The Carboxy-Terminal Domain of Hsc70 Provides Binding Sites for a Distinct Set of Chaperone Cofactors

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Mol Cell Biol, April 1998, p. 2023-2028, Vol. 18, No. 4
0270-7306/98/$04.00+0
Copyright © 1998, American Society for Microbiology. All rights reserved.

The Carboxy-Terminal Domain of Hsc70 Provides Binding Sites for a Distinct Set of Chaperone Cofactors

Jens Demand, Jens Lüders, and Jörg Höhfeld^*

ZMBH, Zentrum für Molekulare Biologie, Universität Heidelberg, D-69120 Heidelberg, Germany

Received 15 October 1997/Returned for modification 16 December 1997/Accepted 6 January 1998

	ABSTRACT

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The modulation of the chaperone activity of the heat shock cognate Hsc70 protein in mammalian cells involves cooperation withchaperone cofactors, such as Hsp40; BAG-1; the Hsc70-interactingprotein, Hip; and the Hsc70-Hsp90-organizing protein, Hop. Byemploying the yeast two-hybrid system and in vitro interactionassays, we have provided insight into the structural basis thatunderlies Hsc70's cooperation with different cofactors. The carboxy-terminaldomain of Hsc70, previously shown to form a lid over the peptidebinding pocket of the chaperone protein, mediates the interactionof Hsc70 with Hsp40 and Hop. Remarkably, the two cofactors bindto the carboxy terminus of Hsc70 in a noncompetitive manner, revealingthe existence of distinct binding sites for Hsp40 and Hop withinthis domain. In contrast, Hip interacts exclusively with the amino-terminalATPase domain of Hsc70. Hence, Hsc70 possesses separate nonoverlappingbinding sites for Hsp40, Hip, and Hop. This appears to enablethe chaperone protein to cooperate simultaneously with multiplecofactors. On the other hand, BAG-1 and Hip have recently beenshown to compete in binding to the ATPase domain. Our data thusestablish the existence of a network of cooperating and competingcofactors regulating the chaperone activity of Hsc70 in the mammaliancell.

	INTRODUCTION

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Molecular chaperones of the 70-kDa heat shock protein (Hsp70) family participate in various cellular processes under normalgrowth conditions as well as under cellular stress (7, 15).Hsp70 apparently stabilizes nonnative polypeptides through thebinding of hydrophobic peptide segments, which are exposed duringprotein synthesis, protein translocation, and protein degradation(26). Recognition of a polypeptide substrate is mediated byHsp70's 18-kDa peptide binding domain and appears to involve a10-kDa carboxy-terminal domain that forms a lid over the peptidebinding pocket (26, 34). Substrate recognition is controlledby the binding of ATP to the amino-terminal 45-kDa ATPase domainof Hsp70, ATP hydrolysis, and nucleotide exchange (8, 21,26). The ATP-bound form of Hsp70 binds and releases substratesrapidly, resulting in a low overall affinity, whereas the ADPform binds substrates slowly but more stably (24, 27). Thecycling of Hsp70 between the different nucleotide states is regulatedby chaperone cofactors, which modulate the ATPase activity ofHsp70 and thus influence the affinity of the chaperone for polypeptidesubstrates (12, 15, 21, 26).

We have recently characterized cofactors that participate in the regulation of the cytosolic and nuclear heat shock cognateHsc70 in mammals (16-18, 22). Efficient association of Hsc70with a polypeptide substrate is achieved through the cooperationof the chaperone protein with Hsp40 (also known as Hdj-1). Hsp40stimulates the conversion of Hsc70-bound ATP to ADP, resultingin the stable association of Hsc70 with a polypeptide substrate(11, 22). Subsequent ADP release and ATP rebinding can occurspontaneously to a significant extent when Hsc70 cooperates withHsp40 (16, 22). However, the ADP-bound state of Hsc70, generatedduring interaction with Hsp40, can be affected by the Hsc70-interactingprotein, Hip (also known as p48), and the BAG-1 cofactor (alsoknown as Rap46 and Hap46) in opposite ways (16, 17). Bothproteins bind to the ATPase domain of Hsc70 (16, 31, 33).However, while Hip appears to stabilize the ADP-bound conformationof Hsc70, BAG-1 has been shown to stimulate ADP release from thechaperone protein (16). The physiological consequences of theregulation of Hsc70 by BAG-1 remain to be established. On theother hand, Hip-mediated stabilization of the ADP-bound form ofHsc70 may be of particular importance for the cooperation of Hsc70with other chaperone systems in the mammalian cell (12, 35).For example, Hsc70 cooperates with the abundant cytosolic chaperoneHsp90 during the conformational regulation of signaling molecules,such as steroid hormone receptors and certain protein kinases(2, 12). Intriguingly, Hip was found to be associated withthe progesterone receptor and the oncogenic tyrosine kinase pp60^v-src, respectively, as part of an Hsc70-Hsp90 chaperone complex (17,25, 30). It was therefore speculated that Hip stabilizes theinteraction of Hsc70 with the signaling molecule until Hsp90 isrecruited to the chaperone-substrate complex (12, 35). Notably,the cooperation of Hsc70 with Hsp90 also involves the Hsc70-Hsp90-organizingprotein, Hop (also known as p60 in mammals and Sti1 in Saccharomycescerevisiae) (23, 29). Hop has been identified as a componentof chaperone complexes containing Hsp70 and Hsp90 in mammals andyeast and appears to act as a coupling factor mediating the interactionbetween the chaperone proteins (4-6, 29, 30).

