key: cord-0750442-g1muealp authors: Belov, George A; van Kuppeveld, Frank JM title: (+)RNA viruses rewire cellular pathways to build replication organelles date: 2012-10-01 journal: Curr Opin Virol DOI: 10.1016/j.coviro.2012.09.006 sha: 80949ce99e6ecb18f6e030334e48d3712431c4dd doc_id: 750442 cord_uid: g1muealp Positive-strand RNA [(+)RNA] viruses show a significant degree of conservation of their mechanisms of replication. The universal requirement of (+)RNA viruses for cellular membranes for genome replication, and the formation of membranous replication organelles with similar architecture, suggest that they target essential control mechanisms of membrane metabolism conserved among eukaryotes. Recently, significant progress has been made in understanding the role of key host factors and pathways that are hijacked for the development of replication organelles. In addition, electron tomography studies have shed new light on their ultrastructure. Collectively, these studies reveal an unexpected complexity of the spatial organization of the replication membranes and suggest that (+)RNA viruses actively change cellular membrane composition to build their replication organelles. (+)RNA viruses rewire cellular pathways to build replication organelles George A Belov 1 and Frank JM van Kuppeveld 2 Positive-strand RNA [(+)RNA] viruses show a significant degree of conservation of their mechanisms of replication. The universal requirement of (+)RNA viruses for cellular membranes for genome replication, and the formation of membranous replication organelles with similar architecture, suggest that they target essential control mechanisms of membrane metabolism conserved among eukaryotes. Recently, significant progress has been made in understanding the role of key host factors and pathways that are hijacked for the development of replication organelles. In addition, electron tomography studies have shed new light on their ultrastructure. Collectively, these studies reveal an unexpected complexity of the spatial organization of the replication membranes and suggest that (+)RNA viruses actively change cellular membrane composition to build their replication organelles. (+)RNA viruses infect almost all eukaryotic organisms, often inducing devastating diseases in humans, animals and plants. Despite adaptation to diverse hosts, the replication mechanisms of (+)RNA viruses display remarkable conservation. These viruses universally require cellular membranes for assembly of their replication complexescontaining viral proteins, RNA, and host factorsto amplify their genome. To convert cellular membranes into replication sites, (+)RNA viruses must have evolved efficient ways of manipulating the highly regulated cellular membrane metabolism. The small genome size of these viruses and thus limited repertoire of available resources suggests that they rely on only a few evolutionarily successful strategies shared among different viruses. Recently, major advances have been made in understanding of virus-cell interaction of several groups of (+)RNA viruses. The pioneering research of picornavirus-induced membrane remodeling has been complemented lately by detailed examinations of the biochemistry and morphology of replication organelles of flaviviruses, alphaviruses and nidoviruses. Many important insights into virus-induced membrane modifications were gained from studies on Flock House virus and Brome Mosaic virus (BMV), which can replicate in yeast, allowing application of yeast genetic tools to elucidate the role of specific host factors. These studies revealed important similarities in the principles of remodeling cellular membranes and organizing replication sites among diverse (+)RNA viruses. The development and functioning of these structures require rewiring of cellular pathways into new configurations that are induced and regulated by viral proteins. In this review, we will describe new data on the organization and development of replication structures and focus on the emerging concept that viral membranous replication complexes are bona fide new organelles with unique lipid and protein compositions. Recently, 3D electron tomography (ET) was applied to resolve the complex spatial organization of replication membranes of picorna, flavi, corona, arteri and nodaviruses [1 ,2 ,3 ,4 ,5 ,6 ]. Conventional EM and ET studies collectively show that different (+)RNA viruses initiate development of their replication structures on different cellular organelles and that the degree of the remodeling of the original cellular membrane architecture varies greatly. However, it appears that there are only a few basic configurations of replication-associated membranes: invaginations, tubular-vesicular networks, double or multimembrane vesicles, and convoluted membranes without identifiable topological units. Different combinations of membranous structures