2′-C-methylated nucleotides terminate virus RNA synthesis by preventing active site closure of the viral RNA-dependent RNA polymerase

The 2′-C-methyl ribonucleosides are nucleoside analogs representing an important class of antiviral agents, especially against positive-strand RNA viruses. Their value is highlighted by the highly successful anti-hepatitis C drug sofosbuvir. When appropriately phosphorylated, these nucleotides are successfully incorporated into RNA by the virally encoded RNA-dependent RNA polymerase (RdRp). This activity prevents further RNA extension, but the mechanism is poorly characterized. Previously, we had identified NMR signatures characteristic of formation of RdRp–RNA binary and RdRp–RNA–NTP ternary complexes for the poliovirus RdRp, including an open-to-closed conformational change necessary to prepare the active site for catalysis of phosphoryl transfer. Here we used these observations as a framework for interpreting the effects of 2′-C-methyl adenosine analogs on RNA chain extension in solution-state NMR spectroscopy experiments, enabling us to gain additional mechanistic insights into 2′-C-methyl ribonucleoside-mediated RNA chain termination. Contrary to what has been proposed previously, poliovirus RdRp that was bound to RNA with an incorporated 2′-C-methyl nucleotide could still bind to the next incoming NTP. Our results also indicated that incorporation of the 2′-C-methyl nucleotide does not disrupt RdRp–RNA interactions and does not prevent translocation. Instead, incorporation of the 2′-C-methyl nucleotide blocked closure of the RdRp active site upon binding of the next correct incoming NTP, which prevented further nucleotide addition. We propose that other nucleotide analogs that act as nonobligate chain terminators may operate through a similar mechanism.

RNA viruses represent some of the greatest threats to global health systems, including positive-strand RNA viruses like those belonging to the Flaviviridae (1) and Picornaviridae (2,3) families. Although vaccines have been or are currently being developed against many of these viruses (4,5), there has also been a recognized need for small-molecule therapeutic agents to complement or even overtake these approaches (6,7). One important drug tar-get is the viral RNA-dependent RNA polymerase (RdRp) 2 (8,9), responsible for virus RNA replication. Replication inhibitors that target the conserved core of the RdRp may have broad antiviral activity. For example, 2Ј-C-methyl nucleotide analogs have wide antiviral activity against many flaviviruses, picornaviruses, and other positive-strand RNA viruses (10 -12), although they may have limited utility against negative-strand RNA or DNA viruses (13). This class includes the highly successful anti-hepatitis C drug sofosbuvir (14). The RdRp incorporates the triphosphorylated 2Ј-C-methyl nucleotide analogs into RNA, but further RNA extension is prevented, despite these molecules containing a 3Ј-hydroxyl necessary for further nucleotide incorporation (10,15,16); such molecules are known as nonobligate chain terminators. The antiviral activity of these compounds is likely due to RNA chain termination (10,13,16), but the molecular mechanisms behind RNA chain termination are poorly understood. A better appreciation of these molecular mechanisms may provide insights into further development of this important class of antiviral agents.
The RdRp three-dimensional structure has been described as a cupped right hand with fingers, thumb, and palm subdomains, similar to the overall architecture of other single-subunit nucleic acid polymerases (17). Viral RdRps are unique compared with other nucleic acid polymerases in that there are extensive interactions between the fingers and thumb subdomains, providing completely encircled active sites (18) (Fig.  1). The enclosure of the RdRp active site means that mechanisms of nucleotide selection, addition, and translocation may differ from other nucleic acid polymerases. There are available X-ray crystal structures for a number of RdRps, including those for flaviviruses and picornaviruses (18). Unfortunately, the only X-ray crystal structures with RdRp (in this case, from hepatitis C virus (HCV)) in complex with 2Ј-C-methyl nucleotides represent a step before nucleotide incorporation, with the triphosphorylated 2Ј-C-methyl nucleotide acting as the next incoming NTP (19). Although these structures have revealed molecular determinants important for nucleotide analog recognition, they provide little insight into the mechanism of RNA termination.
A series of X-ray crystal structures of poliovirus (PV) and related RdRps provides insights into the steps of nucleotide incorporation and subsequent translocation (20 -22), including insights into the functional roles of the seven conserved structural motifs in RdRps (i.e. motifs A-G). After base-pairing with the template nucleotide, the 2Ј-and 3Ј-hydroxyls of the incoming NTP make key hydrogen bonding interactions with Ser-288 and Asn-297 in motif B (PV numbering), triggering structural rearrangements to "close" the active site and prepare for the phosphoryl transfer reaction (21,22). Critically, structural motif A is realigned to form a complete three-stranded ␤-sheet with motif C, which causes motif A residue Asp-233 to swing toward the RNA, allowing it to coordinate the magnesium ions necessary for catalysis (21) (Fig. 1). The triphosphate of the incoming NTP is also realigned to promote inline nucleophilic attack from the primer 3Ј-hydroxyl, aided in part by conserved residues in motifs D and F (21)(22)(23). The phosphoryl transfer reaction then takes place, according to the two metal ion mechanism shared by other nucleic acid polymerases (24), with Asp-233 and motif C residue Asp-328 coordinating the metals (21). We have also proposed that there is a repositioning of motif D residue Lys-359 so that it can act as a general acid to protonate the pyrophosphate leaving the group (25)(26)(27). Following nucleotide addition, the active site reopens to release the pyrophosphate, but this conformational change is not tightly coupled to translocation as it is in other nucleic acid polymerases (22,28). It has been proposed that additional structural changes in motif B then mechanically aid translocation (29,30) to eventually reset the protein to accept the next incoming NTP.
The 2Ј-C-methyl ribonucleotides may act at any of these steps to terminate RNA synthesis. Initial modeling studies have proposed that the next incoming NTP is prevented from binding because of a steric clash with the 2Ј-C-methyl group (13). Excision of the incorporated 2Ј-C-methyl nucleotide through pyrophosphorolysis (i.e. the reverse of the nucleotide addition reaction) was not sensitive to the next NTP, which, the authors suggested, was also evidence that NTP binding was impeded (31). Incorporation of the 2Ј-C-methyl nucleotide might also disrupt interactions between the RdRp and RNA to promote RNA release, diminish the ability of the RdRp to form the catalytically competent closed conformation, and/or inhibit translocation after nucleotide analog incorporation.
In the absence of X-ray crystal structure data, we used solution-state NMR studies of PV RdRp, along with steady-state kinetics, to provide insight into the mechanism of RNA chain termination by 2Ј-C-methyl ribonucleotides. These studies suggest that incorporation of 2Ј-C-methyl nucleotide prevents subsequent active-site closure, a prerequisite step for incorporation of the next incoming nucleotide.

