Characterization of Soluble Hepatitis C Virus RNA-Dependent RNA Polymerase Expressed in Escherichia coli

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Journal of Virology, February 1999, p. 1649-1654, Vol. 73, No. 2
0022-538X/99/$04.00+0
Copyright © 1999, American Society for Microbiology. All rights reserved.

Characterization of Soluble Hepatitis C Virus RNA-Dependent RNA Polymerase Expressed in Escherichia coli

Eric Ferrari, Jacquelyn Wright-Minogue, Jane W. S. Fang, Bahige M. Baroudy, Johnson Y. N. Lau, and Zhi Hong^*

Antiviral Therapy, Schering-Plough Research Institute, Kenilworth, New Jersey 07033-0539

Received 18 June 1998/Accepted 20 October 1998

	ABSTRACT

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Production of soluble full-length nonstructural protein 5B (NS5B) of hepatitis C virus (HCV) has been shown to be problematicand requires the addition of salts, glycerol, and detergents.In an effort to improve the solubility of NS5B, the hydrophobicC terminus containing 21 amino acids was removed, yielding a truncatedNS5B (NS5B $Delta$ CT) which is highly soluble and monodispersed in theabsence of detergents. Fine deletional analysis of this regionrevealed that a four-leucine motif (LLLL) in the hydrophobic domainis responsible for the solubility profile of the full-length NS5B.Enzymatic characterization revealed that the RNA-dependent RNApolymerase (RdRp) activity of this truncated NS5B was comparableto those reported previously by others. For optimal enzyme activity,divalent manganese ions (Mn²⁺) are preferred rather than magnesium ions (Mg²⁺), whereas zinc ions (Zn²⁺) inhibit the RdRp activity. Gliotoxin, a known poliovirus 3DRdRp inhibitor, inhibited HCV NS5B RdRp in a dose-dependent manner.Kinetic analysis revealed that HCV NS5B has a rather low processivitycompared to those of other knownpolymerases.

	TEXT

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Hepatitis C virus (HCV) is currently the leading etiological agent of non-A non-B hepatitis. According to a press releasefrom a recent World Health Organization meeting, more than 170million people worldwide may be infected with HCV. About 80% ofpatients with acute HCV infection will progress to chronic hepatitis;20% of these will develop cirrhosis, and 1 to 5% of these willdevelop hepatocellular carcinoma (28a). More than four millionindividuals in the United States are estimated to be infectedwith HCV (2).

Current therapies with alpha interferon alone and the combination of alpha interferon-ribavirin have been shown to be effectivein a portion of patients with chronic HCV infection (20, 24).Vaccine development has been hampered by the high degree of immuneevasion and the lack of protection against reinfection, even withthe same inoculum (7, 14, 26, 29). Development of smallmolecule inhibitors directed against specific viral targets hasthus become the focus of anti-HCV research. The determinationof crystal structures for NS3 protease (16, 19, 30) andNS3 RNA helicase (15, 31) has provided important structuralinsights for rational design of specificinhibitors.

One key enzyme encoded by HCV is NS5B, which has been shown to be an RNA-dependent RNA polymerase (1, 4, 6, 17,32). NS5B is thus believed to be responsible for genome replicationof HCV. Cellular localization studies revealed that NS5B is membraneassociated and distributed in the perinuclear region (12). Thiscoincides with the distribution of NS5A (27), suggesting thatNS5A and NS5B may stay together after proteolytic cleavage atNS5A/NS5B. It has been postulated that the nonstructural proteinsof HCV (NS3 to -5B) may assemble into membrane-associated replicationcomplexes which are competent for authentic RNA genomereplication.

By itself, HCV NS5B RdRp appears to lack the specificity for HCV RNA and can "copy back" heterologous nonviral RNA (4).This lack of specificity for HCV RNA may reflect the notion thatadditional viral or cellular factors are required for specificrecognition of the replication signal, most likely present atthe 3' untranslated region. Recent studies by Lohmann et al. (17)demonstrated that NS5B alone can replicate the entire HCV genomevia a copy-back mechanism initiated from the end of the 3' untranslatedregion.

Our earlier attempts to express and purify full-length NS5B were hampered by its poor solubility. Recent reports demonstratedthat detergents, salts, and glycerol are required to solubilizethe NS5B protein (4, 6, 17). The hydropathy profile ofNS5B revealed that there is a highly hydrophobic domain at theC terminus (Fig. 1A), which may affect the solubility of NS5B.In an effort to improve the solubility of NS5B, the C-terminalhydrophobic domain containing 21 amino acids was removed and thetruncated protein was compared in parallel with the full-lengthNS5B for expression and purification.

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FIG. 1. (A) Hydropathy profile of NS5B. (B) Parallel expression and purification of full-length and truncated NS5B from HCV-1b, the BK isolate. NS5B cDNAs were cloned into the pET-21b vector (Novagen, Inc.) between the NheI and XhoI sites. The resulting plasmids were transformed into the bacterial host, JM109(DE3), for expression driven by T7 polymerase. Induction by 0.2 mM isopropyl- $beta$ -thiogalactopyranoside (IPTG) was carried out at 24°C for 4 h. Polyhistidine tags (His $-$ ) were engineered into the NS5B clones at either the N terminus or the C terminus to facilitate the purification. All engineered NS5B plasmids were verified by sequencing with the automated sequencer (ABI 377) from Perkin-Elmer (Foster City, Calif.). The purification procedures were similar to those previously reported for the purification of the NS3 protease domain (16) with minor modifications. Protein samples in lanes 2 to 8 are from the full-length His-NS5B, and those in lanes 9 to 15 are from the truncated NS5B $Delta$ CT21-His. Lanes 2 and 9, total soluble lysates; lanes 3 and 10, flowthrough unbound proteins; lanes 4 and 11, proteins from high-salt wash; lanes 5 to 8 and 12 to 15, elution fractions off the Ni-NTA resin. (C) Parallel expression and purification of full-length and truncated NS5B from HCV-1a, the Hutchinson (H77) isolate. The NS5B cDNAs were cloned into pET-28a between 14, total soluble lysates; lanes 3, 9, and 15, flowthrough unbound proteins; lanes 4, 10, and 16, high-salt wash; lanes 5 to 7, 11 to 13, and 17 to 19, elution fractions. M.W., molecular weight.

