Versatile Role for hnRNP D Isoforms in the Differential Regulation of Cytoplasmic mRNA Turnover

doi:10.1128/MCB.21.20.6960-6971.2001

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Molecular and Cellular Biology, October 2001, p. 6960-6971, Vol. 21, No. 20
0270-7306/01/$04.00+0 DOI: 10.1128/MCB.21.20.6960-6971.2001
Copyright © 2001, American Society for Microbiology. All rights reserved.

Versatile Role for hnRNP D Isoforms in the Differential Regulation of Cytoplasmic mRNA Turnover

Nianhua Xu, Chyi-Ying A. Chen, and Ann-Bin Shyu^*

Department of Biochemistry and Molecular Biology, The University of Texas Houston Medical School, Houston, Texas 77030

Received 10 May 2001/Returned for modification 21 June 2001/Accepted 16 July 2001

	ABSTRACT

Top Abstract Introduction Materials and Methods Results Discussion References

An important emerging theme is that heterogeneous nuclear ribonucleoproteins (hnRNPs) not only function in the nucleus butalso control the fates of mRNAs in the cytoplasm. Here, we showthat hnRNP D plays a versatile role in cytoplasmic mRNA turnoverby functioning as a negative regulator in an isoform-specificand cell-type-dependent manner. We found that hnRNP D discriminatesamong the three classes of AU-rich elements (AREs), most effectivelyblocking rapid decay directed by class II AREs found in mRNAsencoding cytokines. Our experiments identified the overlappingAUUUA motifs, one critical characteristic of class II AREs, tobe the key feature recognized in vivo by hnRNP D for its negativeeffect on ARE-mediated mRNA decay. The four hnRNP D isoforms,while differing in their ability to block decay of ARE-containingmRNAs, all potently inhibited mRNA decay directed by another mRNAcis element that shares no sequence similarity with AREs, thepurine-rich c-fos protein-coding region determinant of instability.Further experiments indicated that different mechanisms underliethe inhibitory effect of hnRNP D on the two distinct mRNA decaypathways. Our study identifies a potential mechanism by whichcytoplasmic mRNA turnover can be differentially and selectivelyregulated by hnRNP D isoforms in mammalian cells. Our resultssupport the notion that hnRNP D serves as a key factor broadlyinvolved in general mRNAdecay.

	INTRODUCTION

Top Abstract Introduction Materials and Methods Results Discussion References

Control of mRNA turnover is a powerful means to regulate levels of protein expression (17, 29, 34). One class of regulatorycis elements that dictates the rate of mRNA turnover comprisesthe AU-rich elements (AREs) found in the 3' untranslated regions(UTRs) of many short-lived mRNAs (3). Previously, distinctsequence features and decay characteristics displayed by differentAREs have led to the classification of AREs into three types (6,32). Class I AREs, found in mRNAs like c-fos and c-myc, contain1 to 3 scattered copies of the pentanucleotide AUUUA embeddedwithin U-rich regions. Class II AREs, only found in cytokine mRNAssuch as granulocyte-macrophage colony-stimulating factor (GM-CSF)and tumor necrosis factor alpha (TNF- $alpha$ ), contain multiple overlappingcopies (5 to 8 copies) of the AUUUA motif. Class III AREs, suchas the one in c-jun mRNA, lack the hallmark AUUUA pentanucleotidebut require a U-rich sequence and possibly other unknown featuresfor their destabilizing function. mRNA turnover mediated by AREsfrom all three classes is characterized by rapid shortening ofthe poly(A) tail followed by rapid decay of the mRNA body. Intriguingly,actinomycin D, a transcription inhibitor extensively used in mRNAturnover studies, was found to block the rapid decay directedby both class I and class II AUUUA-containing AREs but to havelittle effect on class III non-AUUUA AREs (6, 31). Thesedistinct features and properties of AREs point to the possibilitythat, in vivo, different classes of AREs are differentially regulated,e.g., through recognition by different ARE-binding proteins (ARE-BPs).

Several in vivo observations lend support to this notion. In a monocytic tumor cell line, c-fos and c-myc 3' UTRs, containingclass I AREs, destabilized a reporter mRNA, whereas the GM-CSF3' UTR containing a class II ARE did not (36). A similar discriminationbetween the two classes of AREs has also been suggested in twoother studies. Stimulation of quiescent primary T lymphocyteswith antibodies to CD3/CD28 receptors specifically stabilizeslymphokine mRNAs containing class II AREs, while c-fos and c-mycmRNAs remain unstable (24). The interleukin-3 (IL-3) ARE, havingclass II characteristics, is required in a mast tumor cell linefor the destabilization of IL-3 mRNA induced by the immunosuppressantcyclosporine A (30). Significantly, the role of IL-3 AREs cannotbe substituted by class I AREs from either c-fos or c-myc. Thus,it appears that in vivo a fine-tuning mechanism is likely to existthat differentially regulates the RNA destabilizing function betweenclass I and class IIAREs.

In an effort to understand the mechanism and regulation of ARE-mediated mRNA turnover, many laboratories have used in vitroapproaches to identify proteins that bind AU- or U-rich sequences(16, 21, 33; also reviewed in references 25 and 43).Among ARE-BPs, heterogeneous nuclear ribonucleoprotein (hnRNP)D, also termed AUF1 (49), has been widely studied for its potentialrole in ARE-mediated mRNA decay (for examples, see references10, 25, and 41). In vitro RNA-binding studies using recombinantproteins made in Escherichia coli showed that hnRNP D displayshigh affinity, with dissociation constants at a nanomolar range,for a variety of AREs and a (UUAG)_n sequence, as well as a stretchof 32-nucleotide (nt) uridylates (1, 10, 18, 44). Itwas also concluded in one of these in vitro studies that the hallmarkmotif of most AREs, AUUUA, is not required for hnRNP D binding(43). In vitro binding studies of other recombinant ARE-BPs,e.g., HuR (27), have often led to the similar conclusion thatARE-BPs indiscriminately bind AREs showing distinctly differentsequence features and that the U-rich sequence serves as an effectivecompetitor to abolish ARE-BP binding to nativeAREs.

