(Received for publication, April 23, 1996, and in revised form, November 20, 1996)
From the Instituto de Investigaciones
Citológicas, 46010 Valencia, Spain and the
§ Department of Physiology, Tufts University School of
Medicine, Boston, Massachusetts 02111
Two populations of rat liver lysosomes can be distinguished on the basis of their density. A major difference between these populations is that one contains the heat shock cognate protein of 73 kDa (hsc73) within the lysosomal lumen. The lysosomal fraction containing hsc73 exhibits much higher efficiencies in the in vitro uptake and degradation of glyceraldehyde-3-phosphate dehydrogenase and ribonuclease A, two well established substrates of the selective lysosomal pathway of intracellular protein degradation. Preloading of the lysosomal population that is devoid of lumenal hsc73 with hsc73 isolated from cytosol activated the selective transport of substrate proteins into these lysosomes. Furthermore, treatment of animals with leupeptin, an inhibitor of lysosomal cathepsins, or 88 h of starvation also increased the amount of hsc73 within their lysosomal lumen, and these in vivo treatments also activated the selective transport of substrate proteins in vitro. Thus, the hsc73 located within lysosomes appears to be required for efficient uptake of cytosolic proteins by these organelles. The difference in hsc73 content between the lysosomal populations appears to be due to differences in their ability to take up hsc73 combined with differences in the intralysosomal degradation rates of hsc73. The increased stability of hsc73 in one population of lysosomes is primarily a consequence of this lysosomal population's more acidic pH.
In eukaryotic cells, lysosomes participate in intracellular protein degradation by a variety of pathways including macroautophagy, microautophagy, crinophagy, endocytosis, and a selective uptake of cytosolic proteins (1-4). The selective pathway of lysosomal proteolysis, first described in serum-deprived confluent cultured fibroblasts (5), is also operative in rat liver, especially after prolonged starvation (6, 7). The pathway has been reconstituted in vitro with lysosomes isolated from human fibroblasts (8, 9) and from rat liver (10, 11). Specific substrates of this pathway include: ribonuclease A (RNase A)1 and RNase S-peptide (residues 1-20 of RNase A), where the pentapeptide KFERQ appears to be required for their lysosomal uptake (12, 13), and glyceraldehyde 3-phosphate dehydrogenase (GAPDH; Ref. 10).
The selective pathway of lysosomal proteolysis resembles in many respects the import of proteins synthesized on cytosolic ribosomes into the endoplasmic reticulum, mitochondria, peroxisomes, and nucleus. Thus, uptake of cytosolic proteins by lysosomes is saturable and time- and temperature-dependent (9-11). Substrates for lysosomal import compete with each other (11), and intermediates in the import process can be identified for certain protein substrates (11). In addition, uptake of selective cytosolic proteins by lysosomes is stimulated by ATP/MgCl2 and a cytosolic heat shock protein, the heat shock cognate protein of 73 kDa (hsc73; Ref. 8), and requires protein-containing components of the lysosomal membrane (9, 11). Recently, lgp96 has been identified as the protein responsible for the binding of RNase A and GAPDH to the lysosomal membrane (14). Furthermore, import of proteins into the endoplasmic reticulum (15, 16) and mitochondria (17, 18) requires an organellar form of a heat shock protein of 70 kDa (hsp70), and some hsc73, most probably a specific isoform, is localized to the lysosomal lumen and is required for the operation of this pathway of proteolysis (19, 20), most likely for the import of protein substrates into the lysosomal lumen.
It is well known that lysosomes are morphologically and biochemically heterogeneous (i.e. Refs. 21-24 and references cited therein). In our previous studies of the uptake of GAPDH and RNase A by rat liver lysosomes we noticed, by immunogold procedures, apparent differences among individual lysosomes in their ability to take up selective protein substrates (7, 10). We also observed that hsc73 was present within some, but not all, lysosomes, and that it colocalized with RNase A transported into the lysosomes (7). The amount of lysosomal hsc73 increased by 5-10-fold during prolonged starvation, and this increase was due to both an increase in the number of hsc73 molecules per lysosome and also to an increase in the percentage of lysosomes containing hsc73 (7).