Incorporation of 2-C-Me-AMP by PV RdRp terminates RNA synthesis and inhibits virus replication
We first tested the ability of PV RdRp to incorporate 2Ј-Cmethyl nucleotide. Here we used 2Ј-C-methyladenosine (2Ј-C-Me-A) as a representative member of the 2Ј-C-methyl nucleotide analogs (Fig. 2), and the ssAU RNA, which contains a 6-bp duplex flanked by four nucleotide 5Ј overhangs (i.e. 5Ј-GCAU- GGGCCC-3Ј) (32) (Fig. 2). For the ssAU RNA, the next correct incoming nucleotides would be ATP followed by UTP. PV RdRp was able to incorporate 2Ј-C-Me-AMP, but this resulted in RNA chain termination, preventing the second nucleotide from being incorporated (Fig. 2). Previous kinetics studies had indicated that incorporation of 2Ј-C-Me-AMP occurs with reduced catalytic efficiency (33), as evidenced by a decreased second-order rate constant k pol /K d,app , where k pol is the maximum polymerase rate constant and K d,app is the apparent dissociation constant for the incoming NTP (Fig. 2). Interestingly, the second-order rate constants for 2Ј-C-Me-AMP and 2Ј-dAMP incorporation were very similar, but 2Ј-C-Me-AMP was more efficiently incorporated than GMP (33) (Fig. 2). As shown previously (13), our studies also indicated that 2Ј-C-Me-A has anti-PV activity (Fig. 2).

