Multiple 40-kDa Heat-Shock Protein Chaperones Function in Tom70-dependent Mitochondrial Import

Melanie K. Bhangoo, Stefan Tzankov, Anna C.Y. Fan, Kurt Dejgaard, David Y. Thomas, and Jason C. Young

Department of Biochemistry, McGill University, Montreal, QC, H3G 1Y6, Canada

Submitted January 31, 2007; Accepted June 19, 2007
Monitoring Editor: Jeffrey Brodsky

ABSTRACT

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Mitochondrial preproteins that are imported via the translocaseof the mitochondrial outer membrane (Tom)70 receptor are complexedwith cytosolic chaperones before targeting to the mitochondrialouter membrane. The adenine nucleotide transporter (ANT) followsthis pathway, and its purified mature form is identical to thepreprotein. Purified ANT was reconstituted with chaperones inreticulocyte lysate, and bound proteins were identified by massspectrometry. In addition to 70-kDa heat-shock cognate protein(Hsc70) and 90-kDa heat-shock protein (Hsp90), a specific subsetof cochaperones were found, but no mitochondria-specific targetingfactors were found. Interestingly, three different Hsp40-relatedJ-domain proteins were identified: DJA1, DJA2, and DJA4. TheDJAs bound preproteins to different extents through their C-terminalregions. DJA dominant-negative mutants lacking the N-terminalJ-domains impaired mitochondrial import. The mutants blockedthe binding of Hsc70 to preprotein, but with varying efficiency.The DJAs also showed significant differences in activation ofthe Hsc70 ATPase and Hsc70-dependent protein refolding. In HeLacells, the DJAs increased new protein folding and mitochondrialimport, although to different extents. No single DJA was superiorto the others in all aspects, but each had a profile of partialspecialization. The Hsp90 cochaperones p23 and Aha1 also regulatedHsp90–preprotein interactions. We suggest that multiplecochaperones with similar yet partially specialized propertiescooperate in optimal chaperone–preprotein complexes.

INTRODUCTION

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

The majority of mitochondrial proteins are encoded in the nucleus,translated on cytosolic ribosomes, and subsequently importedinto mitochondria (Reichert and Neupert, 2004). The translocaseof the mitochondrial outer membrane (TOM) is responsible forpolypeptide translocation across the outer membrane; and insidethe organelle, various mechanisms sort these polypeptides totheir appropriate compartment—matrix, inner membrane orintermembrane space. The TOM complex contains integral membraneimport receptors, Tom20 and Tom70, which mediate targeting ofmitochondrial preproteins, and a general import pore that providesan aqueous channel for translocation. Tom20 is thought to beresponsible for the import of preproteins bearing classicalmatrix-directed N-terminal signal sequences, or leader peptides.Tom70, the alternate receptor, is thought to mediate the importof preproteins that contain targeting information within theirmature sequences (Koehler, 2004; Rehling et al., 2004). Althoughmuch of our knowledge of import derives from work in Saccharomycescerevisiae and Neurospora crassa, the biological functions ofthe human Tom70 and Tom20 receptors seem to be largely conserved(Iwahashi et al., 1997; Schleiff et al., 1997; Yano et al.,1997; Suzuki et al., 2002).

The Tom70 receptor seems to be most critical for the importof particularly hydrophobic preproteins, such as members ofthe inner membrane metabolite carrier family (Sollner et al.,1990; de Marcos-Lousa et al., 2006). Before import, these preproteinstypically depend on cytosolic chaperones to maintain their solubility.The ATP-dependent chaperones 70-kDa heat-shock cognate protein(Hsc70) and 90-kDa heat-shock protein (Hsp90) have key rolesin this mechanism (Young et al., 2004). In addition to maintainingthe solubility of the bound preprotein, Hsc70 and Hsp90 canboth dock onto to a specific binding site in Tom70, an essentialfirst step in preprotein targeting. The chaperone docking sitelies in the central region of Tom70 next to the single N-terminaltransmembrane domain (Young et al., 2003). At this stage, preproteinis thought to contact Tom70 directly in a C-terminal regionseparate from the chaperone docking site (Brix et al., 2000;Wu and Sha, 2006). ATP-dependent cycling by Hsp90 and most probablyHsc70 then assists the translocation of preprotein via the outermembrane TOM machinery (Fan et al., 2006).

In their other cellular functions, Hsc70 and Hsp90 interactwith a wide range of cochaperone proteins, which connect additionalspecific chaperoning functions or biochemical activities tochaperone complexes. In some cases, the type of substrate polypeptidebound by a chaperone complex determines which specific cochaperoneis recruited to Hsp90. For example, the immunophilin FKBP52usually associates with, and assists in the maturation of, steroidhormone receptors, whereas Cdc37 has a comparable role for kinases(Pratt and Toft, 2003). Such specificity is not absolute: bothCdc37 and the immunophilin FKBP8 have been found in chaperonecomplexes with a folding-deficient mutant of the cystic fibrosistransmembrane conductance regulator (CFTR) chloride channel(Wang et al., 2006). Many cochaperones contain functionallyconserved chaperone–interaction domains. Some interactionswith Hsp90 and Hsc70 are mediated by structurally conservedtetratricopeptide repeat (TPR) clamp domains that recognizethe C-terminal motifs of the chaperones. The TPR-domains inFKBP52 and the related cyclophilin Cyp40 connect to Hsp90. Thosein the cochaperone Hop recognize Hsc70 and Hsp90 separately,allowing Hsc70–substrate complexes to recruit Hsp90 (Prattand Toft, 2003). Also, a conserved TPR clamp domain in Tom70forms its chaperone docking site (Young et al., 2003). J-domains,found in various cochaperones including the Hsp40-related proteins,stimulate ATP hydrolysis and substrate binding by Hsc70. J-domainsdo not form stable contacts with Hsc70, but they are essentialfor all known functions of Hsc70 (Walsh et al., 2004; Qiu etal., 2006). Several nucleotide exchange factors including Bag-1transiently promote ATP rebinding and Hsc70 dissociation fromsubstrate (Mayer and Bukau, 2005). Cochaperones that do notbelong to these structural families include Cdc37, p23, andAha1. p23 stabilizes the ATP- and substrate-binding state ofHsp90, whereas the recently discovered Aha1 stimulates the Hsp90ATPase (Panaretou et al., 2002; Sullivan et al., 2002; Lotzet al., 2003; Morishima et al., 2003; Pearl and Prodromou, 2006).

It is not known what proteins in addition to Hsc70 and Hsp90are complexed with Tom70-dependent preproteins before import,or what proteins are involved in complex formation. It seemscertain that cochaperone proteins participate in these complexes.The preproteins are not related to structural families of proteinsknown to prefer specific cochaperones, and the involvement ofmany cochaperones cannot be predicted. The preproteins seemto be in high-molecular-weight complexes of $~$ 600 kDa, similarto other Hsp90-bound complexes, but with some heterogeneity(Young et al., 2003; Fan et al., 2006). The identity and functionof bound cochaperones would lead to significant insight. First,are the cochaperones present specifically bound? Second, arethere components unique to chaperone–preprotein complexes,and what role might they have? Third, do the cochaperones boundhave implications for the function of Hsc70 and Hsp90?

To address these questions, we reconstituted chaperone complexesin reticulocyte lysate (RL) as a model cytosol. This methodwas used to originally identify most of the cochaperones involvedin steroid receptor and kinase maturation (Pratt and Toft, 2003).RL is uniquely suited for such experiments. Although it containsessentially no organellar contamination, it is the basis forall experiments reconstituting cell-free mitochondrial import;therefore, it contains all necessary factors. A mitochondrialpreprotein, the adenine nucleotide transporter (ANT) is uniquelypurifiable in biochemical amounts (Pebay-Peyroula et al., 2003),and it was used as the starting point for the reconstitutionof complexes.