Little is known about the mechanism(s) by which hsc73 reaches the lysosomal matrix, but hsc73, like many cytosolic proteins, can presumably enter lysosomes through macroautophagy and microautophagy. In addition, hsc73 may enter lysosomes by the selective import pathway that it stimulates, because two KFERQ motif peptides exist in hsc73 (13). Once in the lysosomal matrix hsc73 is relatively resistant to intralysosomal hydrolysis (19).
In this paper we characterize in rat liver the specific lysosomal population containing hsc73 to gain more insights into the role of intralysosomal hsc73 in the selective uptake of cytosolic proteins. We show that the hsc73 located within lysosomes is of paramount importance for the uptake of cytosolic proteins by these organelles. Lysosomes that contain hsc73 have increased rates of uptake and decreased rates of intralysosomal proteolysis of hsc73, when compared with lysosomes that do not contain hsc73. Finally, the resistance of hsc73 to intralysosomal hydrolysis is explained, at least in part, by the slightly more acidic pH of this population of lysosomes.
Male Wistar rats weighing 200-250 g were fasted for 20 h prior to use. In some experiments fasting was prolonged for 88 h. For experiments with leupeptin, rats received the drug (2 mg/100 g of body weight by intraperitoneal injection) 1 h before sacrifice. All rats were fed ad libitum for at least 7 days before the experiments began.
ChemicalsSources of chemicals and antibodies were as described previously (7, 9-11) with the following additions: fluorescein isothiocyanate-dextran (FITC-dextran) (average molecular weight, 67 kDa; 0.007 mol fluorescein/mol glucose), glutathione-agarose and bafilomycin A were from Sigma; Trans35S-labelTM was from ICN Pharmaceuticals Inc. (Costa Mesa, CA); antibodies against cathepsin L and against the cation-insensitive mannose 6-phosphate receptor were generous gifts from Dr. G. Sahagian (Tufts University, Boston, MA), and the antibody against the lysosomal glycoprotein of 120 kDa (lgp120) was from Dr. I. Mellman (Yale University, New Haven, CT); antibodies against hexokinase, aldolase, 3-phosphoglycerate kinase, and phosphoglycerate mutase were raised in rabbits against the purified proteins following standard procedures (25). Other reagents were of the best analytical quality available. Glutathione transferase (GST)-hsc73, a fusion protein of hsc73 with GST at its amino terminus was obtained from a plasmid (pGX-2T, Pharmacia Fine Chemicals, Uppsala, Sweden) containing a human cDNA encoding hsc73 (26).
Isolation of Lysosomal FractionsLysosomes were isolated from a light mitochondrial fraction in a discontinuous metrizamide density gradient (27) by the shorter method previously reported (10). Fractions from the top layer (fraction 1) and the 26.3/19.8% metrizamide interface (fraction 2) were collected separately, diluted five times with 0.3 M sucrose, and sedimented at 37,000 × g for 10 min in a Sorvall centrifuge (rotor SS-34; DuPont Instruments, Herts, UK). Lysosomes from fractions 1 and 2 were resuspended in 0.3 M sucrose and centrifuged again at 10,000 × g for 5 min in a Heraeus Biofuge 28RS (rotor HFA 22.1; Heraeus Sepatech, Osterode, Germany) to separate pellets (P1 and P2, respectively) and supernatants (S1 and S2, respectively).
Lysosomal membranes from P1 and P2 were obtained as described by Ohsumi et al. (28). Briefly, P1 and P2 were subjected to hypotonic shock in 0.025 M sucrose for 30 min at 0 °C and centrifuged for 30 min at 105,000 × g in a Beckman L8M ultracentrifuge (rotor 60 Ti) (Beckman Instruments Inc., Palo Alto, CA). The supernatants (lysosomal matrix) were used as such, and the pelleted membranes were washed once with 0.5 M NaCl and then resuspended in 0.3 M sucrose to the original volume.
