Somatic mRNA Turnover Mutants Implicate Tristetraprolin in the Interleukin-3 mRNA Degradation Pathway

doi:10.1128/MCB.20.11.3753-3763.2000

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Molecular and Cellular Biology, June 2000, p. 3753-3763, Vol. 20, No. 11
0270-7306/00/$04.00+0
Copyright © 2000, American Society for Microbiology. All rights reserved.

Somatic mRNA Turnover Mutants Implicate Tristetraprolin in the Interleukin-3 mRNA Degradation Pathway

Georg Stoecklin, Xiu-Fen Ming, Renate Looser, and Christoph Moroni^*

Institute of Medical Microbiology, University of Basel, CH-4003 Basel, Switzerland

Received 16 December 1999/Returned for modification 25 January 2000/Accepted 8 March 2000

	ABSTRACT

Top Abstract Introduction Materials and Methods Results Discussion References

Control of mRNA stability is critical for expression of short-lived transcripts from cytokines and proto-oncogenes. Regulationinvolves an AU-rich element (ARE) in the 3' untranslated region(3'UTR) and cognate trans-acting factors thought to promote eitherdegradation or stabilization of the mRNA. In this study we presenta novel approach using somatic cell genetics designed to identifyregulators of interleukin-3 (IL-3) mRNA turnover. Mutant celllines were generated from diploid HT1080 cells transfected witha reporter construct containing green fluorescent protein (GFP)linked to the IL-3 3'UTR. GFP was expressed at low levels dueto rapid decay of the mRNA. Following chemical mutagenesis andselection of GFP-overexpressing cells, we could isolate threemutant clones (slowA, slowB, and slowC) with a specific, trans-actingdefect in IL-3 mRNA degradation, while the stability of IL-2 andtumor necrosis factor alpha reporter transcripts was not affected.Somatic cell fusion experiments revealed that the mutants aregenetically recessive and form two complementation groups. Expressionof the tristetraprolin gene in both groups led to reversion ofthe mutant phenotype, thereby linking this gene to the IL-3 mRNAdegradation pathway. The genetic approach described here shouldallow identification of the defective functions by gene transferand is also applicable to the study of other mRNA turnoverpathways.

	INTRODUCTION

Top Abstract Introduction Materials and Methods Results Discussion References

Expression of a number of cytokines, including interleukin 2 (IL-2), IL-3, granulocyte-macrophage colony-stimulating-factor(GM-CSF) and tumor necrosis factor alpha (TNF- $alpha$ ), in responseto extracellular stimuli involves transient stabilization of correspondingmRNAs, which are otherwise degraded rapidly in the cytoplasm.Transcripts of proto-oncogenes, e.g., c-myc, c-fos, and c-jun,are also very short-lived, which allows the cell to limit theirexpression to a narrow time window after receiving a mitogenicsignal. Selective degradation of these mRNAs involves recognitionof cis elements (reviewed in reference 37), is generally precededby shortening of the poly(A) tail (1), and, in some cases,appears to occur cotranslationally (17). In c-myc and c-fostranscripts, different cis elements have been identified: rapidmRNA decay is mediated by sequences in the 5' untranslated region(5'UTR), potent destabilizing elements in the coding region, andan equally important AU-rich element (ARE) located in the 3'UTR(19, 40, 46, 47). In cytokine transcripts, where the functionof the ARE was initially revealed (5, 39), it appears tobe the major destabilizing element. In the case of IL-3, pointmutations in the ARE are sufficient to stabilize the full-lengthtranscript, which implies that no additional elements mediatedestabilization (41). In general, the AREs of cytokines arecomposed of multiple, partially overlapping AUUUA pentamers, whilethose of c-myc and c-fos contain only a few AUUUA motifs in aU-rich context. A correlation between these sequence featuresand different deadenylation kinetics has allowed the classificationof AREs into types I, II, and III (7). While these cis-actingelements have been extensively studied, we are only at the beginningof understanding how the corresponding trans-acting factors targetARE-containing transcripts to the degradation machinery in a regulatedfashion. A functional role in ARE-dependent turnover control hasbeen documented at this time for a small number of genes includingthe HuR, AUF1, tristetraprolin (TTP), and von Hippel-Lindau (VHL)genes.

HuR, cloned as a gene with homology to HuD, is an RNA binding protein which can interact in vitro with the AREs of c-fos andIL-3 mRNA (26), as well as with synthetic, mRNA-destabilizingAREs (31). In vivo, overexpression of HuR caused stabilizationof reporter transcripts containing the AREs of c-fos and GM-CSF,as well as of vascular endothelial growth factor (VEGF) mRNA (11,22, 36).

AUF1 was first purified from a postribosomal supernatant by its ability to accelerate the decay of c-myc mRNA in an in vitrosystem (3, 4). Later the gene was cloned (49), but itsdestabilizing activity in vivo could be demonstrated only recently,as overexpression of AUF1 in K562 erythroleukemia cells antagonizedthe stabilizing effect of hemin on reporter transcripts bearingthe AREs of c-fos and GM-CSF (24).

TTP was initially cloned from NIH3T3 cells as an immediate-early response gene (25, 45). It belongs to a small familyof zinc finger proteins which have two copies of the unusual Cys-Cys-Cys-Hiszinc finger domain. Its function was discovered in TTP knockoutmice, which develop a severe inflammatory syndrome due to an increasein TNF- $alpha$ production (43). Overproduction of TNF- $alpha$ by macrophagesderived from TTP^/ mice appeared to be the result of increased stability of TNF- $alpha$ mRNA (6). Indeed, TTP was shown to bind to the ARE of TNF- $alpha$ mRNA, and binding was dependent on the integrity of the two zincfinger domains (20).

VHL has been identified as a tumor suppressor gene which is inactivated in von Hippel-Lindau tumors and in some sporadic renalcarcinomas (21). VEGF production is elevated in these tumorsand can be suppressed under normoxic conditions by ectopic expressionof wild-type (wt) VHL. Suppression appears to occur at the posttranscriptionallevel (12) by promoting rapid degradation of VEGF mRNA (16).Recent experiments have identified VHL as a component of an E3ubiquitin-protein ligase complex (23), suggesting that VHL mightact upstream by inducing ubiquitination of a regulator that controlsrapid mRNA turnover of hypoxia-induciblegenes.

ARE-dependent control of mRNA stability involves a complex interplay between the RNA, stabilizing factors (e.g., HuR), destabilizingfactors (e.g., AUF1 and TTP), upstream regulators (e.g., VHL),and probably additional proteins which remain to be identified.As an alternative to biochemical strategies based on purificationof ARE-binding proteins, tumor cells with impaired mRNA turnoverare potentially helpful tools for a functional approach. Tumorswith trans-acting defects, due to lack of regulatory functions,could serve for genetic complementation and cDNA transfer experimentswhich should eventually allow the identification of the defectiveregulators. Indeed, Schuler and Cole have reported a mouse monocytictumor which expressed abnormally stable GM-CSF mRNA (38). Stabilizationoccurred in trans, since mRNA of a reporter construct containingthe 3'UTR of GM-CSF also showed a prolonged half-life. However,no further work has been reported on this model tumor. Anothersystem with similar characteristics has been developed in ourlaboratory. Tumor lines derived from v-H-ras-transformed PB-3cmast cells overexpress IL-3, which serves as a growth stimulusin an autocrine fashion (32). In some of these tumors, IL-3overproduction is the result of an IL-3 gene rearrangement thatleads to enhanced transcription. In the majority of the tumors,however, IL-3 is upregulated by stabilization of the mRNA (15,33). The corresponding mutation acts in trans, since mRNA ofa heterologous IL-3 reporter construct is also abnormally stable(14). Fusion of these tumor cells with the PB-3c precursor linesuppressed the tumor phenotype and restored rapid IL-3 mRNA decay,indicating that the mutation in these tumors is recessive (8).PB-3c and derivative tumor lines exhibit a rather low transfectionefficiency and are therefore not suitable for identification ofthe mutant genes by cDNAtransfer.

As an alternative, we decided to develop a system where cellular mutants with a defect in mRNA decay could be generated andisolated. While many mammalian regulators have been identifiedand studied in yeast mutants, this powerful approach could notbe used because the IL-3 ARE is not recognized as a destabilizingelement in yeast. Compared to haploid yeast cells, the use ofmammalian cells is less convenient for somatic genetics. Apartfrom their slower generation time, the occurrence of recessivemutants requires inactivation of both alleles and hence representsa rare event. Nevertheless, the group of G. R. Stark has succeededin isolating recessive mutants unresponsive to interferons. Themutants were generated from diploid human HT1080 fibrosarcomacells and selected in 6-thioguanine by their failure to activatean interferon-responsive guanine phosphoribosyltransferase reportergene (18, 28, 35). In the work presented here, we have adopteda modified strategy to study IL-3 mRNA turnover. Three mutantswere isolated which display a trans-acting, recessive defect inIL-3 mRNA degradation. Somatic cell fusion experiments revealedthat the mutants belong to two complementation groups. In bothgroups, ectopic expression of TTP restored rapid decay of IL-3mRNA, thereby linking this gene to the IL-3 mRNA degradationpathway.

	MATERIALS AND METHODS

Top Abstract Introduction Materials and Methods Results Discussion References

Plasmid constructs. To generate GFPIL3-wt, the 5'UTR and proximal promoter region of murine IL-3 were amplified by PCR using primers M1217 (5'-AGCTGCTTCTGATGCCT-3')and M1216 (5'-GTGGATCCTGTCTCGTTCTGGTCCT-3') and inserted as anApaI-BamHI fragment into the multiple cloning site of pEGFP-N1(Clontech). The genomic 1.9-kb HindIII-ApaI fragment upstreamof IL-3 was placed 5' to the proximal promoter. Green fluorescentprotein (GFP) linked to the IL-3 promoter was then inserted asa HindIII-XbaI fragment into the previously described vector IL3MXh-wt(41), which was cut with HindIII and XbaI. This step placedGFP under the control of the IL-3 3'UTR and introduced the hphgene, coding for hygromycin B phosphotransferase (2), as aselection marker. For the control plasmid GFPIL3-3a, the sameHindIII-XbaI fragment was inserted into IL3MXh-3a (41).

Construct HindIL3neo was made by subcloning the 2.7-kb BamHI fragment of pMAMneo (Clontech) containing a neomycin resistancegene (neoR) under the control of the simian virus 40 (SV40) promoterand polyadenylation sequences first into pGEM-3Z (Promega). Fromthis vector (pGEMneo), neoR was excised as a KpnI-SalI fragmentand inserted into pSP72 containing the 5.4-kb HindIII-EcoRI regionof murine genomic IL-3 (48). MXIL3neo was generated by ligationof the 2.7-kb BamHI fragment of pMAMneo into the AatII site ofMXIL3-wt, which contains the IL-3 gene driven by a 0.6-kb HindIII-SacIfragment of the Moloney murine leukemia virus (MMLV) long terminalrepeat (LTR) promoter (41).