MATERIALS AND METHODS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Chemicals and Reagents
Unless stated otherwise, all chemical reagents were from SigmaDiagnostics Canada or BioShop Canada (Mississauga, ON, Canada).Restriction enzymes and other recombinant DNA reagents werefrom New England Biolabs (Ipswich, MA), Invitrogen (Carlsbad,CA), and Stratagene (San Diego, CA). Geldanamycin (GA) was fromLC Laboratories (Boston, MA). Untreated rabbit RL was from GreenHectares (Oregon, WI). Antibodies against Hsp90, Hsc70, Hop,FKBP52, and Hsp40 were from Assay Designs (Ann Arbor, MI); thoseagainst Cdc37, Cyp40, and p23 were from Affinity BioReagents(Golden, CO); that against DJA1 was from Labvision/NeoMarkers(Fremont, CA); and that against luciferase was from Sigma DiagnosticsCanada. The antibody against Tpr2 was a gift from Dr. W.M.J.Obermann (Houston, TX); those against DJA2 and DJA4 were giftsfrom Dr. M. Mori (Kumamoto, Japan), and that against Hsp60 wasa gift from Dr. F. U. Hartl (Martinsried, Germany). Additionalantibodies specific for DJA1, DJA2, and DJA4 were raised inrabbits against the synthetic peptides LVDFDPNQER, PEVPNIIGET,and PNEQNWRQHR, respectively, and they were confirmed with immunoblotsagainst the purified DJA proteins, and HeLa cells were transfectedwith each antibody. Antibodies against the myc (9E10) and hemagglutinin(HA.11) epitope tags were from Covance/BAbCO (Richmond, CA).

Plasmids
The sequences encoding bovine phosphate carrier (PiC) and N.crassa Rieske iron-sulfur protein (ISP) were in pGEM-3 (Promega,Madison, WI) (Sollner et al., 1989; Zara et al., 1992). Thesequence encoding murine ANT2 (NM_007451 [GenBank] ) was amplified by polymerasechain reaction (PCR) from a cDNA library and inserted into pGEM-11Z(Promega) (Fan et al., 2006). The sequences encoding nontaggedhuman Hsp90 ${alpha}$ and rat Hsc70 were in pET15b and pET11a (Novagen,San Diego, CA), respectively, and the sequences encoding residues566-732 of human Hsp90 ${alpha}$ (C-90) and residues 151-263 of humanBag-1 (C-Bag) were in pProExHTa (Clontech, Mountain View, CA)(Young and Hartl, 2000; Sondermann et al., 2001; Young et al.,2003). Recombinant nontagged human p23 was in pET28 (Novagen)(Young and Hartl, 2000), and the sequence encoding human DJA1(NM_001539 [GenBank] ) also in pET28a was a gift from C.H.I. Ramos (LaboratórioNacional de Luz Síncrotron, Campinas SP, Brazil) (Borgeset al., 2005). The sequences encoding human Hsc70 (NM_006597 [GenBank] ),DJA2 (NM_005880), and DJA4 (NM_018602) as well as the sequencesencoding amino acids 98-397 of human DJA1 (C-A1), amino acids100-412 of human DJA2 (C-A2), and amino acids 99-397 of humanDJA4 (C-A4) were amplified from a cDNA library and insertedinto pProExHTa (Clontech). Sequences of DJA1, DJA2, and DJA4were inserted into pGEM-11Z (Promega) without tags, and intopcDNA3.1 myc-His C (Invitrogen). Human Aha1 in pProExHTa wasa gift from W.M.J. Obermann (Houston, TX) (Lotz et al., 2003).The sequence encoding firefly luciferase was amplified by PCRfrom pGL3 (Promega) and inserted into pcDNA3.1 (Invitrogen)without a tag; the pSV40- $beta$ -galactosidase vector was from Promega.The vectors pCAGGS-PiC-3HA, pGR- ${Delta}$ LBD, and pMTV-luciferase (glucocorticoidresponsive element [GRE]-luciferase) were as reported previously(Hollenberg et al., 1987; Hollenberg and Evans, 1988; Brychzyet al., 2003; Young et al., 2003).

Protein Purification
The expression vectors for full-length His-tagged DJA1, DJA2,and DJA4 were grown in Rosetta 2 Escherichia coli cells (Novagen),and protein expression was induced with 1 mM isopropyl- $beta$ -D-thiogalactopyranosideat 30°C for 1 h, at 37°C for 30 min, and at 30°Cfor 3 h, respectively. The cells were harvested and resuspendedin buffer containing 750 mM NaCl, 60 mM imidazole and 20 mMKH₂PO₄, pH 7.5, with Complete protease inhibitors (Roche Diagnostics,Indianapolis, IN). Cells were lysed by cavitation in a Frenchpress, and the cell debris was removed by centrifugation. Thesupernatant was loaded onto a 5-ml nickel-Sepharose high-performancecolumn (GE Healthcare, Little Chalfont, Buckinghamshire, UnitedKingdom), and proteins were eluted with buffer containing 1M imidazole, 500 mM NaCl, and 20 mM KH₂PO₄, pH 7.5. Peak fractionswere loaded on a Superdex 200 Hi-Load 16/60 column (GE Healthcare)and eluted with buffer HS (500 mM NaCl, 20 mM HEPES-KOH, pH7.5, and 5 mM MgOAc₂). Nonaggregated peak fractions were collected,and the yield was determined by absorbance at 280 nm. The DJAproteins lacking the N-terminal J-domain, C-A1, C-A2, and C-A4,were purified identically to the full-length proteins. Hsc70was expressed for 4 h at 30°C and purified on nickel-Sepharosehigh-performance equlibrated in buffer containing 500 mM NaCl,20 mM imidazole, and 20 mM KH₂PO₄, pH 7.5, and eluted in buffercontaining 300 mM imidazole and 20 mM KH₂PO₄, pH 7.5. Hsc70was further purified by ion exchange on a Mono Q 5/50 GL columnand gel filtration on a Superdex 200 Hi-Load 16/60 column (GEHealthcare) equilibrated in buffer CG (100 mM KOAc, 20 mM HEPES-KOH,pH 7.5, and 5 mM MgOAc₂). Bovine ANT was purified as describedpreviously (Klingenberg et al., 1979; Pebay-Peyroula et al.,2003), with the following modifications. Mitochondria were preparedfrom bovine heart and treated with atractyloside, and then theywere solubilized in buffer AB (500 mM NaCl, 10 mM HEPES-KOH,pH 7.5, and 1 mM EDTA) containing 2% Triton X-100. Insolublematerial was removed by ultracentrifugation at 140,000 x g for30 min, and the supernatant was loaded onto a hydroxyapatiteHTP-gel column (Bio-Rad, Hercules, CA) equilibrated in bufferAB containing 0.1% Triton X-100, and peak flow-through fractionscontaining ANT were collected. Recombinant C-90, C-Bag, Aha1,p23, and firefly luciferase were purified as described previously(Young and Hartl, 2000; Brychzy et al., 2003; Lotz et al., 2003;Young et al., 2003).

Chaperone–ANT Complexes
RL was desalted into buffer CG on NAP-10 columns or a Hi-Prep26/10 fast desalting column (GE Healthcare). Purified ANT waschemically biotinylated on cysteine side chains with maleimidePEO₂-biotin (Pierce Chemical, Rockford, IL) for 3 h at roomtemperature, and excess biotin was removed with NAP-10 columnsequilibrated in buffer MT (100 mM NaCl, 10 mM HEPES-KOH, 1 mMEDTA and 0.1% Triton X-100). The biotinylated ANT (ANT-B) wasbound to immobilized streptavidin-agarose (Pierce Chemical)for 1 h. The ANT-B was washed twice with buffer CG to removestabilizing detergent, and it was reconstituted by incubationwith 50% RL in buffer CG, supplemented with 2 mM ATP. After15 min at room temperature, the reactions were terminated with0.1 U/µl apyrase, grade VII. The reconstituted ANT-B complexeswere reisolated, and the protein components were eluted withLaemmli loading buffer. After separation by Laemmli SDS-polyacrylamidegel electrophoresis (PAGE) and total protein staining with CoomassieBlue, bands were excised and subjected to in-gel tryptic digestionas described previously (Shevchenko et al., 1996). Peptideswere analyzed by C18 reverse phase separation followed by iontrap liquid chromatography-tandem mass spectrometry on a DaltonicsEsquire HCT+ instrument (Bruker, Newark, DE). Spectra were formattedand searched against mammalian sequences in the National Centerfor Biotechnology Information database by using the Mascot searchengine (Matrix Science, Boston, MA). Data were validated manually.