Proteolysis MeasurementsFreshly isolated lysosomes (25 µg of protein) were incubated (final volume, 60 µl) with protein substrates. The substrates used were: GAPDH (230 nM) radiolabeled by reductive methylation with [14C]formaldehyde (29) to a specific radioactivity of 1.2 × 106 dpm/nmol, RNase S-peptide (35 nM) radiolabeled by reductive methylation with NaB3H4 (30) to a specific radioactivity of 1.1 × 107 dpm/nmol or GST-hsc73 (200 nM) metabolically labeled in Escherichia coli with a mixture of [35S]methionine and cysteine (Trans35S-labelTM) to a specific radioactivity of 7.3 × 106 dpm/nmol. Except where indicated, incubations were carried out at 37 °C for 30 min in 0.3 M sucrose, 10 mM MOPS, pH 7.2. They were stopped by the addition of trichloroacetic acid to a final concentration of 10% or, in the RNase S-peptide experiments, phosphotungstate in HCl to a final concentration of 3.25 and 5%, respectively. The acid-soluble material was collected as flow through after filtration in the Millipore Multiscreen Assay System (Millipore, Bedford, MA) using a 0.45-µm pore membrane. Radioactivity in the samples was measured in a Beckman LS-7800 liquid scintillation counter (Pharmacia Biotech, Brussels, Belgium), and quenching was corrected by the external standard method. Proteolysis, after subtracting the acid-soluble radioactivity at time zero, was expressed as percentage of the initial acid-insoluble radioactivity converted to acid-soluble radioactivity and normalized to lysosomal protein. ATP and MgCl2 were used at 10 mM each alone or with 10 µg/ml hsc73 in some experiments.
Incubation Conditions to Study the Uptake of Proteins into LysosomesFreshly isolated lysosomes (100 µg of protein) were
incubated in a final volume of 30 µl with protein substrates (25 µg
of RNase A or 50 µg of GAPDH) at 37 °C for 20 min in 0.3 M sucrose and 10 mM MOPS buffer (pH 7.2). When
studying hsc73 uptake, incubations were carried out with a GST-hsc73
fusion protein (2 µg) metabolically labeled with a mixture of
[35S]methionine and cysteine (see above) and purified
over a glutathione-agarose column. Chymostatin and other protease
inhibitors, when used, were added to the lysosomes at 0 °C for 10 min at three times their final concentrations and then diluted 3-fold
into the incubation medium with substrates. Proteinase K treatments
were carried out as described previously (10). The integrity of the
lysosomal membranes was judged by the latency of the lysosomal enzyme,
-hexosaminidase (11), or by the leakage of proteolytic activity into
the medium (10).
For conventional electron microscopy, isolated lysosomes were double fixed (glutaraldehyde and OsO4), embedded in Vestopal W, and stained with lead citrate by standard procedures (10). Ultrathin sections were cut with a LKB 4801 A ultramicrotome and observed in a Philips CM-10 electron microscope. Morphometric analysis (7) was performed in randomly selected electron micrographs at a final magnification of 25,000-35,000×. Average diameters and areas of the lysosomal profiles were measured in the electron micrographs. Form factors (1.00 for a perfect circle and decreasing with increasing deviation from this form) were calculated as described by Lüers et al. (31).
Intralysosomal pH MeasurementsThe intralysosomal pH was monitored by measuring FITC-dextran fluorescence as described in Ohkuma et al. (32). Briefly, FITC-dextran was injected intraperitoneally into rats (15 mg/100 g of body weight), and after 20 h lysosomes were isolated. FITC florescence in lysosomes was measured in a spectrofluorometer at 25 °C at 495 nm (pH-sensitive fluorescence) and 450 nm (pH-insensitive fluorescence) excitation and 550 nm emission wavelengths. Double standard curves were prepared by measuring the ratio of fluorescence intensities at 495 nm/fluorescence at 450 nm for 2 mg of FITC-dextran at different pHs and in different buffers and by comparing the fluorescence intensities, at 495 nm excitation wavelengths, in intact lysosomes and after disruption of lysosomes with 0.1% Triton X-100. Intralysosomal pHs in the isolated lysosomes were calculated with these curves from their ratio of the 495/450 nm fluorescence intensities, after subtracting the background fluorescence.
