Originally published In Press as doi:10.1074/jbc.M111497200 on January 25, 2002
J. Biol. Chem., Vol. 277, Issue 17, 14821-14828, April 26, 2002
Abnormal Acidification of Melanoma Cells Induces Tyrosinase
Retention in the Early Secretory Pathway*
Ruth
Halaban
§,
Robin S.
Patton¶,
Elaine
Cheng,
Sherri
Svedine¶,
E. Sergio
Trombetta
,
Miriam L.
Wahl**,
Stephen
Ariyan, and
Daniel N.
Hebert¶§§
From the Departments of Dermatology, Cell
Biology, and Plastic Surgery, Yale
University School of Medicine, New Haven, Connecticut 06520, the
¶ Department of Biochemistry and Molecular Biology, Program in
Molecular and Cellular Biology, University of Massachusetts,
Amherst, Massachusetts 01003, and the ** Department of
Biochemistry and Molecular Pharmacology, Thomas Jefferson University,
Philadelphia, Pennsylvania 19107
Received for publication, December 3, 2001, and in revised form, January 10, 2002
 |
ABSTRACT |
In tyrosinase-positive amelanotic melanoma cells,
inactive tyrosinase accumulates in the endoplasmic reticulum. Based on
studies described here, we propose that aberrant vacuolar proton ATPase (V-ATPase)-mediated proton transport in melanoma cells disrupts tyrosinase trafficking through the secretory pathway. Amelanotic but
not melanotic melanoma cells or normal melanocytes display elevated
proton export as observed by the acidification of the extracellular
medium and their ability to maintain neutral intracellular pH.
Tyrosinase activity and transit through the Golgi were restored by
either maintaining the melanoma cells in alkaline medium (pH 7.4-7.7)
or by restricting glucose uptake. The translocation of tyrosinase out
of the endoplasmic reticulum and the induction of cell pigmentation in
the presence of the ionophore monensin or the specific V-ATPase
inhibitors concanamycin A and bafilomycin A1 supported a role for
V-ATPases in this process. Because it was previously shown that
V-ATPase activity is increased in solid tumors in response to an
acidified environment, the appearance of hypopigmented cells in
tyrosinase-positive melanoma tumors may indicate the onset of enhanced
glycolysis and extracellular acidification, conditions known to favor
metastatic spread and resistance to weak base chemotherapeutic drugs.
| |
INTRODUCTION |
Tyrosinase (monophenol monooxygenase, EC 1.14.18.1) is a
copper-binding enzyme that catalyzes the oxidation of monohydric and
dihydric phenols (catechols) to their corresponding quinones, the
rate-limiting reaction in melanin synthesis (1, 2). Peptides derived
from tyrosinase are frequently presented on melanoma cells by major
histocompatibility molecules (3, 4). The development of immunotherapies
for patients with melanoma is based in part on employing cytotoxic
T-cell recognizing tyrosinase peptides as the immunogen (5). The
production of these peptides is contingent on the presence of
tyrosinase and its proteolytic degradation products. However,
tyrosinase peptide presentation is an aberrant phenotype of melanoma
cells, because tyrosinase in normal melanocytes is a stable enzyme that
is localized to the melanosomes, the site of melanin synthesis.
The production of antigenic peptides involves an accumulation of
tyrosinase in the endoplasmic reticulum
(ER)1 as a 70-kDa high
mannose glycoform and its subsequent routing to the cytoplasm for
degradation by the proteasome (6, 7). Failure of tyrosinase in these
melanoma cells to be processed in the medial Golgi as indicated by
endoglycosidase H (Endo H) digestion and confocal microscopy (6) is
reminiscent of albino mutant forms of tyrosinase that contain
loss-of-function mutations and are retained in the ER (8-10). The
observations that incubating melanoma cells with the cofactor DOPA or
high concentrations of the substrate tyrosine enhanced the exit of
tyrosinase from the ER, its carbohydrate modification in the Golgi, and
transport to the melanosomes and melanin production suggested that
tyrosinase inactivation is associated with aberrant misfolding and ER
retention (11). However, the cause of inactivation of non-mutated
tyrosinase in melanoma cells has not yet been elucidated.
We reasoned that inactivation of tyrosinase is probably linked to
tumor-induced metabolic changes. A common phenotype shared by melanoma
cells is acidification of the extracellular milieu and poor response to
chemotherapy (12-15). Melanoma cells adapted to grow under hypoxic
conditions acidify their immediate extracellular environment because of
high rates of glucose uptake, increased glycolysis, and the
accumulation of lactic acid (12, 16-18), a process known as the
Warburg effect (19, 20). In fact, increased glucose uptake is currently
the basis for melanoma tumor staging by PET
(18F-fluorodeoxyglucose positron emission tomography) (21).
These metabolic changes are likely to contribute to the drug-resistance phenotype, because the extent of multidrug resistance in
advanced melanoma lesions does not correlate with the expression of
P-glycoprotein, multidrug resistance-1, even after chemotherapeutic
treatment (13-15).
An alternative mechanism shared by drug-resistant cells is
sequestration of weak base chemotherapeutics in acidic organelles away
from their sites of action in the cytosol and nucleus (22-24). Increased V-ATPase activity has been implicated in the acidification of
endosomes, trans-Golgi network, and lysosomes in solid
tumors to accommodate the acidic environment (25-27). Substances that cause alkalinization of vesicular compartments such as the
Na+/K+ and proton ionophore monensin or the
V-ATPase-specific inhibitors concanamycin A or bafilomycin A1 also
induce the release of chemotherapeutic drugs and enhance their
accumulation in the nucleus (28). Because tyrosinase activity can be
suppressed by acidified conditions (2, 29), we explored the possibility
that increased proton pump activity also affects tyrosinase activity
and processing in melanoma cells. We show here that tyrosinase
trafficking and activity in amelanotic melanoma cells were restored
after alkaline treatment or inhibition of V-ATPase activity. The data
support the hypothesis that protonation, possibly in the ER-Golgi
interface, disrupts tyrosinase maturation in melanoma cells resulting
in the amelanotic phenotype, tyrosinase degradation, and antigen production.
| |
MATERIALS AND METHODS |
Cell Culture--
Normal human melanocytes were cultured from
newborn foreskins in Ham's F-10 medium supplemented with glutamine (2 mM), penicillin-streptomycin (100 units/ml), and 7% fetal
bovine serum (all from Invitrogen) termed basal medium, which was
further enriched with several ingredients required for normal
melanocyte proliferation. These ingredients included 85 nM
12-O-tetradecanoylphorbol-13-acetate, 0.1 mM
isobutylmethylxanthine, 2.5 nM cholera toxin, 1 µM Na3VO4, and 0.1 mM
N6,2'-O-dibutyryladenosine-3-AMP
(
2AMP) (TICVA, Sigma) (30).
