A foldable CFTR{Delta}F508 biogenic intermediate accumulates upon inhibition of the Hsc70-CHIP E3 ubiquitin ligase

doi:10.1083/jcb.200410065

Published 20 December 2004. doi:10.1083/jcb.200410065
The Rockefeller University Press, 0021-9525 $8.00
JCB, Volume 167, Number 6, 1075-1085

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Article

A foldable CFTR ${Delta}$ F508 biogenic intermediate accumulates upon inhibition of the Hsc70–CHIP E3 ubiquitin ligase

J. Michael Younger¹^,2, Hong-Yu Ren¹^,2, Liling Chen¹^,2, Chun-Yang Fan¹^,2, Andrea Fields¹^,2, Cam Patterson¹, and Douglas M. Cyr¹^,2

¹ Department of Cell and Developmental Biology, School of Medicine, University of North Carolina, Chapel Hill, NC 27599
² The Cystic Fibrosis Center, School of Medicine, University of North Carolina, Chapel Hill, NC 27599

Correspondence to D.M. Cyr: dmcyr{at}med.unc.edu

Abstract

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Abstract
Introduction
Results
Discussion
Materials and methods
References

CFTR ${Delta}$ F508 exhibits a correctable protein-folding defect thatleads to its misfolding and premature degradation, which isthe cause of cystic fibrosis (CF). Herein we report on the characterizationof the CFTR ${Delta}$ F508 biogenic intermediate that is selected for proteasomaldegradation and identification of cellular components that polyubiquitinateCFTR ${Delta}$ F508. Nonubiquitinated CFTR ${Delta}$ F508 accumulates in a kineticallytrapped, but folding competent conformation, that is maintainedin a soluble state by cytosolic Hsc70. Ubiquitination of Hsc70-boundCFTR ${Delta}$ F508 requires CHIP, a U box containing cytosolic cochaperone.CHIP is demonstrated to function as a scaffold that nucleatesthe formation of a multisubunit E3 ubiquitin ligase whose reconstitutedactivity toward CFTR is dependent upon Hdj2, Hsc70, and theE2 UbcH5a. Inactivation of the Hsc70–CHIP E3 leads CFTR ${Delta}$ F508to accumulate in a nonaggregated state, which upon loweringof cell growth temperatures, can fold and reach the cell surface.Inhibition of CFTR ${Delta}$ F508 ubiquitination can increase its cellsurface expression and may provide an approach to treat CF.

Abbreviations used in this paper: ApoB48, apolipoprotein B48;BFA, brefeldin A; CF, cystic fibrosis; ERQC, endoplasmic reticulumquality control system; NBD, nucleotide binding domain; TCR ${alpha}$ ,T cell receptor ${alpha}$ subunit; TPR, tetratricopeptide repeat motifs.

Introduction

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Abstract
Introduction
Results
Discussion
Materials and methods
References

CFTR is a Cl^– ion channel that is localized to the apicalsurface of epithelial cells that line lung airways and glands(Riordan et al., 1989). Cystic fibrosis (CF) is an autosomalrecessive disease and most CF patients inherit at least oneCFTR ${Delta}$ F508 mutant allele. CFTR ${Delta}$ F508 lacks F508 in nucleotide bindingdomain (NBD) I and has a temperature-sensitive folding defect,which causes its premature degradation by the ubiquitin proteasomesystem (Denning et al., 1992; Jensen et al., 1995a; Ward et al., 1995).Loss of CFTR function at the cell surface leadsto mortality in CF patients because of altered hydration ofairway epithelia and persistent lung infections (Welsh and Smith, 1993).

An interesting feature of CFTR ${Delta}$ F508 is that when growth conditionsare altered, it can fold, escape the endoplasmic reticulum qualitycontrol system (ERQC), and function at the cell surface (Denning et al., 1992;Brown et al., 1996). Thus, the development ofagents that promote the folding or block the degradation ofnascent CFTR ${Delta}$ F508 has the potential to provide a therapeuticavenue for the treatment of CF. Rational design of such therapeuticsrequires a basic understanding of the mechanism for CFTR ${Delta}$ F508misfolding and the identification of the ERQC machinery thatselects CFTR ${Delta}$ F508 for degradation.

CFTR is a 1,480 residue glycomembrane protein whose proper functionrequires the formation of intramolecular contacts between itstwo transmembrane domains, two cytoplasmic NBDs, and a regulatorydomain (R-domain; Xiong et al., 1997). CFTR and CFTR ${Delta}$ F508 biogenesisis inefficient with 60–75% of CFTR and nearly 99% of CFTR ${Delta}$ F508being degraded before reaching the cell surface (Ward and Kopito, 1994).Thus, the kinetics of CFTR and CFTR ${Delta}$ F508 folding are slowand nonnative biogenic intermediates of each appear to be activelyselected for degradation by ERQC systems. The nature of theCFTR ${Delta}$ F508 biogenic intermediate that is selected for degradationis unknown, but CFTR and CFTR ${Delta}$ F508 appear to assume similar conformationsat early stages of assembly (Zhang et al., 1998). Because F508is located on the surface of NBD1, CFTR ${Delta}$ F508 assembly is proposedto go off pathway at a late stage (Lewis et al., 2004). Theinability of CFTR ${Delta}$ F508 to fold properly makes it prone to aggregation(Qu and Thomas, 1996) and causes some of its degradation intermediatesto accumulate in detergent-insoluble aggregates (Ward et al., 1995).

The mechanism by which the cell monitors the conformationalstate of CFTR ${Delta}$ F508 and makes protein triage decisions that determineits fate are unclear. Current models suggest that the foldedstate of CFTR and CFTR ${Delta}$ F508 is surveyed by the cytosolic chaperoneHsc70 and Hsp90 (Yang et al., 1993; Loo et al., 1998; Zhang et al., 2001).The ER luminal lectin-binding chaperone calnexincan form a complex with the immaturely glycosylated B form ofCFTR ${Delta}$ F508, but a direct role for calnexin in CFTR folding and/ordegradation has not been demonstrated (Pind et al., 1994; Okiyoneda et al., 2004).

Cytosolic Hsc70 functions in complexes with either folding ordegradatory cochaperones to mediate steps in CFTR folding anddegradation (Cyr et al., 2002). The type I Hsp40 cochaperoneHdj-2 is farnesylated and localized to the cytoplasmic faceof the ER where it recruits Hsc70 to bind ribosome associatedCFTR to promote early stages of its assembly (Meacham et al., 1999).Hsc70 can also interact with the degradatory cochaperoneCHIP to facilitate the proteasomal degradation of ER forms ofCFTR and CFTR ${Delta}$ F508 (Meacham et al., 2001). Thus, cochaperonesof Hsc70 play a central role in determining the fate of nascentCFTR.

