Polypyrimidine Tract-Binding Protein Binds to the Leader RNA of Mouse Hepatitis Virus and Serves as a Regulator of Viral Transcription

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Journal of Virology, January 1999, p. 772-777, Vol. 73, No. 1
0022-538X/99/$04.00+0
Copyright © 1999, American Society for Microbiology. All rights reserved.

Polypyrimidine Tract-Binding Protein Binds to the Leader RNA of Mouse Hepatitis Virus and Serves as a Regulator of Viral Transcription

Hsin-Pai Li,¹ Peiyong Huang,¹ Sungmin Park,¹ and Michael M. C. Lai¹^,²^,^*

Department of Molecular Microbiology and Immunology¹ and Howard Hughes Medical Institute,² University of Southern California School of Medicine, Los Angeles, California 90033-1054

Received 29 April 1998/Accepted 25 September 1998

	ABSTRACT

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A cellular protein, previously described as p55, binds specifically to the plus strand of the mouse hepatitis virus (MHV)leader RNA. We have purified this protein and determined by partialpeptide sequencing that it is polypyrimidine tract-binding protein(PTB) (also known as heterogeneous nuclear ribonucleoprotein [hnRNP]I), a nuclear protein which shuttles between the nucleus and cytoplasm.PTB plays a role in the regulation of alternative splicing ofpre-mRNAs in normal cells and translation of several viruses.By UV cross-linking and immunoprecipitation studies using cellularextracts and a recombinant PTB, we have established that PTB bindsto the MHV plus-strand leader RNA specifically. Deletion analysesof the leader RNA mapped the PTB-binding site to the UCUAA pentanucleotiderepeats. Using a defective-interfering RNA reporter system, wehave further shown that the PTB-binding site in the leader RNAis critical for MHV RNA synthesis. This and our previous study(H.-P. Li, X. Zhang, R. Duncan, L. Comai, and M. M. C. Lai, Proc.Natl. Acad. Sci. USA 94:9544-9549, 1997) combined thus show thattwo cellular hnRNPs, PTB and hnRNP A1, bind to the transcription-regulatorysequences of MHV RNA and may participate in itstranscription.

	TEXT

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Mouse hepatitis virus (MHV) is a single-stranded, positive-sense RNA virus and belongs to the Coronaviridae family. MHV containsan RNA genome of approximately 31 kb (22), which encodes sevento eight viral genes. MHV synthesizes six to seven subgenomicmRNAs, all of which share 5' and 3' ends identical to those ofthe genomic RNA (18). The common 5' end, termed leader sequence(72 to 77 nucleotides [nt] long), is derived from the 5' end ofthe genomic RNA (20, 38). The 3' end of the leader RNA containsa consensus UCUAA repeat sequence (30), and the copy numberof UCUAA repeats varies among different MHV strains. Another consensussequence, UCUAAAC or a similar sequence, termed intergenic (IG)sequence, is present between each viral gene (5). The IG sequence,which is homologous to the UCUAA repeat of the leader RNA, servesas the initiation site for subgenomic mRNA synthesis (14, 29).Each of the seven subgenomic mRNAs starts from a different IGsite and extends to the 3' end of the genome; thus, the subgenomicmRNAs have a 3'-coterminal, nested-set structure (17, 23).Furthermore, the subgenomic mRNA synthesis involves fusion oftwo stretches of noncontiguous sequence by a discontinuous-transcriptionmechanism, such that the leader RNA is joined to the 5' end ofeach mRNA (13, 25, 43). This fusion occurs between the UCUAArepeats of the leader and the consensus IG sequence. Based onthis unique subgenomic mRNA structure, several models have beenproposed to explain the discontinuous nature of coronavirus RNAtranscription (16, 18, 35). All of these models requirethat the leader sequence interact with the IG sequence in theminus-strand template RNA or plus-strand genomic RNA. Such aninteraction has been inferred from the findings that the efficiencyof mRNA transcription is affected by different combinations ofthe leader and IG sequences, particularly in the region of UCUAArepeats (21, 36, 43). Interestingly, this interaction appearsto occur between the leader and IG sequences in two differentRNA molecules (in trans) as well as within the same RNA molecule(in cis) (43). Furthermore, the 3'-end sequence of MHV RNA isrequired for viral mRNA transcription (26), suggesting thatthe 3' untranslated region (UTR) of viral RNA may also interactwith the upstream transcription-regulatory sequences. Since sequencecomplementarity is not always present in these interacting RNAregions, these interactions may be mediated by protein-RNA andprotein-protein interactions, involving either viral or cellularproteins (19, 42).