Here we provide insight into structural and functional aspects of the interaction of Hsc70 with different cofactors. We showthat the 10-kDa carboxy-terminal domain of Hsc70 provides nonoverlappingbinding sites for Hop (p60/Sti1) and Hsp40 (Hdj-1). In contrast,the binding of Hip to Hsc70 is exclusively mediated by the amino-terminalATPase domain of Hsc70. The existence of distinct binding sitesfor different Hsc70 cofactors appears to provide the structuralbasis for the functional cooperation of Hsc70 with multiple chaperonecofactors as it occurs during Hsc70-Hsp90-mediated processes.

	MATERIALS AND METHODS

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Cloning of the rat hop cDNA. To investigate the interaction of Hop with rat Hsc70, we cloned the rat hop cDNA by PCR, with a rat liver cDNA library (ClontechLaboratories) as a template. Primers covering the 3' and 5' regionswere designed based on the nucleotide sequences of mouse and humanhop as follows: 5'-GTGCGGACCGGCCGTCGACCTATGGAGCAGGTGAATGAGC-3'and 5'-GGTGTGCCTCTAGAATATTCACCGAATTGCGATGAGACC-3'. To excludePCR-induced mutations, four independently isolated clones werecompletely sequenced and found to be identical. The deduced primarystructure of the rat Hop protein displays 99.1% similarity tomouse Hop and 97.4% similarity to human Hop (mouse and human Hopproteins have 97.2% similarity). The open reading frame of rathop was subcloned into plasmid pAD in frame with the GAL4 activationdomain coding region (pAD-hop). pAD is based on plasmid pGAD-GH(Clontech Laboratories) but carries the 695-bp HindIII/HindIIIcassette, including the multiple cloning site of plasmid pGAD424(Clontech Laboratories). For expression of Hop in Sf9 insect cellsafter infection with recombinant baculovirus, the open readingframe of hop was subcloned into vector pVL1392 (PharMingen).

Construction of plasmids containing hsc70. The complete open reading frame of rat hsc70, including a portion of the 3' noncoding region, was obtained by restrictionenzyme digestion of plasmid pET-hsc70 (28) and was subclonedinto vector pGBT9 (Clontech Laboratories) (pGBT-hsc70). Fragmentsof hsc70 encoding the carboxy-terminal 139 and 110 amino acidsand a mutant form of the 70C139 domain lacking the EEVD motifwere amplified by PCR and subcloned into pGBT9 (pGBT-70C139, pGBT-70C110,and pGBT-70C139 $Delta$ EEVD). PCR-amplified fragments were sequencedto confirm the wild-type character. The construction of a plasmidencoding the GAL4 DNA-binding domain fused to the Hsc70 ATPasedomain was previously described (17) (it is designated pGBT-70N383in this paper). For expression as glutathione S-transferase (GST)fusion proteins, hsc70 fragments were subcloned into vector pGEX-4T-1(Pharmacia).

Protein expression and purification. Rat Hsc70, rat Hip, human Hsp40, and human BAG-1 were purified after recombinant expression in insect cells (Hsc70, Hip, andBAG-1) or bacteria (Hsp40) as previously described (16). RatHop was expressed in Sf9 insect cells after infection with recombinantbaculovirus. After growing for ~60 h, the infected cells weredisrupted with a French pressure cell (Aminco) and spun at 100,000× g for 30 min. Hop was purified by chromatography of the supernatantfraction on DEAE-Sepharose (Pharmacia), Bio-Gel HT hydroxyapatite(Bio-Rad), butyl-Sepharose (Pharmacia), and a MonoP column (Pharmacia).Prior to final concentration and dialysis, the Hop preparationwas passed over an ATP-agarose column (Sigma) to remove minuteamounts of associated Hsp70. Nontagged GST and GST fusion proteinswere expressed by addition of 0.1 mM isopropyl-1-thio- $beta$ -D-galactopyranosideto Escherichia coli TG1 cells transformed with corresponding pGEX-4T-1plasmids. After induction at 37°C for 3 h, the cells were disruptedwith a French pressure cell and centrifuged at 100,000 × g. GST,GST-70C139, and GST-70C110 were purified on glutathione-Sepharose(Pharmacia) as described by the manufacturer.