Mechanistic insight into how CHIP functions as a degradatorycochaperone is now required to understand how the cell makesprotein triage decisions for CFTR ${Delta}$ F508. CHIP contains three NH₂-terminaltetratricopeptide repeat motifs (TPR) that bind the COOH terminusof Hsc70 (Scheufler et al., 2000) and a noncanonical RING domain,termed the U box, which promotes interactions with E2 enzymes(Ballinger et al., 1999). The TPR repeat motifs and U box areessential for CHIP to mediate CFTR and CFTR ${Delta}$ F508 degradation(Meacham et al., 2001). Thus, CHIP is proposed to interact withHsc70 to form an E3 ubiquitin ligase that targets CFTR ${Delta}$ F508 forproteasomal degradation. However, CHIP can function in a U boxindependent manner to alter the Hsc70 polypeptide binding andrelease cycle and negatively influence the folding of some clientproteins (Ballinger et al., 1999; Dai et al., 2003). Thus, itis plausible that CHIP targets CFTR and CFTR ${Delta}$ F508 for degradationby acting as an antifolding factor.

Herein, we reconstituted CFTR ubiquitination with purified componentsand demonstrated that Hsc70 and CHIP functionally interact withthe E2 UbcH5a to form a multisubunit E3 ubiquitin ligase thatpolyubiquitinates the cytosolic subdomains of CFTR. Inactivationof the Hsc70–CHIP E3 in cultured cells drove the accumulationof a nonaggregated and foldable CFTR ${Delta}$ F508 degradation intermediate.These data support a model for quality control in which aggregationof CFTR ${Delta}$ F508 is suppressed by Hsc70 and Hdj-2. However, whenCFTR ${Delta}$ F508 folding intermediates become kinetically trapped ina nonnative state, CHIP attracts UbcH5a to Hsc70–CFTR ${Delta}$ F508complexes and thereby facilitates CFTR ${Delta}$ F508 ubiquitination anddegradation.

Results

Top
Abstract
Introduction
Results
Discussion
Materials and methods
References

Purified CHIP functions as an Hdj-2–, Hsc70-, and UbcH5a-dependent E3 ubiquitin ligase to polyubiquitinate CFTR
To investigate whether CHIP targets CFTR for degradation byacting as a U box–dependent E3 ubiquitin ligase we soughtto reconstitute CFTR ubiquitination. To accomplish this goalCHIP, Hsc70, Hdj-2, and the E2 UbcH5a were overexpressed andpurified from Escherichia coli. UbcH5a was chosen as the E2for these experiments because it cooperates with CHIP to promotepolyubiquitin chain assembly (Jiang et al., 2001). The CFTRsubstrate used for this ubiquitination reaction was gst–NBD1–R(Naren et al., 1999), which contains binding sites for Hdj-2and Hsc70 (Meacham et al., 1999).

Gst–NBD1–R was incubated with different combinationsof chaperones and ubiquitination enzymes and its ubiquitinationwas monitored by analyzing the retardation of its mobility onSDS-PAGE gels (Fig. 1 A). E1 and UbcH5a were unable to facilitatethe ubiquitination of gst–NBD1–R and the additionof CHIP lead to the formation of a small quantity of ubiquitinatedgst–NBD1–R. The presence of Hsc70 or Hdj-2 in combinationwith CHIP further stimulated the ubiquitination by UbcH5a, butthe efficiency of this reaction remained low with <3% ofgst–NBD1–R being detected as a mono-, di-, or triubiquitinatedspecies. However, >85% of gst–NBD1–R was polyubiquitinatedwhen E1, UbcH5a, Hsc70, Hdj-2, and CHIP were jointly present.Mutation of conserved residues in CHIPs U box, H260A and P269A,greatly reduced gst–NBD1–R polyubiquitination. Inaddition, mutation of K30A in the TPR repeat domain reducedCHIPs ubiquitination activity to levels observed when CHIP andHdj-2 were present, but Hsc70 was omitted (Fig. 1, A and C).CHIP cooperates with UbcH5a, Hsc70, and Hdj-2 in a TPR repeatand U box–dependent manner to facilitate CFTR polyubiquitination.

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Figure 1. Reconstitution of CFTR ubiquitination. (A) Ubiquitination of gst–NBD1–R. (B) Ubc6 and Ubc7 cannot cooperate with Hsc70 and CHIP to ubiquitinate gst–NBD1–R. (C) CHIP K30A is defective in polyubiquitination. (D) UbcH5a C85A cannot ubiquitinate Gst–NBD–R. Ubiquitination of Gst–NBD–R (1 µM) was performed at 37°C and where indicated the following components were present: UbcH5a (4 µM), UbcH5a C85A (4 µM), Ubc6 (4 µM), Ubc7 (4 µM), CHIP (3 µM), CHIP K30A (3 µM), Hsc70 (2 µM), and Hdj2 (4 µM). In 1B-D Hsc70 and Hdj-2 were in all reactions except for lane 1. Incubations in A, C, and D were for 2 h. Ubiquitination of Gst–NBD–R was determined by Western blot with ${alpha}$ -R domain antibody. In the x-ray films shown in A–D the band that corresponds to Gst–NBD–R is overexposed to allow for the visualization of its ubiquitinated forms. Quantitation of shorter exposures of these x-ray films indicates that >85% of Gst–NBD–R is polyubiquitinated by the joint action of UbcH5a, Hsc70, Hdj-2, and CHIP (A, lane 5). When Hsc70 or Hdj-2 were absent (A, lanes 2 and 3), UbcH5a and CHIP ubiquitinated <3% of Gst–NBD–R.

U box proteins function as E3 enzymes to stimulate E2 dependentpolyubiquitin chain assembly and in some cases act as E4 enzymesto elongate ubiquitin chains on monoubiquitinated proteins (Koegl et al., 1999;Cyr et al., 2002). The data presented indicatesthat CHIP acts in concert with Hsc70 and Hdj-2 as an E3 to stimulateUbcH5a ubiquitination activity. This conclusion is supportedby the observation that UbcH5a does not monoubiquitinate, andCHIP cooperates with Hsc70 and Hdj-2 to stimulate the rate atwhich UbcH5a converts gst–NBD1–R into a polyubiquitinatedspecies (Fig. S1).

To evaluate the specificity of CHIPs ubiquitination activity,its ability to cooperate with the mammalian E2s Ubc6 and Ubc7(Tiwari and Weissman, 2001; Lenk et al., 2002) to facilitategst–NBD1–R ubiquitination was examined (Fig. 1 B).Ubc6 and Ubc7 were used because these E2s mediate the ubiquitinationof ERAD substrates in cultured cells and their purified formsfunction in vitro to facilitate polyubiquitin chain assembly(Tiwari and Weissman, 2001). In reaction cocktails that containedE1, UbcH5a, Hsc70, Hdj2, and CHIP, gst–NBD1–R wasconverted to a polyubiquitinated species in time-dependent fashion(Fig. 1 B). However, after 180 min of incubation a polyubiquitinatedform of gst–NBD1–R was not detected when the purifiedE2 domain of Ubc6 or Ubc7 was substituted for UbcH5a in otherwiseidentical reaction cocktails. Thus, CHIP appears to specificallyrecognize UbcH5a.