Human metastatic amelanotic melanoma cells (YUGEN8, 501 mel, YUSIT1,
and YUSAC2) (30), were maintained in the Ham's F-10 basal medium. The
melanotic Heik178 cells were grown in the Ham's F-10 basal medium
supplemented with growth factors (2 ng/ml fibroblast growth factor 2, 10 nM endothelin 1, 10 nM hepatocyte growth
factor plus 0.2 ng/ml heparin) and used during the second
passage in culture. The melanotic MNT1 melanoma cells (31) (obtained
from Dr. M. S. Marks, Department of Pathology and Laboratory
Medicine, University of Pennsylvania School of Medicine, Philadelphia,
PA) were grown in Dulbecco's modified Eagle's medium plus 20%
serum and 10% AIM-V medium (Invitrogen) as described previously (32). When needed, the extracellular pH (pHe) of the medium was
monitored daily and adjusted to pH 7.7 with 1 N NaOH. Cells
were incubated in the basal medium, unmodified OptiMEM (Invitrogen)
plus 2% fetal bovine serum, Dulbecco's modified Eagle's glucose-free
medium, or RPMI 1640 medium select®-amine (Invitrogen) reconstituted
with sodium pyruvate, tyrosine, and glucose or galactose as
indicated. In some experiments, the medium was supplemented with
50 µM freshly prepared DOPA (1 mM stock
solution in PBS, Sigma), monensin (10 mM stock solution in
Me2SO, Sigma), concanamycin A or bafilomycin A1 (20 µM stock solutions dissolved in Me2SO, both
from Calbiochem), pepstatin (10 mg/ml stock solution), or leupeptin (20 mg/ml stock solution, Sigma) using Me2SO as a control when needed.
Western blot Analysis, Precipitation, and Antibodies--
CHAPS
lysis buffer (2% CHAPS in 50 mM HEPES and 200 mM NaCl, pH 7.5) containing protease inhibitors
(CompleteTM protease inhibitor mixture, Roche Molecular
Biochemicals) was used to lyse cells and wash bead-bound precipitated
material as described previously (6). Western blot analyses were
performed on whole cell lysates (40 µg of protein/lane as measured by
the Bio-Rad protein assay reagent, Bio-Rad), anti-tyrosinase
immunoprecipitated proteins (C-19 goat, Santa Cruz Biotechnology, Santa
Cruz, CA), or affinity-purified glycoproteins using wheat germ
agglutinin (WGA) bound to beads (lectin from Triticum
vulgaris) following standard procedures or the manufacturer's
instructions (Sigma). Endo H (Roche Molecular Biochemicals)
digestion of precipitated proteins was performed as described
previously (6, 11). Tyrosinase was detected with mouse mAb T311 (33),
and protein loading in each lane was assessed by staining the gels with
Coomassie Brilliant Blue after transfer of the proteins to membranes
and by immunoblotting with anti-actin rabbit polyclonal antibodies (Sigma).
Tyrosinase Activity--
Tyrosinase assays were performed with
L-[3,5-3H]tyrosine (PerkinElmer Life
Sciences) as a substrate (34-36). Reaction mixtures (200 µl of final
volume) containing 150 µg of cell extract protein prepared in 2%
CHAPS buffer, 50 µM L-tyrosine, 1 µCi/assay
L-[3,5-3H]tyrosine, and 50 µM
L-DOPA were incubated for 60 min at 37 °C. Reactions
were stopped with 200-µl solution of 10% activated charcoal in 0.1 M citric acid (w/v), the charcoal slurries passed through Dowex columns (350 µl), and radioactivity of the eluate in
scintillation fluid was measured with a scintillation counter. One unit
of tyrosinase was defined as the amount of enzyme that catalyzed the
oxidation of 1 mmol tyrosine in 1 min. All reactions were performed in
triplicates or duplicates, and the standard errors were in the range of
15% total counts.
Intracellular pH (pHi) Measurements--
Normal and malignant
melanocytes were grown on 18-mm glass coverslips precoated with a 1:1
mixture of collagen I and fibronectin-like RGD fragments at a
final concentration of 50 µg/ml for 48-72 h. Cells were then
incubated with the pH-sensitive dye BCECF AM at a final
concentration of 5 µM for 4 min at pH 7.3 at room
temperature and 5% CO2 as described previously (37, 38).
Following a medium change to pH 7.3 or 7.0, the cells were maintained
for an additional 20 min at 37 °C, 5% CO2 to allow
complete hydrolysis of the dye ester. The plates were then mounted on
the microscope stage, and pH was monitored at 37 °C under humidified
air containing 5% CO2. Cellular pHi values were calculated
based on data from whole excitation spectra (37, 38). All measurements
were done in triplicates.
Metabolic Labeling--
Pulse-chase experiments were performed
as described previously (8). Cells were pulse-labeled for 15 min with
[35S]Met/Cys (0.7 mCi/ml, EasyTag, PerkinElmer Life
Sciences) in methionine/cysteine-free RPMI 1640 medium (Invitrogen) and
either collected immediately or after chase incubation with
non-radioactive medium (Ham's F-10 medium) for the indicated period of
time. Experiments were performed in medium supplemented with tyrosine
as indicated and then subjected to immunoprecipitation with rabbit
anti-tyrosinase antibodies. Following extensive washing with
radioimmune precipitation buffer, half of the precipitated products
were digested with Endo H overnight. Eluted proteins were fractionated
in SDS-PAGE, and dried gels were analyzed by autoradiography. Densities
of radioactive tyrosinase bands on the x-ray films were determined
using a Molecular Dynamics PhosphorImager.
Immunofluorescence Microscopy--
Melanoma cells were grown on
chamber slides in unmodified Ham's F-10 medium at pH 7.4. Treated and
untreated cells were washed with PBS, fixed in 4% formaldehyde/PBS,
and permeabilized with 0.1% Triton X-100/PBS. The permeabilized and
fixed cells were then incubated with antibodies against tyrosinase
(C-19 goat), ERGIC-53 (mAb, a gift from Dr. H.-P. Hauri, Geneva,
Switzerland; a marker of ER-ER Golgi intermediate compartment), COPI
(rabbit polyclonal anti--COPI antibodies, a gift from Dr. G. Warren, Department of Cell Biology, Yale University, New Haven, CT; a marker
for ER-ERGIC-Golgi compartments), or calnexin (mAb, StressGen Biotechnologies Corporation, Victoria, British Columbia, Canada; an ER
marker). The primary antibodies were detected with fluorescein anti-goat conjugates (Santa Cruz Biotechnology) or rhodamine anti-mouse or anti-rabbit conjugates (Molecular Probes, Eugene, OR). All dilutions
were in 0.1% bovine serum albumin/PBS. Indirect immunofluorescence was
visualized with an inverted Bio-Rad MRC-600 laser confocal microscope
system. Images were processed with Bio-Rad confocal assistant software.
| |
RESULTS |
Stabilization of Tyrosinase by Raising Extracellular pH--
Under
normal conditions, the medium from amelanotic melanoma cells
becomes rapidly acidified within a day of medium change (pH 7.0-7.2),
whereas that of normal melanocytes or the pigmented metastatic melanoma
Heik178 remain basic (pH 7.4-7.5). Therefore, we evaluated
pigmentation and tyrosinase processing in YUGEN8 melanoma cells
subcultured in Ham's F-10 medium, adjusted daily to pH 7.7, and
compared it to cells that were continuously grown in unmodified Ham's
F-10 medium. Alkalinization of the pHe had a marked effect as the cells
became pigmented during 2 weeks of culture (Fig.
1A). An analysis of
steady-state tyrosinase levels demonstrated an increase in the
abundance of tyrosinase protein (Fig. 1B, lanes 1 and 2, normalized to actin and total protein concentration).
Most striking was the increase in the level of the higher molecular
weight mature tyrosinase (Fig. 1B, compare lane 1 with 2, arrow) (6).
View larger version (45K):
[in this window]
[in a new window]
|
Fig. 1.
Extracellular pH-dependent
pigmentation, stabilization, and Golgi processing of tyrosinase.
YUGEN8 melanoma cells were grown in Ham's F-10 medium (pHe ~7.2) or
in medium adjusted to pH 7.7 for 2 weeks. A, pellets of
amelanotic and melanotic cells grown at the indicated pHe.