To facilitate the purification, both full-length NS5B and C-terminally truncated NS5B were expressed as polyhistidine (His $-$ )-taggedfusion proteins. The N-terminally tagged proteins are designatedHis-NS5B or His-NS5B $Delta$ CT21, whereas the C-terminally tagged proteinsare designated NS5B-His or NS5B $Delta$ CT21-His. The results in Fig.1B show that the C-terminally truncated NS5B, NS5B $Delta$ CT21-His, derivedfrom the BK (HCV-1b) isolate, is soluble and yields good purificationwhen applied to a nickel-chelated (Ni-nitrilotriacetic acid [NTA])column (lanes 12 to 15, elution fractions 1 to 4). On the otherhand, the full-length NS5B, His-NS5B, is not soluble under thelysis conditions and thus not purifiable on an Ni-NTA column (lanes5 to 8). The expression levels for both proteins were comparablein the total lysates as detected by Western blot analysis (datanot shown). Further studies using NS5B from a different isolate,H77 (HCV-1a), showed the same results. The full-length NS5Bs (His-NS5Band NS5B-His) are not soluble with little, if any, purificationover the Ni-NTA column (Fig. 1C, lanes 8 to 19), whereas the truncatedprotein (NS5B $Delta$ CT21-His) has good solubility and can be purifiedreadily (Fig. 1C, lanes 2 to 7). Attempts to purify the full-lengthNS5B from the bacterial lysates by the protocols described byLohmann et al. (17) failed, possible due to the problem thatfull-length NS5B expressed in bacterial cells accumulated in theinclusion bodies, which are resistant to the solubilizationmethod.

The truncated proteins were further subjected to a more stringent solubility test by ultracentrifugation at 100,000 × g for30 min. The results (Fig. 2, lanes 3 and 4 and 6 and 7) demonstratedthat the truncated proteins remained in the supernatant underthese conditions in the presence or absence of detergent (0.1%octyl- $beta$ -glucoside). The location of the His tag does not affectthe solubility (His-NS5B $Delta$ CT21 versus NS5B $Delta$ CT21-His), and the Histag can be removed without any loss of solubility (data not shown).In a separate experiment, glycerol (10%) was dialyzed out of theprotein samples and no significant loss of solubility was observed.In fact, a high concentration of salt (NaCl at $>=$ 300 mM) is theonly essential requirement for solubility. The truncated proteinswere well monodispersed in solutions containing high concentrationsof salt as detected by light scattering analysis (data not shown).The above results suggest that the entire or part of the 21-amino-aciddomain at the C terminus plays an important role in determiningthe solubility of NS5B. Its removal improves the solubility ofNS5B in a detergent-glycerol-free and strain-independent manner.

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FIG. 2. Solubility analysis of the truncated NS5B proteins. RCF represents relative centrifugal force (g force). Protein samples were subjected to ultracentrifugation at 100,000 × g for 30 min (at 4°C) with a Beckman Optima TLX Benchtop Ultracentrifuge (in a TLA-45 rotor at a speed of 41,000 rpm), in the presence (+) or absence ( $-$ ) of a nonionic detergent, 0.1% octyl- $beta$ -glucoside. Polyclonal antibodies ( $alpha$ -NS5) raised in rabbits were used for the Western blotting analysis as described previously (11) in lanes 8 to 13.

To map the minimum sequence in the 21-amino-acid domain that is responsible for the lack of solubility, amino acids from thehydrophobic domain were added back sequentially to the C terminusof truncated NS5B (Fig. 3A). The resulting proteins were expressed,and the soluble lysates were applied to the Ni-NTA columns foraffinity purification. Figure 3B shows that up to 5 amino acidscan be added back to the truncated NS5B without significant lossof purifiable proteins (lanes 10 and 13, representing His-NS5B $Delta$ CT19and His-NS5B $Delta$ CT16). However, when an LLLL motif was added back,it rendered the protein (His-NS5B $Delta$ CT12) virtually unpurifiable(lane 16), indicating a dramatic reduction in solubility. Addingback additional amino acids (in His-NS5B $Delta$ CT7 and His-NS5B $Delta$ CT2)failed to improve its solubility. These results demonstrate thatthe LLLL motif-containing proteins, His-NS5B, His-NS5B $Delta$ CT2, His-NS5B $Delta$ CT7,and His-NS5B $Delta$ CT12, have reduced solubility compared to those thatlack the motif, suggesting that the LLLL motif contributes tothe insolubility of NS5B. Multiple alignments of the C-terminaldomains from different genotypes of HCV revealed that this LLLLmotif is absolutely conserved.