By UV cross-linking assays, several cellular proteins have been detected to bind specifically to the transcription-regulatoryregions of MHV RNA (7, 27, 41, 44). Among these proteins,p35/38 binds to the minus-strand leader RNA and minus-strand IGsequences (7, 44), while another protein, p55, binds to theplus-strand leader RNA (7). The binding of p35/38 to the minus-strandIG sequence correlates with the efficiency of subgenomic mRNAtranscription (44), suggesting that p35/38 may act as a transcriptionfactor. Recently, this protein has been identified as heterogeneousnuclear ribonucleoprotein (hnRNP) A1 (24), a nuclear proteininvolved in the alternative splicing of cellular RNAs (6).It is hypothesized that the binding of hnRNP A1 to both the leaderand IG sequences on the minus-strand template may bring thesetwo distant RNA domains together and facilitate the formationof either an MHV-specific RNA transcription complex or an MHVRNA processing (splicing)complex.

Since plus-strand leader RNA interacts with the template RNA during MHV RNA transcription, p55 may serve as a mediator ofthis interaction. Therefore, we are interested in understandingthe nature of this protein. In this report, we identified thep55 as polypyrimidine tract-binding protein (PTB), also knownas hnRNP I. This protein has previously been shown to interactwith hnRNP A1 in a pre-mRNA splicing complex in normal cells (3).Thus, the binding of hnRNP A1 and PTB to the minus-strand leaderand IG site and the plus-strand leader RNA, respectively, maybring together these RNAs, fulfilling a requirement for MHV RNAtranscription.

Purification of MHV plus-strand leader RNA-binding protein p55. Although p55 was originally found in the cytoplasm of a murine cell line (DBT) (12), a similar protein was detected in boththe nuclear and the cytoplasmic fractions of HeLa cells (datanot shown). Therefore, HeLa cell lysates were used for proteinpurification according to the previously published procedures(24). After three steps of purification (ammonium sulfate precipitationand Q-Sepharose and heparin agarose chromatography), partiallypurified proteins were UV cross-linked to ³²P-labeled plus-strand leader RNA, 182(+) RNA (7), representingthe 5'-end 182 nt of viral genomic RNA, as previously described(24). The RNA-protein complex was digested with RNase A andanalyzed by nonequilibrium two-dimensional (2-D) gel electrophoresisaccording to the procedure of O'Farrell et al. (31). The silver-stainedprotein profile of the 2-D gel (Fig. 1A) was then compared withthe autoradiogram of the UV cross-linked ³²P-labeled proteins (Fig. 1B). Two streaks of radiolabeled spotsranging from 55 to 57 kDa, each with a correspondingly decreasingisoelectric point (pI) that represents different numbers of nucleotideslinking to the same protein (24), were detected on the autoradiogram(Fig. 1B). Since nucleotide attachment to a protein will increasethe molecular weight and correspondingly lower the pI value ofthe protein, the radiolabeled spot with the lowest molecular weightand the highest pI (indicated by two arrows; Fig. 1B) representsthe minimally cross-linked protein, which corresponded to spotno. 1 and spot no. 4 identified on the silver-stained gel (Fig.1A). These two spots, thus, are the most likely candidates forp55. Four other protein spots, no. 2, 3, 5, and 6 (Fig. 1A), arein close proximity to spot no. 1 and no. 4 and have the same molecularweights; they may represent isoforms of p55. Because these sixprotein spots were not well separated, they were collected astwo groups: p55a (spot no. 1 to 3) and p55b (spot no. 4 to 6).Each of these six protein spots has a pI value close to that ofthe translation factor eEF-1 $alpha$ (50 kDa, pI 9.5) (4) (Fig. 1A),and all were detected in both cytoplasmic and nuclear fractions(data not shown). Another streak of radiolabeled protein representsp70 (44). The identity of this protein was not further pursuedin this study.

