Overexpression of Essential Splicing Factor ASF/SF2 Blocks the Temporal Shift in Adenovirus Pre-mRNA Splicing and Reduces Virus Progeny Formation

doi:10.1128/JVI.74.19.9002-9009.2000

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Journal of Virology, October 2000, p. 9002-9009, Vol. 74, No. 19
0022-538X/00/$04.00+0
Copyright © 2000, American Society for Microbiology. All rights reserved.

Overexpression of Essential Splicing Factor ASF/SF2 Blocks the Temporal Shift in Adenovirus Pre-mRNA Splicing and Reduces Virus Progeny Formation

Magnus Molin and Göran Akusjärvi^*

Department of Medical Biochemistry and Microbiology, BMC, Uppsala University, SE-751 23 Uppsala, Sweden

Received 30 March 2000/Accepted 14 July 2000

	ABSTRACT

Top Abstract Introduction Materials and Methods Results Discussion References

Expression of cytoplasmic mRNA from most adenovirus transcription units is subjected to a temporal regulation at the levelof alternative pre-mRNA splicing. The general tendency is thatsplice site selection changes from proximal to distal late afterinfection. Interestingly, ASF/SF2, which is a prototypical memberof the SR family of splicing factors, has the opposite effecton splice site selection, inducing an increase in proximal splicesite usage. We have previously shown that SR proteins late duringan adenovirus infection become partially inactivated as splicingregulatory proteins. A prediction from these results is that overexpressionof an SR protein, such as ASF/SF2, during virus growth will interferewith virus replication by disturbing the balance of functionaland nonfunctional ASF/SF2 in the infected cell. To test this hypothesis,we reconstructed a recombinant adenovirus expressing ASF/SF2 underthe transcriptional control of a regulated promoter. The resultsshow that, as predicted, induction of ASF/SF2 during lytic virusgrowth prevents the early to late shift in mRNA expression fromboth early (E1A and E1B) and late (L1) transcription units. Furthermore,ASF/SF2 overexpression blocks viral DNA replication and reducesselectively cytoplasmic accumulation of major late mRNA, resultingin a lower virus yield. Collectively, our results provide additionalsupport for the hypothesis that viral control of SR protein functionis important for the proper expression of viral proteins duringlytic virusgrowth.

	INTRODUCTION

Top Abstract Introduction Materials and Methods Results Discussion References

Adenovirus gene expression is to a large extent regulated at the level of pre-mRNA alternative splicing (reviewed in reference21). Thus, the majority of adenovirus transcription units producemultiple differently spliced cytoplasmic mRNAs. The productionof several mRNAs from each viral transcription unit increasesthe coding potential of the viral genome and, furthermore, enablesthe virus to control viral gene expression by regulating the specificityof RNA splicing. Importantly, the accumulation of alternativelyspliced mRNAs is subjected to a temporal regulation, with distinctmRNA species accumulating at different time points of infection(reviewed in reference 21).

Although the mechanism(s) responsible for this shift in RNA splice site choice is far from clear, a number of studies havesuggested that the cellular SR family of splicing factors playsa critical role in this regulation. SR proteins constitute a familyof splicing factors that are essential for generic pre-mRNA splicing(reviewed in references 12 and 28). They contain one or twoamino-terminal RNA binding domains and a characteristic carboxy-terminalRS domain consisting of repeats of serine/arginine dipeptidesof variable length, hence the name SR proteins. The RNA recognitionmotif determines the RNA binding specificity, whereas the RS domainfunctions as an effector domain mediating interaction with othersplicing factors (reviewed in references 12 and 28). SR proteinsparticipate at multiple steps during the initial stages of splicesite recognition. Most SR proteins interact with simple RNA elementscontaining a high content of purines (reviewed in reference 42)and have the capacity to enhance or repress splicing, dependingon the position of the RNA recognition motif in the pre-mRNA (22).SR proteins appear to serve the same function in spliceosome assemblyas regulatory transcription factors in preinitiation complex formationat a promoter (reviewed in reference 17). Importantly, SR proteinsare highly phosphorylated, primarily within the RS domain (9),a modification that is required for their function as initiatorsof spliceosome assembly (7, 47) and which controls theiractivity in alternative splicing (23). During splicing catalysis,SR proteins become dephosphorylated. Thus, cycles of SR proteinphosphorylation/dephosphorylation occur during spliceosome assemblyand pre-mRNA splicing in vitro (7, 31).

The adenovirus E1A and L1 pre-mRNAs have been subjected to the most thorough investigation (reviewed in reference 21). TheE1A pre-mRNA gives rise to three major mRNAs, the 13S, 12S, and9S mRNAs, by use of three alternative 5' splice sites which arespliced to a common 3' splice site (Fig. 1). The 13S mRNA is themost abundant E1A mRNA expressed at early times of infection,whereas the 9S mRNA becomes the predominant E1A mRNA expressedlate after infection. Different members of the SR protein familyhave been shown to have distinct effects on E1A pre-mRNA splicing.Thus, ASF/SF2 and SC35 activate 13S splicing, both in vitro (11,16, 48) and in transient transfection assays (6, 45).In contrast, SR protein p54 promotes selectively 9S splicing (49).Other SR proteins, e.g., SRp20, 9G8, SRp55, and SRp75, promote12S splicing (18, 37, 48). The early to late shift from13S to 9S mRNA splicing has been proposed to be triggered by atitration of functionally active SR proteins by high-molecular-weightadenovirus major late transcript, produced late after infection(13, 18, 25).

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FIG. 1. Schematic illustration showing the spliced structure of mRNAs expressed from regions E1A, E1B, E2A, L1, L2, and L4. For simplicity, the exon structures of mRNAs expressed from the major late transcription unit are shown as open boxes.

The adenovirus major late region 1 (L1) pre-mRNA produces two major mRNAs by alternative 3' splice site selection (reviewedin reference 21). Thus, a common 5' splice site is joined toeither of two alternative 3' splice sites (Fig. 1), resultingin the formation of the 52/55K mRNA (mRNA with an M_r of 52,000to 55,000) (proximal 3' splice site) or the IIIa mRNA (distal3' splice site). At early times of infection, the 52,55K mRNAis the exclusive L1 mRNA produced, whereas the IIIa mRNA becomesthe predominant L1 mRNA expressed at late times of infection.In contrast to E1A pre-mRNA splicing, L1 IIIa mRNA splicing issuppressed by SR proteins. Thus, all SR proteins tested exceptSRp20 (22, 36) inhibit IIIa splicing in vitro, with the SRp30fraction, which include ASF/SF2, being most effective. HeLa SRproteins block IIIa 3' splice site usage by binding to the intronicIIIa repressor element (3RE), located immediately upstream ofthe IIIa branch site (22). SR proteins binding to the 3RE suppressIIIa splicing by preventing U2 snRNP recruitment to the spliceosome.Activation of IIIa splicing, late after infection, has been shownto be accompanied by a virus-induced dephosphorylation of HeLaSR proteins (23). This modification reduces the RNA bindingcapacity of SR proteins and as a consequence relieves their repressionof IIIa 3' splice site usage, resulting in a shift toward an increasein IIIa mRNAproduction.