Localization of cofactor binding sites on Hsc70 by the yeast two-hybrid system. To analyze the interaction of Hip and Hop with Hsc70 and Hsc70 fragments in the two-hybrid assay, yeast strain HF7c (ClontechLaboratories) was transformed with corresponding two-hybrid constructs.Expression of GAL4 DNA-binding domain and GAL4 activation domainfusion proteins was investigated by immunoblotting of crude cellextracts after sodium dodecyl sulfate-polyacrylamide gel electrophoresis(SDS-PAGE) with monoclonal anti-GAL4 activation domain and anti-GAL4DNA-binding domain antibodies (Clontech Laboratories), revealingsimilar expression levels of the different fusion proteins. Interactionwith Hsc70 or Hsc70 fragments was analyzed by growth of correspondingtransformants on synthetic dextrose minimal medium lacking histidine,leucine, and tryptophan for 7 days at 30°C (1).

In vitro binding assays. For in vitro binding assays, GST, GST-70C139, GST-70C110, and GST-70C139 $Delta$ EEVD were purified as described above on glutathione-Sepharosewithout final elution with glutathione. The proteins were storedat 4°C bound to the Sepharose beads in an equal amount of solutioncontaining 20 mM HEPES-KOH (pH 7.2), 25 mM KCl, 1 mM EDTA, 1 mMNaN₃, and 0.002% phenylmethylsulfonyl fluoride. Immobilized GST,GST-70C139, and GST-70C110 (160 µg each) were incubated with 45µg of Hop, 35 µg of Hip, 35 µg of BAG-1, or 30 µg of Hsp40 in500 µl of buffer A (20 mM HEPES-KOH [pH 7.2], 50 mM KCl) at 4°Cfor 2 h. Following collection of the flowthrough fraction, theSepharose beads were washed five times with 500 µl of buffer A.Bound protein was finally eluted by addition of 500 µl of bufferA containing 100 mM glutathione. All fractions were trichloroaceticacid-precipitated and subsequently analyzed by SDS-PAGE. Hop,Hip, and BAG-1 were detected by Coomassie blue staining. Due tothe similar molecular masses of Hsp40 and the GST fusion proteins,Hsp40 was detected in the eluted fractions by immunoblotting witha polyclonal rabbit anti-Hsp40 antibody. Competition between full-lengthHsc70 and GST-70C139 in binding to Hsp40 was analyzed by incubationof 40 µg of immobilized GST-70C139 with 10 µg of Hsp40, as wellas 73 µg of Hsc70 when indicated. Binding of Hop to immobilizedGST-70C139 in the presence of Hsp40 was analyzed by incubationof 40 µg of immobilized GST-70C139 with 20 µg of Hop (correspondingto 0.67 µM) and the indicated amount of Hsp40. About 45% of theadded Hop protein was bound to GST-70C139 after incubation for2 h at 4°C.

Complexes of Hop and Hsc70 were formed by incubation of 60 µg of Hop and 73 µg of Hsc70 in 50 µl of buffer A containing 5%glycerol-1 mM EDTA for 1 h at 4°C. Samples were centrifuged at100,000 × g for 20 min and subsequently size fractionated on aSuperose 12 column (Pharmacia) equilibrated in the same buffer.Fractions were trichloroacetic acid-precipitated and analyzedby SDS-PAGE. The amounts of Hop and Hsc70 were quantified afterCoomassie blue staining.

Miscellaneous. Rates of ATP hydrolysis were determined as described previously (20). Protein concentrations were determined with the Bio-RadBradford assay reagent with gamma globulin as the standard. RecombinantDNA techniques were performed as described previously (1).

Nucleotide sequence accession number. The nucleotide sequence of the rat hop open reading frame has been submitted to the EMBL Nucleotide Sequence Database (accessionno. Y15068).

