Activation of Chaperone-mediated Autophagy during Oxidative Stress

Roberta Kiffin^*, Christopher Christian^*, Erwin Knecht, and Ana Maria Cuervo^*

^* Department of Anatomy and Structural Biology, Marion Bessin Liver Research Center, Albert Einstein College of Medicine, Bronx, NY 10461; Instituto de Investigaciones Citológicas, Fundación Valenciana de Investigaciones Biomédicas, Valencia 4010, Spain

Submitted June 11, 2004; Revised August 3, 2004; Accepted August 18, 2004
Monitoring Editor: Jennifer Lippincott-Schwartz

ABSTRACT

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
ACKNOWLEDGMENTS
REFERENCES

Oxidatively damaged proteins accumulate with age in almost allcell types and tissues. The activity of chaperone-mediated autophagy(CMA), a selective pathway for the degradation of cytosolicproteins in lysosomes, decreases with age. We have analyzedthe possible participation of CMA in the removal of oxidizedproteins in rat liver and cultured mouse fibroblasts. Addedto the fact that CMA substrates, when oxidized, are more efficientlyinternalized into lysosomes, we have found a constitutive activationof CMA during oxidative stress. Oxidation-induced activationof CMA correlates with higher levels of several components ofthe lysosomal translocation complex, but in particular of thelumenal chaperone, required for substrate uptake, and of thelysosomal membrane protein (lamp) type 2a, previously identifiedas a receptor for this pathway. In contrast with the well characterizedmechanism of CMA activation during nutritional stress, whichdoes not require de novo synthesis of the receptor, oxidation-inducedactivation of CMA is attained through transcriptional up-regulationof lamp2a. We conclude that CMA is activated during oxidativestress and that the higher activity of this pathway under theseconditions, along with the higher susceptibility of the oxidizedproteins to be taken up by lysosomes, both contribute to theefficient removal of oxidized proteins.

INTRODUCTION

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
ACKNOWLEDGMENTS
REFERENCES

Accumulation of oxidized protein is a common feature of agedcells (Dunlop et al., 2002; Grune and Davies, 1997; Grune etal., 2001, 2002b; Stadtman, 2001). Many physiological and pathologicalprocesses lead to the generation of free radicals and consequentdamage of intracellular components, including proteins. In mostof these oxidative events, damaged proteins are removed fromthe cell through degradation by proteases (Dunlop et al., 2002).The activity of different intracellular proteolytic systemsdecreases with age (Terman, 1995; Cuervo and Dice, 1998a; Friguetet al., 2000; Carrard et al., 2002; Donati et al., 2001; Merkeret al., 2001; Friguet, 2002; Keller et al., 2002; Ward, 2002),and this impaired activity is considered responsible for thedeficient removal of oxidized proteins in old organisms (Grune,2000; Merker and Grune, 2000; Dunlop et al., 2002; Szweda etal., 2002).

The susceptibility of oxidized proteins to proteases changeswith the duration and degree of oxidative damage (Dunlop etal., 2002; Mehlhase and Grune, 2002). Thus, mild oxidation inducespartial protein unfolding and facilitates proteolytic cleavage(Grune et al., 1995, 1997). However, persistent or extensiveoxidative damage usually promotes protein aggregation, due tothe exposure of patches of hydrophobic amino acids. Once a proteinaggregates, it becomes less susceptible to proteolytic cleavage(Hoff et al., 1993; Grune et al., 1997; Davies, 2001; Demasiand Davies, 2003). Kinetics of degradation of oxidized proteinsin vitro have been analyzed using different types of proteases(Merker and Grune, 2000; Dunlop et al., 2002; Szweda et al.,2002). One of the most extensively analyzed protease in thisrespect has been the proteasome. Although most of the studieslinking the proteasome to the degradation of oxidized proteinshave been carried out in vitro (Rivett, 1985; Davies, 2001),recent evidence supports the participation of the proteasomein the removal of oxidized proteins in vivo also (Hosler etal., 2003; Shringarpure et al., 2003). Thus, treatment of culturecells with proteasome inhibitors or antisense oligonucleotidesagainst essential proteasome subunits results in accumulationof oxidized proteins inside cells and diminished rates of cellsurvival during oxidative stress. The degradation of most oxidizedproteins by the proteasome is ATP and ubiquitin independent(Shringarpure et al., 2003), suggesting that the exposure ofhydrophobic regions in the surface of the protein acts as recognitionsignal for this protease.

The lysosomal system, the other major proteolytic system incells, has not been often considered as a possible candidatefor the removal of oxidized proteins because of its lack ofselectivity. In mammalian cells three different main mechanismscontribute to the degradation of intracellular components insidelysosomes (autophagy) (Dice, 2000; Reggiori and Klionsky, 2002;Wang and Klionsky, 2003; Cuervo, 2004a,b). Two of those mechanisms,macroautophagy and microautophagy, result in the degradationof complete regions of the cytosol, including organelles, inthe lysosomal lumen. Although degradation of organelles by theseautophagic pathways can be selective (i.e., specific removalof damaged mitochondria sparing normal functioning ones) (Lemasterset al., 2002), there is no evidence supporting selectivity forthe degradation of soluble cytosolic proteins. In contrast,the main characteristic of a third form of autophagy, chaperone-mediatedautophagy (CMA), is its selectivity regarding the substrates(cytosolic proteins) degraded through this pathway (Cuervo andDice, 1998b; Dice, 2000; Dice et al., 2003).

CMA is a generalized form of autophagy present in most celltypes and tissues (Massey et al., 2004). All the CMA substrateproteins described to date are soluble cytosolic proteins containinga targeting motif biochemically related to the pentapeptideKFERQ (Chiang and Dice, 1988; Dice et al., 2003). This motif,present in $~$ 30% of the proteins in the cytosol, is recognizedby a cytosolic chaperone, the heat shock cognate protein of73 kDa (cyt-hsc70) (Chiang and Dice, 1988; Chiang et al., 1989).The interaction with this chaperone, modulated by the hsc70cochaperones (Agarraberes and Dice, 2001), targets the substrateto the lysosomal membrane, where it interacts with the lysosomalmembrane protein (lamp) type 2a (Cuervo and Dice, 1996). Substratesneed to be unfolded before translocation into the lysosomallumen, and several cytosolic chaperones associated to the lysosomalmembrane have been proposed to assist in the unfolding (Agarraberesand Dice, 2001). Translocation of the substrate requires thepresence of a variant of hsc70, lyshsc70, in the lysosomal lumen(Agarraberes et al., 1997; Cuervo et al., 1997) and is followedby the rapid proteolysis of the substrate by resident lysosomalproteases (half-life in the lysosomal lumen of 5–10 min).

Although some basal level of CMA activity is probably presentin most cells, nutritional stress has been shown to maximallyactivate this pathway (Wing et al., 1991; Cuervo et al., 1995).Activation during nutrient deprivation is associated with higherlevels of lys-hsc70 in the lysosomal lumen and of lamp2a atthe lysosomal membrane (Cuervo et al., 1995; Agarraberes etal., 1997; Cuervo and Dice, 2000b). Because the interactionof substrate proteins with lamp2a is a limiting step for thispathway, changes in levels of lamp2a at the lysosomal membranemodulate CMA activity (Cuervo and Dice, 2000b,c). Interestingly,all the conditions known to activate CMA, up-regulation of thelysosomal levels of lamp2a does not require de novo synthesisof the protein, but instead it is attained through down-regulationof its degradation and by relocation of a fraction of the proteinfrom the lysosomal lumen into the membrane (Cuervo and Dice,2000b).