Collectively, the work on E1A and L1 alternative splicing has suggested that SR proteins play a critical role in the earlyto late shift in adenovirus pre-mRNA splicing. However, the conclusionsreached so far are based solely on in vitro splicing experimentsor transient transfection studies. Thus, the significance of SRproteins as regulators of viral pre-mRNA splicing during lyticvirus growth has not beentested.

Assuming that SR proteins are important regulatory factors controlling viral gene expression, one would predict that overexpressionof an SR protein during a lytic infection would have a significantimpact on viral mRNA expression by shifting the balance of functionaland nonfunctional SR proteins toward the active form and thereforeinterfere with viral multiplication. Here we test this hypothesisby constructing a recombinant adenovirus expressing the prototypicalSR protein ASF/SF2 under the inducible control of an RU 486-regulatedgene cassette (32). The results show that ASF/SF2 overexpressionblocks the early to late shift in viral mRNA expression. Thus,the early splice patterns of the E1A, E1B, and L1 mRNAs were retainedalso at late time points of infection. Furthermore, ASF/SF2 overexpressionreduced the efficiency of viral DNA replication, major late mRNAaccumulation, and new virus particle formation. Collectively,our data emphasize the significance of viral control of alternativeRNA splicing as a mean to regulate adenovirus gene expressionduring lytic virusgrowth.

	MATERIALS AND METHODS

Top Abstract Introduction Materials and Methods Results Discussion References

Construction of a recombinant adenovirus expressing ASF/SF2. Plasmid maps and sequences are available on request or online (http://www.bmc.uu.se/IMIM/res/GA.html). Transfer plasmid pAdG5Trip(His)-ASF/SF2was constructed by replacing the chloramphenicol acetyltransferase(CAT) gene in plasmid pAdG5Trip-CAT (32) with a synthetic double-strandedoligonucleotide encoding six histidines followed by a cDNA encodingthe human ASF/SF2 protein (taken from Prey-ASF [46]). PlasmidpAdG5Trip(His)-ASF/SF2 was reconstructed into a recombinant adenovirusessentially as described by Stow (39). Briefly, a vector armwas produced by double digestion of genomic adenovirus type 5(Ad5) dl309 DNA with XbaI and ClaI, followed by sucrose gradientpurification of the long right-hand genomic fragment (from 3.71to 100 map units [m.u.]). Recombinant viruses were generated byin vivo recombination. Thus, 5 µg of pAdG5Trip(His)-ASF/SF2 DNAwas mixed with 1 µg of Ad5 dl309 vector arm and cotransfectedby the calcium phosphate coprecipitation technique to 293 cells(14). Plaques typically appeared 5 to 6 days posttransfection.Recombinant viruses were verified by restriction enzyme cleavageof Hirt-extracted viral DNA (19). One plaque expressing His-ASF/SF2was selected and purified by a second round of plaque assay. Thefinal reporter virus was named AdG5(His)-ASF. The activator virusAdCMVProg has previously been described (32).

Purification of recombinant adenovirus. High-titer stock of recombinant virus was produced essentially as described elsewhere (20). Briefly, six 15-cm plates of293 cells were infected with recombinant virus. Three days postinfection,when a clear cytopathic effect was visible, cells were harvestedby low-speed centrifugation. The cell pellet was freeze-thawedonce and resuspended in 2 ml of 0.1 M Tris-HCl (pH 8.0) followedby lysis with 0.1 volume of 5% sodium deoxycholate on ice for30 min. Subsequently, the cell lysate was sonicated on ice. Viruswas purified by CsCl centrifugation. The virus band was collectedand dialyzed against 100 volumes of phosphate-buffered saline(PBS) containing 1 mM CaCl₂, 1 mM MgCl₂, and 10% glycerol, usinga Slide-A-Lyzer cassette (Pierce). Virus titer was determinedby plaque assay. Typical virus titers exceeded 10¹⁰ PFU/ml.

Infections. Virus stocks were diluted in 1 ml of Dulbecco modified Eagle medium (DMEM) supplemented with 2% newborn calf serum and usedto infect subconfluent 6-cm-diameter plates of 293 or HeLa cells(final concentration, 10 PFU/cell). In all experiments, 5 PFUof AdCMVProg and 5 PFU of AdG5(His)-ASF per cell were used. InFig. 6, 10 PFU of dl309 per cell was added to the activator-reportermix. Inoculum was removed after a 1-h incubation at 37°C, cellswere washed two times with fresh DMEM, and then 4 ml of DMEM supplementedwith 10% newborn calf serum with or without 0.5 µM RU 486 wasadded. Infected cells were harvested at different time pointsand used to prepare RNA, DNA, or proteinextracts.

Western blot analysis. Protein extracts were prepared at 12 to 24 h postinfection (hpi) by lysis of infected cells with radioimmunoprecipitationassay buffer (10 mM Tris buffer [pH 7.4], 150 mM NaCl, 1% NP-40,1% deoxycholate, 0.1% sodium dodecyl sulfate [SDS], 1 µg of aprotonin/ml,50 µg of phenylmethylsulfonyl fluoride/ml, 10 mM $beta$ -glycerophosphate).Extracts were subjected to SDS-polyacrylamide gel electrophoresis(PAGE) on a 15% gel and transferred to a nitrocellulose membrane.Filters were treated as previously described (36), and proteinswere visualized by chemiluminescence as instructed by the manufacturer(Amersham). His-ASF/SF2 was detected using a His₆ monoclonal antibody(Clontech), total ASF/SF2 was detected using a peptide antiserum(kind gift from J. Stevenin), and E2A-72K was detected with monoclonalantibody B610 (kindly provided by E. Bridge). In Fig. 2C, 2 µgof 293 cell extract, prepared at 18 hpi from AdG5(His)-ASF/AdCMVProg-infectedcells treated with RU 486, was incubated with 5 U of calf intestinalalkaline phosphatase (Fermentas) for 30 min at 30°C before separationby SDS-PAGE on a long 15% gel. His-ASF/SF2 was visualized by chemiluminescenceusing a His₆ monoclonal antibody(Clontech).

Northern blot analysis. Total cytoplasmic RNA was prepared by lysis with IsoB-NP-40 (10 mM Tris-HCl [pH 7.9], 150 mM NaCl, 1.5 mM MgCl₂, 1% NP-40),followed by two rounds of phenol-chloroform-isoamyl alcohol extractionand one extraction with chloroform-isoamyl alcohol (3). Twomicrograms of cytoplasmic RNA was separated on a 1% agarose gelcontaining 2.2 M formaldehyde, transferred to a nitrocellulosefilter, and hybridized with probe DNA ³²P labeled by random priming as previously described (3). TheDNA probes used were as follows: L1, SmaI-HindIII (36.3 to 37.9m.u.); L2, KpnI-SphI (42.8 to 49.5 m.u.); L4, SmaI-L (76.1 to76.7 m.u.); and E1B, BglII-SmaI (9.2 to 10.9 m.u.).

S1 protection assay. Ten micrograms of total cytoplasmic RNA prepared as described above was hybridized with an EcoRI/XbaI fragment 5'-end labeledat the XbaI site (41). Single-stranded RNA was digested withS1 nuclease, and RNA-DNA duplexes were separated on a nondenaturing1% agarose gel as previously described (41).

