key: cord-0703069-mrxtr416
authors: Ding, Siyuan; Zhu, Shu; Ren, Lili; Feng, Ningguo; Song, Yanhua; Ge, Xiaomei; Li, Bin; Flavell, Richard A; Greenberg, Harry B
title: Rotavirus VP3 targets MAVS for degradation to inhibit type III interferon expression in intestinal epithelial cells
date: 2018-11-21
journal: eLife
DOI: 10.7554/elife.39494
sha: fcd821f2f9391938a54442ec69f64e2370597be5
doc_id: 703069
cord_uid: mrxtr416

Rotaviruses (RVs), a leading cause of severe diarrhea in young children and many mammalian species, have evolved multiple strategies to counteract the host innate immunity, specifically interferon (IFN) signaling through RV non-structural protein 1 (NSP1). However, whether RV structural components also subvert antiviral response remains under-studied. Here, we found that MAVS, critical for the host RNA sensing pathway upstream of IFN induction, is degraded by the RV RNA methyl- and guanylyl-transferase (VP3) in a host-range-restricted manner. Mechanistically, VP3 localizes to the mitochondria and mediates the phosphorylation of a previously unidentified SPLTSS motif within the MAVS proline-rich region, leading to its proteasomal degradation and blockade of IFN-λ production in RV-infected intestinal epithelial cells. Importantly, VP3 inhibition of MAVS activity contributes to enhanced RV replication and to viral pathogenesis in vivo. Collectively, our findings establish RV VP3 as a viral antagonist of MAVS function in mammals and uncover a novel pathogen-mediated inhibitory mechanism of MAVS signaling.

Timely induction of the interferon (IFN) response is pivotal for the host to mount a successful defense against invading viruses and other intracellular microbial pathogens and requires precise orchestration of several signaling cascades (Ivashkiv and Donlin, 2014) . Cytoplasmic RNA pathogen-associated molecular patterns (PAMPs) generated during virus replication, including viral double-stranded RNA (dsRNA) intermediate or genome, 5'-triphosphate RNA and other byproducts, are sensed by host pattern recognition receptors (PRRs) including RIG-I and MDA5 (Kato et al., 2006; Uzri and Greenberg, 2013) . PRRs in turn activate the mitochondrial antiviral signaling protein (MAVS), a predominantly mitochondria and partially peroxisome-resident protein (Bender et al., 2015; Odendall et al., 2014) , for downstream signal transduction and IFN production . Due to its central role in host antiviral immunity, Mavs -/mice are highly susceptible to multiple RNA virus infections, such as West Nile virus (WNV) (Pinto et al., 2014) , respiratory syncytial virus (RSV) (Bhoj et al., 2008) , coxsackievirus B3 (CVB3) , rotavirus (RV) (Broquet et al., 2011) , and vesicular stomatitis virus (VSV) (Sun et al., 2006) . MAVS expression in the hematopoietic compartment is also critical for proper T cell functions (Zhao et al., 2016 ) and a T cell-independent antibody response (Zeng et al., 2014) . Since virus evolution is driven, in part, by host antiviral selection pressure, MAVS provides a useful tool to study virus immune evasion strategies (Patel et al., 2012) . Multiple virus-encoded factors, including hepatitis C virus (HCV) NS3/4A protease (Bender et al., 2015; Li et al., 2005; Ferreira et al., 2016) , hepatitis A virus (HAV) 3ABC precursor (Yang et al., 2007) , enterovirus (EV) 71 2Apro (Wang et al., 2013) and coronavirus SARS-CoV ORF9b , all inhibit MAVS signaling through its cleavage or degradation. In fact, the ability of HAV to block human but not murine MAVS constitutes the basis of the HAV relative host range restriction to humans in vivo (Hirai-Yuki et al., 2016) . Interestingly, the viral MAVS antagonists identified to date have been mostly non-structural proteins with the exception of influenza PB2 (Long and Fodor, 2016) . In the present study, we report the unexpected discovery that the RV RNA capping enzyme VP3, an important RV structural protein, recently shown to also possess phosphodiesterase (PDE) activity , also mediates MAVS degradation in an RV strain-specific manner. Of note, replication of a simian RV, which is unable to degrade murine MAVS, is significantly enhanced in Mavs -/mice. Additionally, VP3 expression during RV infection induces specific degradation of the full-length functional MAVS protein but not the truncated 'mini'-MAVS that does not activate IFN signaling (Brubaker et al., 2014) , thereby highlighting several previously unrecognized specificities in the virus-host arms race.

RVs are segmented, dsRNA viruses that primarily infect the mature intestinal epithelial cells (IECs) located at the tip of the villi in the host small intestine (Estes and Greenberg, 2013) . A large number of mammalian and avian species are infected with their own host specific RV strains in a host range restricted fashion (Ciarlet et al., 1998) . Previous studies demonstrated that both type I and type III IFNs are able to effectively restrict the replication of heterologous (non-murine) but not homologous (murine) RVs in suckling mice (Lin et al., 2016) . It was also noted that in RV infected suckling mice, the bulk of type I IFNs (IFN-a/b) derive from the CD45 + hematopoietic compartment whereas type III IFNs (IFN-ls) are produced primarily by the intestinal epithelium (Lin et al., 2016; Sen et al., 2012; Hernández et al., 2015) . Here, to further delineate the IFN induction pathway in intestinal cell lines and primary IECs, we first generated, via CRISPR-Cas9, a single clonal MAVS knockout in the human colonic epithelial HT-29 cell line. Complete knockout of both full-length (FL) MAVS (75 kD) and mini-MAVS (52 kD) was confirmed by western blot and Sanger sequencing . We noted that wild-type (WT) HT-29 cells expressed and secreted significantly more IFNL3 mRNA (40-60 fold) and IFN-l protein (31-34 fold) than type I IFN (IFNB) ( Figure 1A) , in response to RNA PAMPs, such as stimulation with poly(I:C), a dsRNA mimic, or RV infection, as previously reported (Pervolaraki et al., 2017; Saxena et al., 2017) . In contrast, MAVS -/-HT-29 cells were completely defective in both, suggesting that: (1) HT-29 cells produced more IFN-l than IFN-b, and (2) that this IFN secretory process was mediated through the RIG-I/MDA5-MAVS RNA sensing pathway in HT-29 cells. To validate these findings in a more physiologic system, we utilized a human origin ileum enteroid preparation that consisted entirely of primary IECs (Saxena et al., 2016) . Consistent with the findings in HT-29 cells, we found that following infection with RV or vesicular stomatitis virus (VSV), an excellent source of RNA PAMPs (Kell and Gale, 2015) , human IECs expressed much more (50 fold) IFNL3 than IFNB ( Figure 1B) . Importantly, this type III IFN signature is specific for IECs, since IFNB was robustly expressed in RV-infected or poly(I:C) stimulated HEK293 cells, a human non-intestinal epithelial origin cell line ( Figure 1C ). Both IFNB and IFNL3 expression were reduced to baseline levels in the absence of MAVS ( Figure 1C and Figure 1 figure supplement 1B). Collectively, these data suggest that human IECs intrinsically differ from some human non-intestinal origin cells and preferentially express IFN-l over IFN-b in response to RNA PAMP stimulation.

