ATF4 Degradation Relies on a Phosphorylation-Dependent Interaction with the SCF{beta}TrCP Ubiquitin Ligase

doi:10.1128/MCB.21.6.2192-2202.2001

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Molecular and Cellular Biology, March 2001, p. 2192-2202, Vol. 21, No. 6
0270-7306/01/$04.00+0 DOI: 10.1128/MCB.21.6.2192-2202.2001
Copyright © 2001, American Society for Microbiology. All rights reserved.

ATF4 Degradation Relies on a Phosphorylation-Dependent Interaction with the SCF^TrCP Ubiquitin Ligase

Irina Lassot,¹ Emmanuel Ségéral,¹ Clarisse Berlioz-Torrent,¹ Herve Durand,¹ Lionel Groussin,² Tsonwin Hai,³ Richard Benarous,¹^,^* and Florence Margottin-Goguet¹

INSERM Unite 529, Interactions Moléculaires Hôte-pathogène¹ and CNRS, UPR 1524, Institut Cochin de Génétique Moléculaire,² 75014 Paris, France, and Department of Molecular and Cellular Biochemistry and Neurobiotechnology Center, Ohio State University, Columbus, Ohio³

Received 7 August 2000/Returned for modification 19 September 2000/Accepted 12 December 2000

	ABSTRACT

Top Abstract Introduction Materials and Methods Results Discussion References

The ubiquitin-proteasome pathway regulates gene expression through protein degradation. Here we show that the F-box protein $beta$ TrCP, the receptor component of the SCF E3 ubiquitin ligase responsiblefor I $kappa$ B $alpha$ and $beta$ -catenin degradation, is colocalized in the nucleuswith ATF4, a member of the ATF-CREB bZIP family of transcriptionfactors, and controls its stability. Association between the twoproteins depends on ATF4 phosphorylation and on ATF4 serine residue219 present in the context of DSGXXXS, which is similar but notidentical to the motif found in other substrates of $beta$ TrCP. ATF4ubiquitination in HeLa cells is enhanced in the presence of $beta$ TrCP.The F-box-deleted $beta$ TrCP protein behaves as a negative transdominantmutant that inhibits ATF4 ubiquitination and degradation and,subsequently, enhances its activity in cyclic AMP-mediated transcription.ATF4 represents a novel substrate for the SCF^TrCP complex, which is the first mammalian E3 ubiquitin ligase identifiedso far for the control of the degradation of a bZIP transcriptionfactor.

	INTRODUCTION

Top Abstract Introduction Materials and Methods Results Discussion References

Proteasome-mediated protein degradation requires the covalent attachment of polyubiquitin to the substrate proteins (11,25, 38). The cascade of ubiquitin transfer reactions involvesthe ubiquitin-activating enzyme E1, an E2 ubiquitin-conjugatingenzyme that operates with specificity factor E3. The selectivityof the reaction is due to the E3 ubiquitin ligase, which interactswith both E2 and thesubstrate.

SCF (Skp1/Cullin/F-box protein) complexes were initially shown to function as E3 ubiquitin ligases for a variety of phosphorylatedproteins involved in the yeast cell cycle (1, 15, 35, 52,60). The core components of these complexes include Skp1, Cul-1(Cdc53), and the newly identified protein Rbx1 (Roc1 or Hrt1),which is thought to stabilize the interaction between Cul-1 andthe E2 enzyme Cdc34 (12, 14, 30, 61). The SCF complexesalso contain a variable receptor subunit, an F-box-containingprotein, that provides substrate specificity. The F-box motifserves to anchor the receptor subunit to the SCF complex by itsinteraction with Skp1 (12, 14, 52, 60). For ubiquitination,substrate proteins are recruited to the SCF E3 ubiquitin ligasecomplexes through interaction with the substrate binding domain(WD-40 or leucine-rich repeats) of the F-box receptor subunits.SCF complexes are the largest and most versatile class of E3 ubiquitinligases. To date, only two human SCF complexes, SCF^Skp2 and SCF^TrCP, have been analyzed in detail and have had some of their substratescharacterized (6, 7, 23, 36, 39, 41-44, 49, 62,63, 67, 68). We made the first identification of human $beta$ TrCP(beta-transducin repeat-containing protein) as the F-box receptorcomponent of the E3 ubiquitin ligase SCF^TrCP responsible for the degradation of CD4 induced by the human immunodeficiencyvirus type 1 (HIV-1) protein Vpu (43). Subsequently, we andothers showed that SCF^TrCP is also responsible for phosphorylation-dependent ubiquitinationand then for the degradation of I $kappa$ B $alpha$ and $beta$ -catenin (23, 36,39, 42, 62, 67, 68). Vpu, I $kappa$ B $alpha$ , and $beta$ -catenin sharea common motif, DSGXXS. Phosphorylation of its serine residuesis required for interaction with $beta$ TrCP. I $kappa$ B $alpha$ is phosphorylatedon the DS₃₂GXXS₃₆ motif by IKK $alpha$ and IKK $beta$ protein kinases activatedthrough various signaling events (31). It is commonly thoughtthat I $kappa$ B $alpha$ is subsequently ubiquitinated and degraded in the cytoplasm,resulting in NF- $kappa$ B nuclear translocation and transcription stimulationof target genes (31). Similarly, it is also thought that $beta$ -cateninubiquitination and subsequent degradation take place in the cytoplasm,preventing nuclear translocation of the protein which is requiredfor TCF/LEF transcriptional activation of target genes (53).

ATF4 is a member of the ATF/CREB proteins that include CREB (cAMP responsive element binding protein), CREM (CRE modulator),ATF1, ATF2, and ATF3 (for reviews, see references 4, 22,46, 57 and 69). These proteins bind to DNA via their basicregion and dimerize via their leucine zipper domain to form alarge variety of homodimers and/or heterodimers that allow thecell to coordinate signals from different pathways (4, 22,46, 57, 69). Thus far, two other names have been used torefer to human ATF4 (21): CREB2 (32) and TAXREB67 (65).In addition, mouse cDNAs with 85% homology to human ATF4 havebeen referred to as mATF4 (47), C/ATF (66), or mTR67 (8).In the rest of this report, we will refer to it as ATF4. The E2ubiquitin-conjugating enzymes involved in the degradation of somemembers of the ATF/CREB family have recently been identified;they include Cdc34 and Rad6B for hICER $gamma$ and ATF5 (ATFx), respectively(51), and hUBC9 for ATF2 (16). However, the E3 ubiquitin ligasesrequired to make mammalian ATF/CREB transcription factor substratesfor the proteasome remain unknown. While this paper was in preparation,Meimoun et al. identified the E3 ubiquitin ligase SCF^Cdc4 complex as responsible for degradation of the bZIP transcriptionfactor Gcn4 in yeast (45).

