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Molecular and Cellular Biology, August 2000, p. 5712-5721, Vol. 20, No. 15
0270-7306/00/$04.00+0
Copyright © 2000, American Society for Microbiology. All rights reserved.
Effect of Phosphoinositide-Dependent Kinase 1 on
Protein Kinase B Translocation and Its Subsequent Activation
Nathalie
Filippa,1
Carol L.
Sable,1
Brian A.
Hemmings,2 and
Emmanuel
Van Obberghen1,*
INSERM U145, IFR 50, Faculté de
Médecine, 06107 Nice Cedex 2, France,1 and
Friedrich Miescher Institute, CH 4002 Basel,
Switzerland2
Received 2 August 1999/Returned for modification 23 September
1999/Accepted 17 April 2000
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ABSTRACT |
In this report we investigated the function of
phosphoinositide-dependent protein kinase 1 (PDK1) in protein kinase B
(PKB) activation and translocation to the cell surface. Wild-type and PDK1 mutants were transfected into HeLa cells, and their subcellular localization was analyzed. PDK1 was found to translocate to the plasma
membrane in response to insulin, and this process did not require a
functional catalytic activity, since a catalytically inactive kinase
mutant (Kd) of PDK1 was capable of translocating. The PDK1 presence at
the cell surface was shown to be linked to phospholipids and therefore
to serum-dependent phosphatidylinositol 3-kinase activity. Using
confocal microscopy in HeLa cells we found that PDK1 colocalizes with
PKB at the plasma membrane. Further, after cotransfection of PKB and a
PDK1 mutant (Mut) unable to translocate to the plasma membrane, PKB was
prevented from moving to the cell periphery after insulin stimulation.
In response to insulin, a PKB mutant with its PH domain deleted
(
PH-PKB) retained the ability to translocate to the plasma membrane
when coexpressed with PDK1. Finally, we found that PH-PKB was highly
active independent of insulin stimulation when cotransfected with PDK1
mutants defective in their PH domain. These findings suggest that PDK1
brings PKB to the plasma membrane upon exposure of cells to insulin and
that the PH domain of PDK1 acts as a negative regulator of its enzyme activity.
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INTRODUCTION |
Protein kinase B
(PKB), also
known as c-Akt or RAC (related to protein kinase A and C), is composed
of a N-terminal pleckstrin homology (PH) domain followed by a kinase
catalytic domain which shares homology with the A and C protein
kinases. Two other isoforms of PKB (termed PKB
and PKB
) have been
identified and are expressed in ovarian, pancreatic, and breast cancer
cells (10, 11). This serine/threonine kinase is rapidly
activated in response to stimulation of tyrosine kinase receptors such
as those for platelet-derived growth factor (PDGF), insulin, basic
fibroblast growth factor, and epidermal growth factor (9, 15,
18). PKB stimulation by insulin or growth factors is thought to
be dependent on phosphatidylinositol 3'-kinase (PI 3-kinase) for the
following reasons: (i) it is sensitive to pharmacological inhibitors of
PI 3-kinase (18), (ii) dominant-negative PI 3-kinase mutants block PKB activation (24), and (iii) constitutively active PI 3-kinase mutants stimulate PKB (9).
A model has been proposed to explain activation of PKB in response to
hormones and growth factors (2). According to this model,
stimulation of cell surface receptors leads to an increase in the level
of phosphatidylinositol-3,4,5-trisphosphate
(PtdIns-3,4,5-P3) and PtdIns-3,4-P2 via PI
3-kinase. Although it was initially reported that phospholipids could
directly activate PKB by interacting with its PH domain
(16), more recently it has been shown that this process most
likely fulfills other and/or additional functions. Indeed, it may
facilitate PKB localization to the plasma membrane. This view stems
from the observation that translocation of PKB has been observed in
response to interleukin-2 (1), peroxyvanadate (25), insulin-like growth factor 1 (7), and
insulin (17). Further, this movement is prevented by PI
3-kinase inhibitors and by deletion of the PKB PH domain
(21). In response to insulin or insulin-like growth factor
1, PKB is phosphorylated on Thr308 and
Ser473, phosphorylation on both of these residues being
required for full PKB activation. A PKB kinase has been purified from
muscle (5) and brain (23); it was cloned (3,
22) and found to phosphorylate PKB on Thr308
(5), PKB on Thr309, and PKB on
Thr305 (24). This 63-kDa monomeric enzyme was
named 3-phosphoinositide-dependent protein kinase 1 (PDK1),
since it requires PtdIns-3,4,5-P3- or PtdIns-3,4-P2-containing vesicles in order to phosphorylate
PKB in vitro (3, 22). PDK1 is composed of a C-terminal PH
domain and a catalytic domain similar to A, B, and C protein kinase. The fact that PDK1 possesses a PH domain that binds to phospholipids in
vitro (22) points to a possible role in plasma membrane
targeting and subsequent PKB activation. PDK1 in which
Arg474 to Ala has been mutated in the PH domain or a PDK1
with a deletion of its PH domain shows a loss of the ability to
localize at the plasma membrane (6). Whether PDK1 in fact
translocates in response to cell stimulation remains controversial.
Indeed, Anderson et al. (6) have shown that in PAE cells
PDK1 could move to the membrane in response to PDGF in a PI
3-kinase-dependent manner, while Currie et al. have found that in 293 overexpressing cells PDK1 is constitutively located at the plasma
membrane (13).
In our present work, we clarify the role of PDK1 in PKB activation and
translocation. Using confocal microscopy and subcellular fractionation,
we show that PDK1 moves to the plasma membrane in response to insulin.
Interestingly, it appears that PDK1 promotes PKB translocation and
subsequent activation. Finally, we provide evidence for the idea that
the PH domain of PDK1 functions as a negative regulator of PDK1
activity in intact cells.
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MATERIALS AND METHODS |
Antibodies.
The antibody to Akt1 N-19 is an
affinity-purified goat polyclonal antibody raised against a peptide
corresponding to amino acids 3 to 21 located at the amino terminus of
human Akt1 (Santa Cruz Biotechnology, Santa Cruz, Calif.). Monoclonal
(12CA5) antibody to hemagglutinin (HA) was generated against a peptide
(YPYDVPDYA) corresponding to the sequence of influenza virus HA and was
provided by BAbCO (Richmond, Calif.). The monoclonal antibody (9E10) to the Myc epitope was from Santa Cruz Biotechnology. Monoclonal antibodies to green fluorescent protein (GFP) were obtained from Clontech (Palo Alto, Calif.). The secondary Texas red-conjugated mouse
anti-sheep antibody (100-fold dilution) was provided by Amersham
(Little Chalfont, Buckinghamshire, United Kingdom). The phosphorus-specific Akt (Thr308) antibody is a polyclonal
antibody obtained from New England Biolabs (Beverly, Mass.). The
monoclonal antibody to PDK1 was from Transduction Laboratories
(Lexington, United Kingdom).
Materials.
Culture media and Geneticin were from Life
Technologies, Inc. (Gaithersburg, Md.). Reagents for sodium dodecyl
sulfate-polyacrylamide gel electrophoresis (SDS-PAGE) were purchased
from Bio-Rad (Richmond, Calif.). Enzymes for molecular biology assays
were from New England Biolabs. Unless stated otherwise, all chemicals
were from Sigma (St. Louis, Mo.). P81 phosphocellulose paper was
purchased from Whatman (Maidstone, United Kingdom). Insulin was a kind
gift from Novo-Nordisk (Copenhagen, Denmark). The Crosstide peptide was provided by Neosystem (Strasbourg, France). [-32P]ATP
was purchased from ICN (Orsay, France). The QuickChange site-directed
mutagenesis kit was from Stratagene (La Jolla, Calif.). All
oligonucleotides were from Life Technologies. The T7 sequencing kit was
from Pharmacia (Uppsala, Sweden), and plasmid purification kits were
from Qiagen (Courteb
uf, France).
DNA constructs and expression vectors.
HA-tagged PKB in the
mammalian expression vector pECE was from B. A. Hemmings (Basel,
Switzerland) and has been described previously (8).
Site-directed mutagenesis was performed with the QuickChange
mutagenesis kit from Stratagene. The GFP-PKB fusion protein was created
by cloning PKB into EcoRI and BamHI sites within
the pEGFP-C2 vector (Clontech). The Myc-tagged PDK1 constructs in the
mammalian expression vector pCDNA3 as well as the purified PH-PKB
and PDK1 proteins from baculovirus-infected Sf9 cells were kindly
supplied by P. T. Hawkins (Cambridge, United Kingdom) and have
been described previously (6). His-tagged PH-PDK1 was cloned
in the mammalian express vector pCDNA 3.1/HISC. Myc-tagged PH-PDK1
was cloned in the mammalian expression vector pCDNA 3.1/Myc-HisA.
Cell culture.
293 EBNA cells are human embryonic kidney
cells that constitutively express the EBNA-1 protein from Epstein-Barr
virus (Invitrogen, San Diego, Calif.). These cells were grown in
Dulbecco's modified Eagle's medium (DMEM) supplemented with 5%
(vol/vol) fetal calf serum and 500 µg of Geneticin per ml.
Exponentially growing cells were trypsinized, seeded at 1.25 × 105 cells/well in six-well tissue culture dishes (3.5-cm
diameter), and incubated for 3 days in 2 ml of growth medium. One
microgram of supercoiled DNA was mixed with 100 µl of 0.25 M
CaCl2 and 100 µl of 2× BES (buffered saline containing
50 mM N,N-bis-2-hydroxyethyl-2-aminoethane sulfonic acid [pH 6.95], 280 mM NaCl, and 1.5 mM
Na2HPO4). The mixture was incubated for 30 min
at room temperature before being added dropwise to the cells. After
incubation for 15 to 18 h at 35°C under 3% (vol/vol)
CO2, the cells were moved to an incubator at 37°C and 5%
(vol/vol) CO2 for 8 h before starvation in DMEM containing 0.2% (wt/vol) bovine serum albumin (BSA) for 14 h. Transfection protocols used for confocal microscopy experiments of HeLa
cells were essentially identical to these used with 293 EBNA cells with
the following exceptions. Cells were trypsinized and directly plated
onto sterile glass coverslips at 100,000 cells/well in six-well tissue
culture dishes. The next day, cells were transfected with 4 µg of
DNA/well by the calcium phosphate method. Two days after transfection,
cells were analyzed by confocal microscopy. COS-7 monkey kidney cells
were cultured in DMEM supplemented with 10% (vol/vol) fetal calf serum
and 500 µg of Geneticin per ml. They were placed in 100-ml-diameter
dishes at 106 cells/dish and incubated for 3 days in 10 ml
of growth medium.
Immunoprecipitation and in vitro PKB kinase assay.
After
stimulation with the reagents indicated above, 293 cell extracts were
prepared by lysing cells in a buffer containing 50 mM HEPES (pH 7.6),
150 mM NaCl, 10 mM EDTA, 10 mM
Na4P2O7, 2 mM sodium orthovanadate,
100 mM NaF, 0.5 mM phenylmethylsulfonyl fluoride (PMSF), 100 IU of
aprotinin per ml, 20 µM leupeptin, and 1% (vol/vol) Triton X-100 for
15 min at 4°C. The lysates were clarified by centrifugation at
15,000 × g for 15 min at 4°C, and PKB was
immunoprecipitated with an HA (12CA5) antibody coupled to protein
G-Sepharose. After washing of the immunocomplexes, kinase activity was
assayed using Crosstide (12) in a reaction mixture
containing 50 mM Tris, 10 mM MgCl2, 1 mM dithiothreitol, 5 µM ATP, 30 µM Crosstide, and 3.3 µCi of
[-32P]ATP per assay. The phosphorylation reaction was
allowed to proceed for 30 min at 30°C, and then was stopped by
spotting 40 µl onto Whatman P81 filter papers and immersion in 1%
(vol/vol) orthophosphoric acid. The papers were washed several times,
rinsed in ethanol, and air dried, and the radioactivity was determined
by Cerenkov counting. Background values obtained from a mixture lacking
cell lysate were subtracted from all values. For detecting association between PDK1 and PKB, immunoprecipitates were washed three times in 1×
phosphate-buffered saline (PBS)-1% NP-40 and twice in 10 mM Tris (pH
7.5)-100 mM NaCl-1 mM EDTA and then boiled in SDS sample buffer and
resolved by SDS-10% PAGE.
In vitro phosphorylation of PDK1 and PH-PKB.
Myc-PDK1
constructs were immunoprecipitated from 293 EBNA cells. Immunocomplexes
were extensively washed as previously described. Myc-PDK1-immunoprecipitated proteins as well as 1 µg of PDK1 purified from baculovirus-expressing Sf9 cells was added to a mixture containing 50 mM Tris, 10 mM MgCl2, 1 mM dithiothreitol, 5 µM ATP,
and 3.3 µCi of [-32P]ATP per assay and 1 µg of
PH-PKB purified from baculovirus-expressing Sf9 cells as a
substrate. The phosphorylation reaction was allowed to proceed for 20 min at 30°C and then was stopped by adding Laemmli buffer. Samples
were subjected to SDS-PAGE under reducing conditions. Proteins were
visualized by Coomassie blue staining, and autoradiography was performed.
Immunoblot analysis.
Samples were resolved by SDS-PAGE and
transferred to polyvinylidene difluoride membranes (Immobilon;
Millipore Corp.). Membranes were blocked for 30 min in a blocking
buffer containing 5% (wt/vol) BSA in TBS (10 mM Tris-HCl, 140 mM NaCl
[pH 7.4]) and then incubated for 1 h with the appropriate
antibody diluted 1,000-fold in the same buffer. The membranes were
washed extensively in TBS containing 1% (vol/vol) NP-40. Detection was
performed with horseradish peroxidase-conjugated anti-rabbit,
anti-mouse, or anti-goat antibody and enhanced-chemiluminescence reagents (Pierce, Bezons, France) according to the manufacturer's instructions.
Subcellular fractionation.
293 cells were washed and
collected in ice-cold hypotonic buffer containing 10 mM Tris (pH 7.5),
10 mM NaF, 1 mM EDTA, 2 mM sodium orthovanadate, 0.5 mM PMSF, and 20 µM leupeptin and lysed by 20 strokes in a 1-ml syringe. Nuclei were
removed by centrifugation for 10 min at 13,000 × g at
4°C. The P100 and S100 fractions were obtained by additional
centrifugation at 100,000 × g for 30 min at 4°C.
P100 fractions were resuspended in lysis buffer.
Fluorescent staining and confocal microscopy.
HeLa cells
transfected with GFP-PKB and/or Myc-tagged PDK1 constructs and grown on
coverslips were placed on ice and washed three times with ice-cold PBS
prior to fixation with 4% (vol/vol) paraformaldehyde for 30 min at
room temperature. Cells were then washed, treated with 50 mM ammonium
chloride, and rewashed. Staining of the membrane was accomplished by
incubating the cells in a humid chamber for 30 min with wheat germ
agglutinin (WGA)-rhodamine (10
7 M). PDK1 constructs were
visualized by incubating the cells for 1 h with a 9E10 monoclonal
antibody to Myc as a primary antibody followed by another 1-h
incubation with a Texas red-conjugated anti-mouse secondary antibody.
Coverslips were mounted onto slides with Mowiol (Calbiochem, La Jolla,
Calif.) and viewed using a Leica upright confocal microscope equipped
with a Leica 63× lens objective (numerical aperture, 1.0). The
molecules were excited with the 600 line of an argon-krypton laser and
imaged using a 488 (GFP)-, 600 (rhodamine)-, or 568 (Texas red)-nm
band-pass filter. Images were acquired with a scanning mode format of
512 by 512.
PI 3-kinase activity assays.
293 cells were washed twice
with a buffer containing containing 50 mM HEPES (pH 7.5), 150 mM NaCl,
100 mM EDTA, 10 mM Na4P2O7, and 2 mM sodium vanadate (NaVO4) and lysed in the same buffer containing 1% (vol/vol) NP-40, 20 mM leupeptin, 100 U of aprotinin per
ml, and 1 mM PMSF. Cell lysates were incubated with polyclonal antibodies to IRS-1 preadsorbed to protein G-Sepharose for 3 h at
4°C. Pellets were then washed twice in PBS, pH 7.4, containing 1%
(vol/vol) NP-40 and 0.2 mM NaVO4; twice in 100 mM Tris-HCl (pH 7.4) supplemented with 500 mM LiCl and 0.2 mM NaVO4;
and twice in 10 mM Tris-HCl (pH 7.4) containing 100 mM NaCl, 1 mM EDTA, and 0.2 mM NaVO4. Pellets were further resuspended in 40 mM
HEPES, pH 7.4, containing 20 mM MgCl2, and the kinase
reaction was initiated by the addition of phosphatidylinositol (0.2 mg/ml) and 75 µM [-32P]ATP (7,000 Ci/mol) and
performed for 20 min at room temperature. The reaction was stopped by
the addition of 4 M HCl, and the phosphoinositides were extracted with
a mixture of methanol and chloroform. Finally, phospholipids were
analyzed by thin-layer chromatography.
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RESULTS |
PDK1 catalytic activity is not required for its
insulin-induced translocation.
In response to PDGF, PDK1 has been
shown to move to the plasma membrane (6). However, more
recent studies have not supported this initial report. Indeed, PDK1 was
not found to translocate to the membrane in response to either PDGF or
insulin, while it is to a small extent constitutively present at the
membrane (13). In an attempt to clarify these contradictory
results, we transfected HeLa cells with expression vectors coding for a
63-kDa PDK1 tagged with a Myc epitope at its amino terminus. A PDK1
variant (Myr), modified by the addition of a
myristoylation-palmitoylation sequence to the amino-terminal end and
containing a Myc tag at the carboxy-terminal end, was used as a control
to show constitutive localization of PDK1 at the plasma membrane. A
third construct used consisted of a PDK1 catalytically inactive due to
K110 substitution to Q (designated Kd for kinase deficient). Cells were
transfected with these constructs and serum starved for 12 h prior
to stimulation with insulin. As shown in Fig.
1, in nonstimulated cells PDK1 is
partially located at the plasma membrane, but in response to insulin
there is an increased amount at the membrane. Myr-PDK1 was present for
the greater part at the plasma membrane either with or without insulin
treatment of the cells. Finally, we found that the kinase-deficient
PDK1 mutant retained its ability to translocate to the plasma membrane
in response to insulin. This indicates that the catalytic activity of
PDK1 is not required for the hormone-induced translocation process.
Taken together, our results confirm that PDK1 translocation to the
plasma membrane occurs in response to insulin similar to what we have
seen for PKB in the same cells (21).
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FIG. 1.
Effect of insulin on localization of PDK1 mutants. HeLa
cells were transfected with 4 µg of either wild-type (Wild),
myristoylated (Myr), or kinase dead (Kd) PDK1 as described in Materials
and Methods. Forty-eight hours later, HeLa cells were incubated for 5 min with buffer or insulin (106 M). Cells were washed and
fixed with paraformaldehyde (4%) prior to incubation with an antibody
to Myc followed by incubation with a Texas red-linked mouse antibody to
label PDK1 mutants. Slides were mounted and analyzed by confocal
microscopy. Images represent the center section of the x-y
plane.
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Expression of a kinase-deficient PDK1 mutant permits normal PKB
activation by insulin while basal PKB activity is reduced.
Since
catalytically inactive PDK1 still translocates to the plasma membrane
in response to insulin, we determined its effect on PKB activity. It
has been previously shown that PH-PKB can serve as an efficient in
vitro substrate for PDK1 even in the absence of phospholipids (4,
13, 20). First, we performed an in vitro kinase assay to confirm
that Kd-PDK1 had completely lost its ability to autophosphorylate and
to phosphorylate PH-PKB. As shown in Fig.
2A, although wild-type PDK1 (purified
from PDK1-expressing baculovirus-infected Sf9 cells or
immunoprecipitated from 293 cells) remains phosphorylated and able to
phosphorylate PH-PKB in vitro, the kinase-deficient PDK1 is
essentially not phosphorylated under basal conditions and is unable to
phosphorylate PH-PKB. Next, 293 cells were transfected with PKB and
the different PDK1 constructs. In response to insulin there was a
6.1-fold stimulation of PKB (Fig. 2B). When PDK1 was coexpressed in the
absence of insulin, there was a 5.1-fold stimulation of PKB. A similar
observation has been made by others (6) and was interpreted
to mean that PDK1 is a constitutively active kinase, the overexpression
of which leads to potentiation of PKB activity even in the absence of
insulin. This view is supported by the observation that coexpression of
Kd-PDK1 and PKB does not change basal PKB activity. Surprisingly, there
was no significant difference in insulin-induced PKB activation when
Kd-PDK1 is expressed compared to when wild-type PDK1 is expressed. Western blot analysis showed that the increase in PKB activity was not
due to enhanced protein levels. Experiments using an antibody to
phospho-Thr308 of PKB were also performed in transfected
HeLa cells (Fig. 2C). We see an increase in PKB Thr308
phosphorylation in response to insulin compared to basal conditions when PKB was transfected alone, and a higher phosphorylation under basal conditions when PKB is expressed jointly with PDK1. Together these observations confirm the results obtained in 293 cells. Further,
we found an increase in the level of PKB phosphorylation in response to
insulin when coexpressed with Kd-PDK1. This indicates that at least in
these two cell types Kd-PDK1 does not act as a dominant-negative
molecule on endogenous PDK1.
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FIG. 2.
Effect of kinase-dead PDK1 on PKB activation. (A)
Myc-PDK1 constructs (Wild and Kd) were expressed separately in 293 cells. Immunoprecipitates and PDK1 purified from baculovirus were
incubated with [-32P]ATP (20 min at 30°C) and
PH-PKB purified from baculovirus-expressing Sf9 cells. Samples were
subjected to SDS-10% PAGE under reducing conditions followed by
autoradiography. Arrows point to the positions of Myc-PDK1, PDK1, and
PH-PKB. Asterisks indicate proteins purified from
baculovirus-expressing Sf9 cells. (B) 293 cells were transfected with
wild-type PKB and, where indicated, with PDK1 constructs. Serum-starved
cells were incubated for 5 min in the absence (white bars) or presence
(black bars) of insulin (106 M). After incubation, cells
were lysed, PKB was immunoprecipitated, and its kinase activity was
determined using Crosstide as described in Materials and Methods. PKB
activity is expressed as fold stimulation compared to basal levels, and
the corresponding value is indicated above each column. Values shown
are representative of at least four independent experiments performed
in triplicate. The levels of the expressed enzymes measured by
immunoblotting are shown below the bar graph. (C) HeLa cells were
transfected with wild-type PKB and, where indicated, with PDK1
constructs. Serum-starved cells were incubated for 5 min with buffer
(B) or insulin (I). After incubation, cells were lysed and 50 µg of
the lysates was subjected to SDS-PAGE. PKB phosphorylation was
determined by immunoblot analysis with an antibody specifically
recognizing phospho-Thr308.
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PDK1 subcellular localization and PKB basal activity depend on
IRS-1-associated PI 3-kinase activity.
We have shown in Fig. 1
that without insulin stimulation a small fraction of PDK1 was found
close to the cell membrane. This localization could explain the basal
PKB activity (5.1-fold stimulation) seen after PDK1 coexpression. To
further test this hypothesis, we serum starved cells in 0.1% (wt/vol)
BSA instead of 0.2% (wt/vol) BSA and for 24 h instead of 12 h. Then confocal microscopy was performed on PDK1-transfected cells in
the absence of insulin stimulation. As can be seen in Fig.
3A, when cells are serum starved in the
presence of 0.2% (wt/vol) BSA, PDK1 is found at the plasma membrane.
However, after a longer serum starvation period in 0.1% (wt/vol) BSA,
PDK1 was no longer found to be cell membrane associated. This
disappearance of plasma membrane association of PDK1 seen in 0.1%
(wt/vol) BSA-treated cells is accompanied by a loss in basal PKB
stimulation compared to results seen in Fig. 2, with "basal" being
defined as prior to addition of growth factors or hormones (Fig. 3B).
However, this treatment did not modify the effect of insulin, since a
20-fold stimulation of PKB activity is maintained when PKB and PDK1 are
coexpressed. Upon coexpression of Kd-PDK1, no significant decrease in
PKB activity was observed (0.8-fold stimulation) in the absence of
insulin, and a normal level of activation following insulin stimulation
(20-fold) is found. To determine whether the reduction in membrane
association of PDK1 was linked to the basal level of phospholipids, we
measured PI 3-kinase activity associated with IRS-1 immunopurified from 293 cells cultured in different BSA concentrations. We observed a
decrease in the estimated PI 3P production in the presence of 0.1%
(wt/vol) BSA compared to 0.2% (wt/vol) BSA (Fig. 3C). However, with
insulin no significant difference is seen in PI 3P production. This
decrease in IRS-1-associated PI 3-kinase activity observed with 0.1%
(wt/vol) BSA compared to that found with 0.2% (wt/vol) BSA could
explain both the basal localization of PDK1 to the cell surface and the
PKB activity observed with PDK1 cotransfected compared to PKB
transfected alone. According to our hypothesis, 24-h starvation reduces
the basal PI 3-kinase activity compared to a 12-h-long treatment. If
this view is correct, fewer PKB molecules should be phosphorylated on
Thr308 after 24 h of serum starvation. To check this,
we transfected HeLa cells with PKB either alone or together with PDK1
as described in the legend to Fig. 3D. When PKB activity was monitored
using the phospho-Thr308 antibody, we saw a clear reduction
in basal PKB phosphorylation after depletion in 0.1% BSA for 24 h
compared to a 0.2% BSA treatment for 12 h. This was also the case
for PKB cotransfected with PDK1, which correlated with the results
obtained with 293 cells in Fig. 3B. Finally, to further illustrate the
involvement of phospholipids in PDK1 activation, we transfected 293 cells with constitutively active Myr-PKB. This PKB mutant has been
reported to be attached to the cell membrane and to be highly active in
the absence of growth factor stimulation. After a 24-h starvation in
0.1% BSA, Myr-PKB was 40% less active than after serum depletion for
12 h in 0.2% BSA (Fig. 3E). Further, after cotransfecting a
dominant-negative form of PI 3-kinase (p85), we saw a decrease
in basal PKB activation in the absence of insulin stimulation and, as
expected, a decrease after insulin stimulation, similar to previous
reports (9).
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FIG. 3.
Role of phospholipids in PDK1 localization and PKB basal
activation. (A) Wild-type PDK1 (Wild) was expressed in HeLa cells and
after 24 h, cells were serum starved with either 0.2% (wt/vol)
BSA for 12 h or 0.1% (wt/vol) BSA in DMEM for 24 h. Cells
were washed and fixed with paraformaldehyde (4%) prior to incubation
with an antibody to Myc followed by incubation with a Texas red-linked
mouse antibody to label PDK1. Slides were mounted and analyzed by
confocal microscopy. Images represent the center section of the
x-y plane. (B) 293 cells were transfected with wild-type PKB
and PDK1 mutants. Cells were serum starved with 0.1% (wt/vol) BSA and
incubated for 5 min in buffer (white bars) or insulin
(106 M) (black bars). Then, PKB activity was determined
as described in Materials and Methods. PKB activity is expressed as
fold stimulation compared to basal levels, and the corresponding value
is indicated above each column. Values shown are representative of
three independent experiments performed in triplicate. The levels of
the expressed enzymes measured by immunoblotting are shown below the
bar graph. (C) 293 cells were serum starved in either 0.2% (wt/vol) or
0.1% (wt/vol) BSA for 24 h prior to exposure for 5 min to insulin
(I) (106 M) or to buffer. Total cellular protein lysates
were subjected to immunoprecipitation with an antibody to IRS-1, and
associated PI 3-kinase activity was measured with PtdIns or PtdIns-4-P
plus PtdIns-4,5-P2 as substrates. The position of
32P-labeled Pi (PIP) is indicated.
Radioactivity associated with each spot was quantified using
phosphorimaging and is indicated below the autoradiograph. (D) HeLa
cells were transfected with wild-type PKB and where indicated with PDK1
constructs. Cells were serum starved with either 0.2% (wt/vol) BSA for
12 h or 0.1% (wt/vol) BSA for 24 h and incubated for 5 min with buffer
or insulin (I). After incubation, cells were lysed and 50 µg of the
lysates was subjected to SDS-PAGE. PKB phosphorylation was revealed by
immunoblotting with an antibody specific for phospho-Thr308
peptide. (E) 293 cells were transfected with Myr-PKB or wild-type PKB
and, where indicated, with p85. Cells were serum starved and lysed,
PKB was immunoprecipitated, and its activity was determined as
described in Materials and Methods.
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PDK1 affects PKB subcellular localization.
HeLa cells were
transfected with plasmids coding for GFP-PKB and different Myc-tagged
PDK1 constructs. As previously described, cells expressing GFP-PKB
exhibit both cytosolic staining and a labeled nucleus, whereas
following insulin stimulation a clear cell membrane staining appears,
reflecting PKB translocation (14). To test the hypothesis
that PDK1 could modify PKB movement, HeLa cells were cotransfected with
PKB and various PDK1 mutants. In the presence of myristoylated PDK1
(Myr), PKB clearly localized to the plasma membrane, which was
visualized as a yellow ring due to the colocalization of green GFP-PKB
(PKB) and red myrPDK1 (Myr) (Fig. 4A).
Next, we used a PDK1 mutant which lacks the ability to translocate to
the plasma membrane due to the replacement of arginine 474 by alanine
(Mut) (6). When GFP-PKB and this translocation-deficient PDK1 mutant were cotransfected, no membrane localization of PKB was
seen after insulin stimulation. We determined then the effect of
Myr-PDK1 on PKB activity after their cotransfection in HeLa cells. As
shown in Fig. 4B the activity of PKB obtained from cells transfected
with Myr-PDK1 is higher than that seen in cells transfected with PDK1
under basal conditions (14.4-fold in the case of Myr-PDK1 compared to
2.2-fold stimulation in the case of PDK1). Further, no increase in PKB
activity compared to basal levels is seen upon insulin stimulation when
cells are cotransfected with Myr-PDK1 (14.2-fold stimulation). In
contrast, when wild-type PDK1 is transfected into cells, increased
basal PKB activity is observed (2.2-fold stimulation) as well as an
increased response to insulin compared to the control (8-fold
stimulation). This is expected since Myr-PDK1, which is constitutively
present at the plasma membrane, will of course not translocate upon
insulin stimulation. To see whether PDK1-induced PKB plasma membrane
localization can account for the increased PKB activity, we performed
fractionation studies in transfected 293 cells and COS cells. PKB
activity was monitored using the phospho-Thr308 antibody.
Upon coexpression of PDK1 and PKB in 293 cells, PKB activity in the
particulate fraction was higher under basal conditions (Fig. 4C). Upon
insulin stimulation, we saw an increase in PKB phosphorylation when 293 cells were cotransfected with PDK1 compared to PKB activity when the
cells were transfected with PKB alone. Next, we looked at endogenous
PKB and PDK1 localization in COS cells, which we previously found to
express measurable levels of endogenous PKB (14).
Fractionation studies showed that upon insulin stimulation the
occurrence of PKB and its phospho-Thr308 form are increased
in the particulate fraction (Fig. 4D). However, most of the
phospho-Thr308 PKB was seen in the cytosolic fraction. For
endogenous PDK1 as for PKB, we found an increased occurrence in the
particulate fraction with insulin stimulation. However, as for PKB,
most of the protein was localized in the cytosolic fraction (data not
shown).
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FIG. 4.
Effect of PDK1 mutants on PKB subcellular localization
and activation. (A) GFP-PKB was coexpressed in HeLa cells together with
wild-type PDK1 (Wild), myristoylated PDK1 (Myr), or PDK1 point
mutated in its PH domain (Mut). Forty-eight hours later, HeLa cells
were exposed for 5 min to buffer or to insulin (106 M),
washed, and fixed with paraformaldehyde (4%) prior to incubation
with an antibody to Myc, followed by an incubation with a Texas
red-linked mouse antibody to label PDK1 constructs. Slides were mounted
and analyzed by confocal microscopy. Images represent the center
section of the x-y plane. (B) HeLa cells were transfected
with wild-type PKB and wild-type PDK1 (Wild) or Myr-PDK1 (Myr). Cells
were serum starved in 0.2% (wt/vol) BSA and incubated for 5 min in the
presence (black bars) or absence (white bars) of insulin
(106 M). Then, PKB activity was determined as described
in Materials and Methods. PKB activity is expressed as fold stimulation
compared to buffer conditions, and the corresponding value is indicated
above each column. Values shown are representative of at least three
independent experiments performed in triplicate. The levels of the
expressed enzymes measured by immunoblotting are shown below the bar
graph. (C) 293 cells were transfected with HA-PKB or both Myc-PDK1 and
HA-PKB. The cytosolic (S100) and particulate (P100) fractions were
prepared as described in Materials and Methods. The PKB phosphorylation
state was revealed by immunoblotting with an antibody specific for
phospho-Thr308 peptide. (D) COS-7 cells were serum starved
in 0.2% (wt/vol) BSA and incubated for 5 min with insulin (I)
(106 M) or buffer (B). Then, cytosolic (S100) and
particulate (P100) fractions were prepared as described in Materials
and Methods. PKB was immunoprecipitated (IP) from 500 µg of the
cytosolic or particulate fraction, and changes in PKB and PDK1
distributions were detected by immunoblotting (IB) with antibodies to
PKB or PDK1. PKB phosphorylation was revealed by immunoblotting with an
antibody specific for phospho-Thr308 peptide.
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|
In response to insulin, PDK1 promotes PH-PKB translocation to
the plasma membrane.
To further investigate the effect of PDK1 on
PKB movement, we transfected HeLa cells with a PKB mutant devoid of its
PH domain (PH-PKB). We showed earlier that this construct was not
capable of translocating to the plasma membrane in response to insulin (Fig. 5A) (21). When
GFP-PH-PKB is coexpressed with Myr-PDK1, the cells show the
following features: (i) red staining around their cell membranes,
corresponding to Myr-PDK1; (ii) green staining in the cytosol,
corresponding to GFP-PH-PKB; and (iii) yellow staining just under
the plasma membrane, corresponding to colocalization of PH-PKB and
Myr-PDK1. The third colocalization is visible without or with insulin
treatment. Taken together, these results support the idea that PDK1
translocates jointly with PKB but more importantly support the idea
that PDK1 brings PKB to the cell surface. To ascertain that the yellow
ring was not an artifact due to protein overexpression, we
performed a negative control experiment for colocalization by staining
the membrane in red (WGA-rhodamine) and transfecting green PH-PKB.
The absence of a yellow ring in the insert of Fig. 5B illustrates that
after insulin stimulation PH-PKB is not found around the cell
membrane. Next we looked at PH-PKB activity in the presence of the
wild type or Myr-PDK1. The activity of PH-PKB was found to be much
higher in the presence of Myr-PDK1 than in the presence of wild-type
PDK1, even without insulin stimulation (Fig. 5B). This result is in
agreement with what we have shown in Fig. 4B, i.e., that PKB basal
activity in the presence of Myr-PDK1 is higher than that seen in
cells transfected with PDK1. As PH-PKB is more active when
cotransfected with Mut-PDK1 (Fig. 6B), we thought that the interaction
between those two proteins could be sufficiently strong to allow
its detection. Indeed, as seen in Fig. 5C, Mut-PDK1
coimmunoprecipitates with PH-PKB. In contrast, we have been unable
to visualize coimmunoprecipitation between wild-type PKB and the PDK1
mutants (data not shown).
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FIG. 5.
Effect of PDK1 mutants on PH-PKB subcellular
localization and activation. (A) GFP-PH-PKB was coexpressed in HeLa
cells together with wild-type PDK1 (Wild), myristoylated PDK1 (Myr), or
PDK1 point mutated in its PH domain (Mut). Forty-eight hours later,
HeLa cells were exposed for 5 min to buffer or to insulin
(106 M), washed, and fixed with paraformaldehyde (4%)
prior to incubation with an antibody to Myc, which was followed by an
incubation with a Texas red-linked mouse antibody to label PDK1
constructs. Slides were mounted and analyzed by confocal microscopy.
Images represent the center section of the x-y plane. (B)
293 cells were transfected with PH-PKB and wild-type PDK1 (Wild) or
Myr-PDK1 (Myr). Cells were serum starved in 0.2% (wt/vol) BSA and
incubated for 5 min in the presence (black bars) or absence (white
bars) of insulin (106 M). Then, PKB activity was
determined as described in Materials and Methods. PKB activity is
expressed as fold stimulation compared to buffer conditions, and the
corresponding value is indicated above each column. Values shown are
representative of at least three independent experiments performed in
triplicate. HeLa cells were transfected with 8 µg of PH-PKB
construct as described in Materials and Methods. Forty-eight hours
later, cells were stimulated for 5 min with insulin (106
M). Cells were washed and fixed with paraformaldehyde (4%) prior to
incubation with WGA-rhodamine (red) to label the plasma membrane.
Slides were mounted and analyzed by confocal microscopy. Images
represent the center section of the x-y plane. Membrane
staining is in red, and GFP is in green. Areas of colocalization appear
as yellow. The levels of the expressed enzymes measured by
immunoblotting are shown below the bar graph. (C) 293 cells were
transfected with PH-PKB with or without Mut-PDK1. Anti-HA
(PH-PKB) immunoprecipitates were resolved by SDS-PAGE followed by
Myc (Mut-PDK1) immunoblotting. Whole-cell lysates (100 µg) were
resolved; Mut-PDK1 and PH-PKB expression are detected using the Myc
and HA antibodies, respectively.
|
|
PDK1 activity is negatively regulated by its PH domain.
Next,
we examined the role of the PDK1 PH domain in PKB activation. It has
been shown by Anderson et al. (6) that a point mutation in
the PH domain (R474A) of PDK1 (Mut) results in a loss of its ability to
localize to the plasma membrane. A similar phenomenon has been found
for PKB since the PKB-PH R25C mutant has lost both its ability to
move to the cell surface and most of its activity. Further, as for PKB,
a PDK1 with its PH domain deleted fails to localize to the cell surface
(data not shown). The ability of PH-PDK1 and Mut-PDK1 to
induce PKB activation was tested (Fig. 6A).
Stimulation of PKB activity is seen after coexpression of either
Mut-PDK1 (4.6-fold) or PH-PDK1 (2.8-fold) even in the absence
of insulin. This is not significantly different from the stimulation seen upon cotransfection of the wild-type PDK1 construct (5.1-fold stimulation). In contrast, insulin-stimulated PKB activity is
significantly diminished upon coexpression of the PDK1 PH domain mutants. This reduced stimulation was not surprising, since PDK1 cannot
translocate to the cell surface, and consequently PKB will not either.
Note that the activity seen was comparable to that found with PKB
transfected alone. This reflects very likely the action of endogenous
PDK1, which can bring PKB to the cell surface, leading to its
phosphorylation on Thr308 and on Ser474 by
PDK2 activity. In this case basal activity can be linked to a small
quantity of PDK1 going to the membrane, as seen for the wild-type PDK1
construct in 0.2% (wt/vol) BSA. To confirm this hypothesis, cells were
depleted in 0.1% (wt/vol) BSA. This led to a return to basal activity
values for PKB cotransfected with wild-type PDK1, but increased PKB
activity was maintained with the PDK1 mutants. To further approach this
phenomenon, a similar experiment with PH-PKB was performed. As seen
in Fig. 6B, PH-PKB is robustly activated by Mut- and PH-PDK1
mutants. Indeed, a 75- to 85-fold stimulation was seen, which we have
never found for PKB in these cells and under these conditions. We
interpret these findings to mean that the PH domain of PDK1 acts as a
negative modulator of PDK1 enzyme activity. If this hypothesis is
correct, we should be able to obtain a decrease in PH-PKB activity
when Mut-PDK1 is transfected together with its nonmutated wild-type PDK1 PH domain alone. This was indeed the case, since PH-PKB is 25%
less active when transfected together with Mut-PDK1 and the PH domain
of PDK1 compared to PH-PKB activity seen after transfection of
Mut-PDK1 alone (Fig. 6C). As a control, we have transfected PH-PKB
only with the PH domain of PDK1 to be sure that the PH domain impacts
on PDK1 activity and not PH-PKB activity (Fig. 6C).
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FIG. 6.
Role of the PDK1 PH domain in PKB activation. (A)
PKB and PDK1 proteins (Wild, Mut, or PH) were expressed in 293 cells. Cells were serum starved in 0.2% (wt/vol) (white bars) or 0.1%
(wt/vol) (dashed bars) BSA and stimulated for 5 min with insulin
(106 M) (black bars), and PKB kinase activity was
determined as described in Materials and Methods. Kinase activity is
expressed as fold increase compared to that of nonstimulated wild-type
cells. The levels of the expressed enzymes measured by immunoblotting
are shown below the bar graph. (B) PH-PKB and PDK1 constructs (Wild,
Mut, or PH) were expressed in 293 cells. Prior to stimulation for 5 min with insulin (106 M) (black bars) cells were serum
starved in 0.2% (wt/vol) BSA, and PH-PKB kinase activity was
determined as described in Materials and Methods. Kinase activity is
expressed as fold increase compared to that of PH-PKB nonstimulated
cells. Values shown are representative of at least three independent
experiments performed in triplicate. The levels of the expressed
enzymes measured by immunoblotting are shown below the bar graph. (C)
293 cells were transfected with PH-PKB and with PDK1 and PH-PDK1 as
indicated. PH-PKB activity was determined as described in Materials
and Methods. The levels of the expressed enzymes measured by
immunoblotting are shown below the bar graph.
|
|
| |
DISCUSSION |
We have approached here the mechanism of PKB activation by PDK1
using immunocytochemistry and biochemical analysis. One of the key
observations of our work is that in HeLa cells PDK1 translocates to the
plasma membrane in response to insulin. This translocation does not
require the catalytic activity of PDK1. Our results are consistent with
those published by Anderson et al. (6) showing PDK1
translocation in PAE cells exposed to PDGF. However, another recent
study from Currie et al. is at variance with this view (13).
Indeed, these authors found that in 293 cells PDK1 is constitutively
localized at the plasma membrane and that no increase in its membrane
presence is observed after either insulin or PDGF stimulation. Here we
provide evidence which helps to explain the contradictory results
obtained by the two groups. Indeed, it is possible that the discrepancy
could be due at least in part to differences in the basal level of the
3'-phospholipid products of PI 3-kinase in resting cells. We found that
a proportion of PDK1 was at the plasma membrane under basal conditions;
this occurred with a modest amount of PI 3-kinase associated with
IRS-1. The use of more-stringent deprivation conditions, i.e., 0.1%
BSA, was sufficient to (i) reduce basal PI 3-kinase activity, (ii) decrease basal phosphorylation of PKB Thr308, and (iii)
reduce the corresponding PDK1 plasma membrane localization. Since the
affinity of PDK1 for PI-3,4,5-P3 has been shown to be 22-fold higher than that of PKB (13)
(Kd = 1.6 nM for PDK1 versus 35 nM for
PKB), it is reasonable to assume that the basal levels of 3'
phospholipids are sufficient to promote the localization of PDK1 to the
plasma membrane whereas they are not high enough to result in PKB
plasma membrane recruitment.
We next examined the effects of coexpression of different mutants of
PDK1 with PKB on the PKB kinase activity. Coexpression of PKB with
wild-type PDK1 resulted in an increment in activity in the absence of
insulin as compared to that seen without coexpression of PDK1.
Expression of PKB together with kinase-inactive PDK1 did not result in
an increase in the basal PKB kinase activity, indicating that the
kinase activity of PDK1 is essential for PKB stimulation under these
conditions. Ectopic expression of wild-type PDK1 also resulted in a
significant enhancement of the insulin-induced PKB activation.
Surprisingly, coexpression of the Kd-PDK1 resulted in a similar
potentiation of the insulin-induced PKB activation. Those results
illustrate that Kd-PDK1 does not act as a dominant-negative form in
response to insulin as it was shown by Pullen et al. (20) with p70S6k activation by PDK1 in insulin-stimulated 293 cells. Indeed, cell surface translocation and phospholipids are not
required for p70S6k phosphorylation and activation
(3), while they are for PKB. The activation mechanism of PKB
differs from the one occurring for p70S6k at least for
those two major aspects. Therefore, it is not surprising that Kd-PDK1
differently affects PKB activity and that of p70S6k.
At first glance our data would seem at variance with the widely
accepted model in which PDK1 is one of the major kinases responsible for the phosphorylation and activation of PKB in response to growth factor stimulation. However, these apparent contradictions can be
explained if the key role of PDK1 is in fact to cause translocation of
PKB to the plasma membrane and if this is the rate-limiting step in PKB
activation. As we have shown in this report, kinase-deficient PDK1
is still able to be transported to the cell surface in
response to insulin. Therefore, ectopic expression of Kd-PDK1 with
PKB could increase the efficiency of PKB translocation to
the plasma membrane where it can be activated by endogenous PDK1
and a putative PDK2.
To verify that PDK1 is involved in promoting the intracellular movement
of PKB, we localized these two kinases using confocal microscopy in
HeLa cells and subcellular fractionation in 293 cells. For confocal
microscopy analysis, HeLa cells were used instead of 293 cells, since
we found that 293 cells are difficult cells on which to perform
imaging. While preliminary data indicated that the distribution of PKB
in 293 cells was similar to that seen in HeLa cells, these data are not
conclusive at this point in time. Cotransfection of GFP-PKB along with
different PDK1 constructs clearly showed that PDK1 was able to promote
PKB translocation to the plasma membrane. In addition, a PDK1 mutant
defective in its PH domain was unable to induce PKB translocation,
demonstrating the role of the PDK1 PH domain in PKB translocation.
However, the PH domain of PKB does not appear to be essential for
intracellular movement, since ectopic expression of PDK1 resulted in
translocation of a PKB mutant lacking its PH domain.
In a previous report we investigated the role of the PKB PH domain in
activation of the enzyme and found that it was required for PKB
translocation to the cell surface (21). This membrane targeting likely resulted in a change in PKB conformation allowing its
phosphorylation and subsequent activation by PDK1 and PDK2. In the
present report, we analyzed the role of the PDK1 PH domain. We have
shown, as previously reported (13), that PH domain-defective PDK1s are unable to translocate to the plasma membrane. However, it is
not known whether binding to phospholipids is the only important function of the PDK1 PH domain. To determine if the PH domain of PDK1
fulfills other functions as well, we cotransfected with PKB or
PH-PKB different PDK1 constructs mutated in or devoid of their PH
domain. An intriguing result was obtained when PH-PKB was
cotransfected with either PH-PDK1 or Mut-PDK1. Under these conditions, PH-PKB was active to the same extent without or with stimulation by insulin, demonstrating that generation of 3'
phospholipids by PI 3-kinase does not contribute to this activation
process. This can be explained if the PH domain of PDK1 is somehow
acting in an inhibitory fashion to prevent PKB activation by PDK1 and if phospholipid binding to the PH domain removes this negative constraint. However, when we performed in vitro phosphorylation of
PH-PKB by PH-PDK1 versus that by PDK1, we did not see a much higher activation of PH-PKB by PH-PDK1 than by PDK1 (data not shown). This could be explained if in intact cells another protein is
required to produce increased PH-PDK1-mediated activation of
PH-PKB. PDK1 appears to be a constitutively active kinase that
does not require phosphorylation by another kinase for its activation,
since its autophosphorylation seems to be activating. Several recent
reports, including our own, support the view that both kinases may be
functionally regulated by PtdIns-3,4,5-P3. This
evidence can be summarized as follows: (i) PDK1-induced
phosphorylation of a PH domain-deleted mutant of PKB (PH-PKB)
in vitro is enhanced by PtdIns-3,4,5-P3 (23);
(ii) although a fraction of PDK1 is constitutively associated with the
plasma membrane, more molecules become associated via a PH
domain-dependent mechanism following PDGF stimulation (6,
13); (iii) suboptimal doses of PDGF and insulin synergize
with PDK1 to activate PKB (6); (iv) phosphorylation, but not
membrane association, of myristoylated PKB is partially inhibited by
wortmannin or by depletion of transfected 293 cells in 0.1% BSA for
24 h (19).
Taking our results as a whole, we propose the following model to
explain the activation of PKB by PDK1 and the requirement for
phospholipids. When PKB resides in the cytosol, its conformation is
such that its PH domain blocks access to residue Thr308,
which therefore cannot be phosphorylated by PDK1 (Fig.
7A). After stimulation by insulin, 3'
phospholipids which promote PDK1 translocation to the membrane together
with PKB are produced. There, PKB is phosphorylated by PDK1 and
probably by PDK2 (Fig. 7C). At that point, both kinases are in the
proper conformation and in the adequate compartment for optimal
activation. When PKB is in the favorable conformation but located in
the cytosol, such as is the case with PH-PKB, PDK1 is not in a
functionally active configuration due to its folded PH domain (Fig.
7B). When both PKB and PDK1 PH domains are removed, negative
constraints are relieved and the molecules are in configurations
allowing maximal activity independent of phospholipids (Fig. 7E).
Finally, PKB in the presence of PH-PDK1 is slightly activated, but
because PKB is not in an optimal conformation, the extent of activation is less than that seen with PH-PKB (Fig. 7F). This is the case even
after insulin stimulation, since translocation is not possible due to
the lack of the PDK1 PH domain. Elevated basal PKB activation (4.6-fold
stimulation in the case of mutPDK1 and 2.8-fold in the case of
PH-PDK1) under these conditions is independent of the presence of
phospholipids.
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FIG. 7.
Working hypothesis for activation of PKB by PDK1. (A and
B) Activation without insulin; (C and D) activation with insulin; (E
and F) activation with or without insulin.
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|
Considered together, our results strengthen the concept that certain PH
domains can act as specific membrane recruitment devices, regulating
the translocation of soluble proteins such as PKB. Moreover, we
demonstrate that some PH domains can exert functions other than just
binding to phospholipids in that they also appear to control the
activity level of the kinase. Indeed, our data indicate that the PH
domain of PDK1 appears to modulate the enzyme conformation, which
permits it to modify the kinase activity depending on intracellular localization.
| |
ACKNOWLEDGMENTS |
Our research was supported by the Institut National de la
Santé et de la Recherche Médicale, the Association
pour la Recherche sur le Cancer, the Université de Nice-Sophia
Antipolis, the Ligue contre le Cancer, Groupe LIPHA-Merck (Lyon,
France), and the European Community (grant QLG1-CT-1999-00674). C.S.
was a recipient of a Poste Vert from INSERM.
We thank P. T. Hawkins for the generous gift of Myc-tagged PDK1
constructs and proteins purified from baculovirus-expressing Sf9 cells.
| |
FOOTNOTES |
*
Corresponding author. Mailing address: INSERM U
145, IFR 50, Faculté de Médecine, Avenue de Valombrose,
06107 Nice Cedex 2, France. Phone: 33-4-93-81-54-47. Fax:
33-4-93-81-54-32. E-mail: vanobbeg{at}unice.fr.
| |
REFERENCES |
| 1.
|
Ahmed, N. N.,
H. L. Grimes,
A. Bellacosa,
T. O. Chan, and P. N. Tsichlis.
1997.
Transduction of interleukin-2 antiapoptotic and proliferative signals via Akt protein kinase.
Proc. Natl. Acad. Sci. USA
94:3627-3632[Abstract/Free Full Text].
|
| 2.
|
Alessi, D., and P. Cohen.
1998.
Mechanism of activation and function of protein kinase B.
Curr. Opin. Genet. Dev.
8:55-62[CrossRef][Medline].
|
| 3.
|
Alessi, D.,
M. T. Kozlowski,
Q.-P. Weng,
N. Morrice, and J. Avruch.
1997.
3-Phosphoinositide-dependent protein kinase 1 (PDK1) phosphorylates and activates the p70 S6 kinase in vivo and in vitro.
Curr. Biol.
8:69-81.
|
| 4.
|
Alessi, D. R.,
M. Deak,
A. Casamayor,
F. B. Caudwell,
N. Morrice,
D. G. Norman,
P. Gaffney,
C. B. Reese,
C. N. MacDougall,
D. Harbison,
A. Ashworth, and M. Bownes.
1997.
3-Phosphoinositide-dependent protein kinase-1 (PDK1): structural and functional homology with the Drosophila DSTPK61 kinase.
Curr. Biol.
7:776-789[CrossRef][Medline].
|
| 5.
|
Alessi, D. R.,
S. R. James,
C. P. Downes,
A. B. Holmes,
P. R. J. Gaffney,
C. B. Reese, and P. Cohen.
1997.
Characterization of a 3-phosphoinositide-dependent kinase which phosphorylates and activates protein kinase B.
Curr. Biol.
7:261-269[CrossRef][Medline].
|
| 6.
|
Anderson, K. E.,
J. Coadwell,
L. R. Stephens, and P. T. Hawkins.
1998.
Translocation of PDK-1 to the plasma membrane is important in allowing PDK-1 to activate protein kinase B.
Curr. Biol.
8:684-691[CrossRef][Medline].
|
| 7.
|
Andjelkovic, M.,
D. Alessi,
R. Meier,
A. Fernandez,
N. Lamb,
M. Frech,
P. Cron,
P. Cohen,
J. Lucocq, and B. Hemmings.
1997.
Role of translocation in the activation and function of protein kinase B.
J. Biol. Chem.
272:31515-31524[Abstract/Free Full Text].
|
| 8.
|
Andjelkovic, M.,
T. Jakubowicz,
P. Cron,
X.-F. Ming,
J.-W. Han, and B. A. Hemmings.
1996.
Activation and phosphorylation of a pleckstrin holology domain containing protein kinase (RAC-PK/PKB) promoted by serum and protein phosphatase inhibitors.
Proc. Natl. Acad. Sci. USA
93:5699-5704[Abstract/Free Full Text].
|
| 9.
|
Burgering, T.,
M. Boudewijn, and P. J. Coffer.
1995.
Protein kinase B (c-Akt) in phosphotidylinositol-3-OH kinase signal transduction.
Nature
376:599-602[CrossRef][Medline].
|
| 10.
|
Cheng, J. Q.,
A. K. Godwin,
A. Bellacosa,
T. Taguchi,
T. F. Franke,
T. C. Hamilton,
P. N. Tsichlis, and J. R. Testa.
1992.
AKT2, a putative oncogene encoding a member of a subfamily of protein-serine/threonine kinases is amplified in human ovarian carcinomas.
Proc. Natl. Acad. Sci. USA
89:9267-9271[Abstract/Free Full Text].
|
| 11.
|
Cheng, J. Q.,
B. Ruggeri,
W. M. Klein,
G. Sonoda,
D. A. Altomare,
D. K. Watson, and J. R. Testa.
1996.
Amplification of AKT2 in human pancreatic-cancer cells and inhibition of AKT2 expression and tumorigenicity by antisense RNA.
Proc. Natl. Acad. Sci. USA
93:3636-3641[Abstract/Free Full Text].
|
| 12.
|
Cross, D. A. E.,
D. R. Alessi,
P. Cohen,
M. Andjelkovich, and B. A. Hemmings.
1995.
Inhibition of glycogen synthetase kinase-3 by insulin mediated by protein kinase B.
Nature
378:785-789[CrossRef][Medline].
|
| 13.
|
Currie, R. A.,
K. S. Walker,
A. Gray,
M. Deak,
A. Casamayor,
C. P. Downes,
P. Cohen,
D. R. Alessi, and J. Lucocq.
1999.
Role of phosphatidylinositol 3,4,5-trisphosphate in regulating the activity and localization of 3-phosphoinositide-dependent protein kinase-1.
Biochem. J.
337:575-583.
|
| 14.
|
Filippa, N.,
C. L. Sable,
C. Filloux,
B. A. Hemmings, and E. Van Obberghen.
1999.
Mechanism of protein kinase B activation by cyclic AMP-dependent protein kinase.
Mol. Cell. Biol.
19:4989-5000[Abstract/Free Full Text].
|
| 15.
|
Franke, T. F.,
S.-I. Yang,
T. O. Chan,
K. Datta,
A. Kazlauskas,
D. K. Morrison,
D. R. Kaplan, and P. N. Tsichlis.
1995.
The protein kinase encoded by the Akt proto-oncogene is a target of the PDGF-activated phosphatidylinosital 3-kinase.
Cell
81:727-736[CrossRef][Medline].
|
| 16.
|
Frech, M.,
M. Andjelkovic,
E. Ingley,
K. K. Reddy,
J. R. Falck, and B. A. Hemmings.
1997.
High affinity binding of inositol phosphates and phosphoinositides to the pleckstrin homology domain of RAC/protein kinase B and their influence on kinase activity.
J. Biol. Chem.
272:8474-8481[Abstract/Free Full Text].
|
| 17.
|
Göransson, O.,
J. