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J. Biol. Chem., Vol. 277, Issue 38, 35282-35288, September 20, 2002
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From the
Received for publication, November 9, 2001, and in revised form, June 3, 2002
The proteolytic processing of amyloid precursor
protein (APP) through the formation of membrane-bound C-terminal
fragments (CTFs) and of soluble The cytoplasmic region of the amyloid precursor protein
contains an NPXY motif, which is present in the cytodomains
of several tyrosine kinase receptors and in non-receptor tyrosine
kinase (1, 2). In tyrosine kinase receptors the tyrosine residue of
this motif is phosphorylated upon tyrosine kinase activation, and the
NPXpY motif (where pY is phosphotyrosine) functions as a
docking site for the phosphotyrosine-binding domain present in several
adaptor proteins interacting with tyrosine kinase receptors and
non-receptor tyrosine kinase, such as the proteins belonging to the Shc
family (3, 4). In APP1 and in
APP-related proteins APLP1 and APLP2 the NPTY motif interacts with
several adaptor proteins, such as Fe65 (5), X11 (6), mDab1 (7), and
JIP-1 (8), but this interaction has been demonstrated to be independent
of tyrosine phosphorylation (9, 10). Recent data (11) show that in
human brain CTFs can be tyrosine-phosphorylated and that in
vitro the APP cytodomain is tyrosine-phosphorylated by the
non-receptor tyrosine kinase Abl, which phosphorylates a tyrosine
residue upstream (Tyr-682), the NPTY motif (11, 12). This
phosphorylation generates a motif pYXXP that is recognized
by the SH2 domain of Abl itself and that might be a docking site for
SH2-containing adaptors such as Shc and Grb2 proteins (11). Here we
describe that in human brain tyrosine-phosphorylated CTFs represent
docking sites for Shc and Grb2 proteins and generate stable complexes
with these adaptors that are up-regulated in AD cases. ShcA formation
is strictly confined to activated astroglial cells only, and its levels
are highly enhanced in AD brains in comparison to control subjects. In
AD brains it is also up-regulated in the expression of Erk1,2 kinase,
likely as a consequence of ShcA activation. In vitro
experiments show that thrombin triggers the ShcA-CTFs interaction and
Erk phosphorylation in cultured astrocytes, whereas in neuronal cells these complexes are undetectable. Therefore, our data suggest an
involvement of APP in cell signaling through its CTFs and correlate APP
metabolism and ShcA to the reactive gliosis and inflammatory phenomena
that occur in AD.
Brain Samples Preparation and Western Blotting--
Cerebral
cortex was obtained at autopsy from clinically and neuropathologically
verified (according to the Consortium to Establish a Registry for
Alzheimer's Disease (CERAD)) (13) cases of sporadic AD
(n = 6, age 72 ± 7, postmortem interval, 5.2 ± 2.4 h), control subjects (n = 6, age 73 ± 9, postmortem interval, 4.7 ± 2 h) in which AD had been
excluded by clinical and autopsy examination, including
immunohistochemical analysis. Monoclonal antibodies 4G8 and 6E10,
specific for residues 17-21 and 6-10 of A Immunohistochemistry--
Immunohistochemistry was carried out
in formalin-fixed and paraffin-embedded brain specimens from frontal
cortex and hippocampus. Briefly, deparaffined sections were pretreated
in citrate buffer at pH 5 in a microwave and probed with the indicated
antisera. Development reaction was carried out with AP-labeled
secondary antibody visualized by fast red chromogen (Dako, Glostrup, Denmark).
Cell Culture--
Primary cultures of rat cortical neurons were
obtained from 18- to 20-day-old Sprague-Dawley embryos as published
previously (14). Briefly, cortices were excised, trypsinized, and
resuspended in Neurobasal medium supplemented with 2% B27
(Invitrogen), 0.5 mM glutamine, and antibiotics. Cells were
seeded in poly-L-lysine-coated wells, and after 8-9 days
the cell population was determined to be at least 95% neuronal by MAP2
immunostaining. Primary cultures of rat cortical type 1 astrocytes were
prepared from 2-day-old Sprague-Dawley pups. Cortices were dissected
out, trypsinized, and cells cultured in Dulbecco's modified Eagle's
medium supplemented with 10% fetal bovine serum and antibiotics.
