Natural Variation in Translational Activities of the 5' Nontranslated RNAs of Hepatitis C Virus Genotypes 1a and 1b: Evidence for a Long-Range RNA-RNA Interaction outside of the Internal Ribosomal Entry Site

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Journal of Virology, June 1999, p. 4941-4951, Vol. 73, No. 6
0022-538X/99/$04.00+0
Copyright © 1999, American Society for Microbiology. All rights reserved.

Natural Variation in Translational Activities of the 5' Nontranslated RNAs of Hepatitis C Virus Genotypes 1a and 1b: Evidence for a Long-Range RNA-RNA Interaction outside of the Internal Ribosomal Entry Site

Masao Honda,¹^,² Rene Rijnbrand,¹ Geoff Abell,¹ Desok Kim,³ and Stanley M. Lemon¹^,^*

Department of Microbiology and Immunology, The University of Texas Medical Branch at Galveston, Galveston, Texas 77555-1019¹; First Department of Internal Medicine, Kanazawa University, Kanazawa, Japan²; and Department of Surgery, The University of North Carolina at Chapel Hill, Chapel Hill, North Carolina 27599³

Received 16 September 1998/Accepted 4 March 1999

	ABSTRACT

Top Abstract Introduction Materials and Methods Results Discussion References

The 5' nontranslated RNA (5'NTR) of a genotype 1b hepatitis C virus (HCV-N) directs cap-independent translation of the HCV-Npolyprotein with about twofold less efficiency than the 5'NTRof a genotype 1a virus under physiologic conditions (Hutchinsonstrain, or HCV-H) (M. Honda et al., Virology 222:31-42, 1996).Here, we show by mutational analysis that substitution of theAG dinucleotide sequence at nucleotides (nt) 34 and 35 of HCV-Nwith GA (present in HCV-H) restores the translational activityto that of the HCV-H 5'NTR both in vitro and in vivo. These nucleotidesare located upstream of the minimal essential internal ribosomeentry site (IRES), as a 6-nt deletion spanning nt 32 to 37 alsoincreased the translational activity of the HCV-N 5'NTR to thatof HCV-H. Thus, the upstream AG dinucleotide sequence has an inhibitoryeffect on IRES-directed translation. Surprisingly, however, thisinhibitory effect was observed only when the translated, downstreamRNA sequence contained nt 408 to 929 of HCV (capsid-coding RNA).Further analysis of RNA transcripts containing frameshift mutationsdemonstrated that the nucleotide sequence of the transcript, andnot the amino acid sequence of the expressed capsid protein, determinesthis difference in translation efficiency. The difference betweenthe translational activities of the HCV-N and HCV-H transcriptswas increased when translation was carried out in reticulocytelysates containing high K⁺ concentrations, with a sevenfold difference evident at 130 to150 mM K⁺. These results suggest that there is an RNA-RNA interaction involving5'NTR and capsid-coding sequences flanking the IRES and that thisis responsible for the reduced IRES activity of the genotype 1bvirus, HCV-N.

	INTRODUCTION

Top Abstract Introduction Materials and Methods Results Discussion References

Hepatitis C virus (HCV) is a positive-stranded, enveloped RNA virus which is classified within the Hepacivirus genus of thefamily Flaviviridae (3). This virus establishes persistentinfection in most infected humans, leading to the developmentof chronic hepatitis, cirrhosis, and hepatocellular carcinoma(1, 14). There is extensive genetic heterogeneity among differentHCV strains, with at least six major genotypes and a series ofrelated subtypes recognized thus far (5, 24). Among these,genotype 1 is predominant worldwide and comprised of two majorsubtypes, genotypes 1a and 1b (5). Although some clinical studieshave found no differences in the clinical expression of liverdisease related to the genotype of the infecting virus (15),others have suggested that genotype 1b infections may be moreresistant to interferon therapy (17, 30) and may confer greaterrisk for development of hepatocellular carcinoma than infectionwith non-genotype 1b strains including genotype 1a viruses (23).

Despite the considerable genetic diversity that exists among different HCV strains, the 5' nontranslated RNA (5'NTR) sequencesof these viruses are relatively invariant. In large part, thisreflects the presence of conserved, highly ordered RNA structureswithin the viral internal ribosome entry site (IRES) which arerequired for the internal entry of ribosomes on the viral RNAand subsequent cap-independent initiation of translation of theviral polyprotein (8, 12, 19-21, 27, 29). The RNA segmentwhich comprises the IRES occupies most of the 5'NTR, as the 5'limit of the IRES has been mapped to between nucleotides (nt)29 and 46 (11, 12). While the 3' boundary of the IRES is lesscertain, several recent studies indicate that the activity ofthe HCV IRES is dependent on sequence located immediately downstreamof the initiator AUG (12, 16, 19). The initiator AUG appearsto be located within the single-stranded segment of a stem-loop(stem-loop IV) which is formed in part by the capsid protein-codingsequence at the extreme 5' end of the large open reading frameof HCV (10) (Fig. 1). Mutations which enhanced the stabilityof this putative stem-loop significantly reduced the efficiencyof internal initiation of translation, suggesting that the stem-loopmay play a role in controlling translation of the viral polyprotein(10). Larger RNA structures that are upstream of stem-loop IVare absolutely essential for translational activity (12, 21,28), but the most 5' stem-loop within the 5'NTR (stem-loop I,nt 5 to 20) appears to have an opposing action, as its deletionenhances the activity of the downstream IRES both in vitro andin vivo (12, 21).

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FIG. 1. Proposed secondary and tertiary RNA structures within the 5'NTR and the immediately downstream segment of the long open reading frame of the genotype 1b virus HCV-N (10, 11). Major structural domains are labeled I, II, IIIa, IIIb, etc.; the initiator AUG codon in stem-loop IV is highlighted. The circled nucleotides indicate differences between the sequences of HCV-N and the genotype 1a HCV-H virus, which are clustered at four loci: UGA, GA, A₁, and A₂.