Using our MAVS -/-HEK293 cells that completely lack FL and mini-MAVS (Figure 1-figure supplement 1B), we investigated the ability of different MAVS variants to induce IFN-b and IFN-l expression ( Figure 1-figure supplement 1C ). Through reconstitution of WT MAVS, mitochondriaonly MAVS (mito-MAVS), peroxisome-only MAVS (pex-MAVS) and mini-MAVS, we found that, consistent with a previous study (Brubaker et al., 2014) , mini-MAVS was defective in IFN induction. However, we also found that despite the controversy in literature (Bender et al., 2015; Odendall et al., 2014) , in our system pex-MAVS expression in a MAVS-depleted background strongly activated both type I and type III IFNs to a similar degree as WT MAVS and mito-MAVS ( 

To investigate the role of MAVS signaling in RV replication in cell culture, we examined the ability of human and animal RVs to replicate in WT and MAVS -/-HT-29 cells. Interestingly, although replication Human intestinal enteroids were infected with VSV-GFP (MOI = 5) or the human RV WI61 strain (MOI = 5) for 16 hr. Expression of IFN-b and IFN-l expression was measured by RT-qPCR and normalized to that of GAPDH. (C) WT and MAVS -/-HEK293 cells were stimulated with LMW poly (I:C) (200 ng/ml) or infected with RRV (MOI = 1) for 24 hr. Expression of IFN-b and IFN-l expression was measured by RT-qPCR and normalized to that of GAPDH. For all figures, experiments were repeated at least three times with similar results. Data are represented as mean ± SEM. Statistical significance is determined by Student's t test (*p 0.05; **p 0.01; ***p 0.001). DOI: https://doi.org/10.7554/eLife.39494.002 The following figure supplement is available for figure 1: of the simian RV RRV strain was enhanced approximately 10-fold in the absence of MAVS, the replication of the human RV Wa strain was not significantly increased ( Figure 2A , top panel). In addition to intracellular viral RNA levels, the amount of infectious RRV, but not Wa RV, was also markedly increased in the supernatant of MAVS -/-HT-29 cells compared to WT cells ( Figure 2A , lower panel), suggesting the possibility that human RVs (such as the Wa strain) may possess a mechanism to block MAVS signaling in HT-29 cells, thereby enhancing their replication capacity by inhibiting MAVSmediated IFN induction.

To identify a potential RV inhibitor of IFN signaling other than the well-characterized RV nonstructural protein 1 (NSP1) antagonism of IRF3 (Arnold et al., 2013a; Barro and Patton, 2005) (by simian and murine RV strains), b-TrCP (Ding et al., 2016; Graff et al., 2009 ) (by human and some bovine and porcine RV strains) (Sherry, 2009 ) and IFN receptor degradation by all RVs (Sen et al., 2017) , we examined a large panel of key adaptor proteins, kinases and transcription factors in the RNA sensing pathway. We observed a significant decrease in the levels of FL-MAVS (by 6 hr) and IRF1 (by 12 hr) in African Green Monkey MA104 cells following simian RRV infection ( Figure 2B ). The FL-MAVS down-regulation was highly specific, as the levels of mini-MAVS, a truncated isoform that is unable to trigger IFN induction (Brubaker et al., 2014) , other signaling molecules (RIG-I, TBK1, IKKe, TRAF2, b-TrCP), control mitochondrial (Fis1, COXIV), and peroxisomal (PMP70) proteins were only affected at a high multiplicity of infection (MOI) of 10 and only at the latest time point examined (12 hr post infection) ( Figure 2B ). Moreover, transcript levels of MAVS mRNA, from which both FL and mini-MAVS are translated (Brubaker et al., 2014) , remained stable during RV infection ( Surprisingly, we also noted that RV infection induced FL-MAVS degradation in an RV straindependent manner. Compared to several other animal and human RV strains, only the simian RRV and, to a much lesser extent, the porcine SB1A strain, were able to induce MAVS degradation in rhesus origin MA104 cells ( Figure 2C , upper panel; Figure 2 -figure supplement 1B, middle panel). In contrast, infection of the human origin HT-29 cells with the human RV Wa strain, but not the simian RRV strain, was capable of degrading human MAVS ( Figure 2C , middle panel; Figure 2 -figure supplement 1B, lower panel), highlighting a unique pattern of virus-strain host-species co-segregation with the MAVS degradation phenotype. These associations were further documented in NIH3T3 cells, a mouse origin fibroblast cell line, where only the murine RV ETD strain efficiently degraded murine MAVS ( Figure 2C , lower panel). Species-specific MAVS degradation was recapitulated using human RV infection and Flag-tagged MAVS from human, African Green monkey and rhesus monkey ( Figure 2D ). Since MAVS acts upstream of both IRF3 and NF-kB signaling, we next examined the functional significance of RV-induced MAVS degradation. As expected, we found diminished luciferase production driven by IFN and ISG promoters in RRV infected MA104 cells in response to ensuing RNA PAMP stimulation ( Figure 2E ).

Inactivated RVs has been shown to inhibit RNaseL activation through a yet-to-identified mechanism independent of virus replication (Sánchez-Tacuba et al., 2015) . However, efficient MAVS degradation requires active RV replication and likely de novo synthesis of viral proteins, as either psoralen UV-inactivation or neutralizing antibody pre-incubation prevented MAVS inhibition (Figure 2-figure supplement 1C ). Based on a supernatant transfer experiment and the use of specific inhibitors of exosome pathways GW4869 and spiroepoxide (Li et al., 2013) , we excluded the involvement of extracellular vesicles and secreted factors in MAVS degradation (Figure 2-figure supplement 1D and E). Previous studies have shown that apoptosis-activated caspases may trigger MAVS cleavage (Scott and Norris, 2008) . However, we found that among the nearly 50 drug compounds tested, only proteasome inhibitors MG132, lactacystin and bortemozib, but not lysosome inhibitors chloroquine and concanamycin A, pan-caspase inhibitor Z-VAD-FMK, or mTOR inhibitor rapamycin, rescued MAVS expression to WT levels ( Figure 2F and 

UI R R V W a R R V W a UI R R V E T D R R V E

In order to identify the viral protein(s) responsible for MAVS degradation, we genetically and biochemically screened each of the 12 RV proteins using unbiased experimental approaches. Rhesus origin MA104 cells were transfected with plasmids encoding a GFP epitope on the N-terminus of each RRV protein as described (Ding et al., 2016) and then subjected to sorting for GFP positive cells followed by western blot analysis ( Figure 3A ). There is controversy in the current literature regarding a possible NSP1-MAVS interaction (Ding et al., 2016; Nandi et al., 2014) . The present data indicate that only the expression of RV RNA methyl-and guanylyl-transferase VP3 and viroporin NSP4 could possibly lead to the degradation of endogenous FL-MAVS in MA104 cells ( Figure 3A ). IRF3, a well-characterized substrate of NSP1 (Barro and Patton, 2005) , served as a positive control and was only degraded following NSP1 expression ( , suggesting that the host range restricted MAVS degradation during RV infection can be recapitulated by VP3 derived from several different RV strains. Taken together, these findings strongly suggest that MAVS degradation is mediated by VP3, not NSP1.