B, lanes 1 and 2 represent
anti-tyrosinase Western blot analysis of whole cell lysates prepared
from the cell pellets presented in A. Solid and
empty arrows and spearhead mark mature and
immature tyrosinase and proteolytic degradation products, respectively.
Protein loading in each well was normalized by subsequent
immunoblotting the same membrane with anti-actin antibodies
(actin). Lanes 3-6 represent anti-tyrosinase
Western blot of proteins bound to WGA beads undigested ( ) or digested
(+) with Endo H. Arrow indicates mature partially Endo
H-resistant tyrosinase and the deglycosylated (DG) form of
the immature glycoform (empty arrow). C, low
pHe-suppressed DOPA-induced Golgi maturation. Western blot analysis of
cell extracts derived from YUGEN8 melanoma cells incubated in OptiMEM
medium containing 200 µM tyrosine with 50 µM DOPA at pHe 7.2 (lanes 1-3) or pHe 7.5 (lanes 4-7). Solid and empty arrows
indicate the mature and immature tyrosinase forms as noted above.
Numbers on the left-hand side of Western blot
images here and in all other figures indicate molecular mass markers in
kDa.
|
|
The identification of the higher molecular weight tyrosinase glycoform
as a protein that had been modified by Golgi enzymes was verified by
Endo H digestion. Endo H cleaves N-linked oligosaccharides between the two N-acetylglucosamine residues in the core
region of the oligosaccharide chain of high mannose but not complex
carbohydrates. Because the addition of complex sugars occurs in the
medial Golgi, the limited substrate specificity of this enzyme provides
a useful tool for monitoring the subcellular location of glycoproteins. Endo H treatment had only a slight effect on the electrophoretic mobility of mature tyrosinase (Fig. 1B, lanes 4 and 6, solid arrow) indicating that the majority
of the seven tyrosinase N-linked glycans had been modified
with complex sugars in the Golgi (39). In contrast, the faster
migrating immature glycoform (Fig. 1B, bands
marked with empty arrow) was digested to its 58-kDa
polypeptide indicative of complete sensitivity of all of seven glycans
in tyrosinase, a characteristic of ER or cis-Golgi residency
(Fig. 1B, lanes 4 and 6,
band marked DG). Species of low molecular
mass of ~58 kDa (Fig. 1B, lane 2 marked
with spearhead) also accumulated after incubation in
alkaline pHe. This protein band represents the non-glycosylated
tyrosinase as shown by its inability to bind WGA (Fig. 1B,
lanes 5) as reported previously (6, 11).
Further evidence that alkaline pHe promoted tyrosinase maturation and
activation was obtained by analyzing the effect of DOPA on this
process. We have previously shown that the addition of the cofactor
DOPA to the growth medium in the presence of catalytic amounts of the
substrate tyrosine promoted tyrosinase activation and maturation in
melanoma cells within hours (11). Because DOPA activation of tyrosinase
is dependent on pH (2, 29), we tested whether low pHe could suppress
the DOPA effect. Indeed maintaining the cells at low pHe hampered the
DOPA/tyrosine-induced maturation (Fig. 1C, compare
lanes 1-3 with 4-7), suggesting that long term
growth in acidified pH suppresses DOPA activation, tyrosinase maturation, and pigmentation.
Tyrosinase Processing Is Induced by Glucose Restriction in Melanoma
Cells--
Because increased glucose consumption can increase acidity
as a result of the accumulation of lactic acid in the cell environment (17), we tested whether eliminating glucose in the medium could affect
pigmentation, tyrosinase activity, and maturation. Toward this end, melanoma cells (YUGEN8 and YUSIT1) were grown for 3 days in
glucose-free medium with 1 mM pyruvate supplemented with 25 mM glucose (+) or 2 mM galactose () (Fig.
2). The source of energy affected the pH
of the external medium because at the end of 3 days of incubation, the
pHe was 7.1 and 7.5-7.7, in the glucose-containing and glucose-free
(galactose-supplemented) medium, respectively. The levels of
pigmentation were also dramatically increased in YUGEN8 and YUSIT1
melanoma cells grown in the glucose-free medium compared with
glucose-supplemented medium (Fig. 2A, compare + to ). Time-course analysis revealed the accumulation of
the 80-kDa tyrosinase glycoform in melanoma cells after 28 h in
glucose-free medium (Fig. 2B, TYR) accompanied by
a large increase in tyrosinase activity (Fig. 2C). These
results demonstrated that glucose metabolism has an impact on
tyrosinase activity and processing, probably because of acidification
of the extracellular milieu and endomembraneous compartments.
View larger version (46K):
[in this window]
[in a new window]
|
Fig. 2.
Restoration of pigmentation, increased
tyrosinase activity, and Golgi maturation by glucose restriction.
Melanoma cells were incubated in glucose-free Dulbecco's modified
Eagle's medium with 7% fetal bovine serum plus 1 mM
pyruvate supplemented with 25 mM glucose (+) or with 2 mM galactose (). A, melanoma cell pellets
(YUGEN8 and YUSIT1) after 3 days of incubation in
the experimental medium. B, time course analysis of
tyrosinase in response to glucose deprivation. YUGEN8 melanoma cells
were grown in galactose-supplemented Dulbecco's modified Eagle's
glucose-free medium for increasing periods of time. Cell extracts were
subjected to Western blot analysis first with anti-tyrosinase T311 mAb
(TYR) and then with anti-actin antibodies
(actin). C, DOPA-stimulated tyrosinase activity
in cell extracts of YUGEN8 melanoma cells grown in the presence or
absence of glucose as shown in A. D, maturation of
tyrosinase in glucose-free medium supplemented with different
concentrations of tyrosine. Western blots with T311 anti-tyrosinase mAb
of whole cell lysates derived from YUGEN8, YUSIT1, and 501 mel melanoma
cells grown for 3 days in glucose-free or glucose-supplemented medium
with 10 or 100 µM tyrosine.
|
|
Because tyrosinase maturation has been shown previously to be induced
by its activation (11), we further investigated whether the restoration
of tyrosinase processing obtained with direct alkalinization of the pHe
(Fig. 1) or by restricting glucose consumption (Fig. 2) could be
modulated by the concentrations of tyrosine in the medium. As the
glucose-free medium used above contained a high tyrosine concentration
(400 µM), we incubated three melanoma cell lines, YUGEN8,
501 mel, and YUSIT1, in RPMI 1640 select®-amine medium
supplemented with glucose or galactose in the presence of low (10 µM) or high (100 µM) tyrosine for 3 days.
Tyrosinase was processed to the 80-kDa form in cells grown in
glucose-free medium at both low and high tyrosine concentrations in
melanoma cells exhibiting relatively modest levels of tyrosinase (Fig. 2D, YUGEN8, compare lane 1 with 2 and
lane 3 with 4, solid and empty arrows). Melanoma cells with lower levels of
tyrosinase displayed different thresholds of activation. The 501 mel
cells required at least 100 µM tyrosine for stabilization
(Fig. 2D, compare lane 6 with 8),
whereas the enzyme remained as the ER 70-kDa glycoform in YUSIT1
melanoma cells even at 100 µM tyrosine (Fig.
2D, lanes 9-12, empty arrow).
Therefore, in agreement with previous observations (11), the
effectiveness of glucose restriction and alkaline extracellular pH was
dependent on the concentration of tyrosine in the medium and the levels
of endogenous tyrosinase, suggesting that the maturation process was
dependent on tyrosinase activity.