For plasmid neoMX $beta$ globin-IL2, the 3'UTR of murine IL-2 was amplified by PCR using primers M1458 (5'-CAATAACATTGTACCTCCTGC-3')and M1758 (5'-AGAGGAGAGCTTTATTTCTTG-3') from cDNA of T-cell line9-6 (10). The 388-bp fragment was blunt-end ligated into theSmaI site of pSP73 (Promega). From this vector, the insert wasexcised as a BamHI-BglII fragment to replace the BglII fragmentof plasmid Mxh- $beta$ -globin-IL3 (29). Finally, the hph sequencebetween the XmnI and ClaI sites was replaced by the neoR-containingXmnI-AccI insert of pGEMneo. Similarly, the 3'UTR (763 bp) ofmurine TNF- $alpha$ was amplified by PCR using primers M1750 (5'-AAGCGATCTTTATTTCTCTC-3')and M1751 (5'-AGGGAATGGGTGTTCATCCA-3') and ligated into pSP73.For neoMX $beta$ globin-TNF $alpha$ , the HindIII-BglII fragment from Mxh- $beta$ -globin-IL3(29) was inserted into the HindIII and BamHI sites, and neoRwas introduced as describedabove.

To generate mTTP.tag, murine TTP was cloned from cDNA of NIH3T3 cells by PCR using primers M1804 (5'-ATGAATTCGCGCCACCATGGATCTC-3')and M1803 (5'-ATTCTAGACTCAGAGACAGAGATACG-3'). After digestionwith EcoRI and XbaI, the 965-bp fragment was ligated in frameinto the EcoRI and XbaI sites of pcDNA3.1/Myc-HisA (Invitrogen).The absence of mutations and presence of correct boundaries wereconfirmed bysequencing.

Cell culture and transfection. HT1080 cells were grown in Iscove's modified Dulbecco medium (IMDM) supplemented with 10% fetal calf serum (FCS), 50 µM 2-mercaptoethanol,2 mM glutamine, 100 U of penicillin/ml, and 100 µg of streptomycin/ml.Transfections were performed in 6-well plates with 1 µg of plasmidDNA and 3 µl of Lipofectamine (Gibco) following the manufacturer'sprotocol. Hygromycin (1 mg/ml), G418 (1 mg/ml), or puromycin (10µg/ml) was added 48 h later for selection of stably transfectedcells. Whenever needed, cells were subcloned by limiting dilutionin 60-well Terazaki plates to achieve uniform expression of thetransgene.

Cell fusion. To obtain hybrids with the precursor cell line, HT1080 was first transfected with pBABEpuro (30), kindly provided by H.Hirsch. This cell line could then be directly crossed either witha trans mutant (slowA, slowB, or slowC), or with the control cis-mutantHT-GFPIL3-3a, since all these mutants express hph on the GFP reporterplasmid. For intermutant hybrids, resistance to puromycin or G418was conferred by transfecting the fusion partners with eitherpBABEpuro or HindIL3neo. The following combinations were used:slowA-HindIL3neo × slowB-pBABEpuro, slowA-HindIL3neo × slowC-pBABEpuro,and slowB-HindIL3neo × slowC-pBABEpuro. In order to induce fusion,cells were trypsinized and 10⁶ cells of each partner were mixed and centrifuged. The pelletwas resuspended in 50 µl of medium, and 700 µl of 50% (wt/vol)polyethylene glycol 1500 in IMDM was added and carefully mixed.After incubation for 90 s at 37°C, 9 ml of medium was added, andcells were washed once, resuspended in 15 ml of medium, and platedin a 10 cm-dish. Twenty-four hours later, selection was startedby addition of the selection markers puromycin (10 µg/ml) andhygromycin (1 mg/ml) or puromycin and G418 (1 mg/ml). Selectionwas completed after 2 to 3weeks.

Mutagenesis and selection. Prior to mutagenesis, the optimal concentration of the frameshift mutagen was determined. HT-GFPIL3-wt cells were seeded atmedium density (2 × 10⁶ cells per 10-cm dish) and exposed for 2 h to different concentrationsof ICR191 (Sigma). Cell survival was estimated by measuring platingefficiencies after mitogen treatment, and 6 µg/ml was chosen,which corresponds to a survival rate of 15%. For mutagenesis,HT-GFPIL3-wt cells were seeded at a density of 5 × 10⁶ per 15-cm dish 1 day before treatment with ICR191 (6 µg/ml) for2 h. Cells were washed twice with medium and allowed to grow tosubconfluency for 4 to 5 days before the next round of mutagenesis.Pools 9, 10, 11, and 12 underwent 8, 10, 11, and 12 rounds,respectively.

After recovery from the last round of mutagenesis, cells were either frozen or prepared for sorting by flow cytometry usinga FACSorter (Becton Dickinson) and Cellquest software. Duringsorting, cells were kept in FCS-free medium at 4°C. A small fractionof cells (0.02 to 0.05%) displaying fluorescence emissions abovean arbitrarily chosen threshold was recovered and either expandedfor a second round of sorting or directly subcloned in 60-wellTerazaki plates using medium supplemented with 20% FCS. Eightto 10 days later, clones were examined under the fluorescencemicroscope to select candidates for furtheranalysis.

Flow cytometry. Cells were grown in 6-well dishes, trypsinized, and resuspended in 500 µl of phosphate-buffered saline (PBS) containing 5µg of propidium iodide/ml. A total of 10⁴ cells were analyzed using a FACScan (Beckton Dickinson) and Cellquestsoftware. The fluorescence of GFP was excited at 488 nm, and emissionwas measured using a 510-nm filter. Propidium iodide stainingwas detected with a 580-nm filter, which allowed exclusion ofdead cells and cellular particles during dataanalysis.

Actinomycin D chase experiments and Northern blot analysis. Cells were seeded in 10-cm dishes and grown to subconfluency, and fresh medium was added 12 to 16 h prior to blocking of transcriptionwith actinomycin D (5 µg/ml). RNA was extracted 0, 1, 2, and 3h later using the method described by N. M. Gough (13). Twenty-fivemicrograms of total cytoplasmic RNA was resolved in 1.1% agarose-formaldehydegels, blotted onto Hybond N+ membranes (Amersham) for 3 h with50 mM NaOH, hybridized at 55°C overnight in the presence of 50%formamide, and washed at 65°C as described previously (34).GFPIL3 mRNA was detected either with an SP6 RNA probe from theXbaI-EcoRI fragment of murine IL-3 cDNA directed against the 3'UTRor with an SP6 probe from the 760-bp ApaI-XbaI fragment of pEGFP-N1which spans the coding region of GFP. Full-length IL-3 mRNA wasdetected using an SP6 probe from pSP65-multi-CSF containing the368-bp HindIII-XbaI fragment located in the coding region of IL-3cDNA. $beta$ -Globin reporter mRNA was detected with an SP6 probe generatedfrom the 86-bp BglII-EcoRI fragment of rabbit $beta$ -globin. Endogenoushuman TTP (hTTP) mRNA was detected using a random-primed probefrom an hTTP cDNA template. In this case, hybridization was carriedout at 45°C, and washing at 55°C. hTTP cDNA was amplified by reversetranscription-PCR (RT-PCR) from HT1080 cells using primers M1933(5'-ATGAATTCCACTCTCGGCCGACAC-3') and M1938 (5'-ATAAGCTTCGCTGAGATCCAGCTG-3').All filters were stripped in 0.5% sodium dodecyl sulfate (SDS)at 100°C and rehybridized with an SP6 probe from a 567-bp PstIfragment of chicken $beta$ -actin. Signal intensities were quantifiedusing a PhosphorImager (Molecular Dynamics) and ImageQuantsoftware.

Western blot analysis. Cell lysates were prepared from confluent 10-cm dishes by addition of 100 µl of radioimmunoprecipitation assay (RIPA) buffer(120 mM NaCl, 50 mM Tris-HCl [pH 8.0], 1% Triton X-100, 0.5% deoxycholate,0.1% SDS) supplemented with 10 µg of aprotinin/ml, 1 mM phenylmethylsulfonylfluoride (PMSF), 10 µg of leupeptin/ml, and 10 µg of pepstatin/ml.Forty microliters of lysate was resolved on a 12% polyacrylamidegel, blotted onto an Immobilon-P (Millipore) membrane, equilibratedfor 30 min in TBS (150 mM NaCl-50 mM Tris [pH 7.5]), blocked for1 h with TBS containing 1% milk powder and 1% Tween 20, and incubatedovernight at 4°C with the mouse anti-myc antibody 9E10. The membranewas washed twice for 10 min with 0.1% Tween 20 in TBS and twicefor 10 min with blocking solution. Incubation with the secondary,alkaline phosphatase-coupled anti-mouse antibody was performedfor 30 min at room temperature, and the final washing was donewith 0.1% Tween 20 in TBS four times for 15 min. Proteins werevisualized with CDP-tar (Roche) and subsequent autoradiography.mTTP.tag migrates at approximately 46 kDa, as calculated by additionof the molecular size of murine TTP (mTTP) (43 kDa [see reference44]) and the 26 amino acid residues of the myc-Histag.

	RESULTS

Top Abstract Introduction Materials and Methods Results Discussion References

A reporter system for IL-3 mRNA turnover. With the aim of establishing a system that allowed for isolation of mutant cell lines defective in cytokine mRNA turnover,we followed a strategy where GFP, linked to the ARE-containing3'UTR of murine IL-3, served as a reporter gene in a pool of chemicallymutagenized cells. Mutants lacking a regulator of rapid mRNA decaywould overexpress GFP and hence should be selectable by flow cytometry,cloning, and subsequent analysis of reporter mRNAstability.

As target cells we chose the diploid human HT1080 fibrosarcoma cell line, which had previously been successfully used to isolatemutants defective in an interferon response pathway (28, 35).As depicted in Fig. 1A, the reporter construct (GFPIL3-wt) containsat its 5' end a 1.9-kb fragment of the murine IL-3 promoter andat its 3' end the entire 3'UTR of IL-3, including a small portionof exon 5 starting from the XbaI site. Upon stable transfectioninto HT1080 cells, GFP was expressed at low levels, and the correspondingmRNA showed the expected short half-life when transcription wasblocked by actinomycin D (Fig. 2A). Quantitation revealed thatthe mRNA decayed with an apparent half-life of about 1 h due tothe presence of the IL-3 ARE in the reporter transcript. When,as a control, construct GFPIL3-3a, whose destabilizing elementwas mutated (Fig. 1B), was used, GFP expression was elevated abouteightfold and reporter mRNA was very stable (Fig. 2B), consistentwith the effect of this mutation in PB-3c mast cells (41). Weconcluded that GFPIL3-wt-transfected HT1080 cells could serveas a reporter system to isolate trans mutants defective in mRNAdecay. Such mutants could be expected to overexpress GFP, likethe cis mutant HT-GFPIL3-3a used here as a control.

