Translation Initiation at the CUU Codon Is Mediated by the Internal Ribosome Entry Site of an Insect Picorna-Like Virus In Vitro

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Journal of Virology, February 1999, p. 1219-1226, Vol. 73, No. 2
0022-538X/99/$04.00+0
Copyright © 1999, American Society for Microbiology. All rights reserved.

Translation Initiation at the CUU Codon Is Mediated by the Internal Ribosome Entry Site of an Insect Picorna-Like Virus In Vitro

Jun Sasaki and Nobuhiko Nakashima^*

National Institute of Sericultural and Entomological Science, Owashi, Tsukuba, Ibaraki 305-8634, Japan

Received 19 August 1998/Accepted 2 November 1998

	ABSTRACT

Top Abstract Introduction Materials and methods Results Discussion References

AUG-unrelated translation initiation was found in an insect picorna-like virus, Plautia stali intestine virus (PSIV). Thepositive-strand RNA genome of the virus contains two nonoverlappingopen reading frames (ORFs). The capsid protein gene is locatedin the 3'-proximal ORF and lacks an AUG initiation codon. We examinedthe translation mechanism and the initiation codon of the capsidprotein gene by using various dicistronic and monocistronic RNAsin vitro. The capsid protein gene was translated cap independentlyin the presence of the upstream cistron, indicating that the geneis translated by internal ribosome entry. Deletion analysis showedthat the internal ribosome entry site (IRES) consisted of approximately250 bases and that its 3' boundary extended slightly into thecapsid-coding region. The initiation codon for the IRES-mediatedtranslation was identified as the CUU codon, which is locatedjust upstream of the 5' terminus of the capsid-coding region bysite-directed mutagenesis. In vitro translation assays of monocistronicRNAs lacking the 5' part of the IRES showed that this CUU codonwas not recognized by scanning ribosomes. This suggests that thePSIV IRES can effectively direct translation initiation withoutstable codon-anticodon pairing between the initiation codon andthe initiator methionyl-tRNA.

	INTRODUCTION

Top Abstract Introduction Materials and methods Results Discussion References

Many insect viruses that are morphologically and biophysically similar to mammalian picornaviruses have been reported (20),and they have been called insect picorna-like viruses. Recently,the complete nucleotide sequences of the genomes of several insectpicorna-like viruses have been determined (7, 11, 19, 28,37). Of these viruses, Drosophila C virus (DCV) (11), Rhopalosiphumpadi virus (RhPV) (19) and Plautia stali intestine virus (PSIV)(28) were found to have a novel type of genome organization.The genomes of mammalian picornaviruses consist of positive-strandRNA containing a single large open reading frame (ORF) that codesfor the capsid protein precursor in its 5' part and the nonstructuralprotein precursor in its 3' part (27). In contrast, the genomesof DCV, RhPV, and PSIV contain two ORFs that are separated byan intervening region (Fig. 1A). The nonstructural protein precursoris encoded in the 5'-proximal ORF, and the capsid protein precursoris encoded in the 3'-proximal ORF. Previous studies of these threeviruses have disclosed two unusual features concerning the translationof capsid proteins: the lack of an in-frame AUG initiation codonand the absence of subgenomic RNA (11, 19, 28).

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FIG. 1. Genome organization of PSIV. (A) Schematic diagram of the PSIV genome. ORFs are shown in open boxes. The numbers indicate nucleotide positions. The first nucleotide of the capsid protein gene represents the 5'-terminal nucleotide of the capsid-coding region. (B) Nucleotide and deduced amino acid sequences of the segment between the nonstructural protein gene and the capsid-coding region. The asterisk indicates the stop codon for the nonstructural protein gene.

Several non-AUG initiation codons are used in the translation of viral and cellular mRNAs; however, their translation efficiencyis generally lower than that of the AUG initiation codon (14).Most positive-strand RNA viruses have genome organizations thatproduce an excess of capsid proteins over nonstructural proteins.When capsid proteins are encoded in the 3' part of the genome,as in caliciviruses and togaviruses, the viruses produce subgenomicRNA to translate the capsid proteins (31). The excess productionof capsid proteins is also observed in DCV in vivo (21), butthe virus does not produce subgenomic RNA (11). These observationsraise the question of how DCV, RhPV, and PSIV produce capsid proteinseffectively.

Previously, we showed that translation of the capsid protein of PSIV occurred independently of the nonstructural protein precursorand that the upstream region of the capsid protein gene was necessaryfor the translation (28). This observation suggested that thecapsid protein of PSIV was translated by internal initiation.Internal initiation of translation was first characterized inmammalian picornavirus RNAs (10, 23). Picornavirus genomicRNAs lack the 5' cap structure and have long 5' untranslated regions(5' UTR). The 5' UTRs form multiple stem-loop structures, whichare in contact with ribosomes. This region is called the internalribosome entry site (IRES) and conducts cap-independent translationfor protein synthesis from the genomic RNA (1, 2, 9,30). Internal ribosome entry has also been reported for someviral and cellular RNAs such as hepatitis C virus (HCV) RNA (35,38), cowpea mosaic virus RNA (33), and immunoglobulin heavy-chainbinding protein mRNA (18).