For gel filtration analysis, ANT-B was bound to monomeric avidinagarose (Pierce Chemical) for 1 h, washed with buffer CG, andeluted with 1% SDS and 8 M urea. The eluted ANT-B was diluted1:400 into 50% RL in buffer CG, supplemented with 2 mM ATP.After 15 min at room temperature, the reaction was terminatedwith apyrase as described above and loaded onto a Superose 610/300 GL column (GE Healthcare) equilibrated in buffer CG.Fractions were collected and separated by SDS-PAGE, transferredonto nitrocellulose, detected with horseradish peroxidase-conjugatedstreptavidin (Pierce Chemical), and visualized on chemiluminescent-sensitivefilm. In control reactions, cell-free translation reactionsof ANT were performed using the TNT coupled RL system with SP6polymerase (Promega), and they were labeled with [³⁵S]methionine(GE Healthcare). Reactions were diluted 1:4 into buffer CG andanalyzed by gel filtration as described above. Fractions wereanalyzed by SDS-PAGE and autoradiography. Phosphorimager quantitationwas performed with a FujiFilm BAS-1800II analyzer (FujiFilm,Stamford, CT) and ImageGauge software (Fuji, Tokyo, Japan).

Mitochondrial Import Assays
Rat liver mitochondria were isolated and import reactions wereperformed as described previously (Lingelbach et al., 1986;Young et al., 2003; Fan et al., 2006). For cleaner mitochondrialpreparations by gradient centrifugation (Vijayasarathy et al.,1989), mitochondria were layered over 12-ml steps of 42, 45,and 60% sucrose in 10 mM HEPES-KOH, pH 7.5, and 1 mM EDTA, inSW28 tubes (Beckman Coulter, Fullerton, CA). After centrifugationat 100,000 x g for 1 h, mitochondria were harvested from the45–60% interface, diluted in the same buffer without sucrose,collected by centrifugation, and resuspended at 10 mg/ml inbuffer MC (250 mM sucrose, 80 mM KOAc, 20 mM HEPES-KOH, pH 7.5,and 5 mM MgOAc₂) supplemented with 10 mM Na-succinate, 1 mMdithiothreitol, 2 mM ATP, and 0.4 mM ADP. Cell-free translationsof the preproteins were performed with the TNT-coupled RL systemwith SP6 or T7 polymerase supplemented with [³⁵S]methionine,and then reactions were terminated with 1 mM methionine andadjusted to 250 mM sucrose. Typical import reactions contained25% reticulocyte lysate and 5 mg/ml mitochondria at 30°Cfor 30 min, and negative control reactions were inhibited with1 µM valinomycin. Mitochondria were reisolated and digestedwith 250 µg/ml proteinase K (PK) at 4°C for 10 min,followed by 1 mM phenylmethylsulfonyl fluoride to stop the digestion.Undigested and digested samples were analyzed by SDS-PAGE andautoradiography or phosphorimager analysis.

Inhibition of import by C-90, C-Bag, and geldanamycin (GA) wasassayed as reported previously (Young et al., 2003; Fan et al.,2006). Purified C-90 and C-Bag were added to reactions at afinal concentration of 20 and 5 µM, respectively. Then,18 µM GA or the equivalent volume of vehicle control dimethylsulfoxide (1%) was added to the translation reactions, and excessGA was removed before import reactions by using MicroBioSpin6 columns (Bio-Rad) pre-equilibrated in buffer MC containing0.4 mM EGTA, centrifuged at 16°C with 2 mM ATP added tothe collection tube. Inhibition of import by C-A1, C-A2, andC-A4 was assayed as for C-90, with each mutant added at 20 µM,and reactions adjusted to a final concentration of 90 mM NaClin buffer MC to maintain solubility of the mutants. Controlreactions adjusted to 90 mM NaCl with no additional proteinshowed that the added ionic strength had no significant effecton import.

Purified ANT was radiolabeled with Na-[¹²⁵I] (GE Healthcare)by using Iodo-Beads (Pierce Chemical) according to the manufacturer'sinstructions. ¹²⁵I-ANT was desalted using a NAP-10 column inbuffer MT to remove excess radiolabel, concentrated by trichloroaceticacid precipitation, and resuspended in 0.1% SDS. Import wasinitiated by 1:100 dilution into reactions containing 4 mg/mlmitochondria and 40% RL in buffer MC, supplemented with 2 mMsuccinate, 0.2 mM dithiothreitol, 2 mM ATP, and 0.4 mM EGTA.To assay import of ANT-B, the biotinylated protein was recoveredwith monomeric avidin agarose as described for gel filtrationanalysis. The eluted ANT-B was diluted 1:10 into distilled waterand then a further 1:100 dilution into reactions containingRL and mitochondria as described for ¹²⁵I-ANT. Control reactionsusing cell-free translated ANT showed that the final concentrationof 0.001% SDS did not interfere with mitochondrial import inany way.

Coprecipitation Experiments
To assay binding of preproteins to the DJA proteins, an assayestablished for Tom70 (Young et al., 2003; Fan et al., 2006)was adapted. DJA1, DJA2, and DJA4 or the truncation mutantsC-A1, C-A2, and C-A4 were prebound on nickel-Sepharose in bufferHS for 30 min at 4°C. Cell-free translations of ANT andPiC were performed as described above with SP6 polymerase, diluted1:20 into buffer CG containing 20 mM imidazole, 0.1% TritonX-100, and 2 mg/ml ovalbumin, and added to the immobilized DJAproteins. The final reactions contained 5 µM wild-typeDJA protein or 10 µM truncation mutant, and 5% translationmixture. After 5 min at room temperature, the binding reactionswere terminated by the addition of 0.1 U/µl apyrase. Theprotein complexes were recovered at 4°C for 30 min, andthen they were washed with buffer CG containing 20 mM imidazoleand 0.1% Triton X-100. Protein complexes were eluted with Laemmliloading buffer, and they were analyzed by SDS-PAGE and autoradiographyor phosphorimager quantitation. To form DJA heterocomplexes,ANT-B was diluted into 50% RL as described for the gel filtrationanalysis, but binding reactions were supplemented 1:20 withcell-free translations of each nontagged DJA. The reactionswere then coprecipitated with different His-tagged DJAs as describedabove.

To assay formation and dissociation of Hsc70, Hsp90, and DJAcomplexes with ANT, methods established for the ligand bindingdomain of the glucocorticoid receptor (Young and Hartl, 2000;Sondermann et al., 2001; Brychzy et al., 2003) were adapted.To assay binding, ANT-B was prebound to streptavidin-agaroseand washed with buffer CG as described above. Cell-free translationreactions of Hsc70, Hsp90, or each DJA were performed as describedabove with T7 or SP6 polymerase, diluted 1:10 or 1:14 into 40%RL in buffer CG containing 2 mM ATP, and added to the immobilizedANT-B. Aliquots were taken at the indicated time points, andcomplexes were reisolated and washed with buffer CG containing0.1% Triton X-100. Protein complexes were eluted and analyzedas described above. Where indicated, binding reactions wereperformed in the presence of 20 µM C-A1, C-A2, C-A4 orC90, or 4 µM Aha1. To assay dissociation of complexes,cell-free translation reactions of Hsc70 and Hsp90 were complexedwith ANT-B as described above for 15 min at room temperature,and complexes were reisolated and washed with buffer CG. Dissociationreactions consisting of buffer CG with or without 2 mM ATP,4 µM Aha1, 5 µM C-Bag, 5 µM p23, or 20 µMC-90 were incubated with the complexes for 10 min at room temperature.Released and remaining immobilized fractions were separatedand analyzed by SDS-PAGE and autoradiography or phosphorimagerquantitation.

Hsc70 Activity
ATPase activities were measured as described previously (Youngand Hartl, 2000; Brychzy et al., 2003). Briefly, reactions contained4 µM Hsc70, 20 µM C-Bag, and the indicated concentrationof each DJA protein, in buffer CG supplemented with 78 mM NaClto maintain solubility of the DJA proteins, 4 mM ATP, and 5µCi/ml ${alpha}$ -[³²P]ATP. Reactions were assembled on ice andinitiated by incubation at 30°C. At various times, aliquotswere removed and terminated by adjusting to 25 mM EDTA. Sampleswere separated by thin layer chromatography (TLC) on polyethylene-iminecellulose (Mallinckrodt Baker, St. Louis, MO) developed in 0.5M LiCl and 0.5 M formic acid. ADP produced was quantified byphosphorimager analysis and linear rates calculated.

To assay refolding of firefly luciferase, the protein was denaturedin buffer CG containing 6 M guanidinium-HCl and 1 mM dithiothreitolfor 15 min at room temperature. Refolding reactions were preassembledon ice, containing 4 µM Hsc70, 4 µM DJA protein,and 0.5 µM C-Bag, either with 1 mM ATP or treated with0.1 U/µl apyrase, in buffer CG supplemented with 39 mMNaCl, and warmed to 30°C immediately before use. Luciferasewas diluted 1:100 into reactions to a final concentration of5.4 nM and incubated at 30°C. Control reactions contained50% RL in buffer CG supplemented with 39 mM NaCl and 1 mM ATP.At various times, aliquots were diluted 1:45 into luciferaseassay reagent (Promega), and luciferase activity was measuredin a Lumat LB 9507 luminometer (Berthold Technologies, Bad Wildbad,Germany).