Amelanotic Melanoma Cells Maintain Higher Intracellular pH
Values--
The enhanced extracellular acidification observed for
amelanotic melanoma cells indicated an increased proton pump activity at their plasma membrane. In addition, the surface proton pumps, Na+/H+ antiporters and
Cl
/HCO3 exchangers are known to be activated
in tumor cells to maintain pHi and protect the cells from the acidic
extracellular environment (reviewed in Ref. 24). Therefore, we assessed
the pHi in response to external acidification in normal melanocytes and
compared it with melanotic and amelanotic melanoma cells.
A shift to extracellular pH 7.0 induced a dramatic drop in
intracellular pH in normal melanocytes and pigmented melanoma cells (Heik178 and MNT1). In contrast, the pHi of the amelanotic melanoma cells (YUGEN8 and 501 mel) remained relatively alkaline and was persistently 0.4-0.5 pH units above that of cells that retained their pigmented phenotype in culture (normal and malignant
melanocytes), indicating high compensating proton pump activity in
amelanotic melanoma cells (Fig. 3).
Changes in the activity of the proton pumps in melanoma cells in
response to growth in low extracellular pH for several days were
recently reported (16).
View larger version (17K):
[in this window]
[in a new window]
|
Fig. 3.
Amelanotic melanoma cells maintain high pHi
values after acidification. The pHi of normal human melanocytes
( ), amelanotic YUGEN8 ( ) and 501 mel ( ) melanoma cells,
and melanotic Heik178 ( ) and MNT1 ( ) melanoma cells was measured
after exposure to pH 7.0. Measurements were done in growth medium at pH
7.3, 10 min before pH changes (10 data point) and up to 60 min after
a shift to pHe 7.0 (acidification). Reduction in pH during initial
recording before time 0 is sometimes seen when the lost CO2
during transfer to the microscope was not completely reequilibrated. A
shift to pH 7.3 did not cause a change in intracellular pH in any of
the cell lines. At least five consecutive measurements were taken on
each of three fields. Data are means of triplicate measurements in a
representative experiment of three experiments, and error
bars indicate the means ± S.D. Dashed and
solid lines indicate amelanotic and melanotic cells,
respectively.
|
|
Inhibition of Proton Pump Activity Promotes Tyrosinase
Maturation--
Activation of proton pumps in cultured amelanotic
melanoma cells can be inferred from the highly acidified conditioned
medium and their ability to compensate their pHi when exposed to pH
7.0. V-ATPases have been implicated in neutralizing cytosolic pH by pumping protons away from the cytoplasm to the outside milieu as well
as into acidic organelles such as the Golgi, endosomes, and lysosomes
(25, 40, 41). Therefore, we tested the effect of the
Na+/K+ and proton ionophore monensin known to
reversibly raise the pH of endocytic vesicles (22, 42) and the high
affinity V-ATPase inhibitors concanamycin A and bafilomycin A1 (43) on
tyrosinase maturation and activity. Four different strains of
amelanotic melanoma cells became highly pigmented within 2 h of
incubation with each of these compounds in the presence of 100 µM tyrosine without any manipulation of the extracellular
pH (data not shown). In agreement with published observations (44, 45),
the three agents also increased the level of pigmentation of the
already highly melanized normal human melanocytes derived from
Caucasian donors. The increase in pigmentation in all cell types was
probably because of an increase in in situ tyrosinase
activity in response to alkalinization of vesicular compartments known
to be acidified under normal conditions (46, 47). In vitro
tyrosinase activity of cell extracts from normal melanocytes and
melanoma cells (YUGEN8 and 501 mel) increased 5- and 2-fold in a
pH-dependent manner between pH 6.6 and 8.0, respectively,2 suggesting
that mature and immature forms of tyrosinase are activated at basic pH.
Analyses of steady-state tyrosinase levels showed that in normal human
melanocytes, the mature 80-kDa enzyme, the predominant glycoform, was
not affected by monensin, concanamycin A, or bafilomycin A1 (Fig.
4A, compare lane 1 with 2-4). In contrast, the treatment of melanoma cells
with nanomolar concentrations of the two V-ATPase inhibitors induced
the conversion of the 70-kDa glycoform to the mature 80-kDa glycoform
(Fig. 4A, lanes 7, 8, 11,
12, 15, 16, 19, and
20). Although high concentrations of tyrosine were not required to elicit maturation (Fig. 4A, lanes
17-20, B, as indicated, and C
and D), higher levels of tyrosine enhanced the effect of the
V-ATPase inhibitors on tyrosinase (Fig. 4B). Dose response analysis showed that concanamycin A and bafilomycin A1 were optimally effective at 20 and 50 nM, respectively. However, 5 nM of each inhibitor was sufficient to induce tyrosinase
maturation (Fig. 4C). At optimal concentrations, high
molecular weight forms of tyrosinase began to accumulate within 30 min
of incubation with maximum effect reaching within 3 h (Fig.
4D). The low concentration required to elicit an effect and
the higher effectiveness of concanamycin A over bafilomycin A1 on
tyrosinase maturation are indicative of specific inhibition of V-ATPase
and in agreement with the relative potency of each compound toward
V-ATPase inhibition (43).
View larger version (79K):
[in this window]
[in a new window]
|
Fig. 4.
Inhibitors of V-ATPase enhance tyrosinase
maturation. A, Western blot analyses for tyrosinase
(TYR) normalized to actin using whole cell lysates derived
from normal melanocytes (NM) and melanoma cells (YUGEN8, 501 mel, and YUSIT1) or WGA-bound glycoproteins from YUSAC2 melanoma cells.
The various cell types were incubated for 4 h before harvest in
medium supplemented with the diluent 1 µl/ml Me2SO
(DMSO), 10 µM monensin (Mon),
concanamycin A (CCM), or bafilomycin A1 (Baf) at
100 nM each. Ham's F-10 medium supplemented with low (10 µM, lanes 1-4) or high tyrosine (100 µM, lanes 5-20) was used. Solid
and empty arrows indicate mature and immature unprocessed
tyrosinase proteins, respectively. B, high concentration of
tyrosine in the medium enhanced the concanamycin A-induced tyrosinase
maturation in melanoma cells. YUGEN8 cells were harvested after 4-h
incubation in Ham's F-10 medium with low (10 µM) or high
(100 µM) tyrosine in the absence and presence of
concanamycin A (100 nM). C, dose response of
YUGEN8 melanoma cells to CCM and Baf supplemented to Ham's F-10 medium
(10 µM tyrosine). Cells were harvested after incubation
in the experimental medium for 4 h. D, kinetics
of tyrosinase maturation in melanoma cells. YUGEN8 melanoma cells were
incubated in unmodified Ham's F-10 medium (10 µM
tyrosine) supplemented with CCM (20 nM) or Baf (50 nM) for increasing duration.
|
|
Interestingly, despite a marked increase in pigmentation (data not
shown), monensin did not affect the SDS-PAGE migration pattern and
abundance of tyrosinase (Fig. 4A, lanes 6,
10, 14, and 18). Modification of
tyrosinase in the Golgi in response to the V-ATPase inhibitors but not
after monensin treatment was further confirmed by the accumulation of
the 80-kDa mature tyrosinase (Fig.