In this study, we confirmed that the capsid protein gene of PSIV was translated by internal ribosome entry in vitro by showingthat translation of the gene occurs cap independently under dicistronicconditions. The 5' and 3' boundaries of the IRES were mapped,and the 3' boundary was found to slightly overlap the capsid-codingregion. We also identified the translation initiation codon ofthe capsid protein gene by using various site-directed mutantsin vitro. The results indicated that translation of the capsidprotein gene is initiated at the CUU codon that is located onecodon upstream of the 5' terminus of the capsid-coding region.CUU differs from AUG by two nucleotides, and such an AUG-unrelatedinitiation codon has not been reported to date. When the 5' partof the IRES was deleted from a monocistronic RNA carrying thecapsid protein gene, scanning ribosomes did not recognize theCUU codon. These data suggest that the PSIV IRES can effectivelydirect AUG-unrelatedinitiation.

	MATERIALS AND METHODS

Top Abstract Introduction Materials and methods Results Discussion References

Plasmid constructs. All the RNA templates used for in vitro translation were transcribed from plasmid vectors containing the T7 RNA polymerasepromotersequence.

pCAT3 control vector (Promega) was digested with HindIII and XbaI, and the resultant 0.7-kb fragment, carrying the chloramphenicolacetyltransferase (CAT) gene, was ligated into those sites inpT7Blue (Novagen), generating pT7CAT. A HindIII (blunt-ended)-EcoRIfragment (corresponding to nucleotides [nt] 5375 to 7096) of acDNA clone of PSIV (28) was ligated into pT7CAT that had beendigested with XbaI, blunt ended, and then digested with EcoRI,generating pT7CAT-5375. This plasmid contains two cistrons underthe control of the T7 promoter. The first is the CAT gene, andthe second is the 5' part of the capsid protein gene. The upstreamsequence of the capsid-coding region is located between the twocistrons.

A series of forward primers (nt 5650 to 5667, 5800 to 5817, 5898 to 5919, 5950 to 5968, 6002 to 6021, and 6100 to 6119) wassynthesized to introduce deletions of the 5' part of the PSIVsequence in pT7CAT-5375. The PSIV sequences with this series ofdeletions were amplified by PCR with synthesized primers and a3' vector-specific primer (5' GTAAAACGACGGCCAGT), using pT7CAT-5375as a template. The amplified fragments were blunt ended, digestedwith EcoRI, and then ligated into pT7CAT that had been digestedwith XbaI, blunt ended, and digested with EcoRI.

The CAT-IRES-LUC series of constructs have a CAT gene as the first cistron and a luciferase (LUC) gene as the second cistron.PGV-CS2 (Toyo Inki Inc.) was digested with HindIII and EcoRI,and the resultant 1.7-kb fragment, containing a LUC gene, wasligated into those sites in pT7Blue, generating pT7LUC. The LUCgene was amplified by PCR with a synthesized primer and the 3'vector-specific primer, using pT7LUC as a template. The initiationcodon of the LUC gene was deleted and a BamHI site was introducedat the 5' end by the PCR. The amplified LUC gene was digestedwith BamHI and EcoRI and then ligated into those sites in pT7CAT,generating pT7CAT-BamLUC. PSIV sequences from nt 5800 to 6192,6195, 6201, and 6264 were amplified by PCR with a forward primerand reverse primers that contained a BamHI site in their 3' ends.The amplified fragments were blunt ended, digested with BamHI,and then ligated into pT7CAT-BamLUC that had been digested withSpeI, blunt ended, and digested with BamHI. The constructs generatedwere named pCAT-IRES₆₁₉₂-LUC, pCAT-IRES₆₁₉₅-LUC, pCAT-IRES₆₂₀₁-LUC,and pCAT-IRES₆₂₆₄-LUCrespectively.

Plasmids used to synthesize monocistronic RNAs were generated by inserting PCR products into pT7Blue. Two PSIV cDNA fragmentswere amplified by PCR with forward primers (corresponding to nt5800 to 5817 and 6173 to 6193) and the 3' vector-specific primer,using pT7CAT-5375 as a template. Two PSIV sequences with an AUC-UAAmutation at nt 6184 to 6187 and a CUU-AUG mutation at nt 6190to 6192 were amplified with forward primers (nt 6173 to 6202)containing the respective mutations and the 3' vector-specificprimer, using p6184TAA or p6190ATG as templates, respectively.These PCR products were blunt ended, digested with EcoRI, andthen ligated into pT7Blue that had been digested with HindIII,blunt ended, and digested with EcoRI.

Site-directed mutagenesis. Site-directed mutagenesis was carried out with a Transformer site-directed mutagenesis kit (Clontech) as described by themanufacturer. Mutations introduced in pT7CAT-5375 were confirmedby nucleotide sequencing with an ABI PRISM Dye Terminator cycle-sequencingkit and a model 377 sequencing system (Perkin-Elmer).