Cell Culture
HeLa cells were maintained in DMEM containing 4.5 g/l glucose,36 mg/l pyruvate, 2 mM glutamine, and 10% fetal bovine serum(Invitrogen). Cells were transfected using Lipofectamine andPLUS Reagent (Invitrogen) in six-well plates with 4 µgof myc-His-tagged DJA plasmid or vector alone, 0.5–1.5µg of pSV40- $beta$ -galactosidase, and 0.5 µg of eitherpcDNA3.1-luciferase, or pCAGGS-PiC-3HA, or pMTV-luciferase with0.5 µg of pGR- ${Delta}$ LBD. Two days after transfection, cellswere harvested and lysed by freeze-thaw in $beta$ -galactosidase Reporterlysis buffer (Promega). Lysates were cleared by centrifugationat 20,000 x g for 10 min and assayed for $beta$ -galactosidase andluciferase activities with the appropriate kits (Promega). Equalamounts of lysate were analyzed by immunoblots. The immunoblotswere quantified with a FujiFilm LAS-1000 CH luminescent imageanalyzer and the ImageGauge software.

RESULTS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Mitochondrial Import of ANT
Mammalian ANT is an inner membrane metabolite carrier protein,and it was expected to follow the chaperone–Tom70 mitochondrialimport pathway (de Marcos-Lousa et al., 2006), as has been establishedfor PiC. Like many such carriers, ANT lacks a signal sequence,and it contains targeting information within its mature sequence,consistent with Tom70 dependence. ANT is composed almost entirelyof six transmembrane helices, and its hydrophobicity suggestedreliance on chaperones. Our previous work also showed that theHsp90 inhibitor novobiocin blocked import of ANT, consistentwith strong chaperone involvement (Fan et al., 2006). However,the relative importance of Hsc70 and Hsp90 to ANT import remainedunknown, and this was addressed using previously establishedassays.

Both Hsc70 and Hsp90 dock onto a juxtamembrane TPR clamp domainof Tom70, a key step in the targeting of chaperone-bound preproteins.The C-terminal 16-kDa fragment of Hsp90 (C-90), containing theTPR clamp domain recognition motif, competes with Hsc70 andHsp90 for binding to Tom70, thereby blocking Tom70-dependentimport (Young et al., 2003). The import of ANT was thereforetested in the presence of excess C-90 competitor. RadiolabeledANT was generated by cell-free translation in RL, and it wasimported into isolated rat liver mitochondria. ANT is not proteolyticallyprocessed upon import, so the extent of import was assessedby resistance to externally added PK. Imported ANT was resistantto digestion (Figure 1A, lanes 2 and 6), but when import wasabolished by valinomycin disruption of the inner membrane potential,PK resistance was reduced to a low background level (Figure 1A,lanes 3 and 7). Addition of the C-90 competitor also reducedthe amount of imported ANT, although not to the valinomycinbackground, whereas the addition of the control protein serumalbumin had no effect (Figure 1A, lanes 8 and 9). Quantitationrevealed that C-90 impaired ANT import to below 40% of controlreactions (Figure 1A). This effect was similar to that observedfor Tom70-dependent PiC (Young et al., 2003), whereas importof the Tom20-dependent Rieske ISP was only marginally affected.ANT thus seems to follow the Tom70 import route.

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Figure 1. Mitochondrial import of ANT. (A) ANT (input, lane 1) was radiolabeled by cell-free translation and imported into isolated rat liver mitochondria (+ mito, lanes 2–9). As a negative control, import was abolished with valinomycin (val, lanes 3 and 7). The true extent of import was determined by resistance to added PK (lanes 6–9). Import was assayed in the presence of 20 µM C-90 fragment, a competitor of chaperone-Tom70 interactions (C-90, lanes 4 and 8), or the same mass concentration of bovine serum albumin as a negative control (BSA, lanes 5 and 9). Reactions were analyzed by SDS-PAGE and autoradiography. Right, phosphorimager quantitation of import of ANT, PiC, and ISP are shown relative to control reactions. Standard deviations here, and in all figures, were determined from at least three independent experiments. (B) Import of ANT, PiC, and ISP was assayed upon inhibition with 5 µM C-Bag, treatment with 18 µM GA, or combined inhibition with both reagents, and the quantitation relative to control reactions is shown.

The individual contributions of Hsc70 and Hsp90 to ANT importwere tested. Hsc70 can be dysregulated by an excess of its nucleotideexchange factor, the C-terminal domain of Bag-1 (C-Bag), whichpromotes the release of polypeptide substrate from Hsc70 (Sondermannet al., 2001

; Mayer and Bukau, 2005

). C-Bag inhibited the importof ANT to $~$ 50% of control reactions (Figure 1B), and as establishedpreviously (Young et al., 2003

), PiC import was inhibited to $~$ 60%. The specific Hsp90 inhibitor GA (Pearl and Prodromou, 2006

)was used to block Hsp90 function during import, and it partiallydiminished ANT import to $~$ 72% of the control (Figure 1B). Asreported previously (Young et al., 2003

), GA inhibition of PiCimport was also partial, to $~$ 60% of the control (Figure 1B).Most importantly, combined inhibition of Hsc70 and Hsp90 byC-Bag and GA further reduced ANT import to $~$ 40% of the control,similar to the established level of $~$ 30% observed for PiC. Incontrast, combined C-Bag and GA treatment had no inhibitoryeffect on ISP import (Figure 1B). In PiC, the combined effectof Hsc70 and Hsp90 inhibition indicated that the chaperonessubstitute for each other when one chaperone is inhibited (Younget al., 2003

). For ANT, combined chaperone inhibition had aneffect closer to that of Hsc70 inhibition alone, suggestingthat ANT is more dependent on Hsc70 relative to Hsp90 for itsimport. Combined chaperone inhibition blocked the import ofANT to the same level as C-90 competition for Tom70 (Figure 1,A and B), as expected from the chaperone docking mechanism.

Reconstitution of Chaperone–ANT Complexes
ANT can be purified in biochemical amounts from bovine heart(Pebay-Peyroula et al., 2003). Mass spectrometry analysis determinedthat the purified protein was identical in mass to that predictedby the cDNA sequence (data not shown), indicating that matureANT should be reverted to its preprotein state by denaturation.Dilution of denatured ANT into RL should then reconstitute thechaperone–preprotein complexes involved in targeting.We confirmed that purified ANT could indeed be reimported intoisolated mitochondria. First, purified ANT was radiolabeledby tyrosine iodination (Figure 2A, lane 6) and diluted intoimport reactions containing RL and mitochondria. After PK digestion,PK-resistant ANT was observed significantly above that in reactionstreated with valinomycin (Figure 2A, lanes 7 and 8). The PK-resistantmaterial in the valinomycin control reactions was similar tothat normally observed in reactions using cell-free translatedANT (Figure 2A, lanes 1–5). In a second approach, purifiedANT was chemically biotinylated on its cysteine side chains(Figure 2C, lanes 2–4, Coomassie stain). Import of ANT-Bafter dilution into reactions containing RL and mitochondriawas detected by streptavidin blots (Figure 2A, lanes 9–11).A number of high-molecular-weight background bands were observeddue to endogenous biotinylated mitochondrial proteins (datanot shown). Nevertheless, imported ANT-B was detected abovethe valinomycin background after PK digestion (Figure 2A, lanes9 and 10), and mock reactions lacking ANT-B showed no correspondingband (Figure 2A, lane 11). Thus, the purified ANT can be reimportedinto mitochondria, even after chemical modification.