5A, lanes 1-8,
compare bands marked with empty and solid arrows, respectively). The simultaneous addition of monensin and concanamycin A prevented the concanamycin A induced tyrosinase maturation (Fig. 5A, lanes 9-12), suggesting a
block in the ER, ERGIC, or cis-Golgi, because monensin
blocks trafficking in a pre-Golgi compartment without interfering with
Golgi enzymes (48-50). Pulse-chase experiments confirmed that
concanamycin A and bafilomycin A1 but not monensin enhanced the Golgi
modification of newly synthesized tyrosinase in melanoma cells (Fig.
5B, YUGEN8, lanes 1-12,
17-20, bands marked with arrow).
View larger version (45K):
[in this window]
[in a new window]
|
Fig. 5.
Golgi modification of tyrosinase in response
to V-ATPase and protease inhibitors. A, steady-state
tyrosinase as revealed by anti-tyrosinase Western blotting. Cells were
treated with 1 µl/ml Me2SO (DMSO), 20 µM monensin (Mon), 20 nM
concanamycin A (CCM), 50 nM bafilomycin A1
(Baf), or 10 µg/ml leupeptin and 25 µg/ml pepstatin
(Leu/Pep) for 3 h. Tyrosinase was precipitated from
melanoma cell extracts (YUGEN8 and 501 mel) with
WGA-bound beads. Endo H-digested (lanes 1-8) or
non-digested (lanes 9-12) proteins were subjected to
SDS-PAGE and Western blotting. Alternatively, immunoprecipitated
tyrosinase (C-19 antibodies) was subjected to treatment with or without
Endo H (lanes 13-20). Solid and empty
arrows indicate mature and immature tyrosinase, respectively.
Band marked is the deglycosylated (DG) tyrosinase
polypeptide. Note that the x-ray film representing lanes
17-20 was overexposed to rule out the presence of any minor
bands. B, autoradiogram of metabolically radiolabeled
tyrosinase immunoprecipitated from YUGEN8 melanoma cells incubated in
Ham's F-10 medium containing 100 µM tyrosine with
inhibitors noted above. Cells were metabolically labeled with
[35S]Met/Cys for 15 min and harvested immediately (0 h)
or after a 3-h chase in non-radioactive medium (3 h). The indicated
agents were present during the 2-h starvation in Cys/Met-free
medium.
|
|
To determine whether tyrosinase stabilization by alkalinization or
inhibition of V-ATPases could be attributed to the interference with
lysosomal proteolysis, tyrosinase was monitored after inhibition of the
lysosomal proteases with leupeptin and pepstatin. Treatment of melanoma
cells with leupeptin and pepstatin caused only a slight increase in the
levels of steady-state or newly synthesized tyrosinase with complex
carbohydrates in YUGEN8 (Fig. 5A, lanes 13-16,
and B, lanes 13-16) but not in 501 mel cells
(Fig. 5A, lanes 17-20). The results indicated
that although tyrosinase in small amounts was able to reach a
post-Golgi compartment in some melanoma cell strains, lysosomal
protease inhibition could not account for the pigmentation and enhanced
maturation of tyrosinase observed after alkalinization or V-ATPase inhibition.
Exit of Tyrosinase from the ER in Response to Intracellular
Alkalinization--
Confocal immunofluorescence analyses indicated
that tyrosinase remained in the ER in melanoma cells under steady-state
conditions (Fig. 6). Antibodies to
ERGIC-53 and COPI stained normal melanocytes and melanoma cells in a
characteristic perinuclear crescent shape pattern representing the
Golgi as well as in punctate structures peripheral to the ER region
corresponding to the ERGIC and the ER. In normal melanocytes, only
partial overlap was seen between tyrosinase and ERGIC-53 or COPI (Fig.
6, NM). In contrast, in the melanoma cells, tyrosinase
colocalized with ERGIC-53 and COPI in the ER region but not in the
ERGIC or Golgi regions as shown by the red rhodamine vesicles
containing ERGIC-53 or COPI that did not merge with green fluorescein
isothiocyanate-tyrosinase (Fig. 6, YUGEN8). Therefore,
if tyrosinase travels beyond the ER in untreated melanoma cells, its
presence there must be short-lived, as it cannot be detected under
steady-state conditions by immunostaining.
View larger version (42K):
[in this window]
[in a new window]
|
Fig. 6.
Tyrosinase is not present in the ERGIC or
cis-Golgi in melanoma cells.
Immunofluorescence confocal microscopy images are shown with
immunostaining of tyrosinase (green) and ERGIC-53 or COPI
(red) in normal human melanocytes (NM) and
melanoma cells (YUGEN8). The panels on the right
display merged images. Notice that tyrosinase is spread out in regions
that do not include the ERGIC in melanoma cells. The non-overlapping
red punctated vesicles are particularly obvious above the nucleus of
YUGEN8 melanoma cells stained with either ERGIC-53 or COPI
(MERGE).
|
|
Simultaneous immunostaining with tyrosinase and the ER
marker calnexin showed that tyrosinase exited from the ER in response to concanamycin A and monensin (Fig. 7).
Within 1-h treatment with concanamycin A, tyrosinase appeared in
structures that did not coincide with the ER (Fig. 7,
CCM, 1 h). After 2-h treatment, tyrosinase
localized in tubules extending from perinuclear compartments across the
cell (Fig. 7, CCM, 2 h). Tyrosinase was also
distributed outside the ER and did not colocalize with calnexin after a
2-h incubation with monensin (Fig. 7, Mon). The
confocal images confirmed the steady-state immunoblotting results
demonstrating exit of tyrosinase from the ER in response to imposed
alkalinization. Although the nature of the tyrosinase-positive post-ER
structures after monensin and concanamycin A treatment has yet to be
determined, it is possible that the enzyme was exported to distant
sites by two different pathways, one that involved the Golgi
medial-processing compartment and the other that did not.
View larger version (69K):
[in this window]
[in a new window]
|
Fig. 7.
Tyrosinase export from the ER is induced by
V-ATPase inhibition. Forced pH changes across vacuolar
compartment-induced export of tyrosinase to distal sites.
Immunofluorescence confocal microscopy was performed on YUGEN8 melanoma
cells grown in Ham's F-10 medium after treatment with 1 µl/ml
Me2SO (DMSO) for 2 h, 10 µM
monensin (Mon) for 2 h, or 20 nM
concanamycin A (CCM) for 1 or 2 h as indicated. The
left green panels represent tyrosinase (TYR)
detected with anti-tyrosinase antibodies (C-19), the red middle
panels show the localization of the ER resident protein calnexin
(CNX), and the right panels display merged images in
yellow (Merge).
|
|
| |
DISCUSSION |
We provided evidence that abnormal acidification of the
extracellular milieu is the probable reason for the decline in
tyrosinase catalytic activity in tyrosinase-positive amelanotic
melanoma cells. In these cells, tyrosinase catalytic activity was
restored by alkalinization in a manner dependent on the presence of
extracellular tyrosine. Alkalinization was accomplished by adjusting
the pH of the extracellular medium, by glucose deprivation, or by using agents that inhibit vacuolar proton ATPases or dissipate pH gradients across membranes. Therefore, the inactivation of tyrosinase is likely
to be the consequence of increased proton pump activity in the
malignant cells compared with normal melanocytes. This change was also
reflected by the appearance of higher pHi under steady-state conditions
in melanoma cells. The higher proton pump activity is probably
localized at both the cell membrane and within the endomembranes.