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FIG. 3. Fine deletional mapping of an LLLL motif in the C-terminal hydrophobic domain. (A) The N-terminally His-tagged NS5B proteins from HCV-1b (BK isolate) were used to map the motif responsible for the insolubility of NS5B. The sequence for the C-terminal 24 amino acids is shown in the full-length protein (NS5B). Removal of the C-terminal 21 amino acids yields a truncated NS5B ending with a C-terminal sequence of RPR. Adding back the C-terminal 21 amino acids in a sequential manner results in NS5B proteins with different C termini. These truncated proteins are designated according to the number of amino acids deleted from the C-terminal end. (B) Purifiability analysis of NS5B deletion mutants by polyacrylamide gel electrophoresis. Only total soluble lysates, flowthrough proteins, and elution fractions are analyzed for NS5B (lanes 2 to 4), CT $Delta$ 21 (lanes 5 to 7), $Delta$ CT19 (lanes 8 to 10), $Delta$ CT16 (lanes 11 to 13), $Delta$ CT12 (lanes 14 to 16), $Delta$ CT7 (lanes 17 to 19), and $Delta$ CT2 (lanes 20 to 22). M.W., molecular weight.

Further truncations from the C-terminal end of NS5B were constructed, and the resulting proteins, NS5B $Delta$ CT55-His, NS5B $Delta$ CT63-His,NS5B $Delta$ CT70-His, NS5B $Delta$ CT77-His, NS5B $Delta$ CT84-His, and NS5B $Delta$ CT92-His,were subjected to the same purification procedures as that forNS5B $Delta$ CT21-His. Only NS5B $Delta$ CT55-His and NS5B $Delta$ CT63-His could be purifiedfrom the soluble lysates, whereas the further truncated proteinswere not soluble and thus unpurifiable (data not shown). We concludedthat at least 63 amino acids can be removed from the C terminuswithout significant loss of solubility, whereas deletions of morethan 70 amino acids lead to insoluble products. Similar resultswere reported by Lohmann et al., who demonstrated that 55 aminoacids could be deleted without loss of activity, whereas NS5Bwith 84 amino acids deleted could not be purified (17).

To characterize the activity of these soluble NS5B proteins, an RNA-dependent RNA polymerase assay was developed with poly(C)as the template and biotinylated oligo(G)₁₂ as the primer. Incorporationof [³H]GMP into the primer was measured by the scintillation proximityassay (SPA) after the end products were captured by streptavidin-coatedSPA beads (illustrated in Fig. 4A). Under our optimized assayconditions, similar to those described by others (4, 17),NS5B $Delta$ CT21-His was shown to catalyze ribonucleotide polymerization(RNA synthesis) in an RNA template-dependent and primer-dependentmanner. With the activity of NS5B $Delta$ CT21-His normalized to 100%(incorporation of ~6,500 cpm with 0.25 µg of poly(C)-25 ng ofoligo(G)₁₂, 5 µM or 0.05 µCi of GTP, and 50 nM NS5B RdRp at roomtemperature for 3 h with approximately 10% product formation),the activities of other soluble NS5B proteins were compared (Fig.4B). The background of this assay was very low at less than 50cpm. The comparison showed that (i) the truncated NS5Bs with 55or 63 amino acids deleted (NS5B $Delta$ CT55-His and NS5B $Delta$ CT63-His, respectively)were consistently more active than NS5B $Delta$ CT21-His; (ii) truncationswith 19 and 16 amino acids deleted (His-NS5B $Delta$ CT19 and His-NS5B $Delta$ CT16,respectively) did not affect or slightly reduced activities comparedto that of His-NS5B $Delta$ CT21; (iii) the C-terminally tagged proteins(NS5B $Delta$ CT21-His) are about fourfold more active than the N-terminallytagged proteins (His-NS5B $Delta$ CT21); and (iv) NS5Bs from the BK (HCV-1b)isolate are about 5- to 10-fold more active than those correspondingones derived from the H77 (HCV-1a) isolate. Recent studies byLohmann et al. also demonstrated that the N terminus of NS5B isimportant for the RdRp activity and that deletion from the N terminusis detrimental to the RdRp activity (17, 18). Interestingly,the N terminus of poliovirus 3D is also very sensitive to deletion(8, 23) as well as modification: adding two amino acids (alanineand serine) to the N-terminal glycine residue completely abolishesthe 3D RdRp activity (10). It has been suggested that the Nterminus of poliovirus 3D plays an important role in oligomerizationof the polymerase, which is believed to be the functional unitof the viral replicase (8, 21).

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FIG. 4. (A) Illustration of the SPA for RdRp. An SPA (Amersham Life Science) was established for the HCV NS5B RdRp with an RNA homopolymer [poly(C)] as the template complexed with a biotinylated primer [oligo(G)₁₂]. The assay specifically measures the incorporation of tritium-labeled [³H]GMP into the biotinylated RNA products of NS5B which can be captured by the streptavidin-coated SPA beads. The assay conditions were similar to those of a previously described protocol with modifications (4). The assay was carried out at room temperature ( $approx$ 22°C) for 3 h in a final reaction volume of 50 µl and stopped by adding 50 µl of 100 mM EDTA in phosphate-buffered saline. Unless specified, 50 nM RdRp enzymes were used in the assay containing 250 ng of poly(C)-25 ng of oligo(G)₁₂ and 5 µM or 0.05 µCi of GTP. (B) Comparisons of RdRp activities from different soluble and truncated NS5B proteins. The activity of NS5B $Delta$ CT21-His from HCV-1b (BK) is normalized to 100%, which represents a total incorporation of approximately 6,500 cpm. The specific activity is calculated at approximately 870 cpm/pmol of RdRp/h.