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FIG. 1. 2-D PAGE analysis of the partially purified proteins from HeLa cytoplasmic extracts. HeLa cytoplasmic extract was separated by ammonium sulfate precipitation and Q-Sepharose and heparin agarose chromatography. The partially purified proteins were UV cross-linked to ³²P-labeled plus-strand leader [5'-182(+)] RNA and separated by 2-D nonequilibrium pH gradient gel electrophoresis according to the procedures of O'Farrell et al. (31), by using Ampholine pH 3 to 10 (Bio-Rad) and pH 7 to 9 (Pharmacia) at a 1:1 ratio and separation for 5 h at 650 V for the first dimension. The second dimension was performed by SDS-PAGE on 10% polyacrylamide gels. (A) Silver-stained gel. p55 (spots 1 to 6) and molecular mass markers in kilodaltons are indicated, and eEF-1 $alpha$ is identified. (B) Autoradiogram of the same gel as in panel A. The two arrows indicate the radiolabeled spots that match spots no. 1 and no. 4 in the silver-stained gel.

Identification of p55 as PTB or hnRNP I. The identity of p55a and p55b was determined by partial peptide sequencing and amino acid composition analysis (performedby W. M. Keck Foundation Biotechnology Resource Laboratory ofYale University). The high-pressure liquid chromatography patternsof the tryptic peptides of p55a and p55b were very similar (datanot shown), suggesting that they were related proteins. One trypticpeptide from p55a, which was shared with p55b, was selected forpeptide sequencing. The sequence of this peptide, DYGNSPLHR, matchedthe C-terminal sequence (amino acid 429 to 437) of a human PTB,also known as hnRNP I. Upon further analysis, the high-pressureliquid chromatography profiles of tryptic peptides of p55a andp55b were found to be similar to that of PTB (data not shown),further indicating the identity of p55 as PTB. PTB has been reportedto consist of at least four isoforms (9, 10, 32), due toalternative splicing, and their molecular masses range from 57to 62 kDa, and their pI range from 8.0 to 8.5 (6). The p55(PTB) protein pattern in the silver-stained 2-D gel (Fig. 1A)was also similar to that of the immunopurified hnRNP I complex(9). The amino acid sequence of human PTB shows greater than97% identity to its murine counterpart (3).

The identity of p55 as PTB was then tested by immunoprecipitation studies of UV cross-linked protein with a monoclonal antibodyspecific for human PTB (kindly provided by E. Wimmer, State Universityof New York, Stony Brook). The cytoplasmic extracts from HeLaand DBT cells were UV cross-linked with the MHV plus-strand leaderRNA, and the RNA-protein complex was immunoprecipitated with antibodiesagainst several different nuclear proteins (PTB, TFIIB, and Sam68).Only the PTB-specific monoclonal antibody (Fig. 2, lanes 2 and6), and not the other two antibodies (Fig. 2, lanes 3, 4, 7, and8), could precipitate the UV cross-linked p55 from both HeLa andDBT cells. These data established that the MHV plus-strand leaderRNA-binding protein (p55) is PTB.

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FIG. 2. Immunoprecipitation of UV cross-linked proteins. Cytoplasmic extracts from HeLa (lanes 1 to 4) and DBT (lanes 5 to 8) cells were UV cross-linked with ³²P-labeled plus-strand leader RNA; digested with RNase A; and precipitated with monoclonal antibody for PTB (lanes 2 and 6), monoclonal antibody for TFIIB (lanes 3 and 7), or polyclonal antibody for Sam68 (Santa Cruz Biotechnology) (lanes 4 and 8). The precipitated proteins were collected with protein A-Sepharose beads (Zymed) and analyzed by SDS-PAGE. Lanes 1 and 5 are UV cross-linked proteins without immunoprecipitation (IP). Numbers at left show molecular mass in kilodaltons.

RNA-binding property of the recombinant murine PTB (GST-PTB). To further confirm that PTB is the protein that binds to the plus-strand MHV 5' UTR, a recombinant glutathione S-transferase(GST)-fused murine PTB (GST-PTB) was prepared and used for UVcross-linking to the ³²P-labeled 182-nt plus-strand 5' UTR. The results showed that thepurified GST-PTB fusion protein (Fig. 3B, lane 1) bound to thisRNA (Fig. 3A, lane 3), whereas the purified GST protein (Fig.3B, lane 2) did not bind the same RNA (Fig. 3A, lane 4). The bindingof GST-PTB to the ³²P-labeled 5'-end leader RNA [5'-182(+)] could be competed completelyby a 10-fold excess of the cold homologous RNA but not by otherRNAs, such as 3' end of MHV RNA [3'-350(+)] or tRNA (Fig. 3C).These results indicate that PTB is indeed the protein that bindsspecifically to the 5'-end leader RNA.