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Figure 2. Reconstitution of chaperone–ANT complexes. (A) Left, a representative reaction of cell-free translated ANT (lane 1) imported into mitochondria (+ mito, lanes 2–5) as in Figure 1 is shown. Middle, purified ANT was radioiodinated (ANT-I125, lane 6) and diluted into reactions containing RL, ATP, and mitochondria (lanes 7 and 8). Right, purified ANT was biotinylated (ANT-B) and diluted into reactions containing RL, ATP, and mitochondria (lanes 9 and 10), whereas mock reactions contained no ANT-B (lane 11). Negative control reactions were treated with valinomycin (val) to abolish import (lanes 3, 5, 8, and 10). The extent of import was assessed by resistance to PK (lanes 4, 5, 7, 8, and 9–11). (B) Top, ANT was radiolabeled by cell-free translation and resolved on a Superose 6 10/300 GL column. The amount of ANT in each fraction was determined by SDS-PAGE and phosphorimager quantitation, and arbitrary phosphorimager units are represented. The column void volume (V₀) and elution volumes of molecular size standards (indicated in kilodaltons) are marked. Bottom, ANT-B was diluted into reactions containing RL and ATP and resolved on the same gel filtration column. The ANT-B in each fraction was detected by SDS-PAGE and streptavidin blots. The elution volume corresponding to the fractions is marked (indicated in milliliters). (C) Molecular weight markers (indicated in kilodaltons) are shown (lane 1) and purified ANT (lane 2), ANT after the biotinylation reaction (ANT-B, lane 3) and removal of excess biotin by desalting (lane 4). ANT-B bound to streptavidin-agarose was incubated in reactions containing RL (lane 5) and ATP. Complexes were recovered and eluted with Laemmli loading buffer (lane 7). Negative control reactions contained no ANT-B or RL (lane 6) or no ANT-B (lane 8). Discrete bands labeled a, b, c, and the range between d and e, were analyzed by mass spectrometry. Bands in the negative control reactions labeled f, g, h, and i also were analyzed.

Chaperone complexes with Tom70-dependent preproteins in RL havea characteristic profile on gel filtration chromatography. Asreported previously (Young et al., 2003

; Fan et al., 2006

),cell-free translated ANT eluted in a broad peak at $~$ 13-ml elutionvolume on a 24-ml Superose 6 column, with an apparent molecularsize of $~$ 600 kDa (Figure 2B). Some ANT was also observed in thevoid volume of the column (8-ml elution volume), most likelyrepresenting aggregated material (exclusion limit $~$ 5 MDa). Inparallel, ANT-B was diluted into chaperone binding reactionscontaining RL and ATP for 15 min at room temperature (Youngand Hartl, 2000

; Brychzy et al., 2003

), and then it was analyzedon the same gel filtration column. Streptavidin blots detecteda similar peak eluting around 13 ml (Figure 2B), in additionto void volume material. The reconstituted ANT-B complexes,therefore, reproduce those normally studied by cell-free translationas preimport intermediates, in molecular size as well as importcompetence.

To identify the components of chaperone–ANT complexes,ANT-B (Figure 2C, lane 4) was incubated with RL (Figure 2C,lane 5) as described above but in larger reactions. ANT-B complexeswere then isolated with streptavidin-agarose and analyzed bytotal protein staining (Figure 2C, lane 7). Several bands werevisible in the 40- to 100-kDa range. Very little ANT-B was observed,because the streptavidin–biotin interaction was mostlyresistant to the SDS-containing buffer used to elute the beads.The protein pattern was clearly distinct from that of the RL(Figure 2C, lane 5). Mock reactions lacking ANT-B returned farfewer bands (Figure 2C, lane 8), and no bands were detectedwith streptavidin-agarose alone (Figure 2C, lane 6). Visiblebands were subjected to tryptic digestion followed by mass spectrometryidentification of peptides. Relevant proteins identified aresummarized in Table 1. Although the exact rabbit sequences formany of the proteins are not known, the very high degree ofconservation between chaperones and cochaperones within mammals(>97% identity) allowed unambiguous identification basedon human, rat, mouse or pig sequences. Accession numbers arefor human sequences, unless otherwise indicated.

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Table 1. Proteins identified by mass spectrometry from reconstituted chaperone—ANT complexes (Figure 2C, lanes 7 and 8)

The band at $~$ 90 kDa (Figure 2C, lane 7, labeled a) was identifiedas a mixture of Hsp90 ${alpha}$ and Hsp90 $beta$ , the two highly similar cytosolicforms of the chaperone. The heavy band $~$ 70 kDa (labeled b) wasfound to be Hsc70. The greater amount of Hsc70 compared withHsp90 is in agreement with higher dependence on Hsc70 for import(Figure 1B). The bands below 70 kDa (labeled c, and a rangebetween d and e) contained a number of cochaperones of Hsc70and Hsp90. Samples from regions of the gels below the 40-kDamolecular weight did not return reliably identifiable peptidesexcept for ANT itself. The major visible bands in negative controlreactions (Figure 2C, lane 8, labeled f, g, h, and i) were alsoanalyzed, and they were found to be exclusively keratins andhemoglobin multimers (keratin 1, NP_006112 [GenBank] ; keratin 10, NP_000412 [GenBank] ;keratin 9, NP_000217 [GenBank] ; and hemoglobin $beta$ , NP_000509 [GenBank] ). These wereunavoidable background proteins and ruled out as chaperone complexcomponents. Importantly, no peptides from the chaperone-relatedcomponents were identified in the negative controls.

Components of the Chaperone–ANT Complexes. In addition to the Hsc70 and Hsp90 chaperones, several cochaperoneproteins were found (Table 1). Hop recognizes Hsc70 and Hsp90through two separate TPR domains. It is thought to coordinatethe transfer of substrates from Hsc70 to Hsp90, which is themajor pathway for many Hsp90-dependent substrates (Chen andSmith, 1998; Scheufler et al., 2000; Pratt and Toft, 2003; Younget al., 2004). Hop is found in many Hsp90–substrate complexes,and its presence in complexes with ANT was not unexpected. Tpr2binds both Hsc70 and Hsp90 through its two TPR domains, andit activates the Hsc70 ATPase through its J-domain. It has beenproposed to return substrates from Hsp90 to Hsc70, and its expressionlevel in cells optimized the maturation of the Hsc70- and Hsp90-dependentglucocorticoid receptor (Brychzy et al., 2003; Young et al.,2004). The presence of Tpr2 in ANT complexes suggests that ithas a similar role to optimize the balance between Hsc70 andHsp90, in this case favoring Hsc70. Furthermore, three distinctHsp40-related J-domain cochaperones were found. DJA1 (Hdj2,HSDJ) and DJA2 (Hdj3, HIRIP4) have been reported to be the constitutivelyexpressed members of the Hsp40 family (Terada and Mori, 2000).DJA4 (Hdj4) has been only recently discovered, and it has beenhypothesized to be functionally specialized (Hafizur et al.,2004). Mouse DJA4 is highly expressed in testis, but we havealso identified it in other tissues (data not shown). The presenceof these proteins in the chaperone–preprotein complexeswas tested directly by immunoblots (Figure 3). The main componentsdescribed above were detected in the reconstituted ANT-B complexes:Hsp90 and Hsc70 as well as Hop, Tpr2, DJA1, DJA2, and DJA4,confirming the mass spectrometry data.

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Figure 3. Components of chaperone–ANT complexes. Complexes associated with ANT-B were reconstituted in RL and coprecipitated as in Figure 2C, and then they were analyzed by immunoblots with antibodies against the indicated proteins. Samples shown are total RL (lane 1), ANT-B complexes (lane 2), and negative control reactions lacking ANT-B (lane 3).

Importantly, many other known cochaperones of Hsp90 and Hsc70were not detected by mass spectrometry. These included the immunophilinFKBP52, the cyclophilin Cyp40 and the kinase-binding Cdc37,all of which have been reported to have general chaperone activity,in the sense of unfolded polypeptide binding (Bose et al., 1996

;Freeman et al., 1996

; Kimura et al., 1997

). Also, the Hsp90cochaperone p23 (Pearl and Prodromou, 2006

), which stabilizesthe substrate-binding ATP-bound state of Hsp90, was not detected.p23 is common to many Hsp90 complexes, and it has intrinsicchaperone activity. The presence or absence of these proteinswas tested independently by immunoblots. First, immunoblotsunambiguously detected p23 in chaperone–ANT complexesbut not in negative control reactions (Figure 3). It is possiblethat the small size (predicted molecular weight 18 kDa) andstrong acidic charge of p23 limited the identifiable trypticpeptides derived from the protein or that the poorly stainingprotein was simply missed in the excision from gels. Next, immunoblotsdetected FKBP52 at similar low levels in both the ANT complexesand the negative control reactions (Figure 3), suggesting itwas nonspecifically bound and therefore not a major componentof the ANT complex. Cyp40 and Cdc37 were not detected at allin the ANT-B complexes, supporting the mass spectrometry data.Hsp40 (DJB1, Hdj1), the stress-inducible J-domain cochaperonethat is structurally divergent from the DJAs (Cintron and Toft,2006

; Qiu et al., 2006

) also seemed to be nonspecifically bound.