Previous reports showed that divalent magnesium ions (Mg²⁺) were required for NS5B RdRp activity (4, 17). We further investigatedthe divalent metal ion requirement of HCV NS5B. Our data showedthat manganese ions (Mn²⁺) were, in fact, approximately four times more effective thanMg²⁺ in coordinating the catalytic reaction of NS5B RdRp and thuspreferred for optimal RdRp activity (Fig. 5A). Zinc ions (Zn²⁺), on the other hand, not only failed to support the RdRp activitybut also inhibited the Mn²⁺-Mg²⁺-dependent RdRp with a 50% inhibitory concentration of approximately60 µM (Fig. 5B). In contrast, the assay conditions for poliovirus3D RdRp consist of zinc ions (60 µM) (9). Given that polymerasesrequire divalent metal ions for activities (3, 13), inhibitionby zinc ions presents several interesting scenarios: (i) is Zn²⁺ a potent competitor of Mg²⁺ or Mn²⁺ for binding to the carboxylate cluster formed by the side chainsof three aspartic acids from motif A and C (8), or (ii) doesZn²⁺ bind to somewhere other than the active site, which allostericallyhinders the nucleophilic attack on the $alpha$ -phosphate by the 3' hydroxylgroup of the primer? If the first scenario is true, Zn²⁺ has to be supercompetent in competing for binding, since theconcentration of Mg²⁺ or Mn²⁺ (5 to 10 mM) is much higher than that of Zn²⁺ (50% inhibitory concentration $approx$ 60 µM). Interestingly, a calciumion (Ca²⁺) was found in the crystal structure of poliovirus 3D polymerasecoordinated by the carboxylate ligands at the active site (8),even though Ca²⁺ does not support the RdRp activity of 3D polymerase.

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FIG. 5. (A) Divalent metal ion requirement for NS5B RdRp. (B) Dose-dependent inhibition of NS5B RdRp activity by zinc ion. The RdRp enzyme used here is NS5B $Delta$ CT21-His from HCV-1b (BK). The assay conditions are described in Materials and Methods. IC50, 50% inhibitory concentration.

Michaelis-Menten steady-state kinetics were analyzed to characterize the enzymatic activity of NS5B RdRp. In a polymerasereaction, multiple substrates including a template-primer complexand a ribonucleotide are involved. Reaction at each step follows,presumably, a sequential order: the polymerase binds to the template-primerfirst to form a binary complex which then takes up a nucleotideto form the catalytically competent ternary complex (5, 13).To determine the kinetic parameters for one substrate, the enzymehas to be saturated by the other. Also, the product formationhas to be limited to less than 10%. The initial velocities (v)at increasing amounts of each substrate were determined. The datawere processed and analyzed with kinetics software (k·cat, version1.5; BioMetallics, Inc.). To estimate the K_m for the template-primer[poly(C)-oligo(G)₁₂] substrate, 200 µM GTP (near saturating amount)was used in the assay in the presence of increasing amounts ofpoly(C)-oligo(G)₁₂ [0.025 to 2.5 µg of poly(C) with a template/primerratio of 10). Based on the results from Fig. 6A, the K_m for thetemplate is about 0.5 µg, which corresponds to approximately 30nM primer [oligo(G)₁₂]. To determine the K_m and the turnover rate(k_cat) for the nucleotide (GTP), saturating amounts of template-primerat 1.25 µg of poly(C)-0.125 µg of oligo(G)₁₂ were used. As shownin Fig. 6B, the K_m for GTP was calculated at 52 µM and the k_catis about 0.3 min¹, indicating that NS5B has a rather low processivity. The lowk_cat value might be in part due to the use of unnatural substratein an assay measuring both the rate-limiting initiation step andthe elongation step (which normally has a higher turnover rate).In a recent report by Lohmann et al., the elongation rate forHCV RdRp was determined at about 150 to 200 nucleotides per min(18). This estimate was based on the size increase of the RNAproduct as a function of time. However, the number of NS5B moleculesrequired for achieving this elongation rate was not determined.A similar study was also conducted to estimate the elongationrate for poliovirus RdRp at about 1,250 nucleotides per min (28).However, it is difficult to compare such elongation rates (differentfrom k_cat values) from these in vitro assays which were carriedout under different conditions (for example, the differences intemperatures or the amount of enzymes, etc.). In fact, when weincreased the assay temperature from room temperature (~22°C)to 30 or 37°C, the k_cat value for HCV NS5B RdRp was significantlyincreased (data not shown).

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FIG. 6. Kinetic analysis of NS5B RdRp activity. (A) Titration of the template-primer at various concentrations; (B) titration of GTPs in the absence and presence of an RdRp-specific inhibitor, gliotoxin. Enzyme HCV-1b NS5B $Delta$ CT21-His (0.1 µM) was used in the kinetic study.

Finally, a panel of known polymerase inhibitors was screened for inhibition of HCV NS5B RdRp. Gliotoxin, a natural product(fungal metabolite), was found to inhibit HCV NS5B RdRp in a dose-dependentmanner (Fig. 6B). Interestingly, gliotoxin also inhibited poliovirus3D RdRp with a similar potency (25), suggesting that gliotoxinmay be an RdRp-specific inhibitor. A recent report by Paul etal. further demonstrated that gliotoxin inhibited both priming(uridylylation of VPg) and elongation mediated by 3D polymerase(22). The kinetic study demonstrated that gliotoxin is a mixednoncompetitive inhibitor with a K_i value of approximately 230µM (Fig. 6B).