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FIG. 3. UV cross-linking analysis of recombinant PTB. Plasmid pGEX-4T-1/PTB, which expresses a GST-murine PTB fusion protein, was constructed by subcloning a reverse-transcribed PCR-synthesized cDNA fragment (1,587 bp), containing the entire open reading frame of murine PTB (GenBank/EMBL data bank with accession no. X52101 [3]), made from the RNA of DBT cells. The expression of GST fusion protein in Escherichia coli was induced by addition of 0.2 mM isopropyl-1-thio- $beta$ -D-galactoside (IPTG) for 3 to 5 h at 37°C. GST fusion protein was purified from bacterial lysates with glutathione-Sepharose 4B beads (Pharmacia). (A) Purified recombinant PTB (GST-PTB) (lane 3) and GST (lane 4) were UV cross-linked with ³²P-labeled plus-strand leader RNA and separated by SDS-PAGE. Cytoplasmic extracts from HeLa (lane 1) and DBT (lane 2) cells cross-linked to the same RNA were included as controls. (B) Coomassie blue-stained gel of the purified GST-PTB (lane 1) and GST (lane 2). (C) Competition analysis of GST-PTB binding to 5'-182(+) RNA. The purified GST-PTB was first incubated with increasing concentrations of unlabeled RNAs (cold competitors, 2.5×, 5×, or 10× molar excess over the labeled RNA) and then with ³²P-labeled 5'-182(+) RNA. The UV cross-linked proteins were separated by SDS-PAGE. Numbers to the left of panels A and B show molecular mass in kilodaltons.

Mapping of the PTB-binding site on the plus-strand MHV 5' UTR. To locate the binding site of PTB on the MHV plus-strand 5' UTR, various truncated, ³²P-labeled RNAs of this region (Fig. 4A) were UV cross-linked toHeLa cell extract, followed by RNase A digestion and sodium dodecylsulfate-polyacrylamide gel electrophoresis (SDS-PAGE). Figure4B shows that the amounts of PTB bound to 182(+) (lane 1, 100%)and 112(+) (lane 2, 70%) RNAs were comparable but that the amountof its binding to RNA 56(+) (lane 3) was significantly lower (19%).No PTB was found to bind RNA 35(+) (lane 4). As expected, PTBdid not bind to the minus-strand, 182-nt RNA (lane 5), furtherconfirming that PTB binds specifically to plus-strand 5' UTR.These data indicated that nt 56 to 112 of the plus-strand leaderRNA are the sequence most critical for the binding of PTB. Withinthis region, there is a stretch of four UCUAA repeats (nt 60 to80 from the 5' end), which has been demonstrated to be importantfor the MHV transcription (2, 21, 37, 43). The regionbetween nt 35 and 56 from the 5' end may also contribute to PTBbinding to some extent since 56(+) RNA bound PTB weakly; thisregion includes part of the UCUAA repeat sequence and has twosequences similar to UCUU, which has been reported to be one ofthe PTB-binding consensus sequences (33). However, the extentof PTB binding to this region was variable. In some experiments,very little PTB binding was detected (see below) (Fig. 4C). Thus,PTB binding to nt 35 to 56 was very weak at best. Therefore, themajor PTB-binding site is within nt 56 to 112 from the 5' end.There was a slight difference in PTB binding between the 182(+)and 112(+) RNAs, suggesting that the extent of PTB binding tont 56 to 112 may be affected by other RNA sequences or overallRNA conformation.

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FIG. 4. Mapping of PTB-binding sites on the MHV 5'-UTR RNA. (A) Schematic diagrams of the structure of plasmids and their transcribed RNAs used in this study. The unfilled box represents the MHV 5' UTR, and shaded boxes indicate the four UCUAA repeats in the RNA. Vertical arrows represent the enzyme sites for linearizing the plasmids. The numbers under the boxes denote nucleotide numbers from the 5' end of the MHV RNA. Horizontal arrows represent the in vitro transcribed RNAs. The open arrows represent T7 and T3 RNA polymerase promoters. The RNA *35 (+) was transcribed from synthetic DNA oligomers containing the T7 promoter. pNX1 $Delta$ 4R is identical to pNX1 but lacks the four UCUAA repeats. (B) UV cross-linking of HeLa cytoplasmic extracts with various 5'-end RNAs. The amounts of PTB binding were quantitated by using the Ambis Radioanalytic Imaging System. (C) UV cross-linking of 5'-UTR RNA with or without the UCUAA repeat. Cytoplasmic extracts from HeLa (lanes 1 and 4), DBT (lanes 2 and 5), and A59-infected DBT (lanes 3 and 6) cells were used. (D) UV cross-linking of GST-PTB with 5'-182(+) and 5'-182 $Delta$ 4R(+) RNAs. H/C and D/C represent cytoplasmic extracts of HeLa and DBT cells, respectively. Numbers at left of panels B and C show molecular mass in kilodaltons.

