 1 (PRMT1) [109], and PRMT5 [110]. Right, Alternatively, transcriptionally active cccDNA contains a preponderance of hyperacetylated histones (filled circles) and associates with other factors including cyclic adenosine monophosphate (cAMP) responsive element binding protein 1 (CREB) [108], CREB binding protein (CBP), P300, P300/CBP-associated factor (pCAF), PSME4 (red font, identified in this study) and HBx [10,11]. We propose that PSME4 is a viral restriction factor because of its ability to degrade acetylated histones [70,71], thereby helping to return cccDNA to an inactive state unless HBx is present to promote the degradation of PSME4.
A similar CUL4 IP/MS study performed on a transfected human BT474 breast cancer line recovered two DCAF receptors: DCAF11 and human immunodeficiency virus type 1 Viral Protein R (Vpr)-binding protein (VPRBP) [30], of the approximately 60 DCAFs encoded in the human genome (reviewed in Reference [33]). Our finding of six DCAF receptors is a similarly small number. Our results showed that HBx does not compete with CRBN for binding to DDB1 in the CRL4 complex, which contrasts with two previous studies that concluded that HBx competed with the binding of (b) Proposed model to explain a role for ZEB2 as an HBV restriction factor. Left, ZEB2 is a DNA binding transcriptional repressor previously shown to bind to the HBV core promoter and significantly decrease HBV transcription [73]. Right, HBx relieves ZEB2-mediated transcriptional suppression by upregulating miR146a [107], which promotes HBV replication by targeting ZEB2 [106]. In the current study, we propose that HBx utilizes the CRL4 complex to target ZEB2 for degradation. (c) Proposed mechanism for restriction factor PSME4. Left, Transcriptionally inactive cccDNA has a preponderance of hypoacetylated histones (empty circles) and associates with specific factors ((histone deacetylases (HDACs), transcriptional repressors, and methyltransferases)] such as HDAC1 and Nicotinamide adenine dinucleotide (NAD)-dependent protein deacetylase sirtuin 1 (Hsirt1) [10], yin yang 1 (YY1) and enhancer of zeste homolog 2 (Ezh2) [111], protein arginine methyltransferase 1 (PRMT1) [109], and PRMT5 [110]. Right, Alternatively, transcriptionally active cccDNA contains a preponderance of hyperacetylated histones (filled circles) and associates with other factors including cyclic adenosine monophosphate (cAMP) responsive element binding protein 1 (CREB) [108], CREB binding protein (CBP), P300, P300/CBP-associated factor (pCAF), PSME4 (red font, identified in this study) and HBx [10,11]. We propose that PSME4 is a viral restriction factor because of its ability to degrade acetylated histones [70,71], thereby helping to return cccDNA to an inactive state unless HBx is present to promote the degradation of PSME4.
A subset of proteins not pursued in our study includes those unique to CRL4 HBV (n = 76) and/or enriched in CRL4 HBV (n = 65). Proteins in these groups could be cellular proteins targeted by HBx or other HBV proteins for recruitment to and degradation by the CRL4. Alternatively, they may be upregulated as a normal response to viral infection and thus appear in the CRL4 HBV . Data from other laboratories support both of these scenarios. For example, included as a protein unique to CRL4 HBV is DEAD box protein 5 (DDX5), an RNA helicase that has an emerging regulatory role in viral infections, including HBV (reviewed in Reference [112]). DDX5 was identified as an HBx interacting protein in HepG2-HBx cells that were treated with MLN4924 [14]. Previous studies showed that HBV infection or expression of HBx alone caused downregulation of DDX5, preventing its ability to regulate the stability and function of the chromatin modifying polycomb repressive complex and leading to increased viral transcription [113]. The finding of DDX5 in the population of proteins unique to CRL4 HBV is consistent with it being recruited to the CRL4 for degradation and supports the idea that DDX5 downregulation can occur through the CRL4 pathway. A second cellular protein of interest is Protein Phosphatase 2 Catalytic Subunit Alpha (PPP2CA), also previously identified as an HBx-interacting protein [114]. HBx inhibits PPP2CA phosphatase activity and associated cell death. With PPP2CA recruited to the CRL4 HBV complex for degradation, the survival of infected cells that might normally undergo apoptosis could contribute to HBV-associated hepatocarcinogenesis [114]. A final example is the RUVBL2 component of the nucleosomal acetyltransferase of the histone H4 (NuA4) complex [115]. This complex binds to the HBV precore/core promoter to inhibit HBV transcription, and knockdown of RUVBL2 leads to increased HBV replication [115]. Our finding of RUVBL2 enriched in CRL4 HBV (Supplementary Table S5b) suggests that a mechanism of RUVBL2 downregulation involves a CRL4 pathway.

Conclusions
This study investigated the impact of HBV infection and replication on the CRL4 complex isolated from human hepatocytes in vivo. Using an authentic virus infection model and a sophisticated CUL4 IP/MS approach, we identified a list of potential host HBV restriction factors that led to testable hypotheses. Our results suggest that HBx interacts with the CRL4 complex in a DDB1-dependent manner to play an intricate role in altering host cell protein levels, which leads to enhanced virus replication. Because a high viral load is a significant predictor of the development of HCC, this observation may have clinical relevance. The unbiased comparison of CRL4-associated proteins from uninfected and HBV infected human hepatocytes provides a rich dataset from which testable hypotheses can be generated.