The major finding in this report is the identification of a hydrophobic domain at the C terminus of NS5B and mapping of aconserved LLLL motif in this domain which significantly affectsthe solubility on NS5B. Although we have characterized the solubilityof the truncated NS5B extensively, a similar solubility test forthe full-length NS5B has not been performed due to our inabilityto purify the products from bacterial lysates. In a previous report,full-length NS5B products were solubilized from insect cell lysatesin the presence of high concentrations of salt, detergent, andglycerol (17). We failed to solubilize similar full-length NS5Bproducts expressed in bacterial cells. This may be due to theproblem that insoluble NS5Bs produced in bacterial cells accumulatein the inclusion bodies and can be purified only under denaturingconditions. Interestingly, in a recently published report, thefull-length NS5B solubilized in salt, detergent, and glycerolappeared to form high-molecular-weight aggregates (18) whichwere unlikely to remain in solution uponultracentrifugation.

Also, a highly sensitive and quantitative SPA was developed to characterize the RdRp activity. We have demonstrated that thetruncated NS5B from Escherichia coli is as active as those NS5Bsproduced in insect cells reported previously (4, 17), basedon a comparison of radioactivity incorporation under each assaycondition. Another important finding is that Mn²⁺, rather than Mg²⁺, is preferred for optimal RdRp activity, whereas Zn²⁺ is inhibitory. Whether there are any differences in RdRp activitiesamong NS5Bs expressed in various systems will be the subject ofa futurestudy.

Finally, NS5B RdRp activity is sensitive to the presence of gliotoxin, a fungal metabolite. It is a known inhibitor of poliovirus3D RdRp (22, 25). Based on our kinetic analysis, gliotoxinis a mixed noncompetitive inhibitor and is not potent. More importantly,it is a very toxic compound with limited pharmaceutical uses.However, a better understanding of its mechanism of action againstRdRp may shed light on the structural and enzymatic characterizationofRdRp.

	ACKNOWLEDGMENTS

We thank Gregory Reyes and Patricia Weber for support and Charles Lesburg and Michael Cable for helpful discussions. We alsoappreciate the excellent technical assistance of Lin Cheng andMichele Beaudet-Miller.

	FOOTNOTES

^* Corresponding author. Mailing address: Antiviral Therapy, K-15-4945, Schering-Plough Research Institute, 2015 Galloping HillRd., Kenilworth, NJ 07033-0539. Phone: (908) 298-3152. Fax: (908)298-3918. E-mail: zhi.hong{at}spcorp.com.

REFERENCES

Top
Abstract
Text
References

1. Al, R. H., Y. Xie, Y. Wang, and C. H. Hagedorn. 1998. Expression of recombinant hepatitis C virus non-structural protein 5B in Escherichia coli. Virus Res. 53:141-149[Medline].

2. Alter, M. J., and E. E. Mast. 1994. The epidemiology of viral hepatitis in the United States. Gastroenterol. Clin. N. Am. 23:437-455[Medline].

3. Beese, L. S., and T. A. Steitz. 1991. Structural basis for the 3'-5' exonuclease activity of Escherichia coli DNA polymerase I: a two metal ion mechanism. EMBO J. 10:25-33[Medline].

4. Behrens, S.-E., L. Tomei, and R. De Francesco. 1996. Identification and properties of the RNA-dependent RNA polymerase of hepatitis C virus. EMBO J. 15:12-22[Medline].

5. Benkovic, S. J., and C. E. Cameron. 1995. Kinetic analysis of nucleotide incorporation and misincorporation by Klenow fragment of Escherichia coli DNA polymerase I. Methods Enzymol. 262:257-269[Medline].

6. De Francesco, R., S. E. Behrens, L. Tomei, S. Altamura, and J. Jiricny. 1996. RNA-dependent RNA polymerase of hepatitis C virus. Methods Enzymol. 275:58-67[Medline].

7. Farci, P., H. J. Alter, S. Govindarajan, D. C. Wong, R. Engle, R. R. Lesniewski, I. K. Mushahwar, S. M. Desai, R. H. Miller, N. Ogata, and R. H. Purcell. 1992. Lack of protective immunity against reinfection with hepatitis C virus. Science 258:135-140[Abstract/Free Full Text].

8. Hansen, J. L., A. M. Long, and S. C. Schultz. 1997. Structure of the RNA-dependent RNA polymerase of poliovirus. Structure 5:1109-1122[Abstract/Free Full Text].

9. Hey, T. D., O. C. Richards, and E. Ehrenfeld. 1986. Synthesis of plus- and minus-strand RNA from poliovirion RNA template in vitro. J. Virol. 58:790-796[Abstract/Free Full Text].

10. Hong, Z. Unpublished data.

11. Hong, Z., M. Beaudet-Miller, J. Durkin, R. Zhang, and A. D. Kwong. 1996. Identification of a minimal hydrophobic domain in the herpes simplex virus type 1 scaffolding protein which is required for interaction with the major capsid protein. J. Virol. 70:533-540[Abstract].

12. Hwang, S. B., K. J. Park, Y. S. Kim, Y. C. Sung, and M. M. C. Lai. 1997. Hepatitis C virus NS5B protein is a membrane-associated phosphoprotein with a predominantly perinuclear localization. Virology 227:439-446[Medline].

13. Joyce, C. M., and T. A. Steitz. 1994. Function and structure relationships in DNA polymerases. Annu. Rev. Biochem. 63:777-822[Medline].

14. Kao, J. H., P. J. Chen, J. T. Wang, P. M. Yang, M. Y. Lai, T. H. Wang, and D. S. Chen. 1996. Superinfection by homotypic virus in hepatitis C virus carriers: studies on patients with post-transfusion hepatitis. J. Med. Virol. 50:303-308[Medline].