To investigate whether the UCUAA pentanucleotide repeat sequence in the leader RNA was responsible for the PTB binding, amutant 5'-UTR RNA, 182 $Delta$ 4R(+), in which the four UCUAA repeatshave been deleted (Fig. 4A), was used to perform a UV cross-linkingassay. The results showed that this mutant leader RNA bound verylittle PTB from the lysates of uninfected or MHV-A59-infectedHeLa or DBT cells (Fig. 4C, lanes 4 to 6). This was significantlyless than that bound to the wild-type leader RNA (lanes 1 to 3).Similarly, GST-PTB also bound strongly to 182(+) RNA but onlyweakly to 182 $Delta$ 4R(+) RNA (Fig. 4D). These results combined thusindicate that the UCUAA repeat sequence is most crucial for PTBbinding.

The PTB-binding site is crucial for the viral subgenomic mRNA transcription. Previous studies have shown that the number of the UCUAA repeats at the 3' end of the leader sequence determines the efficiencyof transcription of viral subgenomic mRNAs in both a trans- anda cis-acting manner (21, 40, 43). Since PTB binds to thisUCUAA region, we asked whether the elimination of this PTB-bindingsite would affect the transcription of MHV subgenomic mRNA. Weconstructed a variant of defective-interfering (DI) RNA reportervector p25- $Delta$ 4R-CAT, in which the four UCUAA repeats in the leadersequence were deleted but which contains a chloramphenicol acetyltransferase(CAT) reporter gene placed behind an IG sequence (25) (Fig.5). Previous studies have shown that the CAT activity detectedfrom this DI RNA in the presence of a helper virus reflects mRNAtranscription from the IG site (25, 44). Various DI RNAs,including p25CAT (with the wild-type leader), p25- $Delta$ 4R-CAT (witha mutant leader), and p25CAT/RIS (without the IG site) (Fig. 5),were transfected into A59-infected DBT cells at 1 h postinfection.Cell lysates were collected at 9 h postinfection for CAT assay.The results indicated that the CAT activity expressed by p25- $Delta$ 4R-CATwas approximately 15% of that of the wild-type DI vector, whereasthe RNA without the IG sequence (p25CAT/RIS) was totally devoidof the CAT activity (data not shown). These results are consistentwith the previous reports that the UCUAA repeat sequence in theleader RNA modulates mRNA transcription in cis and in trans (25,43). Since PTB binds to this repeat sequence, PTB may play arole in this regulation.

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FIG. 5. Structure of various DI RNAs. 25CAT RNA (25) contains a wild-type leader RNA sequence; 25- $Delta$ 4R-CAT contains a mutant leader RNA without the four UCUAA repeats. IG 7 is the promoter sequence for gene 7; 25CAT/RIS is similar to 25 CAT but lacks the IG site (25). The plasmids for these RNAs were made by PCR amplification of p25CAT with appropriate primers.

The results presented here have demonstrated that PTB binds to the MHV leader RNA at the UCUAA repeat region. This UCUAA repeatis the site where the leader RNA interacts with the IG sequenceson the template RNA in both a trans- and a cis-acting manner andwhere the leader joins subgenomic mRNAs (43). The deletion ofthe UCUAA repeat sequence resulted in the loss of PTB bindingand the corresponding reduction of mRNA transcription from a downstreamIG site. This finding further confirmed that the leader sequencehas a cis-acting effect on subgenomic mRNA transcription (43)and that the UCUAA sequence plays an important role in mRNA initiation.Conceivably, the effect of the UCUAA repeats on transcriptionis mediated throughPTB.