can often be simultaneously observed in one infected cell, or they can develop in a defined succession during the course of infection. It is not always clear whether these structures contribute equally to RNA replication or have other specialized functions in the viral life cycle. For enveloped viruses, distinct membrane structures may be expected to be associated with genome replication and virion maturation. Indeed, genome replication of HCV is associated with a membranous web believed to originate from ER membranes [7] , while RNA encapsidation is linked to the surface of lipid droplets [8, 9] . Polyprotein processing, RNA replication and virion maturation each appear to be confined to different membrane compartments in cells infected with arthropod-borne flaviviruses [3 ,10,11] . Time-dependent evolution of membrane structures, implicated to reflect distinct stages of virus propagation, has been described for coronaviruses [1 ,12] , and recently for enteroviruses (i.e. poliovirus and coxsackievirus). Early in infection enteroviruses replicate their RNA on single membrane convoluted tubular clusters that later in infection are converted into double-membrane vesicles (DMV) and complex multimembrane structures [4 ,5 ] . Although DMV may contribute to enterovirus RNA replication, they have also been implicated in non-lytic release of newly formed virions [13] . Morphology of replication structures is conserved among large taxa of viruses (+)RNA viruses can be divided into three superfamilies: picorna-like, alpha-like and flavi-like viruses [14] [15] [16] . Interestingly, flavi-and alpha-like viruses induce formation of discrete membrane invaginations with negative membrane curvature [3 ,17 ,18,19] , while picorna-like viruses rely on positively curved convoluted tubular-vesicular membrane networks [1 , 4 ,5 ,20-23] . In the invaginations, the replication machinery is located on the inner membrane surface and the replication compartment is connected to the cytoplasm with an opening wide enough to provide a supply of nucleotides and to export synthesized RNA [2 ,3 ] . In tubulo-vesicular replication structures, the viral replication proteins are localized on the external membranous surface facing the cytoplasm [24] . This division may reflect an evolutionary divergence between (+)RNA virus groups and suggest that the mechanisms of membrane remodeling may be significantly different between picorna-like and other (+)RNA viruses ( Figure 1 ). In general, remodeling of cellular membranes requires coordinated lipid sorting and/or actions of specific membrane shaping protein complexes [25, 26] . Here, we will discuss the roles of autophagy, the secretory pathway, and lipid biosynthesis in the development and/or functioning of replication organelles. For the role of protein-dependent membrane-shaping mechanisms, the reader is referred to a recent review [27] . Activation of at least initial steps of the autophagy pathway is well documented in cells infected with diverse (+)RNA viruses. Since a double membrane is a distinctive feature of autophagosomes, it was initially suggested that autophagy-like processes may be responsible for the generation of double membrane replication structures. However conflicting data on the importance of autophagy for replication of coronaviruses [1 , [28] [29] [30] [31] and enteroviruses [32] [33] [34] suggest that DMV are either not essential for replication, or that they bear only superficial resemblance to autophagosomes. Recently, an autophagy-independent role of LC3 in tuning the ER-associated degradation (ERAD) pathway was suggested to be important for coronavirus replication, indicating that viruses may selectively utilize autophagy/ERAD pathway components to generate replication membranes [35, 36] . Although an intact autophagy pathway may not be required for bona fide genome replication of (+)RNA viruses, autophagy may be induced upon infection as it plays an important regulatory role in the type I interferon response [37] . Indeed, activation of autophagy by HCV and Dengue virus has recently been shown to suppress the cellular capacity to activate this antiviral innate response [38, 39] . Replication of most (+)RNA viruses is intimately associated with cellular secretory pathway(-derived) membranes ( Figure 2 ). Below the roles of some common membrane-remodeling host factors identified to be required for (+)RNA virus replication are discussed. GBF1, a guanine nucleotide exchange factor for the small GTPase Arf1 and a target of brefeldin A (BFA), coordinates the formation and fusion of transport vesicles in trafficking between ER and early Golgi [40] . GBF1 was recognized as an essential factor for replication of enteroviruses [41] [42] [43] , but not other picornaviruses such as cardioviruses and aphthoviruses [44, 45] . GBF1 has also been implicated in replication of HCV and