The hnRNP D gene is also unique among other ARE-BPs in that it is transcribed into a pre-mRNA that undergoes alternative pre-mRNAsplicing of two coding exons, exon 2 and exon 7, to give riseto four different protein isoforms with apparent molecular massesof 37, 40, 42, and 45 kDa (Fig. 1A) (12, 42). The hnRNP Dprotein exhibits structural motifs that are arranged in a similarway to hnRNP A1: an N-terminal domain followed by two consecutiveRNA recognition motifs (RRMs) and a C-terminal domain containingArg-Gly-Gly (RGG) motifs (13). Transfection studies have shownthat hnRNP D functions as an mRNA destabilizing factor in humanerythroleukemic K562 cells (25) and is targeted for degradationby the ubiquitin-proteasome pathway (22). More recently, theparticipation of hnRNP D in RNA turnover was extended to includethe mRNA decay directed by the c-fos major coding determinant(15), a purine-rich sequence that shares no sequence similaritywith AREs. It was found that hnRNP D is an integral componentof a multiprotein complex that mediates c-fos major coding determinant-directedmRNA decay (15). These observations suggest that hnRNP D mayplay multiple roles in cytoplasmic mRNA turnover.

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FIG. 1. Ectopic expression of human hnRNP D isoforms in mouse NIH 3T3 cells differentially inhibits rapid mRNA decay directed by the c-fos ARE. (A) Schematic diagram of the four hnRNP D isoforms. The open box indicates the N-terminal domain. RRMI and RRMII depict RNA recognition motifs. The gray box represents the C-terminal domain. The black box at the very N terminus indicates the myc-epitope tag. The striped box represents the additional peptide sequences included as a result of alternative RNA splicing. (B) Semi-log plot showing the effects of four hnRNP D isoforms on mRNA decay directed by the c-fos ARE. Quantitation of mRNA was obtained by scanning radioactive blots with an imager (Packard) and the data were plotted as a function of time. (C) RNA blots showing deadenylation and decay of $beta$ -globin mRNA bearing the c-fos ARE (BBB+ARE^fos) in the absence (control) or presence of ectopically expressed individual isoforms of hnRNP D (indicated by their molecular masses). (D) Northern blots showing decay of $beta$ -globin mRNA (BBB) in NIH 3T3 B2A2 cells expressing individual isoforms of hnRNP D or vector only (control). To determine mRNA half-life, NIH 3T3 B2A2 cells were transiently cotransfected with a control plasmid (pSV $alpha$ -globin/GAPDH) and one of the test plasmids as indicated under each blot. Total cytoplasmic mRNA was isolated at various time intervals after serum stimulation of quiescent cells and analyzed by Northern blot analysis. Transcription of BBB+ARE^fos or BBB mRNA was driven by the serum-inducible c-fos promoter. The control mRNA ( $alpha$ -globin/GAPDH) was expressed constitutively and served as an internal standard. The times given at the top correspond to hours after serum stimulation. Poly(A) RNA was prepared in vitro by treating RNA samples from the 1-h time point with oligo(dT) and RNase H. The positions corresponding to 1,230 and 984 nt are indicated.

In view of these observations, several critical issues arise concerning the in vivo relationships among AREs, ARE-BPs, andmolecular mechanisms controlling ARE-mediated mRNA decay. Forexample, what are the critical features of AREs that are recognizedin vivo by different ARE-BPs? Do all ARE-BPs share similar bindingspecificities in vivo and thereby indiscriminately regulate thefunction of all AREs, or do they regulate a specific class ofAREs or even a particular ARE in a cell-specific manner in responseto environmental cues? What role(s) does each ARE-BP play in ARE-mediatedturnover? In theory, ARE-BPs could play a destabilizing or stabilizingrole or even dual roles in vivo. For instance, their associationwith an ARE could promote assembly of a decay complex necessaryfor RNA destabilization in the cytoplasm. Alternatively, theirbinding could prevent the formation of such a decay complex, thusleading to RNA stabilization. A relevant question is whether ARE-BPschange their RNA binding affinity or specificity, e.g., via interactionwith other proteins in vivo, thus playing multiple roles in mRNAturnover involving decay pathways other than the ARE-directedpathway.

In an effort to address these issues, we investigated the roles of hnRNP D in controlling mRNA decay directed by two distinctdecay pathways involving the ARE and the c-fos coding determinants.We showed that hnRNP D plays dual roles in ARE-mediated RNA turnoverin a cell-type-specific manner: a stabilizing role observed inNIH 3T3 cells (this study) and a destabilizing role identifiedpreviously in K562 cells (25). In contrast to indiscriminatebinding of hnRNP D to AREs observed in vitro using E. coli recombinantproteins, we found that its in vivo action on AREs is selective.hnRNP D effectively down-regulates the destabilizing functionof class II AREs containing multiple clustered AUUUA motifs. Thedata provide a molecular basis that explains how class II ARE-containingcytokine mRNAs are differentially stabilized in lymphocytes andin lymphoid cells as described above. Moreover, there exists asignificant difference among the four isoforms of hnRNP D in termsof their stabilizing effect on ARE-mediated decay with the followingrank order: p37 $>=$ p42 > p45 $>=$ p40. It was striking to find thatall hnRNP D isoforms are able to inactivate the rapid RNA decaydirected by the c-fos protein-coding region that is distinct fromthe ARE. Our experiments further indicate that distinct mechanismsunderlie the blockage by hnRNP D of these two mRNA decay pathways.Thus, our study identified a potential mechanism by which hnRNPD isoforms differentially and selectively regulate cytoplasmicmRNA turnover. Our results suggest that hnRNP D serves as a keyfactor broadly involved in mRNA decay directed by many differentstabilitydeterminants.

	MATERIALS AND METHODS

Top Abstract Introduction Materials and Methods Results Discussion References

Plasmid construction. The construction of plasmids pSV $alpha$ 1/GAPDH, pBBB, pBBB+ARE^c-fos, pBBB+ARE^GM-CSF, pBBB+ARE^c-jun, pBBB+ARE^c-myc, pBBB+ARE^Syn2, pBBB+ARE^GM1, pBBB+ARE^TNF-, pBBB+ARE^fII/jIII, pTet-Myc-Ovep, and pT3ARE^fos has been described previously (4, 5, 31, 38, 46,48). Plasmids expressing different isoforms of myc-tagged hnRNPD were generated in the following steps. For plasmids pTet-Myc-p40and pTet-Myc-p45, which express the p40 and p45 isoforms, respectively,a standard PCR was performed to amplify the protein-coding regionof the hnRNP D cDNA portion, using pET21(c)-cDx7His6 and pET21(c)-cDx9His6as templates, which were kindly provided by F. Ishikawa (18).The PCR-amplified fragments were digested with SalI and EcoRVand then inserted into SalI-EcoRV-digested pTet-Myc-Ovep to createan in-frame fusion of hnRNP D downstream of the myc-tag. To constructpTet-Myc-p37 and pTet-Myc-p42, the BglI-BglII DNA region containingthe C-terminal alternatively spliced sequence of hnRNP D cDNA(Fig. 1) present in pTet-Myc-p40 and pTet-Myc-p45 was replacedwith the BglI-BglII DNA region from pcDNA3.AUF37, which lacksthe C-terminal alternatively spliced sequence (kindly providedby G. Brewer) (49). The proper in-frame insertion of AUF1 cDNAswas confirmed by DNA sequencing. To generate the plasmid pT₃ARE^GM63, a BstXI (fill-in)-BglII fragment covering the 63-bp ARE regionfrom plasmid pBBB+ARE^GM-CSF was subcloned into the unique BamHI site of plasmid pT₃/T_7-18(Gibco BRL). Plasmid pT7fos was kindly provided by InderVerma.

RNA blot analysis and preparation of NIH 3T3 cytoplasmic and nuclear extracts. Cell culture, DNA transfection, isolation of total cytoplasmic RNA, Northern blot analysis, and lysate preparation were conductedas described previously (26, 39). Briefly, NIH 3T3 B2A2 cellsstably harboring the tetracycline-responsive trans-activator (tTA)(47) were transfected for $approx$ 16 h with a total of 20 µg of DNAwhich included 3 µg of pBBB+ARE, 3 µg of pTet-Myc-hnRNP D isoformor vector (pTet-Myc-Ovep) (31), 2 µg of pSV $alpha$ 1/GAPDH, and enoughcarrier plasmid pT₃/T_7-18 (Gibco BRL) to make a final amountof 20 µg of DNA. The cells were then serum starved for 25 h followedby stimulation with 20% bovine serum (Gibco BRL). Total cytoplasmicRNA was extracted at time intervals according to time course experiments.Gene-specific DNA probes were prepared by the method of randomoligonucleotide priming for Northern blot analysis. The ³²P-labeled probes were produced by inclusion of [ $alpha$ -³²P]dCTP (>6,000 Ci/mmol; DuPont). All experiments described herewere repeated at leastonce.

For lysate preparation, two plates of transfected cells (15-mm-diameter culture dish) were pooled together and then splitinto two portions: one for cytoplasmic RNA extraction and theother for preparing cytoplasmic and nuclear extracts as describedpreviously (31). Protein concentrations were analyzed by usinga bicinchoninic acid protein assay reagent (Pierce). These proteinsamples were used in Western blot analysis and gel mobility shiftand supershiftassays.

Western blot analysis. Cytoplasmic or nuclear lysates were resolved on a sodium dodecyl sulfate-12% polyacrylamide gel and analyzed by using an ECLWestern blotting kit (Amersham, Arlington Heights, Ill.). Theblots were probed with specific antibodies as described elsewhere(see the legends for Fig. 2 and 4). The antibody for the myc tagwas obtained by collecting culture medium from hybridoma cells(9E10; American Type Culture Collection) (8) and was used ata 1:100 dilution. The purified monoclonal antibody (MAb) against $alpha$ -tubulin (DM1A) was purchased from Sigma and was used at a 1:20,000dilution as a positive control for cytoplasmic protein preparations.The antibody against the U1 70K (mouse immunoglobulin G) was kindlyprovided by Sue Berget and was used at a 1:100 dilution as a positivecontrol for nuclear proteinpreparations.

Immunofluorescence microscopy study. Indirect immunofluorescence microscopy was conducted as described previously (31). Briefly, NIH 3T3 B2A2 cells were grownon coverslips and transfected with plasmids expressing individualmyc-tagged isoforms of hnRNP D or vector only. After 48 h, cellswere fixed with 100% methanol, permeabilized with 0.5% TritonX-100, and then stained using a MAb against myc epitope tag (9E10)as primary antibody. The secondary antibody for anti-mouse-immunoglobulinG (purchased from Sigma) was coupled to fluorescein isothiocyanate.All images were viewed and captured by a Spot-Digital camera (Diagnostics)and processed for publication at 300 dots per in. using AdobePhotoShop (version 4.0)software.