PTB is predominantly a nuclear protein, particularly localized in a discrete perinucleolar structure (9). It contains fourrepeated domains, each of which consists of 80 amino acids, constitutingRNA-binding domains (9). Therefore, one molecule of PTB canpotentially interact with several different RNA regions. PTB bindspreferentially to the polypyrimidine tract of pre-mRNAs, nearthe 3' splice site, and is involved in alternative RNA splicingand RNA transport in normal cells (8-10, 32, 33). In addition,PTB has been shown to regulate translation of some viral RNAs(1, 11, 15) and cap-independent cellular mRNAs (28).So far, we have identified two cellular proteins, hnRNP A1 (24)and PTB, which bind to several different regions of MHV RNA. hnRNPA1 binds to minus-strand leader sequence and the IG site, whereasPTB binds to plus-strand leader. Previous studies have suggestedthat these three regions may interact with each other to regulatemRNA transcription (19). It is conceivable that these interactionsare mediated through hnRNP A1 and PTB by protein-RNA and protein-proteininteractions. Our preliminary data have, indeed, shown that minus-strandleader sequence and the IG site can interact with each other throughhnRNP A1 (45). Furthermore, PTB and hnRNP A1 have been shownto interact with each other in spliceosome complexes in normalcells (3). Therefore, once PTB and hnRNP A1 bind to plus-strandleader RNA and minus-strand IG and leader sequences, respectively,these two proteins may bring together these RNAs to form a ribonucleoproteincomplex.

One intriguing feature about these proteins is that both hnRNP A1 and PTB are primarily nuclear proteins (6, 8, 9,32); yet, coronavirus replicates in the cytoplasm. However,both hnRNP A1 and PTB are shuttled between the nucleus and cytoplasmin normal cells (11, 34), and all proteins are synthesizedin the cytoplasm. These cytoplasmic proteins, hnRNP A1 and PTB,have been shown to promote translation in normal cells by facilitatingribosome binding via a 5'-end, cap-mediated mechanism (39).We have previously found that hnRNP A1 is translocated from thenucleus to the cytoplasm in MHV-infected cells (24). However,there is only a marginal increase in the amount of PTB in thecytoplasm of MHV-infected cells (unpublished observation). Nevertheless,since PTB participates in the regulation of mRNA translation innormal cells, sufficient PTB may be present in the cytoplasm ofMHV-infected cells to allow its participation in MHV RNA transcription.The functional role of the cytoplasmic PTB in normal and MHV-infectedcells should be of greatinterest.

	ACKNOWLEDGMENTS

We thank Daphne Shimoda for assistance in preparing themanuscript.

This study was supported by grant 19244 from the National Institutes of Health. M. M. C. Lai is an Investigator of the HowardHughes MedicalInstitute.

	FOOTNOTES

^* Corresponding author. Mailing address: Howard Hughes Medical Institute, Department of Molecular Microbiology and Immunology,University of Southern California School of Medicine, 2011 ZonalAve., HMR-401, Los Angeles, CA 90033-1054. Phone: (323) 442-1748.Fax: (323) 442-9555. E-mail: michlai{at}hsc.usc.edu.

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26. Lin, Y.-J., X. Zhang, R. C. Wu, and M. M. C. Lai. 1996. The 3' untranslated region of coronavirus RNA is required for subgenomic mRNA transcription from a defective interfering RNA. J. Virol. 70:7236-7240[Abstract/Free Full Text].

27. Liu, Q., W. Yu, and J. L. Leibowitz. 1997. A specific host cellular protein binding element near the 3' end of mouse hepatitis virus genomic RNA. Virology 232:74-85[Medline].

28. 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].

29. Makino, S., M. Joo, and J. K. Makino. 1991. A system for study of coronavirus mRNA synthesis: a regulated, expressed subgenomic defective-interfering RNA results from intergenic site insertion. J. Virol. 65:6031-6041[Abstract/Free Full Text].

30. Makino, S., and M. M.-C. Lai. 1989. Evolution of the 5'-end of genomic RNA of murine coronaviruses during passages in vitro. Virology 169:227-232[Medline].

31. O'Farrell, P. Z., H. M. Goodman, and P. H. O'Farrell. 1977. High resolution two-dimensional gel electrophoresis of basic as well as acidic proteins. Cell 12:1133-1142[Medline].

32. Patton, J. G., S. A. Mayer, P. Tempst, and B. Nadal-Ginard. 1991. Characterization and molecular cloning of polypyrimidine tract-binding protein: a component of a complex necessary for pre-mRNA splicing. Genes Dev. 5:1237-1251[Abstract/Free Full Text].

33. Perez, I., C. H. Lin, J. G. McAfee, and J. G. Patton. 1997. Mutation of PTB binding sites causes misregulation of alternative 3' splice site selection in vivo. RNA 3:764-778[Abstract].

34. Piñol-Roma, S., and G. Dreyfuss. 1992. Shuttling of pre-mRNA binding proteins between nucleus and cytoplasm. Nature 355:730-732[Medline].