In addition to starvation, activation of CMA has also been observedin rat liver and kidney after exposure to gasoline derivatives(Cuervo et al., 1999); in fibroblasts from galactosialidosispatients, which lack the protective protein/cathepsin A (Cuervoet al., 2003); and in cells overexpressing lamp2a (Cuervo andDice, 1996). CMA activity is reduced during renal tubular cellgrowth (Franch et al., 2001) and in aging (Cuervo and Dice,2000a). The decrease in CMA activity in old cells, known toaccumulate oxidized proteins (Cuervo and Dice, 2000a), combinedwith the fact that activation of CMA during toxic exposure resultsin the selective degradation of a protein altered by the toxiccompound (Cuervo et al., 1999), and with our finding that inthe presence of antioxidants degradation of the inhibitor ofthe nuclear factor ${kappa}$ B by CMA decreases (Cuervo et al., 1998),prompted us to analyze a possible role of CMA in the removalof oxidized proteins from cells. We show in this work that oxidationof CMA substrates facilitates their translocation into lysosomesfor degradation via CMA and also that CMA itself is activatedduring oxidative stress. Unexpectedly, the oxidative stress-mediatedactivation of CMA is attained through a novel mechanism, differentfrom the previous well-characterized activation of CMA in responseto nutritional stress.

MATERIALS AND METHODS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
ACKNOWLEDGMENTS
REFERENCES

Animals and Cells
Male Wistar rats (200–250 g) were fed ad libitum or starvedfor 20 or 48 h before sacrifice. An age-controlled rat strain(Fisher 344) was used for the study of age-related changes and3-, 12-, and 22-mo-old rats were compared. Mild oxidative stresswas induced in rats with two single i.p. injections of paraquat(40 mg/100 g body weight) separated by 24 h. Lysosomal isolationwas carried out 24 h after the last injection. Mouse fibroblasts(NIH3T3) were from the American Type Culture Collection (Manassas,VA). Cells were maintained in DMEM (Sigma-Aldrich, St. Louis,MO) in the presence of 10% newborn calf serum. To deprive cellsfrom serum, plates were extensively washed with Hanks' balancedsalt solution (Invitrogen, Carlsbad, CA), and fresh medium withoutserum was added. Mild oxidative stress was induced in culturecells by supplementation of the culture medium with 100 µMH₂O₂ or 40 µM paraquat for 1 h. Assays were carried out12–24 h after removing the oxidizing compound.

Chemicals
Sources of chemicals and antibodies were as described previously(Cuervo and Dice, 1996; Cuervo et al., 1997; Cuervo and Dice,2000a; Martin et al., 2002). The antibodies against the cytosolictail of rat and mouse lamp2a and lamp2c were prepared in ourlaboratory (Cuervo and Dice, 1996; Zhang, Bandhyopadhyay, Kiffin,Massey, and Cuervo, unpublished data). The antibody againstmouse lamp1 (1D4B [PDB] ) was from the Developmental Studies HybridomaBank (University of Iowa, Iowa City, IA), and antibodies againsthsp90 (SPA-845), hsp72 (SPA-810), hsp40 (SPA-400), hip (SPA-766),and Bag-1 (AAM-400E) were from Stressgene Biotechnologies (Victoria,BC, Canada). Carbonyl groups in oxidized proteins were detectedusing the OxyBlot oxidized protein detection kit from ChemiconInternational (Temecula, CA). Glyceraldehyde-3-phosphate dehydrogenase(GAPDH) and ribonuclease A (RNase A) were radiolabeled with[¹⁴C]formaldehyde by reductive methylation as described previously(Jentoft and Dearborn, 1983). Cytosolic proteins from mousefibroblasts in culture were metabolically radiolabeled by incubationwith [¹⁴C]leucine (2 µCi/ml) at 37°C for 2 d (Cuervoet al., 1997). Cells were disrupted by nitrogen cavitation,and the cytosolic fraction was the supernatant of a centrifugationat 100,000 x g for 1 h at 4°C. Oxidized radiolabeled cytosolicproteins were prepared by the same procedure from cells treatedwith different prooxidants for 24 h before isolation.

Isolation of Lysosomal Fractions
Rat liver lysosomes were isolated from a light mitochondrial-lysosomalfraction in a discontinuous metrizamide density gradient (Wattiauxet al., 1978). Lysosomal fractions with different activitiesfor CMA were separated as described previously (Cuervo et al.,1997). Lysosomes from cultured cells were isolated as describedpreviously (Storrie and Madden, 1990). Preparations with morethan 10% broken lysosomes, measured as ${beta}$ -hexosaminidase latency,were discarded. Lysosomal matrices and membranes were isolatedafter hypotonic shock (Ohsumi et al., 1983).

Uptake and Degradation of Proteins by Isolated Lysosomes
GAPDH or RNase A were incubated in MOPS buffer (10 mM 3-(N-morpholino)propanesulfonicacid [MOPS] pH 7.3, 0.3 M sucrose) with chymostatin-treatedlysosomes as described previously (Cuervo et al., 1997). Transportwas measured after proteinase K treatment of the samples, SDS-PAGE,and immunoblot as the amount of GAPDH associated to lysosomesresistant to the protease. In another group of experiments,to overcome any possible changes in the proteolytic susceptibilityof the oxidized proteins to proteinase K, substrates were incubatedwith chymostatin-treated or untreated lysosomes, and uptakewas calculated as the difference between the amount of substrateassociated to lysosomes (chymostatin-treated lysosomes) andthe amount of substrate bound to their membrane (untreated lysosomes)(Salvador et al., 2000). Degradation of [¹⁴C]GAPDH (260 nM;1.5 x 10⁸ dpm/nmol), [¹⁴C]RNase A (150 nM; 0.9 x 10⁸ dpm/nmol),or a pool of radiolabeled cytosolic proteins (500 dpm/µg)by intact lysosomes or lysosomal matrices was measured as describedpreviously (Terlecky and Dice, 1993; Cuervo et al., 1997). Afterincubation for 30 min at 37°C in MOPS/dithiothreitol (DTT)buffer (10 mM MOPS pH 7.3, 0.3 M sucrose, 5.4 µM cystein,and 1 mM DTT) (for intact lysosomes) or in 0.03 M sucrose (forlysosomal matrices), samples were precipitated in 10% trichloroaceticacid and filtered through a multiscreen assay system (Millipore,Bedford, MA) using a 0.45 µm pore filter. Radioactivityin the flow through and in the filter was converted to disintegrationsper minute in a WinSpectral 1414 liquid scintillation analyzer(PerkinElmer Life and Analytical Sciences, Boston, MA) by correctingfor quenching using an external standard. Proteolysis was expressedas the percentage of the initial acid-insoluble radioactivity(protein) transformed into acid-soluble radioactivity (aminoacids and small peptides) at the end of the incubation.

Rates of degradation of lamp2a in the isolated membranes werefollowed by immunoblot with a specific antibody against thecytosolic tail of lamp2a as described previously (Cuervo andDice, 2000b). Briefly, isolated lysosomal membranes were incubatedin MOPS buffer at 37°C, and at different times aliquotswere removed and subjected to SDS-PAGE and immunoblot for lamp2a.

GAPDH Oxidation
Metal-catalyzed oxidation of rabbit muscle D-glyceraldehyde-3-phosphatedehydrogenase EC 1.2.1.12 [EC] (Roche Diagnostics, Indianapolis,IN) was carried out as described previously (Rivett and Levine,1990). GAPDH (10 mg of protein) was dialyzed against 50 volumesof HEPES buffer (50 mM HEPES, pH 7.2, 100 mM KCl, 10 mM MgCl₂)supplemented or not (Mock) with 25 mM ascorbic acid and 0.1mM FeCl₃ at 37°C. The oxidative reaction was stopped adding1 mM EDTA, and the samples were dialyzed against HEPES bufferfor 24 h with four changes. The two first changes were supplementedwith 1 mM EDTA. The efficiency of oxidation was monitored bymeasuring the enzymatic activity of GAPDH after being exposedto the oxidant mixture for different periods of time. As describedin Figure 2, incubation of GAPDH with the oxidant mixture for30 min resulted in 70% decrease of its enzymatic activity.