To complement the genetic analysis, we comprehensively profiled MAVS interacting proteins, using an immunoprecipitation (IP)-mass spectrometry (MS) approach. We infected MA104 cells with RRV in the presence or absence of the proteasome inhibitor MG132, performed IP with anti-MAVS antibody, and identified bound RV proteins ( Figure 3C , left panel and Supplementary file 1). We hypothesized that the use of MG132 would block MAVS degradation and stabilize any MAVS-RV protein complex. Notably, although the total levels of VP3 did not increase in MG132-treated cells (data not shown), only VP3 and not NSP3 or NSP4, was enriched in the immune-precipitate of the MG132 group in which MAVS proteasomal degradation was inhibited ( Figure 3C , right panel). These data support the hypothesis that VP3 rather than other RV proteins, physically interacts with MAVS to target it for degradation. In fact, the pull-down of NSP4 from MAVS interactome decreased in the presence of MG132 ( Figure 3C , right panel). We further interrogated possible VP3-MAVS interactions using traditional IP with both ectopic expression of Flag-tagged MAVS and GFP-tagged VP3 ( Figure 3D ) and purified recombinant MAVS and VP3 proteins (Figure 3-figure supplement 1C). While NSP4 did not co-precipitate with MAVS ( Figure 3D ), in both cases, we observed VP3 in the IP lysates, again suggesting that the VP3-MAVS, but not the NSP4-MAVS, interaction is likely to be direct.

To delineate the molecular basis underlying VP3-mediated MAVS degradation, we generated a series of RRV VP3 mutants containing N7-MTase, 2'-O-MTase, GTase/RTPase and PDE domains (Ogden et al., 2014 ) ( Figure 3E , left panel), and examined their respective ability to were transfected with Flag-tagged MAVS from Homo sapiens (human, hu), Chlorocebus aethiops (African Green monkey, AGM), Macaca mulatta (rhesus monkey, rh) for 12 hr and infected with Wa (MOI = 3) for 12 hr. The protein levels of MAVS, VP6 and GAPDH were measured by western blot. (E) MA104 cells were transfected with luciferase expression constructs driven by IFN-b, NF-kB, or ISRE promoters, mock or infected with RRV (MOI = 3) for 8 hr, and stimulated with LMW poly (I:C) (pIC) for 8 hr. The level of firefly luciferase (FFL) was measured and normalized to that of renilla luciferase (RL), which serves as internal control. (F) MA104 cells were infected with RRV (MOI = 3) for 12 hr and treated with indicated proteasome and lysosome inhibitors for 12 hr. The lysates were harvested and MAVS level was measured by western blot. (MG: MG132; epo: epoxomicin; lac: lactacystin; conA: concanamycin A; bort: bortezomib). For all figures, experiments were repeated at least three times with similar results. Data are represented as mean ± SEM. Statistical significance is determined by Student's t test (*p 0.05; **p 0.01; ***p 0.001). (* represents mini-MAVS in all western blots). DOI: https://doi.org/10.7554/eLife.39494.004

The following figure supplement is available for figure 2: 

Relative levels (MAVS/viral protein) In contrast, NSP1 was largely localized to the Golgi apparatus as previously reported (Ding et al., 2016) and did not co-localize with MAVS ( Figure 3 figure supplement 1D). Importantly, the N-terminal domain itself, which turns out to be the most variable region with VP3 (Ogden et al., 2014) , was sufficient to induce MAVS degradation ( Figure 3E , right panel). Co-IP experiments also pinpointed the N-terminal domain to be the MAVSinteracting part of VP3 ( Figure 3F ). We found that the C-terminal PDE domain, recently shown to prevent RNaseL activation Sánchez-Tacuba et al., 2015) , was not required for MAVS degradation ( Figure 3G ). Importantly, neither pharmacological inhibitors of PDE activity nor site-directed mutagenesis of the two key histidine residues (H718, H797) within the PDE catalytic sites rescued MAVS levels ( Figure 3G and Figure 3 -figure supplement 1E), suggesting that unlike RNaseL inhibition , the PDE enzymatic activity itself was not involved in MAVS degradation.

To further verify the role of the VP3 N-terminal region in mediating RV strain-specific MAVS degradation, we ectopically expressed VP3 derived from different RV strains. Consistent with our observation in the context of virus infections (Figure 2) , we observed a specific interaction between simian MAVS and VP3 from simian RV RRV strain, and not with VP3 from murine and human RV strains ( Figure 3H ). Importantly, replacing the first 171 N-terminal amino acids from simian RRV strain with those from murine ETD RV strain completely abrogated the VP3-MAVS interaction ( Figure 3H) , verifying a key role of VP3 N-terminus in MAVS binding. We also found that, similar to RV infection, blocking the proteasome by MG132 prevented MAVS degradation by VP3 ( Figure 3I) . We have not yet been able to identify a single host E3 ligase that is responsible for the ubiquitination event of MAVS (Figure 3-figure supplement 1F and G) , despite multiple efforts to use siRNA to knock down several E3 ligases such as TRIM25, AIP4 and MARCH5, all previously reported to induce MAVS ubiquitination (Castanier et al., 2012; Yoo et al., 2015; You et al., 2009) . Nevertheless, our results clearly indicate that using its N-terminal region, RV structural protein VP3 localizes to the mitochondria and interacts with and targets MAVS for proteasomal degradation (Figure 3 and 

Previous studies uncovered several regulatory motifs within MAVS that are essential to its antiviral function and oligomerization capacity (Hou et al., 2011; Liu et al., 2015; Shi et al., 2015; Xu et al., 2014) . To identify the minimal subunit of MAVS that is subject to VP3-mediated degradation, we constructed a series of chimeric simian MAVS proteins with GFP fused to distinct regions, including the N-terminal caspase activation and recruitment domain (CARD), the proline-rich region (PRR), and the transmembrane (TM) region (Figure 4A ). Although CARD-PRR alone is sufficient for MAVS-VP3 interaction ( Figure 4B) , the levels of EGFP-TM and CARD-PRR-EGFP remained Figure 4C ). Taken together, these data suggest that while the CARD domain may be important for VP3 binding, multiple MAVS domains, in particular its mitochondrial localization, may be required for efficient degradation by RV VP3. The MAVS N-terminal CARD domain, involving two key lysine residues at the very N-terminus: K7 and K10, is frequently targeted by several E3 ubiquitin ligases such as TRIM25, AIP4 and MARCH5 and other negative regulators for ubiquitination (Castanier et al., 2012; Yoo et al., 2015; You et al., 2009; Moore et al., 2008; Zhong et al., 2010) . It is intriguing that this CARD domain is missing from the signaling-defective mini-MAVS protein that is not degraded by RV infection ( Figure 2B ). We found that lysine 10 is more important in VP3-mediated MAVS degradation, as mutation of K10 partially rescued MAVS levels in both single and double mutants K10A and K7AK10A respectively ( Figure 4D, upper panel) . Changing lysines to arginines to conserve the positive charge (K7RK10R) also partially blocked RV-infection induced MAVS degradation ( Figure 4D , lower panel). K10 is highly conserved among MAVS from different species and is also required for its degradation by human RV infection (Figure 4-figure supplement 1A) . Through the use of a panel of ubiquitin mutants, we noted that during RRV infection, MAVS was modified by K48 poly-ubiquitination ( Figure 4E) , consistent with its degradation by the ubiquitin-proteasome pathway ( Figure 2F ).