In vitro transcription and in vitro translation. In vitro transcription of linearized plasmids was carried out with T7 RNA polymerase and an RNA transcription kit (Stratagene).The RNAs were synthesized in the presence or absence of a capanalog, 7mGpppG (Stratagene), as recommended by the manufacturer.After DNase I treatment and phenol-chloroform extraction, transcriptswere precipitated with ethanol and ammonium acetate. A portionof the transcripts in each reaction was quantified by agarosegel electrophoresis. Equimolar amounts of RNAs, which correspondedto 10 µg/ml for the transcript of pT7CAT-5375, were used for eachin vitro translation reaction. We used an ECL in vitro translationsystem (Amersham) with 100 mM potassium chloride and 0.5 mM magnesiumacetate in a rabbit reticulocyte lysate. The translation productswere separated by sodium dodecyl sulfate-polyacrylamide gel electrophoresis(12% polyacrylamide), blotted onto a polyvinylidine difluoridemembrane (Bio-Rad), and then detected by enhancedchemiluminescence.

In the in vitro translation assays, a protein band of about 55 kDa were frequently observed in addition to the expected products(see Fig. 2, 3, 4, and 6). We considered that this protein wasinsufficiently denatured capsid protein, because this band wasobserved even under monocistronic conditions (see Fig. 6) andwas detected by Western blotting with antiserum to PSIV particles(data notshown).

	RESULTS

Top Abstract Introduction Materials and methods Results Discussion References

The PSIV capsid protein precursor is translated cap independently by IRES-mediated initiation. We previously indicated that the PSIV capsid protein gene is translated independently of the first ORF and that the upstreamsequence of the capsid-coding region is necessary for translation(28). The mechanisms by which a downstream ORF in a eukaryoticpolycistronic mRNA is translated are known to include leaky scanning,stop codon readthrough, reinitiation (13), and internal initiation(8, 16). Of these mechanisms, translation by internal initiationis cap independent while translation by the other mechanisms iscap dependent. To confirm that translation of the PSIV capsidprotein occurs by internal initiation, the effect of cap structureon translation of the capsid protein gene was investigated invitro. The dicistronic vector, pT7CAT-5375, contains a CAT geneas the first cistron and the 5' part of the PSIV capsid proteingene with its upstream sequence as the second cistron (Fig. 2A).The uncapped RNA transcribed from pT7CAT-5375 produced 39- and25-kDa proteins; the former was much more efficiently translatedthan the latter (Fig. 2B, lane 3). Antiserum directed againstpurified PSIV particles confirmed that this 39-kDa protein wasthe second cistron product (28), while the 25-kDa protein wasbelieved to be the CAT gene product, based on the molecular massof the product from an RNA containing only the CAT gene (pT7CAT;lane 2). When the capped RNA transcribed from pT7CAT-5375 wastranslated, the yield of the first cistron product increased significantlywhereas the yield of the second cistron product was not affected(lane 4). It is known that cap analogs in the translation reactionmixture compete with the 5' cap structure of mRNA. Therefore,cap-dependent translation should be inhibited by cap analogs.When the capped RNA was translated in the presence of a cap analog,7mGpppG (0.8 mM), translation of the first cistron was apparentlyinhibited but that of the second cistron was not affected (lane5). These results indicate that translation of the second cistronoccurs cap independently. Taking our previous result into consideration,we concluded that the PSIV capsid protein is produced by IRES-mediatedtranslation.

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FIG. 2. (A) Schematic diagram of pT7CAT-5375. The thin line indicates the vector sequence, and the triangle on the line represents the location of the T7 RNA polymerase promoter. The thick line indicates the PSIV sequence. The open and shaded boxes show the CAT gene and PSIV capsid-coding region, respectively. The nucleotide positions in the PSIV genome are indicated above the line. The EcoRI site used to linearize the plasmid is also shown. (B) Cap influence on in vitro translation of the RNAs transcribed from pT7CAT-5375. Capped and uncapped RNAs were translated in a rabbit reticulocyte lysate with or without a cap analog, m⁷GTP. To examine the electrophoretic mobility of the CAT protein, uncapped RNA from pT7CAT, which contains only a CAT gene, was also translated. Each product was separated by sodium dodecyl sulfate-polyacrylamide gel electrophoresis (12% polyacrylamide), blotted onto a polyvinylidene difluoride membrane, and then detected by enhanced chemiluminescence. The positions of the translation products (CAT and capsid protein) and molecular mass markers are indicated on the right and left of the panel, respectively. The 55-kDa bands observed in lanes 3 to 5 were thought to be insufficiently denatured proteins translated from the second cistron (see Materials and Methods).