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Figure 2. Oxidation of CMA substrates facilitates their uptake by lysosomes. (A) GAPDH was exposed to an ascorbic acid/iron oxidizing reaction for 30 min as described under Materials and Methods. The remaining specific enzymatic activity of untreated GAPDH (CTR) and of GAPDH exposed to the oxidant mixture (ASCORB/FeCl₃) or to the dialysis buffer only (MOCK) is shown. Values are mean ± SE of two different preparations with triplicate measurements. (B) Unmodified GAPDH (Ctr) or GAPDH exposed to the oxidant mixture for the indicated periods of time was incubated for 30 min under standard conditions with intact chymostatin-treated liver lysosomes isolated from 20-h starved rats. Where indicated, samples were treated with proteinase K to remove GAPDH bound to the cytosolic side of the lysosomal membrane. At the end of the incubation, lysosomes were collected by centrifugation and subjected to SDS-PAGE and immunoblot for GAPDH. (C) The different forms of GAPDH (50 µg) described in A were incubated with lysosomal enzymes (25 µg of protein of broken lysosomes; pH 4.5) (left) or proteinase K (0.1 µg) (right) at 37 or 0°C, respectively. At the indicated times aliquots were taken and subjected to SDS-PAGE and Coomassie Blue staining. Values are the mean + SE of the densitometric values for GAPDH from three different experiments. (D) Mouse fibroblasts were metabolically labeled with [³H]leucine for 48 h. A group of fibroblasts was exposed to 100 µM H₂O₂ (left) or 40 µM paraquat (Pq) for 1 h during the labeling. After cavitation, cytosolic fractions (Cyt) from untreated (Ctr) and H₂O₂ or paraquat-treated fibroblasts were prepared and incubated for 30 min at 37°C with intact rat liver lysosomes (25 µg of protein) or with lysosomes disrupted by a hypotonic shock (broken lysosomes; 15 µg of protein) under standard conditions. At the end of the incubation proteolysis was calculated as the amount of acid precipitable radioactivity (protein) transformed in acid soluble (amino acids and small peptides). Values are the mean + SE of six different experiments (^*p < 0.05, ^**p < 0.01, ^***p < 0.001).

Immunocytochemical Staining
Immunofluorescence studies of cultured cells were performedfollowing conventional procedures (Cuervo and Dice, 2000c).Cells grown on coverslips until confluent and kept in the presenceor absence of serum for 20 h were fixed with a 3% formaldehydesolution, blocked, and then incubated with the primary and correspondingfluorescein isothiocyanate or Cy5-conjugated secondary antibodiesas described previously (Cuervo and Dice, 2000c). Mounting mediumcontained 4,6-diamidino-2-phenylindole staining to highlightthe cellular nucleus. Images were acquired with an Axiovert200 fluorescence microscope (Carl Zeiss, Thornwood, NY) andsubjected to deconvolution with the manufacturer's software.Colocalization was determined using MetaMorph (Universal Imaging,Downingtown, PA). All digital microscopic images were preparedusing Adobe Photoshop 6.0 software (Adobe Systems, MountainView, CA).

mRNA Quantification
Total RNA was extracted from rat livers using the RNeasy protectmini kit (QIAGEN, Valencia, CA) following the manufacturer'sindications and stored at -80°C until use. The first strandcDNA was synthesized from 1 µg of the total RNA with theSuperScript II RNase H Reverse Transcriptase (Invitrogen) andoligo-(dT)_12–18 primer. A region of the exon 5 of lamp2aand of actin were amplified with specific primers (lamp2a, 5'-GTCTCAAGCGCCATCATACT-3'[forward] and 5'-TCCAAGGAGTCTGTCTTAAGTAGC-3' [reverse]; actin,5'-AAGGACTCCTATAGTGGGTGACGA-3' [forward] and 5'-ATCTTCTCCATGTCGTCCCAGTTG-3'[reverse]) by using the SYBR green polymerase chain reaction(PCR) kit (PE Biosystems, Warrington, United Kingdom). Amplificationof the lamp2a and actin DNA products (120 and 108 bp, respectively)was measured in real time in a light cycler (SmartCycler; Cepheid,Sunnyvale, CA). For both genes, the presence of a single amplifiedproduct was verified by agarose gel electrophoresis, and byanalysis of the melting curves of the reverse transcription-PCRreaction. The expression levels of lamp2a in different sampleswere normalized with respect of those of actin in the same samples.Differences between samples were calculated based in their differencesof the cycle numbers to reach a certain fluorescence intensitylevel. Because the size of the amplified fragments was verysimilar we did not need to correct for fragment length. StandardPCR was carried out with the same primers but increasing dilutionsof the cDNA pool. PCR products were subjected to electrophoresisin 1.2% agarose gels and densitometry. The densitometric intensityof the lamp2a products was normalized with respect to the intensityof the actin products for the same sample.

General Methods
Protein concentration was determined by the Lowry method (Lowryet al., 1951) by using bovine serum albumin as a standard. Lysosomalenzymatic activities were measured as reported previously (Storrieand Madden, 1990). After SDS-PAGE (Laemmli, 1970) and immunoblotting(Towbin et al., 1979), the proteins recognized by the specificantibodies were visualized by chemiluminescence methods (Renaissance;PerkinElmer Life and Analytical Sciences). Oxidized proteinswere visualized after derivatization with DNPH by immunoblotwith an antibody against the DNP moiety following the manufacturer'srecommendation. Densitometric quantification of the immunoblottedmembranes and stained gels was done with an Image Analyzer System(S1800; Inotech, Sunnyvale, CA). Student's t test was used forstatistical analyses.

RESULTS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
ACKNOWLEDGMENTS
REFERENCES

Oxidized Proteins in Lysosomes
To test the contribution that the lysosomal system, and in particularCMA, might play in the removal of oxidized cytosolic proteins,we first analyzed the presence of those proteins inside lysosomesafter oxidative stress. We induced mild oxidative stress inrats by treatment with bleomycin, 1,1'-dimethyl-4,4'-bipyridiniumdichloride (paraquat), a superoxide-generating drug with well-characterizedprooxidant effects (Haly, 1979). To verify the oxidative effectof paraquat in rat liver we compared the content of carbonyl-containingproteins in the cytosol of untreated and paraquat-treated rats(Figure 1A, lanes 1 and 2). Although some oxidized proteinscan be observed in the cytosol of untreated rats, we found asignificant increase in the content of these modified proteinsin the cytosol of rats injected with a sublethal dose of paraquatfor two consecutive days. Lysosomes active for CMA can be isolatedfrom rat liver based on their high content of the lumenal chaperonelys-hsc70 required for substrate uptake (Cuervo et al., 1997).When we isolated this particular lysosomal population from treatedand untreated rats and separated their membranes from theirlumenal content, we found carbonyl-containing proteins in boththe membrane and lumenal fraction of the lysosomes from paraquat-treatedrats (Figure 1A, compare lanes lanes 3 and 5 to lanes 4 and6). Washing the lysosomal membranes with 1 M NaCl released mostof the oxidized proteins (Figure 1A, lanes 7 and 8), suggestingthat they were likely cytosolic proteins associated to the membrane,rather than the result of oxidation of integral lysosomal membraneproteins. Likewise, when we incubated the lysosomal matricesat 37°C before electrophoresis to promote the degradationof nonlysosomal proteins in the lysosomal lumen, the level ofoxidized proteins in this fraction decreased drastically (Figure 1A,lanes 9 and 10). Note that the new lower molecular weightbands detected in the matrices of paraquat-treated animals afterthe incubation at 37°C could be proteolytic products ofthe proteins detected in the freshly isolated matrices. Theseresults support that the oxidized proteins detected inside thelysosomes were most likely nonlysosomal proteins delivered thereto be degraded. Interestingly, despite of their cytosolic origin,the electrophoretic pattern of the oxidized proteins associatedwith the lysosomal fraction differs from the ones in the cytosol.Because these differences are also observed in the membraneassociated proteins, we do not think that they are due to distinctsusceptibility of some of the oxidized proteins to proteases;instead we consider it an indication that a subset of oxidizedproteins is selectively taken up by lysosomes.