Astrocyte-enriched cultures were obtained from mixed glial cultures by
the shaking off method and were composed of greater than 95% glial
fibrillary acidic protein-positive cells. Untreated and
thrombin-treated cells were lysed in a Hepes buffer containing 1%
Nonidet P-40 and 0.5% sodium deoxycholate, pH 7.4. After a 10-min
centrifugation at 1500 × g, cell lysates were either
cold methanol-precipitated, and the resulting pellets analyzed by
Western blotting after protein counting (Bio-Rad protein assay), or
immunoprecipitated and analyzed as described above.
Characterization of the Expression of Tyrosine-phosphorylated
CTFs and Shc in Human Brain--
We have described recently (11) the
presence in human brain of tyrosine-phosphorylated CTFs in both AD and
non-AD control subjects. Here we analyze the pattern of tyrosine
phosphorylation identified in APP and CTFs of AD and age-matched normal
brains. Brain extracts were immunoprecipitated with antibodies
recognizing the A
The tyrosine phosphorylation of APP, although very weak, and of CTFs
suggests that they can be involved in tyrosine
kinase-dependent signaling, by functioning as docking
molecules for phosphotyrosine-interacting proteins. Shc proteins
possess SH2 and phosphotyrosine-binding domains that may recognize the
pYENP or NPTpY motifs in the APP C terminus, respectively (3, 4).
Therefore, they likely represent candidates as interacting proteins
with the tyrosine-phosphorylated C terminus of APP. To examine this
point, we first analyzed brain extracts by Western blotting, looking at
the expression of ShcA and ShcC in AD and non-AD control subjects. The
results are summarized in Fig. 1c, where the levels of ShcA
proteins were analyzed in hippocampal and frontal cortex extracts. p46,
p52, and p66 ShcA isoforms were detected in normal and Alzheimer's
brains, but their levels were significantly increased in the latter.
Immunoblotting with anti-ShcC and anti-Grb2 antibodies showed also that
these proteins were expressed in human but without significant
difference between AD and control subjects (Fig. 1c). The
presence of ShcA in human senile brain contrasts with previous
observations (3, 23) that ShcA accumulates in rat fetal brains, whereas
ShcC is more abundant in rat adult brains as shown in Fig.
1c as control. This might due in part to the fact that in
our samples, cells from small meningeal vessels, which may contain
ShcA, likely were also present, but this also suggests that Shc
isoforms may undergo an aging-specific change of expression (3).
Moreover, our data are in agreement with previous observations
indicating that proliferating glia and injured cells may also express
abnormally high levels of ShcA (3, 23, 24).
Tyrosine-phosphorylated CTFs Interact with Shc-Grb2 Adaptors,
Enhanced CTFs-ShcA-Grb2 Complexes and ERK1,2 Activation in
AD--
To verify if APP or CTFs may interact with Shc proteins, we
immunoprecipitated protein extracts from Alzheimer's and normal brains
with anti-ShcA, anti-phosphotyrosine, and anti-Grb2 antibodies. Immunoprecipitated proteins were analyzed by Western
blotting, and immunodetection was carried out with the anti-APP
C-terminal antibody 643-695/Jonas. This experiment demonstrated that
tyrosine-phosphorylated CTFs migrating at 22, 16, and 12.5 kDa were
co-immunoprecipitated with ShcA protein, whereas neither full-length
APP nor ShcA Localization at Reactive Astrocytes Around Plaques, Enhanced
Expression in AD--
To identify the cellular localization of ShcA
signaling, we analyzed by immunohistochemistry hippocampal sections of
formalin-fixed and paraffin-embedded brain samples from control and AD
patients. The immunostaining demonstrated that ShcA signal is
significantly more intense in AD brain than in non-demented control
samples (Fig. 3, a and
b) and occurred mainly at perivascular astrocytes, white
matter astrocytes, and also at reactive astrocytes surrounding amyloid
plaques (Fig. 3, c and d). In normal brains ShcA
staining appeared very weak and when barely present was localized in
non-activated astrocytes as well (Fig. 3a). Under our
conditions, neurons remained unstained by anti-ShcA antibody both in AD
and in non-AD subjects. As hypothesized previously (3), in the adult
normal human brain ShcA is mainly expressed in astrocytes and may be
overexpressed under degenerative conditions where astrogliosis is
present or in glial brain tumors (3, 23). To ascertain the identity of
ShcA-positive cells as astrocytes, we probed adjacent slides from AD
subjects with anti-ShcA and anti-GFAP antibodies. Although astrocytes
are cells with a typically fine and flat morphology (4-6 µm thick)
and eventually difficult to detect in adjacent slides (5 µm thick),
in our conditions, activated astrocytes were heavily stained by
anti-ShcA antibody and were also labeled in the adjacent section by
anti-GFAP antibody (Fig. 3, e-h). Our data suggest that the
interaction between CTFs and ShcA, which may occur in glial cells, is
likely related to astrogliosis and to the reactive inflammatory
phenomena observed in AD (26), as also suggested by ERK activation
(Fig. 2f). The phosphorylation and interaction of
CTFs with Shc, besides AD, may occur in age-matched control brain as
well, although to a lesser extent. This could suggest that either
normal brain aging is accompanied by a certain degree of astrogliosis
or that in normal conditions a basal level of proliferative activity
through ShcA signaling exists.