	RESULTS

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Hip and Hop recognize distinct regions of the Hsc70 chaperone. We investigated the capacity of the carboxy terminus of Hsc70 to mediate an interaction with chaperone cofactors. For thispurpose, we expressed deletion fragments of rat Hsc70 which comprisethe carboxy-terminal 110 (70C110) and 139 (70C139) amino acids(residues 537 to 646 and 508 to 646, respectively) (Fig. 1A).Residues 508 and 537 are located at the junction between the peptidebinding pocket and the carboxy terminus of Hsc70. Each fragmentincludes a tightly folded $alpha$ -helical subdomain that forms a lidover the peptide binding site (34), multiple degenerate repeatsof the tetrapeptide GGMP, and the regulatory EEVD motif at theextreme carboxy terminus of Hsc70 (3, 9). Interaction withthe Hsc70 cofactors Hip and Hop was analyzed by the yeast two-hybridsystem (Fig. 1B). We have previously shown that rat Hip interactswith the ATPase domain of Hsc70 in the two-hybrid assay (17,18). In contrast, an interaction of Hip with the two carboxy-terminalfragments of Hsc70 was not observed (Fig. 1B), although thesefragments were expressed at levels similar to that of the ATPasedomain construct (data not shown). To analyze the interactionof Hop with rat Hsc70, we cloned the hop cDNA from a rat livercDNA library (see Materials and Methods). Similarly to Hip, theHop protein interacted with full-length Hsc70 in the two-hybridassay (Fig. 1B). However, Hop did not bind to Hsc70's ATPase domain.Instead, it efficiently recognized the carboxy-terminal fragmentsof Hsc70, 70C110, and 70C139. Encouraged by these results, weattempted to further localize the region within the carboxy terminusof Hsc70 that mediates binding to Hop. For this purpose the followingdeletion fragments of Hsc70 were expressed in the two-hybrid systemand examined for their interaction with Hop: (i) a carboxy-terminalfragment that lacks the EEVD motif (amino acids 508 to 642), (ii)a fragment that comprises primarily the $alpha$ -helical subdomain (aminoacids 508 to 612), and (iii) a fragment that comprises only theGGMP repeats and the EEVD motif (amino acids 613 to 646). Allof the deletion fragments were expressed to levels similar tothose of the 70C139 and 70C110 fragments in the two-hybrid system(data not shown), yet an interaction with Hop was not observed(data not shown). It appears that the $alpha$ -helical subdomain, theGGMP repeats, and the carboxy-terminal EEVD motif of Hsc70 forma structural entity that mediates interaction with Hop. Thus,distinct binding sites have evolved in Hsc70 for the chaperonecofactors Hip and Hop.

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FIG. 1. Interaction of Hsc70 and Hsc70 deletion fragments with Hip and Hop in the yeast two-hybrid assay. (A) Full-length rat Hsc70 (amino acids 1 to 646) (70) and deletion fragments of Hsc70 (70N383, 70C139, and 70C110) were fused to the Gal4 DNA-binding domain of plasmid pGBT9 and expressed in yeast strain HF7c. Peptide-bdg., peptide-binding domain. (B) Interaction with Hip and Hop was analyzed after growth of double transformants, carrying pAD-Hip (Hip) or pAD-Hop (Hop) and the indicated Hsc70 construct, on synthetic dextrose minimal medium lacking histidine for 7 days at 30°C. " $-$ " indicates a control strain that carries the unmodified plasmid pGBT9 instead of an Hsc70 construct.

Hop directly interacts with Hsc70's carboxy terminus. To exclude the possibility that the interaction between Hop and the carboxy terminus of Hsc70 observed in the two-hybrid assayinvolved additional proteins, a biochemical interaction assaywas developed. Hop was purified to homogeneity after expressionin insect cells infected with a recombinant baculovirus. The carboxy-terminalfragments of Hsc70 fused to GST were expressed in E. coli andaffinity purified. While purified Hop did not significantly bindto unmodified GST immobilized on glutathione-Sepharose, the chaperonecofactor was quantitatively retained on immobilized GST-70C139and GST-70C110 (Fig. 2). In contrast, purified Hip and BAG-1,previously shown to bind to Hsc70's ATPase domain (16, 17,31, 33), did not interact with the carboxy terminus of Hsc70(Fig. 2). The in vitro assay thus confirms the specific recognitionof Hsc70's carboxy terminus by Hop and reveals that Hop interactsdirectly with the carboxy terminus without a requirement for additionalprotein components. Direct interaction between Hop and Hsc70 wasalso observed with purified full-length Hsc70. Incubation of Hopwith Hsc70 gave rise to an ~300-kDa Hop-Hsc70 complex that wasdetectable after gel filtration chromatography (Fig. 3). About40% of the added Hsc70 coeluted with Hop in fractions 6 to 9.Notably, Hop alone eluted from the gel filtration column withan apparent native mass of ~130 kDa, which would be consistentwith a dimeric structure of the chaperone cofactor. Moreover,the apparent mass of the Hop-Hsc70 complex (~300 kDa) may reflectthe binding of two molecules of Hsc70 to the dimeric Hop protein.However, additional structural data are required to determinethe exact stoichiometry of Hop-Hsc70 complexes.