Identification of the capsid protein translation initiation codon. The N terminus of the PSIV capsid protein precursor was mapped at the CAA codon at nt 6193 to 6195 (28). The nucleotidesequence between the stop codon of the nonstructural protein geneand the CAA codon had no in-frame AUG initiation codon or stopcodon (Fig. 1B). To identify the initiation codon for capsid proteintranslation, stop codons were introduced into the upstream sequenceof the capsid-coding region in pT7CAT-5375 by site-directed mutagenesisand transcripts from the mutants were translated in rabbit reticulocytelysate (Fig. 3). The mutation of the codons at nt 6109 to 6111,6154 to 6156, 6172 to 6174, and 6184 to 6186 to stop codons (p6109TAG,p6154TAA, p6172TGA and p6184TAA, respectively) did not affecttranslation of the second cistron (Fig. 3B, lanes 2 to 5). Whenthe UCA codon at nt 6187 to 6189 was mutated to a UGA stop codon(p6187TGA), expression of the second cistron was reduced but noteliminated (lane 6). These results mean that translation of thecapsid proteins is initiated at either the CUU codon at nt 6190to 6192 or the CAA codon at nt 6193 to 6195. When the CUU codonat nt 6190 to 6192 was converted to a UAA stop codon (p6190TAA),there was no translation of the second cistron (lane 7). Thissuggests that the CUU codon at nt 6190 to 6192 was the initiationcodon or that initiation at the CAA codon at nt 6193 to 6195 wasaffected by this mutation.

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FIG. 3. Identification of the initiation codon for capsid protein translation. (A) RNA sequences of mutants derived from pT7CAT-5375. The numbers above the sequence indicate nucleotide positions. Stop codons and inserted nucleotides introduced by site-directed mutagenesis are underlined, and a deleted nucleotide is shown by a dash (p6193Cins-rev). (B) In vitro translation products from uncapped RNAs synthesized from pT7CAT-5375 and the site-directed mutants shown in panel A. The positions of the translation products (CAT and capsid protein) are indicated on the right.

To examine these possibilities, we constructed p6193Cins (Fig. 3A). This plasmid has a cytosine inserted immediately downstreamof the CUU codon to change the reading frame of the capsid proteingene. We assumed that if CAA was the initiation codon, this insertionshould not severely affect translation of the capsid protein.However, a transcript from this plasmid did not produce the secondcistron product (Fig. 3B, lane 8). This result strongly suggeststhat the CUU codon is the initiation codon. To rule out the possibilitythat this insertion affects initiation at the CAA, p6193Cins-revwas constructed (Fig. 3A). In this plasmid, a guanosine at nt6255 was deleted compared with p6193Cins. Therefore, the readingframe of the capsid-coding region was consistent with the CUUcodon. When the RNA transcribed from p6193Cins-rev was translated,the second cistron product reappeared (Fig. 3B, lane 9). Theseresults indicate that the CUU codon at nt 6190 to 6192 is thetranslation initiation codon of the PSIV capsid proteingene.

Mapping the 5' boundary of the IRES for translation initiation of the capsid protein gene. To map the 5' boundary of the IRES for PSIV capsid protein translation, we introduced a series of deletions into the intercistronicregion of pT7CAT-5375 (Fig. 4A). When the nucleotide sequencefrom nt 5375 to 5949 was deleted (pTCAT-5950), the second cistronwas translated as efficiently as in pT7CAT-5375 (Fig. 4B). However,translation of the second cistron was not observed when the nucleotidesequence was deleted up to nt 6001. These results indicate thatthe 5' boundary of the IRES is located between nt 5950 and 6001.

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FIG. 4. Mapping the 5' boundary of IRES for PSIV capsid protein translation. (A) Schematic diagrams of pT7CAT-5375 and a series of deletion mutants. The thin lines indicate vector sequences, and the triangles represent the location of the T7 promoter. The thick lines indicate the PSIV sequence. The CAT genes and PSIV capsid-coding regions are shown by open and shaded boxes, respectively. The numbers above the lines indicate nucleotide positions. Deleted regions are shown by angled lines. (B) In vitro translation products of uncapped RNAs synthesized from pT7CAT-5375 and the deletion mutants shown in panel A. The positions of the translation products (CAT and capsid protein) are indicated on the right.

Mapping the 3' boundary of the IRES for initiation of translation of the capsid protein gene. To map the 3' boundary of the IRES, a LUC gene was used as the second cistron. In the CAT-IRES-LUC series of constructs, LUCgenes without an AUG initiation codon were ligated to the PSIVsequences so that they were in frame (Fig. 5A). When the LUC genewas fused just downstream of the CUU initiation codon (pCAT-IRES₆₁₉₂-LUC),translation of the LUC gene was not observed (Fig. 5B, lane 2).An RNA synthesized from pCAT-IRES₆₁₉₅-LUC also failed to producethe second cistron product (lane 3). The LUC gene was efficientlytranslated when fused downstream of nt 6201 (pCAT-IRES₆₂₀₁-LUC)and nt 6264 (pCAT-IRES₆₂₆₄-LUC) (lanes 4 and 5). These resultsindicate that the 3' boundary of the IRES is located between nt6196 and 6201. This means that the IRES extends into the capsid-codingregion.