Thrombin Triggers the CTF-ShcA Interaction in Cultured Rat
Astrocytes but Not in Neurons--
To investigate the conditions
whereby phosphorylated CTFs interact with Shc adaptor proteins, we have
carried out a series of experiments in vitro in primary
cultures of rat astrocytes and cortical neurons. These cells possess
high levels of APP, ShcA, and CTFs (Fig.
4a) with significant
differences in amount and electrophoretic pattern. The APP profile in
astrocytes showed an increased amount of Kunitz protease
inhibitor-containing isoforms and a lower amount of "neuronal"
APP695 isoform in comparison to neurons, as described previously (27)
(Fig. 4a, upper panel). ShcA expression was
enhanced in astrocyte cultures in comparison to neuronal cultures
treated with AraC, in order to minimize the glial component; this
overexpression is mainly concerned with p66 and p46 isoforms. The
electrophoretic profile of CTFs showed a higher amount of 16-, 22-, and
32-kDa migrating forms in astrocytes than in neurons and a relatively
more abundant presence of 8-12.5-kDa migrating CTFs in neurons than in
astrocytes (Fig. 4a).
In both cell types the immunoprecipitation with anti-ShcA antibody in
normal conditions was completely ineffective in co-immunoprecipitating APP or CTFs (Fig. 4b). It is well known that thrombin, a
major coagulant and inflammatory mediator, regulates cleavage and
secretion of APP as well as Shc phosphorylation through specific
protease-activated receptors, which are present in astrocytes (28-30).
Furthermore, thrombin is a well known ERK1,2 activator in astrocytes,
and it has been related to the inflammatory response in AD (31-33).
Brief (15 min) thrombin treatments do not significantly alter the total amount of APP holoproteins, Shc proteins, or CTFs (Fig. 4a).
Only in thrombin-treated astrocytes CTFs migrating at 12.5, 22, and 32 kDa were all co-immunoprecipitated by anti-ShcA antibody and detected
by 4G8 staining (Fig. 4b). CTFs co-immunoprecipitated by
ShcA antibody were also recognized by anti-phosphotyrosine staining
(Fig. 4b) as shown previously for CTFs detected in human brain. On the contrary, anti-ShcC antibody was ineffective in co-immunoprecipitating CTFs (data not shown). As shown above in human brain and also in cultured rat astrocytes, APP holoproteins were
not co-immunoprecipitated with ShcA and CTFs (Fig. 4b).
Similar results were obtained also when other glial-derived cells (C6) were used (data not shown). In primary cultures of post-mitotic rat
cortical neurons, the thrombin treatment was unable to induce the
formation of such complexes, and neither APP nor CTFs were co-immunoprecipitated by anti-ShcA antibody in control or in
thrombin-treated neurons (Fig. 4b), although both APP and
CTFs are abundantly represented in cell extracts (Fig. 4a).
Also in these cells, Our data show that a subset of CTFs interact with Shc and
Grb2 proteins, suggesting that they may transduce an intracellular signal through SH2 or phosphotyrosine-binding domain interacting adaptors. The effect of such interaction is likely linked to the activation of the MAPK pathway, as shown here in AD brain and in
thrombin-treated astrocytes as well. The enhanced level of ShcA protein
in Alzheimer's patients, the peculiar staining of activated astrocytes
around amyloid plaques, and the increased CTFs-ShcA interaction in AD
subjects altogether suggest that the activation of this pathway may
play a role in Alzheimer's disease. The fact that the levels of
tyrosine-phosphorylated APPs are weak and that only We thank Elena Cattaneo for helpful
discussions, Pierluigi Gambetti for providing tissues and antibodies
for APP, and Diane Kofskey for support in immunohistochemistry preparation.