We noted previously that the 5'NTR of a genotype 1a virus (Hutchinson strain, or HCV-H) directed translation with greaterefficiency than that of a genotype 1b virus (HCV-N) when placedin the context of nearly genome-length viral RNA (12). We foundthe IRES of the genotype 1a virus to be about twofold more activethan the IRES of the genotype 1b virus, both in a cell-free translationsystem and in transfected Huh-T7 cells in vivo (12). Althoughit is not certain that a twofold difference in translational efficiencywould have a significant impact on either virus replication ordisease expression, we considered it likely that the identificationof the molecular basis for this difference in activity could contributeto a better understanding of the HCV IRES and the structure ofthe 5'NTR. This would be important, because the IRES is increasinglyrecognized as a potential target for antiviral drug development.The sequences of the HCV-H and HCV-N 5'NTRs differ at only sevenbase positions, located at four separate sites (Fig. 1). Significantly,none of the involved nucleotides are involved in base pairingwithin recognized secondary or tertiary RNA structures (2,10).

	MATERIALS AND METHODS

Top Abstract Introduction Materials and Methods Results Discussion References

Plasmids. Plasmids pMN2-1G and PMN2/H have been described previously (12). Plasmid pN-C $Delta$ E1 contains cDNA representing nt 1 to 1357(5'NTR, capsid-coding, and 5' E1-coding sequences) of the HCV-Nvirus (9) (genotype 1b) genome under the transcriptional controlof the T7 promoter. It was constructed by subcloning the XmnI-BamHIfragment of pMN2-1G into pBluescript IISK (Stratagene). pH-C $Delta$ E1is a similar plasmid which contains the 5'NTR of the HCV-H genotype(1a) fused to the 5' open reading frame of HCV-N. It was constructedby subcloning the XhoI-NheI fragment (containing the T7 promotersequence and nt 1 to 249 of the 5'NTR) from pMN2/H into pN-C $Delta$ E1.pN-CLuc contains the 5'NTR sequences of HCV-N and the first 66nt of the HCV open reading frame fused in frame to the fireflyluciferase sequence, under control of the T7 promoter. It wasconstructed by inserting a PCR-amplified fragment of pGEM-Luc(Promega) into the AatII and BamHI sites of pN-C $Delta$ E1. pH-CLuc wasconstructed subsequently by inserting the luciferase sequencefrom pN-CLuc into the AatII and BamHI sites of pH-C $Delta$ E1. pN-CATand pH-CAT contain the 5'NTR sequences of HCV-N and HCV-H, respectively,with 8 nt of the open reading frame fused in frame to the bacterialchloramphenicol acetyltransferase (CAT) sequence under T7 promotercontrol. These were constructed by inserting the small NheI-BamHIfragment of pWT-CAT (21) into pN-C $Delta$ E1 or pH-C $Delta$ E1.

The bicistronic construct pCAT-N(A2)-CLuc contains a T7 transcriptional unit in which the CAT sequence is fused at its 3'end to the 5'NTR of HCV-N (with a change of G to A at nt 243)and 66 nt of the HCV open reading frame fused in frame with theluciferase sequence. It was constructed by inserting the NheI-XmnIfragment of pN-CLuc into pKCUS2 (gift from B. Clarke, Glaxo-Wellcome).pCAT-N-CLuc and pCAT-H-CLuc are similar constructs containingthe 5'NTR sequences of HCV-N and HCV-H, respectively. pCAT-N-C $Delta$ E1is another bicistronic plasmid in which the naturally fused HCVcapsid and 5' E1-coding sequences represent the second cistron.It was constructed by inserting the NheI-BamHI fragment of pN-C $Delta$ E1into pCAT-N-CLuc. The nearly genome-length bicistronic constructspCAT/N, pCAT/H, pCAT/N(UGA), pCAT/N(GA), pCAT/N(A1), and pCAT/N(A2)were constructed by ligating XmnI-BamHI fragments excised frommutated subgenomic bicistronic plasmids with the large BamHI-XmnIfragment of pMN2-1G (HCV nt 1358 to 9454). pN-C $Delta$ E1(H) and pH-C $Delta$ E1(H)are monocistronic constructs that contain the 5'NTR of HCV-N andHCV-H, respectively, fused naturally to the HCV-H open readingframe as the second cistron. These were created by inserting theNheI-BamHI fragment of pRC/CMV/HCV-H (gift from H. Lerat) intopN-C $Delta$ E1 and pH-C $Delta$ E1,respectively.

pCAT-N-C $Delta$ E1(Fs) and pCAT-H-C $Delta$ E1(Fs) contain frameshift mutations in the capsid-coding region. These were constructed by amplifyingthe capsid region with the 5' primer, 5'-ATAGAATTCGACGTCAGTTCCCGGGCGG-3',which lacks A-409 and the 3' primer, 5'-TATAGATCTCCTAGGGGGGCCGCCGACGAGCGGA-3',which inserts a cytosine at nt 769, thus restoring the originalreading frame and maintaining its patency. The amplified PCR fragmentwas inserted into EcoRI and BglII sites of pSP73 (Promega). Theresultant plasmid was digested with AatII and AvrII, and the smallfragment was cloned into pCAT-N-C $Delta$ E1 and pCAT-H-C $Delta$ E1 to make pCAT-N-C $Delta$ E1(Fs)and pCAT-H-C $Delta$ E1(Fs),respectively.

Site-directed mutagenesis of these plasmids (see Results) was carried out by using a standard PCR-based strategy, with Pfu(Pyrococcus furiosus) DNA polymerase. Reactions were for 35 cyclesof 95°C for 1 min, 42°C for 1.5 min, and 75°C for 3 min. The sequencesof the PCR-manipulated regions and the presence of expected mutationswere confirmed by DNA sequencing. Plasmid DNAs were purified onQiagen-tip 500 columns (Qiagen, Chatsworth, Calif.).

Cells. Huh-T7 cells (22), which are derived from Huh-7 human hepatocellular carcinoma cells, are stably transformed and constitutivelyexpress bacteriophage T7 RNA polymerase. Cell cultures were maintainedin Dulbecco's modified Eagle's medium supplemented with 10% fetalbovine serum, penicillin, streptomycin, and 400 µg (active compound)of geneticin (Gibco/BRL) perml.

Antibodies. Murine monoclonal antibody to the HCV capsid protein, 27D5G5, was generously provided by Michel Jolivet, BioMerieux. Rabbitpolyclonal antibody against CAT was purchased from 5' $right-arrow$ 3', Inc.(Boulder, Colo.).