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FIG. 1. (A) Schematic representation of the reporter constructs GFPIL3-wt and -3a. GFP is flanked 5' by a 1.9-kb fragment of the IL-3 promoter and 3' by an XbaI-SpeI fragment of murine IL-3 containing part of exon 5 including the entire 3'UTR and the poly(A) site. Dark shaded box, GFP, light shaded boxes, IL-3 cDNA sequences. (B) Nucleotide sequence of the core AUUUA motif cluster within the ARE of IL-3, which contains 6 partially overlapping AUUUA pentamers. In mutation 3a, three pentamers were mutated to AGGUA, as indicated by double asterisks. This is the minimal mutation that abrogates the destabilizing effect of the ARE (41).

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FIG. 2. Expression of the GFP reporter construct in the parental cell line HT-GFPIL3-wt (A), the control mutant HT-GFPIL3-3a (B), and the mutants 12-2 (C), slowA (D), slowB (E), and slowC (F). (Left) Analysis of GFP expression by flow cytometry. (Center) Analysis of reporter mRNA stability by actinomycin D chase experiments and Northern blotting. RNA was isolated 0, 1, 2, and 3 h after inhibition of transcription with 5 µg of actinomycin D/ml. Twenty-five micrograms of total RNA was resolved on 1.1% agarose-formaldehyde gels and transferred onto Hybond N+ membranes, and GFPIL3 reporter mRNA was detected with a radiolabeled SP6 probe against the IL-3 3'UTR. All blots were stripped and rehybridized with a $beta$ -actin probe as a loading control. (Right) Signal intensities were quantified using a PhosphorImager and ImageQuant software. Values of GFPIL3 were normalized to actin and plotted as relative mRNA levels against time. mRNA half-lives were calculated by means of linear regression and are summarized in Table 2.

Mutagenesis and isolation of mutant cell lines. As recessive mutations require inactivation of all alleles of a given gene, we verified that the HT1080 indicator line wasdiploid and not polyploid. Indeed, about half of the HT1080 cellstransfected with GFPIL3-wt were tetraploid or nearly tetraploidwhen assayed for DNA content using propidium iodide staining andfluorescence-activated cell sorter (FACS) analysis. Cells weretherefore subcloned, a suitable clone (no. 16) was selected, andits diploid chromosome number was confirmed by microscopic examinationof chromosome spreads (data not shown). This clone will be referredto as HT-GFPIL3-wt.

For mutagenesis, we essentially followed the protocol published by G. R. Stark's laboratory (28), which is based on multiplerounds of treatment with the frameshift mutagen ICR191. A totalof 8 × 10⁷ HT-GFPIL3-wt cells were divided into four pools and exposed for2 h to 6 µg of ICR191/ml. At this concentration, about 15% ofthe cells survived (data not shown); these were allowed to recoverfor 4 to 5 days and then were subjected to the next round of mutagenesis.The efficiency of mutagenesis was monitored by determining thenumber of cells that had become resistant to 6-thioguanine, reflectingloss of the hypoxanthin phosphoribosyltransferase (HPRT) gene.This occurred at a relatively high frequency, since HPRT is X-chromosomelinked and therefore monoallelic. The frequency of colonies resistantto 6-thioguanine had continuously risen from 3 × 10⁶ in unmutagenized cells to a plateau value of about 0.8 × 10³ after 8 to 12 rounds ofmutagenesis.

Selection of GFP-overexpressing cells from the four mutagenized pools was achieved by a combination of automated sorting byflow cytometry, subsequent cloning, and direct analysis by fluorescencemicroscopy. Table 1 gives a summary of the recovery rates ateach step. From a total of 6 × 10⁷ cells subjected to FACS sorting, the 0.03% (2 × 10⁴) with the highest fluorescence intensities were retained. Thesecells were directly cloned in microtiter plates, whereby cloningefficiency was very low (~7%). When examined by eye, roughly one-third(444) of the clones displayed increased fluorescence. About half(237) of these promising candidates could be further expanded.FACS analysis confirmed increased GFP levels (twofold or moreabove the basal level) for 156 clones. For further characterization,Northern blot analysis was performed and revealed increased mRNAlevels corresponding to the GFP levels. However, most clones didnot show a change in reporter mRNA stability. In this class ofmutants, overexpression of GFP appeared to result from transcriptionalactivation. Clone 12-2 (Fig. 2C) is an example of a transcriptionalmutant with the typical characteristics (see Table 2): increasedlevels of GFP (18.5-fold) and reporter mRNA (11.4-fold), and anmRNA half-life (1.3 h) similar to that in the parental cell lineHT-GFPIL3-wt (1.0 h).

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TABLE 1. Selection of GFP-overexpressing clones

Nevertheless, three clones could be identified in which reporter mRNA degradation was consistently and significantly slowerthan in the wt precursor (Fig. 2D through F). These mutants weretermed slowA, slowB, and slowC, and they displayed GFPIL3 mRNAhalf-lives of 4.3, 3.5, and 8.6 h, respectively (summarized inTable 2). For slowA and slowC, these values correlated well withthe increased levels of mRNA expression (3.5- and 7.5-fold, respectively)and GFP fluorescence (7.5- and 13.2-fold, respectively). In slowBcells, the mRNA half-life of 3.5 h seemed to be too short forits considerably high mRNA (16.3-fold) and GFP (20.6-fold) levels,and it remained unclear whether additional transcriptional activationoccurred in this mutant, or whether the more-pronounced accumulationof GFP is a consequence of its lower proliferation rate (datanot shown).

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TABLE 2. Reporter gene expression in parental and mutant cell lines

The defect in slowA, slowB, and slowC acts in trans and is restricted to IL-3. Since cytokine mRNA stabilization can occur via cis mutations located on the mRNA itself, or in trans through loss of a regulatoryfunction, we had to distinguish between these two possibilities.For this purpose, murine genomic IL-3 was introduced as a secondreporter gene into the mutants and also, as a control, into thecis mutant HT-GFPIL3-3a. As shown in Fig. 3A, IL-3 mRNA was overexpressedand clearly more stable in slowA, slowB, and slowC compared toHT-GFPIL3-3a. To visualize the mRNA turnover rates, signal intensitieswere quantified (right panel). Stabilization was more pronouncedin slowA and slowC than in slowB, consistent with the half-livescalculated for the GFPIL3 transcripts (Table 2). The same resultwas obtained in a parallel set of transfections with an IL-3 genedriven by the MMLV LTR promoter (Fig. 3B), indicating that upregulationof IL-3 in the mutants occurred independently of the nature ofthe promoter. We concluded that all three mutants are defectivein a trans-acting function essential for rapid IL-3 mRNA decay.This conclusion was confirmed by direct sequencing of the 3'UTRof reporter mRNA amplified by RT-PCR from slowA, slowB, and slowCcells, where we failed to detect any mutation (data not shown).

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FIG. 3. Decay of mRNA from stably transfected IL-3, IL-2, and TNF- $alpha$ reporter constructs in control and mutant cell lines. Actinomycin D chase experiments and Northern blot analysis were performed as described for Fig. 2. For quantification (right), signal intensities were normalized to that of actin and plotted as percentages of the initial value against time. (A) Cells were transfected with HindIL3neo, a 5.3-kb genomic IL-3 construct that uses the IL-3 promoter. (B) Expression of MXIL3neo, where transcription of IL-3 is driven by an MMLV LTR promoter. For panels A and B, a HindIII-XbaI fragment of the IL-3 coding region was used to generate a radiolabeled SP6 RNA probe that specifically recognizes IL-3 mRNA but not GFPIL3 mRNA, which is also expressed in the mutants. (C) Cells were transfected with neoMX $beta$ globin-IL2, a plasmid that contains a $beta$ -globin reporter gene linked to the entire 3'UTR of murine IL-2. (D) Expression of neoMX $beta$ globin-TNF- $alpha$ , containing the 3'UTR of murine TNF- $alpha$ . In panels C and D, an SP6 probe against $beta$ -globin was used to detect reporter mRNA.

For a specificity control, we decided to examine whether mRNA turnover of two different cytokines, IL-2 and TNF- $alpha$ , would alsobe affected in the mutants. For this purpose, a $beta$ -globin reportergene was linked to the 3'UTRs of IL-2 and TNF- $alpha$ in constructsneoMX $beta$ globin-IL2 and neoMX $beta$ globin-TNF $alpha$ , respectively, and stablytransfected into control and mutant cell lines. In slowA and slowB,the IL-2 reporter mRNA decayed as rapidly as in the parental cells(Fig. 3C). The degradation rate was slightly reduced in slowC,yet not comparable to the stabilization observed with all IL-3transcripts. Likewise, TNF- $alpha$ reporter mRNA underwent rapid decayin both the mutants and the control cell line (Fig. 3D). Theseresults imply that the mutants do not exhibit a general lack ofrapid mRNA degradation, but rather a defect restricted to IL-3.

slowA, slowB, and slowC are recessive mutants and form two complementation groups. To address the question whether the decay mutants are dominant or recessive in nature, somatic cell fusion experiments wereperformed. The hygromycin-resistant mutants slowA, slowB, andslowC were fused with parental, pBABEpuro-expressing HT1080 cells.After selection with hygromycin and puromycin, the stability ofthe reporter mRNA was tested in the hybrids (Fig. 4A). Fusionled to reversion of the mutant phenotype, since rapid decay wasrestored in all three hybrids. To validate the approach, the dominantcis mutant HT-GFPIL3-3a was also fused with HT1080, and, as expected,the mutant phenotype was retained in this hybrid. We concludedthat slowA, slowB, and slowC are recessive mutants reverting whencomplemented with the parental genome.

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FIG. 4. Decay of GFPIL3 mRNA in hybrid cell lines. (A) Somatic cell fusion was performed between parental HT1080 cells expressing pBABEpuro and the hygromycin-resistant trans mutants slowA, slowB, and slowC, as well as the cis mutant HT-GFPIL3-3a. After selection with puromycin and hygromycin, hybrids were analyzed by actinomycin D chase experiments and Northern blotting, as described for Fig. 2. (B) Intermutant hybrids were generated by crossing mutants slowA, slowB, and slowC with each other (as specified in Materials and Methods). GFPIL3 reporter mRNA, expressed by both fusion partners, was detected with an SP6 probe directed against the GFP coding region in order to prevent hybridization with IL-3 mRNA from the HindIL3neo-transfected fusion partner.

It was of interest now to examine whether the mutants themselves could complement for each other's defect or whether theybelong to one complementation group. After transfection of eachpartner with a plasmid that confers resistance to either puromycinor G418 (specified in Materials and Methods), the following fusionswere performed: slowA × slowB, slowA × slowC, and slowB × slowC.Again, the stability of GFPIL3 mRNA was measured in the hybrids(Fig. 4B). It appeared that rapid mRNA decay was reinstalled byfusion of slowA × slowB and slowA × slowC, although the effectwas less pronounced than that observed upon fusion with parentalHT-1080 cells. In hybrid slowB × slowC, however, the mutant phenotypewas retained, as GFPIL3 mRNA remained stable. These results wereconfirmed in a repeat experiment, and we concluded that the defectin slowA is distinct from that in slowB and slowC, while slowBand slowC belong to the same complementation group. It is possiblethat mutants slowB and slowC are actually siblings, as they wereboth isolated from the same pool of mutagenized cells. But theyalso showed marked differences with respect to cell morphologyand growth rate (data not shown), as well as a reproducible differenceof about twofold in the GFPIL3 mRNA half-life (see Table 2).