Next, the ability of UbcH5a C85A to facilitate the polyubiquitinationof gst–NBD1–R was determined (Fig. 1 D). UbcH5aC85A is a form of UbcH5a in which its active site cysteine thataccepts a charged ubiquitin from E1 has been mutated. UbcH5aC85A is predicted to interact with the U box on CHIP, but shouldnot facilitate polyubiquitin chain assembly because it cannotbe conjugated to ubiquitin. This supposition was found to betrue as UbcH5a C85A was unable to cooperate with CHIP to promotethe polyubiquitination of gst–NBD1–R. Hence, theHsc70- and Hdj-2–dependent reconstitution of CFTR polyubiquitinationrequires the action of the CHIP TPR and U box domains and theactive site cysteine of UbcH5a.

Overexpression of UbcH5a C85A in cultured cells inhibits CFTR and CFTR ${Delta}$ F508 degradation
To access whether or not UbcH5a is an in vivo component of Hsc70–CHIPE3, the effect that UbcH5a and UbcH5a C85A overexpression inHEK293 cells had on CFTR biogenesis was determined (Fig. 2 A).In addition, we compared the effect of UbcH5a or UbcH5a C85Aoverexpression on CFTR biogenesis to that of wild-type and dominantnegative mutant forms of the human E2s Ubc6 and Ubc7 (Fig. 2A). Elevation of UbcH5a levels caused a decrease in the accumulationof the immaturely glycosylated ER localized B form and the maturelyglycosylated plasma membrane localized C form of CFTR. In contrast,overexpression of UbcH5a C85A led to a severalfold increasein the steady-state level of the B and C form of CFTR. Ubc6and Ubc6 C91S overexpression were also observed to influenceCFTR expression levels, but the effect that Ubc6 C91S had onthe accumulation of the B form of CFTR was modest when comparedwith results obtained with UbcH5a C85A. On the other hand, Ubc7and Ubc7 C89S overexpression did not cause a detectable changein the steady-state level of CFTR and CFTR ${Delta}$ F508. Because Ubc6does not appear to interact with CHIP (Fig. 1), the effect thatits overexpression has on CFTR biogenesis appears to resultfrom its ability to function with additional quality controlfactors that monitor the folded state of CFTR (Gnann et al., 2004).

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Figure 2. Degradation of CFTR and CFTR ${Delta}$ F508 is inhibited by overexpression of UbcH5A C85A. (A) Western blot analysis of CFTR levels upon overexpression of the E2s UbcH5A, Ubc6, and Ubc7. HEK293 cells were transfected transiently with expression plasmids that encode the indicated proteins. Total cell extracts were prepared 24 h after transfection in SDS-PAGE sample buffer. Nitrocellulose was probed with ${alpha}$ -CFTR and developed. The immaturely glycosylated ER localized B form and maturely glycosylated plasma membrane associated C form of CFTR are denoted as B and C, respectively. (B and C) UbcH5A C85A overexpression slows the rate of CFTR and CFTR ${Delta}$ F508 degradation. Cells were labeled for 20 min with ³⁵S-translabel and a chase period was initiated by the addition of cycloheximide. At the indicated times, ³⁵S-CFTR or ³⁵S-CFTR ${Delta}$ F508 was immunoprecipitated from cell extracts. CFTR or CFTR ${Delta}$ F508 isolated in this manner was detected by SDS-PAGE and fluorography. (D and E) Graphs illustrate the processing efficiency and half-life of CFTR and CFTR ${Delta}$ F508. Relative CFTR and CFTR ${Delta}$ F508 levels were quantitated by laser densitometry of the x-ray films shown in B and C, respectively. Values were normalized to the quantity of the B form of CFTR and CFTR ${Delta}$ F508 present at t = 0 under the indicated experimental condition levels. t = 0 values for the B form of CFTR were 1.1 and 1.8 OD, in the absence and presence of UbcH5a C85A, respectively. t = 0 values for the B form of CFTR ${Delta}$ F508 were 2.3 and 7.0 OD, in the absence and presence of UbcH5a C85A, respectively. (F) CHIP and UbcH5a jointly reduce levels of CFTR ${Delta}$ F508 in Western blots.

To explore the reason why overexpression of UbcH5a C85A drovethe B form of CFTR to accumulate, its effect on the kineticsof CFTR and CFTR ${Delta}$ F508 degradation was determined (Fig. 2, B and C).In pulse-chase experiments, UbcH5a C85A overexpression increasedthe quantity of the B form of CFTR and CFTR ${Delta}$ F508 present at thebeginning of the chase period $~$ 1.5–3-fold (Fig. 2, legend).The UbcH5a C85A induced increase in CFTR and CFTR ${Delta}$ F508 levelsappeared to result from the impaired degradation of nascentCFTR and CFTR ${Delta}$ 508 because the half-life of the B form of eachwas increased two to threefold (Fig. 2, D and E). In addition,the maturation efficiency of CFTR in the presence or absenceof UbcH5a C85A was around 25% (Fig. 2 D). Thus, inhibition ofthe Hsc70–CHIP E3 complex via UbcH5a C85A overexpressioninhibits CFTR degradation, but does not interfere with CFTRfolding efficiency.

To gain additional support for the interpretation that CHIPand UbcH5a interact with each other to select nascent CFTR andCFTR ${Delta}$ F508 for degradation we demonstrated that the coexpressionof CHIP and UbcH5a enhanced the effect that individual formsof each had on CFTR ${Delta}$ F508 degradation (Fig. 2 D). When CHIP orUbcH5a was overexpressed alone, steady-state levels of CFTR ${Delta}$ F508were reduced to 30 and 41% of control levels, respectively.Yet, when CHIP and UbcH5a were coexpressed, CFTR ${Delta}$ F508 accumulationwas reduced by >98%.

Overexpression of Ubch5a C85A does not generally inhibit ERAD
To ascertain whether or not UbcH5a C85A overexpression generallyinhibited ERAD or specifically blocked CFTR degradation, itseffect on the degradation of the T cell receptor ${alpha}$ subunit (TCR ${alpha}$ )was examined (Fig. 3 A). TCR ${alpha}$ is a transmembrane protein thatexposes a large extracellular domain in the ER lumen whose unassembledform is degraded via an ERAD pathway that uses the E2s Ubc6and Ubc7 (Tiwari and Weissman, 2001; Lenk et al., 2002). Pulsechase analysis revealed that TCR ${alpha}$ had a half-life of around 1h in absence or presence of UbcH5a C85A (Fig. 3, A and C). Inaddition, the overexpression of CHIP was not observed to influencethe rate of TCR ${alpha}$ turnover (unpublished data). In contrast, overexpressionof either Ubc6 C91S or Ubc7 C89S led to an increase in the half-lifeof TCR ${alpha}$ from 1 h to 1.5 and 2 h, respectively. Thus, UbcH5a C85Aoverexpression does not detectably hinder the turnover of atransmembrane ERAD substrate whose degradation can be blockedby interference with the action of Ubc6 and Ubc7.