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FIG. 5. Mapping the 3' boundary of IRES for PSIV capsid protein translation. (A) Schematic diagrams of the pCAT-IRES-LUC series of constructs. The triangles represent the location of the T7 promoter. The CAT and LUC genes are shown by open and hatched boxes, respectively. The thick lines indicate the PSIV sequences, and the shaded boxes show the PSIV capsid-coding regions. The numbers above the lines indicate the positions of the 5'- and 3'-terminal nucleotides of PSIV sequences. (B) In vitro translation products of uncapped RNAs synthesized from the pCAT-IRES-LUC series of constructs. To examine the electrophoretic mobility of the LUC protein, uncapped RNA synthesized from pT7LUC, which contains only a LUC gene, was also analyzed. The positions of the translation products (CAT and LUC) are indicated on the right of the panel.

The CUU initiation codon does not function in scanning-dependent translation. The initiator methionyl-tRNA (Met-tRNA_i) is the only initiator tRNA (25), and methionine is the initiating residue evenwhen translation is initiated at non-AUG triplets (22). Sincepreviously reported non-AUG initiation codons, such as CUG, GUG,ACG, and AUU, differ from AUG by only one nucleotide, it is thoughtthat at least two base pairs should be required between the initiationcodon and the anticodon of Met-tRNA_i to initiate translation andthat a codon that is completely unrelated to AUG cannot functionas an initiation codon (14). The initiation codon for translatingthe PSIV capsid protein gene, CUU, differs from AUG by two nucleotides.This raised the question whether base pairing between the CUUinitiation codon and the anticodon of Met-tRNA_i is important fortranslation initiation of the PSIV capsid protein. If it is important,a mutation of the CUU initiation codon to AUG is assumed to increasethe yield of the capsid protein. To examine this, we first introduceda CUU-AUG mutation into pT7CAT-5375 to construct p6190ATG (Fig.3A). The in vitro translation assay of the RNA transcribed fromp6190ATG showed that the CUU-AUG mutation reduced the yield ofthe second cistron product (Fig. 3B; lane 10). This was an unexpectedresult because the translation efficiency of most of the previouslyreported non-AUG codons was improved by mutation to AUG (14,32, 36).

Therefore, we carried out an experiment to examine whether the CUU codon is recognized by Met-tRNA_i. Monocistronic RNAs thatare designed to be translated by the scanning mechanism were synthesizedand assayed (pT7-6173; Fig. 6A), because codon-anticodon pairingis essential for scanning-dependent translation initiation. Cappingof the RNA transcribed from pT7-6173 increased the translationalefficiency (Fig. 6B, lanes 3 and 4), indicating that this translationoccurred by the scanning mechanism. Transcripts from pT7-6173generated a product with a slightly larger molecular mass (39.3kDa) than the 39-kDa product observed in the IRES-mediated translation(pT7-5800) (Fig. 6B and C). This larger protein was thought tobe the product of translation initiated at AUC at nt 6184 to 6186,since the codon was the only in-frame potential initiation codonupstream of the CUU codon in the RNA synthesized from pT7-6173(Fig. 6A). Indeed, a transcript with an AUC-AUG mutation at nt6184 to 6186 produced a polypeptide with the same size as theproduct from pT7-6173 (data not shown). A mutation of the AUCcodon to UAA (pT7-6184TAA) abolished production of the largerprotein (Fig. 6B, lanes 5 and 6), and the RNAs with a CUU-AUGmutation at nt 6190 to 6192 (pT7-6190ATG) produced a major proteinwith the same molecular mass as the product in the IRES-mediatedtranslation (lanes 7 and 8). These results show that the CUU codonis not recognized by Met-tRNA_i in scanning-dependent translation.This suggests that translation mediated by the PSIV IRES is initiatedwithout stable codon-anticodon pairing between the CUU initiationcodon and Met-tRNA_i.

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FIG. 6. (A) Schematic diagrams of plasmids used to synthesize monocistronic RNAs. The lines indicate PSIV sequences and the capsid-coding regions are shown as shaded boxes. Triangles represent the location of the T7 promoter. The 5'-terminal nucleotide sequence of the RNA transcribed from the plasmid pT7-6173 is shown. Italic and roman letters indicate the vector and PSIV sequences, respectively. +1 represents the transcription start site for T7 RNA polymerase. The CUU initiation codon is underlined. For pT7-6184TAA and pT7-6190ATG, only mutated codons are shown. (B) In vitro translation products of uncapped and capped RNAs synthesized from pT7-5800, pT7-6173, pT7-6184TAA, and pT7-6190ATG. The position of the translation products (capsid protein) is indicated on the left of the panel. (C) Comparison of the molecular masses of the translation products from pT7-5800 and pT7-6173. To show the difference in mobility, the same amounts of products were electrophoresed.

	DISCUSSION

Top Abstract Introduction Materials and methods Results Discussion References

The PSIV capsid proteins are encoded in the 3' part of the genome. Since PSIV produces no subgenomic RNA and the capsid proteingene lacks an AUG initiation codon (28), the unusual mechanismmust be involved in capsid protein translation. In this study,we have provided data explaining this unusual mechanism: initiationof translation of the PSIV capsid protein gene occurs at a CUUcodon by internal ribosome entry invitro.

