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J Biol Chem, Vol. 275, Issue 16, 12281-12289, April 21, 2000
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From the Department of Pathology and Laboratory Medicine, University of Pennsylvania, Philadelphia, Pennsylvania 19104-6082
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ABSTRACT |
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 TOP
 ABSTRACT
 INTRODUCTION
EXPERIMENTAL PROCEDURES
RESULTS
DISCUSSION
REFERENCES
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Oculocutaneous albinism type 1TS is caused by
mutations that render the melanocyte-specific enzyme tyrosinase
temperature-sensitive (ts); the enzyme is inactive in cells grown at
37 °C but displays full activity in cells grown at 31 °C. To
distinguish whether the ts phenotype of the common R402Q variant of
human tyrosinase is due to altered enzymatic activity or to misfolding
and a defect in intracellular trafficking, we analyzed its localization
and processing in transiently transfected HeLa cells. R402Q tyrosinase accumulates in the endoplasmic reticulum (ER) at 37 °C but exits the
ER and accumulates in endosomal structures in cells grown at 31 °C.
The inability of the R402Q variant to exit the ER is confirmed by the
failure to acquire endoglycosidase H resistance at 37 °C and cannot
be accounted for solely by enhanced proteasome-mediated degradation. ER
retention at 37 °C is mediated by the lumenal domain of R402Q
tyrosinase, is not dependent on tethering to the membrane, and is
irreversible. Finally, a wild-type allelic form of tyrosinase is
partially ts in transiently transfected HeLa cells. The data show that
human tyrosinase expressed in non-melanogenic cells folds and exits the
ER inefficiently and that R402Q tyrosinase exaggerates this defect,
resulting in a failure to exit the ER at physiologic temperatures.
Oculocutaneous albinism type 1 (OCA1)1
comprises a group of human disorders
characterized by reduced or absent skin pigmentation, vision defects
due to reduced optical pigmentation and to misrouting of optic nerve
fibers, and enhanced sensitivity to skin and optical cancers (1). These
disorders are caused by germline mutations within the coding region of
the melanocyte-specific gene product tyrosinase (2-4). Tyrosinase, a
key enzyme in the synthesis of melanin (reviewed in Ref. 5) is a type I
integral membrane glycoprotein that is specifically expressed in cells
of the melanocyte lineage, where it localizes to a specialized late
endosome-like compartment, the melanosome (6). Within melanosomes,
tyrosinase initiates melanin formation by enzymatic tyrosine
hydroxylase and L-3,4-dihyroxyphenylalanine (DOPA) oxidase
activities that are associated with its lumenal domain; a
5,6-dihydroxyindole oxidase activity, also a property of the tyrosinase
lumenal domain, may contribute to a subsequent step in melanin
synthesis (reviewed in Ref. 1). Lack of tyrosinase activity results in
the absence of melanin formation due to the inability to form the
melanin precursors, L-3,4-dihyroxyphenylalanine and
L-3,4-dihyroxyphenylalanine quinone. OCA1 is a direct
result of the absence or reduction of melanin.
Different germline mutations within the tyrosinase coding region
underlie OCA1 disorders of varying severity. In one unusual subset of
OCA1, OCA1 TS, the mutations render tyrosinase temperature-sensitive (ts). Consequently, melanin synthesis only occurs in cooler areas of
the body, such as the arms and legs. The resultant pattern of
peripheral pigmentation is analogous to that of the Siamese cat and the
Himalayan mouse (7, 8). A number of ts variants of tyrosinase have been
molecularly cloned. One variant results from a single base missense
mutation that alters an arginine at amino acid position 402 to a
glutamine (R402Q). The allele encoding the R402Q variant of tyrosinase
is extremely prevalent, representing about 15% of the gene pool among
Caucasians (8). Studies in cultured transfected cells of the R402Q
variant and the similar but less prevalent R422Q variant have shown
that they have ts activity; transfected cells grown at 37 °C display
none of the described tyrosinase enzymatic activities, whereas
transfected cells grown at 31 °C display all three activities,
comparable with that of wild-type (9, 10). Both variants contain
mutations that affect residues close to a defined copper binding site
within the lumenal domain (11). Nevertheless, the molecular mechanisms by which these mutations render the variants ts have not been elucidated.
ts enzyme activity is a reflection of a conformational defect at
elevated temperatures and stabilization of an active conformation at
reduced temperatures. Defects at the restrictive temperature may be
subtle such that only specific molecular contacts required for function
are lacking, as in the ts mutants of dynamin from Drosophila
melanogaster (12) and humans (13). Alternatively, defects may be
dramatic such that the ts protein is grossly misfolded at the
restrictive temperature (14), as seen in a number of genetic diseases
(15-18). Such ts mutants would be expected to be substrates for the
cellular quality control system. The quality control system
recognizes misfolded or unassembled polypeptides and either sequesters
them or targets them for degradation to prevent large scale protein
aggregation and consequent loss of cellular function (19, 20).
The major site for quality control within the secretory pathway is the
endoplasmic reticulum (ER) (21). Within the ER, newly synthesized
polypeptides are retained by the activity of resident chaperone
proteins until they are fully folded and assembled, at which point they
are released for transport to distal secretory compartments (19, 22,
23). Defective polypeptides that fail to fold and/or assemble are
retained within the ER and/or degraded by ER-associated or cytosolic
proteolytic systems, particularly the proteasome, after reverse
translocation into the cytosol (24). Should partially folded or
assembled proteins escape ER quality control and progress to distal
secretory compartments, they can be recognized at one of several
secondary sites for quality control, as evidenced by several examples
in yeast (25, 26), and targeted to lysosomes/vacuoles for degradation.
Finally, specific chaperones may act to prevent unfolding and
degradation within late endosomal/lysosomal compartments (27, 28).
Thus, quality control can be exerted at multiple sites within the
secretory/endosomal system. ts enzymes with gross defects in folding
would be expected to be subject to one or all of these quality control checkpoints.
For ts gene products that result in human disorders, distinguishing
between subtle and dramatic protein folding defects and determining the
intracellular site at which the ts phenotype emerges is important in
designing therapeutics to allay clinical symptoms. Here, we analyze the
localization and processing of the R402Q variant of human tyrosinase
and show that the ts phenotype is due to a defect in protein folding
that prevents ER exit. The partial ts phenotype of a wild-type (WT)
allelic form of tyrosinase and the lack of an apparent significant
increase in ER-associated degradation of the R402Q variant suggest that
the R402Q variation exaggerates an inefficient folding process inherent
in human tyrosinase when expressed in non-melanogenic cells.