In vitro transcription and translation reactions. Plasmids were linearized by digestion with BamHI or MluI (pN-C $Delta$ E1, pN-CLuc, pN-CAT, pCAT-N-C $Delta$ E1, pCAT-N-CLuc, and relatedmutants) or XhoI (pCAT/N and related mutants). RNA was transcribedby T7 RNA polymerase, using Riboprobe System II (Promega) or Megascript(Ambion) reagents as recommended by the manufacturer. Transcriptionproducts were treated with RQ1 DNase (Promega) for 15 min at 37°C,extracted with phenol-chloroform, precipitated with ethanol-7.5M ammonium acetate, and examined by agarose gel electrophoresis.The concentration of RNA was estimated by spectrophotometry. Insome experiments, RNA was separated from nonincorporated nucleotidesby chromatography through a Sephadex G-25 column and quantifiedby gel analysis. In vitro translation was carried out in micrococcalnuclease-treated rabbit reticulocyte lysate, with or without caninepancreatic microsomal membranes (Promega). The effects of variedKCl concentration were determined by using the Flexilysate system(Promega). Unless otherwise specified, translation reactions (25µl) were programmed with 0.5 to 2.0 µg of RNA and incubated at30°C for 1 h. Total translation products were separated by 12or 13% sodium dodecyl sulfate (SDS)-polyacrylamide $---$ 6 M urea gelelectrophoresis (PAGE) followed by autoradiography. Translationproducts were quantified by PhosphorImager (Molecular Dynamics,Inc.)analysis.

Stability of HCV-H and HCV-N RNAs in reticulocyte lysate. Synthetic RNA transcripts of pN-C $Delta$ E1 and pH-C $Delta$ E1 were trace labeled with ³²P (2.4 × 10⁵ cpm/µg of RNA) and used to program reticulocyte lysate for invitro translation as described above (1 µg of RNA per 25 µl ofreaction mixture); 3-µl aliquots of the reaction mixture weresampled at 0, 20, 40, and 60 min and analyzed by electrophoresisin a 2% agarose-0.1% SDS gel. The gel was dried and then subjectedto autoradiography and PhosphorImageranalysis.

Vaccinia virus-T7 hybrid expression of bicistronic RNA transcripts in transfected Huh-T7 cells. Huh-T7 cells were seeded into four-well tissue culture chamber slides 24 h prior to transfection. Cells (90% confluent) wereinfected with recombinant vaccinia virus vTF7-3 (expressing T7RNA polymerase) (7) in 100 µl of Opti-MEM (Gibco/BRL) at amultiplicity of infection of 10. Following a 1-h incubation at37°C, the virus inoculum was removed and replaced with a mixturecontaining 1 µg of bicistronic plasmid DNA [pCAT/N, pCAT/H, pCAT/N(UGA),pCAT/N(GA), pCAT/N(A1), or pCAT/N(A2)] and 3 µl of Lipofectin(Gibco/BRL) in 40 µl of Opti-MEM at 37°C, followed 15 min laterby an additional 200 µl of Opti-MEM (12). Cells were subsequentlyincubated at 37°C in a 5% CO₂ atmosphere for 24h.

Fluorescence image cytometry. Transfected Huh-T7 cells were washed with phosphate-buffered saline fixed in acetone-methanol (1:1), and stained with rabbitantibody to CAT (1:50 final dilution; 5' $right-arrow$ 3', Inc.) and murinemonoclonal antibody to the HCV capsid protein (27D5G5; 1:12,000dilution; generous gift from Michel Jolivet). After a furtherwash, the cells were incubated with a mixture of fluorescein isothiocyanate(FITC)-conjugated swine antibody to rabbit immunoglobulin (DAKO)and tetramethyl rhodamine isothiocyanate (TRITC)-conjugated goatantibody to mouse immunoglobulin (Organon-Teknika-Cappel, Durham,N.C.), each diluted 1:40. The stained cells were washed extensivelyin phosphate-buffered saline and examined at a magnification of×40 with a Microphot FXA epifluorescence microscope (Nikon), usingfilter sets for TRITC or FITC fluorescence. Fluorescence imageswere recorded with a charge-coupled device camera (Optronics Engineering)and NIH Image acquisition software. Duplicate FITC- and TRITC-labeledimages from 30 dually stained cells from each transfected culturewere transferred to a DEC 5000/200 workstation (Digital EquipmentCorporation), and the boundaries of positive cells were automaticallyextracted by using IGLOO (Image Graphics Library Object-Oriented)(4) and newly developed algorithms allowing automatic generationof cell masks (13). The contribution of nonspecific labelingto the image was eliminated by subtracting the average grey scaleintensity of the background image from the integrated intensity.The ratio of the integrated intensities of the TRITC- and FITC-labeledimages was subsequently calculated for eachcell.

	RESULTS

Top Abstract Introduction Materials and Methods Results Discussion References

Relative efficiency of translation directed by genotype 1a (HCV-H) and genotype 1b (HCV-N) 5'NTRs in vitro. To better quantify the difference in translational activities of the IRESs of HCV-N and HCV-H, we examined the abilities ofRNAs transcribed in vitro from plasmids pN-C $Delta$ E1 and pH-C $Delta$ E1 todirect translation of HCV proteins in rabbit reticulocyte lysates.These transcripts represented the 5'NTR sequences of HCV-N andHCV-H, respectively, fused naturally to nt 342 to 1357 of theopen reading frame of HCV-N. The in vitro translation reactions(25 µl each) were programmed with 0.25 to 2 µg of RNA (10 to 80µg/ml) and supplemented with microsomal membranes to allow signalasecleavage at the capsid-E1 junction. The major products of translationincluded the 21-kDa capsid protein, a 30-kDa truncated, glycosylatedE1 protein ( $Delta$ E1), and a 34-kDa unprocessed precursor protein (C- $Delta$ E1)(Fig. 2A). Lesser quantities of two higher-molecular-mass proteins(46 and 54 kDa) were also observed in some experiments. Althoughno efforts were made to specifically identify these proteins,they likely represent aggregates of the major products. At eachRNA concentration, greater quantities of all of these proteinswere produced by the HCV-H transcripts. PhosphorImager (MolecularDynamics) analysis indicated that the quantities of the capsidand $Delta$ E1 proteins increased in a linear fashion over the rangeof the RNA concentrations used to program translation (Fig. 2B).On average, pH-C $Delta$ E1 transcripts produced 2.4-fold more capsidprotein and 1.8-fold more $Delta$ E1 compared with pN-C $Delta$ E1 transcripts.