Dot blot analysis of viral DNA replication. Viral DNA was prepared from infected 293 cells by Hirt extraction (19). RNase-treated viral DNA was adjusted to 6× SSC (1×SSC is 0.15 M NaCl plus 0.015 M sodium citrate) and denaturedby boiling for 10 min. DNA was transferred to a nitrocellulosefilter using a vacuum device. The filter was subsequently incubatedfor 10 min on Whatman paper wetted with 1.5 M NaCl-0.5 M NaOH.The pH was neutralized by placing the filter on Whatman paperwetted with 1 M NaCl-0.5 M Tris (pH 7.0). The DNA was UV cross-linkedto the filter and hybridized with the Ad5 XhoI G fragment (27.0to 28.6 m.u.) ³²P labeled by random priming (3).

Titration of virus production. Infected 293 cells were collected 40 hpi by low-speed centrifugation, washed once with PBS, and then resuspended in PBS containing1 mM CaCl₂, 1 mM MgCl₂ and 10% glycerol. Cell suspensions werefreeze ( $-$ 70°C) thawed (37°C) three times. Serial dilutions offreeze-thawed extracts were used for infections of 293 cells.Plaques were counted 13 dayspostinfection.

³⁵S labeling of infected cells. Infected 293 cells were pulse-labeled with 100 µCi of ³⁵S-Promix (Amersham) for 2 h beginning at 16 or 22 hpi. Protein extractswere prepared by IsoB-1% NP-40 extraction, and 70-µg aliquotsof total proteins were separated by SDS-PAGE on a 10% gel, whichwas then subjected toautoradiography.

	RESULTS

Top Abstract Introduction Materials and Methods Results Discussion References

High ASF/SF2 expression using a recombinant adenovirus. To determine the effect of SR protein overexpression on virus multiplication, we constructed a recombinant adenovirus expressinga His-tagged ASF/SF2 protein under the transcriptional controlof a progesterone antagonist-induced promoter (32). The experimentalapproach is based on a double-infection strategy, where equalnumbers of PFU of an activator and a reporter virus are mixedand used for infection. Thus, activator virus, AdCMVProg (32),encoding a chimeric Gal4-VP16-progesterone transactivator proteinwas mixed with reporter virus, AdG5(His)-ASF, expressing His-ASF/SF2from a Gal4-regulated promoter. Transcription of the His-ASF/SF2gene was activated by addition of the progesterone antagonistRU 486 to the culturemedium.

As shown in Fig. 2A, His-ASF/SF2 expression is tightly regulated in HeLa cells with a high level of induced expression (lane3) and no detectable background (lane 2). Infection of 293 cellsresulted in an approximately 100-fold increase in His-ASF/SF2expression compared to HeLa cells (data not shown). The higherexpression level results from the fact that the E1-deleted viralvectors replicate in 293 cells. Importantly, infection of 293cells also results in a detectable background of His-ASF/SF2 inthe absence of inducer (Fig. 2A, lane 5). Thus, the fold inductionof His-ASF/SF2 is substantially lower in 293 cells than in HeLacells. Note that much less extract was analyzed in lanes 4 to6 (293 cells) than in lanes 1 to 3 (HeLa cells). This was donein order to show that the background expression of His-ASF/SF2in 293 cells was not due to the higher levels of expression obtainedin this cell line. The troublesome background expression of His-ASF/SF2in 293 cells appears to result, in part, from aberrant transcriptionactivation by the promiscuous E1A transactivator protein expressedin the 293 cell line (data not shown).

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FIG. 2. Western blot analysis of His-ASF/SF2 expression in AdG5(His)-ASF/AdCMVProg-infected HeLa and 293 cells. Fifty micrograms of protein from HeLa cells and 2 µg of protein from 293 cells were separated by SDS-PAGE on a 15% gel and probed with an anti-His monoclonal antibody (A) or ASF/SF2 peptide antiserum (B). His-ASF/SF2 was induced at the start of infection (A) or at 8 hpi (B), and cells were harvested at 18 (A) or 24 (B) hpi. Panel A shows a short exposure of His-ASF/SF2 expression in 293 cells, to enable comparison of the background expression of His-ASF/SF2 in the absence of added inducer in HeLa and 293 cells. (C) 293 cell protein extracts prepared from AdG5(His)- and ASF/AdCMVProg-infected cells at 18 hpi were treated with calf intestinal alkaline phosphatase (CIP), separated on a long SDS-polyacrylamide gel, and probed with an anti-His monoclonal antibody. Lanes 1 and 4, mock-infected cells.

Interestingly, probing a filter with a peptide antibody that recognizes both endogenously and exogenously expressed ASF/SF2shows that AdG5(His)-ASF overproduces His-ASF/SF2 more than 20-foldcompared to endogenous ASF/SF2 in 293 cells (Fig. 2B). In fact,at 24 hpi the His-ASF/SF2 protein constitutes as much as 2% oftotalproteins.

We have previously shown that SR proteins late during an adenovirus infection are hypophosphorylated (23). As shown in Fig.2C, separation of extracts prepared at 18 hpi on a long gel revealedthat His-ASF/SF2 overexpression resulted in the accumulation ofmultiple protein species (lane 2). Treatment of the sample withcalf intestinal alkaline phosphatase generated a single faster-migratingprotein species (lane 3), indicating that the slower-migratingHis-ASF/SF2 species vary in phosphorylatedstatus.

IIIa mRNA splicing is inhibited by ASF/SF2 overexpression. Since addition of an excess of ASF/SF2 blocks IIIa mRNA splicing in vitro (22), we predicted that His-ASF/SF2 overexpressionduring a lytic infection would block the early to late shift inL1 alternative splicing. As shown in Fig. 3A, addition of inducerfrom the start of infection resulted in a dramatic reduction inL1 mRNA accumulation compared to wild type (compare lanes 8 and9). In contrast, addition of inducer at the start of the latephase of infection (8 hpi) resulted in a less severe effect ontotal L1 mRNA accumulation (Fig. 3B, lanes 2 and 3). We interpretthese results to indicate that His-ASF/SF2 perturbation of earlyviral pre-mRNA splicing and protein synthesis causes a block inL1 mRNA accumulation (see below).

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FIG. 3. ASF/SF2 overexpression inhibits L1 mRNA production. Cytoplasmic RNA was prepared from AdG5(His)-ASF/AdCMVProg (A and B)- or AdG5Trip-CAT/AdCMVProg (C)-infected 293 cells at the indicated time points and separated on a 1% agarose gel containing 2.2 M formaldehyde. RNA was transferred to a nitrocellulose filter and hybridized with a ³²P-labeled probe specific for region L1. His-ASF/SF2 was induced from the start of infection (A and C) or at 8 hpi (B).

However, His-ASF/SF2 overexpression also blocked the temporal shift in L1 alternative splicing. Noteworthy, because of theleakiness of the viral vector system (see above), a substantialproduction of His-ASF/SF2 is also detectable in the absence ofinducer (Fig. 2A, lane 5). The effects on alternative RNA splicingare, in fact, best seen in the uninduced samples (Fig. 3A, lanes1, 4, and 7), with a stronger trend observed after induction (Fig.3A, lanes 2, 5, and 8). As predicted from our in vitro experiments(22, 23, 36), the relative expression of the IIIa mRNA comparedto the 52,55K mRNA was dramatically reduced in AdG5(His)-ASF-infectedcells compared to the wild type. Also, the i-leader, which isselectively retained on the 52,55K mRNA population expressed atearly and intermediate times of a wild-type infection (Fig. 3A,lane 3), is not efficiently spliced out in AdG5(His)-ASF-infectedcells. This results in an almost exclusive accumulation of the52,55K+i mRNA also at late times of infection (Fig. 3A, lanes7 and 8). Similarly, the small amounts of IIIa mRNA produced inthe recombinant virus-infected cells accumulate with approximatelyhalf of the population containing the i-leader (Fig. 3A, lanes4 and 7). The IIIa+i mRNA has previously been detected only underexperimental conditions where late viral protein synthesis wasstringently blocked with protein synthesis inhibitors (25).

Collectively, the observed effects of His-ASF/SF2 on the L1 mRNA profile are compatible with the known effects of ASF/SF2on splicing. Thus, ASF/SF2 has previously been shown to stimulateproximal splice site usage both in vitro and in transiently transfectedcells (4, 15, 24, 30, 38), here resulting in the formationof the 52,55K mRNA. ASF/SF2 also stimulates exon inclusion (6,27, 29), here resulting in the preferential accumulation ofL1 mRNAs containing the i-leader.

The effect of His-ASF/SF2 on L1 mRNA accumulation is specific and not a consequence of protein overexpression since AdG5TripCAT(32), overproducing the enzyme CAT, has an L1 phenotype almostidentical to that of the parental virus, dl309 (Fig. 3C).

The CAT enzyme serves as a good control for unspecific effects of protein overexpression on viral mRNA accumulation sinceCAT is of bacterial origin and therefore is not expected to interferewith regulatory circuits in human cells. Furthermore, CAT accumulatespredominantly in the nucleus in AdG5TripCAT-infected cells (datanot shown). A careful quantitation of His-ASF/SF2 and CAT expressionin recombinant virus-infected cells demonstrates that at 18 hpi,His-ASF/SF2 is expressed at approximately fivefold-higher levelscompared to CAT. The negative effects of His-ASF/SF2 expressionon L1 mRNA accumulation (Fig. 3A) could therefore result fromunspecific effects of the high levels of His-ASF/SF2 expression.However, the quantity of His-ASF/SF2 expression at 12 hpi is similarto the CAT expression level at 18 hpi (approximately 0.3 to 0.5%of total protein). Nevertheless, the L1 mRNA profile in CAT-expressingcells is essentially wild type (Fig. 3C), whereas L1 mRNA expressionis essentially abolished in His-ASF/SF2-expressing cells (Fig.3A, lane 2). Collectively, these results suggest that the negativeeffects of His-ASF/SF2 on major late mRNA accumulation are notunspecific.

Different effects of ASF/SF2 overproduction on major late region 2 and 4 mRNA accumulation. In our previous work we have used the L1 region as a model system to study the significance of SR proteins as regulators ofalternative RNA splicing. To determine if ASF/SF2 also affectsmRNA accumulation from other late mRNA families, we probed Northernblot filters with ³²P-labeled probes specific for the L2 and L4 families of mRNAs.As shown in Fig. 4, inducing His-ASF/SF2 expression from the startof infection resulted in dramatic decrease in the steady-statelevels of L2 and L4 mRNAs. Unlike L1 splicing, the spliced structureof the individual L2 mRNA species did not change significantly,suggesting that ASF/SF2 is not a critical factor regulating L2alternative splicing. The mRNA profile from region L4 was intermediate,compared to L1 and L2, and showed a slight shift toward an increasein 100K mRNA production. Thus, the 33K and particularly the pVIIImRNA species were reduced.

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FIG. 4. Effect of ASF/SF2 overexpression on L2 and L4 mRNA expression. Cytoplasmic RNA was prepared from AdG5(His)-ASF/AdCMVProg-infected 293 cells at the indicated time points and separated on a 1% agarose gel containing 2.2 M formaldehyde. RNA was transferred to a nitrocellulose filter and hybridized with ³²P-labeled probes specific for region L2 or L4. Lanes 1, mock-infected cells.

ASF/SF2 overexpression does not block E2A-72K protein expression. The observation that His-ASF/SF2 almost completely eliminated major late mRNA expression could indicate that ASF/SF2 unspecificallyblocks viral gene expression. To test this, we analyzed E2A-72Kprotein levels in AdG5(His)-ASF-infected cells. In contrast tomost adenovirus units, E2A mRNA expression is not regulated atthe level of alternative splicing (reviewed in reference 21).Instead, transcription initiation occur at two alternative promoters(Fig. 1); the distal promoter is used early and the proximal promoteris used late after infection. As shown in Fig. 5, E2A-72K proteinexpression and E2A mRNA accumulation (data not shown) were enhancedapproximately threefold at 18 and 24 hpi in His-ASF/SF2-expressingcells compared to the parental virus, dl309. Similarly, the steady-statelevels of E1A and E1B mRNA accumulation are not significantlyreduced by His-ASF/SF2 overexpression (see below). Taken together,these results suggest that the negative effects of ASF/SF2 overproductionprimarily affect mRNA accumulation from the major late transcriptionunit (MLTU).

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FIG. 5. ASF/SF2 does not block E2A-72K expression. 293 cells infected with AdG5(His)-ASF/AdCMVProg were harvested at the indicated time points, and E2A-72K protein expression was analyzed by a Western blot assay. The faster-migrating species most likely represent degradation products of the E2A-72K protein.

ASF/SF2 overexpression inhibits the temporal shift in E1A and E1B alternative splicing. The E1A and E1B transcription units represent examples of genes where a common 3' splice site is joined to alternative 5'splice sites (Fig. 1). During a lytic infection, the relativeratios of individual E1A and E1B mRNAs change. Thus, the E1A 13Sand the E1B 22S mRNAs are the predominant mRNAs expressed at earlytimes of infection, whereas the E1A 9S and E1B 13S mRNAs becomethe most abundant mRNAs expressed late afterinfection.

Since the progesterone-regulated gene cassette replaces the E1 region in the recombinant viruses, AdCMVProg and AdG5(His)-ASFdo not express E1A and E1B mRNAs. To investigate the effect ofASF/SF2 overexpression on the accumulation of region E1 mRNAs,we therefore included the parental virus dl309 in the infectioncocktail. Thus, a mixture of AdCMVProg, AdG5(His)-ASF, and dl309was used to infect monolayer cultures of HeLa cells. His-ASF/SF2expression was induced at the start of infection, and cytoplasmicRNAwas isolated at 12 and 18 hpi. The structure of E1A and E1BmRNAs expressed from the dl309 genome was determined by S1 protection(E1A) and Northern blot (E1B)analysis.

As shown in Fig. 6, His-ASF/SF2 induction resulted in an increase in E1A 13S mRNA accumulation, at the expense of E1A 12Sand 9S mRNA accumulation. Similarly, His-ASF/SF2 overexpressionresulted in a substantial shift toward E1B 22S mRNA accumulationaccompanied by a dramatic reduction in E1B 13S mRNA accumulation.The steady-state levels of the pIX mRNA, which is an unsplicedmRNA (2) encoded by a separate transcription unit located withinE1B (Fig. 1), was slightly reduced.