*
This work was supported by Grants from PRIN-MIUR 2000, Telethon Grant E1144, Progetto Finalizzato Strategico MISAN 1999 (to G. S.), grants from PRIN-MIUR 2000 (to N. Z.), V Framework
Program Contract QLK6-1999-02238, European Union e "Progetto
Strategico Basi Biologiche delle Malattie Neurodegenerative" CNR (to
T. R.).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 should be addressed: Farmacologia e
Neuroscienze IST c/o Centro di Biotecnologie Avanzate, Largo R. Benzi
10, 16132 Genova, Italy. Tel.: 39-10-5737256; Fax: 39-10-5737257; E-mail: schettini@cba.unige.it.
Published, JBC Papers in Press, June 26, 2002, DOI 10.1074/jbc.M110785200
The abbreviations used are:
APP, amyloid
precursor protein;
CTFs, C-terminal fragments;
AD, Alzheimer's
disease;
MAPK, mitogen-activated protein kinase;
ERK, extracellular
signal-regulated kinase;
Tricine, N-[2-hydroxy-1,1-bis(hydroxymethyl)ethyl]glycine;
GFAP, glial fibrillary acidic protein;
A
Signal Transduction through Tyrosine-phosphorylated
C-terminal Fragments of Amyloid Precursor Protein via an Enhanced
Interaction with Shc/Grb2 Adaptor Proteins in Reactive Astrocytes of
Alzheimer's Disease Brain*
,,,,¶
Sezione di Farmacologia, Dipartimento di
Oncologia Biologia e Genetica, Università di Genova, e
Dipartimento di Farmacologia e Neuroscienze IST c/o Centro
di Biotecnologie Avanzate, Largo R. Benzi 10, 16132 Genova and
§ Dipartimento di Biochimica e Biotecnologie Mediche,
Università di Napoli Federico II, Via Sergio Pansini 5,
80131 Napoli, Italy
ABSTRACT
TOP
ABSTRACT
INTRODUCTION
EXPERIMENTAL PROCEDURES
RESULTS
DISCUSSION
REFERENCES
-amyloid peptides likely influences
the development of Alzheimer's disease (AD). We show that in human brain a subset of CTFs are tyrosine-phosphorylated and form stable complexes with the adaptor protein ShcA. Grb2 is also part of these
complexes, which are present in higher amounts in AD than in control
brains. ShcA immunoreactivity is also greatly enhanced in patients with
AD and occurs at reactive astrocytes surrounding cerebral vessels and
amyloid plaques. A higher amount of phospho-ERK1,2, likely as result of
the ShcA activation, is present in AD brains. In vitro
experiments show that the ShcA-CTFs interaction is strictly confined to
glial cells when treated with thrombin, which is a well known ShcA and
ERK1,2 activator and a regulator of APP cleavage. In untreated cells
ShcA does not interact with either APP or CTFs, although they are
normally generated. Altogether these data suggest that CTFs are
implicated in cell signaling via Shc transduction machinery, likely
influencing MAPK activity and glial reaction in AD patients.
INTRODUCTION
TOP
ABSTRACT
INTRODUCTION
EXPERIMENTAL PROCEDURES
RESULTS
DISCUSSION
REFERENCES
EXPERIMENTAL PROCEDURES
TOP
ABSTRACT
INTRODUCTION
EXPERIMENTAL PROCEDURES
RESULTS
DISCUSSION
REFERENCES
and CTFs, were
purchased from Signet Pathology Systems (Dedham, MA). The polyclonal
antibody F25608 (a gift from Dr. P. Gambetti, Case Western
Reserve University, Cleveland, OH) and the monoclonal antibody 643/695
Jonas (Roche Diagnostics) are specific for the C terminus of APP and
CTFs. The monoclonal antibody for the N terminus of APP mAb348 was
purchased from Chemicon (Temecula, CA). Monoclonal antibodies to
phosphotyrosine (pY-20), anti-ShcC, anti-Grb2, and anti-
-tubulin
were from Transduction Laboratories (Lexington, KY). The
phospho-ERK-specific antibody was from New England Biolabs (Beverly,
MA). Anti-ShcA antibodies were purchased from Upstate Biotechnology,
Inc. (Lake Placid, NY), and from Transduction Laboratories. All the
chemicals were from Sigma unless otherwise specified. Brain cortical
samples were homogenized in a Tris-buffered saline buffer supplemented
with 1% Triton X-100 and protease inhibitors (CompleteTM,
Roche Diagnostics) and spun down at 68,000 × g 30 min.