Analysis of RNA-protein interactions. RNA probe synthesis, gel mobility shift assays, and antibody supershift assays were carried out as described previously (7,48). In vitro transcription using HindIII-linearized pT₃ARE^c-fos (48), EcoRI-linearized pT₃ARE^GM63, or BlpI-linearized pT7fos as template was carried out to synthesizeRNA probes for the c-fos ARE, GM-CSF ARE, or c-fos coding regions.Briefly, cytoplasmic lysate (8 µg of protein) and ³²P-labeled RNA (1 ng) were incubated at room temperature for 15min in a buffer containing 10 mM HEPES (pH 7.6), 3 mM MgCl₂, 40mM KCl, 2 mM dithiothreitol, 10% glycerol, and 0.5% IGAPEL CA-630.Heparin (5 µg/ml, final concentration) and yeast total RNA (200ng/ml, final concentration) were added to reduce nonspecific binding.The volume of each reaction mixture was 10 µl. Subsequently, unboundRNA was digested by including 0.6 U of RNase T1 (Calbiochem, SanDiego, Calif.) for 20 min at room temperature. RNA-protein complexeswere resolved in 6% nondenaturing polyacrylamide gels. To performgel mobility supershift analyses, following RNA-protein bindingand RNase T1 digestion, 3 µl of a MAb against myc tag (9E10) wasadded into the binding reaction mixture. After a 15-min incubationat room temperature, RNA-protein-antibody complexes were resolvedin 6% nondenaturing polyacrylamidegels.

	RESULTS

Top Abstract Introduction Materials and Methods Results Discussion References

Different isoforms of hnRNP D variably inhibit decay of mRNA bearing the c-fos ARE in NIH 3T3 cells. Previously, we demonstrated in K562 cells that hnRNP D has a destabilizing role in ARE-mediated mRNA decay (25). We showedthat following hemin-induced erythroid differentiation of K562human erythroleukemia cells, ARE-containing mRNAs are stabilized.Ectopic expression of hnRNP D in hemin-treated K562 cells wasable to restore rapid decay of ARE-containing mRNA. However, whenhnRNP D was ectopically overexpressed in non-hemin-treated proliferatingK562 cells, it had no effect on the decay of ARE-containingmRNA.

To explore the possibility that hnRNP D's function in ARE-mediated decay may be cell-type dependent, we examined the decayof $beta$ -globin mRNA bearing a 3' UTR c-fos ARE (BBB+ARE^c-fos) in the presence of ectopically overexpressed hnRNP D in NIH3T3 cells. NIH 3T3 cells were transiently cotransfected with theBBB+ARE^c-fos plasmid and a plasmid expressing an N-terminally myc-epitope-taggedhnRNP D isoform. Because hnRNP D cDNA is driven by the tetracycline-regulatedpromoter system, an NIH 3T3 stable cell line termed B2A2, whichexpresses the tetracycline-responsive trans-activator (tTA) inthe absence of tetracycline (47), was used in our transfectionexperiments. BBB+ARE^c-fos mRNA was transiently transcribed from the c-fos promoter afterserum induction of the growth-arrested B2A2 cells, which alloweddetermination of mRNA decay without using a transcription inhibitorto inhibit transcription (47). The decay of BBB+ARE^c-fos was monitored in transiently transfected B2A2 cells constitutivelyexpressing myc-tagged hnRNP D in the absence of tetracycline.The results showed that rapid deadenylation and decay of BBB+ARE^c-fos mRNA in the cytoplasm is significantly impeded when the p37 orp42 isoform is overexpressed, but it is only modestly affectedby p40 or p45 (Fig. 1). In contrast, BBB+ARE^c-fos mRNA is not affected when a cloning vector without hnRNP D cDNAis overexpressed (Fig. 1). These results showed that hnRNP D caninhibit ARE-mediated mRNA decay and that the extent of inhibitionvaries among different isoforms in the following rank order: p37 $>=$ p42 > p45 $>=$ p40. This order is consistent with the relativeaffinities of hnRNP D isoforms for the ARE determined by in vitrostudies using recombinant proteins (10, 11, 44). These resultsdiffer markedly from our previous finding in K562 cells (25)and demonstrate that hnRNP D can exert opposite effects on ARE-mediateddecay, depending on cell type and cell physiologicalconditions.

As a control for the specificity of hnRNP D's inhibitory effect on ARE-mediated mRNA decay, a parallel experiment measuringthe decay of $beta$ -globin mRNA (BBB) bearing no specific destabilizingelement was also carried out in B2A2 cells overexpressing individualisoforms. The results (Fig. 1D) showed that when $beta$ -globin mRNAdoes not contain any destabilizing element, its deadenylationand decay are not affected by ectopic overexpression of hnRNPDisoforms.

Characterization of expression levels and subcellular distributions of hnRNP D isoforms. To ascertain that differential stabilization effects displayed by different isoforms are not a result of their different levelsof protein expression and/or subcellular localization, cytoplasmicand nuclear extracts were prepared from B2A2 cells transientlytransfected with individual hnRNP D isoforms. Western blot analysisusing a MAb against myc-epitope tag (9E10) (Fig. 2A) showed nosignificant difference in expression levels among the four ectopicallyexpressed isoforms in the cytoplasm or in the nucleus. No cross-contaminationbetween the nuclear extract and cytoplasmic extract was detected,as demonstrated by exclusive detection of $alpha$ -tubulin in the cytoplasmicextracts and U1 70K splicing factor in the nuclear preparations.We thus concluded that the different decay-impeding effects onthe c-fos ARE displayed by hnRNP D isoforms in vivo are not dueto their different levels of expression in the cytoplasm.

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FIG. 2. Expression levels and subcellular distributions of human hnRNP D isoforms in mouse NIH 3T3 cells. (A) Western blot analysis. Cytoplasmic (C) and nuclear (N) lysates prepared from NIH 3T3 B2A2 cells, transfected without (control) or with individual plasmids containing myc-tagged isoforms of hnRNP D, were resolved on a sodium dodecyl sulfate-12% polyacrylamide gel. The blot was probed with a MAb against myc-epitope tag (9E10) (for hnRNP D proteins) and a control MAb against $alpha$ -tubulin (for cytoplasmic lysate) as well as a control polyclonal antibody against U1 70K (for nuclear lysate). (B) Indirect immunofluorescence microscopy study with the 9E10 MAb showing the subcellular distribution of hnRNP D isoforms (depicted by their molecular masses) and control. Both phase contrast (upper panels) and immunofluorescence (lower panels) views are shown.