35. Sawicki, S. G., and D. L. Sawicki. 1990. Coronavirus transcription: subgenomic mouse hepatitis virus replicative intermediates function in RNA synthesis. J. Virol. 64:1050-1056[Abstract/Free Full Text].

36. Shieh, C.-K., H. J. Lee, K. Yokomori, N. La Monica, S. Makino, and M. M. C. Lai. 1989. Identification of a new transcriptional initiation site and the corresponding functional gene 2b in the murine coronavirus RNA genome. J. Virol. 63:3729-3736[Abstract/Free Full Text].

37. Shieh, C.-K., L. H. Soe, S. Makino, M.-F. Chang, S. A. Stohlman, and M. M. C. Lai. 1987. The 5'-end sequence of the murine coronavirus genome: implications for multiple fusion sites in leader-primed transcription. Virology 156:321-330[Medline].

38. Spaan, W., H. Delius, M. Skinner, J. Armstrong, P. Rottier, S. Smeekens, B. A. M. van der Zeijst, and S. G. Siddell. 1983. Coronavirus mRNA synthesis involves fusion of non-contiguous sequences. EMBO J. 2:1839-1844[Medline].

39. Svitkin, Y. V., L. P. Ovchinnikov, G. Dreyfuss, and N. Sonenberg. 1996. General RNA binding proteins render translation cap dependent. EMBO J. 15:7147-7155[Medline].

40. Yokomori, K., L. R. Banner, and M. M. C. Lai. 1991. Heterogeneity of gene expression of hemagglutinin-esterase (HE) protein of murine coronaviruses. Virology 183:647-657[Medline].

41. Yu, W., and J. L. Leibowitz. 1995. A conserved motif at the 3' end of mouse hepatitis virus genomic RNA required for host protein binding and viral RNA replication. Virology 214:128-138[Medline].

42. Zhang, X., and M. M. C. Lai. 1994. Unusual heterogeneity of leader-mRNA fusion in a murine coronavirus: implications for the mechanism of RNA transcription and recombination. J. Virol. 68:6626-6633[Abstract/Free Full Text].

43. Zhang, X., C.-L. Liao, and M. M. C. Lai. 1994. Coronavirus leader RNA regulates and initiates subgenomic mRNA transcription, both in trans and in cis. J. Virol. 68:4738-4746[Abstract/Free Full Text].

44. Zhang, X., and M. M. C. Lai. 1995. Interactions between the cytoplasmic proteins and the intergenic (promoter) sequence of mouse hepatitis virus RNA: correlation with the amounts of subgenomic mRNA transcribed. J. Virol. 69:1637-1644[Abstract].

45. Zhang, X., H.-P. Li, W.-M. Xue, and M. M. C. Lai. Unpublished observation.

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Clin. Vaccine Immunol.	ALL ASM JOURNALS