The supernatant was adjusted to pH 8, 0.5% sodium deoxycholate, and
after protein counting (Bradford method, Bio-Rad) an equal amount of
protein was immunoprecipitated with the antibodies indicated coupled to protein A-Sepharose. Protein A beads were then loaded and
electrophoresed by Tris-Tricine SDS-PAGE and electroblotted on
polyvinylidene difluoride membrane, and proteins were probed with
specific antibodies in Tris-buffered saline plus 0.02% Tween 20 with
5% low fat milk and detected by ECL (Amersham Biosciences AB).
RESULTS
TOP
ABSTRACT
INTRODUCTION
EXPERIMENTAL PROCEDURES
RESULTS
DISCUSSION
REFERENCES
region of APP or phosphotyrosine residues.
Immunoprecipitated proteins were then blotted with the anti-APP
C-terminal antibody 643-695/Jonas. APP holoproteins migrating at
96-110 kDa were immunoprecipitated by 4G8 antibody, whereas no
detectable APP was observed by immunoprecipitating brain extracts with
anti-Tyr(P) antibody (Fig.
1a). Only in prolonged exposures of overloaded samples is a weak signal detectable
corresponding to APP bands when immunoprecipitated with
antiphosphotyrosine antibody (data not shown), suggesting that in human
brain the levels of tyrosine-phosphorylated APP are low. On the
contrary, several low molecular mass bands, migrating at 22, 16, and at 12.5 kDa, were easily immunoprecipitated by both antibodies
(Fig. 1a). In particular, the 12.5-kDa migrating band,
previously identified as the -secretase product C99, was
immunoprecipitated by both antibodies, whereas other CTFs bands
migrating below 12.5 kDa and the -secretase products at 8 kDa
(15-17) were immunoprecipitated by 4G8 antibody but not by
anti-Tyr(P) (Fig. 1a). The identity of 12.5-kDa
migrating bands as -secretase-derived C99 is confirmed by 6E10
immunostaining of similarly immunoprecipitated brain extracts (Fig.
1b), where the antibody detects specifically only
-secretase-cleaved CTFs, in force of its selectivity for residues
6-10 of A (18). CTFs bands migrating at 16 and 22 kDa and
recognized by the anti-Tyr(P) antibody correspond to previously
identified APP fragments (19-22), which have been suggested to be
generated by a non--secretase cleavage. These data suggest that CTFs
derived from different proteolytic pathways undergo different metabolic
destiny and that those derived from -secretase cleavage are not
tyrosine-phosphorylated.
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Fig. 1.
Tyrosine phosphorylation of APP and
CTFs. a, in human brain samples both APP and a subset
of CTF polypeptides migrating at 22, 16, and 12.5 kDa are specifically
immunoprecipitated by an antibody for the A region of APP (4G8). A
subset of CTFs is also immunoprecipitated by an anti-phosphotyrosine
antibody (pY-20). Immunostaining with an anti-APP C-terminal antibody,
besides the above-mentioned bands, also shows other CTFs bands
migrating at around 10 and 8 kDa (-secretase products)
immunoprecipitated by the 4G8 antibody only. Tyrosine-phosphorylated
APP is almost undetectable, and a signal corresponding to APP was
obtained only after prolonged exposures (not shown). No significant
differences are present between AD and non-demented control tissues
(CO) in APP or CTF content. b, the identity of
12.5-kDa migrating bands as -secretase-derived CTFs is ascertained
by 6E10 immunostaining of immunoprecipitated peptides as in
a. 6E10 antibody recognizes only -secretase-derived CTFs
in both AD and control cases, whereas -derived CTFs, which were
previously precipitated by 4G8 antibody, remain undetectable. 6E10
specificity for -secretase APP fragments was confirmed also by
staining of two or three A bands normally present in AD brain
samples. c, Western blottings (WB) of brain
samples from frontal cortex (COFr) and hippocampus
(Hippoc) from Alzheimer, control, and cortical rat brain
homogenates are probed with anti-ShcA, anti-ShcC, anti-Grb2, and
anti--tubulin as control for the amount of protein loaded. A
significantly higher amount of ShcA was present in AD samples
versus controls. As control we analyzed rat brain extracts,
in which high ShcA levels in fetal and high ShcC levels in the adult
animals are present.
-secretase-derived CTFs (see also Fig. 1a) were
complexed with ShcA (Fig. 2a).
Conversely, immunoprecipitation of brain extracts with
anti-phosphotyrosine and Grb2 antibodies pull down ShcA as well as the
22-, 16-, and 12.5-kDa bands of CTFs. Interestingly, a higher amount of
ShcA and CTFs was co-immunoprecipitated in Alzheimer's than in control samples by anti-Grb2 antibody, in agreement with the observation that
ShcA levels are increased in AD brains and suggesting that in AD the
activation of the CTFs-ShcA-Grb2 transduction machinery is enhanced.
Only under prolonged exposure is a weak signal detectable corresponding
to APP bands when immunoprecipitated with anti-phosphotyrosine and
anti-Grb2 antibodies, suggesting that tyrosine-phosphorylated APP
may be involved in such complexes, although weakly (data not shown).
Samples immunoprecipitated with anti-ShcC antibody showed a strong CTFs
signal corresponding to the 22-kDa fragment and a weak signal at 16 kDa
only (data not shown) in both AD and control cases. The
immunoprecipitation of brain extracts with anti-phosphotyrosine and
anti-CTFs antibodies followed by immunoblotting with anti-ShcA or
anti-ShcC antisera showed that both ShcA (Fig. 2b) and ShcC (Fig. 2c) were co-immunoprecipitated by these antibodies. As
negative control we used antibodies for CD26 and for tau proteins which were unable to co-precipitate Shc adaptors (data not shown).
Considering that both ShcA and ShcC co-immunoprecipitated with CTFs, we
examined the presence of CTFs-Shc-Grb2 complexes by searching Grb2 in
the proteins co-immunoprecipitated by anti-ShcA and by anti-APP
antibodies. The 24-kDa migrating band identified by anti-Grb2
immunostaining was co-immunoprecipitated by anti-ShcA, anti-C-terminal
APP 643-695/Jonas, and by the 4G8 antibodies (Fig. 2d). To
ascertain the identity of 12.5-kDa migrating bands as
-secretase-derived CTFs, we probed brain samples immunoprecipitated
with 4G8 and Grb2 antibodies with the 6E10 antibody (Fig.
2e). 6E10 recognizes -secretase-derived CTFs precipitated
by both antibodies both in control and in AD subjects, although in AD
the amount of CTF pull-down by Grb2 is higher than in control (Fig.
2e). Altogether these data indicate that in human brain a
complex involving CTFs, ShcA, and Grb2 is present and that this complex
is more present in AD than in control brain extracts. To investigate
whether the activation of this pathway would lead to the activation of
MAPK (3, 25, 26) in AD, we looked at the phosphorylation status of
ERK1,2 proteins in human brain. A higher amount of phospho-ERK1 and -2 was detected in AD cases in comparison to control subjects as
demonstrated by Western blotting with anti-phospho-ERK1,2 antibody
(Fig. 2f).
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Fig. 2.
Co-immunoprecipitation of CTFs with ShcA in
human brain. a, brain extracts from AD and control
cases (CO) were immunoprecipitated with anti-ShcA,
anti-phosphotyrosine, and anti-Grb2 antibodies. Immunostaining of
electrophoresed proteins with antisera to APP, ShcA, and CTFs shows
that ShcA co-immunoprecipitates only with tyrosine-phosphorylated CTFs
that migrate at 22, 16, and 12.5 kDa and does not precipitate either
APP or -secretase-generated CTFs. Anti-Grb2 antibody
co-immunoprecipitates ShcA and CTFs (mainly the 22- and 16-kDa
fragments and more weakly the C99 at 12.5 kDa) in brain extracts from
control (CO) and AD cases. The amount of ShcA and CTFs
linked to Grb2 protein is higher in AD in comparison to control
subjects. b and c, conversely, brain extracts
from AD and control cases immunoprecipitated with anti-ShcA,
anti-phosphotyrosine, and 4G8 antibodies show the co-precipitation of
ShcA proteins (b) and ShcC (c). HepG2 cell line
and adult rat brain extracts are loaded as positive control for ShcA
and ShcC, respectively. d, brain extracts immunoprecipitated
with anti-ShcA, anti-APP C-terminal antibody, and 4G8 were examined for
the presence of Grb2 protein by immunoblotting. Grb2 is present as a
24-kDa migrating band in both AD and control cases (CO)
co-immunoprecipitated by both ShcA and anti-C-terminal APP antibodies.
The identity of 12.5-kDa migrating bands precipitated by Grb2 as
-secretase-derived CTFs is confirmed by 6E10 immunostaining of
immunoprecipitated peptides as in b. 6E10 antibody
recognizes only -secretase-derived CTFs in both AD and control cases
and a subset of A peptides only in AD extracts precipitated by 4G8.
CTFs and A peptides derived from -secretase cleavage remain
undetectable. f, Western blotting of brain extracts probed
for phospho-ERK1,2, unphosphorylated ERK1,2, and tubulin as protein
loading control. In AD samples an enhanced level of phospho-p42 and p44
is present in comparison to control (CO) both in frontal
cortex (lanes 1 and 2) and in hippocampus
(lanes 3 and 4).
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Fig. 3.
Immunohistochemical localization of
ShcA in adult human brain samples. Immunohistochemistry was
carried out in formalin-fixed and paraffin-embedded brain specimens
from frontal cortex and hippocampus. ShcA is barely detectable in
control samples (a, ×10 magnification), and only few glial
cells possess a weak positive staining. On the contrary in AD samples
ShcA antibody heavily stains activated astrocytes (b, ×10
magnification). In AD the ShcA staining is highly enhanced and
localized mainly in astrocytes around vessels and plaques (white
arrows in b and inset in b). ShcA
immunolocalization in reactive astrocytes cells around amyloid plaques
is shown in c where 4G8 staining identifies amyloid plaques
(black arrow) and in d where immunoprobing of an
adjacent slice with anti-ShcA antibody detects reactive glial cells
(black arrow) around the same plaque identified in
c (×20 magnification). e and f, ShcA
immunostaining co-localize with anti-GFAP staining in astrocytes
present in adjacent slides (the same shapes of arrows
identify the same cell in adjacent slides, ×20 magnification) from an
AD subject. Higher magnification (×40) of ShcA and GFAP staining in
adjacent slides from an AD case are shown. Three astrocytes
(a-c) are identified and are stained by both
antibodies.
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Fig. 4.
Tyrosine-phosphorylated CTFs interact with
ShcA proteins in thrombin-treated primary cultures of rat
astrocytes. a, Western blotting (60 µg of protein in
each lane) of neuronal and astroglial cell lysate shows basically no
differences in the expression of APP (upper panel), ShcA
(middle panel), and CTFs (lower panel) between
control (CO) and thrombin-treated cells for 15 min at the
concentration indicated. b, in thrombin-treated astrocytes
only is present the co-precipitation of ShcA together with a subset of
CTFs, which are stained by both 4G8 (left) and
anti-phosphotyrosine (right) antibodies. Thrombin treatment
in cultured neurons does not generate ShcA-CTFs or ShcA-APP
co-precipitation.
-secretase-derived CTFs were not
tyrosine-phosphorylated and were not bound by either ShcA or ShcC (Fig.
4, a and b). Thrombin treatment, as reported previously (31), activated ERK1,2 proteins with a peak of activation at
15-20 min (data not shown). These data therefore confirm that the
interaction between CTFs and ShcA is an event strictly associated with
astroglial cells when mitogenically stimulated in vitro and correlate the presence of such complexes to the gliosis present in AD brain.
DISCUSSION
TOP
ABSTRACT
INTRODUCTION
EXPERIMENTAL PROCEDURES
RESULTS
DISCUSSION
REFERENCES
-amyloid-bearing
CTFs are tyrosine-phosphorylated and linked to Shc suggests that
in vivo tyrosine phosphorylation and cleavage of APPs are
related events and that likely tyrosine phosphorylation renders APP a
suitable substrate for a non--secretase enzymatic cleavage. In fact,
-secretase-cleaved derivatives remain unphosphorylated at tyrosine
residues and do not interact with the Shc-Grb2 adaptors, both in human
brain and cultured cells (Figs. 1, 2, and 4). We must also remember
that CTFs are per se considered amyloidogenic, neurotoxic
when overexpressed in vitro and in vivo, and that
their expression is increased in Down's syndrome years before the
formation of plaques (11, 34, 35). In this study we provide evidence
that, besides their role as -amyloid precursors, CTFs may be
directly involved in intracellular signaling likely related to glial
activation. We cannot exclude that phosphorylated APP holoprotein might
be first bound by Shc adaptors and then cleaved to form CTFs. We have
described recently (12) that residue Tyr-682 of APP may be
phosphorylated upon activation of Abl kinase, forming a pYENP motif
that is recognized and bound by the SH2 domain of Abl itself. The same
motif seems involved in the binding with Shc proteins as suggested by a
recent study in vitro (36). Therefore, tyrosine
phosphorylation of APP might constitute a regulatory event for cleavage
of APP and interaction with its cytosolic adaptors. We cannot exclude
that also other phosphorylation sites described previously (37) on APP
(likely present also on CTFs) may also contribute to the regulation of
APP/CTFs-Shc interaction, although tyrosine phosphorylation at residue
682 seems pivotal for the interaction with Shc (12, 36). The fact that
thrombin may trigger the CTFs-ShcA interaction suggests that the
signaling activity through CTFs is tightly regulated and that a cascade
of events such as kinase(s) activation, APP/CTFs phosphorylation, and
Shc interaction is required. The increased ERK1,2 phosphorylation,
described here in AD and also present in thrombin-activated astrocytes,
suggests that ShcA activation is likely responsible for the induction
of a glial associated mitogenic pathway. ShcC, which is co-precipitated
with CTFs in human brain as reported (3), is expressed at very low
levels or virtually absent in cultured proliferating astrocytes, and in
the human adult brain is likely produced in neurons or in meningeal vessels with no significant differences between AD and control subjects
(Fig. 1c). At this point it is still unclear if APP and CTFs
participate to the same Shc-mediated signaling addressed to the MAPK
activation or if their role is linked to the activation of a different
intracellular signal, considering also that previous data describe
phosphorylated-APP as an integrin-like molecule involved in cell
motility and cell adhesion (38, 39) and that other adaptors and
cytosolic proteins meet at the C terminus of APP (1, 40)
(Fig. 5). This is the first
identification of a signaling activity involving APP in astrocytes that
to date have been merely considered as "reactive" cells to a
primary amyloidosis of neuronal origin (26). A pathogenic role of
thrombin in inflammation and AD has been proposed previously (30-33,
41) considering also that the central nervous system is exposed to
thrombin upon breakdown of the blood-brain barrier (26, 32, 41, 42).
This occurs in acute conditions such as head injury and stroke and may
also occur in chronic neurodegenerative diseases such as AD (32, 42). Thrombin, besides ShcA activation, is also involved in secretion,
proteolysis of APP in platelets, and in cell cultures (28, 29, 43) and,
as for the hemostatic enzyme factor Xa, may cleave APP generating
potentially amyloidogenic C-terminal fragments (28, 44). Finally, the
Kunitz protease inhibitor-containing isoform of APP/PN2, which is
mainly produced by astrocytes, is a potent inhibitor of factors IXa,
Xa, and XIa, which are involved in the formation of thrombin, itself
suggesting an autoregulatory mechanism (44, 45). Therefore, our data
correlate APP processing to glial proliferation and to the inflammatory
response typical of AD and suggest that the activation of a mitogenic
pathway through a CTFs-ShcA interaction by abnormally high levels of
thrombin, possibly due to a compromised blood brain barrier, may
trigger astrocyte reaction and possibly neurodegeneration.
View larger version (21K):
[in a new window]
Fig. 5.
Schematic hypothesis on proteins interacting
with the cytosolic domain of holoAPP and CTFs. Abl and ShcA
interact with the YENPTY region of APP and CTFs, upon phosphorylation
of Tyr residues on APP. Fe65, X11,
Dab1, and JIP-1 interact with APP independently
of the Tyr phosphorylation status. ShcA binding to CTFs occurs at the
YENPTY motif, likely upon Tyr-682 phosphorylation. The putative
signaling via CTFs-ShcA interaction may contribute to a mitogenic
stimulus through MAPK activation in glial cells.
ACKNOWLEDGEMENTS
FOOTNOTES
ABBREVIATIONS
, beta amyloid;
AP, alkaline phosphatase.
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ABSTRACT
INTRODUCTION
EXPERIMENTAL PROCEDURES
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