The only cochaperone positively identified by mass spectrometrythat could not be validated by immunoblots was Hip, possiblydue to the quality of the antibody (data not shown). Hip stabilizesthe ADP-bound form of Hsc70, but it is mainly thought to counterbalancethe Hsc70 nucleotide exchange factors (Hohfeld et al., 1995;Mayer and Bukau, 2005). A number of subunits of the TCP-1 chaperonin(TRiC, CCT) were matched to low numbers of peptides in the massspectrometry analysis, and their presence could not be validatedby immunoblots (data not shown). Several proteasome subunitswere similarly identified, but they likely represent clearanceof nonproductively targeted preprotein and they were not pursued.In summary, we propose that the proteins in Table 1, with theaddition of p23 and exception of Hip, comprise the major chaperonesand cochaperones involved in Tom70-dependent import. Furthermore,the exclusion of certain proteins from the chaperone–preproteincomplexes suggests a substantial degree of specificity in complexformation.

DJA Interaction with Preprotein
We were struck by the presence of three related DJA proteinsin the chaperone–ANT complexes. Although all three werepresent, it was possible that one in particular might be moreeffective than the others. For example, the higher number ofpeptides derived from DJA4 might suggest a greater involvementof that cochaperone with preprotein complexes. Alternatively,there might be subtler differences between them, such that theyfunction together in import, and perhaps other biological processes.In the yeast S. cerevisiae, the two cytosolic Hsp40-relatedproteins Ydj1 and Sis1 have distinct biological roles (Johnsonand Craig, 2001; Fan et al., 2004); however, Ydj1 is orthologousto the three human DJA proteins, whereas Sis1 is related tothe divergent Hsp40/DJB1. The homology between the human DJAs(70–85% similarity) suggests they have a closer functionalrelationship. The DJA proteins contain the J-domain, zinc fingerdomain, and C-terminal dimerization domain (Figure 4C, diagram)conserved from the eponymous DnaJ of E. coli (Terada et al.,1997; Terada and Mori, 2000; Borges et al., 2005; Qiu et al.,2006). As expected, their N-terminal J-domains were found toactivate ATP hydrolysis by Hsc70 (Terada and Mori, 2000; Hafizuret al., 2004). Based on experiments with the E. coli and S.cerevisiae orthologues, the binding site for unfolded polypeptidesshould reside in the central- to C-terminal regions of the DJAproteins (Walsh et al., 2004; Mayer and Bukau, 2005; Cintronand Toft, 2006; Qiu et al., 2006). Like most J-domains, thosein the DJA proteins are well conserved, and the greatest divergencein sequence is within the expected substrate binding region.This suggested that one difference between the DJAs might bethe range of substrates bound, or the strength of binding. However,sequences outside the J-domains of some proteins have been implicatedin Hsc70 interactions, so there might also be differences betweenthe DJAs in the activation of Hsc70. We therefore addressedthese possibilities systematically.

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Figure 4. DJA interaction with preprotein. A, ANT, and PiC were radiolabeled by cell-free translation (lane 1) and coprecipitated with nickel-Sepharose alone (beads, lane 2), or with nickel-Sepharose and purified His-tagged DJA1, DJA2, or DJA4 at a final concentration 5 µM (lanes 3–5). Recovered material was analyzed by SDS-PAGE and autoradiography. (B) Phosphorimager quantitation is shown of the coprecipitation of ANT and PiC with DJA1, DJA2 and DJA4, as in described in A, relative to that with DJA1 set to 1. (C) Diagram of DJA1, DJA2, and DJA4 architecture. J-domain (J, black), zinc finger (Zn, light gray), and C-terminal domains (C, dark gray) are indicated. The start sites of C-A1, C-A2, and C-A4 deletion mutants are marked (dashed line, amino acid numbers indicated). (D) ANT and PiC were coprecipitated with purified His-tagged C-A1, C-A2, and C-A4 as described in A. Phosphorimager quantitation of the coprecipitation is shown, relative to that with C-A1 set to 1. (E) Cell-free translated ANT and PiC (lane 1) were imported into mitochondria (+ mito, lanes 2–13) as described in Figure 1. As a negative control, import was abolished with valinomycin (val, lanes 3 and 9). Reactions were supplemented with 90 mM NaCl alone (S, lanes 4 and 10) or with 20 µM C-A1, C-A2, or C-A4 with 90 mM NaCl (lanes 5–7 and 11–13). The extent of import was assessed by resistance to PK (lanes 8–13). The mature noncleaved form of ANT (m) is visible, as are the precursor (p) and proteolytically cleaved mature (m) forms of PiC. (F) Phosphorimager quantitation is shown of the import of ANT, PiC, and ISP in the presence of 20 µM C-A1, C-A2, or C-A4, as described in E, relative to control reactions with added NaCl.

The binding of the DJAs to the polypeptide substrate ANT wastested first. The polypeptide binding specificities of the humanDJAs are so far unknown. For ease and accuracy of quantitation,we adapted a coprecipitation assay used to study preproteininteractions with Tom70 (Young et al., 2003

; Fan et al., 2006

).DJA1, DJA2, and DJA4 were purified as N-terminally His-taggedproteins. Radiolabeled ANT produced by cell-free translationwas incubated with identical amounts (5 µM) of each DJAprotein. The His-tagged proteins were reisolated with nickel-Sepharose,and the associated ANT was quantified. All three DJAs boundANT at levels above the low background binding, but DJA2 boundnoticeably less preprotein than DJA1 or DJA4 (Figure 4A, lanes2–5). Quantitation showed that DJA2 binding of ANT was $~$ 40% of DJA1 binding, whereas DJA4 binding was not significantlydifferent from that of DJA1 (Figure 4B). For comparison withanother Tom70-dependent preprotein, the assay was applied toPiC (Figure 4, A and B). Again, DJA1 bound PiC well, and DJA2seemed to have the poorest binding, at $~$ 40% of DJA1. However,DJA4 bound PiC relatively poorly, at <60% of DJA1 binding.These data suggested that the DJAs differ in their binding ofpolypeptides.

The full-length DJA proteins might bind polypeptides in a dynamicequilibrium, because their J-domains promote the transfer ofpolypeptides to Hsc70. The association of ANT and PiC with theDJAs might then depend on interactions with Hsc70 as well asthe actual affinity of binding to the DJAs. To directly addressthe level of polypeptide binding, truncation mutants of theDJAs lacking the N-terminal J-domain were purified. The deletionmutants, C-A1 (residues 98-397 of DJA1), C-A2 (residues 100-412of DJA2), and C-A4 (residues 99-397 of DJA4), were also N-terminallyHis-tagged, and they contained the complete zinc finger andC-terminal regions of the DJAs (Figure 4C). The binding of cell-freetranslated ANT and PiC to the mutants was tested as describedabove. C-A1 was found to bind strongly to both ANT and PiC,and C-A2 binding to both polypeptides was <50% of C-A1 binding(Figure 4D). C-A4 bound slightly less ANT than C-A1 and significantlyless PiC, at $~$ 60% relative to C-A1. Overall, the interactionsof the truncation mutants with polypeptides were similar tothose of the full-length DJAs, suggesting that Hsc70 interactionsdid not greatly change the substrate binding profiles of full-lengthversus truncated DJAs. These results confirmed that the DJAsdiverge in polypeptide binding, with DJA1 apparently bindingthe highest amount of preprotein. Also, as observed for DJA4,different polypeptides can be bound to varying degrees.

We wanted to evaluate the importance of DJA binding to preproteinfor mitochondrial import. Immunodepletion of the DJAs from RLcould not be achieved with the available antibodies (data notshown). So, we reasoned that the truncated DJAs should act asdominant-negative inhibitors of wild-type DJA function, by competingfor the same binding sites in preprotein but disallowing transferto Hsc70. Inhibition of Hsc70 binding should then impair theTom70 docking step required for import. Alternatively, Hsp40can activate substrate binding by Hsc70 without strongly interactingwith substrate (Minami et al., 1996; Cintron and Toft, 2006).If Hsp40 or some mechanism other than the DJAs was sufficientfor Hsc70 binding, the truncated DJAs should have less effect.Therefore, C-A1, C-A2, and C-A4 were added at 20 µM tomitochondrial import reactions of ANT and PiC. Note that PiCis proteolytically processed upon import to produce a fastermigrating band on SDS-PAGE (Zara et al., 1992), but the extentof true import was quantified as described for ANT by resistanceto externally added PK (Figure 4E). Indeed, all three mutantsclearly inhibited import of ANT and PiC to between 40 and 60%of control reactions (Figure 4F). The partial but significantinhibition of import approached the level observed with theC-90 competitor or combined Hsc70 and Hsp90 inhibition in Figure 1.As expected, the mutant DJAs had little effect on the Tom20-dependentimport of ISP (Figure 4F). For ANT and PiC, it seems that theeffect of each dominant DJA mutant cannot be overcome by theother DJA proteins or J-domain cochaperones present in the lysate.These data suggest that each of the DJAs function in the Tom70import pathway.