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FIG. 2. Translation of RNA transcripts containing genotype 1a HCV-H or genotype 1b HCV-N 5'NTR sequences. (A) SDS-PAGE of products of translation from rabbit reticulocyte lysates programmed with 2 (lanes 1 and 2), 1 (lanes 3 and 4), 0.5 (lanes 5 and 6), 0.25 (lanes 6 and 8), or 0 (lane 9) µg of RNA derived from pH-C $Delta$ E1 (containing the 5'NTR of HCV-H; lanes 1, 3, 5, and 7) or pN-C $Delta$ E1 (containing the 5'NTR of HCV-N; lanes 2, 4, 6, and 8) per 25-µl reaction. (B) Quantitative analysis (relative PhosphorImager band volume) of HCV capsid (left) and $Delta$ E1 (right) proteins produced in reticulocyte lysates programmed with increasing concentrations of RNA transcribed from pH-CDE1 (

) or pN-C $Delta$ E1 (

To exclude the possibility that the difference in the amounts of capsid and $Delta$ E1 proteins produced by the pN-C $Delta$ E1 and pH-C $Delta$ E1transcripts could be due to differences in stability of theseRNAs, we programmed reticulocyte lysate with trace-labeled RNAtranscripts. Reactions were sampled at 20, 40, and 60 min, andthe integrity of the RNA was determined by gel electrophoresis.Approximately 60% of each RNA template was degraded during thefirst 20 min of the reaction (data not shown), but there wereno differences in the rates of degradation of the pN-C $Delta$ E1 andpH-C $Delta$ E1 RNAs. These results were confirmed by RNase protectionassays using an RNA probe targeted to the capsid-coding region,which also showed no differences in the rate of disappearanceof the protected RNA fragment following addition of pN-C $Delta$ E1 andpH-C $Delta$ E1 transcripts to reticulocyte lysate (data not shown). Takentogether, these results confirm that the 5'NTR of HCV-H is abouttwice as active as that of HCV-N in directing translation of theHCV polyprotein in rabbit reticulocytelysates.

Genetic basis of the difference in translational activities of HCV-H and HCV-N. As indicated above, the 5'NTR sequences of the these two viruses differ at seven nucleotide positions (Fig. 1). To determinewhich of these differences in the nucleotide sequences of theseRNAs were responsible for the variation in translational activity,we constructed a series of chimeric 5'NTR constructs in whichthe four nucleotide substitution groups present in the HCV-H sequence(Fig. 1) were systematically introduced into the background ofthe HCV-N sequence in pN-C $Delta$ E1 (Fig. 3A). Plasmids pN-UGA, pN-GA,pN-A₁, and pN-A₂ contain the HCV-H substitutions at nt 11 to 13(GAU $right-arrow$ UGA), 34 and 35 (AG $right-arrow$ GA), 204 (C $right-arrow$ A), and 243 (G $right-arrow$ A), respectively.RNAs transcribed from these plasmids in vitro were used to programreticulocyte lysates for translation at a concentration of 40µg/ml (Fig. 3B). The amounts of capsid and $Delta$ E1 proteins producedfrom pN-GA transcripts (Fig. 3B, lane 4) were nearly equivalentto those produced by pH-C $Delta$ E1 transcripts (lane 2), while pN-UGA,pN-A₁, and pN-A₂ transcripts (lanes 3, 5, and 6) had translationalactivities approximating that of RNA transcribed from pN-C $Delta$ E1(lane 1). These differences were reproducible in three separateexperiments and were confirmed by PhosphorImager analysis (Fig.3C).

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FIG. 3. Genetic basis for the difference in translational activities of the HCV-N and HCV-H 5'NTRs. (A) Organization of T7 transcriptional units within chimeric constructs containing the unique nucleotide sequences of HCV-H placed individually and in combination within the background of the HCV-N 5'NTR and immediately downstream segment of the open reading frame encoding C- $Delta$ E1 (pN-C $Delta$ E1). Protein-coding regions are shown as rectangles; noncoding RNA is shown as a solid line. Map positions of the base substitutions are shown at the bottom. (B) SDS-PAGE of products of translation from reticulocyte lysates programmed with RNAs transcribed from the plasmids depicted in panel A. The two panels represent results from separate experiments. The gel positions of the capsid (C), $Delta$ E1, and nonprocessed C- $Delta$ E1 protein products are shown at the right. (C) PhosphorImager analysis of capsid protein quantities produced in translation experiments such as those shown in panel B. The measured band volumes were normalized to that of reactions programmed with RNA from pN-C $Delta$ E1 (=1.0). The error bars represent the standard error calculated from the results of three separate experiments.

We also studied chimeric transcripts which contained combinations of two nucleotide substitution groups: pN-UGA · GA, pN-UGA· A₁, pN-UGA · A₂, pN-GA · A₁, pN-GA · A₂, and pN-A₁ · A₂ (Fig.3A). RNA transcripts derived from pN-UGA · GA, pN-GA · A₁, andpN-GA · A₂ (Fig. 3B, lanes 10, 13, and 14), which all containthe GA substitution at nt 34 and 35, were translated with an efficiencyequivalent to that for pH-C $Delta$ E1 (Fig. 3B, lane 9). In contrast,translation of the remaining chimeric transcripts, which containAG at this locus (pN-UGA · A₁, pN-UGA · A₂, and pN-A₁ · A₂; lanes11, 12, and 15), did not exceed that of pN-C $Delta$ E1 RNA (lane 8).These findings were reproducible and confirmed by PhosphorImageranalysis (Fig. 3C). They strongly support the conclusion thatthe AG $right-arrow$ GA substitution at nt 34 and 35 is responsible for theincreased translational activity of the HCV-H 5'NTR.