TTP reverts the mutant phenotype. In order to characterize the defective functions in the two complementation groups, we decided to test whether expressinggenes known to promote rapid degradation of ARE-containing transcriptshad an effect on reporter mRNA stability in the mutants. The AUF1(p37), TTP, and VHL genes, cloned into the pcDNA3.1/MycHis expressionvector, were introduced into slowA and slowC. After selectionof stable transfectants, expression was confirmed by Western blotanalysis using an antibody against the myc tag. AUF1 and VHL wereexpressed readily in slowA and slowC, but neither GFP fluorescencenor GFPIL3 mRNA stability was altered (data not shown). Hence,AUF1 and VHL did not appear to be directly related to the defectivefunction in slowA and slowC. As shown in Fig. 5A, TTP (mTTP.tag)was well expressed in slowA (lane 2), but hardly at all in slowC(lane 8). Therefore, both mass cultures were subcloned, and fromeach, one negative clone (A-TTP-1 [lane 3] and C-TTP-4 [lane 9])and two TTP-positive clones (A-TTP-13 [lane 5], A-TTP-15 [lane6], C-TTP-10 [lane 10], and C-TTP-18 [lane 11]) were selected.Analysis of GFP expression revealed that TTP had a pronouncedeffect on the mutant phenotype of both slowA and slowC. In theTTP-positive clones, GFP fluorescence was reduced to low levelsand GFPIL3 mRNA decayed rapidly (Fig. 5C, D, F, and G). In contrast,the TTP-negative clones behaved identically to the untransfectedmutants (Fig. 5B and E). We concluded that expression of mTTP.tagcan functionally revert mutants slowA and slowC.

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FIG. 5. Transfection of tristetraprolin (mTTP.tag) into slowA and slowC, and analysis of GFP reporter gene expression in subclones. (A) Western blot analysis with untransfected slowA (lane 1), transfected slowA-TTP (lane 2), and subclones of slowA-TTP (lanes 3 to 6). Similarly, mTTP.tag expression was analyzed in untransfected slowC (lane 7), transfected slowC-TTP (lane 8), and subclones of slowC-TTP (lanes 9 to 11). A lysate of 1 × 10⁶ to 2 × 10⁶ cells was resolved on a 12% polyacrylamide-SDS gel and blotted onto an Immobilon-P membrane, and the anti-myc antibody 9E10 served to detect the myc- and His-tagged protein, which has an approximate molecular weight of 46 kDa. GFP reporter gene expression was analyzed in the following subclones: A-TTP-1 (B), A-TTP-13 (C), A-TTP-15 (D), C-TTP-4 (E), C-TTP-10 (F), and C-TTP-18 (G). GFP levels were assayed by flow cytometry (left panel), and reporter mRNA stability was measured by actinomycin D chase experiments (right panel). Northern blot analysis was performed as described for Fig. 2.

Endogenous TTP is not mutated in either complementation group. The effect of ectopically expressed TTP in slowA and slowC called for testing the possibility that the mutants had lost endogenousTTP expression. Northern blot analysis was performed using a random-primedprobe against human TTP (Fig. 6). RNA was isolated from unstimulatedparental HT-GFPIL3-wt, slowA, and slowC cells (Fig. 6, lanes 1to 3). hTTP mRNA was detected in all three cell lines, albeitat a somewhat reduced level in slowC. Upon stimulation for 45min with 10 ng of tetradecanoyl phorbol acetate (TPA)/ml, hTTPmRNA was induced to similar levels in the parental cell and thetwo mutants (Fig. 6, lanes 4 to 6). Thus, lack of endogenous TTPmRNA expression could not be observed in either mutant. Alternatively,a frameshift mutation might have occurred in the coding regionof the TTP gene, which would lead to an aberrant protein. To checkfor this possibility, cDNA of endogenous TTP mRNA was amplifiedby RT-PCR from parental HT-GFPIL3-wt, slowA, and slowC cells.After ligation into the pGEM7Z vector and cloning, the entire960-bp coding region was sequenced. From all three cell lineswe obtained wild-type sequences identical to the human TTP sequencepublished under GenBank accession no. M92843 (data not shown).These results indicated that in both mutants, at least one TTPallele is intact, and they largely ruled out the possibility thatmutation of TTP itself is the genetic defect in either of thecomplementation groups.

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FIG. 6. Northern blot analysis of endogenous TTP (hTTP) expression in parental HT-GFPIL3-wt cells and mutants slowA and slowC. Cells were grown in low concentrations of serum (0.5% FCS) for 24 h, and RNA was isolated before (lanes 1 to 3) or after stimulation with TPA (10 ng/ml) for 45 min (lanes 4 to 6). Fifty micrograms of total RNA was used for each lane, and the blot was hybridized with a random-primed probe generated from human TTP cDNA. The membrane was stripped and rehybridized with a $beta$ -actin probe as a loading control.

	DISCUSSION

Top Abstract Introduction Materials and Methods Results Discussion References

In this work we present a general strategy for generating mutants of a specific mRNA degradation pathway. To our knowledge,this is the first report where somatic cell genetics has beenused to study mRNA turnover in a mammalian system allowing thedefinition of complementation groups. With the help of a reportergene containing the ARE of the IL-3 3'UTR, changes in mRNA stabilitycould be translated into different steady-state expression levels(Fig. 2A and B). To obtain posttranscriptional mutants, it wasimportant to use GFP as a reporter gene instead of a selectable"all-or-nothing" resistance marker, because alteration of mRNAstability only modulates the levels of gene expression but doesnot completely turn it on or off. Using an efficient mutagenesisprotocol adopted from that of McKendry et al. (28), four poolsof 2 × 10⁷ cells each were exposed to 8 to 12 rounds of treatment with theframeshift mutagen ICR191. The extent of random genomic mutationswas estimated by the frequency of cells that had lost the monoallelic(X-linked) HPRT function, which reached a plateau value at about0.8 in 10³ cells. Based on this frequency, the probability of knocking outboth alleles of any gene could be estimated to (0.8 × 10³)², or 0.64 × 10⁶. Hence, each pool of 2 × 10⁷ cells should contain roughly 13 mutants for an autosomal genepromoting mRNA decay. We thus could believe that isolating a mutantshould be feasible, barring unexpected complications such as redundancyof the putative regulatory gene or a lethal effect of the homozygousmutation.

From the mutagenized cells, GFP-overexpressing clones were selected by a multistep procedure. Automated sorting by flow cytometryallowed us to enrich for highly fluorescent cells. These cellswere immediately subcloned in order to prevent the formation ofmany siblings and to protect slowly dividing cells from beingovergrown. An advantage of using GFP was that the clones couldbe directly analyzed by eye with a fluorescent microscope. Promisingcandidates were expanded, and GFP overexpression could finallybe confirmed for 156 clones by FACS analysis. Altogether, selectionwas rather time-consuming, and a considerable number of cloneswere lost at each step (see Table 1). Increasing the cloningefficiency would certainly help to reduce the amount of work infuture attempts and could perhaps be achieved by the use of conditionedmedium.

The GFP-overexpressing clones were first characterized by performing actinomycin D chase experiments and Northern blot analysis.As expected, all 156 candidate clones displayed increased steady-statelevels of the reporter mRNA. Surprisingly, stabilization of themRNA was found in only three clones, whereas other events, apparentlyleading to transcriptional activation, were more frequent. Thisclass of mutants, exemplified by clone 12-2 (Fig. 2C), might haveundergone amplification of the reporter gene, although it is difficultto imagine how a frameshift mutagen could achieve this. Another,more likely possibility is that loss of a transcriptional repressorhas occurred in these mutants. Interestingly, a repressor element,termed the nuclear inhibitory protein (NIP) region, has been identifiedat position $-$ 260 in the human IL-3 promoter (27). One of threecomplexes that bind to the NIP region in vitro is believed torepresent the repressor activity (9), but the protein has notbeen identified so far. Although it is not known whether the NIPregion, or a second repressor mapped further downstream (42),is also functional in the murine IL-3 promoter, it would be worthwhileto analyze the transcriptional mutants for promoter binding proteinsby DNA footprinting or electromobility shiftassays.

Our interest, however, focused on the three posttranscriptional mutants termed slowA, slowB, and slowC (Fig. 2D through F).First, the mutants were shown to have a trans-acting defect, asdegradation of mRNA from two genomic IL-3 constructs was alsoimpeded, similar to the stabilization observed with the GFP reportertranscript (Fig. 3A and B). Reporter transcripts with the ARE-containing3'UTRs of IL-2 and TNF- $alpha$ , however, were not stabilized in eitherof the mutants (Fig. 3C and D). This might indicate that the AREsof these two cytokines are recognized by a decay pathway differentfrom the one which promotes IL-3 mRNA degradation. Alternatively,the (class II) AREs are targeted by one mechanism $---$ which is defectivein the mutants $---$ yet IL-2 and TNF- $alpha$ , in contrast to IL-3, harboran additional destabilizing element in their 3'UTRs. A more extensiveanalysis using reporter constructs containing different AREs withand without flanking 3'UTR sequences will enable this issue toberesolved.

It was crucial to establish that the mutants displayed recessive defects, since this determines the strategy for later identificationof the defective genes, as outlined below. A dominant mutationwould require a different strategy, as the defective gene couldbe cloned directly by expressing a DNA library from the mutantin wt cells. Fusion of the parental cell line with the three mutantsrevealed that they are genetically recessive, since their phenotypewas corrected in the hybrids (Fig. 4A). Two complementation groupscould be defined by analyzing mRNA decay patterns of intermutanthybrids (Fig. 4B). slowA belongs to one group, while slowB andslowC form a second group. The two groups could not be distinguishedfurther, either with respect to decay of $beta$ -globin-IL2 or $beta$ -globin-TNF- $alpha$ mRNA or by their response to expression of TTP. In this contextit would be worthwhile to generate mutants of different mRNA decaypathways, using the technique described here with GFP reporterconstructs containing AREs of other cytokines or proto-oncogenes,particularly IL-2 and TNF- $alpha$ , as our mutants failed to stabilizethese transcripts. This should allow definition of more complementationgroups and help to identify the common as well as the specifictrans-acting factors that participate in thesepathways.