Whereas Na+/H+ antiporters and
Cl/HCO3 exchangers are known to be activated
in tumor cells in order to maintain pHi, V-ATPases are the major proton
pumps of vesicular compartments (reviewed in Ref. 24). V-ATPases play a
principle role in generating and maintaining the acidic environment in
the lumen of intracellular organelles such as the Golgi, endosomes, and
lysosomes (reviewed in Refs. 51-54). Although the Golgi contains active V-ATPases, the ER does not (47, 55, 56). Therefore, tyrosinase
may encounter an increased activity of this proton pump in a
compartment anterograde to the ER in melanoma cells.
The ionophore monensin and two V-ATPase inhibitors allowed the release
of tyrosinase from the ER and induced pigmentation, yet only the
V-ATPase inhibitors promoted tyrosinase acquisition of complex sugars.
Monensin and the V-ATPase inhibitors affect luminal processes at the
ER-Golgi boundary via different mechanisms. Monensin blocks ER
trafficking of glycoproteins such as IgG and transferrin in a pre-Golgi
compartment without interfering with Golgi enzymes (48-50). On the
other hand, bafilomycin A1 inhibits retrograde transport of proteins
such as ERGIC-53 from the pre-Golgi-compartment back to the ER but not
the anterograde transport of proteins from the ER to the Golgi (55).
Because both agents cause alkalinization of subcellular organelles,
tyrosinase exit from the ER and pigmentation was probably enhanced
because of activation of enzymatic activity by the increased pH.
In vitro tyrosinase activity employing cell extracts from
normal and malignant melanocytes expressing mature and immature forms,
respectively, showed a pH-dependent activity with
tyrosinase being 2-5-fold more active at pH 8.0 compared with pH 6.3 (data not shown). Therefore, like in vivo, the in vitro activation did not require modification to complex carbohydrates.
This conclusion is consistent with published values of pH within the
secretory pathway and their changes in response to V-ATPase inhibition
(46, 48). The ER and the Golgi maintain a pH of 7.2 ± 0.2 and
6.4 ± 0.3, respectively, and bafilomycin A1 induced alkalinization of the various regions of the Golgi complex but did not
affect the pH of the ER (57). Therefore, the aberrant accumulation of
tyrosinase in the ER of melanoma cells raises the possibility that the
acidified ER-Golgi boundary of melanoma cells is hostile to tyrosinase
maturation. Even small changes in luminal pH can cause a significant
change in protein processing and activation as shown for the processing
of adrenocorticotropic hormone from its pro-opiomelanocortin precursor
(58).
Quality control processes that monitor the fidelity of the maturation
process appear to be in place throughout the secretory pathway (59).
Some misfolded or partially assembled proteins that have escaped the ER
can still be subjected to quality control in the early secretory
system, because they can be retrieved from post-ER compartments back to
the ER through COPI vesicles (60-62). In these cases, the inhibition
of the COPI retrieval system induced the accumulation of the respective
protein in post-ER compartments.
In light of these observations, the accumulation of tyrosinase in the
ER of melanoma cells might also be the result of the quality control
system in the ERGIC-cis-Golgi. Tyrosinase under steady-state
conditions colocalized with the ER marker calnexin and with the ER
portion of ERGIC-53 and COPI, suggesting a rapid retrograde transport
to the ER if it reached a post-ER-pre-Golgi compartment. The
observations that monensin, even in the presence of concanamycin A,
elicited tyrosinase activation, ER exit, transport to distant sites,
and pigmentation in the absence of Golgi processing, suggesting that
monensin acts by dissipating a pH gradient upstream of the concanamycin
A-affected site such as the ERGIC. These results also demonstrate that
basic pH is sufficient to activate tyrosinase, which is in agreement
with the pH-dependent in vitro tyrosinase activity, and that the addition of complex oligosaccharides is dispensable for tyrosinase activity.
The concept of abnormal acidification of intracellular organelles
including the melanosomes as the cause for an amelanotic phenotype is
supported also by genetic evidence. Oculocutaneous albinism 2 is
an inherited condition in which individuals suffer loss-of-function
mutation in the P-protein (63-66). The P-protein is a 110-kDa
melanosomal protein (67) with 12 putative membrane-spanning domains and
homology to known transporters (68). In the absence of normal
P-protein, there is an imbalance in the intracellular pH of
melanosomes, disruption in melanosomal structure, and misrouting of
tyrosinase to other sites including the cell membrane (69-71). It was
recently suggested that the P-protein acts as a
Na+/H+ exchanger in the melanosomes (72, 73).
The homology to Escherichia coli
Na+/H+ antiporter and the observation that
dissipating pH gradients or inhibiting V-ATPase activity in mouse
melanocytes carrying the P-mutation restored pigmentation (72) supports
this possibility.
We suggest that tyrosinase maturation is particularly vulnerable to pH
changes, because of its oxidoreductase activity and its dependence on
DOPA for activation. The acidic pH may have inactivated tyrosinase by
the protonation of DOPA, the critical cofactor and substrate for
tyrosinase (1, 2, 74-76). Unlike tyrosine, DOPA and other catechols
can be oxidized to the corresponding quinone by the oxidized
form of the enzyme (Cu II state without bound dioxygen), thus reducing
the copper atoms in the active site and enabling the generation of the
active oxygen-bound form (2, 75, 76). Protonation of DOPA prevents the
formation of DOPAquinone, the intermediate required for DOPA
regeneration (2, 29, 76). The precise mechanism by which DOPA is
regenerated from DOPAquinone is not yet determined, but it is possible
that DOPAquinone is reduced to DOPA through the oxidation of critical sulfhydryl groups on tyrosinase, forming the final disulfide bond(s) required to stabilize the protein in its native/active form. In this
scenario, the depletion of DOPAquinone leads to the accumulation of
misfolded tyrosinase in the ER or the ER-Golgi boundary. The requirement for a tyrosinase reaction product in tyrosinase proper folding may explain the uniqueness of tyrosinase sensitivity to proton
changes, because the maturation of the homologous melanocyte-specific glycoprotein, gp75/TRP1, within melanoma cells is unaffected (77).
Our results provide an explanation for the appearance of amelanotic
clones in primary and metastatic pigmented tumors in which tyrosinase
accumulates in the ER as a result of organelle acidification in
vivo. It would be of interest to correlate the appearance of amelanotic clones in primary and metastatic pigmented tumors with rates
of glucose uptake and the acquisition of drug resistance to further
substantiate that down-regulation of tyrosinase is a consequence of
these metabolic changes in vivo.
| |
ACKNOWLEDGEMENTS |
We thank Drs. L. Old (Memorial
Sloan-Kettering Cancer Center, New York, NY) for anti-tyrosinase 3T11
mAb, H.-P. Hauri for the ERGIC-53 antibodies, G. Warren for the rabbit
polyclonal anti--COPI antibodies, and M. S. Marks for the MNT1
melanoma cells.
| |
FOOTNOTES |
*
This work was supported by U. S. Public Health Service
Grants AR39848 and CA44542 (to R. H.), AR41942 (to R. E. Tigelaar, Yale Skin Diseases Research Center), and CA79864 (to D. N. H.).The costs of publication of this
article were defrayed in part by the
payment of page charges. The article
must therefore be hereby marked
"advertisement" in
accordance with 18 U.S.C. Section
1734 solely to indicate this fact.
§
To whom correspondence may be addressed: Dept. of Dermatology, Yale
University School of Medicine, P. O. Box 208059, HRT 610, 15 York St.,
New Haven, CT 06520-8059. Tel.: 203-785-4352; Fax: 203-785-7637;
E-mail: ruth.halaban@yale.edu.
