key: cord-331802-wo462anq
authors: Xia, Hongjie; Wang, Peipei; Wang, Guang-Chuan; Yang, Jie; Sun, Xianlin; Wu, Wenzhe; Qiu, Yang; Shu, Ting; Zhao, Xiaolu; Yin, Lei; Qin, Cheng-Feng; Hu, Yuanyang; Zhou, Xi
title: Human Enterovirus Nonstructural Protein 2C(ATPase) Functions as Both an RNA Helicase and ATP-Independent RNA Chaperone
date: 2015-07-28
journal: PLoS Pathog
DOI: 10.1371/journal.ppat.1005067
sha: 
doc_id: 331802
cord_uid: wo462anq

RNA helicases and chaperones are the two major classes of RNA remodeling proteins, which function to remodel RNA structures and/or RNA-protein interactions, and are required for all aspects of RNA metabolism. Although some virus-encoded RNA helicases/chaperones have been predicted or identified, their RNA remodeling activities in vitro and functions in the viral life cycle remain largely elusive. Enteroviruses are a large group of positive-stranded RNA viruses in the Picornaviridae family, which includes numerous important human pathogens. Herein, we report that the nonstructural protein 2C(ATPase) of enterovirus 71 (EV71), which is the major causative pathogen of hand-foot-and-mouth disease and has been regarded as the most important neurotropic enterovirus after poliovirus eradication, functions not only as an RNA helicase that 3′-to-5′ unwinds RNA helices in an adenosine triphosphate (ATP)-dependent manner, but also as an RNA chaperone that destabilizes helices bidirectionally and facilitates strand annealing and complex RNA structure formation independently of ATP. We also determined that the helicase activity is based on the EV71 2C(ATPase) middle domain, whereas the C-terminus is indispensable for its RNA chaperoning activity. By promoting RNA template recycling, 2C(ATPase) facilitated EV71 RNA synthesis in vitro; when 2C(ATPase) helicase activity was impaired, EV71 RNA replication and virion production were mostly abolished in cells, indicating that 2C(ATPase)-mediated RNA remodeling plays a critical role in the enteroviral life cycle. Furthermore, the RNA helicase and chaperoning activities of 2C(ATPase) are also conserved in coxsackie A virus 16 (CAV16), another important enterovirus. Altogether, our findings are the first to demonstrate the RNA helicase and chaperoning activities associated with enterovirus 2C(ATPase), and our study provides both in vitro and cellular evidence for their potential roles during viral RNA replication. These findings increase our understanding of enteroviruses and the two types of RNA remodeling activities.

For both cells and viruses, the functionality of RNA molecules usually requires correct folding into proper tertiary structures and the association with correct RNA-binding proteins [1, 2] . To make the scenario more complex, RNA molecules frequently function via transient base pairing with target RNAs and/or dynamic association/dissociation with distinct RNA-binding proteins [3] . However, correct folding of RNAs is quite challenging and time-consuming, because RNAs can easily become trapped in thermodynamically stable intermediates that are misfolded and inactive. In response, cells and viruses encode a variety of "helper" or RNA remodeling proteins, such as RNA helicases and RNA chaperones, that can destabilize RNA-RNA or RNA-DNA base pairing, thereby lowing the thermodynamic barrier between RNA conformations and promoting the proper formation of RNA tertiary structures [4] [5] [6] . It is believed that RNA remodeling proteins play pivotal roles in nearly all processes involving RNA molecules.

RNA helicases are highly similar to DNA helicases, contain ATPase activity, and utilize the energy of ATP binding and/or hydrolysis to translocate along and unwind RNA duplexes. They are thought to participate in most ATP-dependent remodeling of structured RNAs and are classified into six superfamilies (SFs), designated SF1 to SF6, on the basis of conserved helicase motifs [7] . On the other hand, RNA chaperones are a heterogeneous group of proteins that share no consensus sequences or motifs but are able to destabilize RNA duplexes and assist in the formation of more globally stable RNA structures. The major difference between RNA chaperones and helicases is that RNA chaperones do not require ATP binding or hydrolysis for their remodeling activities [8] . (Of note, the definition of RNA chaperones is sometimes blurred, as some publications have defined helicases as a subgroup of ATP-dependent RNA chaperones [2] . Herein, like in most publications, we define RNA helicases and chaperones as two separate classes of the RNA remodelers for the sake of clarity.)

For viruses, particularly RNA viruses, their viral RNAs (vRNAs) contain multiple cis-acting elements that play pivotal roles in vRNA replication and translation. These highly structured RNA elements require RNA helicases or chaperones to aid in their proper folding and re-folding. Moreover, during vRNA replication, replicative intermediate double-stranded RNA (dsRNA) must be unwound by virus-encoded or cellular RNA helicases; therefore, vRNA templates can be efficiently re-utilized to synthesize more progeny vRNA strands. Thus far, a variety of RNA viruses, such as flavivirus NS3 [9] , alphavirus NSP2 [10] , coronavirus nsp13 [11] , and alphatetravirus Hel [12] , have been reported to encode their own RNA helicases, and the majority of them belong to helicase SF1 and SF2 [7] .

Enteroviruses are a large group of positive-stranded RNA viruses in the Picornaviridae family that contain numerous important human pathogens, including poliovirus, enterovirus 71 (EV71), coxsackie viruses, and echoviruses. They cause approximately 3 billion human infections annually and are responsible for a wide spectrum of diseases, ranging from relatively mild conditions, such as common cold, upper respiratory illness, and hand-foot-and-mouth disease (HFMD), to severe conditions such as aseptic meningitis, encephalitis, myocarditis, neonatal sepsis-like disease, and poliomyelitis [13] . So far, although vaccination has almost eradicated poliomyelitis worldwide [14] , no effective vaccine or antiviral therapy is available for many other important human enteroviruses, particularly neurotropic EV71, which is the major causative pathogen for HFMD and a serious lethal threat to children. Enterovirus encodes a single polyprotein that is proteolytically cleaved into separate structural and nonstructural proteins. Among them, the multifunctional protein 2C ATPase is the most conserved and complex but the least understood ( Fig 1A) . Enterovirus 2C ATPase has been reported to participate in diverse processes, including RNA binding [15, 16] , RNA replication [17] [18] [19] , membrane anchoring and rearrangement [20, 21] , autophagy inhibition [22] , encapsidation and viral morphogenesis [23, 24] , and suppression of nuclear factor kappa B activation [25] . 2C ATPase has long been predicted as a putative SF3 helicase on the basis of its AAA+ ATPase activity and conserved SF3 signature motifs (Fig 1B) [26, 27] . Similar to other well-defined SF3 helicases, such as Simian virus 40 (SV40) large T antigen (LTag), human papillomavirus (HPV) E1, and adeno-associated virus (AAV) Rep, enterovirus 2C ATPase has been reported to form homo-oligomeric ringlike structures in vitro, which is required for its ATPase activity [28] . Moreover, this protein appears to associate with vRNA in the vRNA replication complexes in infected cells [29] , implying that 2C ATPase directly participates in enteroviral RNA replication. However, previous attempts to determine the helicase activity associated with 2C ATPase or other enteroviral proteins have been unsuccessful [27] . Thus, whether enteroviral or picornaviral RNA replication requires the involvement of any virus-encoded RNA remodeling activity is not known, and this gap hinders our understanding of this large group of medically important pathogenic viruses.

Interestingly, our previous study of the 2C ATPase protein from Ectropis obliqua picorna-like virus (EoV; genus Iflavirus, family Iflaviridae, order Picornavirales) revealed that EoV 2C ATPase possesses RNA remodeling activity that is more like the activity of an RNA chaperone since EoV 2C ATPase can destabilize RNA duplexes and accelerate strand annealing in an ATP-independent manner [30] . This finding obtained from an insect picorna-like virus prompted us to determine whether enterovirus 2C ATPase could be an RNA remodeler. Herein, we report that although bacterially expressed EV71 2C ATPase did not exhibit any RNA remodeling activity, eukaryotically expressed EV71 2C ATPase functions not only as an RNA helicase that unwinds RNA helices from 3 0 to 5 0 in an ATP-dependent manner but also as an RNA chaperone that destabilizes helices from either direction and facilitates strand annealing and complex RNA structure formation independently of ATP. Moreover, we determined the domain requirements for these two RNA remodeling activities associated with 2C ATPase and showed that protein 2C ATPase facilitates the EV71 RNA-dependent RNA polymerase (RdRP)-mediated synthesis of vRNA from vRNA template in vitro. When the helicase activity of 2C ATPase was disrupted by point mutation, the RNA replication and virus production of EV71 were mostly abolished in cells. These data indicate that 2C ATPase -mediated RNA remodeling plays a critical role in the enteroviral life cycle, particularly in enteroviral replication. In addition, our data show that the RNA helicase and chaperoning activities are also conserved in CAV16 2C ATPase .

To evaluate the potential helicase or RNA remodeling activity of an enterovirus 2C ATPase , we first compared the sequences and consensus motifs of EV71 2C ATPase and three other viral SF3 helicases: SV40 LTag, HPV18 E1, and AAV2 Rep40. Although EV71 2C ATPase is smaller, this protein contains a core helicase region and the conserved SF3 signature A, B, and C motifs, similar to the three other SF3 helicases ( Fig 1B) .

To further analyze the potential function of 2C ATPase , we modeled its three-dimensional (3D) structure using ROBETTA [31] . The computation-generated structural modeling of 2C ATPase indicated that this protein may be comprised of three structurally independent domains: the N-terminal domain (NTD) contains 113 amino acids (a.a.) and is predicted as a helix bundle formed by three α helices; the middle helicase core (HC) domain includes a.a. 114-250 of 2C ATPase , and is predicted as a central five-stranded β-sheet flanked by α helices on both sides; and the C-terminal domain (CTD) includes a.a. 251-329 and contains several α helices. The three domains are linked by flexible loops (Fig 1C) . The crystallographic structures of AAV2 Rep40 and Rep40-ADP complex have been previously resolved [32, 33] . Our structural alignment of EV71 2C ATPase and AAV2 Rep40 shows that the predicted HC domain of 2C ATPase is structurally similar with the counterpart region of Rep40. Moreover, similarly with Rep40, 2C ATPase is also predicted to contain a P-loop connecting with the central β-sheet, and the predicted ATP binding site of 2C ATPase is also exposed to the exterior and perfectly overlapped with the structurally determined ATP/ADP binding site of Rep40 in the structural alignment of these two proteins ( Fig 1D) . Altogether, our sequence and structural analyses indicate that enterovirus 2C ATPase is similar to other viral SF3 helicases in both conserved motifs and structures, implying that this protein should contain some RNA remodeling activity.

To assess the potential RNA remodeling activity of enterovirus 2C ATPase , we first expressed EV71 2C ATPase as an MBP-fusion protein in both prokaryotic (E. coli) and eukaryotic (baculovirus) systems ( Fig 1E) . Interestingly, the eukaryotically expressed MBP-2C ATPase had an apparently higher molecular mass than the prokaryotically expressed one (Fig 1E, lanes 4 vs.  3 ). The identity and purity of the eukaryotically expressed MBP-2C ATPase were further confirmed via SDS-PAGE separation followed by silver staining (S1 Fig) or in-gel digestion and high-performance Liquid chromatography-tandem mass spectrometry (LC-MS/MS) analysis (S1 Table and S1 Text). In total, four proteins (MBP-2C ATPase , α-tubulin, actin and cytochrome P450) were identified with FDR value of 0.97%. MBP-2C ATPase turned out to be the highest scoring protein (score: 11200) identified with high protein coverage of 81.6%. The mass is similar to other viral SF3 helicases in both motifs and structures. (A) Schematic representation of enterovirus genome and the functional motifs in 2C ATPase , including Zinc binding, oligomerization, membrane binding, and RNA binding motifs. Amino acid positions of each motif are numbered. (B) Domain alignments of EV71 2C ATPase and SF3 viral helicases, including SV40 LTag, HPV18 E1, and AAV2 Rep40. SF3 helicase motifs A, B, and C are highlighted in orange. (C) The structure of EV71 2C ATPase was predicted using the HMMSTR/Rosetta server. The N-terminal domain (NTD), the middle helicase core (HC) domain, and the C-terminal domain (CTD) are linked by flexible loops as indicated. (D) Structural alignment of EV71 2C ATPase (slate) and AAV2 Rep40 (yellow). The ATP/ADP binding site is highlighted in red. (E) MBP-fusion EV71 2C ATPase was expressed using a prokaryotic (E. coli) or eukaryotic (baculovirus) system. The purified recombinant proteins were subjected to 10% SDS-PAGE followed by Coomassie brilliant blue R250 staining. spectrometry results showed that the majority (97.8%) of all the spectra obtained in the purified protein sample were originated from MBP-2C ATPase . The quantitation information by Mascot Exponentially Modified Protein Abundance Index (emPAI) further confirmed the purity of our target protein: the emPAI value of MBP-2C ATPase is 126.76, in comparison to the other three identified proteins including α-tubulin, actin and cytochrome P450 from Spodoptera frugiperda Sf9 cell with very low emPAI values of 0.65, 0.11, 0.07, respectively. Furthermore, to examine the oligomerization state of MBP-2C ATPase , the purified eukaryotically expressed MBP-2C ATPase was subjected to the size exclusion chromatography analysis using a Superdex 200 column. The major peak comprised most protein that was eluted as a molecular mass of~600 kDa (S2A Fig) , and the eluted protein was~85 kDa in size as determined by 10% SDS-PAGE and silver staining (S2B Fig), indicating that the eukaryotically expressed MBP-2C ATPase is oligomerized, consistent with previous studies of poliovirus 2C ATPase [28] .

To evaluate the helix unwinding activity of EV71 2C ATPase , a short hexachloro fluorescein (HEX)-labeled RNA and a long non-labeled RNA were annealed to generate a standard RNA helix substrate with both 5 0 and 3 0 single-stranded protrusions (Fig 1F, upper panel and S2  Table) . The helix unwinding assay was conducted by incubating the RNA helix substrate with purified MBP-2C ATPase , followed by gel electrophoresis. Interestingly, our data showed that, although bacterially expressed MBP-2C ATPase did not unwind the RNA helix in the presence of MgCl 2 and ATP ( Fig 1F, lane 5) , consistent with observations reported previously by another group [27] , eukaryotically expressed MBP-2C ATPase efficiently unwound the RNA helix substrate under the same conditions ( Fig 1F and Fig 2A) . Of note, EoV 2C ATPase and Hepatitis C virus (HCV) NS3 [30, 34] were used as positive controls in this assay (Fig 2A) . Moreover, EV71 2C ATPase could unwind the RNA duplex with 42 matched base pairs but not the duplex with 49 matched base pairs (S3 Fig) , as the latter substrate might be too long to be unwound. Altogether, these results indicate that EV71 2C ATPase can unwind an RNA helix when the protein is eukaryotically expressed.

Because some RNA helicases or chaperones also show unwinding activity with DNA helices or RNA-DNA hybrids, we evaluated this possibility for EV71 2C ATPase . To this end, we constructed three different helix substrates that were DNA helix ( Fig 2B) and RNA-DNA hybrids with longer DNA (Fig 2C) or RNA strand ( Fig 2D) . Each helix substrate was reacted with MBP-2C ATPase under the same conditions as illustrated in Fig 1F. Our data showed that EV71 2C ATPase could unwind all of the tested types of helix substrates (Fig 2) , although it unwound the DNA helix less efficiently than it unwound other helices ( Fig 1F) . Thus, we conclude that EV71 2C ATPase possesses a nucleic acid helix unwinding activity for both RNA and DNA duplexes.

EV71 2C ATPase directs both 5 0 !3 0 and 3 0 !5 0 unwinding of RNA helices For helicases, the directionality of helix unwinding is a fundamental characteristic [35] . To assess the unwinding directionality of EV71 2C ATPase , we constructed three different RNA helix substrates containing a 3 0 single-stranded protrusion, a 5 0 single-stranded protrusion, and blunt ends, respectively (Fig 3A, 3B and 3D ). Each substrate was then incubated with 2C ATPase for the helix unwinding assay. Our results showed that EV71 2C ATPase could unwind either the 3 0 -or 5 0 -protruded RNA helix (Fig 3C) , and its efficiency to unwind the 3 0 -protruded helix was apparently higher than its efficiency to unwind the 5 0 -protruded one (Fig 3C, lanes 3 vs. 6 ). Moreover, 2C ATPase could not unwind the blunt-ended helix ( Fig 3E) . All these experiments were independently repeated several times. Based on these results, we conclude that EV71 2C ATPase possesses a bidirectional unwinding activity to RNA helices, while the 3 0 !5 0 unwinding is more preferred.

The helix unwinding activity of 2C ATPase can be promoted by the presence of ATP For helicases, one important property is that their helix-unwinding activities require the presence of ATP, and ATP promotes helicase activities in a dose-dependent manner [36] . Our data showed that EV71 2C ATPase hydrolyzed ATP or GTP, while UTP or CTP was not efficiently hydrolyzed by this protein. To determine the effect of NTPs on 2C ATPase , we conducted a standard unwinding assay in the presence or absence of individual NTPs. Our results showed that the presence of ATP or GTP dramatically promoted helix unwinding (Fig 4B) . To determine whether the promoting effect of ATP on helix unwinding by 2C ATPase is dose-dependent like other helicases, we assessed the unwinding activity of MBP-2C ATPase in the presence of increasing ATP concentrations from 0.5 to 6 mM. Our data showed that increasing ATP concentrations apparently promoted helix unwinding, and the promoting effect reached a steady stage at 5 mM ATP (Fig 4C and 4D ). These results indicate that the helix unwinding activity of EV71 2C ATPase needs the participation of ATP or other NTPs.

Although we determined that ATP is required by EV71 2C ATPase to reach its optimal unwinding activity, very interestingly, this protein was still able to unwind a portion of RNA helix in the absence of ATP ( Fig 4D) . To confirm this phenomenon and exclude the potential interference of trace amounts of ATP in the reactions, we added AMP-PNP, a non-hydrolyzable ATP analog that blocks ATPase activity, to the ATP-free unwinding reaction. Our data showed that although the presence of 5 mM AMP-PNP was able to abolish the unwinding activity of HCV NS3, a classic RNA helicase (S4B Fig) , the presence of 2 or 5 mM AMP-PNP was unable to completely block 2C ATPase to unwind a portion of the RNA helix ( Fig 4E, lanes 4 and 6) .

To further exploit this issue, we sought to determine the necessity of Mg 2+ on the ATPase and helix unwinding activities of EV71 2C ATPase , as these two closely coupled activities of a helicase is normally Mg 2+ -dependent [37] . Our results showed that the ATPase activity of EV71 2C ATPase was strictly Mg 2+ -dependent, as this protein was almost unable to hydrolyze ATP in the absence of Mg 2+ (Fig 4F) . On the other hand, although 2C ATPase requires the presence of Mg 2+ to reach its optimal unwinding activity, it was still able to unwind a portion of the RNA helix in the absence of Mg 2+ or any divalent ions ( Fig 4G, lane 3; S4D Fig, lane 3) , further confirming that 2C ATPase retains partial helix unwinding activity in the absence of its ATPase activity. Moreover, when the Mg 2+ concentration was lower than 2 or 2.5 mM, increasing Mg 2+ concentrations gradually promoted both the ATPase and helix unwinding activities of EV71 (Fig 4F and 4G ), whereas at higher Mg 2+ concentrations (>2.5 mM), Mg 2+ inhibited both activities in a dose-dependent manner (Fig 4F and 4H ). Of note, both no protein supplementation and boiled MBP-2C ATPase were used as negative controls (S4C Fig, lanes 1 and 5) . In addition, the biochemical properties of EV71 2C ATPase , including the requirement of divalent ions (Mn 2+ , Ca 2+ , and Zn 2+ ) and pH, were also determined (S4D- S4F Fig) . Our data showed that while 2.5 mM Ca 2+ is dispensable for the helix unwinding activity of EV71 2C ATPase , 2.5 mM Mn 2+ or Zn 2+ blocked the helix unwinding by 2C ATPase (S4D Fig). When the concentration of Zn 2+ is higher than 0.5 mM, the presence of Zn 2+ completely blocked the helix unwinding activity of 2C ATPase (S4E Fig) . Moreover, EV71 2C ATPase prefers a neutral pH as an optimal reaction condition, as this protein exhibited the highest helix unwinding activity with pH 7.5 (S4F Fig) .

Previous studies reported that the ATPase activity of poliovirus 2C ATPase can be inhibited by guanidine hydrochloride (GnHCl) [26] , which is a potent inhibitor of enterovirus VPg-uridylation and vRNA replication [38, 39] . Our data showed that GnHCl can also inhibit the ATPase and RNA helix unwinding activities of EV71 2C ATPase in a dose-dependent manner (Fig 4I and 4J ). Interestingly, this protein could still unwind a portion of the RNA helix even at high concentrations of GnHCl, consistent with the results of AMP-PNP treatment ( Fig 4E) .

Altogether, our results show that EV71 2C ATPase contains an ATP-dependent helicase-like activity that requires the presence of Mg 2+ , together with an ATP/Mg 2+ -independent non-helicase activity that can also unwind the RNA helix. EV71 2C ATPase contains both RNA helicase and chaperoning activities RNA remodeling proteins include two distinct classes: RNA helicases and RNA chaperones. Their fundamental characteristics and differences are that the helix unwinding of RNA helicases is ATP dependent and normally has directionality, whereas that of RNA chaperones does not require ATP and is bidirectional [40] . Our previous results showed that in addition to its ATP-dependent helicase-like activity, EV71 2C ATPase also contains an ATP-independent helix unwinding activity (Fig 4) ; moreover, this protein can unwind RNA helices bidirectionally ( Fig 3C) . These findings suggested that EV71 2C ATPase contains both RNA helicase and chaperone activities.

To distinguish these two activities, we designed a set of experiments based on their fundamental difference in helix unwinding directionality and ATP dependency. First, we constructed two RNA helix substrates, each of which contained the same 42-bp double-stranded region as well as a 6-nt 3 0 or 5 0 single-stranded protrusion ( Fig 5A) . Then, each helix substrate was reacted with MBP-2C ATPase in the absence or presence of ATP. Our results showed that although the 2C ATPase unwound the 3 0 -protruded helix in an ATP-dependent manner (Fig 5B  and 5E ), it unwound the 5 0 -protruded helix exactly like an RNA chaperone, which was able to unwind the helix in the absence of ATP, and increasing ATP concentrations could not further enhance the helix unwinding (Fig 5C and 5E ). Moreover, since the motif A "GKS" is recognized as the NTP binding site and the core ATPase site of SF3 helicases, we generated the ATPase-defective GK134AA mutant of 2C ATPase . Our data showed that the GK134AA 2C ATPase mutant was able to unwind the 5 0 -protruded helix substrate in the absence or presence of ATP at an efficiency similar to that of wild-type 2C ATPase , further confirming that the unwinding of the 5 0 -protruded helix by 2C ATPase is independent of its ATPase activity (Fig 5D  and 5E ). Furthermore, the unwinding activity of 2C ATPase on the 5 0 -protruded helix could not be promoted by any individual NTP (S5 Fig). Altogether, our data indicate that the 5 0 -protruded helix could be unwound via the RNA chaperone activity but not the helicase activity of 2C ATPase , whereas the 3 0 -protruded helix substrate could be unwound via both activities. These findings are consistent with our previous observation that 2C ATPase unwinds the 3 0 -protruded RNA helix more efficiently than the 5 0 -protruded one in the presence of ATP (Fig 3C) . We conclude that EV71 2C ATPase possesses an ATP-dependent RNA helicase activity that unwinds RNA helices with 3 0 !5 0 directionality, which is consistent with all known SF3 helicases [41] , together with an ATP-independent RNA chaperone activity that unwinds RNA helices from either direction. EV71 2C ATPase destabilizes structured RNA strands and stimulates annealing RNA chaperones are generally thought to destabilize misfolded RNAs and assist in the formation of more globally stable RNA structures. After determining that EV71 2C ATPase possesses an RNA chaperone activity, we adapted a canonical assay [42] to further verify and characterize EV71 2C ATPase . Two 42-nt complementary RNA strands, each of which formed defined stem-loop structures, were designed and constructed (Fig 6A) . Of the two, one strand was 5 0 HEX-labeled, and the other was not labeled as indicated. Equal amounts of HEX-labeled and non-labeled strands were incubated in the presence or absence of MBP-2C ATPase , and then gel shift assays were conducted to examine the hybridization of the two strands. Of note, all the experiments were ATP-free. Our results showed that although minimal spontaneous hybridization could be observed in the absence of 2C ATPase (Fig 6B, lanes 3-4; Fig 6C, lane 3; and Fig 6D, lanes 3-6) , the presence of EV71 2C ATPase dramatically enhanced the two strands' hybridization, as did EoV 2C, which is a well-defined RNA chaperone (Fig 6B, lanes 5-6) . Moreover, increasing either the amount of 2C ATPase or its incubation time resulted in an apparent increase in strand annealing (Fig 6C and 6D) . Overall, our data show that 2C ATPase can destabilize structured RNA strands and accelerate the formation of more stable hybrids, fitting the characteristic of RNA chaperones.

The hammerhead ribozyme is a self-catalytic RNA module that mediates reversible transcleavage at a specific site within an RNA substrate [43] . Since the functionality of a hammerhead ribozyme strictly relies on its correct tertiary structure, hammerhead ribozymes often serve as the models for studying the structure and properties of RNAs. RNA chaperones are probably able to enhance the activity and turnover of ribozymes by promoting ribozyme formation, ribozyme-substrate association, and/or ribozyme dissociation from cleaved substrates. Therefore, a canonical hammerhead ribozyme enhancement assay [44] was used to further verify and characterize the RNA chaperone activity of EV71 2C ATPase . In this assay, unlabeled ribozyme RNA was reacted with a 5 0 HEX-labeled RNA substrate, and the cleavage was expected to take place 16 nts from the 5 0 end (indicated by arrow), resulting in a HEX-labeled 16-nt cleavage product that could be detected by electrophoresis (Fig 7A) . Our data showed that the presence of 2C ATPase effectively enhanced ribozyme activity in a dose-dependent manner (Fig 7B) , indicating that the RNA chaperone activity of EV71 2C ATPase can assist in the proper formation and function of relatively complex RNA structures.

The CTD of 2C ATPase is required for its RNA chaperoning activity

The structure of enterovirus 2C ATPase was previously modeled to contain three domains: the N-terminal domain (NTD), helicase core, and CTD (Fig 1C) . To assess the role of specific domains on the different activities of 2C ATPase , a series of truncations of EV71 2C ATPase were generated and eukaryotically expressed. Moreover, since the motif A "GKS" and motif C "STN" are conserved in SF3 helicases, the GK134AA and ΔSTN mutants of 2C ATPase were also generated. The predicted structures of these 2C ATPase fragments and mutagenesis sites are illustrated in S6A-S6C Fig  Our data showed that the GK134AA mutant of 2C ATPase lost most ATPase activity (Fig 8B) but retained the RNA chaperone activity that is insensitive to ATP, as determined in these and previous experiments (Figs 5D, 8C and 8D); the motif C deletion (ΔSTN) of 2C ATPase resulted in the loss of most helix unwinding activity (S6D Fig). Moreover, although 2C ATPase CTD had no detectable helix unwinding activity and little ATPase activity (Fig 8A, lane 5; and Fig 8B) , the loss of CTD resulted in the complete loss of helix unwinding in the absence of ATP ( Fig  8C, lane 4) , showing that the CTD is required for the RNA chaperone activity of 2C ATPase . Interestingly, in the presence of ATP, the helix unwinding activity of 2C ATPase ΔCTD was partially restored (Fig 8D, lane 4) , indicating that the CTD plays an important but nonessential role in the helicase activity of 2C ATPase , probably by maintaining the proper structure of the 2C ATPase helicase core domain.

After determining the RNA remodeling activity of 2C ATPase , we sought to evaluate its potential role in enteroviral RNA replication. It has been proposed that during vRNA replication of (+) RNA viruses, replicative intermediate double-stranded RNA must be unwound [45] . To assess the potential role of 2C ATPase in enteroviral RNA replication, we first incubated purified His 6tagged 3D pol , the EV71 RdRP, with the (-)RNA template [i.e., we transcribed in vitro the 3 0 -end 1-357 nts of EV71 (-)RNA], and with an excessive amount (at a ratio of 5:1) of primer RNA, which was a long oligonucleotide and was pre-annealed to the template in the presence or absence of 2C ATPase (Fig 9A) . Of note, the RdRP reactions were conducted at 22°C as previously described [46] , and at this temperature, EV71 2C ATPase was still able to hydrolyze ATP and unwind the RNA helix, although both activities were moderately lower at 22°C than at 37°C (S4A and S4C Fig). Our data showed that the presence of 2C ATPase significantly promoted the synthesis of (+)RNA strands from the (-)RNA template by 3D pol , and the promoting effect of 2C ATPase was dose dependent (Fig 9B and 9C; Fig 9D, lower panel; and Fig 9E) . Interestingly, when the amount of primer RNA was less than that of the (-)RNA template (at a ratio of 1:5), the presence of increasing amounts of 2C ATPase was unable to promote (+)RNA synthesis ( Fig  9D, upper panel; and Fig 9E) , indicating that the major role of the 2C ATPase helicase activity is not to directly enhance the RdRP activity of 3D pol or smoothen the template. Of note, when the primer was absent, 3D pol was unable to mediate RdRP or elongation reaction in the presence or absence of 2C ATPase (Fig 9F, lanes 2 and 3) . In addition, the GK134AA mutant of 2C ATPase failed to promote (+)RNA synthesis as expected (Fig 9F, lanes 6-8; and Fig 9G) . Altogether, our results show that 2C ATPase can facilitate the 3D pol -mediated production of enteroviral RNA strands in vitro via promoting the efficiency to re-utilize the RNA template.

The RNA helicase activity of 2C ATPase is critical for the RNA replication and viability of EV71

It has been previously reported that the GK-to-AA mutation in the motif A of poliovirus 2C AT-Pase resulted in the inhibition of virus growth [47] . To determine whether the loss of the helicase activity of 2C ATPase has any consequence on the viral life cycle of EV71, we introduced the were measured via Bio-Rad Quantity One software, and the relative RNA production was determined by comparing the GK134AA mutation, which disrupts the ATPase and helicase activities, in the 2C ATPase coding region of the infectious clone of EV71. Then, Wt and mutant EV71 RNA transcripts were transfected into human rhabdomyosarcoma (RD) cells. RNA replication was measured via quantitative reverse transcription polymerase chain reaction (qRT-PCR) 24 and 48 hours posttransfection, and virus production was detected via immunofluorescent staining of EV71 VP1 in cells. Strikingly, compared to Wt virus, the GK134AA mutation resulted in the loss of EV71 RNA replication ( Fig 10A) and viability (Fig 10B) , suggesting that the GK motif and the RNA helicase activity of 2C ATPase are critical for enteroviral RNA replication and viability.

After determining that EV71 2C ATPase possesses both RNA helicase and chaperone activities, we sought to determine whether 2C ATPase encoded by another enterovirus exhibits similar activities. To this end, 2C ATPase of CAV16 was eukaryotically expressed and then subjected to the helix unwinding assays using either a 3 0 -or 5 0 -protruded helix substrate. Exactly like EV71 2C ATPase (Fig 5) , CAV16 2C ATPase unwound the 3 0 -protruded helix in an ATP-dependent manner (Fig 11A and 11B) , whereas the unwinding of the 5 0 -protruded helix by this protein was ATP independent (Fig 11C and 11D) . These data show that the ATP-dependent RNA helicase and ATP-independent RNA chaperone activities of 2C ATPase are also conserved in CAV16, another enterovirus.

As the most conserved nonstructural protein among all enteroviruses and even picornaviruses, 2C ATPase has been reported to participate in diverse processes critical for the enteroviral life cycle. Although this protein has long been predicted as a putative SF3 helicase on the basis of its AAA+ ATPase activity and conserved SF3 motifs, its potential role in viral RNA remodeling and replication remains elusive. Previous studies have shown that the ATPase activity of poliovirus 2C ATPase could be inhibited by GnHCl. This compound is a potent inhibitor of enteroviral RNA replication in vivo, which has been reported to inhibit poliovirus (-)-vRNA synthesis and the uridylylation of the protein primer VPg [38, 39] , suggesting that the ATPase activity of 2C ATPase is critical for enteroviral RNA replication. Here we report that protein 2C ATPase of EV71 possesses a nonconventional RNA remodeling activity that can function as both an ATP-dependent RNA helicase and an ATP-independent RNA chaperone and facilitates EV71 RdRP-mediated vRNA synthesis from vRNA template in vitro. The mutation of GK134 to AA, which disrupts 2C ATPase helicase activity, mostly abolished EV71 RNA replication and virus production. These data indicate that 2C ATPase -mediated RNA remodeling is pivotal for the enteroviral life cycle. Moreover, our results show that the RNA remodeling activities of 2C ATPase are also conserved in CAV16. Although 2C ATPase contains conserved motifs typical of SF3 helicases, previous attempts to identify its helicase activity were unsuccessful [27] , leading us to ask why the RNA helicase/ chaperoning activity of 2C ATPase can be detected in this study. It is noteworthy that the recombinant poliovirus 2C ATPase protein used in the previous assay was produced in E. coil, while the EV71 and CAV16 2C ATPase proteins used here were expressed using an eukaryotic system (baculovirus). Interestingly, we found that although both the prokaryotically and eukaryotically expressed 2C ATPase proteins possessed similar ATPase activity (S7 Fig), only the eukaryotically expressed 2C ATPase protein possessed the RNA duplex unwinding activity (Fig 1F) . Moreover, the eukaryotically expressed 2C ATPase showed an apparently higher molecular mass than the prokaryotically expressed one (Fig 1E) , implying that the former protein contains some posttranslational modifications that potentially play a critical role(s) in the helicase activity of 2C ATPase . Future research would uncover the potential post-translational modifications of 2C ATPase .

Although they have mainly been characterized in vitro, the RNA remodeling activities of virus-encoded proteins are generally believed to play critical roles in the viral life cycle [48] . The RNA genomes contain multiple cis-acting elements, including the 5 0 cloverleaf, 3 0 UTRpoly(A), internal origin of replication (oriI or cre) [49, 50] , internal ribosomal entry site [51, 52] , and the cloverleaf at the 3 0 -end of (-)-vRNA [53] [54] [55] . These highly structured RNA elements play indispensable roles in the replication, translation, and encapsidation of enteroviral RNAs [23, 24, 54, 56] and probably require the RNA chaperoning activity of 2C ATPase to facilitate their proper folding and refolding. On the other hand, during the RNA replication of RNA viruses, replicative intermediate dsRNA must be unwound, thereby allowing the efficient recycling of vRNA template for progeny vRNA synthesis. It is very likely that the RNA helicase activity of 2C ATPase plays such a dsRNA unwinding role during enteroviral RNA replication, which is consistent with our observations that 2C ATPase can facilitate RdRP-mediated enteroviral RNA synthesis in vitro by promoting the recycling of vRNA template (Fig 9) , and disrupting 2C ATPase RNA helicase activity in EV71 resulted in an almost complete loss of enteroviral RNA replication and virus production in cells (Fig 10) . Interestingly, although RNA chaperones can also unwind/destabilize RNA duplexes, RNA chaperones are normally not considered to be involved in unwinding viral replicative dsRNA, as they usually destabilize short base pairs or hairpins within structured RNA elements. Indeed, Banerjee et al. reported that poliovirus 2C ATPase can bind the 3 0 -end cloverleaf structure of (-)-vRNA [15] , implying a role of 2C ATPase in this structured element. In addition, our finding that disrupting 2C ATPase helicase activity but not chaperone activity mostly abolished enteroviral RNA replication and viability strongly suggests that the functions associated with RNA helicase and chaperone play different roles in the same RNA molecule (vRNA) and cannot replace each other.

We previously reported that 2C ATPase from EoV, an insect picorna-like virus belonging to the family Iflaviridae, possesses an ATP-independent RNA chaperone activity but not helicase activity [30] . Interestingly, although EoV 2C ATPase is predicted to contain conserved SF3 motifs A, B, and C, the GK-to-AA mutation in EoV 2C ATPase motif A did not abolish but instead increased its ATPase activity [30] . This observation obviously contradicts the indispensable role of the motif A "GKS" in the ATPase and helicase activities of defined SF3 helicases, including EV71 2C ATPase (Fig 8) , confirming that EoV 2C ATPase is not a SF3 helicase. And the functional disparity between these two proteins is probably due to the long-time evolution and adaptation of iflavirus and enterovirus in different types of hosts, insects, and mammals.

Interestingly, enterovirus 2C ATPase is not the only RNA remodeling protein encoded by enteroviruses. Previous studies by DeStefano and colleagues showed that poliovirus 3AB is an RNA chaperone [42, 57] ; moreover, our previous report confirmed that EV71 3AB also contains in vitro RNA chaperone activity [58] . In addition, poliovirus 3D pol has been reported to display unwindase activity that does not require ATP hydrolysis but does require an RNA chain elongation reaction [59] . It is plausible that 2C ATPase and 3D pol work synergistically to unwind nascently synthesized vRNA strands from template. On the other hand, the chaperone activities of 2C ATPase and 3AB may function collaboratively or separately on different structured cis-acting elements of enteroviral RNA. However, owing to technical limitations, it is almost infeasible to determine the exact role of RNA helicase or chaperoning activity in the structures and functionalities of RNA molecules in cells or in vivo. Future studies may overcome these technical barriers and provide a mechanistic view of how RNA remodeling proteins function in cells.

RNA helicases and ATP-independent RNA chaperones are recognized as the two distinct classes of RNA remodelers. RNA helicases participate in most ATP-dependent rearrangement of structured RNAs and RNA-protein complexes [60, 61] . On the other hand, RNA chaperones are able to unwind RNA duplexes and facilitate RNA strand annealing, thereby aiding the folding or refolding of RNA molecules into correct structures. The major difference between RNA helicase and chaperone is that the former needs the participation of ATP, but the later does not. Different from previously characterized RNA remodeling proteins, enteroviral 2C ATPase can function as both a typical RNA helicase and an ATP-independent RNA chaperone. That a single protein can contain these two different types of RNA remodeling activities is intriguing. Our structural analyses of protein 2C ATPase may provide some hints. Protein 2C ATPase contains a 137-a.a. middle domain that includes the conserved SF3 signature A, B, and C motifs and is structurally similar to the helicase core domains of other SF3 viral helicases, indicating that the middle domain provides the basis of its RNA helicase activity. On the other hand, although RNA chaperones have been studied for decades, the mechanism(s) governing their ATPindependent remodeling activity remains elusive. A popular model proposed to explain the mechanism is the "entropy or disorder transfer", in which certain intrinsic disordered or unstructured regions of RNA chaperones can transfer their disorder or entropy to RNA molecules, and such a transfer of disorder or entropy can destabilize misfolded RNAs and aids RNA refolding. Indeed, many RNA chaperones, such as HIV-1 Vif, Tat and nucleocapsid, flavivirus core protein, hantavirus N protein, and cypovirus VP5, have been predicted to contain multiple intrinsic disordered regions [40, 48] , providing support for this model. Structure modeling using ROBETTA indicated that the CTD of 2C ATPase contains a highly unstructured or disordered coiled-coil region that links the helicase core domain and the CTD (Fig 1C) . When the CTD was deleted from the protein, the truncation completely abolished the RNA chaperoning activity of 2C ATPase (Fig 8C) . The truncation of CTD reduced but did not abolish the RNA helicase activity (Fig 8D) , suggesting that the presence of CTD is also important for the helicase activity, probably by affecting the protein's global conformation. Moreover, the CTD alone does not contain any RNA remodeling activity (Fig 8A) , suggesting that the RNA chaperoning function of 2C ATPase requires the RNA binding capacities of other 2C ATPase domains. The coiled-coil regions and the middle core domains are highly conserved in enteroviruses and other picornaviruses, such as encephalomyocarditis virus (EMCV) and foot-mouth-disease virus (FMDV) (S8 Fig). On the basis of all these findings, we propose that the RNA helicase function of enteroviral 2C ATPase relies on the conserved helicase motifs and ATPase activity, while specific structural characteristics, like the architecture of RNA binding and intrinsic disorder regions, are the basis of its RNA chaperoning function. Moreover, these findings provide evidence of the correlation between intrinsic disorder and RNA chaperone activity, which supports the "entropy transfer" model of RNA chaperones.

In conclusion, this study determined the RNA helicase and chaperoning activities associated with enterovirus 2C ATPase and provides both in vitro and cellular evidence of their potential functions in enteroviral RNA replication. It also provides the first evidence that the two distinct types of RNA remodeling activities, RNA helicase and ATP-independent RNA chaperoning activities, can be integrated within one protein, introducing an extended view of RNA remodeling proteins. Altogether, these findings increase our understanding of enteroviruses and the two types of RNA remodeling activities.

The generation of pFastBac HTB-MBP and pFastBac HTB-MBP-NS3 HCV have been described previously [30] . The cDNAs for EV71 2C ATPase (GenBank Accession No. KC954662), CAV16 2C ATPase (GenBank Accession No. KC117318) and EV71 2C ATPase fragments were amplified by polymerase chain reaction (PCR) from the plasmid containing full-length EV71 cDNA, and cloned into the vector pFastBac HTB-MBP. Site-directed mutations were generated as previously described [30] . The primers used in this study are listed in Table. The resulting plasmids were subjected to Bac-to-Bac baculovirus system to express the recombinant proteins with an MBP fused at the N-terminal.

The expression and purification of MBP alone and MBP-fusion proteins were performed as previously described [30, 40] . Briefly, Sf9 cells were infected with the recombinant baculoviruses and harvested at 72 h postinfection. Cell pellets were resuspended, lysed by sonication and subject to centrifugation for 30 min at 11 000 g to remove debris. The protein in the supernatant was purified using amylase affinity chromatography (New England BioLabs, Ipswich, MA) according to the manufacturer's protocol, and then concentrated using Amicon Ultra-15 filters (Millipore, Schwalbach, Germany). All proteins were quantified by the Bradford method and stored at -80°C in aliquots. Proteins were separated on 10% SDS-PAGE and visualized by Coomassie blue.

The 3D structure of EV71 2C ATPase was modeled by submitting its amino acid sequence to the HMMSTR/Rosetta server [from Robetta, University of Washington (http://robetta.bakerlab. org/)] [31] . Five models were obtained, and the best one was chosen as a template based on its score, assessed by submitting it to the SWISS-MODEL Server [from Swiss Institute of Bioinformatics and the Biozentrum, University of Basel, Switzerland (http://swissmodel.expasy.org)]. The figure of the modeled EV71 2C ATPase 3D structure and the structural alignment with AAV2 Rep40 (PDB ID code 1U0J) were drawn by PyMOL program 1.1 (DeLano Scientific LLC, South San Francisco, CA) from coordinate file.

In brief, of the two strands, one was labeled at the 5 0 end with hexachloro-fluorescein (HEX), and the other strand was unlabeled. HEX-labeled oligonucleotide strands were purchased from TaKaRa (Dalian, China). Unlabeled DNA strands were synthesized by Invitrogen, and unlabeled RNA strands were in vitro transcribed using T7 RNA polymerase (Promega, Madison, WI). The in vitro transcribed RNA strands were purified by Poly-Gel RNA Extraction Kit (Omega bio-tek, Guangzhou, China) according to the manufacturer's instruction. The two strands were mixed in a proper ratio, and annealed through heating and gradually cooling as previously described [30, 40] . The standard RNA helix substrate with both 5 0 and 3 0 protrusions was annealed with RNA1 and RNA2, the R Ã /D substrate was annealed with RNA1 and DNA1, the D Ã /D substrate was annealed with DNA2 and DNA3, the D Ã /R substrate was annealed with DNA2 and RNA3, the 3 0 -protruded RNA helix was annealed with RNA1 and RNA4, the 5 0 -protruded RNA helix was annealed with RNA1 and RNA5, the blunt-ended substrate was annealed with RNA1 and RNA6, and the 49 matched bps substrate was annealed with RNA7 and RNA8. All oligonucleotides used in this study are listed in S2 Table. Nucleic acid helix unwinding and strand hybridization assays

The standard helix destabilizing assay was performed as previously described [40] with minor modifications. Briefly, 20 pmol of recombinant protein and 0.1 pmol of HEX-labeled helix substrate were added to a mixture containing 50 mM HEPES-KOH (pH 7.5), 2.5 mM MgCl 2 , and 2 mM Dithiothreitol (DTT), 0.01% bovine serum albumin (BSA), and 15 U RNasin (Promega). After incubation at 37°C for 60 min or indicated time, the reaction was terminated by adding proteinase K (final concentration of 1 μg/μl) and 5×loading buffer [100 mM Tris-HCl, 1% SDS, 50% glycerol, and bromophenol blue (pH 7.5)]. The mixtures were then electrophoresed on 15% native-PAGE gels, followed by scanning with a Typhoon 9200 imager (GE Healthcare, Piscataway, NJ). The RNA strand hybridization assay was performed as previously described [40] . The sequences of the stem-loop-structured RNA strands were indicated in Fig 7A. The samples were also resolved on 15% native-PAGE gels, followed by gel scanning a Typhoon 9200 imager (GE Healthcare).

NTPase activities were determined via measuring the released inorganic phosphate during NTP hydrolysis using a direct colorimetric assay as previously described [30] . All of the results given with this quantitative assay were averages of three repeated experiments.

The ribozyme RNA was synthesized from the in vitro transcription using T7 RNA polymerase, and the 5 0 -HEX-labeled substrate RNA was synthesized by TaKaRa. Indicated amount of protein was added in 10 μl reaction volumes containing 0.15 nM substrate, 0.3 nM ribozyme, 50 mM HEPES-KOH (pH 7.5), 2.5 mM MgCl 2 , and 2 mM DTT, 0.01% BSA, 20 U RNasin. The mixtures were incubated at 37°C for 30 min, and then treated by proteinase K (final concentration of 1 μg/μl) at 37°C for 15 min. The digestion reactions were precipitated with 20 μl isopropanol and 2 μg glycogen (-80°C, 30 min), and subjected to by centrifugation at 12 000 g for 15 min. The precipitates were dissolved in formamide and electrophoresed on 15% acrylamide-7 M urea gels, followed by scanning with a Typhoon 9200 imager (GE Healthcare).

The RNA primer and template were in vitro transcribed by T7 RNA polymerase as described above. The primer RNA strand contains the 1-140 nts of the 5 0 end of EV71 (+)RNA, and the (-)-vRNA template contains the sequence complementary with the 1-357 nts of 5 0 end of EV71 (+)RNA. The transcribed products were purified and quantified as described above. Then, the primer RNA was pre-annealed to the template. The EV71 3D pol gene was cloned into the vector pET26b-Ub plasmid, and the protein was purified as the C-terminal His×6 tag fusion protein via a nickel-charged HisTrap HP column (GE Healthcare) as previously described [62] . The RdRP reactions were carried out in a total volume of 10 μl at 22°C as previously described [46] . As previously described [63] , the RdRP reactions were carried out in the reaction mixture containing 500 nM 3D pol in 50 mM HEPES-KOH (pH 7.0), 12.5 mM KCl, 5 mM MgCl 2 , 5 mM DTT, 20 U RNasin (Promega), and 0.25 mM Digoxin (DIG) RNA Labeling Mix (Roche) with total volume of 10 μl at 22°C. The reaction mixtures were supplemented with 10 μl 2×loading buffer (20% 10×MOPS running buffer, 10% glycerol, 50% formamide, 20% formaldehyde and 0.05% bromophenol blue), and then denatured at 65°C for 10 min. The samples were electrophoresed on 1.5% agarose-formaldehyde denaturing gels, and transferred onto N + nylon membranes (Roche). The membranes were incubated with anti-DIG-alkaline phosphatase antibody (Roche), followed by incubation with CDP-Star (Roche) at 37°C for 10 min. The signals were detected by radiography on X-ray film (FujiFilm, Tokyo, Japan). All oligonucleotides used for in vitro transcription are listed in S3 Table. Cells Human rhabdomyosarcoma (RD) cells were obtained from the American Type Culture Collection (ATCC), and cultured in Dulbecco's modified Eagle's medium (DMEM, Gibco) containing 10% fetal bovine serum (FBS, Gibco), 100 units of penicillin and 100 mg/ml of streptomycin. The transfected or infected RD cells were maintained in DMEM containing 2% FBS.

The wild type and mutant plasmids containing full-length EV71 cDNA were linearized with Mlu I digestion. 2 μg of each purified linear plasmid was used as the template to in vitro transcribe EV71 RNA using the SP6 RiboMAX Large Scale Production System (Promega) according to the manufacturer's protocols. The RNA transcript was transfected into 80%-90% confluent RD cells using Lipofectamine 2000 (Invitrogen). 24-48 h post-transfection, the total RNA from transfected RD cells was extracted using RNeasy Mini Kit (QIAGEN, GmBH, Germany), and stored at -80°C.

The amount of viral RNA was quantified by using One Step PrimeScript RT-PCR Kit (Takara, Dalian) according to the manufacturer's protocol as previous described [64] with EV71 specific premiers (Fwd, 5 0 -GGCCATTTATGTGGGTAACTTTAGA-3 0 ; Rev, 5 0 -CGGGCAATCGTGT CACAAC-3 0 ) and probe (5 0 FAM-AAGACAGCTCTCGCGACTTGCTCGTG-BQH1 3 0 ).

RD cells at 90% confluence on glass slides were transfected with indicated EV71 transcript. The cells were fixed at 24 h post-transfection with pre-cooled acetone at -20°C for 30min, followed by washing in PBS for 3 times and incubation with mouse anti-EV71 VP1 monoclonal antibody (Chemicon International, Madison, WI) for 60 min at 37°C. The cells were then washed in PBS and incubated with Alexa Fluor 488-labeled goat anti-mouse IgG (Invitrogen) for another 45 min. Cells were incubated with DAPI at room temperature for 5 min to stain the nuclei. Finally, the cells were rinsed again with PBS and visualized under a fluorescent microscope (Olympus, Tokyo, Japan). 

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EV71 2C Works as Both RNA Helicase and Chaperone PLOS Pathogens

We thank Drs. Peng Gong and Congyi Zheng (Wuhan, China) for providing reagents, and Dr. Hanzhong Wang (Wuhan, China) for helpful discussions. We thank Ms. Markeda Wade (Houston, Texas) for professionally editing the manuscript.

Conceived and designed the experiments: HX XZho. Performed the experiments: HX PW GCW JY XS WW YQ TS. Analyzed the data: HX CFQ XZha LY YH XZho. Contributed reagents/materials/analysis tools: CFQ. Wrote the paper: HX XZho.