General MethodsSDS-polyacrylamide gel electrophoresis (PAGE) (10, 12, or 17% gels for studies with hsc73, GAPDH, or RNase A, respectively) (33), immunoblotting (34), and fluorography (35) were carried out by standard procedures. Hsc73 was purified from bovine brain cytosol by ATP-agarose affinity chromatography (36). Densitometric analysis of the immunoblots was performed with an 2202 LKB Ultroscan laser densitometer (LKB-Pharmacia, Uppsala, Sweden) with a Hewlett-Packard (Palo Alto, CA) 3396 Series II integrator. The linearity of the method was established using different amounts of hsc73, GAPDH, or RNase A. Protein concentrations were measured by a modification of the Lowry et al. (37) method using bovine serum albumin as the standard. Enzymatic activities were measured by the standard procedures reported by Terlecky and Dice (9), Aniento et al. (10), Barrett and Kirschke (38), and Smith and Turk (39). The energy-regenerating system used in some experiments consisted of 10 mM MgCl2, 10 mM ATP, 2 mM phosphocreatine, and 50 µg/ml creatine phosphokinase. Statistical analyses were performed by the Student's t test.
In previous experiments we found that uptake of RNase A by rat liver lysosomes was heterogeneous (7). In addition, we noticed that the uptake efficiency of GAPDH by lysosomes decreased when these organelles were collected by centrifugation at 10,000 × g for 5 min instead of the usual 37,000 × g for 10 min (10, 11). These observations suggested that different populations of lysosomes with distinct activities in the selective uptake of cytosolic proteins might be separable based on centrifugation. In most of our previous experiments we used a pool of two lysosomal fractions from a discontinuous metrizamide gradient: the top layer (fraction 1) and the 26.3/19.8% metrizamide interface (fraction 2) (10, 11). Therefore, in a first approximation to identify a lysosomal population active in selective protein uptake, the top layer and the 26.3/19.8% metrizamide interface were centrifuged separately and in succession at 10,000 × g for 5 min and at 37,000 × g for 10 min, thus giving a total of four different fractions (two pellets, P1 and P2, and their supernatants, S1 and S2) to analyze. The protein content of these four fractions were as follows per rat liver: P1 = 1.5 ± 0.1 mg, P2 = 1.8 ± 0.2 mg, S1 = 0.14 ± 0.01 mg, and S2 = 0.44 ± 0.05 mg (38.7, 46.3, 3.6, and 11.4% of total lysosomal protein, respectively).
Immunoblot analysis of the levels of hsc73 reveals that one of these
fractions, P2, was practically devoid of hsc73, whereas the remaining
fractions had quite similar amounts of hsc73 when corrected for the
amount of protein analyzed (Fig. 1A). The
lysosome fractions referred to as P1 and P2 had similar low levels of
broken lysosomes (<3% as determined by the latency of lysosomal
enzymes (11)), but S1 and S2 contained higher levels of broken
lysosomes (10%). S1 and S2 also contained more unidentified membrane
fragments, as judged by electron microscopy, so the following
experiments were carried out only with the P1 and P2 fractions, which
represent 85% of the total lysosomal protein and which will be
referred to hereafter as HSC+ and HSC lysosomes, respectively.
Fig. 1B shows that hsc73 was present both in the matrix
(about 65% of the total by densitometric analyses of similar
immunoblots, when corrected for total protein) and in the membranes
from HSC+ lysosomes. The small amount of hsc73 (20% or less of the
hsc73 found in HSC+ lysosomes) occasionally observed in HSC lysosomes (lane 3) was exclusively associated with the lysosomal
membrane (lane 7). Proteinase K treatment of both lysosomal
fractions confirmed that the major part of the hsc73 that is found
associated with HSC+ lysosomes is in the lysosomal matrix, whereas all
hsc73 associated with HSC
lysosomes is in the membrane (data not
shown).
Other comparisons between the HSC+ and HSC lysosomal populations
revealed many similarities but also some differences. Thus, the study
of the specific activities of different lysosomal markers (Table
I) showed comparable activities of cathepsin B,
-N-acetyl-glucosaminidase, and
-hexosaminidase in both
fractions. However, lysosomal enzymatic activities in HSC
lysosomes
were always slightly but consistently higher than in HSC+ lysosomes.
Recoveries of lysosomal enzymes (between 3-5% of total) were
consistent with our previous studies working with the complete pool of
lysosomes (5%) (10, 11). Also, contamination of any of the fractions
with mitochondria (based on the activity of ornithine transcarbamoylase
and succinate dehydrogenase) or cytosol (based on the activity of
lactate dehydrogenase and GAPDH) was negligible. A typical late
endosome marker, the cation-independent mannose 6-phosphate receptor,
was not detected in either of the two lysosomal populations (data not
shown), suggesting that both populations are mainly mature lysosomes.