§§
To whom correspondence may be addressed: Dept. of
Biochemistry & Molecular Biology, University of Massachusetts, Lederle
Graduate Research Tower, 818, Box 34505, Amherst, MA 01003. Tel.:
413-545-0079; Fax: 413-545-3291; dhebert@biochem.umass.edu.
Published, JBC Papers in Press, January 25, 2002, DOI 10.1074/jbc.M111497200
2
R. Halaban, E. Cheng, and D. N. Hebert,
unpublished results that are in agreement with the findings published
in Ref. 44.
| |
ABBREVIATIONS |
The abbreviations used are:
ER, endoplasmic reticulum;
Endo H, endoglycosidase H;
BCECF-AM, 2',7'-bis(2-carboxyethyl)-5(6)-carboxyfluorescein acetoxymethyl ester;
ERGIC, ER-Golgi intermediate compartment;
mAb, monoclonal antibody;
pHe, extracellular pH;
pHi, intracellular pH;
CHAPS, 3-[(3-cholamidopropyl)dimethylammonio]-1-propanesulfonic acid;
WGA, wheat germ agglutinin;
V-ATPase, vacuolar proton ATPase;
PBS, phosphate-buffered saline;
DOPA, dihydroxyphenylalanine.
| |
REFERENCES |
| 1.
|
Lerner, A. B.,
Fitzpatrick, T. B.,
Calkins, E.,
and Summerson, W. H.
(1949)
J. Biol. Chem.
178,
185-195[Free Full Text]
|
| 2.
|
Riley, P. A.
(1999)
Cell. Mol. Biol.
45,
951-960[Medline]
[Order article via Infotrieve]
|
| 3.
|
Kang, X. Q.,
Kawakami, Y.,
Elgamil, M.,
Wang, R. F.,
Sakaguchi, K.,
Yannelli, J. R.,
Appella, E.,
Rosenberg, S. A.,
and Robbins, P. F.
(1995)
J. Immunol.
155,
1343-1348[Abstract]
|
| 4.
|
Topalian, S. L.,
Gonzales, M. I.,
Parkhurst, M., Li, Y. F.,
Southwood, S.,
Sette, A.,
Rosenberg, S. A.,
and Robbins, P. F.
(1996)
J. Exp. Med.
183,
1965-1971[Abstract/Free Full Text]
|
| 5.
|
Cormier, J. N.,
Abati, A.,
Fetsch, P.,
Hijazi, Y. M.,
Rosenberg, S. A.,
Marincola, F. M.,
and Topalian, S. L.
(1998)
J. Immunother.
21,
27-31[Medline]
[Order article via Infotrieve]
|
| 6.
|
Halaban, R.,
Cheng, E.,
Zhang, Y.,
Moellmann, G.,
Hanlon, D.,
Michalak, M.,
Setaluri, V.,
and Hebert, D. N.
(1997)
Proc. Natl. Acad. Sci. U. S. A.
94,
6210-6215[Abstract/Free Full Text]
|
| 7.
|
Mosse, C. A.,
Meadows, L.,
Luckey, C. J.,
Kittlesen, D. J.,
Huczko, E. L.,
Slingluff, C. L.,
Shabanowitz, J.,
Hunt, D. F.,
and Engelhard, V. H.
(1998)
J. Exp. Med.
187,
37-48[Abstract/Free Full Text]
|
| 8.
|
Halaban, R.,
Svedine, S.,
Cheng, E.,
Smicun, Y.,
Aron, R.,
and Hebert, D. N.
(2000)
Proc. Natl. Acad. Sci. U. S. A.
97,
5889-5894[Abstract/Free Full Text]
|
| 9.
|
Berson, J. F.,
Frank, D. W.,
Calvo, P. A.,
Bieler, B. M.,
and Marks, M. S.
(2000)
J. Biol. Chem.
275,
12281-12289[Abstract/Free Full Text]
|
| 10.
|
Toyofuku, K.,
Wada, I.,
Spritz, R. A.,
and Hearing, V. J.
(2001)
Biochem. J.
355,
259-269[CrossRef][Medline]
[Order article via Infotrieve]
|
| 11.
|
Halaban, R.,
Cheng, E.,
Svedine, S.,
Aron, R.,
and Hebert, D. N.
(2001)
J. Biol. Chem.
276,
11933-11938[Abstract/Free Full Text]
|
| 12.
|
Engin, K.,
Leeper, D. B.,
Cater, J. R.,
Thistlethwaite, A. J.,
Tupchong, L.,
and McFarlane, J. D.
(1995)
Int. J. Hyperthermia
11,
211-216[Medline]
[Order article via Infotrieve]
|
| 13.
|
Levine, E. A.,
Holzmayer, T. A.,
Roninson, I. B.,
and Das Gupta, T. K.
(1993)
J. Surg. Res.
54,
621-624[CrossRef][Medline]
[Order article via Infotrieve]
|
| 14.
|
Berger, W.,
Elbling, L.,
Minai-Pour, M.,
Vetterlein, M.,
Pirker, R.,
Kokoschka, E. M.,
and Micksche, M.
(1994)
Int. J. Cancer
59,
717-723[Medline]
[Order article via Infotrieve]
|
| 15.
|
Schadendorf, D.,
Makki, A.,
Stahr, C.,
van Dyck, A.,
Wanner, R.,
Scheffer, G. L.,
Flens, M. J.,
Scheper, R.,
and Henz, B. M.
(1995)
Am. J. Pathol.
147,
1545-1552[Abstract]
|
| 16.
|
Burd, R.,
Wachsberger, P. R.,
Biaglow, J. E.,
Wahl, M. L.,
Lee, I.,
and Leeper, D. B.
(2001)
Cancer Res.
61,
5630-5635[Abstract/Free Full Text]
|
| 17.
|
Stubbs, M.,
McSheehy, P. M.,
Griffiths, J. R.,
and Bashford, C. L.
(2000)
Mol. Med. Today
6,
15-19[CrossRef][Medline]
[Order article via Infotrieve]
|
| 18.
|
Dang, C. V.,
Lewis, B. C.,
Dolde, C.,
Dang, G.,
and Shim, H.
(1997)
J. Bioenerg. Biomembr.
29,
345-354[CrossRef][Medline]
[Order article via Infotrieve]
|
| 19.
|
Warburg, O.
(1956)
Science
123,
309-314[Free Full Text]
|
| 20.
|
Racker, E.
(1983)
Science
222,
232[Free Full Text]
|
| 21.
|
Rinne, D.,
Baum, R. P.,
Hor, G.,
and Kaufmann, R.
(1998)
Cancer
82,
1664-1671[CrossRef][Medline]
[Order article via Infotrieve]
|
| 22.
|
Altan, N.,
Chen, Y.,
Schindler, M.,
and Simon, S. M.
(1998)
J. Exp. Med.
187,
1583-1598[Abstract/Free Full Text]
|
| 23.
|
Schindler, M.,
Grabski, S.,
Hoff, E.,
and Simon, S. M.
(1996)
Biochemistry
35,
2811-2817[CrossRef][Medline]
[Order article via Infotrieve]
|
| 24.
|
Simon, S. M.
(1999)
Drug Discov. Today
4,
32-38[CrossRef][Medline]
[Order article via Infotrieve]
|
| 25.
|
Martinez-Zaguilan, R.,
Lynch, R. M.,
Martinez, G. M.,
and Gillies, R. J.
(1993)
Am. J. Physiol.
265,
C1015-C1029[Medline]
[Order article via Infotrieve]
|
| 26.
|
Martinez-Zaguilan, R.,
Raghunand, N.,
Lynch, R. M.,
Bellamy, W.,
Martinez, G. M.,
Rojas, B.,
Smith, D.,
Dalton, W. S.,
and Gillies, R. J.