There has been considerable interest in the role of ATF/CREB transcription factors and regulation of their activity by phosphorylation.In eukaryotes, cyclic (cAMP)-mediated transcription regulatesmultiple physiological processes, including gametogenesis, circadianrhythm, and neuroendocrine functions (13). Stimulation of thispathway is mediated via phosphorylation by protein kinase A (PKA)of a single serine in the structurally similar transcription factorsCREB, CREM, or ATF1 (13). However, ATF4 lacks potential PKAphosphorylation sites and has been demonstrated to be a negativeregulator of CRE-dependent transcription (2, 32). In contrast,ATF4 was proposed to be a positive regulator of transcription(40), increasing the expression of genes, such as somatostatin,serotonin, or interleukin-2 (2, 5, 66), and that of thehuman T-cell leukemia virus type 1 by interacting with the viraltransactivator Tax (19, 54). How the versatile effects ofATF4 are regulated in these different pathways has not been investigatedyet.

We found that ATF4 and $beta$ TrCP are associated in vivo and colocalized in the nucleus. Our results suggest that SCF^TrCP tightly modulates the stability of the transcription factor ATF4and therefore also modulates its transcriptional activity followingactivation of the cAMPpathway.

	MATERIALS AND METHODS

Top Abstract Introduction Materials and Methods Results Discussion References

Two-hybrid assays. Yeast two-hybrid screening was performed as described previously (3). Saccharomyces cerevisiae HF7 cells were transformedwith the bait plasmid containing seven WD-40 repeats of human $beta$ TrCP (residues 251 to 569) fused to the Gal4 DNA binding domainin the pGBT10 plasmid and with a human Jurkat cDNA library fusedto the GAL4 transactivation domain in the pGAD13-18 plasmid. Transformantswere screened on plates lacking tryptophan, leucine, and histidineand were then assayed for $beta$ -galactosidase activity. For interactionassays, $beta$ TrCP, Slimb (27), or Fbw2 (9) and ATF4 or Skp1 werefused, respectively, to Escherichia coli LexA or the Gal4 bindingdomain and the Gal4 activation domain. The yeast reporter strainL40 or HF7 expressing the indicated hybrid protein pairs was analyzedfor $beta$ -galactosidase expression or for histidineauxotrophy.

Plasmid construction and mutagenesis. The ATF4 cDNA found in the screen corresponds to the protein accession number P18848. ATF4 $Delta$ BZ was obtained by PCR withspecific primers and was subcloned in the pGAD13-18 vector (3).ATF4 point mutations (D218N, S219N, G220A, S224N) were constructedby PCR mutagenesis. pGADSkp1 plasmid and pcDNA3 expression vectorsfor $beta$ TrCP-Myc and $beta$ TrCP $Delta$ F-Myc have already been described (23,36). $beta$ TrCP $Delta$ W1, $beta$ TrCP $Delta$ W2-7, and $beta$ TrCP $Delta$ N were obtained by PCRwith appropriate primers and subcloned in the pcDNA3.1A/Myc-Hisvector (Invitrogen). Hemagglutinin (HA)-ATF4, HA- $beta$ TrCP, and HA- $beta$ TrCP $Delta$ Fwere obtained following direct subcloning of ATF4, $beta$ TrCP, and $beta$ TrCP $Delta$ F in the pAS1B vector (59). The Myc-His sequence in thepcDNA3.1/Myc-His vector was replaced by the green fluorescentprotein (GFP) coding sequence, resulting in pcDNA3- $beta$ TrCP-GFP.The pAS2 expression vector for Fbw2 was kindly provided by J.Hsu and P.Jackson.

Coimmunoprecipitation experiments. Samples containing 8 × 10⁶ HeLa cells were transiently cotransfected by electroporation with 10 µg of either pAS1B, pAS1B-ATF4,or pAS1B-ATF4S219N and with 15 µg of the pcDNA3.1A/Myc-His plasmidcontaining wild-type or mutant $beta$ TrCP sequences. Cells were eithernot pretreated or were pretreated with 20 µM Z-LLL-H (N-benzyloxycarbonyl-L-leucyl-L-leucyl-L-leucinal; MG132; Sigma)for 4 h and then cells were harvested 48 h after transfectionand lysed in 1% NP-40 lysis buffer (1% Nonidet P-40, 150 mM NaCl,50 mM Tris-HCl [pH 7.5], 1 mM EDTA). For immunoprecipitations,cell lysates were incubated with 5 µg of rat monoclonal anti-HAantibody per ml (clone 3F10; Boehringer) or 5 µg of mouse monoclonalanti-Myc antibody per ml (clone 9E10; Santa Cruz) for 90 min andthen incubated with protein G-agarose beads (Boehringer) for 1h. To study the association of ATF4 and $beta$ TrCP endogenous proteins,we performed a coimmunoprecipitation in untransfected 293T cellslysed using the NP-40 lysis buffer. The lysate was preclearedwith rabbit nonimmune antibodies and protein A-agarose (Sigma)for 90 min. Supernatant was incubated with anti- $beta$ TrCP antibody(43) or anti-ATF4 antibody [raised in rabbits by immunizationwith the fragment 207-351 of human ATF4 expressed in BL21(DE3)LysSbacteria and purified by sodium dodecyl sulfate-polyacrylamidegel electrophoresis (SDS-PAGE)] or nonimmune rabbit polyclonalantibodies for 90 min and then were incubated with protein A-agarose(Sigma) for 30 min. The beads were washed with lysis buffer. Immunecomplexes were eluted with Laemmli sample buffer, separated bySDS-12% PAGE, and revealed by chemiluminescence using rat anti-HA(clone 3F10; Boehringer) or mouse anti-Myc (clone 9E10; SantaCruz) or goat polyclonal anti- $beta$ TrCP (C-18; Santa Cruz) antibodies.To demonstrate the specificity of the anti-ATF4 antibodies, weused both immunoprecipitation and Western blot experiments withcells transfected by HA-ATF4 and compared the results with thoseobtained by Western blotting with untransfected 293T cells. Whenneeded, quantitation of the chemiluminescent signal was performedusing NIH Image software. Where indicated, treatment of immunoprecipitateswith 32 U of alkaline bovine phosphatase corresponding to a finalconcentration of 180 µg/ml (P6774; Sigma) was administered toimmune complexes for 45 min at 30°C in 50 mM Tris (pH 7.5)-1 mMMgCl₂.