This conclusion is further supported by the high proteolytic activities
(see below) and by the high activities of lysosomal enzymes (Table I)
in both fractions. The SDS-PAGE pattern of bands was similar for total
lysosomes and for lysosomal membrane and matrix fractions (Fig.
2A). However, some qualitative or
quantitative increases in specific protein bands were evident in the
membranes and matrix of HSC+ lysosomes (i.e.: at about 182, 87, 76, and 45 kDa for membranes and 70 and 47 kDa for matrix; marked
by arrowheads in Fig. 2A). These differences were
evident in each of 10 separate analyses, but the degree of difference
varied from experiment to experiment, especially for the matrix
proteins. The levels of lysosomal membrane (lgp120, Fig. 2B;
lgp96, data not shown) and matrix (cathepsin L (CATH L),
Fig. 2C) proteins were quite similar in HSC+ and HSC
lysosomes. Total proteolytic activities of broken HSC+ and HSC
lysosomes at different pHs against a pool of labeled cytosolic proteins
(10) or GAPDH were also indistinguishable (data not shown).
|
The amounts of several cytosolic proteins in HSC+ and HSC lysosomes
were quantitated using specific antibodies. Typical results for
hexokinase and aldolase are shown in Fig. 2D. Hexokinase
(and a presumed immunoreactive breakdown fragment) is preferentially localized in HSC
lysosomes, whereas aldolase is largely confined to
HSC+ lysosomes. Quantitation of this and similar immunoblots indicate
that HSC+ lysosomes are enriched for GAPDH, aldolase, and
phosphoglycerate mutase. However, HSC
lysosomes were enriched for
hexokinase, and both lysosomal populations contained equivalent amounts
of phosphoglycerate kinase (Table II). Enrichment of
HSC+ lysosomes in GAPDH and aldolase does not seem to be related to a
lower proteolytical susceptibility of these enzymes once inside the
lysosomal matrix, since equivalent rates of degradation were obtained
when incubated with broken lysosomes from both populations (data not
shown).
|
The ultrastructural appearance of the HSC+ and HSC lysosomes is shown
in Fig. 3 (A and B). Although
there are not large differences, HSC+ lysosomes are in general smaller
and more elongated than HSC
lysosomes. Morphometric analysis of 40 randomly selected lysosomal profiles from 10 different electron
micrographs per fraction indicates an average area of 0.075 ± 0.017 µm2 for HSC+ lysosomes and 0.102 ± 0.021 µm2 for HSC
lysosomes. This difference is statistically
significant (p < 0.02). Also, the form factor was
0.698 for HSC+ lysosomes and 0.907 for HSC
lysosomes (1.000 is a
perfect circle).
We next investigated the uptake of RNase A and GAPDH by the two
lysosomal populations. These proteins are two well established substrates of the selective lysosomal pathway of intracellular protein
degradation (10, 11). As shown in Fig. 4, HSC+ lysosomes were much more efficient than the HSC lysosomes in taking up both
substrates. We also tested the effect of exogenously added hsc73 plus
ATP/MgCl2 and an energy regenerating system on the proteolysis of GAPDH and RNase S-peptide by the two lysosomal populations (Fig. 5). We found that these compounds were
stimulatory with both lysosomal populations as expected (10, 11) but
that HSC+ lysosomes were more active under all conditions.
Then we studied whether HSC+ and HSC lysosomes exhibit differences in
their abilities to take up hsc73. Fig. 6A
shows that when intralysosomal proteolysis was inhibited and levels of
hsc73 in matrix (after proteinase K treatment) were measured, HSC+
lysosomes were more effective in taking up exogenously added hsc73
(compare lanes 8 and 9), but some hsc73 was also
incorporated into HSC
lysosomes (Fig. 6A, lane
9), as was also the case with GAPDH and RNase A (Fig. 4). Although
the amount of hsc73 associated to lysosomes after the proteinase K
incubation is lower in Fig. 6 than in freshly isolated lysosomes (Fig.