Base substitutions at nt 34 and 35 influence the efficiency of translation only on transcripts containing the complete capsid-coding region. In an effort to develop a sensitive reporter assay to test the effects of these nucleotide substitutions on IRES activityin vivo (see below), we constructed plasmids (pN-CLuc and pH-CLuc)in which sequence encoding the reporter protein, firefly luciferase,was fused in frame at nt 408 of the HCV sequence in pN-C $Delta$ E1 andpH-C $Delta$ E1, thus replacing the sequence downstream of nt 66 of theHCV open reading frame. We also constructed dicistronic variantsof these plasmids (pCAT-N-CLuc and pCAT-H-CLuc), in which sequenceencoding bacterial CAT was placed upstream of the HCV 5'NTR. SyntheticRNA transcripts derived from these plasmids were used to programreticulocyte lysates for translation. Surprisingly, we found thatthe type of 5'NTR sequence (HCV-H or HCV-N) had no influence onthe translational efficiency of either the monocistronic (Fig.4A, lane 1 versus lane 2) or dicistronic (lane 3 versus lane 4)transcripts. The absence of a significant difference in the translationalactivities of the monocistronic transcripts (pN-CLuc and pH-CLuc)was confirmed by direct assay of the translation products forluciferase activity (data not shown), while the absence of a differencebetween the dicistronic transcripts (pCAT-N-CLuc and pCAT-H-CLuc)was confirmed by PhosphorImager analysis of the relative quantitiesof luciferase and CAT produced in each reaction (Fig. 4B). Similarly,we found no differences in the translational activities of dicistronicRNA transcripts which contained the HCV-H base substitutions withinthe background of the HCV-N 5'NTR [pCAT-N(UGA)-CLuc, pCAT-N(GA)-CLuc,pCAT-N(A₁)-CLuc, and pCAT-N(A₂)-CLuc] (data notshown).

To determine whether the absence of a translational difference could be due specifically to the presence of the luciferasesequence, we assessed the translational activity of monocistronictranscripts derived from pN-CAT and pH-CAT (21). These constructscontain the CAT reporter protein sequence fused in frame to HCVcapsid-coding sequence but preserve only 8 nt of the originalHCV open reading frame. As with the luciferase reporter transcripts,there were no differences in the amount of CAT produced from theseRNAs in rabbit reticulocyte lysates (data notshown).

In contrast to these results, dicistronic transcripts in which the truncated HCV open reading frame (C $Delta$ E1) represented thedownstream cistron (pCAT-N-C $Delta$ E1 and pCAT-H-C $Delta$ E1) retained theincreased translational activity observed with the HCV-H 5'NTRin earlier analyses of monocistronic transcripts (Fig. 4A, lane5 versus lane 6; Fig. 4B). The greater translational activityof the HCV-H 5'NTR was evident whether these reaction mixes weresupplemented or not supplemented with microsomal membranes (datanot shown). Although the base substitutions at nt 34 and 35 ofthe HCV-H 5'NTR are responsible for its greater translationalactivity (Fig. 3), these results indicate that the differencein translational activity that these substitutions confer is evidentonly when the transcript contains natural HCV sequences downstreamof nt 408.

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FIG. 4. (A) SDS-PAGE of products of translation from reticulocyte lysates programmed with monocistronic (lanes 1 and 2) or dicistronic (lanes 3 and 4) RNAs in which the HCV capsid sequence beyond nt 66 of the open reading frame was replaced with luciferase sequence. The major luciferase product appears as a band of ~67 kDa, while CAT migrates with an apparent molecular mass of ~24 kDa. Lanes 5 to 10 show a further analysis of the requirements for downstream HCV coding sequence. In pCAT-N-C $Delta$ E1(Fs) and pCAT-H-C $Delta$ E1(Fs) transcripts, the HCV capsid coding sequences contain $-$ 1 and +1 frameshift mutations at nt 409 and 769, respectively, resulting in the expression of the C(Fs) protein which contains nonsense sequence replacing much of the natural capsid sequence. Nucleotides 32 to 37 are deleted from the HCV-N 5'NTR sequence within pCAT-N-C $Delta$ E1( $Delta$ 32-37). The gel positions of the capsid (C), $Delta$ E1, nonprocessed C- $Delta$ E1, luciferase (Luc), and CAT protein products are shown at the right. The most rapidly migrating band observed in lanes 3 to 9 is an unidentified product of the dicistronic RNAs that appears to be derived from the upstream CAT reading frame by an uncertain initiation event. The quantity of this product was closely tied to the quantity of CAT produced in these reactions, and it was not considered in calculating the quantitative estimates of IRES activity shown in Fig. 4B. (B) PhosphorImager analysis of products of translation reactions programmed with dicistronic RNAs in panel A. For each pair of reactions programmed with RNAs containing the HCV-N or HCV-H 5'NTRs, the ratio of the band volumes of the capsid protein and CAT were normalized to the ratio obtained with RNA containing the HCV-N 5'NTR (pCAT-N-CLuc or pCAT-N-C $Delta$ E1 = 1.0). Error bars represent the standard error calculated from replicate experiments.

To further define the downstream sequence required for the enhanced translational activity of the HCV-H 5'NTR, we comparednearly genome-length dicistronic RNA transcripts containing theHCV-H or HCV-N 5'NTR fused naturally to HCV-N sequence extendingto nt 9454 of the HCV genome (plasmids pCAT/N and pCAT/H) (12).While these RNAs produced equivalent amounts of CAT in reticulocytelysates, PhosphorImager analyses indicated that 1.8-fold morecapsid protein was produced from pCAT/H than from pCAT/N (datanot shown). Thus, the inclusion of HCV sequence beyond the truncatedC $Delta$ E1 segment did not influence the relative translational activitiesof the HCV-H and HCV-N 5'NTRs. We next examined the translationalactivities of dicistronic transcripts which contained only thecapsid-coding sequence within the downstream cistron. These RNAswere prepared by runoff transcription of MluI-digested pCAT-N-C $Delta$ E1and pCAT-H-C $Delta$ E1 plasmid DNAs; they terminated at nt 929 of theHCV genome. We again noted significantly greater production ofcapsid protein by transcripts containing the HCV-H 5'NTR (datanot shown). Thus, we conclude that the capsid-coding sequencebetween nt 408 and 929 is required for expression of the differencebetween the translational activities of the HCV-N and HCV-H 5'NTRs.