Ubiquitination assay. In vivo ubiquitination was assayed as described by Treier et al. (64). Six-His tag-ubiquitin (10 µg) and HA-ATF4 (8 µg)expression vectors were transiently cotransfected by electroporationin HeLa cells. Twenty-four hours later, cells were lysed with6 M guanidinium-HCl (pH 8), and His-tagged proteins were purifiedby nickel resins Ni-nitrilotriacetic acid agarose (Qiagen) asdescribed by Treier et al. (64), eluted with Laemmli samplebuffer, and separated by SDS-10% PAGE. Ubiquitin-conjugated HA-ATF4proteins were revealed by chemiluminescence using anti-HA antibody(clone 3F10;Boehringer).

Immunostaining of cells. For ATF4 and $beta$ TrCP localization, HeLa cells were transiently transfected by electroporation with 15 µg of pAS1B-ATF4 and 15µg of pcDNA3- $beta$ TrCP-GFP and seeded onto glass plates at a densityof 50,000 cells/plate. At 48 h, cells were washed with phosphate-bufferedsaline (PBS) and fixed for 20 min in 4% paraformaldehyde, quenchedfor 10 min with 0.1 M glycine in PBS, and permeabilized for 30min at room temperature with 0.05% saponin in PBS-0.2% bovineserum albumin. Cells were incubated with anti-HA antibody (1/10dilution), washed in PBS, and incubated with goat anti-rat Texas-RedRsecondary antibodies (1/125 dilution; Jackson Immunoresearch).Confocal microscopy was carried out under fluorescentlight.

³⁵S metabolic labeling and pulse-chase experiments. At 24 h after electroporation with various plasmids (pAS1B for ATF4 proteins and pcDNA3 for $beta$ TrCP proteins), 10⁶ HeLa cells were incubated for 30 min in Met and Cys-free Dulbeccomodified Eagle medium (DMEM), and then 125 µCi of [³⁵S]methionine-cysteine (NENlife) per ml was added to the same mediumfor 1 h. Similarly, to study the stability of ATF4 endogenousprotein, metabolic labeling was performed with 293T cells thatwere untransfected or were transfected with pcDNA3- $beta$ TrCP and werenot pretreated or were pretreated with Z-LLL-H (Sigma). Cellswere washed in PBS and harvested (time zero) or incubated for0.5, 1, 2, 3, 3.5, or 4 h in complete DMEM, washed again in PBS,and lysed as described previously. Cell lysates were immunoprecipitatedwith mouse monoclonal anti-HA (12CA5; Boehringer) or rabbit polyclonalanti-ATF4 antibodies and incubated with protein G-agarose or proteinA-agarose (Sigma) beads. Beads were washed with lysis buffer supplementedwith NaCl (300 mM final concentration), and immune complexes wereeluted with Laemmli sample buffer, separated on SDS-12% PAGE gels,fixed in acetic acid (10%)-methanol (30%), dried, and exposedto Kodak X-Omat film. Quantitation was performed with an ImageQuantphosphorimager (MolecularDynamics).

Luciferase assays. 293T cells were plated in 6-well flat-bottom plates on the day prior to transfection at a density of 5 × 10⁴ cells/35-mm-diameter well in DMEM. Transfections were performedusing the calcium phosphate coprecipitation method with the MammalianTransfection Kit (Stratagene). We used the luciferase reporterpSS-CRE-LUC containing a sequence of rat somatostatin gene from $-$ 71 to 53 (37) (including the CRE site) placed 5' to the genefor luciferase. Cells were cotransfected with 0.2 µg of pSS-CRE-LUC,3 ng of pRL-TK-renilla (PRL-TK from Promega), and various amountsof plasmids expressing HA-ATF4, HA-TrCP, or HA-TrCP $Delta$ F as indicated.Six hours prior to harvesting, half of the transfected disheswere incubated in a mixture of 10⁵ M forskolin (Sigma) and 0.5 mM 3-isobutyl-1-methylxanthine (IBMX;Sigma). At 24 h posttransfection, cells were lysed and luciferaseand renilla activities were measured with luciferase assay reagent(Dual-Luciferase Reporter Assay System; Promega) by using a LumatLB9507 luminometer (EG&GInstruments).

	RESULTS

Top Abstract Introduction Materials and Methods Results Discussion References

$beta$ TrCP interacts with ATF4. In order to find new substrates of $beta$ TrCP, we used the two-hybrid system. The C-terminal substrate-recruiting domain of $beta$ TrCP,which contains the seven WD-40 repeats (residues 251 to 569),was chosen as a bait (Fig. 1A) and was fused to the Gal4 DNA bindingdomain (43). A cDNA library from Jurkat cells, constructed infusion with the Gal4 activation domain, was screened as previouslydescribed (3). Four clones interacting specifically with theWD-40 repeats of $beta$ TrCP and which corresponded to human ATF4 cDNA,with different 5' ends within the N-terminal region, were isolated.Interaction between $beta$ TrCP and full-length ATF4 is shown in Fig.1B, lane 1. No other proteins from the ATF/CREB family were isolatedfrom our screen. The structure of $beta$ TrCP and ATF4 proteins is schematizedin Fig. 1A. Deletion experiments allowed us to map the interactingdomains between the two proteins, respectively, on the seven WD-40repeats at the C terminus of $beta$ TrCP and between residues 87 to279 of ATF4 (data not shown). The deletion of the basic regionand the leucine zipper domain of ATF4 (ATF4 $Delta$ BZ), both locatedat the C terminus of the protein, did not affect the interactionwith $beta$ TrCP (Fig. 1B, lane 2). The interaction of ATF4 with human $beta$ TrCP was specific since it was not found with other members ofthe WD-40 and F-box proteins, such as Fbw2 (the human homologof mouse MD6; 9, 48) (Fig. 1C, lane 3) or the Drosophila melanogasterhomolog of $beta$ TrCP, Slimb (Fig. 1C, lane 1) (27), although theseproteins both interact with Skp1 (Fig. 1C, lanes 2 and 4). Thehuman isoform of $beta$ TrCP, $beta$ TrCP2, interacts with ATF4 (data notshown).

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FIG. 1. Interaction of $beta$ TrCP with ATF4 is impaired by mutation on the D218 and S219 ATF4 residues. (A) Scheme of protein structures of $beta$ TrCP and ATF4. The diagram of $beta$ TrCP shows the F box responsible for proteasome targeting through Skp1 binding and the seven WD-40 repeats involved in binding substrates. For ATF4, the basic region (b) and the leucine zipper domain (Z) are indicated in addition to the DSGXXXS motif. (B) The yeast reporter strain L40 expressing the indicated hybrid protein pairs was analyzed for $beta$ -galactosidase expression. $beta$ TrCP was fused to the E. coli LexA binding domain in the pLex plasmid. ATF4 sequences were fused to the Gal4 activation domain in pGAD13-18. (C) The yeast reporter strains L40 or HF7 expressing the indicated hybrid protein pairs were analyzed for histidine auxotrophy.

Serine 219 of ATF4 is required for interaction with $beta$ TrCP. The phosphorylation motif DSGXXS required for interaction of $beta$ TrCP with its substrates HIV-1 Vpu (43), I $kappa$ B $alpha$ , and $beta$ -catenin(23, 36, 39, 42, 62, 67, 68) was not found in theATF4 sequence. However, a closely related motif of the type DSGXXXSoccurred at positions 218 to 224 (Fig. 1A). Single amino acidsubstitutions in this motif, D218N or S219N, were sufficient toimpair ATF4 interaction with $beta$ TrCP, whereas mutation of ATF4 residuesG220 and S224 did not affect such interaction (Fig. 1B, lanes3 to6).

ATF4 and $beta$ TrCP were tagged with HA and Myc epitopes, respectively, and were transiently expressed in HeLa cells to determinewhether the ATF4- $beta$ TrCP interaction can take place in vivo. HA-ATF4was then immunoprecipitated using anti-HA antibody. Wild-type $beta$ TrCP was coprecipitated with HA-ATF4 (Fig. 2A, top, lane 2).Deletion of the first WD-40 repeat or the last six WD-40 repeatsin $beta$ TrCP ( $beta$ TrCP $Delta$ W1 and $beta$ TrCP $Delta$ W2-7) abolished the association withATF4, confirming that the WD-40 repeats are the binding site forATF4 (Fig. 2A, top, lanes 4 and 6). Expression of HA-ATF4 waschecked and was shown to be identical irrespective of the $beta$ TrCPmutant proteins expressed (Fig. 2A, bottom). In addition, deletionin $beta$ TrCP of the F-box motif ( $beta$ TrCP $Delta$ F) or of the N-terminal regionupstream of the F-box motif ( $beta$ TrCP $Delta$ N) did not affect associationwith ATF4 (Fig. 2B, top, lane 4, and Fig. 2A, top, lane 8, respectively).In ATF4, mutation of the serine residue at position 219 againabolished the interaction with $beta$ TrCP or $beta$ TrCP $Delta$ F (Fig. 2B, top;compare lanes 6 and 7 with lanes 2 and 4, respectively), althoughthe level of the ATF4 S219N mutant was higher than that of wild-typeATF4 (Fig. 2B, bottom; compare lane 6 to lane 2). In the presenceof the proteasome inhibitor Z-LLL-H, the amount of accumulatedATF4 was fivefold higher (Fig. 2C, right; compare lane 8 to lane6), and subsequently, the ATF4- $beta$ TrCP interaction was stabilized(Fig. 2C, left; compare lane 4 to lane 2).

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FIG. 2. $beta$ TrCP-ATF4 association in HeLa and 293T cells. (A) HeLa cells were transfected with HA-ATF4 expression vector (lanes 2, 4, 6, and 8) or the corresponding empty vector (lanes 1, 3, 5, and 7) and plasmids expressing $beta$ TrCP protein tagged with the Myc epitope, wild-type $beta$ TrCP (lanes 1 and 2), or $beta$ TrCP deleted either from its first WD-40 repeat ( $beta$ TrCP $Delta$ W1, lanes 3 and 4) or from WD-40 repeats 2 to 7 ( $beta$ TrCP $Delta$ W2-7, lanes 5 and 6) or from its N-terminal region from residues 1 to 144 ( $beta$ TrCP $Delta$ N, lanes 7 and 8). Proteins from total cytoplasmic lysates were immunoprecipitated with anti-HA antibodies (IP $alpha$ -HA) and probed with anti-Myc antibodies (WB $alpha$ Myc) (top) or directly probed with anti-Myc antibodies (middle) or anti-HA antibodies (bottom). (B) HeLa cells were transfected with wild-type (wt) ATF4 (lanes 2, 4 and 5), empty vector (lanes 1 and 3), or the S219N ATF4 mutant (lanes 6 and 7) and with $beta$ TrCP (lanes 1, 2, and 6), $beta$ TrCP deleted from its F-box motif ( $beta$ TrCP $Delta$ F, lanes 3, 4, and 7), or the corresponding empty vector (lane 5). Anti-HA immunoprecipitates (IP $alpha$ -HA) were analyzed by immunoblotting with anti-Myc antibodies (WB $alpha$ Myc) (top) or lysates were directly probed with anti-HA antibodies (bottom). (C) At 48 h after transfection of vectors expressing $beta$ TrCP (lanes 1 to 8) and ATF4 (lanes 2, 4, 6, and 8) or empty vector (lanes 1, 3, 5, and 7), cells were exposed to Z-LLL-H for 4 h (lanes 3, 4, 7, and 8) or were left untreated (lanes 1, 2, 5, and 6). Anti-HA immunoprecipitates were analyzed with anti-Myc antibodies (lanes 1 to 4) or lysates were directly probed with HA antibodies (lanes 5 to 8). (D) Anti-ATF4 (lanes 1 and 2) or anti-HA (lane 3) antibodies were used to immunoprecipitate lysates from untransfected 293T cells (lane 1) or transfected cells expressing HA-ATF4 (lanes 2 and 3). The immunoprecipitates were probed with anti-HA (lanes 1 and 2) or with anti-ATF4 (lane 3) antibodies. Anti-ATF4 antibodies were used in Western blotting with total lysates from HA-ATF4 transfected cells (lane 4) or from untransfected cells (lane 5). (E) Proteins from 293T cell total lysate (lane 4) were immunoprecipitated with rabbit anti- $beta$ TrCP (lane 1), anti-ATF4 (lane 2), or nonimmune (lane 3) antibodies and were probed with goat anti- $beta$ TrCP antibodies. Western blotting from a total lysate of untransfected cells with goat anti- $beta$ TrCP antibodies is shown in lane 4.