Once recessive IL-3 mRNA turnover mutants had been obtained, it was possible to test whether expression of known regulatorsof mRNA degradation could rescue the mutant phenotype. With AUF1(p37) and VHL, no effect on GFP levels or reporter mRNA stabilitycould be observed in either complementation group. In the caseof VHL, this is perhaps not surprising, since VHL is mainly involvedin the regulation of hypoxia-induced genes such as the VEGF gene.Interestingly, the p37 isoform of AUF1 also had no effect on reportermRNA decay. Recently, expression of the p42 isoform of AUF1 inK562 erythroleukemia cells has been shown to antagonize hemin-inducedstabilization of $beta$ -globin transcripts containing the AREs of c-fosand GM-CSF, the latter being almost identical to the ARE of IL-3.The p37 isoform of AUF1 is also an effective destabilizer, aswas demonstrated with the ARE of c-fos (24). The gene productmissing in our mutants is obviously not AUF1, but perhaps a componentdownstream, or an essential upstream activator of AUF1. Alternatively,the destabilizing function of AUF1 could be restricted to certaincell lineages and might not be active in HT1080 fibrosarcomacells.

TTP, on the other hand, could correct the defect in slowA and slowC, as its expression reinstalled rapid decay of GFPIL3 mRNA(Fig. 5). Originally, the mRNA turnover-promoting function ofTTP was discovered in macrophages from TTP knockout mice, whichoverexpress TNF- $alpha$ due to enhanced mRNA stability (6). Uponreintroduction of TTP into TTP^/ macrophages, reduced levels of $beta$ -globin reporter transcriptscontaining AREs from TNF- $alpha$ , IL-3, and GM-CSF were observed. Thissuggested a broader role for TTP in regulating mRNA degradationfor various cytokines, but destabilizing activity had been shownonly with TNF- $alpha$ mRNA. Our data establish that TTP is also a componentof the IL-3 mRNA degradation pathway. Since it fully restoredrapid decay in both complementation groups, TTP appears to bea potent mRNA destabilizer that acts downstream in the degradationpathway. The observation that TTP can directly bind to class IIAREs (6, 20) supports thisidea.

On the basis of this finding with TTP, experiments are in progress to investigate whether TTP can antagonize IL-3 overproductionin autocrine tumors which express abnormally stable IL-3 mRNA(32, 33). This can be tested at the levels of mRNA stability,IL-3 secretion, autocrine growth in vitro, and tumor formationin vivo. Should TTP have tumor suppressor activity, this wouldfurther emphasize its role as an important biologicalregulator.

More than one hypothesis could explain the capacity of ectopically expressed TTP to revert the mutant phenotypes. First, bothalleles of the TTP gene itself could be mutated. This was ruledout, as wild-type cDNA sequences of the human TTP coding regionwere obtained from both mutants. Second, a gene dosage effectmight have occurred following a TTP promoter mutation or by lossof a transcription factor. Similar levels of hTTP mRNA were foundin slowA and the parental cell line (Fig. 6). Whether the modestbut consistent reduction of hTTP mRNA observed in unstimulatedslowC (Fig. 6 and data not shown) is of any significance for themutant phenotype remains to be investigated. Northern blot analysisalso largely excluded the possibility of incorrect splicing or3'-end processing, since hTTP mRNA had the same size in the parentalcell and the mutants. Taken together, these data indicate thatthe TTP gene itself is intact in both complementation groups.Therefore, we favor a model where the missing component in theIL-3 mRNA degradation pathway is an activator of decay, locatedupstream of TTP, which can be overruled by ectopic expressionof high levels of TTP. The precise relationship between TTP andthe two functions A and B/C, however, will become clear only aftercloning of the corresponding genes. Taking advantage of the GFPreporter system, we plan to perform complementation by transferof a cDNA library into the mutants and selection of revertantclones. This should hopefully allow identification of the defectivegenes in slowA and slowB/C, and eventually help us understandhow upstream factors function in concert with known regulatorsof ARE-dependent mRNAdegradation.

	ACKNOWLEDGMENTS

We are especially grateful to Verena Jaeggin and Genaro DeLibero (Research Department, Kantonsspital Basel) for help and advicewith cell sorting. We also thank Asha P. K. Nair, Adrian Wyss,and Lyndall Brennan for critical comments on themanuscript.

This work was supported by grant 31-40816.94 to C.M. from the Schweizerischer Nationalfonds zur Foerderung der WissenschaftlichenForschung. G.S. received a fellowship from the SchweizerischeAkademie der MedizinischenWissenschaften.

	FOOTNOTES

^* Corresponding author. Mailing address: Institute of Medical Microbiology, University of Basel, Petersplatz 10, CH 4003, Basel,Switzerland. Phone: 41 61 2673264. Fax: 41 61 2673298. E-mail:christoph.moroni{at}unibas.ch.

REFERENCES

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References

1. Beelman, C. A., and R. Parker. 1995. Degradation of mRNA in eukaryotes. Cell 81:179-183[CrossRef][Medline].

2. Blochlinger, K., and H. Diggelmann. 1984. Hygromycin B phosphotransferase as a selectable marker for DNA transfer experiments with higher eucaryotic cells. Mol. Cell. Biol. 4:2929-2931[Abstract/Free Full Text].

3. Brewer, G. 1991. An A+U-rich element RNA-binding factor regulates c-myc stability in vitro. Mol. Cell. Biol. 11:2460-2466[Abstract/Free Full Text].

4. Brewer, G., and J. Ross. 1989. Regulation of c-myc mRNA stability in vitro by a labile destabilizer with an essential nucleic acid component. Mol. Cell. Biol. 9:1996-2006[Abstract/Free Full Text].

5. Caput, D., B. Beutler, K. Hartog, R. Thayer, S. Brown-Shimer, and A. Cerami. 1986. Identification of a common nucleotide sequence in the 3'-untranslated region of mRNA molecules specifying inflammatory mediators. Proc. Natl. Acad. Sci. USA 83:1670-1674[Abstract/Free Full Text].

6. Carballo, E., W. S. Lai, and P. J. Blackshear. 1998. Feedback inhibition of macrophage tumor necrosis factor-alpha production by tristetraprolin. Science 281:1001-1005[Abstract/Free Full Text].

7. Chen, C.-Y. A., and A.-B. Shyu. 1995. AU-rich elements: characterization and importance in mRNA degradation. Trends Biochem. Sci. 20:465-470[CrossRef][Medline].

8. Diamantis, I. D., A. P. Nair, H. H. Hirsch, and C. Moroni. 1989. Tumor suppression involves down-regulation of interleukin 3 expression in hybrids between autocrine mastocytoma and interleukin 3-dependent parental mast cells. Proc. Natl. Acad. Sci. USA 86:9299-9303[Abstract/Free Full Text].

9. Engeland, K., N. C. Andrews, and B. Mathey-Prevot. 1995. Multiple proteins interact with the nuclear inhibitory protein repressor element in the human interleukin-3 promoter. J. Biol. Chem. 270:24572-24579[Abstract/Free Full Text].

10. Erb, P., M. Troxler, M. Fluri, D. Grogg, and S. S. Alkan. 1991. Functional heterogeneity of CD4-positive T-cell subsets: the correlation between effector functions and lymphokine secretion is limited. Cell. Immunol. 135:232-244[CrossRef][Medline].

11. Fan, X. C., and J. A. Steitz. 1998. Overexpression of HuR, a nuclear-cytoplasmic shuttling protein, increases the in vivo stability of ARE-containing mRNAs. EMBO J. 17:3448-3460[CrossRef][Medline].

12. Gnarra, J. R., S. Zhou, M. J. Merrill, J. R. Wagner, A. Krumm, E. Papavassiliou, E. H. Oldfield, R. D. Klausner, and W. M. Linehan. 1996. Post-transcriptional regulation of vascular endothelial growth factor mRNA by the product of the VHL tumor suppressor gene. Proc. Natl. Acad. Sci. USA 93:10589-10594[Abstract/Free Full Text].

13. Gough, N. M. 1988. Rapid and quantitative preparation of cytoplasmic RNA from small numbers of cells. Anal. Biochem. 173:93-95[CrossRef][Medline].

14. Hirsch, H. H., A. P. Nair, V. Backenstoss, and C. Moroni. 1995. Interleukin-3 mRNA stabilization by a trans-acting mechanism in autocrine tumors lacking interleukin-3 gene rearrangements. J. Biol. Chem. 270:20629-20635[Abstract/Free Full Text].

15. Hirsch, H. H., A. P. Nair, and C. Moroni. 1993. Suppressible and nonsuppressible autocrine mast cell tumors are distinguished by insertion of an endogenous retroviral element (IAP) into the interleukin 3 gene. J. Exp. Med. 178:403-411[Abstract/Free Full Text].

16. Iliopoulos, O., A. P. Levy, C. Jiang, W. G. Kaelin, Jr., and M. A. Goldberg. 1996. Negative regulation of hypoxia-inducible genes by the von Hippel-Lindau protein. Proc. Natl. Acad. Sci. USA 93:10595-10599[Abstract/Free Full Text].

17. Jacobson, A., and S. W. Peltz. 1996. Interrelationships of the pathways of mRNA decay and translation in eukaryotic cells. Annu. Rev. Biochem. 65:693-739[CrossRef][Medline].

18. John, J., R. McKendry, S. Pellegrini, D. Flavell, I. M. Kerr, and G. R. Stark. 1991. Isolation and characterization of a new mutant human cell line unresponsive to alpha and beta interferons. Mol. Cell. Biol. 11:4189-4195[Abstract/Free Full Text].

19. Jones, T. R., and M. D. Cole. 1987. Rapid cytoplasmic turnover of c-myc mRNA: requirement of the 3' untranslated sequences. Mol. Cell. Biol. 7:4513-4521[Abstract/Free Full Text].

20. Lai, W. S., E. Carballo, J. R. Strum, E. A. Kennington, R. S. Phillips, and P. J. Blackshear. 1999. Evidence that tristetraprolin binds to AU-rich elements and promotes the deadenylation and destabilization of tumor necrosis factor alpha mRNA. Mol. Cell. Biol. 19:4311-4323[Abstract/Free Full Text].

21. Latif, F., K. Tory, J. Gnarra, M. Yao, F. M. Duh, M. L. Orcutt, T. Stackhouse, I. Kuzmin, W. Modi, L. Geil, et al. 1993. Identification of the von Hippel-Lindau disease tumor suppressor gene. Science 260:1317-1320[Abstract/Free Full Text].

22. Levy, N. S., S. Chung, H. Furneaux, and A. P. Levy. 1998. Hypoxic stabilization of vascular endothelial growth factor mRNA by the RNA-binding protein HuR. J. Biol. Chem. 273:6417-6423[Abstract/Free Full Text].

23. Lisztwan, J., G. Imbert, C. Wirbelauer, M. Gstaiger, and W. Krek. 1999. The von Hippel-Lindau tumor suppressor protein is a component of an E3 ubiquitin-protein ligase activity. Genes Dev. 13:1822-1833[Abstract/Free Full Text].

24. Loflin, P., C. Y. Chen, and A. B. Shyu. 1999. Unraveling a cytoplasmic role for hnRNP D in the in vivo mRNA destabilization directed by the AU-rich element. Genes Dev. 13:1884-1897[Abstract/Free Full Text].

25. Ma, Q., and H. R. Herschman. 1991. A corrected sequence for the predicted protein from the mitogen-inducible TIS11 primary response gene. Oncogene 6:1277-1278[Medline].