(1999)
Biochem. Pharmacol.
57,
1037-1046[CrossRef][Medline]
[Order article via Infotrieve]
|
| 27.
|
Yamagata, M.,
Hasuda, K.,
Stamato, T.,
and Tannock, I. F.
(1998)
Br. J. Cancer
77,
1726-1731[Medline]
[Order article via Infotrieve]
|
| 28.
|
Simon, S.,
Roy, D.,
and Schindler, M.
(1994)
Proc. Natl. Acad. Sci. U. S. A.
91,
1128-1132[Abstract/Free Full Text]
|
| 29.
|
Naish-Byfield, S.,
and Riley, P. A.
(1998)
Pigment Cell Res.
11,
127-133[CrossRef][Medline]
[Order article via Infotrieve]
|
| 30.
|
Halaban, R.,
Cheng, E.,
Smicun, Y.,
and Germino, J.
(2000)
J. Exp. Med.
191,
1005-1015[Abstract/Free Full Text]
|
| 31.
|
Cuomo, M.,
Nicotra, M. R.,
Apollonj, C.,
Fraioli, R.,
Giacomini, P.,
and Natali, P. G.
(1991)
J. Invest. Dermatol.
96,
446-451[CrossRef][Medline]
[Order article via Infotrieve]
|
| 32.
|
Raposo, G.,
Tenza, D.,
Murphy, D. M.,
Berson, J. F.,
and Marks, M. S.
(2001)
J. Cell Biol.
152,
809-824[Abstract/Free Full Text]
|
| 33.
|
Chen, Y. T.,
Stockert, E.,
Tsang, S.,
Coplan, K. A.,
and Old, L. J.
(1995)
Proc. Natl. Acad. Sci. U. S. A.
92,
8125-8129[Abstract/Free Full Text]
|
| 34.
|
Pomerantz, S. H.
(1976)
Anal. Biochem.
75,
86-90[CrossRef][Medline]
[Order article via Infotrieve]
|
| 35.
|
Halaban, R.,
and Lerner, A. B.
(1977)
Exp. Cell Res.
108,
119-125[Medline]
[Order article via Infotrieve]
|
| 36.
|
Halaban, R.,
Moellmann, G.,
Tamura, A.,
Kwon, B. S.,
Kuklinska, E.,
Pomerantz, S. H.,
and Lerner, A. B.
(1988)
Proc. Natl. Acad. Sci. U. S. A.
85,
7241-7245[Abstract/Free Full Text]
|
| 37.
|
Owen, C. S.,
Pooler, P. M.,
Wahl, M. L.,
Coss, R. A.,
and Leeper, D. B.
(1997)
J. Cell. Physiol.
173,
397-405[CrossRef][Medline]
[Order article via Infotrieve]
|
| 38.
|
Wahl, M. L.,
Pooler, P. M.,
Briand, P.,
Leeper, D. B.,
and Owen, C. S.
(2000)
J. Cell. Physiol.
183,
373-380[CrossRef][Medline]
[Order article via Infotrieve]
|
| 39.
|
Újvári, A.,
Aron, R.,
Eisenhaure, T.,
Cheng, E.,
Smicun, Y.,
Halaban, R.,
and Hebert, D. N.
(2001)
J. Biol. Chem.
276,
5924-5931[Abstract/Free Full Text]
|
| 40.
|
Gillies, R. J.,
Martinez-Zaguilan, R.,
Martinez, G. M.,
Serrano, R.,
and Perona, R.
(1990)
Proc. Natl. Acad. Sci. U. S. A.
87,
7414-7418[Abstract/Free Full Text]
|
| 41.
|
Martinez-Zaguilan, R.,
and Gillies, R. J.
(1992)
Ann. N. Y. Acad. Sci.
671,
478-480[CrossRef][Medline]
[Order article via Infotrieve]
|
| 42.
|
Maxfield, F. R.
(1982)
J. Cell Biol.
95,
676-681[Abstract/Free Full Text]
|
| 43.
|
Dröse, S.,
and Altendorf, K.
(1997)
J. Exp. Biol.
200,
1-8[Abstract]
|
| 44.
|
Fuller, B. B.,
Spaulding, D. T.,
and Smith, D. R.
(2001)
Exp. Cell Res.
262,
197-208[CrossRef][Medline]
[Order article via Infotrieve]
|
| 45.
|
Ancans, J.,
Tobin, D. J.,
Hoogduijn, M. J.,
Smit, N. P.,
Wakamatsu, K.,
and Thody, A. J.
(2001)
Exp. Cell Res.
268,
26-35[CrossRef][Medline]
[Order article via Infotrieve]
|
| 46.
|
Mellman, I.,
Fuchs, R.,
and Helenius, A.
(1986)
Annu. Rev. Biochem.
55,
663-700[CrossRef][Medline]
[Order article via Infotrieve]
|
| 47.
|
Wu, M. M.,
Llopis, J.,
Adams, S.,
McCaffery, J. M.,
Kulomaa, M. S.,
Machen, T. E.,
Moore, H. P.,
and Tsien, R. Y.
(2000)
Chem. Biol.
7,
197-209[CrossRef][Medline]
[Order article via Infotrieve]
|
| 48.
|
Tartakoff, A. M.
(1983)
Cell
32,
1026-1028[CrossRef][Medline]
[Order article via Infotrieve]
|
| 49.
|
Tartakoff, A. M.,
and Vassalli, P.
(1977)
J. Exp. Med.
146,
1332-1345[Abstract/Free Full Text]
|
| 50.
|
Strous, G. J.,
and Lodish, H. F.
(1980)
Cell
22,
709-717[CrossRef][Medline]
[Order article via Infotrieve]
|
| 51.
|
Forgac, M.
(1999)
J. Biol. Chem.
274,
12951-12954[Free Full Text]
|
| 52.
|
Nelson, N.,
and Harvey, W. R.
(1999)
Physiol. Rev.
79,
361-385[Abstract/Free Full Text]
|
| 53.
|
Finbow, M. E.,
and Harrison, M. A.
(1997)
Biochem. J.
324,
697-712[Medline]
[Order article via Infotrieve]
|
| 54.
|
Stevens, T. H.,
and Forgac, M.
(1997)
Annu. Rev. Cell Dev. Biol.
13,
779-808[CrossRef][Medline]
[Order article via Infotrieve]
|
| 55.
|
Palokangas, H.,
Ying, M.,
Vaananen, K.,
and Saraste, J.
(1998)
Mol. Biol. Cell
9,
3561-3578[Abstract/Free Full Text]
|
| 56.
|
Kim, J. H.,
Johannes, L.,
Goud, B.,
Antony, C.,
Lingwood, C. A.,
Daneman, R.,
and Grinstein, S.
(1998)
Proc. Natl. Acad. Sci. U. S. A.
95,
2997-3002[Abstract/Free Full Text]
|
| 57.
|
Wu, M. M.,
Llopis, J.,
Adams, S. R.,
McCaffery, J. M.,
Teter, K.,
Kulomaa, M. S.,
Machen, T. E.,
Moore, H. P.,
and Tsien, R. Y.
(2000)
Methods Enzymol.
327,
546-564[Medline]
[Order article via Infotrieve]
|
| 58.
|
Schmidt, W. K.,
and Moore, H. P.
(1995)
Mol. Biol. Cell
6,
1271-1285[Ab |
TOP
ABSTRACT
INTRODUCTION