Endogenous $beta$ TrCP coimmunoprecipitates with endogenous ATF4. In order to check that both endogenous ATF4 and $beta$ TrCP proteins were also associated, we performed immunoprecipitations ofuntransfected cell lysates with anti-ATF4 antibodies, and theimmunoprecipitate was probed by Western blotting with anti- $beta$ TrCPantibodies. The anti- $beta$ TrCP antibodies have been previously characterizedby us (43) or by the supplier (Santa Cruz). In order to assessthe specificity of the anti-ATF4 antibodies, we checked, as shownin Fig. 2D, that these antibodies can recognize specifically HA-ATF4,in both Western blot and immunoprecipitation experiments (Fig.2D, lanes 2, 3, and 4). In transfected cells expressing HA-ATF4,two bands were detected by Western blotting using anti-ATF4 antibodies(Fig. 2D, lane 4). The upper band corresponds to the exogenousHA-ATF4 since it comigrates with HA-ATF4 precipitated by anti-HAantibodies (Fig. 2D, lane 3). The lower band, with an approximatemolecular mass of 35 kDa, the only one detected in the untransfectedcells, corresponds to the endogenous ATF4 (Fig. 2D, lanes 4 and5). As shown in Fig. 2D, lane 2, anti-ATF4 antibodies efficientlyimmunoprecipitated HA-ATF4. Thus, these antibodies could be usedfor coimmunoprecipitation experiments of endogenous ATF4 and endogenous $beta$ TrCPproteins.

As shown in Fig. 2E (lane 2), a protein recognized by anti- $beta$ TrCP antibodies and migrating as a band with a molecular massof 60 kDa was present in the anti-ATF4 immunoprecipitate. Thisband was clearly identified as $beta$ TrCP since it was also found inthe immunoprecipitate with anti- $beta$ TrCP antibodies (Fig. 2E, lane1) but not in the immunoprecipitate with non-immune antibodies(Fig. 2E, lane 3). Thus, this experiment demonstrates that theendogenous proteins interact in untransfectedcells.

ATF4- $beta$ TrCP interaction depends on ATF4 phosphorylation. In vivo interaction between ATF4 and $beta$ TrCP was confirmed by coimmunoprecipitation of HA-ATF4 with Myc-tagged $beta$ TrCP or Myc-tagged $beta$ TrCP $Delta$ F by using anti-Myc antibody (Fig. 3, lanes 2 and 4). Toassess whether ATF4 that coprecipitated with $beta$ TrCP proteins wasa phosphorylated form of ATF4, treatment of the immunoprecipitateswith alkaline phosphatase was performed prior to denaturationand loading on SDS-PAGE gels. As shown in Fig. 3 (compare lane3 to lane 2 and lane 5 to lane 4), such phosphatase treatmentgave rise to a faster migrating band of HA-ATF4. This result isconsistent with the fact that ATF4 which was associated with $beta$ TrCPin the anti-Myc immunoprecipitate was phosphorylated. Interestingly,when HA-ATF4 was immunoprecipitated with anti-HA antibody, twobands of HA-ATF4 were detected in the immunoprecipitate (Fig.3, lane 6). From these results, one can conclude that only thephosphorylated forms of ATF4 can associate with $beta$ TrCP.

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FIG. 3. ATF4- $beta$ TrCP interaction depends on ATF4 phosphorylation. After transfection of vectors expressing HA-ATF4 (lanes 1 to 6) and $beta$ TrCP-Myc (lanes 2 and 3) or $beta$ TrCP $Delta$ F-Myc (lanes 4 and 5) or the empty vector pcDNA3 (lanes 1 and 6), anti-Myc or anti-HA immunoprecipitates (IP $alpha$ -Myc and IP $alpha$ HA, respectively) were left untreated (lanes 1, 2, 4, and 6) or were exposed to phosphatase treatment (lanes 3 and 5). Immunoprecipitates were probed with anti-HA antibodies (WB $alpha$ HA).

ATF4 ubiquitination is enhanced in the presence of wild-type $beta$ TrCP. To investigate the role of $beta$ TrCP as an E3 ubiquitin ligase for ATF4, we decided to establish an in vivo ubiquitination assayof ATF4. HA-ATF4 was transiently coexpressed with a six-His tag-ubiquitinin HeLa cells. Ubiquitin-conjugated proteins were purified usingnickel beads, and ubiquitin-conjugated ATF4 proteins were revealedby immunoblotting with HA antibodies. In the absence of the proteasomeinhibitor Z-LLL-H, no ubiquitin-conjugated ATF4 was detected onthe nickel beads (data not shown). In the presence of Z-LLL-H,ubiquitin-conjugated ATF4 was retained on the beads (Fig. 4, lane2). In the absence of six-His tag-ubiquitin, no HA-ATF4 was detectedon the beads after a short exposure (Fig. 4, lane 1, middle) althoughsome background signal could be seen after a long exposure (Fig.4, lane 1, top). To further confirm the role of $beta$ TrCP in ATF4ubiquitination, we investigated the effect of the expression of $beta$ TrCP and of the $beta$ TrCP $Delta$ F mutant on ATF4 ubiquitination. In thepresence of $beta$ TrCP, ATF4 ubiquitination was enhanced (Fig. 4, lane3, short exposure) and higher-molecular-weight ubiquitinated formscould be detected (Fig. 4, lane 3, long exposure). In contrast,the expression of $beta$ TrCP $Delta$ F, previously identified as a negativetransdominant able to inhibit degradation of I $kappa$ B $alpha$ , $beta$ -catenin,or CD4 (23, 36, 43), decreased ATF4 ubiquitination (Fig.4, lane 4, short exposure). $beta$ TrCP $Delta$ F behaves as a negative transdominantbecause it binds substrates, but the deletion of the F-box motifimpairs its association to Skp1, which is required for its recruitmentto the SCF-E3 ubiquitin ligase complex, and the targeting of substratesto the proteasome (23, 36, 43). As a control, we checkedthat the total amount of ATF4 in the cells was roughly similar(Fig. 4, bottom). Thus, these results further support the notionthat SCF^TrCP is the E3 ubiquitin ligase required for ATF4 ubiquitination.However, most of the ubiquitinated ATF4 that was recovered fromnickel beads had a low molecular mass and corresponded in majorityto monoubiquitinated ATF4 or to protein-conjugated ATF4 with avery small number of ubiquitin residues. In order to observe higher-molecular-weightforms of ATF4 representing polyubiquitinated protein, the longerexposure was needed. This result raises the question of whetherATF4 is preferentially targeted for monoubiquitination by SCF^TrCP.