26. Ma, W.-J., S. Cheng, C. Campbell, A. Wright, and H. Furneaux. 1996. Cloning and characterization of HuR, a ubiquitously expressed Elav-like protein. J. Biol. Chem. 271:8144-8151[Abstract/Free Full Text].

27. Mathey-Prevot, B., N. C. Andrews, H. S. Murphy, S. G. Kreissman, and D. G. Nathan. 1990. Positive and negative elements regulate human interleukin 3 expression. Proc. Natl. Acad. Sci. USA 87:5046-5050[Abstract/Free Full Text].

28. McKendry, R., J. John, D. Flavell, M. Muller, I. M. Kerr, and G. R. Stark. 1991. High-frequency mutagenesis of human cells and characterization of a mutant unresponsive to both alpha and gamma interferons. Proc. Natl. Acad. Sci. USA 88:11455-11459[Abstract/Free Full Text].

29. Ming, X. F., M. Kaiser, and C. Moroni. 1998. c-jun N-terminal kinase is involved in AUUUA-mediated interleukin-3 mRNA turnover in mast cells. EMBO J. 17:6039-6048[CrossRef][Medline].

30. Morgenstern, J. P., and H. Land. 1990. Advanced mammalian gene transfer: high titre retroviral vectors with multiple drug selection markers and a complementary helper-free packaging cell line. Nucleic Acids Res. 18:3587-3596[Abstract/Free Full Text].

31. Myer, V. E., X. C. Fan, and J. A. Steitz. 1997. Identification of HuR as a protein implicated in AUUUA-mediated mRNA decay. EMBO J. 16:2130-2139[CrossRef][Medline].

32. Nair, A. P., I. D. Diamantis, J. F. Conscience, V. Kindler, P. Hofer, and C. Moroni. 1989. A v-H-ras-dependent hemopoietic tumor model involving progression from a clonal stage of transformation competence to autocrine interleukin 3 production. Mol. Cell. Biol. 9:1183-1190[Abstract/Free Full Text].

33. Nair, A. P., S. Hahn, R. Banholzer, H. H. Hirsch, and C. Moroni. 1994. Cyclosporin A inhibits growth of autocrine tumour cell lines by destabilizing interleukin-3 mRNA. Nature 369:239-242[CrossRef][Medline].

34. Nair, A. P., H. H. Hirsch, and C. Moroni. 1992. Mast cells sensitive to v-H-ras transformation are hyperinducible for interleukin 3 expression and have lost tumor-suppressor activity. Oncogene 7:1963-1972[Medline].

35. Pellegrini, S., J. John, M. Shearer, I. M. Kerr, and G. R. Stark. 1989. Use of a selectable marker regulated by alpha interferon to obtain mutations in the signaling pathway. Mol. Cell. Biol. 9:4605-4612[Abstract/Free Full Text].

36. Peng, S. S., C. Y. Chen, N. Xu, and A. B. Shyu. 1998. RNA stabilization by the AU-rich element binding protein, HuR, an ELAV protein. EMBO J. 17:3461-3470[CrossRef][Medline].

37. Ross, J. 1995. mRNA stability in mammalian cells. Microbiol. Rev. 59:423-450[Abstract/Free Full Text].

38. Schuler, G. D., and M. D. Cole. 1988. GM-CSF and oncogene mRNA stabilities are independently regulated in trans in a mouse monocytic tumor. Cell 55:1115-1122[CrossRef][Medline].

39. Shaw, G., and R. Kamen. 1986. A conserved AU sequence from the 3' untranslated region of GM-CSF mRNA mediates selective mRNA degradation. Cell 46:659-667[CrossRef][Medline].

40. Shyu, A.-B., M. E. Greenberg, and J. G. Belasco. 1989. The c-fos transcript is targeted for rapid decay by two distinct mRNA degradation pathways. Genes Dev. 3:60-72[Abstract/Free Full Text].

41. Stoecklin, G., S. Hahn, and C. Moroni. 1994. Functional hierarchy of AUUUA motifs in mediating rapid interleukin-3 mRNA decay. J. Biol. Chem. 269:28591-28597[Abstract/Free Full Text].

42. Taylor, D. S., J. P. Laubach, D. G. Nathan, and B. Mathey-Prevot. 1996. Cooperation between core binding factor and adjacent promoter elements contributes to the tissue-specific expression of interleukin-3. J. Biol. Chem. 271:14020-14027[Abstract/Free Full Text].

43. Taylor, G. A., E. Carballo, D. M. Lee, W. S. Lai, M. J. Thompson, D. D. Patel, D. I. Schenkman, G. S. Gilkeson, H. E. Broxmeyer, B. F. Haynes, and P. J. Blackshear. 1996. A pathogenetic role for TNF alpha in the syndrome of cachexia, arthritis, and autoimmunity resulting from tristetraprolin (TTP) deficiency. Immunity 4:445-454[CrossRef][Medline].

44. Taylor, G. A., M. J. Thompson, W. S. Lai, and P. J. Blackshear. 1995. Phosphorylation of tristetraprolin, a potential zinc finger transcription factor, by mitogen stimulation in intact cells and by mitogen-activated protein kinase in vitro. J. Biol. Chem. 270:13341-13347[Abstract/Free Full Text].

45. Varnum, B. C., R. W. Lim, V. P. Sukhatme, and H. R. Herschman. 1989. Nucleotide sequence of a cDNA encoding TIS11, a message induced in Swiss 3T3 cells by the tumor promoter tetradecanoyl phorbol acetate. Oncogene 4:119-120[Medline].

46. Wellington, C. L., M. E. Greenberg, and J. G. Belasco. 1993. The destabilizing elements in the coding region of c-fos mRNA are recognized as RNA. Mol. Cell. Biol. 13:5034-5042[Abstract/Free Full Text].

47. Wisdom, R., and R. Lee. 1991. The protein-coding region of c-myc mRNA contains a sequence that specifies rapid mRNA turnover and induction by protein synthesis inhibitors. Genes Dev. 5:232-243[Abstract/Free Full Text].

48. Wyss, A., and C. Moroni. Calcium-dependent and oncogenic IL-3 mRNA stabilization can be distinguished pharmacologically and by sequence requirements in the 3' UTR. Growth Factors, in press.

49. Zhang, W., B. J. Wagner, K. Ehrenman, A. W. Schaefer, C. T. DeMaria, D. Crater, K. DeHaven, L. Long, and G. Brewer. 1993. Purification, characterization, and cDNA cloning of an AU-rich element RNA-binding protein, AUF1. Mol. Cell. Biol. 13:7652-7665[Abstract/Free Full Text].