C-Met probes report on ligand binding and conformational changes throughout the RdRp structure
PV RdRp is 52 kDa in size, which has made analysis of backbone NMR spectra challenging. Nonetheless, it is now wellestablished that larger proteins (Ͼ50 kDa) can be studied by solution-state NMR using 13 C isotopically labeled methyl groups, in part because of their favorable relaxation properties, which can result in higher signal to noise (34). Indeed, we have previously used [methyl-13 C]Met groups in PV RdRp to gain insight into structural and dynamic changes important for nucleotide selection and catalysis (27,35). The [methyl-13 C]Met probes are conveniently located in or near regions that have been shown by X-ray crystallography structures and/or molecular dynamics simulations to undergo structural and/or dynamic changes upon binding RNA and/or NTP (20 -22, 36, 37) (Fig. 1). In this study, we were especially interested in the Met-6, Met-74, Met-187, Met-225, Met-354, and Met-394 probes, as their associated resonances have been shown to undergo chemical shift and/or peak intensity changes upon binding RNA and/or NTP (27,35) (Fig. 3). Other Met probes are more solvent-exposed and so do not respond to ligand binding and/or associated structural changes (35).
Met-6, Met-74, and Met-187 are located in the fingers subdomain and likely respond to structural rearrangements in motifs A, B, and F. Met-6 is part of the N-terminal ␤-strand that makes hydrogen bond interactions with palm structural motifs A and B. Met-6 is also part of the three-strand ␤-sheet that makes contact with residues in structural motif F (Fig. 4). Motif F is important for RNA template and incoming NTP binding (20,21). Arg-174 in motif F is likely responsible for properly aligning the ␣-phosphate with the primer 3Ј-hydroxyl (38); the R174K-substituted variant provides the highest nucleotide selection incorporation fidelity for any PV variant characterized so far (32), and Coxsackievirus encoding the R174K substitution is not viable (39). His-273 is also part of this interaction network, and it has been shown that the H273R substitution results in a lower nucleotide selection fidelity; PV encoding the H273R substitution has reduced virulence in a mouse model (36,40). Met-74 makes van der Waals contact with the motif B ␣-helix (Fig. 4) and with residues on the ␣1-␣2 loop that also interact with motifs A and B. Met-187 makes contact with the motif B loop important for recognition of the ribose of the incoming NTP (Fig. 4), and residues in this loop may be important for inducing translocation along the RNA (29).
Met-225 and Met-354 are both located in the palm subdomain. Met-225 makes contact with residues in motifs A and C ( Fig. 4) and likely responds to structural changes in these regions, including realignment of the ␤-strand in motif A as part of active-site closure (21) (Fig. 1). Met-354 is in motif D (Fig. 4), and we have proposed that this probe is responsive to structural changes that reposition the general acid Lys-359 for catalysis (27). This probe might also be responsive to accompanying structural changes in motifs A and B. Met-394 is on the thumb subdomain, near the nascent RNA channel (Fig. 4), and likely reports on structural changes important for binding and positioning the RNA primer/template.
Our previous NMR studies of RdRp-RNA binary and RdRp-RNA-NTP ternary complexes provide a framework for comparing this study with the 2Ј-C-Me-A analogs. The 1 H and 13 C chemical shifts for all complexes analyzed in this manuscript can be found in Table S1. Upon addition of ssAU RNA to ligand-free PV RdRp, there were chemical shift changes to the Met-6, Met-187, Met-225, Met-354, and Met-394 resonances and a peak intensity change in the Met-74 resonance (35), suggesting structural and/or dynamics changes in all of the associ- . RNA reaction products were resolved by denaturing PAGE and visualized by phosphorimaging. When 2Ј-C-Me-ATP and UTP were incubated with ssAU RNA, there was no band corresponding to two nucleotide addition events (i.e. ϩ2 position) for over 5 h (i.e. under the time necessary for the NMR experiments). D, the secondorder rate constants for single-nucleotide incorporation based on the ssAU RNA as determined previously (33,51). The kinetic parameters k pol and K d are the maximum polymerase rate constant and the apparent dissociation constant for the incoming NTP, respectively. For the kinetics studies with mispaired termini, studies were conducted using the RNA sequence 5Ј-GCAUG-GGCCCG-3Ј so that the RNA terminus contained a G:U mismatch and the next correct incoming NTP was UTP (27). E, 2Ј-C-Me-adenosine has antiviral activity. HeLa S3 cells were incubated with 2Ј-C-methyladenosine for 1 h at the concentrations shown and subsequently infected with 10 6 pfu of PV. Fifteen minutes after the infection, fresh medium containing 2Ј-C-methyladenosine at the appropriate concentration was added, and the infection progressed for 6 h. Cell-associated virus was titered with plaque assays.

NMR studies of 2-C-methylated nucleotide
ated regions ( Fig. 3 and Fig. S1). To gain insight into ternary RdRp-RNA-NTP complexes, we first added 3Ј-dATP, which the RdRp incorporates into the ssAU RNA to produce the ssAU(3ЈdA) RNA, and then the RdRp-RNA complex was passed through a desalting column to remove excess 3Ј-dATP. Previous studies indicated minor chemical shift differences for Met-187 and Met-354 between the RdRp-ssAU and RdRp-ssAU(3ЈdA) binary complexes (35) (Fig. S1). The RdRp-ssAU(3ЈdA) RNA complex can bind but not incorporate the next incoming NTP. Addition of the next correct NTP to form the RdRp-ssAU(3ЈdA)-UTP ternary complex resulted in additional chemical shift changes in the Met-6, Met-74, Met-187, Met-225, and Met-354 resonances ( Fig. 3 and Fig. S1). Addition of incorrect NTP (2Ј-dUTP or CTP) resulted in chemical shift changes to the Met-6, Met-187, Met-354, and Met-394 resonances compared with what was observed for the RdRp-RNA(3ЈdA) binary complex, indicating that the incorrect NTP still binds but does not induce the same conformational changes as the correct NTP (Fig. 3). Notably, the chemical shift patterns were different between the RdRp-ssAU(3ЈdA)-UTP ternary complex and the RdRp-ssAU(3ЈdA)-2Ј-dUTP and RdRp-ssAU(3ЈdA)-CTP ternary complexes (Figs. 3 and 5). These studies established NMR "fingerprints" for when the enzyme is in an "open" (e.g. RdRp-ssAU(3ЈdA)-CTP) or a closed (e.g. RdRp-ssAU(3ЈdA)-UTP) conformation. In the open conformation, it is likely that Asp-233, the triphosphate of the incoming NTP, and/or the general acid Lys-359 are not properly positioned for the nucleotide addition reaction.

The RdRp-RNA ternary complex with 2-C-methyl-ATP does not achieve the closed conformation
To better understand how 2Ј-C-methyl-ATP interacts with PV RdRp, binary and ternary complexes were evaluated using the ssUU RNA (5Ј-GCUUGGGCCC-3Ј), which was 3Ј-Hterminated according to previous procedures. There were some differences in the NMR spectra between the RdRp-ssAU(3ЈdA) and RdRp-ssUU(3ЈdA) binary complexes (Fig. 5). In particular, there were minor chemical shift differences for the Met-225 and Met-354 resonances. Perhaps more interestingly, there was evidence of conformational exchange in regions associated with Met-187 and Met-394. Met-394 was associated with two resonances, and the Met-187 resonance was at very low intensity, suggestive of conformational exchange on the intermediate NMR timescale. These findings suggested that the RdRp complexes with ssUU(3ЈdA) were more structurally dynamic, which complicated spectral analysis.
The ternary complex with correct incoming NTP (i.e. RdRp-ssUU(3ЈdA)-ATP) also exhibited signs of conformational exchange (Fig. 5). In this case, there were (at least) two resonances associated with Met-225, Met-354, and Met-394. The two resonances for Met-354 in the RdRp-ssUU(3ЈdA)-ATP complex had similar chemical shift positions as those observed  (Fig. 2)) and 4 mM 3Ј-dATP so that 3Ј-dAMP is incorporated but lack of the 3Ј-hydroxyl prevents further nucleotide addition. Excess 3Ј-dATP is removed through a desalting column before addition of the second NTP (4 -12 mM) to generate the ternary RdRp-RNA-NTP complexes. The D 2 O-based buffer consisted of 10 mM HEPES (pH 8.0), 200 mM NaCl, 0.02% NaN 3 , 5 mM MgCl 2 , and 10 M ZnCl 2 . NMR spectra were collected at 293 K using a Bruker Avance III 600 MHz spectrometer. Aspects of these NMR experiments have been reported previously (27,35,36).

NMR studies of 2-C-methylated nucleotide
for Met-354 in the RdRp-ssAU(3ЈdA)-UTP and RdRp-ssAU(3ЈdA)-CTP complexes. This result suggested that the RdRp-ssUU(3ЈdA)-ATP complex fluctuated between the closed and open states, although, in this case, it appeared that the open state was more favored. Although this result was not expected, it should be noted that previous single-nucleotide incorporation studies indicated that AMP incorporation templated against U had the lowest k pol /K d,app value for all "correct" nucleotide incorporations (41). This result may be due to a more limited ability of PV RdRp to fluctuate into the more active closed conformation, consistent with the results observed here. NMR studies with other RNA templates may provide more insight. Nonetheless, the Met-187 resonance for the RdRp-ssUU(3ЈdA)-ATP complex was at a similar chemical shift as that observed for the RdRp-ssAU(3ЈdA)-UTP complex, suggesting that motif B and the surrounding region still recognized ATP as the correct incoming nucleotide.
The RdRp-ssUU(3ЈdA)-2Ј-C-Me-ATP ternary complex had substantial spectral differences compared with the RdRp-ssUU(3ЈdA)-ATP complex (Fig. 5). The Met-187 resonance for the RdRp-ssUU(3ЈdA)-2Ј-C-Me-ATP complex had a very low intensity, again suggestive of conformational exchange, although the chemical shift position was different from that for the RdRp-ssUU(3ЈdA) complex (Fig. 5). The Met-225 probe did not show evidence of conformational exchange. In contrast, both Met-354 and Met-394 were associated with two (or more) resonances, but neither of the Met-354 resonances corresponded to chemical shift positions characteristic of the closed conformation, as observed for the RdRp-ssAU(3ЈdA)-UTP and RdRp-ssUU(3ЈdA)-ATP complexes.

A mispaired RNA terminus prevents active-site closure
Because we have established that PV RdRp can successfully incorporate 2Ј-C-Me-AMP but then cannot extend RNA synthesis (Fig. 2), we wanted to better understand the downstream consequences of 2-C-Me-AMP incorporation. We had previously analyzed the consequences of GMP misincorporation (templated against U) (27). For the NMR studies, we incubated ssAU RNA with 3Ј-dGTP and then removed excess 3Ј-dGTP by passage across a desalting column to generate the RdRp-ssAU(3ЈdG) binary complex. We did not note substantial differences between the RdRp-ssAU(3ЈdA) and RdRp-ssAU(3ЈdG) complexes (Fig. 6), except for the Met-187 resonance. This resonance had a very low peak intensity for the RdRp-ssAU(3ЈdG) complex, suggesting conformational exchange on the intermediate NMR timescale for the associated region. The small differences between the RdRp-ssAU(3ЈdA) and RdRp-ssAU(3ЈdG) complexes suggested that these complexes reached similar conformations, except perhaps in or near motif B.
There were additional chemical shift changes for the Met-187, Met-354, and Met-394 resonances upon addition of the

Incorporation of 2-C-Me-AMP prevents active-site closure
The NMR spectra for the RdRp-RNA-NTP ternary complexes with mismatched RNA termini provided insight into 2Ј-C-Me-AMP-induced chain termination (Fig. 7). The NMR spectrum for the RdRp-ssAU(2ЈCA)-UTP complex was very similar to that of the RdRp-ssAU(3ЈdG)-UTP and RdRp-ssAU(3ЈdA)-CTP complexes. The RdRp-ssUU(2ЈCA)-UTP complex also had similar resonances, although analysis of this spectrum was complicated by conformational exchange events observed in the ssUU-bound complexes that appeared to be absent in the ssAU-bound complexes. These results imply that UTP was capable of binding to the RdRp-ssAU(2ЈCA) and RdRp-ssUU(2ЈCA) complexes but that the ternary complex

NMR studies of 2-C-methylated nucleotide
was not able to fluctuate into the closed conformation necessary for nucleotide incorporation.

The next incoming NTP can still bind after 2-C-Me-AMP incorporation
Our NMR studies suggested that the next incoming NTP could still bind after 2Ј-C-Me-AMP incorporation, although the ternary complex is not able to fluctuate into the closed conformation necessary for the phosphoryl transfer reaction. This proposal is in contrast to the previous suggestion that 2Ј-C-Me-AMP incorporation sterically prevents the next NTP from binding (13). To verify our proposal, we conducted steady-state nucleotide incorporation assays (32) to monitor the effects of the next incoming NTP on RdRp-RNA complex dissociation (Fig. 8). Under steady-state conditions, the rate-determining step for nucleotide incorporation is dissociation of the RdRp-RNA nϩ1 complex so that the RdRp can bind to another RNA n for another nucleotide incorporation reaction (32,42) (Fig. 8A). Addition of the next incoming NTP may have an effect on the rate of RdRp-RNA complex dissociation (Fig. 8). For example, the steady-state incorporation of 3Ј-dAMP was reduced in the presence of UTP, likely because the RdRp becomes trapped in a tight closed conformation (i.e. RdRp-ssAU(3ЈdA)-UTP) that prevents complex dissociation. Formation of the closed conformation would also block the entrance of pyrophosphate and protect the 3Ј-dAMP from pyrophosphorolysis, as observed with the HCV RdRp (31). With 2Ј-C-Me-AMP misincorpora-tion, the presence of UTP increased the steady-state rate, implying that UTP reduced the stability of the RdRp-RNA complex (Fig. 8). However, this result also indicates that UTP is still able to bind and form the RdRp-ssAU(2ЈCA)-UTP complex to exert such an effect. In contrast, addition of the noncognate nucleotide CTP had no effect on the steady-state rate (Fig.  8), likely because CTP would not bind sufficiently to form a ternary complex. RNA incorporated with 2Ј-C-Me nucleotide prevents the RdRp from forming the closed conformation and likely compromises the ability of the next incoming NTP to protect the 2Ј-C-Me nucleotide from pyrophosphorolytic excision, as observed with HCV RdRp (31).

Discussion
2Ј-C-Me ribonucleotides have become a very successful class of antiviral agents in the clinic, exemplified by the anti-HCV drug sofosbuvir (14). However, the molecular mechanism by which they terminate RNA synthesis has remained poorly understood. We chose PV RdRp (Fig. 1) as a model system, considering the vast amount of kinetic and structural data available, including our previous solution-state NMR studies (27,35). PV RdRp can incorporate 2Ј-C-Me-AMP into RNA, which then leads to RNA chain termination (Fig. 2). We had previously established [methyl-13 C]Met probes that report on RNA and NTP binding, including structural/dynamic changes representative of the less active open and more active closed conformations (Figs. 3 and 4). The NMR studies indicated that bind-

NMR studies of 2-C-methylated nucleotide
ing of 2Ј-C-Me-ATP as the next incoming NTP did not result in achievement of the closed conformation (Fig. 5), which was consistent with the reduced second-order rate constant (k pol / K d,app ) for 2Ј-C-Me-AMP incorporation compared with AMP incorporation. After 2Ј-C-Me-AMP was incorporated, the resulting RdRp-RNA binary complex resembled that of other RdRp-RNA complexes (Fig. 6). However, addition of the next correct incoming NTP did not result in formation of the closed conformation (Fig. 7). Steady-state kinetics studies also indicated that the next correct NTP can still bind following 2Ј-C-Me-AMP incorporation (Fig. 8). It has been proposed previously that incorporation of 2Ј-C-Me ribonucleotides terminates RNA synthesis because the 2Ј-C-methyl group sterically prevents the next incoming NTP from binding (13). Although the 2Ј-C-methyl group may still interfere with the binding of the next NTP and may increase its apparent dissociation constant, our studies indicate that binding of the next NTP is not completely abolished. These results also imply that translocation to the next register is not impeded, considering that, in PV RdRp, translocation occurs before binding of the next incoming NTP (28). Altogether, our results indicate RNA synthesis is terminated because incorporation of 2Ј-C-Me-AMP prevents the RdRp from fluctuating into the closed conformation necessary for incorporation of the next NTP.
It has been shown previously that the S282T mutation in HCV confers decreased susceptibility to most 2Ј-C-Me ribonucleotides, including sofosbuvir (43). This Ser is important in binding and recognition of the 2Ј-hydroxyl group of the incoming ribonucleotide. It has been suggested that this amino acid substitution may interfere with initial 2Ј-C-Me-NTP binding because of the steric clash from the additional Thr side-chain methyl group (44). However, it is also worth noting that the resistance variant has some ability to extend RNA synthesis past the incorporated nucleotide analog (13). Moreover, the S282T polymerase has lower catalytic efficiency and is associated with a fitness deficit (44,45). These findings suggest that the S282T substitution may also have an effect on the open-toclosed conformational change necessary to incorporate the next incoming NTP, which would affect both polymerase efficiency and the ability to extend past the incorporated nucleotide analog. Additional NMR studies of the corresponding PV RdRp variant may provide further insight.
Other nonobligate chain terminators may likewise prevent the RdRp from fluctuating into the closed conformation. Nucleoside analogs may also interfere with other events of nucleic acid synthesis. For example, it has been shown that incorporation of the antiviral entecavir by the HIV reverse transcriptase results in "delayed" termination when the polymerase reaches the third nucleotide position downstream of the incorporated analog (46). Incorporation of the Thr-1106 analog results in backtracking of PV RdRp, which likely interferes with processivity and RNA yield (47). NMR studies of these analogs may provide new insights into molecular mechanisms behind translocation and processivity and provide new NMR signa-

NMR studies of 2-C-methylated nucleotide
tures diagnostic of these mechanistic classes of antiviral nucleotides.

Production and purification of PV RdRp from heterologous expression in Escherichia coli
PV RdRp was expressed in E. coli B834(DE3) pRARE cells using autoinduction and then purified as described previously (35,48,49). Protein samples used in NMR experiments were 13 C-labeled by addition of [methyl-13 C]Met to the bacterial growth medium.

PV RdRp assays
Steady-state kinetics assays were performed and analyzed as described previously (32). Reactions contained 50 mM HEPES (pH 7.5), 10 mM ␤-mercaptoethanol, 5 mM MgCl 2 , 60 M ZnCl 2 , 1 M PV RdRp, 20 M ssAU RNA (i.e. 10 M duplex RNA), and 500 M appropriate NTPs. Reactions were initiated with addition of NTP(s), incubated at 30°C, and then quenched at appropriate times by addition of EDTA to a final concentration of 50 mM. Products were analyzed by denaturing PAGE, and gels were visualized through use of a Phosphor Imager and quantified by using ImageQuant TL software (GE Healthcare).

Inhibition of PV replication by 2-C-methyladenosine
The antiviral activity of 2Ј-C-methyladenosine was measured using procedures outlined previously (50). Infection with PV employed HeLa S3 host cells (1 ϫ 10 5 ) plated 1 day prior to treatment in 24-well plates. Cells were pretreated by addition of 2Ј-C-methyladenosine nucleoside at the specified concentration in fresh medium adjusted to a final concentration of 1% DMSO. After a 1-h incubation at 37°C, the medium was removed, and cells were infected with PV (1 ϫ 10 6 pfu). Plates were incubated for 15 min at 23°C, PBS was removed by aspiration, and fresh prewarmed (37°C) medium containing the specified amount of nucleoside was added. The infection was allowed to proceed at 37°C for 6 h. Cells were washed with PBS and collected after treatment with trypsin. Cells were pelleted by centrifugation, resuspended in PBS, and subjected to three freeze-thaw cycles. Cell debris was removed by centrifugation, Figure 8. Incorporation of 2-C-Me-AMP does not prevent the next nucleotide from binding. A, experimental design. The rate-determining step in steady-state nucleotide incorporation is dissociation of the RdRp-RNA nϩ1 complex (42), in which RNA n is the ssAU RNA, and RNA nϩ1 is the ssAU RNA following a single-nucleotide incorporation event. Addition of a second NTP may affect RdRp-RNA complex dissociation to affect the steady-state rate constant. B, steady-state incorporation of nucleotides. Reactions contained 20 M ssAU RNA (i.e. 10 M duplex), 5 mM MgCl 2 , 1 M PV RdRp, and 500 M NTPs. Reactions were initiated by addition of NTP(s), incubated at 30°C, and quenched by addition of EDTA to a final concentration of 50 mM at the indicated times. The steady-state rate constants (k) were determined by dividing the slope by the y-intercept of the line indicated. Addition of UTP (i.e. the next correct incoming NTP) increased the rate of dissociation between the RdRp and RNA with incorporated 2Ј-C-Me-AMP (2Ј-CATP, 2Ј-C-Me-ATP). This result suggests that UTP is still able to bind to form the RdRp-ssAU(2ЈCA)-UTP ternary complex.

NMR studies of 2-C-methylated nucleotide
and the supernatant containing the cell-associated virus was saved. Titer was determined by applying serial dilutions of supernatant to HeLa S3 monolayers (plated in 6-well plates 1 day before at 5 ϫ 10 5 cells/well) and overlaying with growth medium containing low-melting-point agarose (1%). Plates were incubated for 2 days at 37°C. Then the agar was removed, and plaques were visualized by staining with crystal violet (1%) in aqueous ethanol (20%).