Cells, Culture Conditions, and Transfections--
HeLa cells
were maintained as described previously (29). Cells were transiently
transfected using calcium phosphate precipitation as described (30)
using 3-5 µg of total DNA in a 6-well dish for immunofluorescence
microscopy (IFM) analyses or 10-20 µg of total DNA/10-cm dish for
other analyses. Except where indicated below, DNA encoding the desired
construct represented a fraction of the total DNA (0.2 µg/well in a
6-well dish, 0.5-1 µg/10-cm dish) with pCDM8.1 used as carrier. In
some experiments, transfections were done using 2 µl of Fugene-6
(Roche Molecular Biochemicals) and 0.3 µg of desired construct/well
in a 6-well dish. After transfection, cells were incubated overnight at
37 °C, the medium was replaced, and the cells were grown at the
indicated temperature. Cells were generally analyzed 2 days
post-transfection.
Antibodies--
Plasmids--
Tyrosinase R402Q cloned in pCI (Promega), a kind
gift of Dr. W. Storkus (Univ. of Pittsburgh, Pittsburgh, PA), was
subcloned into pCDM8.1 (35) as an EcoRI fragment. Tyrosinase
cloned from the 501-mel cell line (36, 37), referred to here as WT
tyrosinase, encodes arginine at position 402 and the S192Y polymorphism
and was the kind gift of Dr. S. Topalian (National Cancer Institute). The WT tyrosinase insert excised from pCDNA3 using EcoRI
and XbaI was subcloned into pCDM8.1. TTT-HA and HA-tagged
chimeras between Tac and tyrosinase were constructed by overlapping
polymerase chain reaction (38) using pCI-tyrR402Q and Tac-Lamp1 (30) as
templates. For chimeric proteins with the tyrosinase lumenal domain, an
EcoRI-BglII fragment containing most of the
coding region for the lumenal domain of R402Q tyrosinase was subcloned into pCDM8.1 to create pYTSxx. Polymerase chain
reaction-generated BglII-XbaI inserts were
subcloned into pYTSxx or Tac-Lamp1 to generate the chimeric
expression vectors. Details of the polymerase chain reaction will be
provided upon request. In all chimeric constructs, the hydrophilic
amino acids surrounding the endogenous transmembrane domain were left
intact. YWTYT-HA and YWTTT-HA were generated by
excising the EcoRI-BglII fragment of
YTSYT-HA and YTSTT-HA, respectively, and
replacing it with the EcoRI-BglII fragment of
pCDM8.1-tyr501. Construction of TTY is described elsewhere (39).
Constructs were verified by automated DNA sequencing at the Nucleic
Acid Core Facility of Children's Hospital of Philadelphia. TT-lamp1
has been previously described (30).
Immunofluorescence Microscopy--
Cells grown on coverslips
were fixed with 2% formaldehyde in PBS and stained with unlabeled
primary antibodies and fluorescein isothiocyanate- and
lissamine-rhodamine-conjugated secondary antibodies as described (29).
Cells were analyzed on a Zeiss Axioplan microscope, photographed using
Kodak ASA 400 film, and digitized using a Nikon LS-1000 slide scanner.
Images were processed using Adobe Photoshop software. Images in Fig. 1
are from cells transfected with 3 µg of WT or R402Q tyrosinase/well
in a 6-well dish. Where indicated, cells were treated with 50 µg/ml
cycloheximide (CHX) for 2 h before fixation.
Metabolic Labeling and Immunoprecipitation--
HeLa cells
transfected in 10-cm dishes were harvested, preincubated, pulse-labeled
for 30 min with [35S]methionine/cysteine labeling mix
(NEN Life Science Products), and chased with excess methionine and
cysteine essentially as described (30), except that all procedures were
done at the indicated temperatures. Where indicated, 50 mM
ammonium chloride or 20 mM methionine methyl ester (MME)
was added to the chase medium. Cells were washed once with ice-cold
PBS, and cell pellets were stored at Western Blotting--
For experiments analyzing the effects of
proteasome inhibitors, transfected HeLa cells were released from 10-cm
plates by incubation in PBS, 10 mM EDTA, or trypsin, then
resuspended in fresh culture medium lacking or containing 0.2%
dimethyl sulfoxide with or without 50 µM MG-132
(Calbiochem) or 50 µM lactacystin (Calbiochem). Cells
were incubated as indicated and then harvested by centrifugation,
resuspended in PBS, divided into aliquots for endoglycosidase
treatment, and then lysed immediately by resuspension in 0.5% SDS, 1%
Expression and secretion of the polyhistidine-tagged soluble tyrosinase
constructs were analyzed as follows. HeLa cells were transfected with
15 µg of the desired construct/10-cm dish and incubated at 37 °C
overnight. The medium was then replaced, and the cells were incubated
at the indicated temperature for an additional 24 h. Where
indicated, 2 days post-transfection culture medium was replaced with
medium containing 10 µg/ml CHX. Cells were incubated for 30 min at
the initial temperature and then were either harvested or shifted to
the final temperature and grown for 7 h in fresh medium
supplemented with CHX, at which point both cells and culture medium
were harvested. Culture medium was clarified by centrifugation and
incubated with nickel nitrilotriacetic acid-Superflow beads (Qiagen,
Chatsworth, CA) for 3 h at 4 °C. The suspension was divided into three aliquots, the beads were pelleted and washed once with PBS,
and then either endoF-, endoH-, or mock-endoH-treated as above.
Proteins were eluted from the beads with SDS sample buffer containing
100 mM EDTA. Cell lysates were prepared as described above
following detachment of cells with PBS, 10 mM EDTA.
Samples were fractionated by SDS-PAGE using gels containing 10%
acrylamide, and proteins were electrophoretically transferred to
polyvinylidene difluoride membranes (Millipore, Bedford, MA). The
membranes were blocked in Blotto (PBS, 5% milk, 0.1% Tween 20),
incubated with NY8K or The R402Q Variant of Human Tyrosinase Accumulates in the ER at the
Nonpermissive Temperature--
We have shown that a WT allelic form of
human tyrosinase localizes predominantly to late endosomes and
lysosomes when expressed in non-melanocytic cells (39). To determine
whether tyrosinase with the R402Q variation is distinctly localized, we
analyzed transiently transfected HeLa cells expressing WT or R402Q
tyrosinase by IFM. As shown in Fig.
1a, WT tyrosinase localizes
primarily to punctate, vesicular structures throughout the cytoplasm of HeLa cells, with some perinuclear concentration. These structures contain lamp1 and lamp2 (not shown), confirming their identity as late
endosomes and lysosomes. In addition, WT tyrosinase is detected in
reticular structures and the nuclear envelope. In contrast, R402Q
tyrosinase localizes exclusively to the nuclear envelope and reticular
structures throughout the cytoplasm (Fig. 1c). This pattern
coincides with that of the ER resident chaperone protein, calnexin
(Fig. 1, e and f), suggesting that the R402Q variant accumulates in the ER. Similar observations were made in
several transfected cell lines, including the human melanoma line,
MelJuSo (data not shown), suggesting that this localization pattern is
specific to the R402Q variant and not merely a characteristic of
tyrosinase expression in HeLa cells.
The R402Q variant was previously shown to be ts, such that extracts
from transfected cells grown at 37 °C had defective tyrosinase activity, whereas extracts from cells grown at 31 °C had normal activity (10). We therefore tested whether the pattern of WT or R402Q
tyrosinase localization is changed in HeLa cells grown at 31 °C. As
shown in Fig. 1b, decreased growth temperature results in a
slight increase in the vesicular form of WT tyrosinase accompanied by a
decrease in reticular staining; this is consistent with enhanced stability and/or ER exit of WT tyrosinase. The effect of decreased temperature was much more dramatic for R402Q tyrosinase, which localized predominantly to vesicular structures in cells grown at
31 °C (Fig. 1d). Parallel experiments indicate that these
vesicular structures contain lamp1 but lack calnexin (data not shown).
These observations suggest that although the R402Q variant is retained within the ER at the nonpermissive temperature, a significant fraction
of it exits the ER and localizes to late endosomes in cells grown at
the permissive temperature.
Failure of the R402Q Variant Glycoprotein to Mature at the
Nonpermissive Temperature--
To confirm the IFM results and begin to
address the molecular basis for ER retention, we analyzed the behavior
of WT and R402Q tyrosinase molecules in transfected cells using
metabolic pulse-chase, immunoprecipitation, and SDS-PAGE. Transport of
tyrosinase through the secretory pathway was monitored by following the
maturation state of N-linked glycans using endoH and endoF,
which cleave only high mannose or all N-linked glycans,
respectively. Because processing of N-linked glycans results
in heterogeneity of tyrosinase migration by SDS-PAGE, acquisition of
resistance to endoH digestion was monitored as the loss of intensity of
the product of endoH digestion relative to the product of endoF digestion.
As shown in Fig. 2A, both WT
and R402Q tyrosinase, expressed in cells grown at either 31 °C or
37 °C, were initially synthesized as ~72-kDa glycoproteins that
are completely digested to ~55-60-kDa forms with either endoH or
endoF. This is consistent with glycosylation at five of the six
consensus sites and localization to the ER during the pulse period; the
endoF product migrates slightly faster than the endoH product most
likely due to the ~1 kDa of mass contributed from the
N-acetyl glucosamine residues remaining after cleavage with
endoH but not with endoF.
In cells grown at 37 °C, WT tyrosinase was degraded with a half-time
of approximately 2.5 h, after an initial lag of about 1 h
(Fig. 2, A and B). It was also slowly converted
to an endoH-resistant form after a 1-h lag, concomitant with decreased
mobility and increased heterogeneity by SDS-PAGE, indicating that some
of the tyrosinase was exported from the ER before degradation. This was confirmed by the partial block in degradation of endoH-resistant tyrosinase by the addition of the lysosomotropic agents, MME or ammonium chloride, to the chase medium (Fig.
3A). The remainder of
tyrosinase was likely degraded in a pre-Golgi compartment (see below).
The overall degradation rate was reduced approximately 2-fold when
cells were grown at 31 °C, and the time-dependent increase in the fraction of endoH-resistant material was much more
dramatic, such that by 4 h, the majority of WT tyrosinase was
endoH-resistant. These data support a slow release of WT tyrosinase from the ER at 37 °C and transport to late endosomes and lysosomes, where it was ultimately degraded; the rate of ER exit was enhanced by
growth of cells at 31 °C, whereas the rate of degradation may be
reduced.
In contrast to WT tyrosinase, endoH-resistant R402Q tyrosinase was
almost never observed in cells grown at 37 °C (Fig. 2, A
and C). The intensity of the endoF-sensitive band is nearly identical to that of the endoH-sensitive band at all time points, suggesting that R402Q tyrosinase does not progress in the secretory pathway beyond the cis Golgi. Furthermore, the loss of
precipitable R402Q tyrosinase over time was largely insensitive to
lysosomotropic reagents (Fig. 3A), suggestive of
prelysosomal degradation. These data are consistent with the
localization of this variant to the ER as observed by IFM. On the other
hand, when cells were grown at 31 °C, a significant fraction of the
R402Q tyrosinase became endoH-resistant (Fig. 2, A and
C). This is less than the fraction of endoH-resistant WT
tyrosinase by 8 h of chase at 31 °C, but nevertheless a
dramatic increase relative to R402Q at 37 °C. Release of R402Q from
the ER at 31 °C and subsequent passage through the Golgi complex to
late endosomes and lysosomes, as evidenced by the degradation of the
endoH-resistant fraction (Fig. 2, A and B), is
consistent with the observed vesicular localization of this isoform by
IFM. The results support an inability of R402Q tyrosinase to exit the
ER at 37 °C rather than enhanced lysosomal degradation.
Lack of a Significant Enhancement of Proteasomal Degradation of the
R402Q Variant at the Restrictive Temperature--
The results thus far
imply that the R402Q mutant fails to exit the ER at the restrictive
temperature. ER retention is associated with incomplete or aberrant
folding and consequent recognition of misfolded polypeptides by the ER
quality control system (22, 23). Misfolded polypeptides also may serve
as substrates for rapid degradation by ER quality control, which is
thought to occur predominantly by reverse translocation to the cytosol
and proteolysis by the proteasome (24, 40). Tyrosinase has been shown
to be a substrate for this pathway in melanoma cells (41), and its degradation by this pathway is enhanced in some amelanotic melanoma cells (42). Thus, the apparent ER retention of R402Q tyrosinase at
37 °C may reflect enhanced proteasomal degradation.
To determine whether R402Q is degraded more rapidly than WT tyrosinase
by the proteasome, transfected HeLa cells grown at 31 °C or 37 °C
were treated for various times with the proteasome inhibitors MG132 or
lactacystin. Cells at each time point were harvested, and total cell
lysates were analyzed by Western blotting with antibodies to
tyrosinase. Treatment of cells expressing WT tyrosinase with MG132
resulted in the time-dependent formation of a band with
Mr ~55,000, which migrates slightly faster
than endoH-treated tyrosinase and is itself resistant to digestion with
endoH (Fig. 4A). An identical
band is detected using antibodies directed against either the lumenal
or the cytoplasmic domain of tyrosinase (Fig. 4, A and
B, and data not shown), suggesting that this band contains
the entire tyrosinase polypeptide and is not a product of proteolytic
degradation. The results are consistent with the stabilization of a
cytosolic intermediate that has been deglycosylated by a cytosolic
N-glycanase activity; similar proteasome inhibitor-dependent intermediates have been observed for
retrotranslocated major histocompatibility complex class I molecules
(43) and have been implicated for tyrosinase (41, 42).
Fig. 4B shows results of 10-h MG132 or lactacystin
treatments of cells expressing either WT or R402Q tyrosinase at
different temperatures. As expected, a similar ~55-kDa band appears
upon either MG132 or lactacystin treatment of cells expressing R402Q tyrosinase. Surprisingly, however, densitometric analysis indicates that this band does not accumulate at any greater rate from the R402Q
variant than from WT tyrosinase. Furthermore, decreased growth
temperature fails to reduce accumulation of this fragment, as would be
expected if the stabilization of R402Q tyrosinase at the permissive
temperature is due to a decrease in ER-associated proteasomal
degradation (Fig. 4B). Although these results support the
notion that some WT and R402Q tyrosinase is degraded by the proteasome,
they demonstrate that the R402Q variant is not degraded any more
rapidly than WT tyrosinase by this pathway.
The Lumenal Domain of the R402Q Variant Is Sufficient to Mediate
Temperature-sensitive ER Retention--
The position of the R402Q
polymorphism within tyrosinase implicated the lumenal domain of this
variant as responsible for the ts ER retention phenotype (5). To
confirm this and to determine whether other domains contribute to the
ts phenotype, we constructed chimeric proteins in which different
topologic domains of WT or R402Q tyrosinase were swapped with the
corresponding domains of a marker protein, Tac. Tac (the human
interleukin 2 receptor
TYT-HA, containing only the transmembrane domain of tyrosinase, was
expressed at the cell surface of transfected cells grown at either
31 °C or 37 °C (Fig. 5, i and j); this
staining was similar to the control, TTT-HA, containing intact Tac with
an HA11 epitope tag (data not shown; see Ref. 45). This shows that the
tyrosinase transmembrane domain contains no information for ER
retention. As expected, staining of cells transfected with YWTYT-HA (Fig. 5, a and b),
containing the lumenal and transmembrane domains of WT tyrosinase, or
YWTTT-HA (Fig. 5, e and f),
containing the lumenal domain only, fail to show extensive steady state
ER localization at either temperature. In contrast,
YTSYT-HA (Fig. 5, c and d) and
YTSTT-HA (Fig. 5, g and h), both
containing the lumenal domain of R402Q tyrosinase, are restricted to
the ER in transfected cells grown at 37 °C but not in cells grown at
31 °C. The phenotype of YTSTT-HA with the heterologous
Tac transmembrane and cytoplasmic domains shows that, within the
context of an integral membrane protein, the lumenal domain of R402Q
tyrosinase is sufficient for ts ER retention.
Curiously, neither YWTTT-HA nor YTSTT-HA are
delivered to the cell surface at 31 °C. Upon exiting the ER, these
proteins appear to accumulate in the region of the Golgi complex. We do
not believe that this is due to specific Golgi localization information
in either the lumenal domain of tyrosinase or the transmembrane domain of Tac, given that YWTYT-HA (Fig. 5, a and
b) and TTT-HA (data not shown) are both expressed at the
cell surface. We suspect that a spurious localization signal was
generated in our fusion protein, as has been previously observed in a
random fusion of two cell surface proteins (46). Importantly, however,
both YTT-HA chimeras express phenotypes comparable with those of the
parent tyrosinase molecule in terms of ER retention at each temperature.
ER Retention of the R402Q Variant Is Not Dependent on Tethering to
the Membrane--
ER quality control operates on both integral
membrane proteins and soluble proteins, but different mechanisms may
control each (40). To determine whether tethering to the membrane is either necessary for recognition of the R402Q variant as a substrate for ER quality control or influences the balance between retention and
degradation, we examined the fate of a soluble form of tyrosinase. The
transmembrane and cytoplasmic domains were deleted from both WT and
R402Q tyrosinase, and a polyhistidine tag was fused to the C terminus
of the lumenal domain to allow easy purification of the transgene
product. Tagged lumenal domains were expressed transiently in HeLa
cells. Given the apparent lack of post-ER targeting information in the
WT tyrosinase lumenal domain (see above), we expected these soluble
forms to be secreted soon after exit from the ER. Thus, both cell
lysates and supernatants from transfected cells grown at 31 °C or
37 °C were analyzed by Western blotting for the tyrosinase lumenal
domain. Samples were mock-treated or treated with endoH and endoF
before SDS-PAGE to facilitate analyses.
As shown in Fig. 6, only endoH-sensitive
forms of either soluble WT or R402Q tyrosinase accumulate in cell
lysates ("cell") from transfected cells grown at either 37 °C or
31 °C. This suggests that any material that progresses beyond the
cis Golgi is either rapidly degraded or secreted from the
cells. Supernatants ("sup") of cells grown at 37 °C contain a
small amount of soluble WT tyrosinase, amounting to less than 5% of
the total expressed material at steady state (see the Fig. 6 legend).
All of this material, however, is endoH-resistant, indicating proper
passage through the secretory pathway. In contrast, essentially no
material can be precipitated from supernatants of cells expressing
soluble R402Q tyrosinase grown at 37 °C. This indicates that
secretion of soluble R402Q is blocked at the restrictive temperature.
The amount of endoH-resistant, soluble WT tyrosinase is dramatically
increased in supernatants from cells grown at 31 °C, confirming the
stabilizing effect of reduced temperatures on even the WT protein.
Importantly, endoH-resistant, soluble R402Q is also recovered from
supernatants of cells grown at 31 °C. These results show that the
R402Q lumenal domain alone exhibits the ts ER export phenotype and that
tethering of the lumenal domain to the membrane is not necessary for
recognition by the ER quality control system. Furthermore, the results
confirm the partial ts phenotype of WT tyrosinase and suggest that the increased half-life of intact WT tyrosinase at 31 °C, observed in
the pulse-chase studies in Fig. 2, was largely due to enhanced ER exit
rather than (or in addition to) protection from post-Golgi degradation.
Finally, the results demonstrate that secretion of soluble tyrosinase,
WT or R402Q, is a relatively inefficient process, likely due to the
failure to export tyrosinase from the ER.
ER Retention Phenotype of the R402Q Variant Is
Irreversible--
The ts folding and ER retention phenotype of R402Q
tyrosinase is similar to that of several other ts glycoproteins. In
some cases, such as with the ts045 variant of the vesicular stomatitis virus glycoprotein, the ts phenotype is reversible such that misfolded polypeptides that accumulate at the restrictive temperature can be
rescued by a subsequent shift to the permissive temperature (47).
Rescue may be indicative of a partially folded intermediate that has
not entered a "dead-end" misfolded pathway. In other examples,
misfolded polypeptides become irreversibly trapped in an unfolded state
and cannot be rescued (20). The placement into one category or the
other may facilitate understanding of the manner in which misfolded
polypeptides are recognized and handled by the quality control
machinery of the ER.
To determine whether the R402Q variation imparted a reversible or
irreversible misfolding event, we took advantage of the ability to
capture fully folded, transport-competent lumenal domain by secretion
of the soluble form. HeLa cells transfected with either soluble WT or
soluble R402Q tyrosinase were grown at 37 °C for 48 h and then
incubated with CHX for 30 min to block further protein synthesis of new
tyrosinase molecules. Cells were then either maintained at 37 °C or
shifted to 31 °C, and the medium was replaced. CHX was maintained in
the medium to limit analyses to only those molecules that had
accumulated at the nonpermissive temperature before the temperature
shift. Cell lysates and supernatants were then assayed after 7-8 h for
the presence of soluble tyrosinase in the medium. Control cultures show
that easily detectable levels (5% of total in a parallel experiment)
of soluble R402Q tyrosinase are recovered in the medium when cells are
initially grown and then maintained at 31 °C during the chase (Fig.
7D, lanes 23-26). However, only trace amounts are detected in supernatants of cells that
are grown at 37 °C before the 31 °C chase (Fig. 7D,
lanes 19-22; 1% of total in a parallel experiment,
relative to 0.4% of total from cells maintained at 37 °C throughout
the experiment). Thus, soluble R402Q tyrosinase that initially misfolds
at 37 °C cannot be rescued by a subsequent chase at the permissive
temperature. Although the small amount of material detected in the
medium after the 31 °C chase may represent a fraction of soluble
R402Q tyrosinase that is capable of refolding, it more likely
represents material synthesized during the chase, since the low level
of CHX used, necessary to maintain viability, only blocked 80% of
protein synthesis (data not shown). In contrast to the R402Q variant,
soluble WT tyrosinase is recovered in the medium when the initial
cultures are maintained at 37 °C regardless of the chase
temperature; however, consistent with the pulse-chase analyses in Fig.
2, significantly more soluble WT tyrosinase is recovered when the chase
is performed at 31 °C (6% of total in a parallel experiment) than
at 37 °C (3.5% of total; Fig. 7B, compare lanes
5 and 6 with 9 and 10). This
indicates that WT tyrosinase, unlike the R402Q variant, does not
irreversibly misfold at 37 °C and can be rescued by a subsequent reduction in growth temperature.
ts allelic isoforms of tyrosinase are abundant throughout the
animal kingdom (2, 8, 9, 48, 49), but the molecular basis for their ts
phenotype has not been characterized. Our data demonstrate that the ts
enzymatic activities of the common R402Q allele of human tyrosinase
(10) are explained by nearly absolute and irreversible ER retention at
the restrictive temperature. Growth at 31 °C permits ER exit of at
least a fraction of newly synthesized tyrosinase and subsequent
transport to late endosomes or melanosomes. Ts ER retention is a
feature of other known ts protein variants in the mammalian secretory
pathway (15-19), and it is likely that other ts allelic forms of
tyrosinase share this phenotype. Indeed, ts ER retention of tyrosinase
has been observed in metastatic amelanotic melanoma cells (42); these
tumor cells may have either accumulated similar mutations during the
development of metastases or derived from donors expressing a ts
allelic form of tyrosinase. Taken together, our results imply that ER
quality control may be a central mechanism for governing variable
pigmentation and vision throughout the animal kingdom.
The mechanism underlying ER retention of tyrosinase at the restrictive
temperature is most likely a defect that prevents competent folding.
The quality control machinery of the ER functions to assure that
misfolded polypeptides are retained in the ER before ultimate
degradation (20, 23). Pathogenic ts mutants of the cystic fibrosis
transporter (16) and the Wilson's copper transporter (15), causative
agents in cystic fibrosis and Wilson's disease, respectively, are
similarly misfolded and retained in the ER at the restrictive
temperature but fold sufficiently to bypass ER quality control at
reduced temperatures. Non-mutant proteins that fold inefficiently, such
as the cystic fibrosis transporter (50) and peptide-free major
histocompatibility complex class I molecules (51), may also escape
quality control and be exported from the ER at reduced temperatures, as
we have shown here for WT tyrosinase. We have observed similar results
for endogenous tyrosinase expressed in a number of highly pigmented
melanoma cell lines,2
suggesting that this is an intrinsic property of human tyrosinase. We
suspect that WT tyrosinase enters a partially folded intermediate at
37 °C that can be stabilized at lower temperatures, because soluble
WT tyrosinase molecules that had accumulated at 37 °C could be
released and secreted by a subsequent shift to 31 °C. In contrast,
the R402Q variant could not be released under these conditions. Perhaps
the R402Q variation stabilizes or favors a nonproductive intermediate
that occurs normally for tyrosinase, eventually leading to entrapment
in a stable misfolded state (14). Stringent kinetic analyses of the
ability to rescue misfolded WT or R402Q tyrosinase at 31 °C and of
disulfide bond formation may help to test this model. Unfortunately,
its inability to be rescued by a post-synthetic reduction in
temperature makes R402Q tyrosinase untenable for use as a synchronous
marker of biosynthetic transport in the manner that the ts045 variant
of the vesicular stomatitus virus glycoprotein has been used (47).
Using Western blotting of cell lysates treated for increasing time
periods with specific inhibitors, both WT and R402Q isoforms of
tyrosinase were shown to be substrates for degradation by the proteasome. Protected fragments similar in size to deglycosylated full-length tyrosinase molecules accumulated in the presence of the
inhibitors. These results support earlier studies demonstrating proteasomal degradation of tyrosinase (41, 42). Despite the differences
between WT and R402Q in ER retention, there appeared to be little
difference in the rate of accumulation of proteasome-protected fragments. Indeed, the persistence of endoH-sensitive tyrosinase up to
4 h of chase indicates that the rate of tyrosinase degradation by
this pathway is slow, and thus, only a fraction of ER-retained WT or
R402Q tyrosinase is degraded by this pathway at any given time. These
results suggest that the ER quality control system distinguishes
between different misfolded states of tyrosinase, targeting some
molecules (perhaps those more severely misfolded) for rapid
retrotranslocation and proteasomal degradation while permitting others
(perhaps those with more subtle folding defects or partially folded
intermediates) to remain in the ER lumen. Our data suggest that similar
fractions of WT and R402Q tyrosinase achieve a state recognized as a
substrate for proteasomal degradation. The remaining molecules serve as
substrates for ER retention, giving the WT tyrosinase an opportunity to
properly fold and exit the ER. Eventually, all tyrosinase unable to
correctly fold is degraded by the proteasome and/or by additional
proteolytic systems.
Because the amino acid variation R402Q is positioned within the lumenal
domain, it was not surprising that membrane-tethered chimeric proteins
containing the R402Q tyrosinase lumenal domain displayed ts ER
retention. Perhaps more surprising was the finding that the lumenal
domain alone, expressed as a soluble fragment, was also ts for ER
retention. This suggests that the mechanisms that operate to retain
this variant within the ER are independent of the membrane association
of the substrate. Such flexibility poses an interesting conformational
problem, since membrane-bound tyrosinase is restrained to move only in
the plane of the membrane, whereas soluble tyrosinase should be free to
diffuse throughout the ER lumen once translation is completed. Thus,
either these proteins are recognized in a manner independent of
topological constraints, there are redundant mechanisms to effect ER
retention, or retention mechanisms initiate during protein
translocation while the soluble form is still tethered to the membrane.
Calnexin, an ER membrane-bound lectin-like chaperone protein, is a
major participant in ER retention of misfolded, unassembled, and
partially folded integral membrane and soluble polypeptides, (reviewed
in Ref. 23; see also Refs. 52 and 53) and likely contributes to ER
retention of membrane-tethered R402Q tyrosinase and of soluble tyrosinase during translation. Calnexin has been reported to be stably
associated with a large fraction of tyrosinase in melanocytes and
melanoma cells (42, 54, 55) and to be required for proper tyrosinase
folding in COS-7 cells (56).
WT tyrosinase that exits the ER in HeLa cells appears to be targeted
for degradation in late endosomes and lysosomes, as suggested by the
loss of endoH-resistant material during long chase times in pulse-chase
experiments, the sensitivity of this loss to ammonium chloride and MME,
and the localization of tyrosinase to late endosomes and lysosomes in
HeLa cells at steady state. By contrast, tyrosinase in cells of the
melanocyte lineage is reported to be highly stable (57-59). At least
two potential explanations may account for this discrepancy. First,
tyrosinase may be inappropriately targeted to a degradative compartment
in HeLa cells but not in pigmented melanocytic cells. This is supported
by the segregation of tyrosinase-positive compartments from the bulk of
lamp1-positive late endosomes and lysosomes in melanoma cells but not
in HeLa cells (data not shown and Ref. 60). Second, HeLa cells may lack
a stabilizing factor for tyrosinase in late endosomal compartments.
This is supported by the lower stability of murine tyrosinase in a
melanocyte cell line lacking expression of the tyrosinase-related
protein TRP1 relative to a melanocyte line from WT mice (57). Further
analyses of the expression of tyrosinase in pigmented versus
nonpigmented cells will be necessary to assess these two mechanisms.
Curiously, lysosomotropic reagents protected not only endoH-resistant
tyrosinase from degradation but also endoH-sensitive tyrosinase in a
pulse-chase experiment (see Fig. 3, A and B). This could potentially be explained by autophagic degradation of
aggregates of misfolded tyrosinase that had accumulated in regions of
the ER, such as "aggresomes" (61). Additional experiments would be
required to test this hypothesis and to determine whether this reflects
a physiological degradation pathway or is merely due to overexpression
of misfolded tyrosinase in transfected cells.
What do our results imply for the etiology and treatment of OCA1? There
are numerous missense mutations within the gene for tyrosinase that
result in OCA1, many of them clustering around the coding region for
the putative CuB copper binding site near residue 402. Given the
inefficient folding of WT tyrosinase and the further defect in folding
of the R402Q variant, it is likely that many of these mutations do not
affect enzyme activity per se but rather cause the protein
to be misfolded and retained and/or degraded in the ER. The accelerated
degradation of tyrosinase observed in amelanotic melanoma cells (42) is
likely due to a similar phenomenon in which these cells accumulated
mutations that further decrease the fidelity of tyrosinase folding. If
such speculation is validated, pharmacological intervention targeted toward enhancing productive folding of tyrosinase in the ER may provide
a common method to enhance pigmentation in OCA1 patients carrying
distinct mutations in tyrosinase. Further analysis of the effects of
enhanced chaperone expression, decreased cell temperature, or cell
treatment with stabilizing agents such as glycerol (50) on the ability
to export various mutants of tyrosinase would help to determine whether
our findings extend to other OCA1 mutants.
INTRODUCTION
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ABSTRACT
INTRODUCTION
EXPERIMENTAL PROCEDURES
RESULTS
DISCUSSION
REFERENCES
EXPERIMENTAL PROCEDURES
TOP
ABSTRACT
INTRODUCTION
EXPERIMENTAL PROCEDURES
RESULTS
DISCUSSION
REFERENCES
Pep7h, kindly provided by Dr. V. J. Hearing (National Cancer Institute, Bethesda, MD), is a rabbit
antiserum prepared against a keyhole limpet hemocyanin-conjugated
synthetic peptide (CPLLMEKEDYHSLYQSHL) corresponding to residues 513 to
529 of the human tyrosinase cytoplasmic domain (31). A second
preparation of Pep7h was generated in our laboratory and was
affinity-purified using SulfoLink beads coupled to the peptide
(Pierce). NY8K, kindly provided by Dr. L. Old (Ludwig Cancer Institute,
New York, NY), is a rabbit antiserum generated against recombinant
tyrosinase lumenal domain prepared from Escherichia coli
(32). Tac was recognized by the monoclonal antibody 7G7.B6 (ATCC,
Manassas, VA) or a polyclonal rabbit antiserum generated in our
laboratory (33). Monoclonal antibody 16D12 against the HA11 epitope was
purchased from Babco (Richmond, CA). Monoclonal antibody AF8 against
calnexin (34) was a kind gift of Dr. M. Brenner (Brigham and Women's
Hospital, Boston, MA). A polyclonal rabbit anti-calnexin serum (CT) was
obtained from Stressgen Biotechnologies (Victoria, BC, Canada). Normal
rabbit antiserum was produced in-house. Fluorescein isothiocyanate-, lissamine-rhodamine-, alkaline phosphatase-, and horseradish
peroxidase-conjugated secondary antibodies were purchased from Jackson
Immunoresearch (West Grove, PA).
70 °C. Immunoprecipitations
were performed essentially as described (29). Briefly, cells were
resuspended in lysis buffer containing 1% Triton X-100 and a panel of
protease inhibitors on ice for 30 min, then cleared of nuclei and cell
debris by centrifugation. Lysates were pre-cleared by incubation with
protein A-Sepharose beads (Amersham Pharmacia Biotech) and then
sequentially immunoprecipitated using protein A-Sepharose that had been
preadsorbed with 1 µl of normal rabbit serum followed by beads
preadsorbed with 1 µl of Pep7h anti-tyrosinase serum. Beads were
washed extensively with buffer containing 0.05% Triton X-100, once
with PBS, and then divided into 3 aliquots that were either protein
N-glycanase F (endoF, New England Biolabs, Beverly, MA)-,
endoglycosidase H (endoH, New England Biolabs)-, or mock-endoH-treated
according to the manufacturer's instructions. Proteins were eluted
from the beads with SDS sample buffer. Samples were fractionated by SDS-PAGE using gels containing 10% acrylamide. Dried gels were subjected to quantitative image analysis using a Molecular Dynamics Storm PhosphorImager and ImageQuant version 1.11 software.
-mercaptoethanol and heating to 95 °C for 10 min. The lysates
were treated with DNase I at 37 °C for 15 min, reheated to 95 °C
for 10 min, and then either enzymatically deglycosylated as above or
mock-treated.
Pep7h anti-tyrosinase serum diluted in
Blotto, and then washed with PBS, 0.2% Tween 20. In some experiments, the membranes were then developed using a horseradish peroxidase detection system, in which membranes were incubated with horseradish peroxidase-conjugated donkey anti-rabbit immunoglobulin in Blotto and
washed as above. Bound antibody was detected by ECL (Amersham Pharmacia
Biotech), exposure to Reflection Film (NEN Life Science Products), and
film processing using a Kodak M35A X-Omat processor. For quantitative
detection, membranes were developed using an alkaline phosphatase
detection system. Membranes were incubated with alkaline
phosphatase-conjugated goat anti-rabbit immunoglobulin in Blotto,
washed as above, developed using ECF (Amersham Pharmacia Biotech), and
detected and quantitated using a Molecular Dynamics Storm 860 PhosphorImager with ImageQuant version 1.11 software.
RESULTS
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ABSTRACT
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EXPERIMENTAL PROCEDURES
RESULTS
DISCUSSION
REFERENCES
View larger version (99K):
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Fig. 1.
Steady state localization of WT and R402Q
tyrosinase at permissive and nonpermissive temperatures. HeLa
cells transiently transfected with plasmids encoding WT (a
and b) or R402Q tyrosinase (c-f) were grown on
coverslips at 37 °C (a, c, e, and
f) or 31 °C (b and d) and then
fixed and processed for indirect intracellular IFM. Cells were stained
with Pep7h antityrosinase serum (a-e) and
lissamine-rhodamine-conjugated anti-rabbit Ig. In e and
f, cells were costained with AF8 (a monoclonal antibody to
calnexin) and fluorescein isothiocyanate-conjugated anti-mouse Ig
(f).
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Fig. 2.
Pulse-chase kinetics and endoglycosidase
susceptibility of WT and R402Q tyrosinase at permissive and
nonpermissive temperatures. A, WT and R402Q tyrosinase
were transiently transfected into HeLa cells. Two days
post-transfection, the cells were metabolically pulse-labeled with
[35S]Met/Cys at the indicated temperatures and then
chased for 1, 4, or 8 h. Cell lysates were sequentially
immunoprecipitated with normal rabbit serum (N) and then
Pep7h anti-tyrosinase serum. Samples were mock ()-, endoH
(H)-, or endoF (F)-treated (endo
tmt.), separated by SDS-PAGE, and visualized by PhosphorImager
analysis. Ab, antibody. Migration of molecular mass
standards (kDa) is indicated to the right. B, degradation of
tyrosinase was determined by quantitating the intensity of the band
corresponding to endoF-treated tyrosinase at each time point, and
expressing these values as a percent of those from the initial,
pulse-labeled tyrosinase. The data represent the average of three
experiments. C, acquisition of endoH resistance was
determined by subtracting the band intensities for endoH-sensitive
tyrosinase from those for the total (endoF-treated) tyrosinase at each
time point. The values are expressed as a percent of the total amount
of tyrosinase (endoF band intensity) at each time point. Shown is a
representative of three experiments.
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Fig. 3.
Degradation of WT, but not R402Q tyrosinase,
is sensitive to inhibitors of lysosomal function. A,
HeLa cells transiently transfected with DNA encoding WT (upper
panel) or R402Q (lower panel) tyrosinase were
metabolically pulse-labeled as in Fig. 2 and chased at 37 °C for 0 or 8 h, as indicated, in the absence ( ) or presence of 20 mM MME or 50 mM ammonium chloride
(NH4Cl), as indicated. Cell lysates were sequentially
immunoprecipitated with normal rabbit serum and then Pep7h
anti-tyrosinase serum; only the Pep7 h immunoprecipitates are shown.
Samples were mock ()-, endoH (H)-, or endoF
(F)-treated (endo tmt), separated by SDS-PAGE,
and visualized by PhosphorImager analysis. Migration of molecular mass
standards (kDa) is indicated to the right. Quantitation of the results
indicated that, relative to the chase with no inhibitor, 3.2-6.8-fold
and 3.9-5.5-fold more wild-type tyrosinase was precipitated after
chase with MME and ammonium chloride, respectively. In contrast, MME
and ammonium chloride resulted in a 1.3-2.1-fold and 0.9-fold change,
respectively, in precipitable R402Q tyrosinase relative to that
obtained with no inhibitor. B, as a control, the lysosomally
targeted chimeric protein, TT-lamp1 (TTL1) was
co-transfected with WT tyrosinase before pulse-chase analysis without
inhibitors () or with MME (M) or ammonium chloride
(N) as indicated above. Cell lysates were immunoprecipitated
with 7G7.B6 anti-Tac antibody, and immunoprecipitates were analyzed
directly by SDS-PAGE. Migration of molecular mass standards (kDa) is
indicated to the right.
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Fig. 4.