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Emmons, J., Townley-Tilson, W.H. D., Deleault, K. M., Skinner, S. J., Gross, R. H., Whitfield, M. L., Brooks, S. A. (2008). Identification of TTP mRNA targets in human dendritic cells reveals TTP as a critical regulator of dendritic cell maturation. RNA 14: 888-902 [Abstract] [Full Text]
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Patil, C.S., Kirkwood, K.L. (2007). p38 MAPK Signaling in Oral-related Diseases. JDR 86: 812-825 [Abstract] [Full Text]
Chang, X., Fan, Y., Karyala, S., Schwemberger, S., Tomlinson, C. R., Sartor, M. A., Puga, A. (2007). Ligand-Independent Regulation of Transforming Growth Factor {beta}1 Expression and Cell Cycle Progression by the Aryl Hydrocarbon Receptor. Mol. Cell. Biol. 27: 6127-6139 [Abstract] [Full Text]
Frasca, D., Landin, A. M., Alvarez, J. P., Blackshear, P. J., Riley, R. L., Blomberg, B. B. (2007). Tristetraprolin, a Negative Regulator of mRNA Stability, Is Increased in Old B Cells and Is Involved in the Degradation of E47 mRNA. J. Immunol. 179: 918-927 [Abstract] [Full Text]
Franks, T. M., Lykke-Andersen, J. (2007). TTP and BRF proteins nucleate processing body formation to silence mRNAs with AU-rich elements. Genes Dev. 21: 719-735 [Abstract] [Full Text]
Sun, L., Stoecklin, G., Van Way, S., Hinkovska-Galcheva, V., Guo, R.-F., Anderson, P., Shanley, T. P. (2007). Tristetraprolin (TTP)-14-3-3 Complex Formation Protects TTP from Dephosphorylation by Protein Phosphatase 2a and Stabilizes Tumor Necrosis Factor-{alpha} mRNA. J. Biol. Chem. 282: 3766-3777 [Abstract] [Full Text]
Benjamin, D., Schmidlin, M., Min, L., Gross, B., Moroni, C. (2006). BRF1 Protein Turnover and mRNA Decay Activity Are Regulated by Protein Kinase B at the Same Phosphorylation Sites. Mol. Cell. Biol. 26: 9497-9507 [Abstract] [Full Text]
Smoak, K., Cidlowski, J. A. (2006). Glucocorticoids Regulate Tristetraprolin Synthesis and Posttranscriptionally Regulate Tumor Necrosis Factor Alpha Inflammatory Signaling. Mol. Cell. Biol. 26: 9126-9135 [Abstract] [Full Text]
Paschoud, S., Dogar, A. M., Kuntz, C., Grisoni-Neupert, B., Richman, L., Kuhn, L. C. (2006). Destabilization of Interleukin-6 mRNA Requires a Putative RNA Stem-Loop Structure, an AU-Rich Element, and the RNA-Binding Protein AUF1. Mol. Cell. Biol. 26: 8228-8241 [Abstract] [Full Text]
Newman, E. A., Muh, S. J., Hovhannisyan, R. H., Warzecha, C. C., Jones, R. B., McKeehan, W. L., Carstens, R. P. (2006). Identification of RNA-binding proteins that regulate FGFR2 splicing through the use of sensitive and specific dual color fluorescence minigene assays. RNA 12: 1129-1141 [Abstract] [Full Text]
Lu, J.-Y., Bergman, N., Sadri, N., Schneider, R. J. (2006). Assembly of AUF1 with eIF4G-poly(A) binding protein complex suggests a translation function in AU-rich mRNA decay. RNA 12: 883-893 [Abstract] [Full Text]
Wang, J. G., Collinge, M., Ramgolam, V., Ayalon, O., Fan, X. C., Pardi, R., Bender, J. R. (2006). LFA-1-Dependent HuR Nuclear Export and Cytokine mRNA Stabilization in T Cell Activation. J. Immunol. 176: 2105-2113 [Abstract] [Full Text]
Barreau, C., Paillard, L., Osborne, H. B. (2006). AU-rich elements and associated factors: are there unifying principles?. Nucleic Acids Res 33: 7138-7150 [Abstract] [Full Text]
Linker, K., Pautz, A., Fechir, M., Hubrich, T., Greeve, J., Kleinert, H. (2005). Involvement of KSRP in the post-transcriptional regulation of human iNOS expression-complex interplay of KSRP with TTP and HuR. Nucleic Acids Res 33: 4813-4827 [Abstract] [Full Text]
Pascale, A., Amadio, M., Scapagnini, G., Lanni, C., Racchi, M., Provenzani, A., Govoni, S., Alkon, D. L., Quattrone, A. (2005). Neuronal ELAV proteins enhance mRNA stability by a PKC{alpha}-dependent pathway. Proc. Natl. Acad. Sci. USA 102: 12065-12070 [Abstract] [Full Text]
Paillusson, A., Hirschi, N., Vallan, C., Azzalin, C. M., Muhlemann, O. (2005). A GFP-based reporter system to monitor nonsense-mediated mRNA decay. Nucleic Acids Res 33: e54-e54 [Abstract] [Full Text]
Ogilvie, R. L., Abelson, M., Hau, H. H., Vlasova, I., Blackshear, P. J., Bohjanen, P. R. (2005). Tristetraprolin Down-Regulates IL-2 Gene Expression through AU-Rich Element-Mediated mRNA Decay. J. Immunol. 174: 953-961 [Abstract] [Full Text]
Groger, M., Loewe, R., Holnthoner, W., Embacher, R., Pillinger, M., Herron, G. S., Wolff, K., Petzelbauer, P. (2004). IL-3 Induces Expression of Lymphatic Markers Prox-1 and Podoplanin in Human Endothelial Cells. J. Immunol. 173: 7161-7169 [Abstract] [Full Text]
Tchen, C. R., Brook, M., Saklatvala, J., Clark, A. R. (2004). The Stability of Tristetraprolin mRNA Is Regulated by Mitogen-activated Protein Kinase p38 and by Tristetraprolin Itself. J. Biol. Chem. 279: 32393-32400 [Abstract] [Full Text]
Lu, J.-Y., Schneider, R. J. (2004). Tissue Distribution of AU-rich mRNA-binding Proteins Involved in Regulation of mRNA Decay. J. Biol. Chem. 279: 12974-12979 [Abstract] [Full Text]
Chrestensen, C. A., Schroeder, M. J., Shabanowitz, J., Hunt, D. F., Pelo, J. W., Worthington, M. T., Sturgill, T. W. (2004). MAPKAP Kinase 2 Phosphorylates Tristetraprolin on in Vivo Sites Including Ser178, a Site Required for 14-3-3 Binding. J. Biol. Chem. 279: 10176-10184 [Abstract] [Full Text]
Raineri, I., Wegmueller, D., Gross, B., Certa, U., Moroni, C. (2004). Roles of AUF1 isoforms, HuR and BRF1 in ARE-dependent mRNA turnover studied by RNA interference. Nucleic Acids Res 32: 1279-1288 [Abstract] [Full Text]
Twizere, J.-C., Kruys, V., Lefebvre, L., Vanderplasschen, A., Collete, D., Debacq, C., Lai, W. S., Jauniaux, J.-C., Bernstein, L. R., Semmes, O. J., Burny, A., Blackshear, P. J., Kettmann, R., Willems, L. (2003). Interaction of Retroviral Tax Oncoproteins With Tristetraprolin and Regulation of Tumor Necrosis Factor-{alpha} Expression. JNCI J Natl Cancer Inst 95: 1846-1859 [Abstract] [Full Text]
Park-Lee, S., Kim, S., Laird-Offringa, I. A. (2003). Characterization of the Interaction between Neuronal RNA-binding Protein HuD and AU-rich RNA. J. Biol. Chem. 278: 39801-39808 [Abstract] [Full Text]
Ji, B., Chen, X.-q., Misek, D. E., Kuick, R., Hanash, S., Ernst, S., Najarian, R., Logsdon, C. D. (2003). Pancreatic gene expression during the initiation of acute pancreatitis: identification of EGR-1 as a key regulator. Physiol. Genomics 14: 59-72 [Abstract] [Full Text]
Stoecklin, G., Lu, M., Rattenbacher, B., Moroni, C. (2003). A Constitutive Decay Element Promotes Tumor Necrosis Factor Alpha mRNA Degradation via an AU-Rich Element-Independent Pathway. Mol. Cell. Biol. 23: 3506-3515 [Abstract] [Full Text]
Frevel, M. A. E., Bakheet, T., Silva, A. M., Hissong, J. G., Khabar, K. S. A., Williams, B. R. G. (2003). p38 Mitogen-Activated Protein Kinase-Dependent and -Independent Signaling of mRNA Stability of AU-Rich Element-Containing Transcripts. Mol. Cell. Biol. 23: 425-436 [Abstract] [Full Text]
Korhonen, R., Lahti, A., Hamalainen, M., Kankaanranta, H., Moilanen, E. (2002). Dexamethasone Inhibits Inducible Nitric-Oxide Synthase Expression and Nitric Oxide Production by Destabilizing mRNA in Lipopolysaccharide-Treated Macrophages. Mol. Pharmacol. 62: 698-704 [Abstract] [Full Text]
Laroia, G., Schneider, R. J. (2002). Alternate exon insertion controls selective ubiquitination and degradation of different AUF1 protein isoforms. Nucleic Acids Res 30: 3052-3058 [Abstract] [Full Text]
Chinn, A. M., Ciais, D., Bailly, S., Chambaz, E., LaMarre, J., Feige, J.-J. (2002). Identification of Two Novel ACTH-Responsive Genes Encoding Manganese-Dependent Superoxide Dismutase (SOD2) and the Zinc Finger Protein TIS11b [Tetradecanoyl Phorbol Acetate (TPA)-Inducible Sequence 11b]. Mol. Endocrinol. 16: 1417-1427 [Abstract] [Full Text]
MacKenzie, S., Fernandez-Troy, N., Espel, E. (2002). Post-transcriptional regulation of TNF-{alpha} during in vitro differentiation of human monocytes/macrophages in primary culture. J. Leukoc. Biol. 71: 1026-1032 [Abstract] [Full Text]
Phillips, R. S., Ramos, S. B. V., Blackshear, P. J. (2002). Members of the Tristetraprolin Family of Tandem CCCH Zinc Finger Proteins Exhibit CRM1-dependent Nucleocytoplasmic Shuttling. J. Biol. Chem. 277: 11606-11613 [Abstract] [Full Text]
Carballo, E., Cao, H., Lai, W. S., Kennington, E. A., Campbell, D., Blackshear, P. J. (2001). Decreased Sensitivity of Tristetraprolin-deficient Cells to p38 Inhibitors Suggests the Involvement of Tristetraprolin in the p38 Signaling Pathway. J. Biol. Chem. 276: 42580-42587 [Abstract] [Full Text]
Mahtani, K. R., Brook, M., Dean, J. L. E., Sully, G., Saklatvala, J., Clark, A. R. (2001). Mitogen-Activated Protein Kinase p38 Controls the Expression and Posttranslational Modification of Tristetraprolin, a Regulator of Tumor Necrosis Factor Alpha mRNA Stability. Mol. Cell. Biol. 21: 6461-6469 [Abstract] [Full Text]
Ming, X.-F., Stoecklin, G., Lu, M., Looser, R., Moroni, C. (2001). Parallel and Independent Regulation of Interleukin-3 mRNA Turnover by Phosphatidylinositol 3-Kinase and p38 Mitogen-Activated Protein Kinase. Mol. Cell. Biol. 21: 5778-5789 [Abstract] [Full Text]
Bakheet, T., Frevel, M., Williams, B. R. G., Greer, W., Khabar, K. S. A. (2001). ARED: human AU-rich element-containing mRNA database reveals an unexpectedly diverse functional repertoire of encoded proteins. Nucleic Acids Res 29: 246-254 [Abstract] [Full Text]
Johnson, M. A., Pérez-Amador, M. A., Lidder, P., Green, P. J. (2000). Mutants of Arabidopsis defective in a sequence-specific mRNA degradation pathway. Proc. Natl. Acad. Sci. USA 10.1073/pnas.240354097v1 [Abstract] [Full Text]
Lai, W. S., Blackshear, P. J. (2001). Interactions of CCCH Zinc Finger Proteins with mRNA. TRISTETRAPROLIN-MEDIATED AU-RICH ELEMENT-DEPENDENT mRNA DEGRADATION CAN OCCUR IN THE ABSENCE OF A POLY(A) TAIL. J. Biol. Chem. 276: 23144-23154 [Abstract] [Full Text]
Laroia, G., Sarkar, B., Schneider, R. J. (2002). Ubiquitin-dependent mechanism regulates rapid turnover of AU-rich cytokine mRNAs. Proc. Natl. Acad. Sci. USA 99: 1842-1846 [Abstract] [Full Text]
Johnson, M. A., Perez-Amador, M. A., Lidder, P., Green, P. J. (2000). Mutants of Arabidopsis defective in a sequence-specific mRNA degradation pathway. Proc. Natl. Acad. Sci. USA 97: 13991-13996 [Abstract] [Full Text]