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FIG. 2. In vitro binding assays with immobilized GST or GST fusion proteins comprising carboxy-terminal fragments of Hsc70 and purified Hop, Hip, and BAG-1. Immobilized GST, GST-70C139, and GST-70C110 were incubated with purified Hop, Hip, and BAG-1 as indicated for 2 h at 4°C. After collection of the flowthrough fraction (FT), the resin was washed five times (1 to 5) and bound protein was eluted with glutathione (E). Hop, Hip, and BAG-1 were detected by Coomassie blue staining after SDS-PAGE analysis of the collected fractions.

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FIG. 3. Gel filtration chromatography of Hop and Hop-Hsc70 complex. Hop (60 µg) was incubated alone (Hop) or in the presence of Hsc70 (73 µg) (Hop/Hsc70) for 1 h at 4°C, followed by gel filtration chromatography on a Superose 12 column. Amounts of Hop were quantified by densitometry of Coomassie blue-stained SDS-polyacrylamide gels.

The carboxy terminus of Hsc70 provides a binding site for Hsp40. It has been shown that the carboxy-terminal EEVD motif of Hsc70 is essential for the regulation of the chaperone protein byHsp40 (9). We therefore analyzed the binding of purified Hsp40to the carboxy terminus of Hsc70, using immobilized GST-70C139and GST-70C110. Hsp40 was quantitatively retained on both fusionproteins but did not bind to a significant extent to GST alone(Fig. 4A). The data reveal the existence of a binding site forHsp40 within the carboxy-terminal domain of Hsc70. This was furthersupported when the binding of Hsp40 to GST-70C139 was performedin the presence of purified full-length Hsc70. Under these conditionsa reduced amount of Hsp40 associated with the immobilized fusionprotein, and Hsp40 was detectable in the flowthrough fraction(Fig. 4B). Apparently, full-length Hsc70 and the carboxy-terminaldomain of the chaperone protein compete in binding to Hsp40. Wealso constructed a fusion protein which comprised GST and thecarboxy-terminal domain of Hsc70 lacking the EEVD motif (GST-70C139 $Delta$ EEVD).An interaction of Hsp40 with the immobilized $Delta$ EEVD carboxy-terminaldomain of Hsc70 was not observed (Fig. 5). This is consistentwith the loss of functional cooperation between Hsp40 and Hsc70observed upon removal of the EEVD motif from full-length Hsc70(9). Furthermore, Hop was unable to bind to the truncated carboxy-terminaldomain of Hsc70 (Fig. 5).

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FIG. 4. In vitro binding assays with immobilized GST or GST fusion proteins comprising carboxy-terminal fragments of Hsc70 and purified Hsp40. (A) Immobilized GST, GST-70C139, and GST-70C110 were incubated with purified Hsp40. Binding and elution conditions were as described in the legend of Fig. 2. Hsp40 was detected with a polyclonal anti-Hsp40 antibody after immunoblotting. (B) Binding of Hsp40 to GST-70C139 was performed in the absence ( $-$ ) of Hsc70 or in the presence (+) of equimolar amounts of Hsc70 and the GST fusion protein, and Hsp40 was detected in the flowthrough fractions by Coomassie blue staining.

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FIG. 5. In vitro binding assays with an immobilized GST fusion protein comprising the 70C139 carboxy-terminal domain of Hsc70 lacking the EEVD motif (GST-70C139 $Delta$ EEVD). The binding of Hop and Hsp40 and subsequent elution was performed as described in the legends of Fig. 2 and 4.

Hop and Hsp40 interact with Hsc70's carboxy terminus in a noncompetitive manner. Since Hsp40 and Hop both interact with the carboxy terminus of Hsc70, we asked whether the two cofactors compete in bindingto Hsc70. To answer this question, the binding of Hop to immobilizedGST-70C139 was analyzed in the presence of increasing concentrationsof Hsp40 (Fig. 6). GST-70C139 was incubated with saturating amountsof Hop and different amounts of Hsp40. Remarkably, even in thepresence of a sixfold molar excess of Hsp40 over Hop, the amountof Hop associated with the carboxy terminus of Hsc70 was not significantlyreduced. In this situation GST-70C139 was already saturated withHsp40, as indicated by the detection of Hsp40 in the flowthroughfraction (Fig. 6). Moreover, under saturating conditions equimolaramounts of Hsp40 and Hop were found associated with the immobilizedcarboxy-terminal domain of Hsc70. It thus appears that Hop andHsp40 interact with the carboxy terminus of the chaperone moleculein a noncompetitive manner.