15. Kim, J. L., K. A. Morgenstern, J. P. Griffith, M. D. Dwyer, J. A. Thomson, M. A. Murcko, C. Lin, and P. R. Caron. 1998. Hepatitis C virus NS3 RNA helicase domain with a bound oligonucleotide: the crystal structure provides insights into the mode of unwinding. Structure 6:89-100[Medline].

16. Kim, J. L., K. A. Morgenstern, C. Lin, T. Fox, M. D. Dwyer, J. A. Landro, S. P. Chambers, W. Markland, C. A. Lepre, E. T. O'Malley, S. L. Harbeson, C. M. Rice, M. A. Murcko, P. R. Caron, and J. A. Thomson. 1996. Crystal structure of the hepatitis C virus NS3 protease domain complexed with a synthetic NS4A cofactor peptide. Cell 87:343-355[Medline].

17. Lohmann, V., F. Korner, U. Herian, and R. Bartenschlager. 1997. Biochemical properties of hepatitis C virus NS5B RNA-dependent RNA polymerase and identification of amino acid sequence motifs essential for enzymatic activity. J. Virol. 71:8416-8428[Abstract].

18. Lohmann, V., A. Roos, F. Korner, J. O. Koch, and R. Bartenschlager. 1998. Biochemical and kinetic analyses of NS5B RNA-dependent RNA polymerase of the hepatitis C virus. Virology 249:108-118[Medline].

19. Love, R. A., H. E. Parge, J. A. Wickersham, Z. Hostomsky, N. Habuka, E. W. Moomaw, T. Adachi, and Z. Hostomska. 1996. The crystal structure of hepatitis C virus NS3 proteinase reveals a trypsin-like fold and a structural zinc binding site. Cell 87:331-342[Medline].

20. Marcellin, P., N. Boyer, A. Gervais, M. Martinot, M. Pouteau, C. Castelnau, A. Kilani, J. Areias, A. Auperin, J. P. Benhamou, C. Degott, and S. Erlinger. 1997. Long-term histologic improvement and loss of detectable intrahepatic HCV RNA in patients with chronic hepatitis C and sustained response to interferon-alpha therapy. Ann. Intern. Med. 127:875-881[Abstract/Free Full Text].

21. Pata, J. D., S. C. Schultz, and K. Kirkegaard. 1995. Functional oligomerization of poliovirus RNA-dependent RNA polymerase. RNA 1:466-477[Abstract].

22. Paul, A. V., J. H. van Boom, D. Filippov, and E. Wimmer. 1998. Protein-primed RNA synthesis by purified poliovirus RNA polymerase. Nature 393:280-284[Medline].

23. Plotch, S. J., O. Palant, and Y. Gluzman. 1989. Purification and properties of poliovirus RNA polymerase expressed in Escherichia coli. J. Virol. 63:216-225[Abstract/Free Full Text].

24. Reichard, O., G. Norkrans, A. Fryden, J. H. Braconier, A. Sonnerborg, O. Weiland, and T. S. S. Group. 1998. Randomised, double-blind, placebo-controlled trial of interferon alpha-2b with and without ribavirin for chronic hepatitis C. Lancet 351:83-87[Medline].

25. Rodriguez, P. L., and L. Carrasco. 1992. Gliotoxin: inhibitor of poliovirus RNA synthesis that blocks the viral RNA polymerase 3D^pol. J. Virol. 66:1971-1976[Abstract/Free Full Text].

26. Shimizu, Y. K., M. Hijikata, A. Iwamoto, H. J. Alter, R. H. Purcell, and H. Yoshikura. 1994. Neutralizing antibodies against hepatitis C virus and the emergence of neutralization escape mutant viruses. J. Virol. 68:1494-1500[Abstract/Free Full Text].

27. Tanji, Y., M. Hijikata, S. Satoh, T. Kaneko, and K. Shimotohno. 1995. Hepatitis C virus-encoded nonstructural protein NS4A has versatile functions in viral protein processing. J. Virol. 69:1575-1581[Abstract].

28. Van Dyke, T. A., R. J. Rickles, and J. B. Flanegan. 1982. Genome-length copies of poliovirion RNA are synthesized in vitro by the poliovirus RNA-dependent RNA polymerase. J. Biol. Chem. 257:4610-4617[Abstract/Free Full Text].

28a. World Health Organization. 1998. Lancet 351:1415.

29. Wyatt, C. A., L. Andrus, B. Brotman, F. Huang, D.-H. Lee, and A. M. Prince. 1998. Immunity in chimpanzees chronically infected with hepatitis C virus: role of minor quasispecies in reinfection. J. Virol. 72:1725-1730[Abstract/Free Full Text].

30. Yan, Y., Y. Li, S. Munshi, V. Sardana, J. L. Cole, M. Sardana, C. Steinkuehler, L. Tomei, R. De Francesco, L. C. Kuo, and Z. Chen. 1998. Complex of NS3 protease and NS4A peptide of BK strain hepatitis C virus: a 2.2 A resolution structure in a hexagonal crystal form. Protein Sci. 7:837-847[Abstract].

31. Yao, N., T. Hesson, M. Cable, Z. Hong, A. D. Kwong, H. V. Le, and P. C. Weber. 1997. Structure of the hepatitis C virus RNA helicase domain. Nat. Struct. Biol. 4:463-467[Medline].

32. Yuan, Z. H., U. Kumar, H. C. Thomas, Y. M. Wen, and J. Monjardino. 1997. Expression, purification, and partial characterization of HCV RNA polymerase. Biochem. Biophys. Res. Commun. 232:231-235[Medline].