To gain additional mechanistic insights into the sequential events leading to MAVS degradation, we sought to identify possible post-translational modifications (PTMs) on MAVS during infection. As previously noted, both FL-MAVS and mini-MAVS expressed in mammalian cells migrate at larger band sizes than their predicted molecular weights (Brubaker et al., 2014) and the same recombinant proteins from a bacterial expression system have correct sizes (Hou et al., 2011) . Although we did not detect any glycosylation (Figure 4-figure supplement 1B, upper panel) or AMPylation (Figure 4-figure supplement 1B, lower panel) , our high-resolution IP-MS using mock or RV-infected cell lysates and antibody against endogenous MAVS revealed three novel arginine methylation sites and a cluster of phosphorylated residues that had not been previously reported in phospho-proteome databases (Hornbeck et al., 2015) and thus represents novel phosphorylation hotspots ( Figure 4F ). Similar to the prior characterization of serine-rich clusters (Liu et al., 2015) , this region consists of 188 SPLTSS 193 and is located in PRR, which we found to be required for VP3-mediated MAVS degradation ( Figure 4A ). Within the SPLTSS motif, two serines and one threonine were phosphorylated during RV infection and these phosphorylation modifications were individual events that totaled to 16.0% of total MAVS proteins ( Figure 4F) . We further detected the same phosphorylation modifications in the SPLTSS motif when recombinant VP3 was expressed alone (data not shown), further indicating that this process is entirely mediated by RV VP3. TBK1, a key kinase downstream of MAVS signaling for IFN activation, was not responsible for MAVS phosphorylation at this novel site for 48 hr and lysates were harvested for immunoprecipitation using anti-V5 antibody. (D) MA104 cells were transfected with indicated GFP-tagged MAVS mutants for 48 hr with or without RRV infection (MOI = 1) for the last 12 hr. The levels of MAVS and viral protein VP6 expression were measured by western blot. (E) MA104 cells were transfected with WT or indicated lysine-mutants of HA-tagged ubiquitin for 48 hr, infected with RRV (MOI = 1) for the last 12 hr and harvested for immunoprecipitation using an anti-MAVS antibody. The levels of ubiquitin-conjugated MAVS were measured using an anti-HA antibody. (F) Mass spectrometry analysis of PTMs on MAVS, immunoprecipitated from RRV-infected MA104 lysates at six hpi. Numbers indicate the mass increase (+79.97: phosphorylation;+14.02: methylation). The novel PTMs identified in this study are highlighted in red. The percentage of phosphorylation and methylation modification in total MAVS proteins is presented as %. (G) MA104 cells were transfected with WT or MAVS mutants (SPLTSS: SPLTSS motif mutated to six alanines; R3A: R232, R236, R239 mutated to three alanines) for 48 hr with or without RRV infection (MOI = 1) for the last 12 hr. The levels of MAVS were measured by western blot. (H) HEK293 cells were co-transfected with GFP-tagged Wa-VP3 and WT or MAVS mutants for 48 hr and treated with MG132. Lysates were harvested for immunoprecipitation using anti-GFP antibody and probed for MAVS levels. (data not shown). Remarkably, mutagenesis of the SPLTSS motif to six alanines completely abolished RV-induced MAVS degradation ( Figure 4G ). In contrast, mutation of all three methylated arginines to alanines did not prevent MAVS degradation ( Figure 4G) . Importantly, disruption of this highly conserved SPLTSS motif in human MAVS also prevented MAVS phosphorylation and inhibited human RV-induced degradation (Figure 4-figure supplement 1C) . To shed more light on the molecular events leading to MAVS degradation, we also tested the ability of different MAVS mutants to bind to VP3. As expected, we observed specific binding of VP3 from human RV to human MAVS but not to simian MAVS ( Figure 4H) , suggesting that the interaction is the prerequisite of subsequent degradation. Interestingly, disruption of either the SPLTSS motif or the three-arginine site did not alter interaction with VP3 ( Figure 4H) , implying that VP3-MAVS interaction occurs independent of the SPLTSS motif. We also found that these MAVS proteins, including the SPLTSS and K7RK10R mutants, were still fully functional at inducing type I and type III IFN expression (Figure 4-figure  supplement 1D) , suggesting that VP3 mediated MAVS degradation is important for blocking the downstream signaling. Taken together, our data highlight the discovery of a novel 'phospho-degron' motif within MAVS that regulates its activity during RV infection.

Finally, we utilized the suckling mouse model of RV infection to evaluate the physiological relevance of VP3 degradation of MAVS in vivo. We first orally infected 5-day-old wild-type B6129SF2/J pups with the homologous EW strain of murine RV (10 4 diarrhea dose 50) or a heterologous simian RV RRV strain (10 7 plaque forming units, PFUs), doses that cause diarrhea in at least 90% of inoculated pups (Lin et al., 2016; Feng et al., 2013) . At 48 hr post infection, we harvested small intestines, isolated crude IECs, and sorted for CD26 + EpCAM + CD44 -CD45mature villous IECs, the primary target cells of RV in the gut (Sen et al., 2012) . Consistent with our findings in cell culture, we observed a pronounced decrease in the total protein levels of MAVS in EW-infected IECs but not in IECs following RRV infection ( Figure 5-figure supplement 1A) . Unlike its human and simian orthologs, murine Mavs gene does not encode a second mini-isoform (Brubaker et al., 2014) . Mavs transcripts within the sorted IECs remained stable during RV infection ( Figure 5-figure supplement 1B) , confirming that the decrease in MAVS occurred at a post-transcriptional level. Despite significantly higher levels of virus replication, EW induced less IFN-l expression than RRV ( Figure 5-figure supplement 1C) . Since RRV infects significantly fewer IECs than EW (Feng et al., 2013) , we would expect that RRVinduced IFN-l expression is even higher on a single-cell level. A diminished IFN-l response to EW infection is consistent with MAVS inhibition and disruption of the IFN induction pathway.