Previously, we indicated that the PSIV capsid protein gene is translated independently of the first ORF encoding nonstructuralproteins and that the upstream sequence of the capsid-coding regionis necessary for translation of the capsid protein precursor (28).Here, we showed that translation of the capsid protein occurscap independently in the presence of the upstream cistron (Fig.2), confirming IRES-mediated translation of the capsid proteinprecursor in vitro. The 5' boundary of the IRES was mapped betweennt 5950 and 6001, and the 3' boundary was mapped between nt 6196and 6201. It is noteworthy that the 3' boundary of the IRES lies6 to 11 nt downstream of the initiation codon (Fig. 5). It hasbeen reported that the activity of the IRESs of a flavivirus,HCV (17, 26) and a picornavirus, hepatitis A virus (HAV) (5),depends on the coding sequences downstream of the initiation codon.The IRESs of picornaviruses and HCV consist of approximately 450and 300 nt, respectively (2, 15). The PSIV IRES, which consistsof approximately 250 nt, is shorter than those of picornavirusesandHCV.

The most noteworthy result described here is that the CUU codon at nt 6190 to 6192 is the initiation codon for capsid proteintranslation. Non-AUG codons are known to act as the initiationcodon for protein synthesis in eukaryotes, such as CUG (6,24), GUG (3, 32), ACG (4), and AUU (29). These differfrom AUG by only one nucleotide, while the CUU codon differs bytwo nucleotides. The in vitro translation assay with monocistronicRNAs showed that scanning ribosomes did not recognize the CUUcodon (Fig. 6). This result suggests that the codon-anticodonpairing between the CUU initiation codon and Met-tRNA_i is notessential for translation initiation mediated by the PSIV IRES.In the HCV IRES, mutation of the authentic AUG initiation codonto CUG or AUU only slightly reduced the efficiency of translationinitiation (26). However, when the AUG codon was mutated toGAG or GCG, the initiation site changed to another downstreamcodon. This means that codon-anticodon pairing plays an importantrole in translation initiation mediated by the HCV IRES. Therefore,the PSIV IRES has different mechanism for translation initiationfrom the HCVIRES.

Picornavirus IRESs are divided into two classes based on their location relative to the authentic AUG initiation codon. Inthe enteroviruses and rhinoviruses, the 3' end of the IRES islocated ~150 bases upstream of the initiation codon and ribosomesthat enter the IRES appear to scan until the initiation codon.On the other hand, in cardiovirus and aphthovirus IRESs, ribosomescontact the initiation codon directly (2). In our in vitrotranslation assay of monocistronic RNAs, the CUU codon did notfunction as the initiation codon in scanning-dependent translation.Instead, the AUC codon at nt 6184 to 6186, which is located 2codons upstream of the CUU codon, was recognized as the initiationsite (Fig. 6). However, under the dicistronic conditions, a mutationat the AUC codon (p6184TAA; Fig. 3) did not affect translationof the second cistron. Considering these results, it is probablethat the 40S ribosomal subunit contacts the CUU initiation codondirectly without scanning. If the tertiary structure of the IRESmakes the CUU initiation codon come into contact with the anticodon-loopof Met-tRNA_i within the 40S subunit, translation initiation mayoccur efficiently without stable codon-anticodonpairing.

Since Met-tRNA_i is the only initiator tRNA (25), methionine would also be the initiating amino acid when the capsid proteinprecursor of PSIV is translated by internal ribosome entry. TheN-terminal amino acid of the capsid protein precursor of PSIVis glutamine, which is encoded by the CAA codon at nt 6193 to6195 (Fig. 1B) (28). Therefore, the initiating residue, methionine,should be removed from the capsid protein precursor. In enterovirusesand rhinoviruses of the family Picornaviridae, the N-terminalmethionine of the capsid protein precursor (P1) is removed andthen the penultimate amino acid, glycine, is myristoylated (27).The N-terminal methionine of nascent polypeptide chains is knownto be removed cotranslationally by a methionine aminopeptidase.This processing depends on the penultimate residue (12). Sincethe Met-Gln pair is poorly cleaved by methionine aminopeptidase(12), removal of the methionine in PSIV may occur during capsidformation or by another host protease or viralprotease.