Expression of the capsid protein is not required for the enhanced translational activity of HCV-H. Experiments with chimeric polioviruses in which the native picornavirus IRES was replaced by the IRES of HCV suggested thatthe HCV capsid protein might play a role in facilitating the internalinitiation of translation (16). If this hypothesis is correct,the fact that we observed differences in the translational activitiesof the HCV-H and HCV-N 5'NTRs only when they were fused to thenative HCV capsid sequence could be explained by differences inthe interaction of these 5'NTRs with the capsid protein. Alternatively,the requirement for capsid sequence could reflect an interactionof this RNA with sequences within the 5'NTR. To distinguish betweenthese two possibilities, we introduced frameshift mutations intothe capsid coding sequence of pCAT-N-C $Delta$ E1 and pCAT-H-C $Delta$ E1. Theresulting plasmids, pCAT-N-C $Delta$ E1(Fs) and pCAT-H-C $Delta$ E1(Fs), eachcontain two mutations: a $-$ 1 frameshift at nt 409 and a +1 frameshiftat nt 769, the latter of which restores the original reading frameand maintains its patency to the end of the truncated E1 sequence.Thus, although transcripts produced from these plasmids differby only 2 nt from the RNAs transcribed from pCAT-N-C $Delta$ E1 and pCAT-H-C $Delta$ E1,they encode a markedly altered capsid protein, C(Fs), which consistsof nonsense sequence between residues 23 and 143, or for approximately63% of itssequence.

As shown in Fig. 4A, both C(Fs) and unprocessed C(Fs) $Delta$ E1 migrated more rapidly than the native capsid and unprocessed C $Delta$ E1proteins in SDS-PAGE (compare lanes 7 and 8 with lanes 5 and 6).However, significantly greater quantities of these nonsense proteinswere expressed from pCAT-H-C $Delta$ E1(Fs) compared with pCAT-N-C $Delta$ E1(Fs)transcripts (compare lanes 7 and 8). By PhosphorImager analysis,there was approximately 1.8-fold more C(Fs) produced from transcriptscontaining the HCV-H 5'NTR (Fig. 4B). Since previous experimentshad demonstrated that the difference in translational activityrequired the presence of sequence between nt 408 and 929, thesedata strongly suggest that the difference in IRES activity isdependent on the nucleotide sequence of the RNA and not the aminoacid sequence of the protein which itencodes.

The AG dinucleotide sequence at nt 34 and 35 of HCV-N has an inhibitory effect on translation. The 5' limit of the minimal essential HCV IRES sequence has not been precisely mapped. However, several studies suggest thatit is located downstream of the dinucleotide sequence at nt 34and 35, which we found to be primarily responsible for the differencein the translational activities of HCV-H and HCV-N transcripts(Fig. 3) (20). Since the nature of the sequence at nt 34 and35 was found to have such an important effect on the translationalactivity of HCV transcripts, it was of interest to further investigatewhether sequence in this region is required for the internal initiationof translation on these RNAs. Thus, we created a 6-nt deletionmutation (nt 32 to 37) in pCAT-N-C $Delta$ E1, resulting in plasmid pCAT-N-C $Delta$ E1( $Delta$ 32-37).Interestingly, dicistronic transcripts derived from this plasmidretained robust IRES activity. The amount of capsid protein producedfrom the pCAT-N-C $Delta$ E1( $Delta$ 32-37) transcripts (Fig. 4A, lane 9) wasapproximately 2.4-fold higher than the amount produced by transcriptsfrom pCAT-N-C $Delta$ E1 (lane 5) and approximately equivalent to theamount produced by transcripts containing the HCV-H 5'NTR (lane6). These results indicate that the AG dinucleotide sequence atnt 34 and 35 is inhibitory to translation directed by the IRESin pCAT-N-C $Delta$ E1. They were confirmed by PhosphorImager analysisin replicate experiments (Fig. 4B). Thus, the sequence at nt 34and 35 is located upstream of the 5' end of the minimal IRES,even though the presence of an AG dinucleotide at this positionhas an inhibitory effect on the activity of the IRES within thegenotype 1b virus. Since we have recently shown that a substitutionof the sequence at nt 45 and 46 significantly reduces IRES activity(11), these results map the 5' border of the IRES to the segmentbetween nt 38 and 46, or at the 5' end of stem-loop II (Fig. 1).

The dinucleotide sequence at nt 34 and 35 determines the efficiency of internal initiation of translation in vivo. Because the studies described above were carried out in vitro with a cell-free translation system, it was important to comparethe translational activities of the HCV-H and HCV-N 5'NTRs invivo. For this purpose, we used the hybrid virus vTF7-3 (7)to direct RNA transcription in Huh-T7 cells (22) transfectedwith the nearly genome-length, bicistronic plasmids pCAT/H andpCAT/N. CAT and capsid protein expression were measured by quantitative,single-cell, double-label, indirect immunofluorescence cytometry.This method allows the ratio of digitally recorded, integratedintensities of the TRITC-labeled capsid image and the FITC-labeledCAT image to be calculated for individual transfected cells (seeMaterials and Methods for details). As the level of CAT reflectsthe abundance of the bicistronic RNA transcripts within each cell,the ratio of capsid protein to CAT should be proportional to thestrength of the IRES in eachtranscript.

In these double-label experiments, approximately 30 to 40% of the cells stained positively for both CAT and capsid proteins(not shown) after transfection with the bicistronic plasmids.Thirty of these cells were sampled from each transfected cultureand subjected to quantitative analysis (Fig. 5). Although therewas considerable cell-to-cell variation in the capsid/CAT (TRITC/FITC)ratio, on average this ratio was approximately 1.9-fold higherin cells transfected with pCAT/H than in those transfected withpCAT/N (P < 0.01). Thus, these results are remarkably concordantwith the in vitro data and confirm that the 5'NTR of HCV-H hasgreater intrinsic activity than the 5'NTR of HCV-N in vivo. Wenext analyzed cells transfected with variants of pCAT/N whichcontained the individual groups of base substitutions presentin the 5'NTR of HCV-H: pCAT/N(UGA), pCAT/N(GA), pCAT/N(A1), andpCAT/N(A2) (Fig. 1). As pCAT/N(GA) was the only one of these plasmidsto express the capsid protein at levels equivalent to that ofpCAT/H (1.74-fold-higher than pCAT/N; P < 0.01), these resultsconfirmed that the dinucleotide sequence at nt 34 and 35 of HCV-His responsible for its increased translational activity in vivo.

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FIG. 5. Quantitative, single-cell, indirect immunofluorescence cytometry for HCV capsid and CAT proteins, following infection of Huh-T7 cells with vTF7-3 and transfection with plasmid DNAs containing nearly genome-length HCV sequences with the 5'NTRs of HCV-N or HCV-H (N, pCAT/N; H, pCAT/H) (see text) or pCAT/N derivatives containing the indicated nucleotide substitutions present in the HCV-H 5'NTR (Fig. 1). Each point represents the ratio of capsid (TRITC label) to CAT (FITC label) content for a single cell. Horizontal bars depict means ± standard deviations (values shown below each data set). P values indicate significant differences from values obtained in cells transfected with pCAT-N-C $Delta$ E1.