1B), it should be noted that in these experiments lysosomes
received additional treatments that may result in some intralysosomal
hsc73 becoming accessible to the exogenously added protease. When RNase
A was incubated with HSC
lysosomes that had incorporated hsc73 in a
prior incubation (as in Fig. 6A), a portion of the RNase A
was found associated with the lysosomal pellets (Fig. 6B,
lane 5), and part of this RNase A was resistant to
proteinase K digestion (Fig. 6B, lane 9). The uptake efficiency of these lysosomes were now at least as good as the
original HSC+ lysosomes (compare lanes 8 and 9).
The presence of intralysosomal hsc73 was apparently sufficient to make
the HSC
lysosomes competent for the selective uptake of cytosolic proteins.
We also increased the content of hsc73 in HSC lysosomes by in
vivo manipulations. In a first approach, rats were treated with
leupeptin to inhibit lysosomal proteases prior to the isolation of the
two lysosomal fractions. Immunoblot analysis with anti-hsc73 (Fig.
7A, upper panel) reveals an
increase in hsc73 (lane 5) in the fraction corresponding to
HSC
lysosomes. Although after leupeptin treatment the quantity of
hsc73 increased in both lysosomal populations, this increase is
considerably higher for HSC
lysosomes (ten times) than for HSC+
lysosomes (two times). The uptake efficiency of proteins (RNase A and
GAPDH) (Fig. 7A, middle and lower
panels) by the two lysosomal populations isolated from rats
treated with leupeptin (lanes 4 and 5) was
similar to the original HSC+ lysosomes (lane 2) and much
higher than the HSC
lysosomes (lane 3).
Other in vivo evidence was provided by prolonged starvation
(Fig. 7B). As reported previously (7), during prolonged
starvation over the range 0-88 h, there is a progressive increase in
the activity of the hsc73-dependent selective lysosomal
proteolytic pathway coincident with an increase in lysosome-associated
hsc73. The two lysosomal populations isolated from rats after 88 h
of starvation were indistinguishable from those isolated after 20 h based on ultrastructural appearance and SDS-PAGE protein patterns (data not shown). However, after 88 h of starvation there was an
increase in hsc73 in both lysosomal populations (Fig. 7B,
upper panel), but the increase was most pronounced for the
HSC lysosomes. The uptake of two substrate proteins of this pathway,
RNase A (Fig. 7B, middle panel) and GAPDH (Fig.
7B, lower panel) by these lysosomal populations
showed a significant increase in the uptake efficiency of the original
HSC
lysosomes after 88 h starvation (compare lanes 3 and 5). From these observations it appears again that the
intralysosomal hsc73 is required for an efficient lysosomal uptake of
proteins.
Hsc73 was taken up most avidly by HSC+ lysosomes (Fig. 6A,
compare lanes 8 and 9), but this difference
cannot completely account for the absence of hsc73 in the HSC
lysosomes. Because of the dramatic effect of leupeptin on the hsc73
content of HSC
lysosomes (Fig. 7A, upper
panel), it seemed possible that hsc73 is also degraded more
efficiently within the HSC
lysosomes than in the HSC+ lysosomes. In
initial attempts to test this idea, we reductively methylated hsc73 but
found that these preparations contained mostly inactive hsc73 in that
the protein no longer could bind to ATP (8). Therefore, we purified a
metabolically labeled [35S]GST-hsc73 fusion protein and
followed its degradation during incubation with freshly isolated HSC+
and HSC
lysosomes. [35S]GST-hsc73 is almost two times
more effectively degraded by HSC
lysosomes than by HSC+ lysosomes
(Fig. 8A). Because lower rates of hsc73
uptake were found for HSC
lysosomes (Fig. 6A), differences in efficiency on hsc73 degradation between both populations may take
place in the lysosomal matrix. To verify this idea, after incubation of
intact lysosomes with a large amount (2 µM) of
[35S]GST-hsc73 so that a signal could be seen in the
HSC
lysosomes (Fig. 8B, inset, lane
5), we reisolated the lysosomes that had incorporated a portion of
the GST-hsc73 and subsequently measured the degradation of the fusion
protein. HSC
lysosomes were again more effective in degrading the
[35S]GST-hsc73 than were HSC+ lysosomes (Fig.