Indirect immunofluorescence was also performed using the 9E10 MAb against myc-epitope tag to further evaluate the subcellulardistributions of hnRNP D isoforms. NIH 3T3 B2A2 cells were grownon coverslips and were transiently transfected with individualmyc-tagged hnRNP D isoform constructs. The results showed thatall ectopically expressed isoforms were located in both the nucleusand the cytoplasm (Fig. 2B). These results are consistent withthe Western blot analysis of cell fractionation (Fig. 2A) andare also consistent with the isoforms being nucleocytoplasmicshuttlingproteins.

Ectopic overexpression of hnRNP D differentially stabilizes mRNAs containing different AREs. To investigate whether hnRNP D differentially regulates the mRNA decay mediated by different classes of AREs in vivo, we performedtime course experiments to monitor the decay of $beta$ -globin mRNAbearing the GM-CSF ARE (class II) and the c-jun ARE (class III)in B2A2 NIH 3T3 cells that ectopically overexpress individualmyc-tagged hnRNP D isoforms. The results (Fig. 3) showed thatall four isoforms display a more profound impeding effect on therapid decay of BBB+ARE^GM-CSF mRNA than their corresponding effect on the decay of BBB+ARE^c-fos mRNA. In contrast, none of the isoforms showed a significantstabilizing effect on the decay of BBB+ARE^c-jun. The poly(A) shortening of BBB+ARE^GM-CSF is significantly impaired, which then prevents decay of the RNAbody. Taken together, our data show that hnRNP D differentiallyinhibits RNA decay mediated by the three classes of AREs in vivowith the following rank order of effect: class II ARE > classI ARE $>=$ class III ARE. There is a positive correlation betweenthe decay-impeding effect on AREs by hnRNP D and the numbers ofAUUUA motifs within AREs.

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FIG. 3. Ectopic expression of human hnRNP D isoforms in mouse NIH 3T3 cells effectively blocks class II ARE- and not class III ARE-mediated mRNA decay. RNA blots show deadenylation and decay of $beta$ -globin mRNA bearing a class II ARE (BBB+ARE^GM-CSF) (A) or bearing a class III ARE (BBB+ARE^c-jun) (B) in the absence (control) or presence of ectopically expressed individual isoforms of hnRNP D (indicated by their molecular masses). Semi-log plots show the effects of four hnRNP D isoforms on mRNA decay directed by the GM-CSF ARE (A) or c-jun ARE (B). Cell culture, transfection, gene expression, RNase H treatment, and quantitation of mRNA and data plotting were as described in the legend to Fig. 1.

The presence of multiple copies of pentanucleotide AUUUA in an ARE correlates with strong in vitro interactions between an ARE and 3T3 cell-made hnRNP D. To further address the importance of AUUUA motifs in determining the differential stabilization effects upon an ARE by hnRNPD, we conducted gel mobility shift assays using whole cytoplasmicextracts containing individual myc-tagged isoforms. Gel mobilityshift assays were carried out using uniformly ³²P-labeled GM-CSF ARE, c-fos ARE, or c-jun ARE RNA. To better assessRNA-protein complexes formed between the myc-tagged exogenoushnRNP D and ARE RNA substrate, antibody-supershift assays using9E10 MAb against the myc-epitope tag were also performed in parallel.The results showed that GM-CSF ARE formed discernible new complexeswith exogenous hnRNP D proteins (Fig. 4) that were readily super-shiftedby MAb 9E10. In addition, c-fos ARE also supports new complexformation, albeit weakly, when lysates containing myc-tagged p37or p42 are used. It appears that both p37 and p42 support moresignificant RNA-protein complex formation than either p40 or p45.In contrast, no RNA-protein complex can be detected by these assayswhen using a c-jun ARE probe (data not shown). The results fromour in vitro studies using hnRNP D proteins made in NIH 3T3 cellsare consistent with our in vivo studies showing that wild-typehnRNP D can discriminate among different classes of AREs and exertsits differential decay-impeding effect in the following rank order:GM-CSF ARE (class II) > c-fos ARE (class I) $>=$ c-jun ARE (classIII).

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FIG. 4. In vitro interactions of hnRNP D isoforms with different AREs correlate with the copy number of AUUUA motifs in AREs. ³²P-labeled RNA transcribed in vitro from human GM-CSF ARE (A) or c-fos ARE (B) was incubated with cytoplasmic lysates from NIH 3T3 B2A2 cells transfected with individual plasmids expressing vector or myc-tagged hnRNP D isoforms. The RNA substrate was incubated with cytoplasmic lysate followed by RNase T1 digestion. The digestion mixtures were left alone ( $-$ ) or further incubated in the presence of MAb against the myc-epitope tag (+9E10) as indicated on the top of each lane. The final reaction mixtures were analyzed by electrophoresis in a 6% nondenaturing polyacrylamide gel. New complexes (asterisks) and supershifted complexes (brackets) are as indicated.

A cluster of overlapping AUUUA motifs observed in class II AREs is a key feature recognized in vivo by hnRNP D for its negative effect on mRNA decay. The above results suggested that multiple overlapping AUUUA motifs found in class II AREs are a key feature recognized byhnRNP D. To test this possibility, we performed two lines of experiments.First, the destabilizing function of three additional AREs, thec-myc ARE from class I, the TNF- $alpha$ ARE from class II, and a syntheticnon-AUUUA ARE (fII/jIII) (32) representing class III, was examinedin B2A2 cells constitutively expressing the p37 isoform of hnRNPD. The results (Fig. 5A) showed that p37 has a very drastic stabilizingeffect on the class II TNF- $alpha$ ARE, whereas it has little effecton the non-AUUUA ARE. The class I c-myc ARE was moderately affected.This rank order of stabilization on three additional AREs by hnRNPD is consistent with the results in Fig. 1 and 3.