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Figure 1. Oxidized proteins in lysosomes active for CMA. (A) Cytosol (20 µg of protein) and lysosomal membranes and matrices (10 µg of protein) separated after hypotonic shock from lysosomes enriched in hsc70 isolated from livers of untreated or paraquat (PQ)-treated rats were derivatized and subjected to SDS-PAGE and immunoblot against 2,4-dinitrophenylhydrazine (DPNH) moieties. To show the protein pattern in all lanes, exposure of lanes 1 and 2 was 5 times shorter than for the other lanes. Lanes 7 and 8 are duplicate samples of lanes 3 and 4, in which membranes were washed with 1 M NaCl before derivatization. Lanes 9 and 10 are duplicate samples of lanes 5 and 6 in which the matrices were incubated for 20 min at 37°C before derivatization. No bands were detected in the same samples when derivatization was omitted (our unpublished data). (B) Cytosol (40 µg of protein) and lysosomal matrices (20 µg of protein) were isolated from livers of 3-, 9- and 22-mo-old rats. Content of oxidized proteins in these fractions was analyzed as in A. Exposure of lanes 1–3 was 3 times shorter than for lanes 4–6. Lanes 7 and 8 show the same sample than lane 5 derivatized or not with DPNH and immunobloted as the others. The film is overexposed (8 times lane 5 exposure) to show the low content of protein bands nonspecifically recognized by the antibody.

As reported previously, even in the absence of treatment witha prooxidant agent, oxidized proteins can be detected in normalliver and their content increases with age (Figure 1B). Whenwe analyzed the association of oxidized proteins to lysosomesfrom livers of 3- and 9-mo-old rats, we found an increase inthe content of oxidized proteins in the lysosomal lumen withage, similar to the one observed in the cytosol (Figure 1B,compare lanes 1 and 2 and 4 and 5). In contrast, in the oldestanimals (22 mo old), for which we have previously describeda severe decrease in CMA activity (Cuervo and Dice, 2000a),despite the higher content of oxidized proteins in the cytosolicfraction, in proportion, the amount of oxidized proteins detectedin lysosomes was lower than in the 9-mo-old animals (Figure 1B,compare lanes 5 and 6). Similar assays to the ones describedabove confirmed that the oxidized proteins were of extralysosomalorigin and could be degraded by the lysosomal proteases (ourunpublished data). The last panel of Figure 1B shows the specificityof the antibody used in these studies against the carbonyl groups,which in nonderivatized samples only weakly cross-reacted witha single protein (compare signal in derivatized (lane 7) andnonderivatized samples (lane 8). Although macroautophagy, anonselective form of autophagy, also decreases with age (Terman,1995; Donati et al., 2001), the fact that the lysosomal populationanalyzed has been shown to be very active for CMA and that onlya subset of oxidized proteins was detected in lysosomes encouragedus to analyze the role of CMA in the removal of oxidized proteins.

Oxidation of CMA Substrates
We first analyzed whether the oxidation of known CMA substratesfacilitated their degradation by CMA. We oxidized GAPDH, a well-characterizedCMA substrate (Aniento et al., 1993), by incubating this proteinwith an ascorbic acid/iron oxidizing mixture. After 30 min ofincubation with this mixture, $~$ 70% of GAPDH activity was lost(Figure 2A), and carbonyl groups were easily detectable in thepurified protein (our unpublished data). We have previouslyoptimized an in vitro system that allows the analysis of bindingand uptake of CMA substrates by isolated lysosomes (Anientoet al., 1993; Cuervo et al., 1997, 1999). When we compared theassociation to lysosomes of untreated GAPDH or of GAPDH exposedfor increasing periods of time to the oxidizing mixture, wefound an increase in both the amount of protein bound to thelysosomal membrane and translocated into the lysosomal lumen(proteinase K resistant) with longer oxidation times of GAPDH(Figure 2B). Oxidation of ovalbumin, a protein that does notcontain a KFERQ-like motif and consequently is not a CMA substrate,did not increase its association to lysosomes (our unpublisheddata). The higher amount of GAPDH detected in the lysosomallumen could also result from an increased resistance of theoxidized protein to degradation, either by the lysosomal proteasesor by proteinase K, which removes the protein associated tothe cytosolic side of the lysosomal membrane. However, as shownin Figure 2C, the oxidized protein was even more readily degradedby both the pool of proteases located in the lysosomal lumenand by exogenously added proteinase K.

An increase in lysosomal translocation of oxidized proteinswas also evident when instead of using a specific CMA substrate,we compared the degradation of a pool of oxidized cytosolicproteins, in which $~$ 30% of them are possible CMA substrates (containKFERQ-related motifs) (Figure 2D). Radiolabeled cytosolic proteinsisolated from fibroblasts exposed to H₂O₂ (Figure 2D, left)or paraquat (Figure 2D, right) were degraded faster than cytosolicproteins from untreated fibroblasts when incubated with intactrat liver lysosomes. Because these differences were greatlyreduced when the lysosomal membranes were disrupted before theincubation with the cytosolic proteins, giving free access ofthe proteases to the substrates, we conclude that, as shownfor GAPDH, increased degradation of the oxidized proteins resultedfrom their higher rates of translocation via CMA into lysosomes.These results support that oxidation of proteins that are substratesfor CMA facilitates their degradation through this pathway.

Activation of CMA during Oxidative Stress
Independently of the effect of oxidation on CMA substrates,which makes them more susceptible to degradation by this pathway,we found a constitutive activation of CMA during oxidative stress.We isolated lysosomes from rats treated with a sublethal doseof paraquat for two consecutive days to generate a mild oxidativestress response. Under these conditions, we did not find significantdifferences with control in lysosomal membrane stability assessedby measuring ${beta}$ -hexosaminidase latency (Supplemental Figure 1)(Storrie and Madden, 1990) and extralysosomal proteolytic activity(Aniento et al., 1993). Lysosomes isolated from rats exposedto paraquat degraded larger amounts of unmodified GAPDH thanlysosomes isolated from untreated animals (Figure 3A, left).Similar results were observed for RNase A, another well-characterizedCMA substrate (Terlecky and Dice, 1993; Cuervo et al., 1994)(Figure 3A, right). In both cases, the increase in substratedegradation was no longer observed if the lysosomal membranewas disrupted. In fact, the degradation of both substrates bylysosomal proteases was slightly lower in the paraquat-treatedanimals. This decrease could result from a decrease in the activityof some lysosomal proteases during oxidative stress, as reportedpreviously (O'Neil et al., 1997; Carr, 2001; Crabb et al., 2002).In any case, the higher ability to degrade substrates of theintact lysosomes from paraquat-treated animals was thus a consequenceof increased binding/uptake rather than of higher proteolysisin the lysosomal lumen.