mouse hepatitis coronavirus [46, 47] . Several lines of evidence suggest that the role of GBF1 in viral replication is unrelated to its normal function in transport vesicle formation and Arf1 activation. Expression of poliovirus and HCV proteins in the presence of BFA resulted in the appearance of new membrane structures that are indistinguishable from those observed without the drug, indicating that GBF1 is more probably involved in the function of replication organelles than in their formation [41, 45] . Moreover, while activated Arf1 accumulates on enterovirus replication organelles, BFA-resistant poliovirus mutants can efficiently replicate without active Arf1, and siRNA knockdown of Arf1 does not affect coxsackievirus replication [42, 48 ] . Lastly, expression of truncated GBF1 deficient in supporting cellular metabolism rescued poliovirus replication in the presence of BFA [48 ] . Replication membranes of enteroviruses were shown to become enriched in PI4KIIIb, but depleted of coat proteins, yielding unique uncoated phosphatidylinositol-4-phosphate (PI4P) lipid-enriched organelles [49 ] . It was proposed that recruitment of PI4KIIIb to replication organelles depends on the interaction of viral protein 3A with GBF1 as well as on the Arf1 activation function of GBF1 [45, 49 ] . However, the observations that Arf1 as well as strong 3A-GBF1 interaction may be dispensable for enterovirus replication [42] (G. Belov, F. van Kuppeveld, unpublished data) argue that this model may be an oversimplification of the actual processes ( Figure 3 ). Another PI4K, PI4KIIIa, is recruited to replication sites of HCV by viral protein NS5A [50, 51 ] . Inhibition of PI4K activity potently blocks replication of enteroviruses and HCV, showing that PI4P is an important component of their replication membranes [49 ,52,53] . As is the case for GBF1, PI4Ks are not required for the replication of all (+)RNA viruses and even viruses from one family may demonstrate different requirements for PI4Ks [51 ,54] product of PI4K activity, is likely to mediate recruitment and/or activation of viral proteins and host factors on replication organelles (e.g. PI4P-binding cellular proteins such as oxysterol binding proteins and ceramide transport protein), where they may support RNA replication directly or indirectly by remodeling membranes (Figure 3 ). Poliovirus polymerase 3D has been shown to preferentially bind PI4P in a biochemical assay, but the relevance of this observation for replication in vivo remains to be elaborated [49 ] . For HCV, the absence of PI4KIIIa activity induced a dramatic change in the ultrastructural morphology of the membranous replication complex, suggesting a role of PI4P in recruiting specific membrane-shaping proteins [51 ] . Taken together, these data suggest that (+)RNA viruses do not rely on a functional secretory pathway, but rather dismantle it and stitch together separate elements in new configurations that serve to support viral genome replication. Despite the critical role of GBF1 and PI4K in replication, enteroviruses can become resistant to inhibitors targeting these factors, suggesting built-in redundancy of essential virus-cell interactions [55, 56] . Other studies have shown that replication of some (+)RNA viruses can be Schematic overview of the secretory pathway and the sites targeted and/or altered by (+)RNA viruses for formation of their membranous replication organelles. For reasons of simplicity, the endocytic pathway and the lysosomes are combined. Secretory pathway transport depends on specific coat complexes that contribute by mediating the bending, deformation and detachment of membranes carriers. Anterograde transport of proteins out of the ER takes place via a COP-II dependent pathway, whereas intra-Golgi transport as well as retrograde transport from the Golgi and intermediated compartment relies on COP-I-coated carries. Endocytosis takes place via clathrin-coated vesicles. The putative sites that are targeted and/or altered by different (+)RNA viruses (Family and Genera names of the viruses are given here below between parenthesis) to form their replication organelles are indicated by their position. Essential host factors and their localization are also indicated. CV, coxsackievirus (Picornaviridae, Enterovirus). redirected to alternative intracellular membranes, suggesting a remarkable plasticity of the viral replication machinery regarding the availability of at least some cellular factors [57, 58, 59 ] . The multiple compensatory mechanisms may be important for replication in different cell types, where availability of cellular components may vary. This may serve as an essential source of evolutionary elasticity, and allow adaptation to changing conditions, including chemotherapeutic interventions. The remarkable conservation of the overall design of the membranous replication complexes among