8B). Similar degradation rates and the same difference
between HSC+ and HSC
lysosomes were obtained with the active fraction
of hsc73 radiolabeled with 14C by reductive methylation
that retained its ability to bind to ATP (data not shown). This result
indicates that the [35S]GST-hsc73 fusion protein was
valid for monitoring intralysosomal degradation of hsc73.
The differences between HSC+ and HSC lysosomes in their degradation
efficiency of hsc73 cannot be explained by differences in the
proteolytic activity of broken lysosomes (see above). Therefore, we
decided to measure the intralysosomal pH of both lysosomal populations
using FITC-dextran. We found that the pH in HSC+ lysosomes was
approximately 0.5 pH units lower than that of HSC
lysosomes (Fig.
9A). Supplying the lysosomal proton pump with
ATP/MgCl2 slightly increased this difference. That the
lysosomal pH could be important in the degradation of intralysosomal
hsc73 was apparent when HSC+ lysosomes were incubated for 30 min with
or without ATP/MgCl2 (Fig. 9B). Without
ATP/MgCl2 most intralysosomal hsc73 was degraded after 30 min of incubation of the HSC+ lysosomes, whereas in the presence of
ATP/MgCl2 when the lysosomes were slightly more acidified
(Fig. 9A) the degradation of hsc73 was retarded. The effect
of ATP/MgCl2 was due to intralysosomal acidification and
not due to some protective effect of ATP on the hsc73 because when the
ATPase inhibitor bafilomycin A was added together with ATP/MgCl2, the ATP-stimulated acidification of the HSC+
lysosomes was blocked (data not shown), and the lysosomal degradation
of the endogenous hsc73 was increased (Fig. 9B,
compare lanes 3 and 4).
We also investigated the proteolysis of hsc73 by HSC+ lysosomes treated
with increasing amounts of NH4Cl to increase their pH (Fig.
9C). Lysosomal pH was modified from 5.4 to 6.4 by
NH4Cl, and the proteolysis of hsc73 was found to be most
effective in the range 5.75-6.20. Therefore, the difference in pH
could explain why HSC lysosomes are more effective than HSC+
lysosomes in degrading their endogenous hsc73.
We have identified two populations of rat liver lysosomes with very different abilities to selectively take up and degrade protein substrates such as GAPDH and RNase A (Figs. 4 and 5). These differences in uptake rates cannot be explained by differences in the amount of lysosomes in both fractions, because only small differences in the activities of lysosomal enzymatic markers were found between both populations (Table I). In addition, analysis of RNase A uptake into individual lysosomes by immunogold and electron microscopy (7 and data not shown) confirmed that lysosomes with higher content of hsc73 incorporate a significantly larger amount of RNase A.
The two populations of lysosomes are similar in many respects, but they
differ markedly in their content of hsc73 (Fig. 1). That the difference
in lysosomal hsc73 in the lumen accounts for the different activities
of HSC+ and HSC lysosomes in their ability to selectively take up and
degrade proteins could be shown experimentally by "loading" HSC
lysosomes with hsc73 in vitro (Fig. 6) and by two different
in vivo treatments, leupeptin injection (Fig. 7A) and long term starvation (Fig. 7B). Importantly, these HSC
lysosomes loaded with hsc73 retained all other characteristics of HSC
lysosomes such as their more alkaline pH and their more rounded shapes
and larger size (data not shown). In addition, membrane stability and
proteolytic activity of HSC
lysosomes were not modified after long
term starvation. These results suggest that the presence of lumenal
hsc73 is the direct cause of the activation of the selective
degradation pathway.