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FIG. 6. ASF/SF2 blocks the temporal shift in E1A and E1B mRNA accumulation. Total cytoplasmic RNA prepared from AdG5(His)-ASF/AdCMVProg/dl309-infected HeLa cells were subjected to neutral S1 analysis to detect individual E1A mRNAs (A) or Northern blot hybridization to detect E1B mRNA expression (B). dl309 was included in this experiment since the recombinant viruses lack the E1 region. Lane 1, mock-infected cells.

Taken together, the results extend previous data by showing that ASF/SF2 promotes proximal splice site usage also during anadenovirus infection. This general activity of ASF/SF2 maintainsE1A and E1B mRNA expression in a prolonged early phase of mRNAexpression.

Viral DNA replication is inhibited by ASF/SF2 overexpression. It has previously been shown that viral DNA replication is coupled to efficient mRNA expression from the MLTU (reviewed inreference 21). Thus, the observation that high levels of His-ASF/SF2expression severely reduced cytoplasmic L1 mRNA accumulation (Fig.3A) suggested that ASF/SF2, directly or indirectly, may blockviral DNA replication. To test this hypothesis, the efficiencyof viral DNA replication in AdG5(His)-ASF-infected cells was measuredat different time points of infection by a dot blot assay. Asshown in Fig. 7, inducing His-ASF/SF2 expression from the startof infection indeed caused a severe reduction in viral DNA replicationcompared to dl309. Interestingly, the background expression ofHis-ASF/SF2, in the absence of inducer, was sufficient to causea delay in viral DNA replication. Thus, viral DNA accumulationwas severely reduced at 18 hpi but back to normal at 24 hpi.

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FIG. 7. Effect of ASF/SF2 on adenovirus DNA replication. Viral DNA was prepared from AdG5(His)-ASF/AdCMVProg-infected 293 cells by Hirt extraction (19) at the indicated time points and analyzed by a dot blot assay (A). The result was quantitated by PhosphorImager scanning (B). The graph represents the mean value of three separate experiments.

ASF/SF2 expression blocks formation of new virus particles. A consequence of the negative effects of ASF/SF2 on the expression of major late mRNA would be less efficient growth of AdG5(His)-ASF.To test this hypothesis, we measured the effect of ASF/SF2 overexpressionon late viral protein synthesis and new virus particle formation.AdG5(His)-ASF was grown in the presence of increasing amountsof inducer, added at the start of infection. Cells were harvested40 hpi, and virus production was quantitated by plaque assay.As shown in Fig. 8, growth of AdG5(His)-ASF in the presence ofincreasing amounts of inducer resulted in a more than 60-foldreduction in virus yield. Noteworthy, growth of the recombinantvirus in the absence of inducer resulted in a 20-fold reductionin virus yield. At first glance, this may seem surprising. However,as shown in Fig. 2A, a high background expression of His-ASF/SF2is detectable also in the absence of inducer. This spurious His-ASF/SF2expression is sufficient to significantly reduce expression oflate viral proteins needed for virion assembly (Fig. 9). Collectively,the results strengthen our hypothesis that viral control of SRprotein function is essential for efficient virus multiplication.

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FIG. 8. ASF/SF2 decreases the formation of infectious virus particles. 293 cells were infected with AdG5(His)-ASF/AdCMVProg in the presence of different concentrations of RU 486. Virus was prepared 40 hpi by freeze-thawing and quantitated by plaque titration.

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FIG. 9. ASF/SF2 overexpression inhibits late viral protein synthesis. 293 cells infected with AdG5(His)-ASF/AdCMVProg were pulse-labeled with [³⁵S]cysteine/methionine for 2 h prior to harvest. Protein extracts prepared at the indicated time points were separated by SDS-PAGE on a 10% gel, which was then subjected to autoradiography. Lane 1, mock-infected cells.

	DISCUSSION

Top Abstract Introduction Materials and Methods Results Discussion References

During a lytic adenovirus infection, the production of viral proteins is regulated, to a large extent, at the level of alternativeRNA splicing, i.e., production of multiple mRNAs with differentcoding capacities from a single transcription unit. The splicedstructure of mRNAs expressed from most transcription units changesduring the infectious cycle. The general tendency is that shortermRNAs, produced by splicing out larger introns, dominate at latertime points of infection. Interestingly, the prototypical SR proteinASF/SF2 has been shown to have the opposite effect on RNA splicesite choice. Thus, addition of an excess of ASF/SF2 in vitro ortransfection of a plasmid expressing ASF/SF2 results in a shifttoward production of long mRNAs, i.e., proximal splice site usage(4, 6, 16, 24, 30, 38). We have previously shownthat SR proteins purified from late adenovirus-infected cellsare partially inactivated as splicing enhancer or splicing repressorproteins by a virus-induced dephosphorylation (23). Based onthis finding, we speculated that the temporal shift from proximalto distal splice site usage in adenovirus alternative splicingwas coupled to this SR protein inactivation. A prediction of thismodel is that overexpression of an SR protein during a productiveinfection should cause a block in the temporal shift in adenovirusalternative splicing, by disturbing the balance of functionaland nonfunctional SR proteins in infectedcell.

Here we test this prediction by analyzing the phenotype of a recombinant adenovirus expressing the prototypical SR protein,ASF/SF2. We show that overexpression of ASF/SF2 has negative effects,particularly on major late gene expression (Fig. 3 and 4), withno (E2A-72K [Fig. 5]) or small (E1A and E1B [Fig. 6]) inhibitoryeffects on early viral mRNA accumulation. As the model also predicts,ASF/SF2 overexpression blocks the early to late shift in E1A,E1B, and L1 alternative splicing (Fig. 3 and 5). Furthermore,high ASF/SF2 expression also caused a severe inhibition of viralDNA replication (Fig. 7), late protein synthesis (Fig. 9), andvirus production (Fig. 8). Collectively, our results support thehypothesis that viral control of SR protein activity is importantfor the correct temporal expression of early and late viral mRNAsduring infection, and as a consequence effective virusmultiplication.

Expression of mRNAs from the MLTU is subjected to a temporal regulation of poly(A) site usage (reviewed in reference 21).Thus, the L1 region is the only part of the MLTU that is expressedat early times of infection (1, 8, 33). At a transientstage following initiation of viral DNA replication, mRNAs fromregions L1 and L4 accumulate preferentially (26, 40). It hasbeen proposed that efficient expression of mRNA from regions L1through L5 requires both viral DNA replication and late proteinsynthesis (26). Previous results also have suggested that viralDNA replication per se is sufficient to induce accumulation ofnormal steady-state levels of L1 mRNAs (25). However, undersuch conditions the temporal shift in alternative splicing wasshown to be incomplete, with a preferential accumulation of the52,55K+i and IIIa+i mRNA species (25). Here we show that inductionof ASF/SF2 expression from the start of infection blocks viralDNA replication (Fig. 7) and results in an almost complete lossof mRNA expression from the MLTU (Fig. 3 and 4). Also, we showthat the small amounts of L1 mRNAs produced are incompletely spliced,with a preferential accumulation of 52,55K+i and IIIa+i mRNAs(Fig. 3A, lanes 7 to 9). The effects of ASF/SF2 on L1 mRNA expressionwere specific since overproduction of the CAT protein in the sametype of experiment did not have an adverse effect on L1 mRNA expression(Fig. 3C).