To further determine the importance and relative contribution of MAVS degradation to RV replication in vivo, we compared fecal RV antigen shedding induced by EW and RRV infection in WT and Mavs -/pups over a 12 day course. In WT animals, the replication of RRV was significantly lower than EW, consistent with our previous publications (Lin et al., 2016; Feng et al., 2011; Feng et al., 2013) and viral protein levels ( Figure 5-figure supplement 1A) . Remarkably, the amount of RRV shedding in the feces was markedly enhanced (1-2 logs) in Mavs -/animals compared to WT littermates ( Figure 5A ). In contrast, the fecal antigen levels of EW were not significantly different ( Figure 5A) . The viral RNA level of intra-intestinal simian RRV replication, but not murine EW RV replication, was increased in Mavs -/mice ( Figure 5B) . RRV replication at certain extra-intestinal sites, such as the liver, also increased by one log in the Mavs -/pups at day 7 post infection ( Figure 5B ). In contrast, the intestinal and systemic replication of the murine EW RV was almost identical between the two groups ( Figure 5A and B) , except that the fecal shedding was prolonged for 3 days, perhaps due to a defect in the induction of the humoral antibody response (Kuklin et al., 2000) , which was previously observed for WNV infection in Mavs -/mice (Pinto et al., 2014) . Taken together, these data highlight a critical role of RV VP3 in antagonizing MAVS antiviral signaling, blocking IFN-l expression in IECs and contributing to RV replication and pathogenesis.

We recently reported that the IEC-specific Nlrp9b inflammasome is involved in the host suppression of homologous murine EW RV infection in vivo (Zhu et al., 2017) . However, whether Nlrp9b signaling also contributes to host control of heterologous (non-murine) RV replication was not examined. Here, we sought to directly compare the anti-RV activity of the inflammasome to the MAVS-IFN inhibitory pathway in response to a heterologous simian RRV infection in suckling mice. We found that the RRV replication in the small intestine was substantially up-regulated (approximately 100-fold) in Ifnar1 -/-, Mavs -/-, Casp1 -/and Nlrp9b -/mice but not in Il18 -/animals ( Figure 5C ).

It is worth noting that the suppressive effect on RV fecal shedding of Nlrp9b was much more profound for simian RV than that for the homologous murine RV (Zhu et al., 2017) . These findings suggest that, in contrast to murine RV replication, which is modestly controlled by the STAT1 signaling (Lin et al., 2016) and inflammasome-mediated pyroptosis (Zhu et al., 2017) , 1) simian RV replication is substantially restricted by both inflammasome and IFN signaling, 2) pyroptosis (cell death), but not were harvested at 3 dpi or 7 dpi from EW or RRV infected animals and the levels of viral NSP5, indicative of virus replication, was measured by RT-qPCR and normalized to that of GAPDH. (C) C57Bl6/J mice with indicated gene deficiencies were infected with RRV (10 7 pfu) or EW (10 4 DD 50 ). Three days later, feces samples were collected and tested by an ELISA assay for viral antigens and the amount of viruses were converted to PFU equivalents based on the standard curve. At least 8 mice were used in each group. For all figures, experiments were repeated at least two times. Data are represented as mean ± SEM. Statistical significance is determined by Student's t test (*p 0.05; **p 0.01; ***p 0.001). DOI: https://doi.org/10.7554/eLife.39494.011

The following source data and figure supplement are available for figure 5:

Source data 1. Source data for Figure 5A . inflammasome-mediated pro-inflammatory cytokine secretion (in particular IL-18), leads to both EW and RRV attenuation in vivo.

An intact MAVS signaling in both parenchymal cells and the hematopoietic compartment plays a critical role in eliciting a full-blown IFN response to PAMPs and is also essential to shaping the adaptive immune response against RNA virus infections (Pinto et al., 2014; Dutta et al., 2017; Lazear et al., 2013) . Since its discovery Kawai et al., 2005; Meylan et al., 2005; Xu et al., 2005) , MAVS has become established as a central component of antiviral innate immunity and has served as a prototypic molecule in the study of virus-host co-evolution (Patel et al., 2012) . In the present study, we add to the current understanding how RV, a ubiquitous dsRNA virus and highly important human pathogen that is very sensitive to the antiviral effects of IFN (Arnold et al., 2013b) , avoids innate immune surveillance. By combining genome editing techniques, proteomics, mutagenesis, intestinal enteroids, and a highly tractable mouse model of homologous and heterologous RV infection and disease, we uncovered a unique mechanism employed by homologous RVs to target MAVS in their homologous host for degradation and inhibit the RNA sensing pathway in infected IECs. We found that human HT-29 cells produce significantly more IFN-l than IFN-b in response to the dsRNA RV infections ( Figure 1A) . This is consistent with the data derived from T84 cells, another human colonic epithelial cell line (Odendall et al., 2014) . That study also revealed a differentiation-dependent increase in the ratio of IFN-l/IFN-b expression, which correlated with the abundance of peroxisomes and IFN-l expression after viral infection. We also confirmed this finding using primary human intestinal enteroids that naturally harbor tight junctions similar to differentiated T84 cells ( Figure 1B) , suggesting that a preferential IFN-l induction appears to be a specific feature of human IECs. Despite the report of anti-RV roles of both type I and type III IFNs using various IFN receptor knockout mice in vivo (Lin et al., 2016; Pott et al., 2011) , whether IFN-l plays a physiological role in suppressing RV replication in an entirely human IEC environment awaits further testing. However, our other observation that pex-MAVS induces both IFN-l and IFN-b expression (Figure 1-figure supplement 1C , right panel) is in contrast to the previously reported role of pex-MAVS capable of specifically activating IFN-l in response to Listeria (Odendall et al., 2014; . In fact, our data are consistent with a more recent publication using viruses as stimuli and indicating that MAVSinduced IFN activation is independent of its subcellular location (Bender et al., 2015) , whether it be mitochondria or peroxisome. It is noteworthy that neither our present study nor the Bender S et al. paper (Bender et al., 2015) used a cytosolic MAVS as a control. It is likely that the extent of IFN-b induction via pex-MAVS occurs in a pathogen (or context)-specific manner.

It was previously noted that although RVs bound with the same efficiency to MA104 cells and HT-29 cells (Bass et al., 1992) , HT-29 cells appeared to be more sensitive to human RV infection than MA104 cells (Superti et al., 1991) . The molecular mechanism behind this cell culture restriction was unclear. Here, we found that human RVs replicate better in human origin cells by employing a novel strategy, a host range restricted MAVS degradation ability, to block IFN-l expression in infected IECs ( Figure 2C and Figure 2-figure supplement 1B) . Such a highly selective inhibitory event is reminiscent of the prototypic HCV NS3/4A protease and HAV ABC protease, both of which specifically inhibit human but not murine MAVS Yang et al., 2007) . This is another instructive example of virus-host co-evolution, resulting in a unique pattern of virus strain-host species matched MAVS degradation. Mechanistically, the RV RNA capping enzyme VP3 localizes to the mitochondria using a previously uncharacterized N-terminal domain (Ogden et al., 2014) (Figure 3figure supplement 1D) , induces MAVS phosphorylation at the SPLTSS motif ( Figure 4F ) and subsequent ubiquitination at the K10 residue within the CARD domain ( Figure 4D) , and this series of events mediates MAVS proteasomal degradation (Figure 2-figure supplement 1F , Figure 3E , and Figure 4E ). The identification of a novel phosphorylated SPLTSS motif is intriguing, given that a host kinase is likely involved. It also invites the question as to whether other proteins with a similar motif are subject to RV regulation. A quick search through the NCBI database reveals human mucin-3 precursor as a potential candidate, which has two SPLTSS motifs and is specifically expressed in the small intestine.