The AG dinucleotide sequence and downstream coding region influence the optimal KCl concentrations for IRES-directed translation in vitro. The results described above are consistent with an interaction between RNA segments positioned upstream and downstream ofthe IRES that is detrimental to translation of the HCV-N sequence(see Discussion). If this interaction were due to base pairingbetween the flanking RNA segments, it should be enhanced at higherionic strengths, leading to a greater reduction in the translationalactivity of the IRES. To test this hypothesis, we assessed thetranslational activity of pN-C $Delta$ E1 and pH-C $Delta$ E1 transcripts in thecell-free system at KCl concentrations ranging from 50 to 150mM. These experiments demonstrated a striking difference in thetranslational activities of the HCV-H and HCV-N 5'NTRs at higherconcentrations of KCl (Fig. 6A). pN-C $Delta$ E1 transcripts were optimallytranslated at about 80 mM KCl, with significantly reduced translationat higher KCl concentrations. In contrast, the translation ofpH-C- $Delta$ E1 transcripts was remarkably preserved at higher KCl concentrations,resulting in a much increased difference in the relative translationalactivities of the two transcripts. At 150 mM KCl, translationof pH-C $Delta$ E1 was approximately sevenfold that of pN-C $Delta$ E1 (Fig. 6A;compare lanes 9 and 10).

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FIG. 6. (A) SDS-PAGE of products of translation of pN-C $Delta$ E1 (lanes 1, 3, 5, 7, and 9) and pH-C $Delta$ E1 (lanes 2, 4, 6, 8, and 10) transcripts in rabbit reticulocyte lysates containing increasing concentrations of KCl. (B) Translation of pN-C $Delta$ E1 (lanes 1 and 4), pH-C $Delta$ E1 (lanes 2 and 5), and pN-GA (Fig. 3A) (lanes 3 and 6) transcripts in rabbit reticulocyte lysates containing 80 mM (lanes 1 to 3) and 150 mM (lanes 4 to 6) KCl. (C) Translation of pN-CLuc (lanes 1 and 3) and pH-CLuc (lanes 2 and 4) transcripts in rabbit reticulocyte lysates containing 80 mM (lanes 1 and 2) and 150 mM (lanes 3 and 4) KCl. Luc, luciferase.

To determine whether the differing responses to increased concentrations of KCl were due to the sequence differences thatwe had found to be responsible for the increased translationalactivity of HCV-H, we assessed the translational activity of pN-GAtranscripts at 80 and 150 mM KCl. Although pN-GA differs frompN-C $Delta$ E1 only by the GA-for-AG substitution at nt 34 and 35, pN-GAtranscripts behaved similarly to pH-C $Delta$ E1 transcripts, with relativelyefficient translation even at 150 mM KCl (Fig. 6B; compare lanes4 to 6). Thus, the marked sensitivity of the HCV-N IRES to increasingconcentrations of KCl is related to the AG dinucleotide sequenceat nt 34 and 35. Similar experiments demonstrated that replacementof the HCV-N open reading frame (downstream of nt 409) with theluciferase-coding sequence in pN-CLuc also eliminated the substantialsuppression of HCV-N translation at higher KCl concentrations(compare lanes 1 and 3 in Fig. 6C with lanes 1 and 4 in Fig. 6B).Thus, as in the experiments described above, the reduced translationof the HCV-N transcripts at high concentrations of KCl is determinedby a combination of sequences within RNA segments flanking theIRES. These data are thus supportive of the hypothesis that thereis an interaction between these flanking RNA segments that isdetrimental to IRES-directed translation in HCV-N.

Finally, we determined whether a similar interaction might exist between the HCV-H 5'NTR and HCV-H polyprotein-coding sequence.Monocistronic transcripts derived from pN-C $Delta$ E1 and pH-C $Delta$ E1(H),or pN-C $Delta$ E1(H) and pH-C $Delta$ E1, contain homologous (H-H and N-N forsimplicity) or heterologous (N-H and H-N) combinations of the5'NTRs and polyprotein-coding sequences of HCV-H and HCV-N, respectively.These were used to program reticulocyte lysates under a rangeof KCl concentrations. At 80 mM KCl, the H-N chimeric sequencetranslated with about 2.5-fold-greater activity than the N-N sequence(Fig. 7A), consistent with earlier observations. Although theH-N chimera demonstrated an optimal KCl concentration of about80 mM, it remained reasonably well translated at 130 or even 150mM KCl, relative to translation of the N-N chimera. Strikingly,H-H transcripts were the most active translationally, with anoptimal KCl concentration of 110 mM KCl, and with translationat 130 mM that was equal to or exceeded that at 80 mM KCl (Fig.7B). These results were reproducible in separate experiments.The results shown in Fig. 7 indicate that either the 5'NTR orthe open reading frame of HCV-N contributes to a lessening oftranslational activity when fused to HCV-H sequence to form achimera. In this context, the suppressive effect of the 5'NTRis greater than that of the polyprotein-coding region.

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FIG. 7. Translation of monocistronic transcripts containing each possible combination of the HCV-H and HCV-N 5'NTRs and downstream coding sequences in rabbit reticulocyte lysates supplemented with increasing concentrations of KCl. Products of translation were separated by SDS-PAGE and quantified by PhosphorImager analysis. Relative band volumes were calculated based on the number of methionine residues in each of the two expressed polyproteins. pN-C $Delta$ E1 (··· $bullet$ ···) and pH-C $Delta$ E1(H) (···

···), or pN-C $Delta$ E1(H) ( $---$ $bullet$ $---$ ) and pH-C $Delta$ E1 ( $---$

$---$ ), contain homologous or chimeric combinations of the 5'NTRs and polyprotein coding sequences of HCV-H and HCV-N, respectively. (A) Quantity of translation product produced at each KCl concentration. (B) Translation efficiency of RNA transcripts relative to translation at 80 mM KCl.