The inhibitory effect of ASF/SF2 on viral DNA replication (Fig. 7) probably results from a block in proper expression of mRNAsfrom the E2B region (Fig. 1). In fact, preliminary experimentssuggest that expression of the mRNA encoding for pTP, the adenovirusprotein functioning as a primer protein for initiation of viralDNA replication (reviewed in reference 44), is reduced by ASF/SF2overexpression (data not shown). However, pTP is expressed atlow amounts during infection, and we were unable to detect pTPby Western blotting in mostexperiments.

Interestingly, the background expression of His-ASF/SF2 observed in 293 cells in the absence of inducer (Fig. 2A) was sufficientto disturb major late mRNA expression (Fig. 3A and 4), and lateprotein synthesis (Fig. 9), also under conditions where viralDNA replication was back to wild-type levels (24 hpi) (Fig. 7).This finding is significant and differs from previous resultsby suggesting that DNA replication per se is not enough to activatemRNA expression from the MLTU. However, all data can be reconciledin a model where it is postulated that an early viral protein(s)is required for efficient mRNA production from the L1 region.Thus, inducing ASF/SF2 expression from the start of infectioninterferes with the temporal shift in early viral mRNA expression(Fig. 6) and, as a consequence, synthesis of the complete repertoireof early viral proteins. Some of these proteins are likely tobe required at various stages of gene expression, such as transcription,RNA processing, RNA transport, and RNA stability. For example,we have previously shown that several E4 proteins have the capacityto modulate RNA splicing. Thus, the E4-ORF4 protein inactivatesSR proteins as IIIa splicing repressor proteins (23). The E4-ORF3protein induces i-leader inclusion, while the E4-ORF6 proteincauses i-leader skipping (35). However, we do not exclude thatASF/SF2 interferes at other levels of adenovirus gene expression.For example, high amounts of ASF/SF2 may block major late poly(A)site usage. It has been well documented that RNA splice site selectioncan affect the efficiency of polyadenylation, and vice versa (10,34, 43). Alternatively, and perhaps more attractive, ASF/SF2overexpression may directly interfere with transcription fromthe major late promoter. Recent data have indicated that RNA polymeraseII transcription and RNA processing are coordinated events. Thus,many RNA processing factors, including ASF/SF2, have been shownto interact with the C-terminal domain tail of RNA polymeraseII (reviewed in reference 5). Such an interaction may have,or induce, adverse effects on transcription initiation and/orelongation at the major late promoter. Clearly the approach describedhere should make it possible to further define the mechanisticdetails of ASF/SF2 inhibition of virusmultiplication.

The experimental strategy used here provides a new in vivo method to study the significance of defined proteins on adenovirusmultiplication. Thus, by reconstructing recombinant viruses expressinga gene of interest under the transcriptional control of an induciblepromoter, it should be possible to use on/off switches of reportergene expression to further define protein function. However, ourexperiments also illustrate an unexpected complexity of gene regulationwith the current generation of our adenovirus vector system. Thus,the vector system functions extraordinarily well under nonreplicativeconditions (HeLa cells [Fig. 2A]), where we reach induction levelsexceeding 500-fold (32). In contrast, a significant backgroundof reporter gene expression is observed in 293 cells, also inthe absence of inducer (Fig. 2A and data not shown). This troublesomeHis-ASF/SF2 expression is, to a large extent, caused by the E1Atranscriptional activator protein expressed in 293 cells, whichappears to activate transcription from the TATA element presentin the G5 minimal major late promoter driving reporter gene expression(data not shown). It is important for our future work to reducethis basal reporter gene expression in 293 cells. We are currentlydeveloping new strategies to silence the 293-cell specific backgroundexpression of the reporter gene (D. Edholm, M. Molin, and G. Akusjärvi,unpublisheddata).

	ACKNOWLEDGMENTS

We are grateful to T. Maniatis for providing the Prey-ASF plasmid, J. Stevenin for the ASF/SF2 peptide antisera, and E. Bridgefor the E2A-72K antibody. RU 486 was kindly provided by Roussel-Uclaf.

This work was supported by the Swedish Cancer Society and the Göran Gustafsson Foundation for Natural and MedicalResearch.

	FOOTNOTES

^* Corresponding author. Mailing address: Department of Medical Biochemistry and Microbiology, BMC, Box 582, Uppsala University,SE-751 23 Uppsala, Sweden. Phone: 46-18-471 41 64. Fax: 46-18-5098 76. E-mail: goran.akusjarvi{at}imim.uu.se.

REFERENCES

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References

1. Akusjärvi, G., and H. Persson. 1981. Controls of RNA splicing and termination in the major late adenovirus transcription unit. Nature 292:420-426[CrossRef][Medline].

2. Aleström, P., G. Akusjärvi, M. Perricaudet, M. B. Mathews, D. Klessig, and U. Pettersson. 1980. The gene for polypeptide IX of adenovirus type 2 and its unspliced messenger RNA. Cell 19:671-681[CrossRef][Medline].

3. Ausubel, F. M., R. Brent, R. E. Kingston, D. D. Moore, J. G. Seidman, J. A. Smith, and K. Struhl (ed.). 1987. Current protocols in molecular biology. John Wiley & Sons, Inc., New York, N.Y.

4. Bai, Y., D. Lee, T. Yu, and L. A. Chasin. 1999. Control of 3' splice site choice in vivo by ASF/SF2 and hnRNP A1. Nucleic Acids Res. 27:1126-1134[Abstract/Free Full Text].

5. Bentley, D. 1999. Coupling RNA polymerase II transcription with pre-mRNA processing. Curr. Opin. Cell Biol. 11:347-351[CrossRef][Medline].

6. Caceres, J. F., S. Stamm, D. M. Helfman, and A. R. Krainer. 1994. Regulation of alternative splicing in vivo by overexpression of antagonistic splicing factors. Science 265:1706-1709[Abstract/Free Full Text].

7. Cao, W., S. F. Jamison, and M. A. Garcia-Blanco. 1997. Both phosphorylation and dephosphorylation of ASF/SF2 are required for pre-mRNA splicing in vitro. RNA 3:1456-1467[Abstract].

8. Chow, L. T., T. R. Broker, and J. B. Lewis. 1979. Complex splicing patterns of RNAs from the early regions of adenovirus-2. J. Mol. Biol. 134:265-303[CrossRef][Medline].

9. Colwill, K., L. L. Feng, J. M. Yeakley, G. D. Gish, J. F. Caceres, T. Pawson, and X. D. Fu. 1996. SRPK1 and Clk/Sty protein kinases show distinct substrate specificities for serine/arginine-rich splicing factors. J. Biol. Chem. 271:24569-24575[Abstract/Free Full Text].

10. Cooke, C., H. Hans, and J. C. Alwine. 1999. Utilization of splicing elements and polyadenylation signal elements in the coupling of polyadenylation and last-intron removal. Mol. Cell. Biol. 19:4971-4979[Abstract/Free Full Text].