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Figure 3. Additive effect of mild oxidative stress on CMA substrate proteins and on lysosomes. (A) Degradation of [¹⁴C]GAPDH (left) and [¹⁴C]RNase A (right) by lysosomes isolated from rats treated with paraquat as described under Materials and Methods. Incubations were carried out as described in Fig. 2D. Values are the mean + SE of five to eight different experiments (^*p < 0.05, ^**p < 0.01, ^***p < 0.001). (B) Degradation of radiolabeled cytosolic proteins prepared as in Figure 2D from untreated fibroblasts (control) or from fibroblasts exposed to H₂O₂ (left) or paraquat (right), by intact liver lysosomes from untreated rats (Lysosomes control) or from rats treated with paraquat (Lysosomes PQ) as described under Materials and Methods. Proteolysis was calculated as in Figure 2D. Values are mean + SE of six different experiments. ^*, differences compared with lysosomes control; +, differences compared with cytosol control; ${dagger}$ , differences comparing lysosomes and cytosol control, to lysosomes and cytosol treated (^*p < 0.05, ^**p < 0.01, ^***p < 0.001).

We then determined whether oxidative stress could increase CMA-mediateddegradation of proteins by acting on both the substrates, increasingtheir ability to be taken up by the lysosomes, and on the lysosomes,increasing their ability to take up substrates. For that purpose,we verified first that, as described above for GAPDH and RNaseA, cytosolic proteins from untreated fibroblasts were more readilydegraded by intact lysosomes from paraquat-treated rats thanby lysosomes from untreated rats (Figure 3B). Then, we analyzedthe effect of combining lysosomes and cytosolic proteins thathad been both exposed to the prooxidant. When we incubated thelysosomes from paraquat-treated rats with the cytosolic proteinsisolated from fibroblasts treated with H₂O₂ (Figure 3B, left)or with paraquat (Figure 3B, right), we found that these proteinswere degraded even faster. We obtained similar results usinglysosomes isolated from H₂O₂ treated fibroblasts (our unpublisheddata). Based on this additive effect, we conclude that not onlyoxidation-induced changes in the substrate proteins, but alsoin the lysosomal compartment, are responsible for the higherrates of CMA observed during oxidative stress.

We further analyzed the activation of CMA during oxidative stressby separately analyzing binding and uptake of unmodified substrateproteins by lysosomes isolated from paraquat-treated rats. Inthese studies, to eliminate any possible differences in theability of exogenous proteases to remove the protein bound tothe cytosolic side of the lysosomal membrane, we compared insteadthe amount of substrate associated to lysosomes previously treatedor not with a strong cocktail of protease inhibitors. In theabsence of protease inhibitors the substrate that translocatesinside the lysosomal lumen is rapidly degraded by the lysosomalproteases (half-life of proteins in the lysosomal lumen is 5–7min; Aniento et al., 1993). Consequently, the protein associatedto the lysosomes at the end of the incubation represents theprotein bound to the cytosolic side of the lysosomal membrane(Salvador et al., 2000). In contrast, if lysosomal proteasesare inhibited, the protein recovered associated to lysosomescorresponds to both protein bound and internalized into thelysosomal lumen. As described previously, the amount of internalizedsubstrate can then be calculated by subtracting the proteinbound from the amount of protein associated (Salvador et al.,2000). Consistent with our previous results, the amount of GAPDHand RNase A bound to the lysosomal membrane was significantlyhigher (4- to 5-fold increase) in lysosomes from paraquat-treatedrats (Figure 4A). A two- to threefold increase was also detectedin the uptake of both substrates by these lysosomes, when calculatedas described above (Figure 4A, bottom). We have previously shownthat CMA is activated under starvation conditions (Cuervo etal., 1995). When we compared both stimuli, starvation and paraquat,we found that treatment with the prooxidant agent resulted instronger activation of CMA. Levels of binding and uptake ofboth substrates were significantly higher in lysosomes isolatedfrom fed rats treated with paraquat than in lysosomes from 48-hstarved animals. To determine whether the observed increasein CMA during paraquat treatment could be due, at least in part,to some degree of starvation in this group of animals, we measuredfood-intake in the animals exposed to paraquat. However, wedid not find significant differences in food consumption betweenthe paraquat-treated and untreated animals when maintained inad libitum conditions, suggesting that activation of CMA afterparaquat treatment was not due to starvation, but to the oxidativestress.

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Figure 4. Activation of CMA during mild oxidative stress. (A) Association and binding of GAPDH and RNase A to intact lysosomes from untreated fed rats, 48-h starved rats (Strv) or fed rats treated with paraquat (PQ). Lysosomes in lanes 1–3 were preincubated with chymostatin to prevent protein degradation. Incubations were carried out in an isotonic buffer, as described under Materials and Methods, and levels of associated proteins were determined by immunoblot of the lysosomes collected by centrifugation. Bottom: densitometric quantification (mean + SE) of 4–6 immunoblots similar to the ones shown here. Values are expressed as the fold of increase in binding and in uptake (association-binding) for the lysosomes from starved or paraquat-treated rats, compared with lysosomes from untreated fed animals. ^*, differences compared with fed animals; +, differences compared with starved animals (^*p < 0.1, ^**p < 0.05, ^***p < 0.01) (B) Immunofluorescence for lamp2a (red) and lamp1 (green) in mouse fibroblasts after removing the serum from the culture medium (serum-) or after treatment with paraquat in cells maintained in serum supplemented medium. The merged image of both fluorochrome channels is shown. Bar, 50 µm.

Activation of CMA is associated with the relocalization towardthe perinuclear region of the lysosomes with higher CMA activity(those with higher levels of lys-hsc70 and lamp2a) (Agarrabereset al., 1997; Cuervo and Dice, 2000c). As shown in Figure 4B,in culture fibroblasts maintained in the presence of serum,lamp2a colocalized with other lysosomal membrane proteins (lamp1is shown here), displaying a typical vesicular punctated pattern.When serum was removed from the culture medium, the lamp2a-enrichedlysosomes preferentially localized in the perinuclear region.Treatment with paraquat displayed a similar perinuclear patternfor lamp2a even when the cells were maintained in the presenceof serum (Figure 4B, right).

These results are consistent with a constitutive activationof CMA during oxidative stress in the two experimental modelsin which CMA has been better characterized, rat liver and fibroblastsin culture (Terlecky and Dice, 1993; Cuervo et al., 1997).

Oxidative Stress-induced Changes in Lysosomes Active for CMA
Several cytosolic chaperones associate with the lysosomal membraneand are required for CMA substrate binding/uptake into lysosomes(Agarraberes and Dice, 2001). Although the specific functionof each of these cochaperones in CMA remains unknown, studieswith human fibroblasts in culture have revealed that the levelsof some of them are up-regulated when CMA is activated by removalof serum, whereas others remain unchanged (Agarraberes and Dice,2001). In lysosomes isolated from livers of rats starved for48 h, in addition to the previously reported increase in lys-hsc70,we found higher levels of hsp90, and, in less extent, of Hip,compared with lysosomes from control-fed animals (Figure 5A).Treatment with paraquat (in fed rats) resulted in similar increasein the lysosomal content of lyshsc70 and of Hip, but only adiscrete increase in the content of hsp90, when compared withuntreated animals. None of the treatments modified the levelsof other associated chaperones (hsp40 or Bag-1), nor did theyresult in lysosomal association of the inducible form of thehsp70 family, hsp72, which was however elevated in the cytosolafter paraquat treatment (Figure 5A). Because the function ofhsp90 in lysosomes is not known, it is not clear why the increasein its lysosomal levels is not as pronounced as the one observedduring starvation, but because rates of uptake are still up-regulatedunder these conditions, it points to a nonlimiting role forhsp90 in the translocation complex.