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Figure 3. Insensitivity of TCR ${alpha}$ and ApoB48 turnover to inhibition of the Hsc70–CHIP E3. (A) TCR ${alpha}$ degradation. (B) ApoB48 turnover. HEK293 cells were transiently transfected with expression plasmids for the indicated proteins. 24 h after transfection, cells were labeled for 20 min with ³⁵S-translabel. A chase period was initiated by the addition of cycloheximide and, at the indicated times, cells were harvested and lysed. TCR ${alpha}$ or ApoB48 were immunoprecipitated from cell extracts and detected by SDS-PAGE and autoradiography. (C) Quantitation of TCR ${alpha}$ and Apob48 levels, the relative amount of each protein present at t = 0 is expressed as 100% of control.

Because the membrane topology of TCR ${alpha}$ differs from that of CFTR,we also examined the sensitivity of apolipoprotein B48 (ApoB48)degradation to overexpression of UbcH5a C85A. ApoB48 is a 2,15–aminoacid residue secretory protein whose nascent form has featuresthat are similar to CFTR because it exposes surfaces in theER lumen and cytosol, and is a substrate of cytosolic Hsp70and Hsp90 (Gusarova et al., 2001). ApoB48 folding and exit fromthe ER requires its assembly into complexes with lipids, andunassembled forms are degraded via a pathway that involves thetransmembrane E3 Gp78, which can interact with Ubc7 (Cyr et al., 2002;Liang et al., 2003). The overexpression of CHIP doesnot accelerate Apob48 degradation (Meacham et al., 2001). Likewise,the overexpression of UbcH5a C85A does not have a detectableeffect on the rate of ApoB48 degradation (Fig. 3, B and C).Thus, the overexpression of UbcH5 C85A does not generally inhibitthe function the cellular quality control machinery.

A detergent-soluble CFTR ${Delta}$ F508 degradation intermediate accumulates upon inactivation of the Hsc70–CHIP E3 complex
CFTR and CFTR ${Delta}$ F508 biogenic intermediates appear to be aggregationprone and therefore are selected for ubiquitination and proteasomaldegradation. When the proteasome is inhibited, polyubiquitinatedCFTR ${Delta}$ F508 accumulates in detergent-insoluble aggregates (Ward et al., 1995),but nonubiquitinated CFTR ${Delta}$ F508 biogenic intermediatesare not well characterized. To investigate the aggregation stateof nonubiquitinated CFTR ${Delta}$ F508, we modulated the activity of theHsc70–CHIP E3 and determined the detergent solubilityof the CFTR and CFTR ${Delta}$ F508 biogenic intermediates that accumulated(Fig. 4). Overexpression of UbcH5a and CHIP caused an overalldecrease in the pool of CFTR and CFTR ${Delta}$ F508 and none of the Bform was detected in the Triton X-100–insoluble fraction.When UbcH5a C85A was overexpressed, severalfold more of theB and C form of CFTR accumulated in the Triton X-100–solublefraction. To our surprise, we also observed UbcH5a C85A overexpressionto drive a severalfold increase in the quantity of the B formof CFTR ${Delta}$ F508 that accumulated in a Triton X-100–solublestate. Under these experimental conditions, we also observeda small quantity of the C form of CFTR in the detergent-insolublefraction. Because the C form of CFTR is typically soluble inTriton X-100, this material appears to represent a minor contaminationof the detergent-insoluble fraction with detergent soluble material.

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Figure 4. Triton X-100–soluble CFTR and CFTR ${Delta}$ F508 degradation intermediates accumulate in response to overexpression of UbcH5a C85A. (A and B) Analysis of the solubility of CFTR or CFTR ${Delta}$ F508. HEK293 were transiently tranfected with vectors that express the indicated proteins. As indicated, the proteasome inhibitor ALLN (200 µM) was added to the growth medium 4 h preceding cell lysis. (C) Coexpression of CHIP and UbcH5a C85A blocks CFTR folding and causes its biogenic intermediates to aggregate. CFTR and CFTR ${Delta}$ F508 were detected by Western blot. The fractionation of cell extracts into Triton X-100–soluble and –insoluble material was performed as described in the Materials and methods. The upper panel represents Triton X-100–soluble material, where as the lower part represents Triton X-100–insoluble material. The immaturely glycosylated B form of CFTR and CFTR ${Delta}$ F508, and maturely glycosylated C form of CFTR are denoted.

Paradoxically, we observed markedly different results when theaction of the Hsc70–CHIP E3 was blocked via overexpressionof CHIP P269A. CHIP P269A inhibited degradation of the B formof CFTR and CFTR ${Delta}$ F508, but the degradation intermediate thataccumulated was insoluble in Triton X-100 (Fig. 4, A and B).In addition, CHIP P269A blocked the glycolytic maturation ofCFTR from the B to C form. The effect that CHIP and CHIP P269Ahad on CFTR and CFTR ${Delta}$ F508 biogenesis was resultant from interactionswith Hsc70 because the TPR mutant CHIP K30A had no effect onCFTR biogenesis (Fig. 4).

How do we explain the observation that the overexpression ofUbcH5a C85A and CHIP P269A block CFTR degradation, but yet causethe degradation intermediates that accumulate to exhibit differentialdetergent solubility? CHIP P269A blocks the glycolytic maturationof CFTR, and thus retains the ability of CHIP to interact withHsc70 to arrest CFTR folding (Meacham et al., 2001). Therefore,because CHIP P269A can hinder Hsc70s protein folding function,but can't promote CFTR degradation, it causes nonnative CFTRto aggregate. In HEK293 cells CHIP levels are normally 10-foldlower than those for Hsc70 (Meacham et al., 2001). Hence, whenUbcH5a C85A is overexpressed the levels of CHIP–UbcH5aC85A complexes that form should not be more than one-tenth thelevel of Hsc70. Ergo, the overexpression of UbcH5a C85A canblock CFTR degradation, but the levels of CHIP–UbcH5aC85A complexes are not high enough to interfere with Hsc70sability to suppress CFTR aggregation. Therefore, UbcH5a C85Adrives the accumulation of a CFTR ${Delta}$ F508 degradation intermediatethat is stabilized in a nonaggregated state.

If the aforementioned interpretations are correct and UbcH5aC85A specifically inactivates the U box of CHIP to block CFTRdegradation, then the coexpression of UbcH5a C85A and CHIP,should have the same effect on CFTR biogenesis as CHIP P269A.Indeed, we observed that the simultaneous overexpression ofCHIP and UbcH5a C85A blocked the glycolytic maturation and degradationof CFTR and drove the B form of CFTR to accumulate as a detergent-insolubleaggregate (Fig. 4 D, lane 1 vs 5).

The data presented in Fig. 4 are important for the followingreasons. First, these data indicate that interference with Hsc70–CHIPE3 activity drives the accumulation of a novel nonaggregatedCFTR ${Delta}$ F508 biogenic intermediate. Second, these data demonstratethat proper chaperone function of Hsc70 is critically importantfor maintenance of nonnative CFTR and CFTR ${Delta}$ F508 in a detergentsoluble state. Third, the observation that UbcH5a C85A and CHIPcoexpression makes CHIP behave like CHIP P269A supports theinterpretation that CHIP and UbcH5a functionally interact invivo to ubiquitinate CFTR.

Characterization of the nonaggregated CFTR ${Delta}$ F508 degradation intermediate
To investigate the nature of the detergent-soluble CFTR ${Delta}$ F508degradation intermediate that accumulated when UbcH5a C85A wasoverexpressed, we compared its ubiquitination state to thatof degradation intermediates that accumulate in response toproteasome inhibition by ALLN, or overexpression of a dominantnegative form of p97 (p97 QQ; Ye et al., 2003). P97 is a cytosolicchaperone that extracts polyubiquitinated proteins from theER and participates in CFTR ${Delta}$ F508 degradation (Ye et al., 2003;Dalal et al., 2004). Nonubiquitinated CFTR ${Delta}$ F508 migrates on SDS-PAGEgels with the same mobility as its B form, where as polyubiquitinatedCFTR ${Delta}$ F508, which accumulated when its degradation was blockedby ALLN or p97 QQ, migrates on SDS-PAGE gels as a high molecularweight smear (Fig. 5 A). CFTR ${Delta}$ F508 that accumulated in responseto UbcH5a C85A overexpression did not migrate as a high molecularsmear and, therefore, represents a nonubiquitinated species.This result is consistent with the notion that UbcH5a C85A inhibitsCFTR ${Delta}$ F508 ubiquitination and thereby blocks its degradation.

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Figure 5. Characterization of the CFTR ${Delta}$ F508 biogenic intermediate that accumulates when UbcH5a C85A is overexpressed. (A) Analysis of CFTR ${Delta}$ 508 levels when its proteasomal degradation is inhibited by different methods. HEK293 cells were transfected with the indicated expression vectors and harvested in SDS sample buffer 24 h later. ALLN (200 µM) was added to culture media 4 h before cell harvest. CFTR ${Delta}$ F508 levels were determined by Western blot. Ubiquitinated CFTR ${Delta}$ F508 runs as a high molecular smear on SDS-PAGE gels and is denoted. (B) Complex formation between Hsc70 and CFTR ${Delta}$ F508. Cells were transfected with the indicated expression plasmids and 24 h after incubation they were radiolabeled for 30 min with ³⁵S-translabel and harvested. Half of each cell pellet was lysed under denaturing or native buffer conditions and immunoprecipitations were performed and analyzed by fluorography. (C) CFTR ${Delta}$ F508 that accumulates in the presence of UbcH5a C85A is glycosylated. Cells were harvested and half of each respective lysate was treated with endoglycosidase H whereas the other half served as the control. A and B denote the mobility of nonglycosylated and immaturely glycosylated forms of CFTR ${Delta}$ F508, respectively.

Next, we examined the effect that modulating Hsc70–CHIPE3 action had on complex formation between Hsc70 and CFTR ${Delta}$ F508degradation intermediates (Fig. 5 B). This was accomplishedby coimmunoprecipitating Hsc70–CFTR ${Delta}$ F508 complexes with ${alpha}$ -Hsc70 antibody from radiolabeled cells that were transfectedwith the indicated form of UbcH5a or CHIP. Overexpression ofUbcH5a or CHIP reduced the levels of immunoprecipitable CFTR ${Delta}$ F508,whereas UbcH5a C85A overexpression caused CFTR ${Delta}$ F508 to accumulateseveral fold. On the other hand, CHIP P269A, which inhibitsCFTR degradation and caused CFTR ${Delta}$ F508 to aggregate (Fig. 4),reduced the total amount of CFTR ${Delta}$ 508 that could be immunoprecipitatedfrom cell extracts. The newly synthesized pool of Hsc70 detectedby immunoprecipitation was not significantly changed when thelevels of the components of the Hsc70–CHIP–UbcH5aE3 complex were altered. Yet, we did observe that the levelsof Hsc70–CFTR ${Delta}$ F508 complexes were lower when UbcH5a andCHIP were overexpressed, and were elevated when UbcH5a C85Awas overexpressed. Nonetheless, under all of the aforementionedexperimental conditions tested, the changes in the levels ofHsc70–CFTR ${Delta}$ F508 complexes appeared proportional to changesin the total amount of immunoprecipitable CFTR ${Delta}$ F508 present inthe cell extracts. The major conclusion drawn from these resultsis that the detergent soluble CFTR ${Delta}$ F508 degradation intermediatethat accumulates upon UbcH5a C85A overexpression is associatedwith Hsc70.

Data presented thus far suggest that inhibition of Hsc70–CHIPE3 activity drives the accumulation of an ER membrane insertedCFTR ${Delta}$ F508 biogenic intermediate that is arrested at a biogenicstage where it has the potential to either fold or be degraded.If this is the case then the CFTR ${Delta}$ F508 that accumulates in responseto UbcH5a C85A overexpression should be glycosylated. Indeed,we observed that the gel mobility of the CFTR ${Delta}$ F508 that accumulatesin response to UbcH5a C85A overexpression was increased whentotal cell extracts were treated with endoglycosidase H, whichremoves ASN-linked glycans from glycoproteins (Fig. 5 C). Thus,inhibition of the Hsc70–CHIP E3 activity promotes theaccumulation of an immaturely glycosylated and detergent solubleform of CFTR ${Delta}$ F508 that is bound to Hsc70.

CFTR ${Delta}$ F508 that accumulates in the ER when Hsc70–CHIP action is blocked can fold to the native state
To ascertain whether or not the CFTR ${Delta}$ F508 biogenic intermediatethat accumulates in response to inhibition of Hsc70–CHIPE3 function is capable of folding we determined if it couldbe chased to its maturely glycosylated C form (Fig. 6 A). Transientlytransfected HEK293 cells were grown for 24 h after transfectionand then treated with cycloheximide to inhibit new protein synthesis.The fate of the accumulated CFTR ${Delta}$ F508 was then monitored by Westernblot after the indicated chase incubation at 37° or 26°C(Fig. 6 A). The low-temperature chase incubation was incorporatedinto the design of this experiment because nascent CFTR ${Delta}$ F508exhibits a temperature-sensitive folding defect and can foldto the native state and accumulate in its maturely glycosylatedC form when cells are cultured at 26°C (Denning et al., 1992).

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Figure 6. Glycolytic maturation of CFTR ${Delta}$ F508 degradation intermediates that accumulate in response to UbcH5a C85A overexpression. (A) The CFTR ${Delta}$ F508 that accumulates when UbcH5a C85A is overexpressed becomes maturely glycosylated when cell growth temperatures are reduced to 26°C. HEK293 cells were transiently transfected with the indicated plasmids and were treated with cycloheximide (25 µg/ml) 24 h later. Cells were then either shifted to 26°C or maintained at 37°C for the indicated time.(B) Glycolytic processing of CFTR ${Delta}$ F508 in cells incubated at 26°C for 16 h is blocked by BFA and enhanced by the chemical chaperone TMAO (75 mM). (C) COS-7 cells are capable of maintaining CFTR ${Delta}$ F508 degradation intermediates in a folding competent state. This experiment was performed as described for panel A except that the chase time was for 24 h at 26°C. The immaturely glycosylated and maturely glycosylated forms of CFTR ${Delta}$ F508 are denoted as B and C, respectively.

When control cells were allowed to synthesize CFTR ${Delta}$ F508 at 37°Cand were then incubated at either 37° or 26°C, >90%of the total protein present at t = 0 was degraded during the8-h chase period. When UbcH5a C85A was coexpressed with CFTR ${Delta}$ F508and a chase incubation was performed at 37°C, 40 to 50%of the total CFTR ${Delta}$ F508 present at t = 0 remained in the cellfor up to 24 h. However, even though UbcH5a C85A stabilizedthe B form of CFTR ${Delta}$ F508, its conversion to the C form was notdetected during the chase reaction at 37°C. In contrast,when chase incubations were performed at 26°C, a significantportion of the CFTR ${Delta}$ F508 that was stabilized in the B form byUbcH5a C85A, was converted to the maturely glycosylated C form.The formation of the maturely glycosylated C form of CFTR ${Delta}$ F508was proportional to the loss of B form and could be detectedin cells after 8 h of chase time and appeared to be completeafter 16 h. The glycolytic maturation of CFTR ${Delta}$ F508 observed inthe presence of UbcH5a C85A during the chase incubation at 26°Cwas inhibited by brefeldin A (BFA) and appears to result fromtrafficking of CFTR ${Delta}$ F508 out of the ER (Fig. 6 B). To determineif we could further increase the folding efficiency of the CFTR ${Delta}$ F508that accumulated in the presence of UbcH5a C85A, cells weretreated with the chemical chaperone TMAO just before the initiationof the chase reaction (Brown et al., 1996). TMAO treatment ofcells increased the quantity of UbcH5a C85A stabilized CFTR ${Delta}$ F508that could be processed to a maturely glycosylated C form aroundtwofold. Thus, a portion of CFTR ${Delta}$ F508 that accumulated in responseto inhibition of its ubiquitination remains in a foldable statethat can be brought back on pathway by alteration of cell growthtemperatures or chemical chaperones.

To probe whether inhibition of the Hsc70–CHIP complexstabilizes CFTR ${Delta}$ F508 in a folding competent conformation in morethan one cell type, we examined the effect that UbcH5a C85Aoverexpression had on CFTR ${Delta}$ F508 expression and folding in COS7cells (Fig. 6 C). UbcH5a C85A overexpression was again observedto drive the accumulation of the B form of CFTR ${Delta}$ F508. In addition,a significant portion of the B form that accumulated in thepresence of Ubc5Ha C85A could be chased at 26°C, in a BFA-sensitivemanner, to the maturely glycosylated C form. Hence, the Hsc70–CHIPcomplex can regulate biogenesis of CFTR ${Delta}$ F508 in more than onecell type.

To demonstrate that the CFTR ${Delta}$ F508 that was converted to the Cform during the 26°C chase incubation was trafficked tothe cell surface the localization of GFP–CFTR ${Delta}$ F508 wasexamined under these experimental conditions and compared withthat of GFP–CFTR (Fig. 7). At 37°C, GFP–CFTRwas detected both at the cell surface and in a perinuclear locationthat corresponds to the ER (Moyer et al., 1998). At 37°C,in the presence or absence of UbcH5a C85A, GFP–CFTR ${Delta}$ F508was only detected in its soluble ER form. However, when UbcH5aC85A-transfected cells were cultured for 24 h at 37°C, treatedwith cycloheximide, and then incubated at 26°C for 4 h,a pool of GFP–CFTR ${Delta}$ F508 accumulated, in a BFA-sensitivefashion, at the cell surface.

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Figure 7. Localization of GFP–CFTR ${Delta}$ F508 in HEK293 cells. Cells grown on glass coverslips were transiently transfected with GFP–CFTR or GFP–CFTR ${Delta}$ F508 with or without UbcH5a C85A and cultured for 24 h at 37°C. Where indicated 25 µg/ml cyclohexamide and/or brefeldin A (10 µM) was added to culture media. After 4 h of culture at 26°C these cells were fixed and the coverslips were mounted on glass slides. Images were collected and processed as described in the Materials and methods section.

The collective data presented in Figs. 5–7 demonstratethat when the activity of the Hsc70–CHIP ubiquitin ligaseis reduced, CFTR ${Delta}$ F508 accumulates as an immaturely glycosylatedspecies that is not a dead-end folding intermediate. Instead,the cell can maintain a pool of kinetically trapped CFTR ${Delta}$ F508folding intermediates in a detergent soluble and foldable state.

Discussion

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Abstract
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Results
Discussion
Materials and methods
References

Herein we provide new insights into how CFTR and CFTR ${Delta}$ F508 biogenicintermediates are partitioned between folding and degradationpathways. The data presented suggest a model for quality controlin which newly synthesized CFTR and CFTR ${Delta}$ F508 initiate folding,but intermediates of each accumulate in a kinetically trappedconformation that is maintained in a soluble state by Hsc70.CHIP then interacts with Hsc70 and functions via a two-stepmechanism to attract UbcH5a into Hsc70–CFTR complexes.Then the Hsc70–CHIP–UbcH5a E3 formed acts to polyubiquitinateCFTR.

Interestingly, inhibition of Hsc70–CHIP E3 activity causedthe accumulation of a nonaggregated and ER localized CFTR ${Delta}$ F508biogenic intermediate that was bound by Hsc70. Addition of chemicalchaperones to growth media and reduction of cell growth temperaturespermitted this nonubiquitinated CFTR ${Delta}$ F508 degradation intermediateto fold, exit the ER, and accumulate on the cell surface. Theseare the first data that describe a nonubiquitinated CFTR ${Delta}$ F508biogenic intermediate and they demonstrate that it can be maintainedin a nonaggregated and foldable state. This new informationsuggests that the development of drug cocktails that containubiquitination blockers and chemical chaperones could increasethe cell surface expression of CFTR ${Delta}$ F508 and provide a treatmentfor CF.

The nature of the folding defect that arrests the progressionof CFTR ${Delta}$ F508 through its folding cascade and what causes it tobe selected for proteasomal degradation is not entirely clear.One school of thought is that CFTR ${Delta}$ F508 is highly prone to misfoldingand aggregation and is therefore selected for ERAD. Such a notionis supported by the observation that inhibition of the proteasomeblocks CFTR ${Delta}$ F508 degradation and drives the accumulation of ubiquitinatedforms of CFTR ${Delta}$ F508 in Triton X-100–insoluble aggregates(Ward and Kopito, 1998). However, because the inactivation ofthe Hsc70–CHIP E3 ligase leads to the accumulation ofa soluble ER localized CFTR ${Delta}$ F508 biogenic intermediate, the datawe present support a different view. It appears that inhibitionof the proteasome leads polyubiquitinated CFTR ${Delta}$ F508 to aggregatebecause it can be extracted from the ER membrane by the p97–UFD1–NPL4complex (Ye et al., 2003), and because it cannot be degraded,polyubiquitinated CFTR ${Delta}$ F508 accumulates in aggresomes (Ward and Kopito, 1998).On the other hand, the nonubiquitinated CFTR ${Delta}$ F508that accumulates in response to inhibition of the Hsc70–CHIPE3 does not aggregate because it is inserted into the ER membraneand is bound by cytosolic Hsc70. Thus, while CFTR ${Delta}$ F508 has afolding defect that prevents it from passing quality controland escaping the ER, it does not appear to be overly aggregationprone and cellular chaperones can maintain it in a foldablestate.