11. Eperon, I. C., D. C. Ireland, R. A. Smith, A. Mayeda, and A. R. Krainer. 1993. Pathways for selection of 5' splice sites by U1 snRNPs and SF2/ASF. EMBO J. 12:3607-3617[Medline].

12. Fu, X. D. 1995. The superfamily of arginine/serine-rich splicing factors. RNA 1:663-680[Medline].

13. Gattoni, R., K. Chebli, M. Himmelspach, and J. Stevenin. 1991. Modulation of alternative splicing of adenoviral E1A transcripts: factors involved in the early-to-late transition. Genes Dev. 5:1847-1858[Abstract/Free Full Text].

14. Graham, F. L., J. Smiley, W. C. Russell, and R. Nairn. 1977. Characteristics of a human cell line transformed by DNA from human adenovirus type 5. J. Gen. Virol. 36:59-574[Abstract/Free Full Text].

15. Harper, J. E., and J. L. Manley. 1991. A novel protein factor is required for use of distal alternative 5' splice sites in vitro. Mol. Cell. Biol. 11:5945-5953[Abstract/Free Full Text].

16. Harper, J. E., and J. L. Manley. 1992. Multiple activities of the human splicing factor ASF. Gene Expr. 2:19-29[Medline].

17. Hertel, K. J., K. W. Lynch, and T. Maniatis. 1997. Common themes in the function of transcription and splicing enhancers. Curr. Opin. Cell Biol. 9:350-357[CrossRef][Medline].

18. Himmelspach, M., Y. Cavaloc, K. Chebli, J. Stevenin, and R. Gattoni. 1995. Titration of serine/arginine (SR) splicing factors during adenoviral infection modulates E1A pre-mRNA alternative splicing. RNA 1:794-806[Abstract].

19. Hirt, B. 1967. Selective extraction of polyoma DNA from infected mouse cells. J. Mol. Biol. 14:365-369.

20. Hitt, M., A. J. Bett, L. Prevec, and F. L. Graham. 1994. Construction and propagation of human adenovirus vectors, p. 479-490. In J. E. Celis (ed.), Cell biology: a laboratory handbook, vol. 1. Academic Press, San Diego, Calif.

21. Imperiale, M. J., G. Akusjärvi, and K. N. Leppard. 1995. Post-transcriptional control of adenovirus gene expression. Curr. Top. Microbiol. Immunol. 199:139-171.

22. Kanopka, A., O. Mühlemann, and G. Akusjärvi. 1996. Inhibition by SR proteins of splicing of a regulated adenovirus pre-mRNA. Nature 381:535-538[CrossRef][Medline].

23. Kanopka, A., O. Mühlemann, S. Petersen-Mahrt, C. Estmer, C. Öhrmalm, and G. Akusjärvi. 1998. Regulation of adenovirus alternative RNA splicing by dephosphorylation of SR proteins. Nature 393:185-187[CrossRef][Medline].

24. Krainer, A. R., A. Mayeda, D. Kozak, and G. Binns. 1991. Functional expression of cloned human splicing factor SF2: homology to RNA-binding proteins, U1 70K, and Drosophila splicing regulators. Cell 66:383-394[CrossRef][Medline].

25. Larsson, S., J. P. Kreivi, and G. Akusjärvi. 1991. Control of adenovirus alternative RNA splicing: effect of viral DNA replication on RNA splice site choice. Gene 107:219-227[CrossRef][Medline].

26. Larsson, S., C. Svensson, and G. Akusjärvi. 1992. Control of adenovirus major late gene expression at multiple levels. J. Mol. Biol. 225:287-298[CrossRef][Medline].

27. Lim, L. P., and P. A. Sharp. 1998. Alternative splicing of the fibronectin EIIIB exon depends on specific TGCATG repeats. Mol. Cell. Biol. 18:3900-3906[Abstract/Free Full Text].

28. Manley, J. L., and R. Tacke. 1996. SR proteins and splicing control. Genes Dev. 10:1569-1579[Free Full Text].

29. Mayeda, A., D. M. Helfman, and A. R. Krainer. 1993. Modulation of exon skipping and inclusion by heterogeneous nuclear ribonucleoprotein A1 and pre-mRNA splicing factor SF2/ASF. Mol. Cell. Biol. 13:2993-3001[Abstract/Free Full Text].

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33. Nevins, J. R., and M. C. Wilson. 1981. Regulation of adenovirus-2 gene expression at the level of transcriptional termination and RNA processing. Nature 290:113-118[CrossRef][Medline].

34. Niwa, M., S. D. Rose, and S. M. Berget. 1990. In vitro polyadenylation is stimulated by the presence of an upstream intron. Genes Dev. 4:1552-1559[Abstract/Free Full Text].

35. Nordqvist, K., K. Öhman, and G. Akusjärvi. 1994. Human adenovirus encodes two proteins which have opposite activities on accumulation of alternatively spliced mRNAs. Mol. Cell. Biol. 14:437-443[Abstract/Free Full Text].

36. Petersen-Mahrt, S. K., C. Estmer, C. Öhrmalm, D. A. Matthews, W. C. Russell, and G. Akusjärvi. 1999. The splicing factor-associated protein, p32, regulates RNA splicing by inhibiting ASF/SF2 RNA binding and phosphorylation. EMBO J. 18:1014-1024[CrossRef][Medline].

37. Screaton, G. R., J. F. Caceres, A. Mayeda, M. V. Bell, M. Plebanski, D. G. Jackson, J. I. Bell, and A. R. Krainer. 1995. Identification and characterization of three members of the human SR family of pre-mRNA splicing factors. EMBO J. 14:4336-4349[Medline].

38. Shih, S. R., and R. M. Krug. 1996. Novel exploitation of a nuclear function by influenza virus: the cellular SF2/ASF splicing factor controls the amount of the essential viral M2 ion channel protein in infected cells. EMBO J. 15:5415-5427[Medline].

39. Stow, N. D. 1981. Cloning of a DNA fragment from the left-hand terminus of the adenovirus type 2 genome and its use in site-directed mutagenesis. J. Virol. 37:171-180[Abstract/Free Full Text].

40. Svensson, C., and G. Akusjärvi. 1986. Defective RNA splicing in the absence of adenovirus-associated RNAI. Proc. Natl. Acad. Sci. USA 83:4690-4694[Abstract/Free Full Text].

41. Svensson, C., U. Pettersson, and G. Akusjärvi. 1983. Splicing of adenovirus 2 early region 1A mRNAs is non-sequential. J. Mol. Biol. 165:475-495[CrossRef][Medline].

42. Tacke, R., and J. L. Manley. 1999. Determinants of SR protein specificity. Curr. Opin. Cell Biol. 11:358-362[CrossRef][Medline].

43. Vagner, S., C. Vagner, and I. W. Mattaj. 2000. The carboxyl terminus of vertebrate poly(A) polymerase interacts with U2AF 65 to couple 3'-end processing and splicing. Genes Dev. 14:403-413[Abstract/Free Full Text].

44. van der Vliet, P. C. 1995. Adenovirus DNA replication. Curr. Top. Microbiol. Immunol. 199:1-30.

45. Wang, J., and J. L. Manley. 1995. Overexpression of the SR proteins ASF/SF2 and SC35 influences alternative splicing in vivo in diverse ways. RNA 1:335-346[Abstract].