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Figure 5. Changes in lysosome-associated chaperones during mild oxidative stress. (A) Cytosol and lysosomes (75 µg of protein) isolated from normally fed, 48-h starved rats (Stv), or fed rats treated with paraquat (PQ) as labeled were subjected to SDS-PAGE and immunoblot for the indicated proteins. Right, densitometric quantification (mean + SE) of the chaperones in the lysosomal fraction in four immunoblots similar to the ones shown here. Levels in lysosomes from fed animals were given an arbitrary value of 1 (dotted line). ^*, differences compared with fed animals (^*p < 0.1, ^**p < 0.05, ^***p < 0.01). (B) Lysosomes with high (CMA+) and low (CMA-) activity for CMA (Cuervo et al., 1997

) were isolated from the same groups of animals as detailed in A. After hypotonic shock and centrifugation, membranes and matrices (50 µg of protein) were separated and subjected to SDS-PAGE and immunoblot for hsc90 (top) or hsc70 (bottom).

Two components have been shown to be rate-limiting in the uptakeof CMA substrates by lysosomes: the chaperone in the lysosomallumen (lys-hsc70) (Cuervo et al., 1997; Agarraberes et al.,1997) and the receptor at the lysosomal membrane (lamp2a) (Cuervoand Dice, 2000b,c). We have previously reported in rat liverthe presence of two lysosomal populations with similar morphologicaland enzymatic characteristics but different CMA activity (Cuervoet al., 1997). The main difference found, so far, between thesetwo groups of lysosomes is the enrichment of lys-hsc70 in thelumen of the lysosomes with higher CMA activity (Cuervo et al.,1997). These two groups of lysosomes are normally purified together(they contribute 75 and 25% high activity and low activity,respectively, to the fraction that we used in these studies),but can be physically separated by further density and differentialcentrifugation (Cuervo et al., 1997). The lysosomes with lowerCMA activity can become more active under specific conditions,such as prolonged (88-h) starvation or aging, which correlateswith an increase in their lumenal levels of lys-hsc70 (Cuervoet al., 1997; Cuervo and Dice, 2000a). Because we found higherlevels of lyshsc70 in the lysosomes from paraquat-treated animals,we separated these two lysosomal subpopulations to determinewhether there was a net increase in lys-hsc70 per lysosome,or it resulted from enrichment of the less active lysosomesin lys-hsc70. As shown in Figure 5B, after treatment with paraquatthere were no significant changes in the content of lys-hsc70in the membranes or matrices of the less active group. Accordingly,the ability of this group of lysosomes to selectively take upCMA substrates did not change in paraquat-treated rats (ourunpublished data). The percentage of hsc70-enriched lysosomes,determined as recovery of hexosaminidase activity in this fraction,was similar in untreated and paraquat-treated rats (our unpublisheddata). For the more active group of lysosomes, as observed duringstarvation, levels of lys-hsc70 at the lysosomal membrane remainedconstant, whereas levels of lys-hsc70 in the lysosomal lumenincreased approximately fourfold. Separation of the lysosomalmembranes and matrices also revealed that hsp90 increased inboth compartments during starvation and after paraquat treatment(Figure 5B, top), but the increase in the lumen of lysosomesfrom paraquat-treated rats was smaller than in starved animals.These differences in the luminal content of hsp90 could explainwhy, when working with total lysosomes (Figure 5A), we foundthat paraquat induced a lower increase in lysosomal levels ofhsp90 than starvation. Whether this hsp90 in the lysosomal lumenis functional, or whether it is only internalized to be degraded(amino acid sequence analysis of hsc90 revealed the presenceof two KFERQ-related motifs) remains unknown.

Levels of lamp2a at the lysosomal membrane directly correlatewith CMA activity (Cuervo and Dice, 2000b). Lysosomes isolatedfrom mouse fibroblasts treated with H₂O₂ (Figure 6A) or fromlivers of rats exposed to paraquat (Figure 6B) had higher levelsof lamp2a at their membrane than lysosomes isolated from thecorresponding untreated controls. This increase seems selectivefor lamp2a, because levels of other lysosomal membrane proteins(lamp1 shown here) remained unchanged. In agreement with thebinding and uptake data (Figure 4A), the increase of lamp2ain the lysosomal membrane induced by paraquat was higher thanthe one induced by starvation (Figure 6C). For the two otherlysosomal membrane proteins analyzed, levels of lamp1 remainedunchanged in both conditions, and levels of lamp2c were notaffected by the treatment with paraquat, but decreased significantlyduring starvation. Whether this decrease in lamp2c content isrelated to the increase in lamp2a or it happens independentlyis currently under investigation.

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Figure 6. Lamp2a levels at the lysosomal membrane increase during mild oxidative stress. (A and B) Immunoblot for lamp2a and lamp1 of homogenates (50 µg of protein), lysosomal membranes (L. Memb) and lysosomal matrices (L. Matrix) (10 µg of protein) isolated from cultured mice fibroblasts, exposed or not to 100 µM H₂O₂ (A) or from liver of rats treated or not with paraquat (PQ). (C) Imunoblot for lamp2a, lamp2c, and lamp1 of lysosomal membranes isolated from livers of fed rats, 48-h starved (Strv) rats, or fed rats treated with paraquat (PQ). Right, densitometric quantification of six to eight immunoblots as the ones shown here. Values are expressed as fold of the values in fed untreated animals and are the mean + SE of six different experiments. Levels in lysosomes from fed animals were given an arbitrary value of 1. ^*, differences compared with fed animals (^*p < 0.05, ^**p < 0.01, ^***p < 0.001).

A Novel Mechanism for Activation of CMA during Oxidative Stress
We have previously shown that CMA activity can be modulatedby changes in the levels of lamp2a at the lysosomal membrane(Cuervo and Dice, 2000b). In fact, overexpression of lamp2aresults in higher rates of CMA proportional to the increasein the receptor protein (Cuervo and Dice, 1996, 2000c). Duringstarvation, the most extensively studied stimuli for CMA, theincrease of lamp2a at the lysosomal membrane does not resultfrom de novo synthesis of the protein. Instead, a decrease inthe degradation rate of lamp2a, along with the relocation ofpart of the lamp2a resident in the lysosomal lumen toward thelysosomal membrane account for most of the lamp2a increase inthe membrane (Cuervo and Dice, 1996, 2000c). To determine whethersimilar mechanisms were responsible for the increased levelsof lamp2a during oxidative stress, we first compared the ratesof degradation of lamp2a in membranes of lysosomes from ratsfed, starved, or treated with paraquat. In contrast with thesignificant reduction in lamp2a degradation induced by starvation,degradation of lamp2a was only slightly slower in rats treatedwith paraquat than in untreated fed rats (Figure 7A). Likewise,the distribution of lamp2a between membrane and matrix was notsignificantly affected by the treatment with paraquat, suggestingthat the increased levels of lamp2a in the membrane were notthe result of recruitment of the lamp2a normally present inthe lumen (Figure 7B).