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FIG. 4. ATF4 ubiquitination is enhanced in the presence of wild-type $beta$ TrCP. HeLa cells were transfected with HA-ATF4 expression vector (lanes 1 to 4), with plasmids expressing $beta$ TrCP (lane 3) or $beta$ TrCP $Delta$ F (lane 4) proteins or the corresponding empty vector (lanes 1 and 2), and with a six-His tag-ubiquitin expression vector (lanes 2 to 4). In vivo ubiquitin-conjugated proteins were purified, and ubiquitin-conjugated HA-ATF4 proteins were revealed by immunoblotting with HA antibody after a long exposure (top) or a short exposure (middle) of the film. The lower panel shows a control immunoblotting analysis of whole-cell extracts of HA-ATF4 expression.

$beta$ TrCP colocalizes with ATF4 in the nucleus. The $beta$ TrCP-ATF4 interaction was further investigated in HeLa cells by confirming the codistribution of the proteins by confocalmicroscopy. In transient-transfection assays, we found by indirectimmunofluorescence that $beta$ TrCP tagged either with GFP at the Cterminus or HA epitope at the N terminus is mainly in the nucleus(Fig. 5A and B). In these assays, the nucleoli were unlabeled.After cotransfection with vectors expressing $beta$ TrCP-GFP and HA-ATF4,which is a nuclear protein (10), $beta$ TrCP-GFP and HA-ATF4 werefound colocalized in the nucleus (Fig. 5C). All cells examinedwhich had been successfully cotransfected with vectors expressing $beta$ TrCP-GFP and HA-ATF4 showed such colocalization of the two proteinsin the nucleus.

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FIG. 5. $beta$ TrCp and ATF4 are codistributed in the nucleus. HeLa cells were transfected with a plasmid expressing $beta$ TrCP fused to the GFP protein at its C terminus ( $beta$ TrCP-GFP) (A), with a plasmid expressing $beta$ TrCP fused to the HA epitope at its N terminus (HA- $beta$ TrCP) (B), or with both $beta$ TrCP-GFP and HA-ATF4 expression vectors (C). (B and C) Cells were stained with a Texas red-conjugated anti-HA antibody. Cells were analyzed by confocal microscopy.

ATF4 is an unstable protein, and $beta$ TrCP modulates its stability. By ³⁵S metabolic labeling and pulse-chase experiments, we studied the stability of the endogenous ATF4 protein in the presenceor absence of the proteasome inhibitor Z-LLL-H in untransfectedcells and in transfected cells overexpressing $beta$ TrCP. As shownin Fig. 6, the addition of the proteasome inhibitor Z-LLL-H stabilizedATF4 considerably, since most of the protein was still detectableafter 3.5 h of chase (Fig. 6A and B). Overexpression of $beta$ TrCPresulted in a significant enhancement of the instability of theATF4 protein, with its half-life decreasing from 30 to 15 min(Fig. 6B). These results demonstrate that the endogenous proteinis an unstable protein with a half-life of about 30 min whichis stabilized in the presence of proteasome inhibitors. In addition,we found that the protein is further destabilized by overexpressionof $beta$ TrCP (Fig. 6A and B).

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FIG. 6. ATF4 is an unstable protein and $beta$ TrCP modulates its stability. (A) Untransfected 293T cells were not treated or were treated with the proteasome inhibitor MG132 (Z-LLL-H) as indicated, cells transfected with expression vector for $beta$ TrCP were [³⁵S]Met-Cys metabolically labeled and chased for 0, 0.5, or 3.5 h, and lysates were immunoprecipitated with anti-ATF4 antibodies and analyzed following SDS-12%PAGE and autoradiography. (B) Scanning of the gel shown in panel A was performed using a phosphorimager. The ratios of the amounts of ATF4 left undegraded at each time point relative to that of the starting material were plotted as a function of time. (C) The ATF4 S219N mutant which has lost its ability to interact with $beta$ TrCP is stabilized in HeLa cells. Vectors expressing wild-type HA-ATF4 or HA-ATF4 S219N were transfected, cells were [³⁵S]Met-Cys metabolically labeled and chased for 0, 1, 2, 3, and 4 h, and lysates were immunoprecipitated using anti-HA antibody and analyzed following SDS-12% PAGE and autoradiography. Immunoprecipitation with a lysate from labeled nontransfected cells (NT) was also performed. (D) Scanning of the gel shown in panel C. (E) Expression of the $beta$ TrCP $Delta$ F mutant inhibits ATF4 degradation. ATF4 was transfected in the presence of $beta$ TrCP, $beta$ TrCP $Delta$ F, or the corresponding empty vector pcDNA3, labeled, and immunoprecipitated as described for panel A. (F) Scanning of the gel shown in panel E.

Because of the critical importance of ATF4 residue serine 219 for interaction with $beta$ TrCP, we hypothesized that if such interactionplays a role in the control of the stability of this transcriptionfactor, the ATF4 S219N mutant should be stabilized by comparisonwith wild-type ATF4 when expressed in cells. The ATF4 wild typeand mutant S219N, both tagged with the HA epitope at the N terminus,were transfected in HeLa cells. At 24 h after transfection, ³⁵S metabolic labeling and pulse-chase experiments from 0 to 4 hwere carried out prior to immunoprecipitation using anti-HA antibodyand SDS-PAGE analysis (Fig. 6C). HA-ATF4 and HA-ATF4 S219N half-liveswere determined after quantification of the amounts of proteinimmunoprecipitated by anti-HA antibodies at each time point byusing a phosphorimager. The half-life of HA-ATF4 was found tobe of about 1 h (Fig. 6D). Of note is that the protein ran asa multiple set of bands, probably because phosphorylation eventshad taken place. The mutation S219N stabilized the protein, givingrise to a half-life of about 2.5 h (Fig. 6C and D). These resultsare in favor of a role for the $beta$ TrCP-ATF4 interaction in the stabilityof ATF4. Interestingly, the half-life of the overexpressed exogenousHA-ATF4 protein is significantly longer than that of the ATF4endogenous protein (1 h instead of 30 min). This observation mayindicate that the activity of the SCF^TrCP machinery to target ATF4 for degradation by the proteasome couldbe relatively limited in a context of overexpression of exogenousATF4.

To further confirm the role of $beta$ TrCP in the control of ATF4 degradation, we investigated the effect on HA-ATF4 stability ofthe expression of the $beta$ TrCP wild type and of the $beta$ TrCP $Delta$ F mutant(Fig. 6E). In the presence of $beta$ TrCP $Delta$ F, we observed that wild-typeATF4 was stabilized, with its half-life increasing from 60 to120 min (Fig. 6F). By contrast, expression of wild-type $beta$ TrCPshortened the half-life of the protein from 60 to 45 min (Fig.6F). We checked that expression of $beta$ TrCP or $beta$ TrCP $Delta$ F did not affectthe half-life of the ATF4 S219N mutant (data not shown). Fromthese results, we conclude that ATF4 behaves like the other substratesof $beta$ TrCP (Vpu/CD4, I $kappa$ B $alpha$ , and $beta$ -catenin) whose degradations wereimpaired by the negative transdominant mutant of $beta$ TrCP ( $beta$ TrCP $Delta$ F).Thus, ATF4 can be considered the fourth substrate of the SCF^TrCP identified sofar.