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FIG. 5. hnRNP D isoforms effectively inhibit class II ARE-mediated mRNA decay by recognizing multiple overlapping AUUUA motifs. (A) RNA blots and semi-log plots showing decay of BBB+ARE mRNAs representing individual classes of AREs in NIH 3T3 B2A2 cells expressing p37 isoform (+p37) or vector (control). (B) RNA blots and semi-log plots showing decay of BBB mRNAs containing a mutant GM-CSF ARE (GM1, class I ARE) and a synthetic ARE representing a class II ARE in NIH 3T3 B2A2 cells expressing the p37 isoform of hnRNP D (+p37) or vector (control). Open rectangles and oval symbols in both panels depict AREs and AUUUA motifs, respectively. Cell culture, transfection, RNase H treatment, and quantitation of mRNA and data plotting were as described in the legend to Fig. 1.

Second, to further substantiate this correlation and determine whether clustering of AUUUA motifs is critical, two additionalAREs were tested. The first was a mutant GM-CSF ARE (GM1) withthree point mutations that knock out the clustering of multipleAUUUA motifs (46). This manipulation transformed the GM-CSFARE from class II, with seven copies of clustered AUUUA motifs,into class I, with four copies of scattered AUUUA motifs. Thesecond ARE, termed syn2, is a synthetic class II ARE consistingof a 54-nt 5' spacer and a 3' sequence with a cluster of threeAUUUA motifs. The 54-nt spacer has no destabilizing effect byitself, whereas the 3' AUUUA cluster is the key sequence featurethat constitutes the destabilizing function for syn2 ARE (46).The results (Fig. 5B) showed that the rapid decay of BBB+ARE^syn2 is nearly completely blocked by p37, whereas BBB+ARE^GM1, like two other class I ARE-containing messages that we tested(BBB+ARE^c-fos and BBB+ARE^myc), is only moderately stabilized by p37. Taken together, we concludefrom these separate lines of evidence that hnRNP D inhibits classII ARE-mediated mRNA decay by recognizing multiple overlappingAUUUA motifs. It has only a moderate stabilization effect on classI AREs that contain a few scattered copies of the AUUUAmotif.

hnRNP D isoforms inhibit the rapid decay of a reporter mRNA bearing the c-fos protein-coding region. Given the above results and previous in vitro studies concerning specific binding of hnRNP D to AREs, it is intriguing thathnRNP D was recently shown to be an integral component of a compleximplicated in rapid mRNA decay directed by the c-fos major codingdeterminant, a purine-rich sequence element in the protein-codingregion (15). One implication of that study is that hnRNP D mayhave a general role in mRNA turnover and may participate in mRNAturnover that does not involve direct binding to a stability determinant.Therefore, we asked whether hnRNP D might regulate RNA decay directedby the entire c-fos protein-coding region, which contains multipleRNA determinants of instability including the major coding determinant(35). To test this possibility, the rapid decay of a hybridmessage (BFB) consisting of the $beta$ -globin 5' and 3' UTRs and theentire c-fos protein-coding region (40) was monitored in B2A2cells that constitutively overexpress individual hnRNP D isoforms.The results (Fig. 6) showed dramatic stabilization of BFB mRNAby all four isoforms, which is different from the differentialeffects seen with AREs. In contrast, overexpression of anotherARE-binding protein, HuR, had little effect on the rapid decayof BFB mRNA. It is of particular significance that hnRNP D isoformsspecifically block decay of BFB transcript, whereas they haveno effect on the decay of $beta$ -globin mRNA bearing no specific decaydeterminant described above (Fig. 1D). These experiments demonstratedthe participation of hnRNP D in mRNA turnover mediated by distinctRNA destabilizing elements.

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FIG. 6. All hnRNP D isoforms effectively block mRNA decay directed by the c-fos coding region instability determinants. (A) RNA blots showing decay of a hybrid mRNA containing the entire c-fos protein-coding region (BFB) in NIH 3T3 B2A2 cells expressing individual isoforms of hnRNP D, HuR (another ARE-BP), or vector (control). Due to comigration of BFB and $alpha$ -globin control mRNAs, blots were first probed with c-fos coding region probe (for BFB message) and then stripped and reprobed with $alpha$ -globin-specific probe (for control message). (B) Semi-log plot showing decay of BFB mRNA. Cell culture, transfection, RNase H treatment, and quantitation of mRNA and data plotting were as described in the legend to Fig. 1.

Different mechanisms underlie the stabilization effect of hnRNP D on the ARE-mediated and c-fos coding determinant-directed decay pathways. To test whether hnRNP D binds directly to the c-fos coding determinants, gel mobility and antibody super-shift assays werecarried out using an RNA probe spanning the entire c-fos openreading frame and B2A2 cell lysate containing individual hnRNPD isoforms. The results (data not shown) showed that all isoformsfailed to support the formation of any RNA-protein complexes thatcould be readily super-shifted by the anti-myc MAb (9E10). Theyall showed a gel-shift pattern identical to that of the controllysate (data not shown). To further substantiate that hnRNP Ddoes not bind directly to the c-fos protein-coding region, theunlabeled c-fos protein-coding-region RNA was used as a competitorin the gel mobility shift assay. The results (Fig. 7) showed thatan increasing amount of c-fos coding-region RNA does not abolishformation of RNA-protein complexes between the ³²P-labeled GM-CSF ARE and myc-tagged p37 in the lysate, whereasthe cold GM-CSF ARE competes well. We concluded from these twoseparate lines of evidence that hnRNP D synthesized in NIH 3T3cells does not bind directly to the c-fos coding region to exertits stabilizing effect in vivo, indicating that different mechanismsunderlie the stabilization effect of hnRNP D of the ARE-mediatedand c-fos coding-determinant-directed decay pathways.