A missing piece in the understanding of the degradative interplay between VP3 and MAVS is the identity of a host E3 ubiquitin ligase. The fact that MAVS is K48 poly-ubiquitinated and degraded at the proteasome suggests the involvement of an E3 ligase activity ( Figures 2F and 4E) . Given the recent report that RV NSP1 requires the host Cullin-E3 ligase complex to degrade b-TrCP (Ding et al., 2016) , it is possible that RV does not possess a virally encoded E3 ligase(s). In an effort to identify host factors critical for VP3-mediated MAVS degradation, we tested the efficacy of MLN4924, a pan-cullin inhibitor (Soucy et al., 2009) , to inhibit MAVS degradation. However, this small molecule did not affect MAVS levels during RV infection (Figure 3-figure supplement 1F ). In addition, siRNA silencing of the expression of a panel of known MAVS negative regulators (Castanier et al., 2012; Yoo et al., 2015; You et al., 2009 ) had minimal effect on MAVS degradation (Figure 3-figure supplement 1F) . We also performed IP-MS and compiled a list of host E3 ligases that interact with MAVS during RV infection. Unfortunately, knocking down any of them did not rescue MAVS from degradation (Figure 3-figure supplement 1G) , leaving the possibility of some redundancy in usurping E3 ligase complexes by VP3 to target MAVS.

We extended our in vitro findings to the whole animal and demonstrated efficient VP3-mediated MAVS degradation during RV infection in the suckling mouse model. The degradation of MAVS at least partially contributes to the successful suppression of host innate immunity and RV host range restriction ( Figure 5) . Compared to the minimal effects of MAVS on homologous murine RV infection of suckling mice, the intra-intestinal replication and fecal shedding of heterologous simian RV was enhanced approximately 100-fold in Mavs -/mice ( Figure 5A and B). This enhancement was significantly more dramatic than the 10-fold difference that we observed in MAVS -/-HT-29 cells ( Figure 2A) . The disparity is likely due to both the type and amount of IFNs induced in these distinct environments: both type I and III IFNs from IECs and hematopoietic cells contribute to virus inhibition in vivo in contrast to a limited IFN-l secretion in HT-29 cells. This proposed model is in agreement with our data that the heterologous RV replication was not significantly different at extraintestinal tissues including the mesenteric lymph nodes in WT and Mavs -/mice ( Figure 5B) , where the dominant immune cell populations that RVs do not infect contribute to the majority of the IFNs (Lin et al., 2016) .

In summary, this work reveals a new phosphorylation motif (SPLTSS) within MAVS that is subject to RV VP3 mediated regulation ( Figure 4 ) and this effect on MAVS appears to be host range restricted. Our data also documents, for the first time, that inflammasome mediated antiviral signaling is comparable to IFN signaling in its ability to suppress heterologous RV replication ( Figure 5C ). As both IFN and inflammasome components are highly expressed in IECs and presumed to be mutually inhibitory (Guarda et al., 2011) , how these two antiviral signaling cascades are coordinated in the small intestine in response to viral infections will be an active focus of future studies. It might also be interesting to test whether other enteric RNA viruses, in particular norovirus, has developed similar approaches to suppress MAVS signaling in the small intestine.

African Green Monkey kidney epithelial cell lines MA104 (CRL-2378.1) and COS-7 (CRL-1651) were originally obtained from American Type Culture Collection (ATCC) and cultured in complete M199 medium. Human embryonic kidney cell line HEK293 (CRL-1573) and mouse embryonic fibroblast cell line NIH3T3 (CRL-1658) were obtained from ATCC and cultured in complete DMEM medium. Human colonic epithelial cell line HT-29 (HTB38) was obtained from ATCC and cultured in complete advanced DMEM/F12 medium. MAVS -/-HT-29 and HEK293 cells were generated using PX458 vector and CRISPR-Cas9 knockout technology as described and cultured in complete DMEM and DMEM/F12 medium respectively. All cell lines were tested negative for mycoplasma contamination.

MG132, Z-VAD-FMK (Selleckchem); MLN4924, GW4869 (Sigma); chloroquine (Invivogen); concanamycin A, rapamycin (Enzo); spiroepoxide (Santa Cruz); staurosporine (CST). Recombinant glycosidases PNGaseF and EndoH, and the substrate recombinant RNaseB protein were purchased from New England Biolabs.

EGFP-S-tandem-tagged RRV 12 genes in LAP6 vector have been previously described (Ding et al., 2016) . V5-tagged RRV VP3, EGFP-tagged VP3 from RRV, Wa, ETD, and chimera of ETD N-terminal 171 amino acids in RRV VP3 were generated. pRK5-HA-Ubiquitin (WT, mutants) was purchased from Addgene (#17608). Flag-tagged human, African Green monkey, and rhesus monkey MAVS constructs were purchased from Addgene (pMP31-1, #45905; pMP34-3, #45368; pMP45-1 #45372 respectively). pMSCV vectors encoding MAVS (WT, pex-MAVS with Pex13 transmembrane domain, mito-MAVS with Fis1 transmembrane domain) were purchased from Addgene (#52008, #44557, #44556 respectively). EGFP-tagged simian MAVS chimeric plasmids were PCR-amplified from pMP34-3 and cloned into EGFP-C1 vector. MAVS mutants K7A, K10A, K7AK10A, K7RK10R, SPLTSS to AAAAAA, R232AR236AR239A were generated using Quikchange II site-directed mutagenesis kit (Agilent). Flag-tagged MAVS and His-tagged VP3 were cloned into CET1019-AS vector (UC0E02, Millipore) for recombinant protein expression in CHO-S cell system.

Human and animal RV strains, including RRV (simian), SA11 (simian), Wa (human), DS1 (human), UK (bovine), OSU (porcine), SB1A (porcine), tissue-culture adapted ETD (murine), wild-type EW (murine), and reassortant RVs (B7/2, 8-1-1, 7-1-1, 14-1-1, 27-3-1, 3-2-1, D10/2, D6/2, and A/11) were propagated and purified by sucrose gradient ultracentrifugation as previously described (Ding et al., 2016; Feng et al., 2011; Feng et al., 2013) . UV-psoralen inactivation of RVs was performed as reported (Groene and Shaw, 1992) . Recombinant VSV (strain Indiana) expressing GFP was a kind gift from Dr. Jack Rose (Yale University).

B6129SF2/J wild-type and Mavs -/mice (B6;129-Mavs tm1Zjc /J) were purchased from the Jackson laboratory (stock number: 101045 and 008634 respectively) and bred in-house at the Veterinary Medical Unit of Palo Alto VA Health Care System (PAVAHCS). C57/BL6, Ifnar1 -/-, Casp1 -/-, Il18 -/-, Nlrp9b -/were used as previously described (Lin et al., 2016; Zhu et al., 2017) . For all RV infections, sex and age-matched suckling pups at 5 days of age were used and whenever possible, littermates were used to minimize the effect of specific microbiome differences on the experiments.