Hsc70–Preprotein Interactions
To further test the importance of the DJAs for Hsc70 bindingto preprotein, the binding of Hsc70 to purified ANT was monitoredover time. As established in previous work on Hsc70 and Hsp90interactions with the glucocorticoid receptor (Young and Hartl,2000; Sondermann et al., 2001; Brychzy et al., 2003), radiolabeledHsc70 generated by cell-free translation was used for ease andaccuracy of quantitation. Although unlabeled Hsc70 is in excessin the binding reactions, the radiolabeled protein acts as atracer and matches the behavior of unlabeled protein. At differenttimes after addition to ANT-B, the preprotein was recoveredwith streptavidin-agarose, and bound Hsc70 was quantified. Hsc70bound with a fast initial increase and reached a maximum at $~$ 10 min (Figure 5A). When C-A1, C-A2, and C-A4 were added tothe reactions at 20 µM, binding of Hsc70 was clearly diminished(Figure 5A). Moreover, C-A2 was the most inhibitory, reducingHsc70 binding as early as 1 min into the reaction, with a finallevel of $~$ 30% of the control reaction. C-A1 and C-A4 were slightlymore moderate in their effect, with inhibition visible by 2–4min and a final Hsc70 level of $~$ 60% of the control. Thus, thethree truncation mutants directly inhibit Hsc70 interactionswith preprotein, albeit to different degrees.

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Figure 5. Hsc70-preprotein interactions. (A) Top, Hsc70 was radiolabeled by cell-free translation, incubated with ANT-B immobilized on streptavidin-agarose, and coprecipitated after the indicated times. Reactions contained either no addition, or 20 µM purified C-A1, C-A2, or C-A4. Recovered material was analyzed by SDS-PAGE and autoradiography. Bottom, quantitation of time courses of Hsc70 binding is shown. (B) Top, cell-free translated Hsc70 was coprecipitated with ANT-B as described in A but after 15 min of binding. Samples were resuspended in dissociation reactions with or without ATP, containing buffer alone, or 5 µM purified p23 or C-Bag. After 10 min, released and remaining bound fractions were separated and analyzed. Bottom, quantitation of dissociation reactions.

The dominant mutants seem to compete with wild-type DJAs forpolypeptide, preventing the wild-type cochaperones from initiatingHsc70 binding (Cintron and Toft, 2006

). The partial effectsof the mutants suggested that competition with the wild-typeDJAs was not complete. This in turn implied that the DJAs havedistinct sets of binding sites that only partly overlap witheach other. Interestingly, C-A2 was the strongest inhibitorof Hsc70 binding (Figure 5A), but it seemed to bind less overallpreprotein than C-A1 or C-A4 (Figure 4D). We suggest that C-A2might bind fewer sites within the polypeptides, but these sitesare relatively more important for Hsc70 binding. In contrast,C-A1 and C-A4 might bind more, but less distinctly important,sites. The overall result is that the three mutants inhibitpreprotein import to a similar degree (Figure 4F).

To confirm that the Hsc70–preprotein complexes observedin these experiments were formed normally, their nucleotidedependence was assayed. In previous experiments with the glucocorticoidreceptor, the C-Bag nucleotide exchange factor promoted Hsc70dissociation from isolated complexes in an ATP-dependent manner(Sondermann et al., 2001). Following a similar approach, Hsc70–ANTcomplexes were isolated after 15 min of binding, and then theywere incubated under varying conditions in the absence or presenceof ATP. Dissociated and bead-bound fractions were analyzed separately.As observed previously, ATP alone did not promote complex dissociationgreatly over buffer without ATP (Figure 5B). As another negativecontrol, the purified Hsp90-specific cochaperone p23 also didnot strongly dissociate Hsc70. However, C-Bag markedly promotedHsc70 dissociation but only in the presence of ATP (Figure 5B).Thus, the Hsc70–preprotein complexes inhibited by theDJA mutants seem to be normally functional complexes.

DJA Heterocomplex Formation
To further examine the formation of DJA–preprotein complexes,we asked whether different DJAs could bind to a polypeptidesimultaneously. Experimental approaches described above weremodified for this purpose. Chaperone complexes with ANT-B wereformed by its dilution into RL with ATP, as performed for thegel filtration analysis of Figure 2B, but with the additionof different cell-free translated, radiolabeled DJA proteinsinto the binding reaction. Each reaction was then allowed tobind to a different purified His-tagged DJA protein identicallyto Figure 4A. Complexes were reisolated with nickel-Sepharoseand analyzed for the presence of the radiolabeled DJA. In thismanner, DJA1 was detected in chaperone–ANT complexes recoveredwith DJA2 and DJA4, at levels above the low background binding(Figure 6A). Similar, DJA2 was recovered with DJA1 and DJA4,and DJA4 with DJA1 and DJA2. Therefore, binding of each DJAcochaperone does not seem to be exclusive of the others, andthey can form heterocomplexes with substrate.

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Figure 6. DJA heterocomplex formation. (A) DJA1, DJA2, and DJA4 were radiolabeled by cell-free translation (input, lanes 1, 5, and 9). ANT-B was diluted into reactions containing RL, ATP, and each radiolabeled DJA, as described in Figure 2B. Complexes were coprecipitated (recovery) with nickel-Sepharose alone (beads, lanes 2, 6, and 10) or nickel-Sepharose and the indicated His-tagged DJA protein, as described in Figure 4A. Recovered material was analyzed by autoradiography. (B) Top, DJA1, DJA2, and DJA4 were radiolabeled by cell-free translation and coprecipitated with ANT-B as described in Figure 5A. Bottom, averaged quantitation of time courses of DJA binding are shown.

It was also possible that the different DJA cochaperones boundpolypeptide substrate in a defined order, or with a characteristickinetic. To investigate this, ANT-B complexes with chaperoneswere formed in RL, and they were reisolated at different timesas in Figure 5A; radiolabeled DJA proteins generated by cell-freetranslation were used to monitor their binding to complexes.All three of the DJA proteins showed the same fast initial rateof binding, with complex formation essentially complete in <5min (Figure 6B). Binding of the DJAs to the preprotein was asfast, if not faster than, the rate of Hsc70 binding (compareFigure 6B with 5A), consistent with the expected mechanism inwhich the Hsp40-related cochaperones activate substrate bindingby Hsc70. Together with the formation of DJA heterocomplexes(Figure 6A), these results suggest that the DJA cochaperonesdo not have a sequential binding mechanism where one DJA displacesanother previously bound DJA. So, it is likely that the DJAsact independently of each other to bind substrate and activateHsc70.

DJA Activation of Hsc70
In addition to binding polypeptides, the DJAs should activatethe Hsc70 ATPase through their J domains. To further exploredifferences between them, we measured the steady-state Hsc70ATPase rates supported by the three full-length DJAs. J-domainsspecifically stimulate ATP hydrolysis to ADP by Hsc70, but notthe exchange of ADP for ATP, so an excess of the C-Bag exchangefactor was used to ensure that ATP hydrolysis was rate limiting(Sondermann et al., 2001; Mayer and Bukau, 2005). Purified Hsc70at 4 µM was supplemented with 20 µM C-Bag and increasingconcentrations of the DJAs. All DJAs could stimulate Hsc70 ATPaseactivity above its basal rate of <1 min^–1 (Figure 7A).Interestingly, at all concentrations above 1 µM, DJA1was clearly more efficient at ATPase stimulation than DJA2 andDJA4, which were similar to each other (Figure 7A). At 8 µMDJA1, Hsc70 activity reached around 7 min^–1, in line withpreviously reported rates, whereas DJA2 and DJA4 at the sameconcentrations supported rates $~$ 5 min^–1. Our results arein the same range as reported previously (Terada and Mori, 2000;Hafizur et al., 2004), with the difference that in our hands,DJA4 is somewhat more active than was thought. Although thedifference between DJA1 and the other two may not seem great,in a finely balanced biological system, the functional consequencesof such variation may be amplified. Also, differences betweenDJA activation of Hsc70 seem to be greatest (at least 2-fold)in the concentration range of 2–4 µM DJAs, whichlies closest to the estimated cellular concentration of theDJAs, and the estimated ratio to Hsc70 in cells.