The other two insect picorna-like viruses, DCV (11) and RhPV (19), have similar genome organizations to that of PSIV.The PSIV RNA sequence containing the IRES was aligned with thesequences upstream of the capsid-coding regions of DCV and RhPVby using CLUSTAL W (34) (Fig. 7A), and the secondary structureof the PSIV RNA of this region was predicted with the programMFOLD (Fig. 7B). In the multiple alignment, PSIV, DCV, and RhPVshared several conserved short RNA segments. These conserved segmentswere located at similar positions when the secondary structuresof the DCV and RhPV RNAs were predicted (data not shown). It islikely that these short conserved RNA segments play importantroles in IRES activity. In addition, we found another characteristicsequence, an inverted repeat at nt 6163 to 6167 and 6188 to 6192(Fig. 7A). In the DCV and RhPV sequences, the inverted repeatin this region was also conserved. When the UCA codon at nt 6187to 6189 and the CUU codon at nt 6190 to 6192 were mutated to othercodons, the translational efficiency of the capsid protein geneby internal ribosome entry was reduced (Fig. 3). This result maysuggest the importance of this inverted-repeat sequence on IRES-mediatedtranslation. Since this inverted repeat is located in the loopsegments of stem-loop structures VI and VII (Fig. 7B), it is possiblethat the segment from nt 6163 to 6167 interacts with that fromnt 6188 to 6192.

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FIG. 7. (A) Multiple alignment of nucleotide sequences upstream of PSIV (28), DCV (11), and RhPV (19) (accession no. AB006531, AF014388, and AF022937, respectively) capsid-coding regions. The numbers on the left indicate the starting nucleotide positions of the aligned sequences, and the numbers above the sequences represent the nucleotide positions in the PSIV sequence. The initiation codon for the PSIV capsid protein translation is shown in reverse type. In the PSIV and DCV sequences, the capsid-coding regions are doubly underlined. The DCV sequence has a stop codon (boxed) 2 codons upstream of the 5' terminus of the capsid-coding region, and the RhPV sequence also has a stop codon in the same position. Asterisks indicate nucleotides conserved in all three viruses, and the conserved short RNA segments are underlined. Two arrows below the sequences show an inverted repeat. The double-headed arrows above the sequences represent stem-loop segments in the secondary structure predicted for the PSIV RNA, and the roman numerals correspond to those shown in panel. (B) Computer-predicted secondary structure of the PSIV RNA sequence containing the IRES for the capsid protein translation. The numbers indicate nucleotide positions. The initiation codon is circled. The lines and curves indicate the conserved short RNA segments. Stem-loop structures are numbered from I to VII.

The capsid protein genes of DCV and RhPV also lack an in-frame AUG initiation codon. The capsid protein gene of RhPV has anAUG codon in a different reading frame, and its translation issuggested to occur through a $-$ 1 frameshift (19), while the translationinitiation site of the DCV capsid protein gene is not clearlydefined (11). The alignment data showed that the RNA segmentsupstream of the capsid-coding regions of PSIV, DCV, and RhPV havesimilar primary and secondary structures. In addition, the DCVand RhPV sequences have stop codons that precede the CCU codonsin the position corresponding to the CUU initiation codon of PSIV(Fig. 7A). These data suggest that translation of the capsid proteinsof PSIV, DCV, and RhPV is initiated by a similar mechanism, namely,IRES-mediated translation initiation at an AUG-unrelatedcodon.

	ACKNOWLEDGMENTS

We thank Hiroaki Noda for critical reading of themanuscript.

This work was supported by Enhancement of Centers of Excellence, Special Coordination Funds for Promoting Science and Technology,Science and Technology Agency,Japan.

	FOOTNOTES

^* Corresponding author. Mailing address: National Institute of Sericultural and Entomological Science, Owashi, Tsukuba, Ibaraki305-8634, Japan. Phone: 81 298 38 6109. Fax: 81 298 38 6028. E-mail:nakaji{at}nises.affrc.go.jp.

REFERENCES

Top
Abstract
Introduction
Materials and methods
Results
Discussion
References

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3. Boeck, R., J. Curran, Y. Matsuoka, R. Compans, and D. Kolakofsky. 1992. The parainfluenza virus type 1 P/C gene uses a very efficient GUG codon to start its C' protein. J. Virol. 66:1765-1768[Abstract/Free Full Text].

4. Curran, J., and D. Kolakofsky. 1988. Ribosomal initiation from an ACG codon in the Sendai virus P/C mRNA. EMBO J. 7:245-251[Medline].

5. Graff, J., and E. Ehrenfeld. 1998. Coding sequences enhance internal initiation of translation by hepatitis A virus RNA in vitro. J. Virol. 72:3571-3577[Abstract/Free Full Text].

6. Hann, S. R., M. W. King, D. L. Bentley, C. W. Anderson, and R. N. Eisenman. 1988. A non-AUG translation initiation in c-myc exon 1 generates an N-terminally distinct protein whose synthesis is disrupted in Burkitt's lymphomas. Cell 52:185-195[Medline].

7. Isawa, H., S. Asano, K. Sahara, T. Iizuka, and H. Bando. 1998. Analysis of genetic information of an insect picorna-like virus, infectious flacherie virus of silkworm: evidence for evolutionary relationships among insect, mammalian and plant picorna(-like) viruses. Arch. Virol. 143:127-143[Medline].