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20.	Lai, M. M. C., C. D. Patton, R. S. Baric, and S. A. Stohlman. 1983. The presence of leader sequences in the mRNA of mouse hepatitis virus. J. Virol. 46:1027-1033[Abstract/Free Full Text].
21.	La Monica, N., K. Yokomori, and M. M. C. Lai. 1992. Coronavirus mRNA synthesis: identification of novel transcription initiation signals which are differentially regulated by different leader sequences. Virology 188:402-407[Medline].
22.	Lee, H.-J., C.-K. Shieh, A. E. Gorbalenya, E. V. Koonin, N. La Monica, J. Tuler, A. Bagdzhadzhyan, and M. M.-C. Lai. 1991. The complete sequence (22 kilobases) of murine coronavirus gene 1 encoding the putative proteases and RNA polymerase. Virology 180:567-582[Medline].
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24.	Li, H.-P., X. Zhang, R. Duncan, L. Comai, and M. M. C. Lai. 1997. Heterogeneous nuclear ribonucleoprotein A1 binds to the transcription-regulatory region of mouse hepatitis virus RNA. Proc. Natl. Acad. Sci. USA 94:9544-9549[Abstract/Free Full Text].
25.	Liao, C.-L., and M. M. C. Lai. 1994. Requirement of the 5' end genomic sequence as an upstream cis-acting element for coronavirus subgenomic mRNA transcription. J. Virol. 68:4727-4737[Abstract/Free Full Text].
26.	Lin, Y.-J., X. Zhang, R. C. Wu, and M. M. C. Lai. 1996. The 3' untranslated region of coronavirus RNA is required for subgenomic mRNA transcription from a defective interfering RNA. J. Virol. 70:7236-7240[Abstract/Free Full Text].
27.	Liu, Q., W. Yu, and J. L. Leibowitz. 1997. A specific host cellular protein binding element near the 3' end of mouse hepatitis virus genomic RNA. Virology 232:74-85[Medline].
28.	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].
29.	Makino, S., M. Joo, and J. K. Makino. 1991. A system for study of coronavirus mRNA synthesis: a regulated, expressed subgenomic defective-interfering RNA results from intergenic site insertion. J. Virol. 65:6031-6041[Abstract/Free Full Text].
30.	Makino, S., and M. M.-C. Lai. 1989. Evolution of the 5'-end of genomic RNA of murine coronaviruses during passages in vitro. Virology 169:227-232[Medline].
31.	O'Farrell, P. Z., H. M. Goodman, and P. H. O'Farrell. 1977. High resolution two-dimensional gel electrophoresis of basic as well as acidic proteins. Cell 12:1133-1142[Medline].
32.	Patton, J. G., S. A. Mayer, P. Tempst, and B. Nadal-Ginard. 1991. Characterization and molecular cloning of polypyrimidine tract-binding protein: a component of a complex necessary for pre-mRNA splicing. Genes Dev. 5:1237-1251[Abstract/Free Full Text].
33.	Perez, I., C. H. Lin, J. G. McAfee, and J. G. Patton. 1997. Mutation of PTB binding sites causes misregulation of alternative 3' splice site selection in vivo. RNA 3:764-778[Abstract].
34.	Piñol-Roma, S., and G. Dreyfuss. 1992. Shuttling of pre-mRNA binding proteins between nucleus and cytoplasm. Nature 355:730-732[Medline].
35.	Sawicki, S. G., and D. L. Sawicki. 1990. Coronavirus transcription: subgenomic mouse hepatitis virus replicative intermediates function in RNA synthesis. J. Virol. 64:1050-1056[Abstract/Free Full Text].
36.	Shieh, C.-K., H. J. Lee, K. Yokomori, N. La Monica, S. Makino, and M. M. C. Lai. 1989. Identification of a new transcriptional initiation site and the corresponding functional gene 2b in the murine coronavirus RNA genome. J. Virol. 63:3729-3736[Abstract/Free Full Text].
37.	Shieh, C.-K., L. H. Soe, S. Makino, M.-F. Chang, S. A. Stohlman, and M. M. C. Lai. 1987. The 5'-end sequence of the murine coronavirus genome: implications for multiple fusion sites in leader-primed transcription. Virology 156:321-330[Medline].
38.	Spaan, W., H. Delius, M. Skinner, J. Armstrong, P. Rottier, S. Smeekens, B. A. M. van der Zeijst, and S. G. Siddell. 1983. Coronavirus mRNA synthesis involves fusion of non-contiguous sequences. EMBO J. 2:1839-1844[Medline].
39.	Svitkin, Y. V., L. P. Ovchinnikov, G. Dreyfuss, and N. Sonenberg. 1996. General RNA binding proteins render translation cap dependent. EMBO J. 15:7147-7155[Medline].
40.	Yokomori, K., L. R. Banner, and M. M. C. Lai. 1991. Heterogeneity of gene expression of hemagglutinin-esterase (HE) protein of murine coronaviruses. Virology 183:647-657[Medline].
41.	Yu, W., and J. L. Leibowitz. 1995. A conserved motif at the 3' end of mouse hepatitis virus genomic RNA required for host protein binding and viral RNA replication. Virology 214:128-138[Medline].
42.	Zhang, X., and M. M. C. Lai. 1994. Unusual heterogeneity of leader-mRNA fusion in a murine coronavirus: implications for the mechanism of RNA transcription and recombination. J. Virol. 68:6626-6633[Abstract/Free Full Text].
43.	Zhang, X., C.-L. Liao, and M. M. C. Lai. 1994. Coronavirus leader RNA regulates and initiates subgenomic mRNA transcription, both in trans and in cis. J. Virol. 68:4738-4746[Abstract/Free Full Text].
44.	Zhang, X., and M. M. C. Lai. 1995. Interactions between the cytoplasmic proteins and the intergenic (promoter) sequence of mouse hepatitis virus RNA: correlation with the amounts of subgenomic mRNA transcribed. J. Virol. 69:1637-1644[Abstract].
45.	Zhang, X., H.-P. Li, W.-M. Xue, and M. M. C. Lai. Unpublished observation.