	DISCUSSION

Top Abstract Introduction Materials and Methods Results Discussion References

The results described in this report have important implications for the structure of HCV RNA, although their relevance topotential differences in the pathogenesis of infections with genotypes1a and 1b is much less certain, as discussed below. First of all,it is important to note that the seven base substitutions whichdistinguish the 5'NTRs of the HCV-H and HCV-N viruses are representativeof differences in the sequences of other genotype 1a and 1b viruses.We compared the complete 5'NTR sequences of 25 different genotype1a and 1b viruses from GenBank (many other 5'NTR sequences listedin GenBank lack the extreme 5' end). The most frequent differencesbetween the 1a and 1b strains were those which distinguish theHCV-H and HCV-N strains, at nt 11 to 13 (UGA versus GAU in 1aand 1b, respectively), nt 34 and 35 (GA versus AG), nt 204 (Aversus C), and nt 243 (A versus G). Importantly, all 17 genotype1b sequences contained the AG dinucleotide sequence at nt 34 and35, while this sequence was present in only 1 of 8 genotype 1astrains. Thus, the differences that we have found in the translationalactivities of the HCV-H and HCV-N 5'NTRs likely typify differencesbetween most genotype 1a and 1bviruses.

Although the reduced translational activity of the genotype 1b 5'NTR was shown to be due to an inhibitory effect of the AGdinucleotide sequence at nt 34 and 35 (Fig. 3 and 4), this differencewas expressed only when transcripts contained the complete HCVcapsid coding sequence (nt 1 to 929). Previous studies have suggestedthat sequence downstream of the 5'NTR, within the most 5' 30 ntof the open reading frame, may influence the activity of the HCVIRES (10, 12, 19). However, the region identified as influencingtranslational activity in this study lies much further downstream.We found no difference in the translational activities of transcriptscontaining the 1a and 1b 5'NTRs and the first 66 nt of the HCVopen reading frame fused to the luciferase-coding sequence (Fig.4). Thus, the downstream nucleotide sequence required for expressionof the difference between genotypes 1a and 1b in translationalactivities resides between nt 408 and 929 of the HCV genome. Theprimary nucleotide sequences of the genotype 1a and 1b virusesthat we studied differ at approximately 12% of base positionswithin this segment. A further striking observation was that deletionof nt 32 to 37, including the AG dinucleotide sequence, from theHCV-N 5'NTR did not impair but actually enhanced translation fromdicistronic transcripts. Thus, both the upstream and downstreamdeterminants of the greater translational activity of the genotype1a 5'NTR are located outside the minimal essential IRESsequence.

The fact that RNA sequences within the coding region as well as upstream of the IRES act cooperatively to influence the activityof the IRES suggests that these upstream and downstream RNA segmentsphysically interact with each other in a fashion that may influencethe secondary or tertiary structure of RNA within the IRES, orotherwise alters its availability to interact with the 40S ribosomesubunit (18). Alternatively, it is possible that an interactionbetween upstream sequence at nt 34 and 35 and sequence withinthe capsid-coding region is inhibitory to passage of ribosomeson the coding sequence, thus leading to premature terminationof translation or a slower rate of translation. We did not observeany HCV-specific products of translation with a molecular massless than that of the capsid protein among the products of thein vitro translation reactions, but very small polypeptide productswould not be detected in the 11 to 12% polyacrylamide gels usedin thesestudies.

The interaction between the upstream and downstream RNA sequences that we have identified could involve base pair formation,multiple RNA-protein contacts, or both. Smith and Simmonds (26)recently have proposed the existence of conserved secondary RNAstructures within the 5' 167 nt of the HCV open reading frame.This region overlaps with the segment of the coding sequence whichwe identified as influencing genotype 1b translational activity.It is tempting to speculate that these newly recognized structuresform higher-ordered interactions with the extreme 5' end of theviral RNA and that these might function as cis-active signalsin RNA replication. The data shown in Fig. 7 indicate that theHCV-H sequence possesses the ability to interact with either the5'NTR or downstream coding region of the HCV-N sequence. Despitethis, the HCV-H 5'NTR is capable of robust translation of itsopen reading frame, even at high KCl concentrations (Fig. 7).Thus, if this interaction occurs within the isolated HCV-H sequence,it appears to be far less stable than in the HCV-Nsequence.

As indicated above, the 5'NTRs of the genotype 1a and 1b viruses that we studied are representative of the HCV genotypes whichcomprise the majority of virus strains identified within eitherthe United States or Japan and which have been suggested (althoughnot proven) to cause infections with subtly different naturalhistories (17, 23, 25, 30). Could a minimal differencein the translational activities of these viruses at physiologicionic conditions, such as that characterized here, lead to significantdifferences in replication capacity and possibly pathogenicity?Unfortunately, it is not possible to address this question inthe absence of cell culture systems which are permissive for HCVinfection and which mimic the replicative environment of the hepatocytein vivo. Nonetheless, the fact that the AG dinucleotide sequencehad similar effects on HCV translation both in rabbit reticulocytelysates and in transfected Huh-T7 cells suggests that its apparentinhibition of IRES function is not cell type specific. The effectwe observed is thus likely to be present during infection in theliver.

It is also important to note that minimal differences in translational activity can be compounded into substantial differencesin replication capacity, if translation is a rate-limiting stepin virus replication. Other work in our laboratory has shown thatmutations within the 5'NTR of hepatitis A virus, which conferonly a 4- to 6-fold increase in the internal initiation of translationby this picornavirus in monkey kidney cells, result in a markedincrease in the size of replication foci and a 10-fold increasein virus yields in these cells (6, 22). Thus, while thereis no direct evidence that the twofold greater translational activityof the genotype 1a 5'NTR has a significant impact on viral replicationor pathogenesis in vivo, this possibility cannot be excluded atpresent.

	ACKNOWLEDGMENTS

This work was supported in part by grants RO1-AI32599 and U19-AI40035 from the National Institute of Allergy and InfectiousDiseases.

	FOOTNOTES

^* Corresponding author. Mailing address: Department of Microbiology and Immunology, The University of Texas Medical Branch atGalveston, 301 University Blvd., Galveston, TX 77555-1019. Phone:(409) 772-2324. Fax: (409) 772-3757. E-mail: smlemon{at}utmb.edu.

REFERENCES

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
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30. Zein, N. N., and D. H. Persing. 1996. Hepatitis C genotypes: current trends and future implications. Mayo Clin. Proc. 71:458-462[Abstract].

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