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FIG. 7. Ectopically expressed human hnRNP D isoforms do not directly interact with the c-fos coding region in vitro. ³²P-labeled RNA transcribed in vitro from human GM-CSF ARE was incubated with cytoplasmic lysates in the presence of increasing amounts of either unlabeled GM-CSF ARE or unlabeled c-fos coding region transcript as competitor. The binding mixtures were analyzed by electrophoresis on a 6% nondenaturing polyacrylamide gel. Gel mobility shift and antibody-supershift assays were carried out as described in the legend to Fig. 4.

	DISCUSSION

Top Abstract Introduction Materials and Methods Results Discussion References

hnRNP D has dual roles in cytoplasmic mRNA decay in a cell-type-specific manner. In this study, we made several findings that provide a molecular basis to explain how differential degradation of mRNAs bearingdifferent classes of AREs may be regulated by specific ARE-BPs.The findings also have general implications for the function ofARE-BPs and their target AREs in vivo. Our experiments showedthat hnRNP D has both a positive and a negative role in ARE-mediatedRNA turnover: a stabilizing role observed in NIH 3T3 cells (thisstudy) and a destabilizing role previously identified in K562cells (25). The contrasting effects of hnRNP D exhibited inNIH 3T3 fibroblasts versus K562 erythroleukemic cells indicatethat hnRNP D's function in RNA turnover is regulated in a cell-type-specificmanner.

In vivo discrimination among three different classes of AREs by hnRNP D. In contrast to a relaxed binding specificity for AREs observed in vitro using recombinant proteins synthesized in E. coli(1, 10, 44), hnRNP D discriminates among the three differentclasses of AREs in vivo. It most effectively down-regulates thedestabilizing function of class II AREs via recognition of multipleoverlapping AUUUA motifs. Consistent with our in vivo characterizations,our in vitro gel-shift assays using cytoplasmic extracts preparedfrom NIH 3T3 cells that overexpress individual hnRNP D isoformsalso showed a similar discrimination among different classes ofAREs. The discrepancy between our results and other in vitro bindingstudies using recombinant proteins could be due to the lack ofposttranslational modifications of recombinant hnRNP D, such asmethylation or phosphorylation (49), and/or the absence of specifichnRNP D-interacting proteins that modulate its ARE-binding specificityand affinity. Thus, our data suggest that in vivo these modificationsand/or interactions are critical for fine-tuning hnRNP D's functionsin cytoplasmic mRNAturnover.

Distinct roles for hnRNP D isoforms in the differential regulation of mRNA decay. The differential regulation of mRNA turnover by hnRNP D isoforms observed in our experimental system defines a potential mechanismof hnRNP D isoform-specific regulation of mRNA turnover. Our datashow that a significant difference exists among four hnRNP D isoformsin their ability to inhibit ARE-mediated decay in NIH 3T3 cellswith the following rank order: p37 $>=$ p42 > p45 $>=$ p40. Surprisingly,all hnRNP D isoforms are equally capable of blocking the rapidRNA decay directed by another mRNA stability determinant, i.e.,the c-fos protein-coding region, which does not share any significantsequence similarity with the AREs. Thus, p40 and p45 isoformshave the ability to down-regulate the destabilizing function ofthe c-fos protein-coding determinants without affecting that ofthe ARE. This implies that these two isoforms could be used toselectively increase the stability of c-fos mRNA without affectingother ARE-containing mRNAs. On the other hand, p37 or p42 couldstabilize c-fos mRNA even more by blocking the destabilizing functionof both the ARE and coding region determinant without affectingclass III (non-AUUUA) ARE-containing mRNAs, such as c-jun mRNA.This point is of particular significance given that the expressionof c-fos mRNA is frequently induced along with a large group oflabile early-response-gene mRNAs and cytokine mRNAs that containan ARE in their 3' UTRs (2, 14, 37). It will be interestingfor a future study to address the physiological consequence andsignificance of producing different isoforms of hnRNP D that displaydifferential binding to AREs and c-fos codingdeterminants.

What might be the structural basis for the isoform-specific effects observed? It is interesting that both p37 and p42 lackan N-terminal peptide insertion that is alternatively includedin the mRNAs encoding p40 and p45 during pre-mRNA splicing ofhnRNP D (Fig. 1). In vitro studies showed that the alternativelyspliced peptide inserted in the first RRM, found in p40 and p45,interferes with their ability to bind target RNA sequences (18).The significance of this structural difference observed in vitrois supported by our in vivo functional characterizations. We showedthat p37 and p42 are much more effective than p40 and p45 in inhibitingARE-mediated mRNA decay in NIH 3T3 cells (this study) or in rescuingARE-directed decay in K562 cells that have been induced for furthererythroid differentiation by hemin (25). On the other hand,the potent inhibition of the c-fos coding-determinant-directedmRNA decay by all hnRNP D isoforms may thus involve common domainspresent in all four isoforms. Functional dissection of hnRNP Dshould shed light on the relationship between the structure andfunction of hnRNPD.