IEC isolation by EDTA-DTT extraction method and flow cytometry of mature villous IECs were performed as previously described (Sen et al., 2012) . Fecal shedding of viral antigens, and detection of RV replication by RT-qPCR were performed as described .

Flag-tagged rhesus MAVS (from pMP34-3) and His-tagged RRV VP3 (from pT-Rex-DEST31-RRV3) were cloned into CET 1019 AS-Puro mammalian expression vector (Millipore). CHO-S cells were transfected with each construct using the DMRIE-C reagent (Invitrogen) as previously described (Yamaguchi et al., 2011) . After 48 hr, the cells were seeded at a density of 5 Â 10 4 cells/ml in 100 ml/well in 96-well plates. Clones were selected with 10 mg/ml puromycin. After 12 days, protein expression was measured by western blot and high production clones were selected. CHO-S cells stably expressing the chemerin isoforms were seeded into 800 ml of CD-CHO medium at 2 Â 10 5 cells/ml in a Spinner flask. After 4 days of culture at 37˚C, the conditioned medium was collected by centrifugation, filtered through a 0.22 mm filter, applied to a HiTrap SP HP column (GE Healthcare) and purified with anti-Flag M2 Affinity Gel (Sigma, A2220) and His60 Ni Resin (Takara, 635659).

HT-29 cells or MA104 cells were infected with human RV Wa strain or simian RV RRV strain (MOI = 3) respectively. Mock or RV-infected cells were harvested at 12 h.p.i. and lysates were subjected to immunoprecipitation using anti-MAVS antibody (Bethyl, #A300-783A) and magnetic bead separation (Pierce). MA104 lysates were further resolved in SDS-PAGE gel and cut into eight pieces for peptide retrieval. HT-29 lysates were subjected to a second-round of immunoprecipitation using another anti-MAVS antibody (Bethyl, #A300-782A). Samples were submitted to Stanford Mass Spectrometry core facility for proteomics and post-translational modification analysis.

Total RNA was extracted from cells using RNeasy Mini kit (Qiagen) and reverse transcription was performed with High Capacity RT kit and random hexamers as previously described (Bolen et al., 2014) . QPCR was performed using the Stratagene Mx3005P (Agilent) with a 25 ml reaction, composed of 50 ng of cDNA, 12.5 ml of Power SYBR Green master mix (Applied Biosystems), and 200 nM both forward and reverse primers. All SYBR Green primers used in this study (listed in Supplementary file 2) have been validated with both dissociation curves and electrophoresis of the correct amplicon size. Taqman primers used in this study are also listed in Supplementary file 2.

Cell lysates were harvested in RIPA buffer supplemented with protease and phosphatase inhibitors. Proteins were resolved in SDS-PAGE gel and analyzed by antibody as previously described . Flag (Sigma, M2, #F3165), GAPDH (BioLegend, #631402), GFP (CST, #2555), SUMO1 (CST, C9H1, #4940), SUMO2/3 (CST, 18H8, #4971), IRF1 (CST, D5E4, #8478), IRF3 (CST, D6I4C, #11904), human MAVS (Bethyl lab, #A300-782A; CST, #3993; Santa Cruz, E-3 clone; sc-166583), mouse MAVS (Santa Cruz, E-6 clone, sc-365334), ubiquitin (CST, #3933), V5 (CST, #13202). Secondary antibodies raised against rabbit (CST, #7074), or mouse (CST, D3H8Q, #7076) IgG were HRP-linked. Bands were visualized with Clarity ECL substrate (Biorad, #170-5061), Amersham Hyperfilm (GE Healthcare) and STRUCTURIX X-ray film processor (GE Healthcare). Relative protein levels were measured by ImageJ on the basis of at least three independent western blots.

Cells were fixed and analyzed as described (Ding et al., 2018) . In brief, cells were fixed with 4% paraformaldehyde and stained with the following primary antibodies or fluorescent dyes: DAPI (Thermo Fisher, P36962). Stained cells were washed with PBS, mounted with Antifade Mountant with DAPI (Thermo, P36962), and imaged with Zeiss LSM 710 Confocal Microscope. Confocal images were analyzed by Volocity v5.2.

MA104 cells were transfected with siRNA using a reverse transfection protocol as previously described (Gutiérrez et al., 2010) . In brief, 15 ml Oligofectamine (Invitrogen) was diluted in 1 ml MEM and incubated for 10 min at RT. This mixture was then added to a well of a 48-well plate containing the siRNA, also diluted in MEM. After an incubation of 20 min at RT, 200 ml of a single-cell suspension of 0.5 Â 10 5 MA104 cells/ml was added to each well, and the cells were incubated at 37˚C. 72 hr later, the transfection mixture was removed and the cells were washed twice with MEM and infected with RV.

All bar graphs were displayed as means ± SEM. Statistical significance in data Figures Figure 5A ) was calculated by the c 2 test. All data were presented as asterisks (*p 0.05; **p 0.01; ***p 0.001). All experiments, unless otherwise noted, have been repeated at least three times.

All in vivo mouse studies were approved under the ACORP number GRH1397 entitled 'Rotavirus: Studies of Intestinal Tropism and Innate and Heterotypic Immunity' approved by The Institutional Animal Care Committee at VAPAHCS. The use of human origin ileum enteroids was approved under the eProtocol number 28908 entitled 'Development of a New Method for Culturing and Growing Human Solid Tumors and Normal Tissues in vitro' by the Panel On Medical Human Subjects at Stanford University.

Rotavirus NSP1 mediates degradation of interferon regulatory factors through targeting of the dimerization domain

The battle between rotavirus and its host for control of the interferon signaling pathway

Rotavirus nonstructural protein 1 subverts innate immune response by inducing degradation of IFN regulatory factor 3

Liposome-mediated transfection of intact viral particles reveals that plasma membrane penetration determines permissivity of tissue culture cells to rotavirus

Activation of type I and III interferon response by mitochondrial and peroxisomal MAVS and inhibition by hepatitis C virus

MAVS and MyD88 are essential for innate immunity but not cytotoxic T lymphocyte response against respiratory syncytial virus

Dynamic expression profiling of type I and type III interferonstimulated hepatocytes reveals a stable hierarchy of gene expression

RIG-I/MDA5/MAVS are required to signal a protective IFN response in rotavirus-infected intestinal epithelium

A bicistronic MAVS transcript highlights a class of truncated variants in antiviral immunity

MAVS ubiquitination by the E3 ligase TRIM25 and degradation by the proteasome is involved in type I interferon production after activation of the antiviral RIG-I-like receptors

Analysis of host range restriction determinants in the rabbit model: comparison of homologous and heterologous rotavirus infections

Epigenetic reprogramming of the type III interferon response potentiates antiviral activity and suppresses tumor growth

Peroxisomal MAVS activates IRF1-mediated IFN-l production

Comparative proteomics reveals strain-specific b-TrCP degradation via rotavirus NSP1 hijacking a host cullin-3-Rbx1 Complex