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1.	Agol, V. I. 1991. The 5'-untranslated region of picornaviral genomes. Adv. Virus Res. 40:103-180[Medline].
2.	Belsham, G. J., and N. Sonenberg. 1996. RNA-protein interactions in regulation of picornavirus RNA translation. Microbiol. Rev. 60:499-511[Abstract/Free Full Text].
3.	Boeck, R., J. Curran, Y. Matsuoka, R. Compans, and D. Kolakofsky. 1992. The parainfluenza virus type 1 P/C gene uses a very efficient GUG codon to start its C' protein. J. Virol. 66:1765-1768[Abstract/Free Full Text].
4.	Curran, J., and D. Kolakofsky. 1988. Ribosomal initiation from an ACG codon in the Sendai virus P/C mRNA. EMBO J. 7:245-251[Medline].
5.	Graff, J., and E. Ehrenfeld. 1998. Coding sequences enhance internal initiation of translation by hepatitis A virus RNA in vitro. J. Virol. 72:3571-3577[Abstract/Free Full Text].
6.	Hann, S. R., M. W. King, D. L. Bentley, C. W. Anderson, and R. N. Eisenman. 1988. A non-AUG translation initiation in c-myc exon 1 generates an N-terminally distinct protein whose synthesis is disrupted in Burkitt's lymphomas. Cell 52:185-195[Medline].
7.	Isawa, H., S. Asano, K. Sahara, T. Iizuka, and H. Bando. 1998. Analysis of genetic information of an insect picorna-like virus, infectious flacherie virus of silkworm: evidence for evolutionary relationships among insect, mammalian and plant picorna(-like) viruses. Arch. Virol. 143:127-143[Medline].
8.	Ivanov, P. A., O. V. Karpova, M. V. Skulachev, O. L. Tomashevskaya, N. P. Rodionova, Y. L. Dorokhov, and J. G. Atabekov. 1997. A tobamovirus genome that contains an internal ribosome entry site functional in vitro. Virology 232:32-43[Medline].
9.	Jackson, R. J., M. T. Howell, and A. Kaminski. 1990. The novel mechanism of initiation of picornavirus RNA translation. Trends Biochem. Sci. 15:477-483[Medline].
10.	Jang, S. K., H. G. Kräusslich, M. J. H. Nicklin, G. M. Duke, A. C. Palmenberg, and E. Wimmer. 1988. A segment of the 5' nontranslated region of encephalomyocarditis virus RNA directs internal entry of ribosomes during in vitro translation. J. Virol. 62:2636-2643[Abstract/Free Full Text].
11.	Johnson, K. N., and P. D. Christian. 1998. The novel genome organization of the insect picorna-like virus Drosophila C virus suggests this virus belongs to a previously undescribed virus family. J. Gen. Virol. 79:191-203[Abstract].
12.	Kendall, R. L., R. Yamada, and R. A. Bradshaw. 1990. Cotranslational amino-terminal processing. Methods Enzymol. 185:398-407[Medline].
13.	Kozak, M. 1986. Regulation of protein synthesis in virus-infected animal cells. Adv. Virus Res. 31:229-292[Medline].
14.	Kozak, M. 1996. Interpreting cDNA sequences: some insights from studies on translation. Mamm. Genome 7:563-574[Medline].
15.	Lemon, S. M., and M. Honda. 1997. Internal ribosome entry sites within the RNA genomes of hepatitis C virus and other flaviviruses. Semin. Virol. 8:274-288.
16.	Liu, D. X., and S. C. Inglis. 1992. Internal entry of ribosomes on a tricistronic mRNA encoded by infectious bronchitis virus. J. Virol. 66:6143-6154[Abstract/Free Full Text].
17.	Lu, H.-H., and E. Wimmer. 1996. Poliovirus chimeras replicating under the translational control of genetic elements of hepatitis C virus reveal unusual properties of the internal ribosome entry site of hepatitis C virus. Proc. Natl. Acad. Sci. USA 93:1412-1417[Abstract/Free Full Text].
18.	Macejak, D. G., and P. Sarnow. 1991. Internal initiation of translation mediated by the 5' leader of a cellular mRNA. Nature 353:90-94[Medline].
19.	Moon, J. S., L. L. Domier, N. K. McCoppin, C. J. D'Arcy, and H. Jin. 1998. Nucleotide sequence analysis shows that Rhopalosiphum padi virus is a member of a novel group of insect-infecting RNA viruses. Virology 243:54-65[Medline].
20.	Moore, N. F., B. Reavy, and L. A. King. 1985. General characteristics, gene organization and expression of small RNA viruses of insects. J. Gen. Virol. 66:647-659.
21.	Moore, N. F., B. Reavy, J. S. K. Pullin, and N. Plus. 1981. The polypeptides induced in Drosophila cells by Drosophila C virus (strain Ouarzazate). Virology 112:411-416.
22.	Peabody, D. S. 1989. Translation initiation at non-AUG triplets in mammalian cells. J. Biol. Chem. 264:5031-5035[Abstract/Free Full Text].
23.	Pelletier, J., and N. Sonenberg. 1988. Internal initiation of translation of eukaryotic mRNA directed by a sequence derived from poliovirus RNA. Nature 334:320-325[Medline].
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