Because the cellular activity of CHIP and UbcH5a influence thepartitioning of CFTR biogenic intermediates between foldingand degradation pathways, we were interested in investigatingwhether inhibition of the Hsc70–CHIP E3 would influencethe processing efficiency of CFTR and CFTR ${Delta}$ F508. In pulse-chaseexperiments UbcH5a C85A overexpression increased the half-lifeof the B form of CFTR and CFTR ${Delta}$ F508 from two- to threefold. Therefore,UbcH5a C85A overexpression increased the steady-state levelsof CFTR and CFTR ${Delta}$ F508 severalfold. However, the processing efficiencyof CFTR from its B form to its C form remained at around 25%whether or not the Hscp70–CHIP E3 complex was active.Thus, while the elevation of cellular Hsc70–CHIP E3 activitycan divert the B form of CFTR away from its folding pathway,the ability of full-length CFTR to stay on pathway and collapseto the native state appears to be limited by its intrinsic foldingpathway and/or additional quality control factors.

We conclude that the E2 UbcH5a is a cytosolic factor that functionswith Hsc70 and CHIP to mediate CFTR ubiquitination. This conclusionis supported by three lines of experimental evidence. First,purified CHIP and UbcH5a cooperated to facilitate the polyubiquitinationof CFTR. Second, when CHIP and UbcH5a were coexpressed togetherthey appeared to act synergistically to reduce the steady-statelevels of CFTR ${Delta}$ F508. Third, the coexpression of UbcH5a C85A withCHIP, blocked CHIPs ability to degrade CFTR and converted itinto a protein that behaved like the CHIP U box mutant P269A.

UbcH5a is a member of a family of conserved E2 proteins thatinclude UbcH5b and UbcH5c that are nearly 90% identical to eachother (Scheffner et al., 1994; Jensen et al., 1995b). In additionto UbcH5a, purified CHIP can interact with UbcH5b and UbcH5c,and mRNAs for each of these E2 proteins is present in all tissuestested (Jiang et al., 2001; Jensen et al., 1995b). Thus, wepropose that CHIP functions with an UbcH5 E2 family member toubiquitinate CFTR and other Hsc70 substrates, but we are notable to state whether it prefers one family member to the other.At this point, it is interesting to note that UbcH5 proteinsare related to the yeast Ubc4/5 proteins that function to targetmisfolded proteins for degradation and protect cells from proteindenaturing physiological stress (Seufert and Jentsch, 1990).In fact, one member of the Ubc4/5 family, Ubc1, has been shownto function on the ER surface to ubiquitinate ERAD substrates(Bays et al., 2001). Thus, it is logical that UbcH5 is a componentof an E3 complex, which contains molecular chaperones, thatserves to prevent the accumulation of toxic protein aggregates.

A potential caveat to the interpretation that Hsc70 and CHIPinteract with a UbcH5 family member to select CFTR for degradationis that the overexpression of UbcH5a C85A may nonspecificallyinhibit the action of other cytosolic quality control factorsthat function on the ER surface to mediate ERAD. Though possible,data from the control studies with the ERAD substrates TCR ${alpha}$ andApoB48, whose degradation relies on cytsolic E2s, demonstratethat their degradation was not delayed by overexpression ofUbcH5a C85A. Thus, it appears that the reduced rates of CFTRdegradation caused by UbcH5a C85A overexpression are due tospecific inactivation of the Hsc70–CHIP–UbcH5 E3complex.

The E2s Ubc6 and Ubc7 function with E3s such as gp78 and Doa10on the cytoplasmic face of the ER to ubiquitinate a varietyof substrates (Cyr et al., 2002). Hence, it is plausible thatE2–E3 complexes that contain Ubc6 and/or Ubc7 functionto select CFTR and CFTR ${Delta}$ F508 for degradation. Sommer and colleagueshave explored this concept and found that overexpression ofUbc6, but not Ubc7, modulates the rate of CFTR ${Delta}$ F508 degradation(Lenk et al., 2002). When we compared the effect that dominantnegative forms of Ubc6, Ubc7, and UbcH5a had on CFTR and CFTR ${Delta}$ F508expression, UbcH5a C85A and Ubc6 C91S drove the accumulationof the B form of CFTR, whereas Ubc7 had no apparent effect.The influence that UbcH5a C85A had on the accumulation of theB form of CFTR and CFTR ${Delta}$ F508, was markedly more dramatic thanthat of Ubc6 C91S, yet Ubc6 clearly plays a role in CFTR qualitycontrol. Studies in yeast demonstrate that Ubc6 cooperates withthe transmembrane E3 Doa10 to degrade membrane and cytosolicproteins (Swanson et al., 2001) and Doa10 is required for efficientCFTR turnover in yeast (Gnann et al., 2004). Thus, the Doa10–Ubc6E3 may function alongside the Hsc70–CHIP–UbcH5 E3to mediate quality control of CFTR. The Hsc70–CHIP–UbcH5E3 recognizes cytosolic regions of CFTR, whereas the Doa10/Ubc6E3 may recognize unassembled transmembrane regions. This scenariowould explain why turnover of the B form of CFTR and CFTR ${Delta}$ F508is delayed, but not completely blocked, by the inactivationof the Hsc70–CHIP E3 complex. A critical question pertainingto the function of CHIP as a quality control factor is relatedto the mechanism by which it regulates Hsc70 polypeptide bindingand protein folding activity. The data presented suggest thatCHIP functions via a two-step mechanism to determine the fateof Hsc70 clients such as CFTR. The first step involves the bindingof CHIP to the COOH-terminal EEVD motif in the lid domain ofHsc70 (Ballinger et al., 1999; Scheufler et al., 2000). Thisevent alters the Hsc70 polypeptide binding and release cycleto arrest CFTR folding and may involve the transient stabilizationof Hsc70–CFTR complexes. This putative event would givethe U box on CHIP the time required to attract UbcH5 to Hsc70–CFTRcomplexes and facilitate CFTR ubiquitination.

Interestingly, the ability of CHIP to ubiquitinate Hsc70 clientscan be modified by other cochaperones. Data presented hereindemonstrate that Hdj-2 cooperates with Hsc70 and CHIP to mediateCFTR ubiquitination. However, the cochaperone HspBP1, whichis a member of a family of nucleotide exchange factors thatpromote substrate release from Hsc70, blocks the ability ofCHIP to ubiquitinate CFTR (Alberti et al., 2004). Thus, thefate of proteins that are bound to Hsc70 is regulated by itsinteractions with multiple cochaperones. To understand thisprocess, the temporal relationship and driving force for interactionsbetween Hsc70 and its folding or degradatory cochaperones needsto be determined.