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Figure 7. A novel mechanism for activation of CMA during mild oxidative stress. (A) Degradation of lamp2a in isolated membranes from normally fed rats, 48-h starved rats, or fed rats treated with paraquat (PQ), as indicated under Materials and Methods. Degradation of lamp2a was followed by immunoblot of the lysosomal membranes with an antibody specific against its cytosolic tail, at different times of the incubation. Values are the mean + SD of the densitometric quantification of immunoblots from four different experiments. A representative immunoblot is shown in the top insets. (B) Distribution of lamp2a between the lysosomal membrane and the matrix in lysosomes isolated from normally fed rats, treated or not with PQ. Values are mean + SE of the densitometric quantification of four immunoblots similar to the one shown in Figure 6B. (C) A 120-nucleotide fragment of lamp2a and a 108-nucleotide fragment of actin were amplified, through PCR, from increasing concentrations of total mRNA isolated from the livers of normally fed, 48-h starved, or paraquat-treated fed rats. The electrophoretic pattern of the products in a 2% agarose gel is shown. (D) Semiquantitative real-time PCR was used to compare mRNA expression levels for lamp2a in the same samples as detailed in C. Values were corrected for actin amplification in each samples and are expressed as fold increase compared to mRNA lamp2a values in fed untreated rats (that was given an arbitrary value of 1). Values are mean + SD for four different experiments. ^*, differences compared with fed animals (^**p < 0.01, ^***p < 0.001).

Contrary to starved animals, levels of lamp2a mRNA in the liverof rats treated with paraquat were significantly higher thanin untreated rats. We used both a dilution-based quantitativePCR method (Figure 7C) and real-time PCR (Figure 7D) to comparelevels of lamp2a mRNA in livers from fed, starved, or paraquat(fed)-treated rats. Treatment with paraquat induced an increasein lamp2a mRNA levels of approximately sixfold in fed animals,whereas starvation resulted in a slight decrease in lamp2a mRNAlevels. Therefore, contrary to starvation, where the increasein lamp2a levels did not require new protein to be synthesized,most of the increase in lamp2a levels detected in paraquat-treatedanimals was a consequence of de novo synthesis of the protein.

We conclude that activation of CMA is part of the normal oxidativestress response and it contributes to the selective removalof oxidized proteins from the cytosol. The higher rates of CMAobserved under these conditions are the combined result of anincrease in the susceptibility of the proteins to be taken upand degraded by lysosomes, and an enhanced ability of the lysosomesfor substrate uptake. Unexpectedly, during mild oxidative stress,activation of CMA is mediated by a novel mechanism differentfrom the previously characterized activation of CMA during nutritionalstress.

DISCUSSION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
ACKNOWLEDGMENTS
REFERENCES

Our results provide for the first time evidence for the participationof lysosomes in the removal of oxidized proteins during mildoxidative stress through CMA. This novel role for CMA is supportedby the fact that 1) oxidized proteins can be detected in thelumen of lysosomes active for CMA (Figure 1); 2) in conditionswith declined CMA, such as aging, the amount of oxidized proteinstranslocated into lysosomes is reduced (Figure 1B); 3) oxidizedCMA substrates bind and are taken up more efficiently by isolatedlysosomes than their unmodified forms (Figure 2); 4) lysosomesfrom cells or rats exposed to prooxidants display higher ratesof binding and uptake of CMA substrate proteins (Figures 3 and4); and 5) blockage of CMA in cultured cells increases theirsusceptibility to prooxidant compounds and decreases their viability(Massey, Kiffin, and Cuervo, unpublished data). Activation ofCMA during oxidative-stress is attained through the up-regulationof specific components of the lysosomal translocation complex(lysosomal chaperones and the lysosomal membrane receptor) (Figures5 and 6). Interestingly, although these changes are similarto the ones described when CMA is activated by nutritional stress,the mechanism involved in the up-regulation is different. Therefore,this finding suggests that stress-mediated activation of CMAvaries depending on the nature of the stress.

Most of the previous studies on the lysosomal role during oxidativestress have focused on the contribution of this subcellularcompartment to the oxidative damage, rather than on a possibleprotective role. In fact, the destabilizing effects of severeoxidative stress (>350 µM hydrogen peroxide) on lysosomeshave been well documented (Brunk et al., 1995; Ollinger andBrunk, 1995), showing that the release of lysosomal enzymesplays a major role in intracellular damage and in cell deathunder these conditions. Lower concentrations of hydrogen peroxide(250 µM for 30 min) still cause leakage of some lysosomalenzymes, although the lysosomal damage is reversible (Brunket al., 1995; Ollinger and Brunk, 1995). In our study, we didnot find changes in the stability of the lysosomal membrane,assayed either as release of specific enzymes or with a moresensitive proteolytic method. It is possible that the lowerdoses of hydrogen peroxide and paraquat used in our study (100µM and 40 mg/100 g body weight, respectively) were enoughto originate cytosolic protein damage, but they did not alterthe lysosomal compartment. Other possibility is that the initiallysosomal damage still takes place. but due to its reversibilityunder these conditions (Brunk et al., 1995; Ollinger and Brunk,1995), it is not longer detectable by the time the lysosomesare isolated (24 h after the second injection). In addition,because most of the studies regarding lysosomal stability andoxidative stress have been performed in intact cells, analyzingthe leakage of fluorescent probes from the lysosomal compartment,we cannot discard that different lysosomal populations mightbe differently affected by prooxidants. In our assays, the cellfractionation method used has been optimized to isolate a subsetof intracellular lysosomes active for CMA (10–15% of total)(Cuervo et al., 1997). Particular characteristics of the CMA-activelysosomes, such as, for example, a lower concentration of ironin their lumen, could explain their higher resistance to prooxidants.Our studies on CMA-active lysosomes in old animals also supporttheir unique characteristics. Thus, although accumulation oflipofuscin in lysosomes is a commonly used biomarker of aging,CMA-active lysosomes from old rat livers rarely accumulate thispigment (Cuervo and Dice, 2000a).

The ability of proteasomes to degrade oxidized proteins hasbeen previously well documented in vitro (Rivett, 1985; Davies,2001), and more recently in vivo (Grune et al., 2002a; Hosleret al., 2003; Shringarpure et al., 2003). Most of the studiesassessing oxidation-induced changes in lysosomal proteolyticbehavior have focused in the analysis of the enzymatic activityof cathepsins, the lysosomal proteases. Moderate oxidative stressdoes not significantly change the activity of most cathepsins,whereas more severe oxidizing conditions result in increasedor decreased cathepsin activity depending on the cellular conditions(Sitte et al., 2000a,b). This lack of correlation between theintracellular accumulation of oxidized proteins and the activityof lysosomal enzymes sets the basis for arguments against thelysosomal participation in removal of oxidized proteins (Sitteet al., 2000a). However, the activity of the lysosomal proteasesis a nonlimiting step for any of the forms of autophagy. Theintralysosomal concentration of cathepsins is such that, oncesubstrates reach the lysosomal lumen, they are rapidly degraded.This makes the delivery of substrates the limiting step. Bergaminiand colleagues were one of the first groups to point out that,if the degradation of proteins by lysosomes, instead of theenzymatic activity of lysosomal proteases, is considered, thereis a good inverse correlation between lysosomal proteolysisand intracellular content of oxidized proteins (Vittorini etal., 1999). Our current study also supports a good correlationbetween the intracellular content of oxidized proteins and thedelivery of substrate to lysosomes via CMA (binding/uptake).We have previously shown that, in the group of lysosomes activefor CMA, the activity of most lysosomal enzymes does not changesignificantly with age, and yet rates of CMA are lower in agedcells (Cuervo and Dice, 2000a). The impaired ability of thisgroup of lysosomes to take up substrates in older animals couldexplain why there is a lower content of oxidized proteins intheir lumen, despite the higher level of oxidized cytosolicproteins (Figure 1B). It is unlikely that the lower levels ofoxidized proteins detected in the lysosomal lumen of old rats,result from faster degradation of these proteins inside lysosomes,because even when we inhibited lysosomal degradation in rats,before lysosomal isolation (by i.p. of leupeptin; our unpublishedresults), we still found lower content of oxidized proteinsin the lysosomes from the oldest animals.

The contribution of proteasomes to the removal of oxidized proteinsin vivo has been demonstrated by analyzing the consequencesof blocking its catalytic activity in oxidized protein removal(Grune et al., 2002a; Hosler et al., 2003; Shringarpure et al.,2003). This approach, however, cannot be used to evaluate thecontribution of autophagy in this process. Even if the lysosomalproteases are inhibited (either with specific protease inhibitorsor by raising the intralysosomal pH), we do not expect to findchanges in the cytosolic content of oxidized proteins, becauseonly their proteolysis, but not their translocation into thelysosomal lumen, would be blocked. The accumulation of undegradedproducts in the lysosomal lumen can be tolerated for a longtime without affecting their translocation ability. An alternativeapproach would be to directly inhibit the delivery of the substrates.No chemical inhibitors are available to block CMA. We have recentlysucceeded in blocking substrate translocation by using RNA interferenceagainst the lysosomal receptor in cultured fibroblasts (Massey,Kiffin, and Cuervo, unpublished data). As mentioned before,these cells have a lower resistance to oxidative stress. However,even in this system, it is difficult to asses lysosomal versusproteasome contribution, because blockage of CMA results inchanges in the composition of the 20S/26S proteasomes and, consequently,in its proteolytic activities (Massey, Kiffin, and Cuervo, unpublisheddata). Likewise, chronic inhibition of proteasomes, similarto the one that occurs in aging, alters the ability of the cellsto activate autophagy in response to stress (Ding et al., 2003).Although an experimental challenge, this cross-talking amongthe different proteolytic systems offers perhaps a more physiologicalview of what is really happening in the cells during oxidativestress. In the same way that the relative contribution of proteasomesand lysosomes to total protein degradation varies dependingon the cell type and on the cellular conditions (Fuertes etal., 2003), participation of these two systems in the removalof oxidized proteins is probably also dynamic. In fact, thereare now numerous examples of proteins that can be degraded bymore than one proteolytic pathway (Cuervo et al., 1998; Lenket al., 1999). Future studies should be directed at understandinghow those fluctuations are regulated and to identify possibleways of stimulating one system to compensate for the failureof another.

Whereas during severe oxidative stress, protein aggregationand cross-linking are common events, mild oxidative stress hasbeen shown to generate excellent proteolytic substrates (Gruneet al., 1995; Gomes-Marcondes and Tisdale, 2002). Our work supportsthat in the case of CMA, mild oxidation of CMA substrates facilitatesnot only their degradation by lysosomal proteases but also theirbinding/translocation across the lysosomal membrane (Figure 4A).Although the exact mechanism behind this facilitated uptakeis still elusive, we hypothesize that protein unfolding, likelyto occur during oxidation (Imai et al., 2003), could accelerateuptake, by diminishing the time required for substrate unfoldingbefore translocation. Oxidized substrates were taken up fasterby lysosomes even when we did not add cytosolic hsc70 in thetranslocation cocktail (our unpublished data). However, becausethe isolated lysosomes contain significant amounts of hsc70in the cytosolic side of the membrane, we cannot discard thatpartial unfolding might make the KFERQ-motif more accessiblefor the interaction with hsc70 and facilitate in this way unfolding/translocationof the substrate. Our unpublished data showing that manipulations,such as partial denaturation of CMA substrates or extensivetruncation, increase their rates of uptake into lysosomes viaCMA (Salvador, Aguado, Cuervo, and Knecht, unpublished data),also support the proposed facilitating role of partial proteinunfolding under mild oxidative conditions. Whether the activationof CMA under these conditions is a response to the presenceof these partially unfolded proteins in the cytosol, or it ismediated by other cytosolic components generated during theoxidative stress remains to be elucidated.

An interesting remaining question is how the cells decide whetheran oxidized protein should be degraded by the proteasome orin the lysosomal compartment. About 30% of cytosolic proteinscontain a KFERQ-motif, suggesting that, in theory, this wouldbe the subset of proteins degraded through CMA during mild oxidativestress (Figure 1A). However, a very intriguing idea proposedby Gracy et al., 1998 is that some amino acid modifications,such as deamidation and oxidation, could result in the generationof KFERQ-like containing motifs in proteins previously lackingthis sequence. As other targeting motifs, the KFERQ-like motifis degenerate, resulting from the combination of a basic, ahydrophobic and an acid residue with a fourth basic or hydrophobicresidue, flanked on either side by a glutamine. Oxidation forexample of a histidine to aspartic acid could provide the acidresidue necessary to complete a KFERQ-like motif. On the otherhand, the same process could eliminate KFERQ-like motifs inproteins that normally are substrates for this pathway, resultingin their impaired degradation in conditions such as aging. Thismodification of the targeting motif, added to the fact thatCMA activity decreases with age, could explain the lower contentof oxidized proteins in the lumen of CMA active lysosomes inold rats, despite the higher levels of oxidized proteins intheir cytosol. Our laboratory is currently trying to identifychanges in the targeting motif of CMA substrates with age usinga shot-gun proteomic approach.

Particularly exciting is the finding that although activationof CMA during oxidative and nutritional stress have the sameconsequences on the levels of the lysosomal translocation components,up-regulation, at least for the lysosomal receptor, obeys differentmechanisms. During starvation CMA is activated to supply thecells with amino acids required for the synthesis of essentialproteins. Under these conditions, de novo synthesis of lamp2ato increase CMA rates is probably not a reasonable option dueto the shortage of amino acids. Instead, more conservative mechanisms(down-regulation of lamp2a degradation and intralysosomal relocation)are adopted (Cuervo and Dice, 2000b). If oxidative damage takesplace under normal nutritional conditions, as the supply ofamino acids would not be compromised, de novo synthesis of lamp2ais up-regulated to activate CMA (Figure 7C). De novo synthesismight be advantageous under these conditions, because it providesa faster mechanism for CMA activation.

In conclusion, we have identified for the first time a roleof CMA as part of the oxidative stress response. Because CMAactivity is severely impaired during aging, we hypothesize thatpart of the accumulation of oxidized proteins observed in oldorganisms may result from the malfunctioning of CMA. Futureefforts aimed to restore normal CMA activity in old cells wouldhelp to understand the relevance of the cross-talk among differentproteolytic pathways, and the compensatory mechanisms activatedwhen the activity of one or more of these pathways is compromised.

ACKNOWLEDGMENTS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
ACKNOWLEDGMENTS
REFERENCES

We gratefully acknowledge Dr. Fernando Macian and the othermembers of our laboratory for valuable suggestions and comments.This work was supported by the National Institutes of Health/NationalInstitute on Aging grant AG-021904, by an Ellison Medical FoundationResearch Award (to A.M.C.), and by the Ministerio de Cienciay Tecnología of Spain grants BMC2001-0816 and SAF2002-00206and Fondo de Investigación Sanitaria grant RGDMG031212(to E.K.). R.K. is a National Institutes of Health/NationalInstitute on Aging postbachelor fellow.

Footnotes

Article published online ahead of print. Mol. Biol. Cell 10.1091/mbc.E04–06–0477.Article and publication date are available at www.molbiolcell.org/cgi/doi/10.1091/mbc.E04–06–0477.

Abbreviations used: CMA, chaperone-mediated autophagy; GAPDH,glyceraldehide-3-phosphate dehydrogenase; hsc70, heat shockcognate protein of 70 kDa; lamp, lysosomal associated membraneprotein; MOPS, 3-(N-morpholino)propanesulfonic acid; RNase A,ribonuclease A.

The online version of this article contains supplementary materialaccessible through http://www.molbiolcell.org.

Corresponding author. E-mail address: amcuervo{at}aecom.yu.edu.