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FIG. 6. Interaction of purified Hop with immobilized GST-70C139 in the presence of different concentrations of Hsp40. Immobilized GST-70C139 was incubated with 0.67 µM Hop and with different concentrations of Hsp40 as indicated. After incubation for 2 h at 4°C, the flowthrough fraction was collected (free), the resin was washed five times, and bound protein was eluted by addition of 100 mM glutathione (bound). Proteins were detected by Coomassie blue staining (free Hsp40 and bound Hop) and by immunoblotting (bound Hsp40) after SDS-PAGE analysis.

Hop does not affect the regulation of Hsc70 by Hsp40. Chaperone cofactors are involved in the regulation of Hsc70's ATPase activity and thus modulate the affinity of the chaperonefor polypeptide substrates (12, 15, 26). However, it appearsthat Hop does not participate in the regulation of the Hsc70 ATPasecycle. When Hsc70 was coincubated with an equimolar amount ofHop, the cofactor did not alter the steady-state rate of ATP hydrolysisby Hsc70 (Fig. 7). In contrast, addition of Hsp40 led to an ~7-foldstimulation of Hsc70's ATPase activity. Again, the Hsp40-mediatedstimulation was not affected by further addition of Hop (Fig.7). Even at a 25-fold molar excess of Hop over Hsp40, Hop didnot inhibit the regulation of Hsc70 by Hsp40 (data not shown).These data are consistent with the previous notion that Hop actsas a structural component mediating Hsc70-Hsp90 cooperation (4-6).Notably, the functional assays were performed under conditionsthat allowed Hop to interact with Hsc70 (Fig. 3). It thus appearsthat the binding of Hop to Hsc70 does not interfere with the functionalcooperation of Hsc70 with Hsp40. The existence of nonoverlappingbinding sites for Hop and Hsp40 apparently enables Hsc70 to interactsimultaneously with both cofactors.

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FIG. 7. Steady-state ATP-hydrolytic activity of Hsc70 in the presence of Hsp40 and Hop. Hsc70 (3 µM) was incubated at 30°C with Hsp40 (1.5 µM) and Hop (3 µM) as indicated (+, present; $-$ , absent), and the rates of ATP hydrolysis were determined. The bars represent averages of values (plus standard deviations) from four independent experiments, with six samples taken during the linear course of the reaction in each experiment.

	DISCUSSION

Top Abstract Introduction Materials & Methods Results Discussion References

In this study we show that the 10-kDa carboxy-terminal domain of Hsc70 provides binding sites for a distinct set of cofactors,i.e., Hsp40 (Hdj-1) and Hop (p60/Sti1). The carboxy-terminal domaincomprises a tightly folded $alpha$ -helical subdomain (residues 537 to606 of rat Hsc70), multiple degenerate repeats of the tetrapeptideGGMP of unknown function (residues 613 to 640), and the EEVD motifat the extreme carboxy terminus (Fig. 8). Determination of thecrystal structure of the peptide binding domain of the bacterialHsp70 homolog DnaK revealed that the $alpha$ -helical subdomain is notdirectly involved in peptide recognition (34). A peptide substrateis bound by the chaperone protein via a channel formed by twosheets of four antiparallel $beta$ strands that are connected by extendedloop structures (Fig. 8) (26, 34). The $alpha$ -helical subdomaindoes not directly contact the peptide but apparently forms a lidover the peptide binding site. Through a latch-like mechanism,the subdomain may regulate the access of a substrate to the peptidebinding pocket (26, 34). Secondary structure predictions andstructural data obtained for rat Hsc70 indicate that the overalltertiary structures of the peptide binding site and the $alpha$ -helicalsubdomain are largely conserved (3, 34). Still, the $alpha$ -helicalsubdomain is less conserved on the amino acid level than the ATPasedomain and the peptide binding pocket (3, 34). Furthermore,cytosolic eukaryotic Hsp70s possess GGMP repeats and the EEVDmotif at the carboxy terminus whereas other Hsp70 family memberslack such structural elements (3, 9). Thus, it appears thatthe carboxy terminus of the chaperone molecule is a rather variabledomain which may determine the functional specificity of individualHsp70s. This notion is supported by recent studies on cytosolicHsp70s of the yeast S. cerevisiae (19). The exchange of thevariable carboxy-terminal domains between distinct Hsp70s wasfound to alter the functional specificities of the resultant chimeras.In this regard, it is intriguing that the carboxy terminus ofHsc70 provides binding sites for the chaperone cofactors Hop andHsp40 (Fig. 1, 2, and 4). Apparently, the recruitment of a distinctset of cofactors mediated by the carboxy-terminal domain participatesin establishing the specific functions of individual Hsp70 familymembers.