distant (+)RNA viruses suggests shared basic mechanisms of their formation. Currently known elements of the autophagy and/or secretory pathways cannot fit the bill, since even related viruses display significant variability in requirements for these factors. The only universal feature of the (+)RNA virus infection that emerges over the years of research seems to be the obligatory modulation of cellular lipid biosynthesis pathways. Picornavirus (picorna-like superfamily) infection is long known to significantly enhance cellular phospholipid synthesis [60] [61] [62] . Investigation of BMV (alpha-like superfamily) replication in yeast system showed that formation of replication structures strongly depends on the 744 Virus replication in animals and plants Possible functions of GBF1 and PI4KIIIb/PI4P in formation and/or activity of enterovirus replication organelles. Enterovirus replication starts at Golgi membranes where the viral 3A protein interacts with GBF1, a GEF for Arf1 that in uninfected cells is involved in recruiting COP-I coats to membranes (left). The interaction of 3A with GBF1 interferes with COP-I recruitment, resulting in uncoated membranes that can no longer function in secretory pathway trafficking. At the same time, 3A causes an increased recruitment of PI4KIIIb to membranes. Although this lipid kinase is an effector of Arf1 in uninfected cells, growing evidence suggests that the interaction of 3A with GBF1/Arf1 is not essential for the massive recruitment of PI4KIIIb observed in infected cells. 3A may directly interact with PI4KIIIb or this interaction may occur via another cellular protein (e.g. ACBD3, which has recently been reported to bind 3A as well as PI4KIIIb [68,69]). Enhanced recruitment of PI4KIIIb results in PI4P enriched membranes, which may serve to activate and/or recruit viral and/or cellular proteins that are directly involved in replication of the viral RNA. One candidate protein is the viral RNA-dependent RNA polymerase, 3D, which has been shown to bind PI4P lipids in vitro. Additionally, PI4P-rich membranes may serve as docking sites for other cellular proteins that exert functions in membrane remodeling that contribute to the formation of the membranous environment suitable for RNA replication. metabolism of fatty acids and other lipids [63, 64] . Recently, new high-throughput lipidomics techniques allowed resolution of profound changes in the lipid spectrum upon Dengue virus (flavi-like superfamily) infection [65 ] . Replication of many viruses has been proposed to depend on the activity of cellular fatty acid synthase (FAS). Expression of FAS is activated in HCV-infected cells [66] and the enzyme is recruited to the replication membranes of Dengue virus [67] . The apparently universal up-regulation of lipid metabolism by (+)RNA viruses raises interesting questions: Are the local changes in structural lipid composition the major driving force for formation of the membranous replication sites? Are these sites further stabilized by interaction with viral and/or cellular proteins? Do (+)RNA viruses remodel pre-existing cellular membranes, as we generally assume, or do they actually build replication membranes de novo and thus can they be truly called ''novel replication organelles''? We are only beginning to understand the complex details of biogenesis of viral replication organelles and their role in infection of (+)RNA viruses, and many questions still need to be resolved. The shared morphology of replication structures and the apparently universal requirement for active lipid synthesis strongly suggest that key steps of their formation are shared among distantly related viruses. (+)RNA viruses actively change cellular membranes, rather than rely on pre-existing membranes. They relocate key cellular regulators of membrane metabolism, and modulate their activities to create new pathways of membrane remodeling. Redundant networks of crucial viruscell interactions that allow the generation of a favorable replication microenvironment may exist, thereby providing viruses the opportunity to adapt to and evolve under changing conditions. Understanding how viral proteins hijack regulatory mechanisms of membrane metabolism will undoubtedly bring new perspective to many areas of cell biology and will be indispensable for the development of a new generation of anti-viral control strategies. 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Work in the lab of GB is supported by the start-up funds of the University of Maryland. Work in the lab of FvK is supported by research grants from the Netherlands Organization for Scientific Research (NWO-VICI-91812628, NWO-ECHO-700.57.001, NWO-ALW-820.02.018) and the European Union 7th Framework (EUVIRNA Marie Curie Initial Training Network, grant agreement number 264286, and SILVER Large Scale Collaborative Project, grant agreement number 260644).