Both WT and R402Q tyrosinase serve as
substrates for degradation by the proteasome. A, HeLa
cells expressing WT tyrosinase were incubated in medium containing
0.2% dimethyl sulfoxide lacking (DMSO) or containing the
proteasome inhibitor, MG132, for 2 or 6 h as indicated. Cell
lysates were then either mock-treated ( ) or treated (+) with endoH as
described under "Experimental Procedures" and fractionated by
SDS-PAGE. Transferred blots were probed with Pep7h serum and
developed using ECL. B, HeLa cells were transiently
transfected with plasmids encoding WT or R402Q tyrosinase and then
grown at either 31 °C or 37 °C for 2 days, as indicated. Cells
were then incubated for 10 h at the same temperature with medium
alone (None) or with medium containing 0.2% dimethyl
sulfoxide (DMSO) alone or with MG132 or lactacystin
(Lact.), as indicated. At the end of the incubation, mock
() or endoH (+) treated lysates were fractionated and probed for
tyrosinase as described above. Migration of molecular mass standards
(kDa) is indicated to the right.
chain), like tyrosinase, is a type I
integral membrane glycoprotein. It is normally expressed at the cell
surface and is efficiently exported from the ER (44). We previously
showed that a chimeric protein with the lumenal and transmembrane
domains of Tac and the cytoplasmic domain of tyrosinase (TTY)
accumulated in late endosomes and lysosomes and not the ER (39); since
the cytoplasmic domains of WT and R402Q tyrosinase are identical, this
excludes the possibility that the cytoplasmic domain contains an ER
retention determinant. A series of chimeric proteins containing other
combinations of tyrosinase and Tac topological domains, tagged at the C
terminus with the HA11 epitope, was then constructed as outlined in
Fig. 5 (top). Chimeric
proteins were transiently expressed in HeLa cells, and localization was
assessed in cells grown at 37 °C or 31 °C by IFM. To enhance the
distinction between ER retention due to the ts defect versus
the WT protein, cells were pretreated for 2 h with CHX to block
protein synthesis, which results in clearance of WT tyrosinase from the
ER (39).
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Fig. 5.
The lumenal domain of R402Q tyrosinase is
sufficient to confer temperature-sensitive ER exit.
Top, schematic diagram of Tac/tyrosinase chimeric proteins.
The lumenal, transmembrane (TM), and cytoplasmic
(Cyt) domains of tyrosinase, Tac, and chimeric constructs
are represented schematically. Tyrosinase domains are represented in
gray, and Tac domains and the HA11 epitope tag (HA) are
represented in white. Names of the schematized proteins are
indicated to the left. Bottom, HeLa cells were transiently
transfected with the indicated chimeric proteins, incubated at the
indicated temperatures for 2 days, and treated with 50 µg/ml CHX for
2 h before fixation. Fixed cells were stained with a rabbit
anti-calnexin antiserum and with a monoclonal antibody to the HA11
epitope, followed by fluorescein isothiocyanate- and
lissamine-rhodamine-conjugated secondary antibodies; shown are only the
images obtained with the anti-HA11 antibody.
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Fig. 6.
Temperature-sensitive secretion of a soluble
form of the R402Q tyrosinase lumenal domain. Control pCDM8.1
plasmid (Vector; lanes 13-18) or plasmids
encoding polyhistidine-tagged, soluble forms of the WT (lanes
1-6) or R402Q (lanes 7-12) tyrosinase lumenal domain,
in which the transmembrane and cytoplasmic domains were deleted, were
transiently transfected into HeLa cells. Transfected cells were then
grown at the indicated temperature. Two days post-transfection, cells
and culture supernatants were harvested. Cell lysates (cell;
5% of total from the experiment; lanes 1-3,
7-9, and 13-15) or nickel-agarose-precipitated
culture supernatants (sup.; 33% of total from the
experiment; lanes 4-6, 10-12, and
16-18) were mock ( )-, endoH (H)-, or endoF
(F)-treated (endo tmt.) as indicated and then
separated by SDS-PAGE. Proteins were transferred to polyvinylidene
difluoride, probed with NY8K anti-tyrosinase serum, and detected by
ECL. Migration of molecular mass standards (kDa) is indicated to the
right.
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Fig. 7.
Temperature-sensitive misfolding of the R402Q
tyrosinase lumenal domain is irreversible. Polyhistidine-tagged,
soluble forms of the WT or R402Q tyrosinase lumenal domain, in which
the transmembrane and cytoplasmic domains were deleted, were
transiently transfected into HeLa cells. Cells were then grown at the
indicated temperature (initial temp.) for 2 days. Two days
post-transfection, the culture medium was replaced with medium
containing 10 µg/ml CHX. Cells were incubated for 30 min at the
initial temperature and then were either harvested (panels A
and C) or shifted to the final temperature (final
temp.) and grown for 7 h in fresh medium supplemented with
CHX, at which point both cells and culture supernatants were harvested
(panels B and D). Cell lysates (cell;
5% of total from the experiment) or nickel-agarose-precipitated
culture medium (sup.; 50% of total from the experiment)
were mock ( )-, or endoH (+)-treated and then separated by SDS-PAGE.
Proteins were transferred to polyvinylidene difluoride, probed with
NY8K anti-tyrosinase serum, and detected by ECL. Migration of molecular
mass standards (kDa) is indicated to the right.
DISCUSSION
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ABSTRACT
INTRODUCTION
EXPERIMENTAL PROCEDURES
RESULTS
DISCUSSION
REFERENCES
| |
ACKNOWLEDGEMENTS |
|---|
We thank Drs. Walter Storkus, Vincent Hearing, Thomas Tüting, Lloyd Old, Suzanne Topalian, and Jean Pieters for generous gifts of reagents.
| |
FOOTNOTES |
|---|
* This work was supported by American Cancer Society Grant RPG-BE-85115 and National Institutes of Health (NEI) Grant R01 EY 12207.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.
Partially supported by National Institutes of Health (NCI)
Training Grant T32 CA 09140.
§ Partially supported by National Institutes of Health (NEI) Training Grant T32 EY 07131.
¶ Partially supported by National Institutes of Health (NCI) Training Grant T32 CA 09671 and by National Research Service Award F32 AI 09946.
To whom correspondence should be addressed: Dept. of Pathology
and Laboratory Medicine, University of Pennsylvania School of Medicine,
277 John Morgan Bldg./6082, 36th and Hamilton Walk, Philadelphia, PA
19104-6082. Tel.: 215-898-3204; Fax: 215-573-4345; E-mail:
marksm@mail.med.upenn.edu.
2 D. W. Frank and J. F. Berson, unpublished information.
| |
ABBREVIATIONS |
|---|
The abbreviations used are: OCA1, oculocutaneous albinism type 1; CHX, cycloheximide; endoF, protein N-glycanase F; endoH, endoglycosidase H; ER, endoplasmic reticulum; IFM, immunofluorescence microscopy; MME, methionine methyl ester; WT, wild-type; ts, temperature-sensitive; HA, hemagglutinin; PBS, phosphate-buffered saline; PAGE, polyacrylamide gel electrophoresis.
| |
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EXPERIMENTAL PROCEDURES
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DISCUSSION
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