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Chen, J., Ahlquist, P. (2000). Brome Mosaic Virus Polymerase-Like Protein 2a Is Directed to the Endoplasmic Reticulum by Helicase-Like Viral Protein 1a. J. Virol. 74: 4310-4318 [Abstract] [Full Text]
Tomei, L., Vitale, R. L., Incitti, I., Serafini, S., Altamura, S., Vitelli, A., De Francesco, R. (2000). Biochemical characterization of a hepatitis C virus RNA-dependent RNA polymerase mutant lacking the C-terminal hydrophobic sequence. J. Gen. Virol. 81: 759-767 [Abstract] [Full Text]
Zhong, W., Uss, A. S., Ferrari, E., Lau, J. Y. N., Hong, Z. (2000). De Novo Initiation of RNA Synthesis by Hepatitis C Virus Nonstructural Protein 5B Polymerase. J. Virol. 74: 2017-2022 [Abstract] [Full Text]
Luo, G., Hamatake, R. K., Mathis, D. M., Racela, J., Rigat, K. L., Lemm, J., Colonno, R. J. (2000). De Novo Initiation of RNA Synthesis by the RNA-Dependent RNA Polymerase (NS5B) of Hepatitis C Virus. J. Virol. 74: 851-863 [Abstract] [Full Text]
Lai, V. C. H., Kao, C. C., Ferrari, E., Park, J., Uss, A. S., Wright-Minogue, J., Hong, Z., Lau, J. Y. N. (1999). Mutational Analysis of Bovine Viral Diarrhea Virus RNA-Dependent RNA Polymerase. J. Virol. 73: 10129-10136 [Abstract] [Full Text]
Oh, J.-W., Ito, T., Lai, M. M. C. (1999). A Recombinant Hepatitis C Virus RNA-Dependent RNA Polymerase Capable of Copying the Full-Length Viral RNA. J. Virol. 73: 7694-7702 [Abstract] [Full Text]
Tesmer, J. J., Sunahara, R. K., Johnson, R. A., Gosselin, G., Gilman, A. G., Sprang, S. R. (1999). Two-Metal-Ion Catalysis in Adenylyl Cyclase. Science 285: 756-760 [Abstract] [Full Text]
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1.	Al, R. H., Y. Xie, Y. Wang, and C. H. Hagedorn. 1998. Expression of recombinant hepatitis C virus non-structural protein 5B in Escherichia coli. Virus Res. 53:141-149[Medline].
2.	Alter, M. J., and E. E. Mast. 1994. The epidemiology of viral hepatitis in the United States. Gastroenterol. Clin. N. Am. 23:437-455[Medline].
3.	Beese, L. S., and T. A. Steitz. 1991. Structural basis for the 3'-5' exonuclease activity of Escherichia coli DNA polymerase I: a two metal ion mechanism. EMBO J. 10:25-33[Medline].
4.	Behrens, S.-E., L. Tomei, and R. De Francesco. 1996. Identification and properties of the RNA-dependent RNA polymerase of hepatitis C virus. EMBO J. 15:12-22[Medline].
5.	Benkovic, S. J., and C. E. Cameron. 1995. Kinetic analysis of nucleotide incorporation and misincorporation by Klenow fragment of Escherichia coli DNA polymerase I. Methods Enzymol. 262:257-269[Medline].
6.	De Francesco, R., S. E. Behrens, L. Tomei, S. Altamura, and J. Jiricny. 1996. RNA-dependent RNA polymerase of hepatitis C virus. Methods Enzymol. 275:58-67[Medline].
7.	Farci, P., H. J. Alter, S. Govindarajan, D. C. Wong, R. Engle, R. R. Lesniewski, I. K. Mushahwar, S. M. Desai, R. H. Miller, N. Ogata, and R. H. Purcell. 1992. Lack of protective immunity against reinfection with hepatitis C virus. Science 258:135-140[Abstract/Free Full Text].
8.	Hansen, J. L., A. M. Long, and S. C. Schultz. 1997. Structure of the RNA-dependent RNA polymerase of poliovirus. Structure 5:1109-1122[Abstract/Free Full Text].
9.	Hey, T. D., O. C. Richards, and E. Ehrenfeld. 1986. Synthesis of plus- and minus-strand RNA from poliovirion RNA template in vitro. J. Virol. 58:790-796[Abstract/Free Full Text].
10.	Hong, Z. Unpublished data.
11.	Hong, Z., M. Beaudet-Miller, J. Durkin, R. Zhang, and A. D. Kwong. 1996. Identification of a minimal hydrophobic domain in the herpes simplex virus type 1 scaffolding protein which is required for interaction with the major capsid protein. J. Virol. 70:533-540[Abstract].
12.	Hwang, S. B., K. J. Park, Y. S. Kim, Y. C. Sung, and M. M. C. Lai. 1997. Hepatitis C virus NS5B protein is a membrane-associated phosphoprotein with a predominantly perinuclear localization. Virology 227:439-446[Medline].
13.	Joyce, C. M., and T. A. Steitz. 1994. Function and structure relationships in DNA polymerases. Annu. Rev. Biochem. 63:777-822[Medline].
14.	Kao, J. H., P. J. Chen, J. T. Wang, P. M. Yang, M. Y. Lai, T. H. Wang, and D. S. Chen. 1996. Superinfection by homotypic virus in hepatitis C virus carriers: studies on patients with post-transfusion hepatitis. J. Med. Virol. 50:303-308[Medline].