Transcriptional activity of ATF4 is inhibited by $beta$ TrCP. To check whether modulation of ATF4 stability by $beta$ TrCP had any functional consequences, we examined the effect of $beta$ TrCP or $beta$ TrCP $Delta$ F expression on the transcriptional activity of ATF4. ATF4was identified as a transcriptional factor capable of inhibitingor activating transcription mediated through CRE (2, 5,19, 32, 40, 54, 66). The activity of a luciferase reportergene under the control of the somatostatin promoter, which containsthe classical CRE binding site for the ATF/CREB transcriptionfactors, was analyzed in 293T human embryo kidney cells aftertransfection with ATF4 and $beta$ TrCP or $beta$ TrCP $Delta$ F expression vectorsand treatment with forskolin as a cAMP pathway stimulator. Consistentwith the results obtained by Karpinski et al. (32), overexpressionof ATF4 inhibited the CRE-dependent transcriptional stimulationinduced by forskolin treatment (Fig. 7A). Expression of $beta$ TrCPimpaired the repressor activity of ATF4, whereas expression of $beta$ TrCP $Delta$ F stimulated its activity (Fig. 7B). These results are consistentwith the stimulation of ATF4 degradation provoked by $beta$ TrCP overexpression(Fig. 6E) and with the stabilization of ATF4 resulting from inhibitionof ATF4 degradation induced by the expression of the $beta$ TrCP $Delta$ F-negativetransdominant mutant (Fig. 6E).

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FIG. 7. Repression transcriptional activity of ATF4 on the somatostatin promoter stimulated by forskolin is controlled by $beta$ TrCP. (A) 293T cells were transiently cotransfected with a reporter plasmid expressing luciferase under the control of the somatostatin CRE sequence and different amounts of ATF4 expression vectors. Cells were left untreated or were stimulated in the presence of forskolin and IBMX. Experiments were repeated three times with duplicate samples, and results of a representative experiment are shown. The stimulation factor is reported to the transcription level observed in the cells without transfected ATF4. (B) Increasing amounts of $beta$ TrCP or $beta$ TrCP $Delta$ F expression vectors were transfected in the presence of the CRE luciferase reporter plasmid and 0.2 µg of ATF4 vector.

	DISCUSSION

Top Abstract Introduction Materials and Methods Results Discussion References

The ubiquitin-proteasome degradation pathway is important at the level of transcription regulation to assure the controlledand timely termination of signaling by irreversible destructionof the activated transcription factors. Because the E3 ubiquitinligases are the factors responsible for the specificity of theubiquitin-dependent proteolysis process, it is essential to identifywhich E3 targets which transcription factors. Here we have identifiedSCF^TrCP as the first mammmalian E3 ubiquitin ligase responsible for degradationof ATF4, a transcription factor belonging to the important bZIPfamily. ATF4 binds to $beta$ TrCP, the component receptor of the E3complex by phosphorylation-dependent interaction, and is colocalizedin the nucleus with this protein. We have found that $beta$ TrCP controlsthe stability of ATF4 and subsequently its transcriptional activity.However, the results of our in vivo ubiquitination experimentsraise the question of whether ATF4 is preferentially targetedfor monoubiquitination by SCF^TrCP.

It was recently reported by Kaiser et al. (29) that the ubiquitination of the transcription factor Met4 mediated by theF-box protein Met30 in yeast would not lead to its degradationas previously shown by Rouillon et al. (56) but neverthelessresults in the inhibition of Met4 transcriptional activity. Since,among the yeast F-box proteins, Met30 is the closest homolog to $beta$ TrCP, one can wonder whether the same phenomenon of regulationof transcription by ubiquitination without proteolysis describedfor Met30 could also be observed with $beta$ TrCP. Although this cannotbe ruled out from our results, we do not favor this hypothesisbecause in contrast with Met4, which was found to be a relativelystable protein (29), we observed that endogenous ATF4 is anunstable protein with a half-life of 30 min, further destabilizedby overexpression of $beta$ TrCP, which shortens the half-life of theprotein by a factor oftwo.

ATF4 has been described as both a negative regulator of CRE-dependent transcription (2, 32) and a positive regulatorof transcription (5, 40, 66). One possibility for the differenceis that forskolin, which activates the PKA pathway, was used inone experiment in which repression was observed (32) but wasnot used in experiments in which activation was observed. Anotherpossibility is that different amounts of ATF4 were used in theexperiments. As suggested previously (40), at high concentrations,ATF4 may repress transcription due to squelching. Alternatively,the difference in activity may be due to dimerization of ATF4with other bZip proteins (20, 21, 57, 66). In our experiments,we showed that the inhibitory effect of ATF4 on CRE-dependenttranscription of the somatostatin promoter is modulated by SCF^TrCP-mediated ATF4 degradation. It remains to be demonstrated whetherthe other ATF4 transcriptional activities are also regulated by $beta$ TrCP.

Our observation that $beta$ TrCP is a nuclear protein differs from the previously reported localization of $beta$ TrCP by Winston et.al. (67) as being largely cytoplasmic. However, our result isin agreement with the nuclear localization found by Hatakeyamaet al. (reference 24 and personal communication). Such descrepancywith the results reported by Winston et al. (67) remains tobe further evaluated. One possibility is that the cytoplasmiclocalization of $beta$ TrCP observed by Winston et al. could correspondto that of the $beta$ TrCP2 homolog of $beta$ TrCP (also called KIAA0696 [18,26]). Indeed, we also found that $beta$ TrCP2, in addition to thenucleus, can be seen in the cytoplasm (unpublished results). Thenuclear localization of $beta$ TrCP and its involvement in controllingthe degradation of ATF4 illustrates the role that E3 ubiquitinligases of the SCF type could play in the nucleus in mammaliancells. The question then arises whether the degradation of SCF^TrCP substrates takes place in the nucleus rather than in the cytoplasm,as it is currently thought for I $kappa$ B $alpha$ and $beta$ -catenin, two substratesof $beta$ TrCP (31, 53). This hypothesis is consistent with recentresults which reveal that tumor necrosis factor alpha can inducethe degradation of nuclear I $kappa$ B $alpha$ (28, 55). Interestingly, othercomponents of the ubiquitination machinery have also been seenin the nucleus. These include the E2 ubiquitin-conjugating enzymeUBC9, which has been implicated in the proteolytic control ofATF2 (16), Cdc34, the E2 enzyme typically recruited by SCF complexes(41), Skp1 (17), Cullin1 (41), and the F-box protein Skp2(41). Because several similar forms of $beta$ TrCP have been identified(26, 43), one can speculate that these isoforms could be differentiallylocalized in cells, directing degradation of their substratesin different cellular compartments. For instance, we cannot atthis point rule out the hypothesis that ATF4 is transported tothe cytoplasm for its ubiquitination anddegradation.