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FIG. 8. (A) Schematic representation of the peptide binding region of bacterial Hsp70. The peptide binding site is formed by two sheets of four antiparallel $beta$ -strands (thick arrows) connected by extended loops. The $beta$ sandwich is followed by five $alpha$ helices (open bars) that appear to form a lid over the peptide binding site. Together, the carboxy-terminal half of the second helix and helices 3 to 5 form a tightly folded subdomain. The carboxy-terminal deletion fragments of Hsc70 used in this study start at positions 508 and 537 at the junction between the peptide binding site and the carboxy terminus (arrows). The numbers indicate the corresponding residues of rat Hsc70. The schematic representation does not include the GGMP repeats and the extreme carboxy terminus of Hsc70. (B) Multiple degenerate repeats of the tetrapeptide GGMP and the EEVD motif (underlined) are found at the carboxy terminus of eukaryotic cytosolic members of the Hsp70 protein family. The numbers indicate residues of rat Hsc70. (C) Domains of Hsc70 mediating interactions with chaperone cofactors. While Hip and BAG-1 bind to the ATPase domain of Hsc70 (amino acids 1 to 383) in a mutually exclusive manner, Hsp40 and Hop recognize distinct binding sites within the carboxy terminus of the chaperone protein (amino acids 537 to 646). bdg., binding.

While our data reveal an Hsp40 binding site within the carboxy-terminal domain of Hsc70, the existence of an additional bindingsite for the cofactor cannot be excluded. A second binding sitefor Hsp40 may be jointly formed by the peptide binding domainand the ATPase domain of Hsc70, similar to the recently proposedbinding site on Hsc70 for the Hsp40-related auxilin (32). Infact, we observed that the ATPase activity of the chymotryptic60-kDa fragment of Hsc70, which lacks the carboxy terminus, canstill be stimulated 2.5-fold by the addition of Hsp40 (data notshown). Remarkably, however, a deletion mutant of Hsc70 lackingthe carboxy-terminal EEVD motif is no longer regulated by Hsp40(9). Since deletion of the EEVD motif abolishes the bindingof Hsp40 to the carboxy-terminal domain of Hsc70 (Fig. 5), cooperationof Hsc70 with Hsp40 may require an initial interaction of thecofactor with Hsc70's carboxy terminus to gain access to a secondbinding site for Hsp40. In the 60-kDa fragment, such a bindingsite for Hsp40 may be permanently exposed. It remains to be seenwhether the EEVD motif directly mediates the interaction betweenHsp40 and Hsc70. Alternatively, the motif could be important forthe correct folding of the carboxy-terminal domain of Hsc70. Notably,the interaction of Hop with the carboxy terminus of Hsc70 is alsoabolished by a deletion of the EEVD motif, but it is similarlyaffected when the $alpha$ -helical subdomain is removed. This may indicatethat the $alpha$ -helical subdomain, the GGMP repeats, and the EEVD motiftogether form a structural entity mediating cofactor binding.

Remarkably, Hsp40 and Hop did not compete in binding to the carboxy terminus of Hsc70 (Fig. 6). Nonoverlapping binding siteshave apparently evolved for both cofactors within the carboxy-terminaldomain. This may allow Hsp40 to cooperate functionally with Hsc70even when the chaperone interacts with Hop. In fact, the presenceof Hop did not affect the stimulation of Hsc70's ATPase activityby Hsp40 (Fig. 7) and Hop did not interfere with the cooperationof Hsc70 and Hsp40 during in vitro refolding of denatured $beta$ -galactosidase(10) and firefly luciferase (data not shown). Notably, Hop haspreviously been purified from rabbit reticulocyte lysate duringan attempt to identify a factor that promotes the recycling ofHsc70 (13, 14). This factor stimulated the release of ADPfrom Hsc70 through an interaction with the ATPase domain of thechaperone protein. In light of the data presented here, it appearsunlikely that Hop fulfills such a function in the Hsc70 reactioncycle. Hop did not alter the ATPase activity of Hsc70, eitheralone or when coincubated with Hsp40 (Fig. 7), and Hop did notinteract with Hsc70's ATPase domain in the two-hybrid assay (Fig.1) and biochemical binding assays (data not shown). We would thereforeconclude that Hop acts primarily as a structural component thatpromotes the cooperation of Hsc70 with Hsp90.