STAG2 deficiency induces interferon responses via cGAS-STING pathway and restricts virus infection

A systems approach reveals mavs signaling in myeloid cells as critical for resistance to ebola virus in murine models of infection

Fields Virology Rotaviruses

Roles of VP4 and NSP1 in determining the distinctive replication capacities of simian rotavirus RRV and bovine rotavirus UK in the mouse biliary tract

Permissive replication of homologous murine rotavirus in the mouse intestine is primarily regulated by VP4 and NSP1

Hepatitis C virus NS3-4A inhibits the peroxisomal MAVS-dependent antiviral signalling response

Rotavirus NSP1 inhibits NFkappaB activation by inducing proteasomedependent degradation of beta-TrCP: a novel mechanism of IFN antagonism

Psoralen preparation of antigenically intact noninfectious rotavirus particles

Type I interferon inhibits interleukin-1 production and inflammasome activation

Different rotavirus strains enter MA104 cells through different endocytic pathways: the role of clathrin-mediated endocytosis

Interferon-l and interleukin 22 act synergistically for the induction of interferon-stimulated genes and control of rotavirus infection

MAVS-dependent host species range and pathogenicity of human hepatitis A virus

PhosphoSitePlus, 2014: mutations, PTMs and recalibrations

MAVS forms functional prion-like aggregates to activate and propagate antiviral innate immune response

Regulation of type I interferon responses

Differential roles of MDA5 and RIG-I helicases in the recognition of RNA viruses

IPS-1, an adaptor triggering RIG-I-and Mda5-mediated type I interferon induction

RIG-I in RNA virus recognition

alpha(4)beta(7) independent pathway for CD8(+) T cell-mediated intestinal immunity to rotavirus

IRF-3, IRF-5, and IRF-7 coordinately regulate the type I IFN response in myeloid dendritic cells downstream of MAVS signaling

Hepatitis C virus protease NS3/4A cleaves mitochondrial antiviral signaling protein off the mitochondria to evade innate immunity

Exosomes mediate the cell-to-cell transmission of IFN-a-induced antiviral activity

Drebrin restricts rotavirus entry by inhibiting dynamin-mediated endocytosis

Distinct roles of type I and type III interferons in intestinal immunity to homologous and heterologous rotavirus infections

Phosphorylation of innate immune adaptor proteins MAVS, STING, and TRIF induces IRF3 activation

The PB2 subunit of the influenza a virus rna polymerase is imported into the mitochondrial Matrix

Cardif is an adaptor protein in the RIG-I antiviral pathway and is targeted by hepatitis C virus

NLRX1 is a regulator of mitochondrial antiviral immunity

MAVS protein is attenuated by rotavirus nonstructural protein 1

Diverse intracellular pathogens activate type III interferon expression from peroxisomes

Predicted structure and domain organization of rotavirus capping enzyme and innate immune antagonist VP3

Convergent evolution of escape from hepaciviral antagonism in primates

Type I and Type III Interferons Display Different Dependency on Mitogen-Activated Protein Kinases to Mount an Antiviral State in the Human Gut

Deficient IFN signaling by myeloid cells leads to MAVS-dependent virus-induced sepsis

IFN-lambda determines the intestinal epithelial antiviral host defense

Rotavirus Controls Activation of the 2'-5'-Oligoadenylate Synthetase/RNase L Pathway Using at Least Two Distinct Mechanisms

Human intestinal enteroids: a new model to study human rotavirus infection, host restriction, and pathophysiology

A paradox of transcriptional and functional innate interferon responses of human intestinal enteroids to enteric virus infection

The mitochondrial antiviral signaling protein, MAVS, is cleaved during apoptosis

Innate immune response to homologous rotavirus infection in the small intestinal villous epithelium at singlecell resolution

Rotavirus degrades multiple type interferon receptors to inhibit IFN signaling and protects against mortality from endotoxin in suckling mice

Identification and characterization of MAVS, a mitochondrial antiviral signaling protein that activates NF-kappaB and IRF 3

Rotavirus and reovirus modulation of the interferon response

SARS-coronavirus open reading frame-9b suppresses innate immunity by targeting mitochondria and the MAVS/TRAF3/TRAF6 signalosome

An autoinhibitory mechanism modulates MAVS activity in antiviral innate immune response

An inhibitor of NEDD8-activating enzyme as a new approach to treat cancer

The specific and essential role of MAVS in antiviral innate immune responses

HT-29 cells: a new substrate for rotavirus growth

Characterization of rotavirus RNAs that activate innate immune signaling through the RIG-I-like receptors

MDA5 and MAVS mediate type I interferon responses to coxsackie B virus

Enterovirus 71 protease 2Apro targets MAVS to inhibit anti-viral type I interferon responses

VISA is an adapter protein required for virus-triggered IFN-beta signaling

Structural basis for the prion-like MAVS filaments in antiviral innate immunity

Proteolytic cleavage of chemerin protein is necessary for activation to the active form, Chem157S, which functions as a signaling molecule in glioblastoma

Disruption of innate immunity due to mitochondrial targeting of a picornaviral protease precursor

The mitochondrial ubiquitin ligase MARCH5 resolves MAVS aggregates during antiviral signalling

PCBP2 mediates degradation of the adaptor MAVS via the HECT ubiquitin ligase AIP4

MAVS, cGAS, and endogenous retroviruses in T-independent B cell responses

Homologous 2',5'-phosphodiesterases from disparate RNA viruses antagonize antiviral innate immunity

MAVS expressed by hematopoietic cells is critical for control of west nile virus infection and pathogenesis

The E3 ubiquitin ligase RNF5 targets virus-induced signaling adaptor for ubiquitination and degradation

Nlrp9b inflammasome restricts rotavirus infection in intestinal epithelial cells

We would like to thank all members of the Greenberg lab for their support. We are grateful to the in-house anti-Tyr-AMP and anti-Thr-AMP antibodies from Dr. Kim Orth (UT Southwestern). We appreciate Drs. Ryan Leib and Christopher Adams from the Stanford MS core facility for carrying out the MS analysis and Lusijah Rott at the VA FACS facility for cell sorting. This work is supported by NIH grants R01 AI125249, U19 AI116484 and by VA Merit review grant GRH0022 awarded to HBG. SD is supported by a Walter V and Idun Berry Postdoctoral Fellowship, a Stanford Institute for Immunity, Transplantation and Infection (ITI) Young Investigator Award, an Early Career Award from the Thrasher Research Fund and NIH Career Development Award K99 AI135031. SZ is supported by grants from the National Natural Science Foundation of China (81788104) and (31770990) 

Ethics Animal experimentation: Age and sex-matched were used in this study. Mice were specific pathogen-free, maintained under a strict 12 hour light cycle, and given a regular chow diet ad libitum. All protocols used in this study were compliant with the Veterinary Medical Unit of Palo Alto VA Health Care System (PAVAHCS) and approved by the IACUC committee. 

The data that support the findings of this study are available in the main text, main figures, supplementary figures or attached as Supplementary files 1 and 2. Additional information is available in the format of Source data.