46. Wu, J. Y., and T. Maniatis. 1993. Specific interactions between proteins implicated in splice site selection and regulated alternative splicing. Cell 75:1061-1070[CrossRef][Medline].

47. Xiao, S. H., and J. L. Manley. 1998. Phosphorylation-dephosphorylation differentially affects activities of splicing factor ASF/SF2. EMBO J. 17:6359-6367[CrossRef][Medline].

48. Zahler, A. M., K. M. Neugebauer, W. S. Lane, and M. B. Roth. 1993. Distinct functions of SR proteins in alternative pre-mRNA splicing. Science 260:219-222[Abstract/Free Full Text].

49. Zhang, W. J., and J. Y. Wu. 1996. Functional properties of p54, a novel SR protein active in constitutive and alternative splicing. Mol. Cell. Biol. 16:5400-5408[Abstract].

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1.	Akusjärvi, G., and H. Persson. 1981. Controls of RNA splicing and termination in the major late adenovirus transcription unit. Nature 292:420-426[CrossRef][Medline].
2.	Aleström, P., G. Akusjärvi, M. Perricaudet, M. B. Mathews, D. Klessig, and U. Pettersson. 1980. The gene for polypeptide IX of adenovirus type 2 and its unspliced messenger RNA. Cell 19:671-681[CrossRef][Medline].
3.	Ausubel, F. M., R. Brent, R. E. Kingston, D. D. Moore, J. G. Seidman, J. A. Smith, and K. Struhl (ed.). 1987. Current protocols in molecular biology. John Wiley & Sons, Inc., New York, N.Y.
4.	Bai, Y., D. Lee, T. Yu, and L. A. Chasin. 1999. Control of 3' splice site choice in vivo by ASF/SF2 and hnRNP A1. Nucleic Acids Res. 27:1126-1134[Abstract/Free Full Text].
5.	Bentley, D. 1999. Coupling RNA polymerase II transcription with pre-mRNA processing. Curr. Opin. Cell Biol. 11:347-351[CrossRef][Medline].
6.	Caceres, J. F., S. Stamm, D. M. Helfman, and A. R. Krainer. 1994. Regulation of alternative splicing in vivo by overexpression of antagonistic splicing factors. Science 265:1706-1709[Abstract/Free Full Text].
7.	Cao, W., S. F. Jamison, and M. A. Garcia-Blanco. 1997. Both phosphorylation and dephosphorylation of ASF/SF2 are required for pre-mRNA splicing in vitro. RNA 3:1456-1467[Abstract].
8.	Chow, L. T., T. R. Broker, and J. B. Lewis. 1979. Complex splicing patterns of RNAs from the early regions of adenovirus-2. J. Mol. Biol. 134:265-303[CrossRef][Medline].
9.	Colwill, K., L. L. Feng, J. M. Yeakley, G. D. Gish, J. F. Caceres, T. Pawson, and X. D. Fu. 1996. SRPK1 and Clk/Sty protein kinases show distinct substrate specificities for serine/arginine-rich splicing factors. J. Biol. Chem. 271:24569-24575[Abstract/Free Full Text].
10.	Cooke, C., H. Hans, and J. C. Alwine. 1999. Utilization of splicing elements and polyadenylation signal elements in the coupling of polyadenylation and last-intron removal. Mol. Cell. Biol. 19:4971-4979[Abstract/Free Full Text].
11.	Eperon, I. C., D. C. Ireland, R. A. Smith, A. Mayeda, and A. R. Krainer. 1993. Pathways for selection of 5' splice sites by U1 snRNPs and SF2/ASF. EMBO J. 12:3607-3617[Medline].
12.	Fu, X. D. 1995. The superfamily of arginine/serine-rich splicing factors. RNA 1:663-680[Medline].
13.	Gattoni, R., K. Chebli, M. Himmelspach, and J. Stevenin. 1991. Modulation of alternative splicing of adenoviral E1A transcripts: factors involved in the early-to-late transition. Genes Dev. 5:1847-1858[Abstract/Free Full Text].
14.	Graham, F. L., J. Smiley, W. C. Russell, and R. Nairn. 1977. Characteristics of a human cell line transformed by DNA from human adenovirus type 5. J. Gen. Virol. 36:59-574[Abstract/Free Full Text].
15.	Harper, J. E., and J. L. Manley. 1991. A novel protein factor is required for use of distal alternative 5' splice sites in vitro. Mol. Cell. Biol. 11:5945-5953[Abstract/Free Full Text].
16.	Harper, J. E., and J. L. Manley. 1992. Multiple activities of the human splicing factor ASF. Gene Expr. 2:19-29[Medline].
17.	Hertel, K. J., K. W. Lynch, and T. Maniatis. 1997. Common themes in the function of transcription and splicing enhancers. Curr. Opin. Cell Biol. 9:350-357[CrossRef][Medline].
18.	Himmelspach, M., Y. Cavaloc, K. Chebli, J. Stevenin, and R. Gattoni. 1995. Titration of serine/arginine (SR) splicing factors during adenoviral infection modulates E1A pre-mRNA alternative splicing. RNA 1:794-806[Abstract].
19.	Hirt, B. 1967. Selective extraction of polyoma DNA from infected mouse cells. J. Mol. Biol. 14:365-369.
20.	Hitt, M., A. J. Bett, L. Prevec, and F. L. Graham. 1994. Construction and propagation of human adenovirus vectors, p. 479-490. In J. E. Celis (ed.), Cell biology: a laboratory handbook, vol. 1. Academic Press, San Diego, Calif.
21.	Imperiale, M. J., G. Akusjärvi, and K. N. Leppard. 1995. Post-transcriptional control of adenovirus gene expression. Curr. Top. Microbiol. Immunol. 199:139-171.
22.	Kanopka, A., O. Mühlemann, and G. Akusjärvi. 1996. Inhibition by SR proteins of splicing of a regulated adenovirus pre-mRNA. Nature 381:535-538[CrossRef][Medline].
23.	Kanopka, A., O. Mühlemann, S. Petersen-Mahrt, C. Estmer, C. Öhrmalm, and G. Akusjärvi. 1998. Regulation of adenovirus alternative RNA splicing by dephosphorylation of SR proteins. Nature 393:185-187[CrossRef][Medline].
24.	Krainer, A. R., A. Mayeda, D. Kozak, and G. Binns. 1991. Functional expression of cloned human splicing factor SF2: homology to RNA-binding proteins, U1 70K, and Drosophila splicing regulators. Cell 66:383-394[CrossRef][Medline].
25.	Larsson, S., J. P. Kreivi, and G. Akusjärvi. 1991. Control of adenovirus alternative RNA splicing: effect of viral DNA replication on RNA splice site choice. Gene 107:219-227[CrossRef][Medline].
26.	Larsson, S., C. Svensson, and G. Akusjärvi. 1992. Control of adenovirus major late gene expression at multiple levels. J. Mol. Biol. 225:287-298[CrossRef][Medline].
27.	Lim, L. P., and P. A. Sharp. 1998. Alternative splicing of the fibronectin EIIIB exon depends on specific TGCATG repeats. Mol. Cell. Biol. 18:3900-3906[Abstract/Free Full Text].
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