Interaction of ATF4 with $beta$ TrCP relies on motif DSGXXXS, similar but not identical to that found in the other substrates of $beta$ TrCP (HIV-1 Vpu, I $kappa$ B $alpha$ , and $beta$ -catenin), which is DSGXXXS (23,36, 39, 42, 43, 62, 67, 68). It is interesting tonote that the first serine residue of this motif seems to playan essential role in this interaction while the second serineresidue, which is important in the case of Vpu and $beta$ -catenin (unpublishedresults), is not required for the interaction of ATF4 with $beta$ TrCP.The recent discovery of the role of $beta$ TrCP in the processing ofNF- $kappa$ B p105 supports the idea that the DSGXXS motif is not theonly determinant of interaction with $beta$ TrCP (50). The $beta$ TrCP recognitionmotif in p105 is very different from the DSGXXS motif althoughit contains three phosphorylation sites important for interaction.However, p105 is a special case in the way it undergoes limitedprocessing rather than complete destruction by the proteasome.Further work will be needed to determine which sequence requirementsin addition to the DSGXXS motif are playing a role in interactionwith $beta$ TrCP.

One crucial step which triggers the interaction of substrates with $beta$ TrCP is their phosphorylation by a distinct protein kinase,which thus confers specificity on the ubiquitination process. $beta$ -catenin, I $kappa$ B $alpha$ , and Vpu are phosphorylated on DSGXXS by GSK3/axin(53), IKK (31), and casein kinase II (58), respectively.To understand more of how ATF4 is regulated, it is thus crucialto identify the kinase that phosphorylates ATF4 on its DSGXXXSmotif. It could be that ATF4 is phosphorylated by the nuclearprotein kinase Zip-kinase/Dlk, recently identified as an ATF4binding protein, favoring ATF4 interaction with $beta$ TrCP (33, 34).

	ACKNOWLEDGMENTS

We thank F. Bantignies for the CRE-luciferase plasmid, M. Kroll for the $beta$ TrCP $Delta$ W1 and $beta$ TrCP $Delta$ W2-7 expression vectors, J. Hsuand P. Jackson for the pAS2Fbw2 expression vector, I. Bouchaertfor help in confocal microscopy analysis, Franck Letourneur forDNA sequencing, J. Bertherat, U. Hazan, Anne Gatignol and P. Chaffeyfor helpful discussions, and Owen Parkes for editing themanuscript.

C. Berlioz-Torrent is supported by FRM (Foundation pour la Recherche Medicale). This work was supported by ANRS (Agence Nationalepour la Recherche contre le SIDA), Sidaction, ARP, Associationpour la Recherche sur le Cancer, and Ligue Nationale contre leCancer.

	FOOTNOTES

^* Corresponding author. Mailing address: INSERM Unite 529, ICGM, 24 rue de Faubourg Saint Jacques, 75014 Paris, France. Phone:33 1 44 41 25 65. Fax: 33 1 44 41 23 99. E-mail: benarous{at}cochin.inserm.fr.

REFERENCES

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References

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1.	Bai, C., P. Sen, K. Hofmann, L. Ma, M. Goebl, J. W. Harper, and S. J. Elledge. 1996. SKP1 connects cell cycle regulators to the ubiquitin proteolysis machinery through a novel motif, the F-box. Cell 86:263-274[CrossRef][Medline].
2.	Bartsch, D., M. Ghirardi, P. A. Skehel, K. A. Karl, S. P. Herder, M. Chen, C. H. Bailey, and E. R. Kandel. 1995. Aplysia CREB2 represses long-term facilitation: relief of repression converts transient facilitation into long-term functional and structural change. Cell 83:979-992[CrossRef][Medline].
3.	Benichou, S., M. Bomsel, M. Bodeus, H. Durand, M. Doute, F. Letourneur, J. Camonis, and R. Benarous. 1994. Physical interaction of the HIV-1 Nef protein with beta-COP, a component of non-clathrin-coated vesicles essential for membrane traffic. J. Biol. Chem. 269:30073-30076[Abstract/Free Full Text].
4.	Brindle, P. K., and M. R. Montminy. 1992. The CREB family of transcription activators. Curr. Opin. Genet. Dev. 2:199-204[CrossRef][Medline].
5.	Butscher, W. G., C. Powers, M. Olive, C. Vinson, and K. Gardner. 1998. Coordinate transactivation of the interleukin-2 CD28 response element by c-Rel and ATF-1/CREB2. J. Biol. Chem. 273:552-560[Abstract/Free Full Text].
6.	Carrano, A. C., E. Eytan, A. Hershko, and M. Pagano. 1999. SKP2 is required for ubiquitin-mediated degradation of the CDK inhibitor p27. Nat. Cell Biol. 1:193-199[CrossRef][Medline].
7.	Charrasse, S., I. Carena, V. Brondani, K. H. Klempnauer, and S. Ferrari. 2000. Degradation of B-Myb by ubiquitin-mediated proteolysis: involvement of the Cdc34-SCF(p45Skp2) pathway. Oncogene 19:2986-2995[CrossRef][Medline].
8.	Chevray, P. M., and D. Nathans. 1992. Protein interaction cloning in yeast: identification of mammalian proteins that react with the leucine zipper of Jun. Proc. Natl. Acad. Sci. USA 89:5789-5793[Abstract/Free Full Text].
9.	Chiaur, D. S., S. Murthy, C. Cenciarelli, W. Parks, M. Loda, G. Demetrick, and M. Pagano. 2000. Five human genes encoding F-box proteins: chromosome mapping and analysis in human tumors. Cytogenet. Cell Genet. 88:255-258[CrossRef][Medline].
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ATF4 Degradation Relies on a Phosphorylation-Dependent Interaction with the SCFTrCP Ubiquitin Ligase

ATF4 Degradation Relies on a Phosphorylation-Dependent Interaction with the SCF^TrCP Ubiquitin Ligase