Analysis of the Hsc70-Hsp90-mediated activation of steroid hormone receptors emphasizes the importance of the interactionof Hsc70 with cofactors such as Hsp40, Hip, and Hop (2, 30).The progesterone receptor, for example, enters its activationpathway through an initial recognition by Hsc70, which apparentlycooperates with Hsp40 at this stage (12, 25, 30). Cooperationof Hsc70 with Hsp40 also stimulates the association of the chaperonewith Hip (17). Conceivably, a transient complex may form thatcomprises both cofactors bound to the Hsc70-receptor complex viatheir distinct binding sites on Hsc70. In fact, the retentionof Hsp40 on immobilized Hip was recently observed when it wascoincubated with Hsc70 (17). This demonstrates that Hsc70 caninteract simultaneously with Hip and Hsp40. Further activationof the progesterone receptor requires the recruitment of Hsp90to the chaperone-receptor complex. Recruitment of Hsp90 appearsto be promoted by a Hip-mediated stabilization of the interactionof Hsc70 with the receptor molecule and by the action of the Hopprotein. Hop is able to bind to Hsc70 and Hsp90, and may thusmediate the coupling of the chaperone proteins (4, 6). Atthis stage a simultaneous interaction of Hop and Hip with Hsc70may be essential for the efficient cooperation of Hsc70 with Hsp90.An Hsc70-Hsp90 chaperone complex containing Hip and Hop has infact been identified as an intermediate complex during receptoractivation (30). Moreover, in immunoprecipitation experimentsHop was coprecipitated with Hsc70 when a Hip-specific antibodywas used (25). The identification of distinct binding sitesfor Hip and Hop now provides us with the structural basis forthe simultaneous interaction of Hsc70 with both cofactors.

The recent characterization of the BAG-1 protein as a binding partner of Hsc70 revealed that competition between distinctcofactors offers additional means for Hsc70 regulation (16,31, 33). While BAG-1 cooperates with Hsp40 to efficientlystimulate the ATPase activity of Hsc70, it competes with Hip inbinding to Hsc70's ATPase domain (16). Hence, a network of competingand cooperating cofactors appears to modulate the chaperone activityof Hsc70 in the mammalian cell.

	ACKNOWLEDGMENTS

We thank Jorgos Pyrowolakis for construction of plasmid pAD, Stefan Jentsch for helpful discussions, and Helle Ulrich andJoachim Rassow for critical reading of the manuscript.

This work was supported by grants from the Deutsche Forschungsgemeinschaft (HO 1518/2-1 and HO 1518/2-2).

	FOOTNOTES

^* Corresponding author. Mailing address: ZMBH, Zentrum für Molekulare Biologie, Universität Heidelberg, Im Neuenheimer Feld282, D-69120 Heidelberg, Germany. Phone: 49 6221 546837. Fax:49 6221 545891. E-mail: j-hoehfeld{at}sun0.urz.uni-heidelberg.de.

REFERENCES

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Abstract
Introduction
Materials & Methods
Results
Discussion
References

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1.	Ausubel, F. J., R. Brent, R. E. Kingston, D. D. Moore, J. G. Seidman, J. A. Smith, and K. Struhl. 1989. . Current protocols in molecular biology. Greene Publishing Associates and Wiley Interscience, New York, N.Y.
2.	Bohen, S. P., and K. R. Yamamoto. 1994. Modulation of steroid receptor signal transduction by heat shock proteins, p. 313-334. In R. I. Morimoto, A. Tissieres, and C. Georgopoulos (ed.), The biology of heat shock proteins and molecular chaperones. Cold Spring Harbor Laboratory Press, Cold Spring Harbor, N.Y.
3.	Boorstein, W. R., T. Ziegelhoffer, and E. A. Craig. 1994. Molecular evolution of the HSP70 multigene family. J. Mol. Evol. 38:1-17[Medline].
4.	Chang, J. H.-C., and S. Lindquist. 1994. Conservation of Hsp90 macromolecular complexes in Saccharomyces cerevisiae. J. Biol. Chem. 269:24983-24988[Abstract/Free Full Text].
5.	Chang, J. H.-C., D. F. Nathan, and S. Lindquist. 1997. In vivo analysis of the Hsp90 cochaperone Sti1 (p60). Mol. Cell. Biol. 17:318-325[Abstract].
6.	Chen, S., V. Prapapanich, R. A. Rimerman, B. Honore, and D. F. Smith. 1996. Interactions of p60, a mediator of progesterone receptor assembly, with heat shock proteins Hsp90 and Hsp70. Mol. Endocrinol. 10:682-693[Abstract].
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