15.	Kim, J. L., K. A. Morgenstern, J. P. Griffith, M. D. Dwyer, J. A. Thomson, M. A. Murcko, C. Lin, and P. R. Caron. 1998. Hepatitis C virus NS3 RNA helicase domain with a bound oligonucleotide: the crystal structure provides insights into the mode of unwinding. Structure 6:89-100[Medline].
16.	Kim, J. L., K. A. Morgenstern, C. Lin, T. Fox, M. D. Dwyer, J. A. Landro, S. P. Chambers, W. Markland, C. A. Lepre, E. T. O'Malley, S. L. Harbeson, C. M. Rice, M. A. Murcko, P. R. Caron, and J. A. Thomson. 1996. Crystal structure of the hepatitis C virus NS3 protease domain complexed with a synthetic NS4A cofactor peptide. Cell 87:343-355[Medline].
17.	Lohmann, V., F. Korner, U. Herian, and R. Bartenschlager. 1997. Biochemical properties of hepatitis C virus NS5B RNA-dependent RNA polymerase and identification of amino acid sequence motifs essential for enzymatic activity. J. Virol. 71:8416-8428[Abstract].
18.	Lohmann, V., A. Roos, F. Korner, J. O. Koch, and R. Bartenschlager. 1998. Biochemical and kinetic analyses of NS5B RNA-dependent RNA polymerase of the hepatitis C virus. Virology 249:108-118[Medline].
19.	Love, R. A., H. E. Parge, J. A. Wickersham, Z. Hostomsky, N. Habuka, E. W. Moomaw, T. Adachi, and Z. Hostomska. 1996. The crystal structure of hepatitis C virus NS3 proteinase reveals a trypsin-like fold and a structural zinc binding site. Cell 87:331-342[Medline].
20.	Marcellin, P., N. Boyer, A. Gervais, M. Martinot, M. Pouteau, C. Castelnau, A. Kilani, J. Areias, A. Auperin, J. P. Benhamou, C. Degott, and S. Erlinger. 1997. Long-term histologic improvement and loss of detectable intrahepatic HCV RNA in patients with chronic hepatitis C and sustained response to interferon-alpha therapy. Ann. Intern. Med. 127:875-881[Abstract/Free Full Text].
21.	Pata, J. D., S. C. Schultz, and K. Kirkegaard. 1995. Functional oligomerization of poliovirus RNA-dependent RNA polymerase. RNA 1:466-477[Abstract].
22.	Paul, A. V., J. H. van Boom, D. Filippov, and E. Wimmer. 1998. Protein-primed RNA synthesis by purified poliovirus RNA polymerase. Nature 393:280-284[Medline].
23.	Plotch, S. J., O. Palant, and Y. Gluzman. 1989. Purification and properties of poliovirus RNA polymerase expressed in Escherichia coli. J. Virol. 63:216-225[Abstract/Free Full Text].
24.	Reichard, O., G. Norkrans, A. Fryden, J. H. Braconier, A. Sonnerborg, O. Weiland, and T. S. S. Group. 1998. Randomised, double-blind, placebo-controlled trial of interferon alpha-2b with and without ribavirin for chronic hepatitis C. Lancet 351:83-87[Medline].
25.	Rodriguez, P. L., and L. Carrasco. 1992. Gliotoxin: inhibitor of poliovirus RNA synthesis that blocks the viral RNA polymerase 3D^pol. J. Virol. 66:1971-1976[Abstract/Free Full Text].
26.	Shimizu, Y. K., M. Hijikata, A. Iwamoto, H. J. Alter, R. H. Purcell, and H. Yoshikura. 1994. Neutralizing antibodies against hepatitis C virus and the emergence of neutralization escape mutant viruses. J. Virol. 68:1494-1500[Abstract/Free Full Text].
27.	Tanji, Y., M. Hijikata, S. Satoh, T. Kaneko, and K. Shimotohno. 1995. Hepatitis C virus-encoded nonstructural protein NS4A has versatile functions in viral protein processing. J. Virol. 69:1575-1581[Abstract].
28.	Van Dyke, T. A., R. J. Rickles, and J. B. Flanegan. 1982. Genome-length copies of poliovirion RNA are synthesized in vitro by the poliovirus RNA-dependent RNA polymerase. J. Biol. Chem. 257:4610-4617[Abstract/Free Full Text].
28a.	World Health Organization. 1998. Lancet 351:1415.
29.	Wyatt, C. A., L. Andrus, B. Brotman, F. Huang, D.-H. Lee, and A. M. Prince. 1998. Immunity in chimpanzees chronically infected with hepatitis C virus: role of minor quasispecies in reinfection. J. Virol. 72:1725-1730[Abstract/Free Full Text].
30.	Yan, Y., Y. Li, S. Munshi, V. Sardana, J. L. Cole, M. Sardana, C. Steinkuehler, L. Tomei, R. De Francesco, L. C. Kuo, and Z. Chen. 1998. Complex of NS3 protease and NS4A peptide of BK strain hepatitis C virus: a 2.2 A resolution structure in a hexagonal crystal form. Protein Sci. 7:837-847[Abstract].
31.	Yao, N., T. Hesson, M. Cable, Z. Hong, A. D. Kwong, H. V. Le, and P. C. Weber. 1997. Structure of the hepatitis C virus RNA helicase domain. Nat. Struct. Biol. 4:463-467[Medline].
32.	Yuan, Z. H., U. Kumar, H. C. Thomas, Y. M. Wen, and J. Monjardino. 1997. Expression, purification, and partial characterization of HCV RNA polymerase. Biochem. Biophys. Res. Commun. 232:231-235[Medline].