A critical issue concerning hnRNP D is the specificity of its inhibitory effect on mRNA decay, given that hnRNP D blocks thefunction of two distinct RNA decay determinants. The followinglines of evidence support a specific regulatory role rather thana nonspecific stabilization effect for hnRNP D. First, HuR, anARE-BP exhibiting a binding affinity similar to that of hnRNPD in vitro (27), has no effect on the c-fos coding-determinant-mediateddecay (Fig. 6). Second, the p40 isoform has essentially no effecton ARE-mediated decay but dramatically blocks the rapid decaydirected by the c-fos coding region. Third, ectopic overexpressionof hnRNP D in proliferating K562 cells does not inhibit ARE-mediateddecay, suggesting a cell-type-specific effect. Fourth, hnRNP D'seffect on AREs is class specific in that it has little effecton class III AREs. Lastly, ectopic overexpression of hnRNP D specificallyimpairs the deadenylation step of the $beta$ -globin mRNA bearing eitheran ARE or the c-fos coding region but has no such effect on the $beta$ -globin mRNA alone, demonstrating that hnRNP D's effects on deadenylationrequire specific RNA stabilitydeterminants.

The negative effect by hnRNP D on mRNA decay mediated by the ARE and the c-fos coding determinants involves two distinct mechanisms. Given that hnRNP D does not bind directly to the coding sequence and there is no sequence similarity between the ARE and thec-fos coding sequence, how might p37 isoform exert its inhibitoryeffect on the two very distinct destabilizing elements? In thecase of AREs, it is possible that stabilization is effected viadirect binding of hnRNP D to an ARE, preventing the assembly ofa decay complex necessary for rapid deadenylation and decay. Forcoding determinants whose function is coupled to translation,a few possibilities may be envisaged. For example, overexpressionof hnRNP D might block translation initiation, leading to blockageof deadenylation. Recently we showed that p37 isoform is an integralcomponent of a multiprotein complex that bridges the interactionbetween the major c-fos coding determinant and the 3' poly(A)tail (15). Deadenylation and decay of the coding-determinant-containingmRNA is induced by disruption or reorganization of the complexas a result of ribosome transit following translation initiation.However, our results from sucrose gradient fractionation experimentsshowed no change of polysome profiles between the absence or presenceof ectopically overexpressed p37 (data not shown), arguing againstthe notion of blockage of translation initiation. As our dataalso demonstrate that there was no direct binding of hnRNP D tothe coding determinants, they point to a possibility of hnRNPD's direct interference with deadenylation activity. For instance,overexpression of hnRNP D affects the efficient recruitment ofa critical factor, e.g., poly(A) nuclease (PARN/DAN) (9, 20),by the coding determinant. Or, overexpression of hnRNP D causesthe formation of an aberrant bridging complex and/or mRNP structurethat is unable to direct deadenylation. While the precise mechanisminvolved awaits further experimentation, our results clearly indicatethat hnRNP D employs at least two distinct mechanisms for controllingmRNAturnover.

Our findings also have an important implication in that hnRNP D may serve as a global factor in controlling general mRNA turnoverin mammalian cells rather than a factor only involved in ARE-mediateddecay. This notion is also supported by two other recent studies.In one study, hnRNP D was found in an RNA-protein complex necessaryfor the stability of $alpha$ -globin mRNA (19). In the other study,p45 isoform was found in RNA-protein complexes formed with a 390-ntdestabilizing sequence from the 3' UTR of cyclin D1 mRNA (23).Significantly, neither RNA stability determinant contained AUUUAmotifs.

Molecular mechanism for selective stabilization of cytokine mRNAs. Since class II AREs are primarily found in mRNAs coding for cytokines, our results provide evidence that hnRNP D, particularlythe p37 and p42 isoforms, may serve as a major ARE-BP that contributesto the transient up-regulation of cytokines during a broad rangeof immune and stress responses. For example, one scenario forhnRNP D acting as a negative regulator is that an up-regulationof levels of p37 or p42 in the cytoplasm during, e.g., T-celland mast cell activation (24, 30), specifically leads to bindingto and then stabilization of the class II ARE-containing cytokinemRNAs, such as GM-CSF, TNF- $alpha$ , and IL-3, without affecting mRNAscontaining other classes of AREs, such as c-fos and c-myc mRNAs.The question then becomes how such up-regulation of hnRNP D expressionmay be elicited. A few recent studies showing alterations of thestability of ARE-containing mRNAs in response to the activationof specific signaling transduction pathways point to the involvementof these signaling pathways in controlling ARE and ARE-BP functions.One study showed that activation of p38 mitogen-activated proteinkinase induced by proinflammatory cytokines specifically inhibitedARE-mediated mRNA decay (45). In another case, the ionomycin-inducedactivation of the c-Jun N-terminal kinase (JNK)-stress-activatedkinase pathway in mast cells was shown to be necessary for stabilizingIL-3 mRNA, a class II ARE-containing mRNA (28). Significantly,the role of IL-3 AREs cannot be substituted by class I AREs fromeither c-fos or c-myc. It will be important to investigate whetherthe multiple yet distinct roles played by hnRNP D in mRNA turnoverare controlled by phosphorylation-dephosphorylation and to identifythe relevant kinase and phosphatase responsible for those directmodifications. Further light may be shed on the roles of individualisoforms of hnRNP D by using transgenic mice that lack or overlyexpress specific isoforms of hnRNPD.

	ACKNOWLEDGMENTS

We thank R. Kulmacz, C. S. Raman, F. R. Cabral, and M. Wilkinson for critical reading of the manuscript and their valuablecomments, S. Berget for anti-U1 70K antiserum, G. Brewer for AUF1plasmids, F. Ishikawa for hnRNP D₀ plasmids, and I. Verma forthe T7fosplasmid.

This work was supported by a grant from the National Institutes of Health (GM 46454) to A.-B.S. A.-B.S. was the recipientof an American Heart Association Established InvestigatorAward.

	FOOTNOTES

^* Corresponding author. Mailing address: Department of Biochemistry and Molecular Biology, The University of Texas Houston MedicalSchool, Houston, TX 77030. Phone: (713) 500-6068. Fax: (713) 500-0652.E-mail: Ann-Bin.Shyu{at}uth.tmc.edu.

REFERENCES

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
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