Materials and methods

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Results
Discussion
Materials and methods
References

Plasmids and antibodies
The plasmids used for cell transfection were: pCDNA3.1CFTR andpCDNA3.1CFTR ${Delta}$ F508 (Meacham et al., 2001); pEGFPC2-CFTR and pEGFPC2-CFTR ${Delta}$ F508(Moyer et al., 1998); pCDM8 2B4 TCR ${alpha}$ (Bonifacino et al., 1989);pCDNA-ApoB48 (H. Ginsberg, Columbia Presbyterian Medical Center,New York, NY); pCAGGS His₆UBCH5A C85A and pCAGGS His₆UBCH5A(Jiang et al., 2001); pCMVPLDmyc-UBC6 and pCMVPLDmyc-UBC6 C91S(Lenk et al., 2002); pCDNA myc-UBC7 and pCDNA myc-UBC7 C89S(Tiwari and Weissman, 2001); pCDNA3.1CHIP, pCDNA3.1CHIP K30A,and pCDNA3.1CHIP P269A (Jiang et al., 2001; Meacham et al., 2001).pGEXCFTR 371–855 was termed pGSTNBD1-R (Naren et al., 1999).

The following plasmids were used for overexpression of the indicatedproteins in E. coli; pET9d Hdj2 and pET11a Hsc70 (Meacham et al., 1999).Plasmids prepared for this study were pET11a His₆UbcH5a,pET11a-His₆UbcH5a C85A, pET11d His₆Ubc7, pET11a His₆Ubc6 1–243,pET30His₆CHIP, pET30His₆CHIPK30A, pET30His₆CHIPH260A, and pET30His₆CHIPP269A. E1 was purchased from Calbiochem.

The antibodies used for Western blots and/or immunoprecipitationswere ${alpha}$ CFTR clone MM13-4 from Upstate Biotechnology and ${alpha}$ CFTR R-domainantibody from R&D Systems. ${alpha}$ TCR was from BD Biosciences and ${alpha}$ Hsc70 was from Stressgen Biotechnologies.

Protein purification
The proteins used in in vitro ubiquitination assays were purifiedafter overexpression in E. coli. Hsc70 was purified by a combinationof ATP–agarose and anion exchange chromatography (Cyr et al., 1992).Hdj-2 was purified by anion exchange and hydroxyapatitechromatography (Meacham et al., 1999). His₆-tagged proteinswere purified by metal chelate chromatography (Lu and Cyr, 1998).

GstNBD1-R was expressed in E. coli strain BL21 (DE3) and cellsfrom a 600-ml culture were harvested after a 16-h inductionat 30°C with 0.2 mM IPTG. Cell pellets were resuspendedand incubated for 30 min on ice in 10 mM Tris-HCl, pH 8.0, 1mM EDTA, 150 mM NaCl, 1 mM phenylmethyl sulfonyl fluoride, 1mM DTT, and lysozyme 0.1 µg/ml. The extract was supplementedwith 1% sarkosyl and sonicated. Gst–NBD1–R was thenpurified with glutathione–agarose beads and had a finalconcentration near 2 mg/ml.

Reconstitution of CFTR ubiquitination
The experimental conditions for the reconstitution of gst–NBD1–Rubiquitination were described previously (Koegl et al., 1999).Ubiquitination assays were performed in a reaction buffer composedof 20 mM Hepes, pH 7.4, 50 mM NaCl, 5 mM MgCl₂, 2.5 mM ATP,2 mM DTT, 10 µM bovine ubiquitin, 0.1 µM rabbitE1 and 1 µM gst–NBD1–R. The indicated E2 proteinwas added at 4 µM and the other factors were includedat the concentration indicated in Fig. 1. Incubations were performedat 37°C for the indicated time and terminated by the additionof 20 µl of SDS sample buffer to 25 µl reactioncocktails. Proteins were resolved on 7% SDS-PAGE gels and thentransferred to nitrocellulose membranes that were decoratedwith ${alpha}$ R domain antibody and developed.

Assays for CFTR biogenesis
HEK293 and Cos-7 cells were maintained in DMEM supplementedwith 10% fetal bovine serum and a mixture of 1% penicillin andstreptomycin at 37°C and transfected with CFTR and CFTR ${Delta}$ F508expression plasmids. Steady-state levels of CFTR and CFTR ${Delta}$ F508levels were determined by Western blot and CFTR processing efficiencywas measured by pulse chase analysis (Meacham et al., 2001).Details of the protocols for direct immunoprecipitations orcoimmunoprecipitations were as described previously (Meacham et al., 2001).To verify the identity of CFTR isolated fromchaperone complexes CFTR was reimmunoprecipitated from coimmunoprecipitateswith ${alpha}$ -CFTR (Meacham et al., 1999). Treatment of cell extractswith endoglycosidase H was conducted as described previously(Meacham et al., 1999).

Fluorescence microscopy
HEK293 cells were cultured on glass coverslips and transfectedtransiently with 1µg pEGFPC2–CFTR or pEGFPC2–CFTR ${Delta}$ F508either alone or in combination with 3 µg pCAGGS His₆UBCH5AC85A. 24 h later, cells were washed twice for 5 min with 2 mlsof PBS and fixed with 4% paraformaldehyde at room temperature.As indicated, cells were grown for 24 h after transfection andthen treated with 25 µg/ml cyclohexamide and incubatedfor an additional 4 h at 26°C. Coverslips were mounted onglass slides with the preservative Fluoromount-G. Images werecollected using a Nikon E600 microscope and a Princeton InstrumentsCCD camera. Images were processed with Metamorph (UniversalImaging Corp.) and Adobe Photoshop software.

Online supplemental material
Data presented in Fig. S1 demonstrate that the joint presenceof Hsc70, Hdj-2, and CHIP stimulates dramatically the rate atwhich UbcH5a conjugates gst–NBD1–R with ubiquitin.When Hsc70 or Hdj-2 were omitted from reactions mono-, di-,and triubiquitination of gst–NBD1–R was observed,but this reaction was slow and inefficient. Thus, Hsc70, Hdj-2,and CHIP act jointly to stimulate the ubiquitination activityof UbcH5a and therefore exhibit an activity that fits the definitionof a multisubunit E3 ubiquitin ligase. Fig. S1 is availableat http://www.jcb.org/cgi/content/full/jcb.200410065/DC1.

Acknowledgments

The authors thank Drs. Bonificano, Ginsberg, Kirk, Sommer, Stanton,and Weissman for providing plasmids.

C. Patterson is funded by the National Institutes of Health(NIH). D.M. Cyr is funded by the NIH and the Cystic FibrosisFoundation. A predoctoral fellowship from the American HeartAssociation supports J.M. Younger.

Submitted: 13 October 2004

Accepted: 10 November 2004

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