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Figure 7. DJA activation of Hsc70. (A) Steady-state ATPase rates of purified Hsc70 were measured in reactions containing 1 mM ATP, 4 µM Hsc70, 20 µM C-Bag, and the indicated concentrations of DJA1, DJA2, or DJA4. Right inset, representative example of the data from which linear rates were calculated. Reactions contained ${alpha}$ -[³²P]ATP and the amount of ADP produced at each time point was determined by separation on TLC and phosphorimager quantitation. (B) Refolding of guanidine-denatured luciferase was monitored in reactions containing 50% RL and 2 mM ATP, or 4 µM Hsc70, 0.5 µM C-Bag, and 4 µM DJA1, DJA2, or DJA4 as indicated, with or without 2 mM ATP. The activity of luciferase refolded in RL reactions at 60 min was set to 100%.

Another property of the DJAs was their expected ability to supportpolypeptide refolding by Hsc70. A polypeptide substrate commonlyused to study Hsc70 function is firefly luciferase, which hasa sensitive and reproducible enzymatic assay. Purified Hsc70has been shown to assist luciferase refolding in numerous studies(Hohfeld et al., 1995

; Freeman and Morimoto, 1996

; Minami etal., 1996

; Hohfeld and Jentsch, 1997

; Terada et al., 1997

; Luderset al., 2000

; Terada and Mori, 2000

). However, in most casesthe stress-inducible cochaperone Hsp40 was used, and a directcomparison between all three DJAs with Hsc70 has not yet beenreported. Thus, we tested the refolding of luciferase afterdilution out of 6 M guanidine into reactions containing 4 µMHsc70 and 4 µM of each DJA in turn, as well as 0.5 µMC-Bag, which was found to be optimal for refolding at this concentration(data not shown). Refolding reactions contained 1 mM ATP, whereasnegative control reactions contained no ATP, and they were treatedwith apyrase to destroy any endogenous ATP. 50% RL with ATPserved as a positive control. Surprisingly, DJA1 seemed to bethe least effective in assisting refolding (Figure 7B), despiteproviding the strongest stimulation of the Hsc70 ATPase activity(Figure 7A). Refolding with DJA1 reached slightly above 20%of the RL control after 60 min (Figure 7B). In marked contrast,DJA2 was very efficient at promoting luciferase refolding, supportinga refolding level essentially the same as the RL control. DJA4,in contrast, was also relatively weak in promoting refolding,although the final activity reached was $~$ 40% of the RL controland somewhat higher than with DJA1. In all cases, the negativecontrol reactions lacking ATP produced no significant refolding(Figure 7B). Overall, the divergent refolding function of theDJAs may result from a more complex combination of differencesin polypeptide binding, Hsc70 ATPase stimulation, and perhapsother factors. In an earlier report, DJA1 and DJA2 promotedluciferase refolding to similar degrees (Terada and Mori, 2000

),and the divergence from our results seems due to apparentlysmall differences in experimental conditions. It might be thatDJA2 is more robust and able to support refolding under a broaderrange of conditions. The variability of the results may alsobe taken as further evidence that minor differences betweenthe DJAs might be amplified depending on the biological context.

DJA Function in Cells
The refolding of a guanidine-denatured protein can be distinctfrom the cellular folding of the same protein during its synthesison ribosomes. Experiments in mammalian and S. cerevisiae cellssuggested that Hsc70 is important for the folding of fireflyluciferase during or shortly after its synthesis. Thus, theDJA proteins were compared in their effects on the cellularfolding of luciferase. A vector expressing luciferase from aconstitutive cytomegalovirus (CMV) promoter was transfectedinto HeLa cells simultaneously with transient overexpressionof each of the DJA proteins. Immunoblots showed that the levelsof transfected myc-tagged DJA1 and DJA2 were in the same rangeas those of the endogenous proteins, although normal levelsof DJA4 were low compared with DJA1 and DJA2 (Figure 8A). Levelsof other chaperones such as Hsp90, Hsc70, and mitochondrialmatrix Hsp60 were unaffected by DJA expression. Cells expressingDJA1 produced markedly higher levels of luciferase enzymaticactivity relative to control cells transfected with noncodingvector, around a threefold increase (Figure 8A). Expressionof DJA2 and DJA4 also enhanced activity around 2.5-fold abovethe control. The activity of cotranfected $beta$ -galactosidase controlledby a simian virus 40 (SV40) promoter showed comparatively littlevariation whether the DJAs were expressed (Figure 8A), and itwas used to correct for transfection efficiency. It was notablethat the amount of luciferase protein detected by immunoblotseemed to be the same between the control and DJA-expressingcells (Figure 8A). This suggested that the DJAs increased theenzymatic activity of the luciferase relative to its total amount,that is, the specific activity of luciferase. Such an effectwould be expected if the folding of the model protein is enhanced.The folding of luciferase newly synthesized in the cells isalso distinct from its refolding from the guanidine-denaturedstate observed in Figure 7B. The change in apparent activitybut not absolute expression also argues against a nonspecificeffect on transcription or translation.

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Figure 8. DJA function in cells. (A) HeLa cells were transfected with plasmids expressing luciferase from a CMV promoter, $beta$ -galactosidase from an SV40 promoter, and either empty vector or the indicated myc-tagged DJA proteins under a CMV promoter. Two days after transfection, cells were harvested and equivalent amounts of lysate analyzed by immunoblots for the indicated proteins (top) and by enzymatic activity assays (bottom). In blots for DJA1, DJA2, and DJA4, positions of the endogenous and overexpressed myc-tagged proteins are marked. Bands cross-reacting with the antibodies are marked with an asterisk; in cells transfected with myc-tagged DJA4 and detected with antibody against DJA4, a band of similar size to endogenous DJA4 seems to be a proteolytic fragment of the myc-tagged protein. To compare enzymatic activities, the average activities of cells transfected with luciferase (luc), $beta$ -galactosidase ( $beta$ -gal), and empty vector was set to 1. The $beta$ -galactosidase activities were then used to correct luciferase activities for variations in transfection. As in all figures, standard deviations were determined from at least three independent experiments. (B) HeLa cells were transfected with plasmids expressing luciferase from a GRE-controlled promoter, constitutive GR- ${Delta}$ LBD and $beta$ -galactosidase, and either empty vector or the indicated myc-tagged DJA proteins as described above. Two days after transfection, cells were analyzed as described above. (C) HeLa cells were transfected with plasmids expressing 3HA-tagged PiC from a chicken $beta$ -actin promoter, constitutive $beta$ -galactosidase, and either empty vector or the indicated myc-tagged DJA proteins as described above. Two days after transfection, cells were analyzed as described above. Quantitation of the HA immunoblot signal is shown, with that of cells transfected with $beta$ -galactosidase and empty vector set to 1.

To confirm these observations, cells were transfected with avector expressing luciferase controlled by a GRE, together witha constitutively expressed glucocorticoid receptor lacking thechaperone-dependent ligand-binding domain (GR- ${Delta}$ LBD). This combinationis known to provide constitutive, hormone-, and Hsp90-independentexpression of the luciferase gene (Hollenberg et al., 1987

;Hollenberg and Evans, 1988

). When the DJA cochaperones wereoverexpressed, a pattern of luciferase activity was observedsimilar to that of the above-mentioned experiments. All threeproduced significant increases in luciferase activity, withDJA1 being most effective at more than threefold of the control(Figure 8B). DJA2 and DJA4 were somewhat less effective at $~$ 1.8-and 2.7-fold of the control, respectively. As mentioned above,immunoblots seemed to detect similar absolute amounts of luciferaseas well as the other control proteins. These results argue againsteffects derived from the luciferase expression vectors or theirpromoters. Overall, it seems that each of the DJA cochaperonescan promote polypeptide folding in the native cellular environment,albeit with different degrees of efficiency.

We next addressed the effect of the DJAs on a Tom70-dependentmitochondrial preprotein in cells. The mitochondrial importof a transiently transfected 3HA-tagged PiC was previously shownto be sensitive to inhibition of Hsp90 by geldanamycin, whichreduced the levels of mature, proteolytically processed PiC