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1.	Beelman, C. A., and R. Parker. 1995. Degradation of mRNA in eukaryotes. Cell 81:179-183[CrossRef][Medline].
2.	Blochlinger, K., and H. Diggelmann. 1984. Hygromycin B phosphotransferase as a selectable marker for DNA transfer experiments with higher eucaryotic cells. Mol. Cell. Biol. 4:2929-2931[Abstract/Free Full Text].
3.	Brewer, G. 1991. An A+U-rich element RNA-binding factor regulates c-myc stability in vitro. Mol. Cell. Biol. 11:2460-2466[Abstract/Free Full Text].
4.	Brewer, G., and J. Ross. 1989. Regulation of c-myc mRNA stability in vitro by a labile destabilizer with an essential nucleic acid component. Mol. Cell. Biol. 9:1996-2006[Abstract/Free Full Text].
5.	Caput, D., B. Beutler, K. Hartog, R. Thayer, S. Brown-Shimer, and A. Cerami. 1986. Identification of a common nucleotide sequence in the 3'-untranslated region of mRNA molecules specifying inflammatory mediators. Proc. Natl. Acad. Sci. USA 83:1670-1674[Abstract/Free Full Text].
6.	Carballo, E., W. S. Lai, and P. J. Blackshear. 1998. Feedback inhibition of macrophage tumor necrosis factor-alpha production by tristetraprolin. Science 281:1001-1005[Abstract/Free Full Text].
7.	Chen, C.-Y. A., and A.-B. Shyu. 1995. AU-rich elements: characterization and importance in mRNA degradation. Trends Biochem. Sci. 20:465-470[CrossRef][Medline].
8.	Diamantis, I. D., A. P. Nair, H. H. Hirsch, and C. Moroni. 1989. Tumor suppression involves down-regulation of interleukin 3 expression in hybrids between autocrine mastocytoma and interleukin 3-dependent parental mast cells. Proc. Natl. Acad. Sci. USA 86:9299-9303[Abstract/Free Full Text].
9.	Engeland, K., N. C. Andrews, and B. Mathey-Prevot. 1995. Multiple proteins interact with the nuclear inhibitory protein repressor element in the human interleukin-3 promoter. J. Biol. Chem. 270:24572-24579[Abstract/Free Full Text].
10.	Erb, P., M. Troxler, M. Fluri, D. Grogg, and S. S. Alkan. 1991. Functional heterogeneity of CD4-positive T-cell subsets: the correlation between effector functions and lymphokine secretion is limited. Cell. Immunol. 135:232-244[CrossRef][Medline].
11.	Fan, X. C., and J. A. Steitz. 1998. Overexpression of HuR, a nuclear-cytoplasmic shuttling protein, increases the in vivo stability of ARE-containing mRNAs. EMBO J. 17:3448-3460[CrossRef][Medline].
12.	Gnarra, J. R., S. Zhou, M. J. Merrill, J. R. Wagner, A. Krumm, E. Papavassiliou, E. H. Oldfield, R. D. Klausner, and W. M. Linehan. 1996. Post-transcriptional regulation of vascular endothelial growth factor mRNA by the product of the VHL tumor suppressor gene. Proc. Natl. Acad. Sci. USA 93:10589-10594[Abstract/Free Full Text].
13.	Gough, N. M. 1988. Rapid and quantitative preparation of cytoplasmic RNA from small numbers of cells. Anal. Biochem. 173:93-95[CrossRef][Medline].
14.	Hirsch, H. H., A. P. Nair, V. Backenstoss, and C. Moroni. 1995. Interleukin-3 mRNA stabilization by a trans-acting mechanism in autocrine tumors lacking interleukin-3 gene rearrangements. J. Biol. Chem. 270:20629-20635[Abstract/Free Full Text].
15.	Hirsch, H. H., A. P. Nair, and C. Moroni. 1993. Suppressible and nonsuppressible autocrine mast cell tumors are distinguished by insertion of an endogenous retroviral element (IAP) into the interleukin 3 gene. J. Exp. Med. 178:403-411[Abstract/Free Full Text].
16.	Iliopoulos, O., A. P. Levy, C. Jiang, W. G. Kaelin, Jr., and M. A. Goldberg. 1996. Negative regulation of hypoxia-inducible genes by the von Hippel-Lindau protein. Proc. Natl. Acad. Sci. USA 93:10595-10599[Abstract/Free Full Text].
17.	Jacobson, A., and S. W. Peltz. 1996. Interrelationships of the pathways of mRNA decay and translation in eukaryotic cells. Annu. Rev. Biochem. 65:693-739[CrossRef][Medline].
18.	John, J., R. McKendry, S. Pellegrini, D. Flavell, I. M. Kerr, and G. R. Stark. 1991. Isolation and characterization of a new mutant human cell line unresponsive to alpha and beta interferons. Mol. Cell. Biol. 11:4189-4195[Abstract/Free Full Text].
19.	Jones, T. R., and M. D. Cole. 1987. Rapid cytoplasmic turnover of c-myc mRNA: requirement of the 3' untranslated sequences. Mol. Cell. Biol. 7:4513-4521[Abstract/Free Full Text].
20.	Lai, W. S., E. Carballo, J. R. Strum, E. A. Kennington, R. S. Phillips, and P. J. Blackshear. 1999. Evidence that tristetraprolin binds to AU-rich elements and promotes the deadenylation and destabilization of tumor necrosis factor alpha mRNA. Mol. Cell. Biol. 19:4311-4323[Abstract/Free Full Text].
21.	Latif, F., K. Tory, J. Gnarra, M. Yao, F. M. Duh, M. L. Orcutt, T. Stackhouse, I. Kuzmin, W. Modi, L. Geil, et al. 1993. Identification of the von Hippel-Lindau disease tumor suppressor gene. Science 260:1317-1320[Abstract/Free Full Text].
22.	Levy, N. S., S. Chung, H. Furneaux, and A. P. Levy. 1998. Hypoxic stabilization of vascular endothelial growth factor mRNA by the RNA-binding protein HuR. J. Biol. Chem. 273:6417-6423[Abstract/Free Full Text].
23.	Lisztwan, J., G. Imbert, C. Wirbelauer, M. Gstaiger, and W. Krek. 1999. The von Hippel-Lindau tumor suppressor protein is a component of an E3 ubiquitin-protein ligase activity. Genes Dev. 13:1822-1833[Abstract/Free Full Text].
24.	Loflin, P., C. Y. Chen, and A. B. Shyu. 1999. Unraveling a cytoplasmic role for hnRNP D in the in vivo mRNA destabilization directed by the AU-rich element. Genes Dev. 13:1884-1897[Abstract/Free Full Text].
25.	Ma, Q., and H. R. Herschman. 1991. A corrected sequence for the predicted protein from the mitogen-inducible TIS11 primary response gene. Oncogene 6:1277-1278[Medline].
26.	Ma, W.-J., S. Cheng, C. Campbell, A. Wright, and H. Furneaux. 1996. Cloning and characterization of HuR, a ubiquitously expressed Elav-like protein. J. Biol. Chem. 271:8144-8151[Abstract/Free Full Text].
27.	Mathey-Prevot, B., N. C. Andrews, H. S. Murphy, S. G. Kreissman, and D. G. Nathan. 1990. Positive and negative elements regulate human interleukin 3 expression. Proc. Natl. Acad. Sci. USA 87:5046-5050[Abstract/Free Full Text].
28.	McKendry, R., J. John, D. Flavell, M. Muller, I. M. Kerr, and G. R. Stark. 1991. High-frequency mutagenesis of human cells and characterization of a mutant unresponsive to both alpha and gamma interferons. Proc. Natl. Acad. Sci. USA 88:11455-11459[Abstract/Free Full Text].
29.	Ming, X. F., M. Kaiser, and C. Moroni. 1998. c-jun N-terminal kinase is involved in AUUUA-mediated interleukin-3 mRNA turnover in mast cells. EMBO J. 17:6039-6048[CrossRef][Medline].
30.	Morgenstern, J. P., and H. Land. 1990. Advanced mammalian gene transfer: high titre retroviral vectors with multiple drug selection markers and a complementary helper-free packaging cell line. Nucleic Acids Res. 18:3587-3596[Abstract/Free Full Text].
31.	Myer, V. E., X. C. Fan, and J. A. Steitz. 1997. Identification of HuR as a protein implicated in AUUUA-mediated mRNA decay. EMBO J. 16:2130-2139[CrossRef][Medline].
32.	Nair, A. P., I. D. Diamantis, J. F. Conscience, V. Kindler, P. Hofer, and C. Moroni. 1989. A v-H-ras-dependent hemopoietic tumor model involving progression from a clonal stage of transformation competence to autocrine interleukin 3 production. Mol. Cell. Biol. 9:1183-1190[Abstract/Free Full Text].
33.	Nair, A. P., S. Hahn, R. Banholzer, H. H. Hirsch, and C. Moroni. 1994. Cyclosporin A inhibits growth of autocrine tumour cell lines by destabilizing interleukin-3 mRNA. Nature 369:239-242[CrossRef][Medline].
34.	Nair, A. P., H. H. Hirsch, and C. Moroni. 1992. Mast cells sensitive to v-H-ras transformation are hyperinducible for interleukin 3 expression and have lost tumor-suppressor activity. Oncogene 7:1963-1972[Medline].
35.	Pellegrini, S., J. John, M. Shearer, I. M. Kerr, and G. R. Stark. 1989. Use of a selectable marker regulated by alpha interferon to obtain mutations in the signaling pathway. Mol. Cell. Biol. 9:4605-4612[Abstract/Free Full Text].
36.	Peng, S. S., C. Y. Chen, N. Xu, and A. B. Shyu. 1998. RNA stabilization by the AU-rich element binding protein, HuR, an ELAV protein. EMBO J. 17:3461-3470[CrossRef][Medline].
37.	Ross, J. 1995. mRNA stability in mammalian cells. Microbiol. Rev. 59:423-450[Abstract/Free Full Text].
38.	Schuler, G. D., and M. D. Cole. 1988. GM-CSF and oncogene mRNA stabilities are independently regulated in trans in a mouse monocytic tumor. Cell 55:1115-1122[CrossRef][Medline].
39.	Shaw, G., and R. Kamen. 1986. A conserved AU sequence from the 3' untranslated region of GM-CSF mRNA mediates selective mRNA degradation. Cell 46:659-667[CrossRef][Medline].
40.	Shyu, A.-B., M. E. Greenberg, and J. G. Belasco. 1989. The c-fos transcript is targeted for rapid decay by two distinct mRNA degradation pathways. Genes Dev. 3:60-72[Abstract/Free Full Text].
41.	Stoecklin, G., S. Hahn, and C. Moroni. 1994. Functional hierarchy of AUUUA motifs in mediating rapid interleukin-3 mRNA decay. J. Biol. Chem. 269:28591-28597[Abstract/Free Full Text].
42.	Taylor, D. S., J. P. Laubach, D. G. Nathan, and B. Mathey-Prevot. 1996. Cooperation between core binding factor and adjacent promoter elements contributes to the tissue-specific expression of interleukin-3. J. Biol. Chem. 271:14020-14027[Abstract/Free Full Text].
43.	Taylor, G. A., E. Carballo, D. M. Lee, W. S. Lai, M. J. Thompson, D. D. Patel, D. I. Schenkman, G. S. Gilkeson, H. E. Broxmeyer, B. F. Haynes, and P. J. Blackshear. 1996. A pathogenetic role for TNF alpha in the syndrome of cachexia, arthritis, and autoimmunity resulting from tristetraprolin (TTP) deficiency. Immunity 4:445-454[CrossRef][Medline].
44.	Taylor, G. A., M. J. Thompson, W. S. Lai, and P. J. Blackshear. 1995. Phosphorylation of tristetraprolin, a potential zinc finger transcription factor, by mitogen stimulation in intact cells and by mitogen-activated protein kinase in vitro. J. Biol. Chem. 270:13341-13347[Abstract/Free Full Text].
45.	Varnum, B. C., R. W. Lim, V. P. Sukhatme, and H. R. Herschman. 1989. Nucleotide sequence of a cDNA encoding TIS11, a message induced in Swiss 3T3 cells by the tumor promoter tetradecanoyl phorbol acetate. Oncogene 4:119-120[Medline].
46.	Wellington, C. L., M. E. Greenberg, and J. G. Belasco. 1993. The destabilizing elements in the coding region of c-fos mRNA are recognized as RNA. Mol. Cell. Biol. 13:5034-5042[Abstract/Free Full Text].
47.	Wisdom, R., and R. Lee. 1991. The protein-coding region of c-myc mRNA contains a sequence that specifies rapid mRNA turnover and induction by protein synthesis inhibitors. Genes Dev. 5:232-243[Abstract/Free Full Text].
48.	Wyss, A., and C. Moroni. Calcium-dependent and oncogenic IL-3 mRNA stabilization can be distinguished pharmacologically and by sequence requirements in the 3' UTR. Growth Factors, in press.
49.	Zhang, W., B. J. Wagner, K. Ehrenman, A. W. Schaefer, C. T. DeMaria, D. Crater, K. DeHaven, L. Long, and G. Brewer. 1993. Purification, characterization, and cDNA cloning of an AU-rich element RNA-binding protein, AUF1. Mol. Cell. Biol. 13:7652-7665[Abstract/Free Full Text].