This interpretation is also consistent with results from cultured human fibroblasts in which intralysosomal hsc73 was neutralized in living cells by the endocytosis of an immunoprecipitating anti-hsc73 antibody (19). This treatment completely blocked the selective lysosomal degradation pathway without affecting other proteolytic pathways. These results together with the results presented here indicate that the intralysosomal hsc73 is required for the selective uptake of protein substrates into lysosomes. Similar roles for other hsp70 familiy members have been documented for the uptake of mitochondrial precursor proteins into mitochondria (15, 16) and for the uptake of endoplasmic reticulum or secreted proteins into the endoplasmic reticulum lumen (17, 18). Two main hypotheses have been presented about the mechanism of action of those lumenal chaperones (see Ref. 40 for review). In both of these models, a chaperone attached to the trans-side of the membrane interacts with the translocating polypeptide chain and prevents back movement of the protein (molecular ratchet model) or actively, by hydrolyzing ATP, pulls the protein across the membrane (translocation motor model). By analogy with these studies intralyosomal hsc73 could interact with the protein emerging into the lysosomal matrix, providing the driving force to pull the import intermediate into the lysosome and preventing also the back movement of the protein to the cytosol. In this regard, a kinetic intermediate in the transport of RNase A through the lysosomal membrane has been identified (11).
Intralysosomal hsp70 appears to be hsc73 itself because the lysosomal hsp70 is recognized by two antibodies specific for hsc73 among all hsp70s tested, and the intralysosomal hsp70 co-migrates with one of the hsc73 isoforms in high resolution two-dimensional gels (19).2 We now provide additional support for this conclusion because cytosolic hsc73 can enter lysosomes in vitro, and this hsc73 functions as well as the lysosomal hsp70 in the selective uptake of proteins.
The preferential uptake of hsc73 by HSC+ lysosomes, evident when proteolysis is previously blocked (Fig. 6A, compare lanes 8 and 9), suggests that hsc73 can enter lysosomes, at least in part, through the selective pathway that it stimulates. Consistent with this finding is the presence of two KFERQ-like motifs in hsc73 and the ability of hsc73 to bind to other hsc73 molecules (13). Also, we repeatedly find a stimulation of the selective lysosomal uptake of protein substrates by low levels of hsc73 (Fig. 5) but competition by higher levels (data not shown) consistent with hsc73 entering lysosomes by the same pathway.
Combined with the reduced ability of HSC lysosomes to take up hsc73,
they also degrade intralysosomal hsc73 more rapidly than do HSC+
lysosomes (Fig. 8, A and B). This enhanced
degradation in HSC
lysosomes appeared to be caused by the more
alkaline pH in this lysosome population (Fig. 9A).
Acidification of HSC+ lysosomes further reduced the degradation of
intralysosomal hsc73 (Fig. 9B), and mild alkalinization
using NH4Cl increased degradation of intralysosomal
[35S]GST-hsc73 (Fig. 9C). In fact, HSC+
lysosomes degraded [35S]GST-hsc73 twice as rapidly at pH
5.8 as at pH 5.4, which accounts well for the twice as rapid
degradation in HSC
than in HSC+ lysosomes.
The significance of other differences between HSC+ and HSC lysosomes
are less clear. The presence of increased levels of certain cytosolic
proteins in HSC+ lysosomes may indicate that they are selective
substrates for this proteolytic pathway. This has been shown to be true
for GAPDH (10, 11) and hsc73 (Fig. 6). Whether aldolase and
phosphoglucomutase are also substrates remains to be tested. The
relative enrichment of other cytosolic proteins in HSC
lysosomes may
indicate that they are not good substrates for the selective import
pathway but that they can enter lysosomes by alternate means such as
microautophagy or macroautophagy and then are relatively resistant to
lysosomal proteolysis.
The physiological significance of the different sizes and shapes of
HSC+ and HSC lysosomes is not known. We also do not know the
significance of different protein bands in the membranes of HSC+ and
HSC
lysosomes. One possibility is that some of the lysosomal membrane
proteins that are preferentially found in the HSC+ lysosomes are
components of the selective protein import pathway.
The low pH, the high hydrolytic activities and the absence of typical
endosomal markers (41) in HSC+ and HSC lysosomes suggest that most
organelles in these populations are mature lysosomes. It appears also
that HSC
lysosomes have all the other components needed for the
selective transport of cytosolic proteins because this population can
be made competent for specific protein uptake by simply preloading it
with hsc73. Accordingly, HSC
lysosomes, which would be inactive under
basal and short starvation times, could be activated and recruited to
participate in the selective pathway under certain conditions
(e.g. prolonged starvation) by increasing hsc73 in their
lumen.
We thank Dr. Sandra Hayes for critical reading of the manuscript. We are grateful to A. Montaner for technical assistance.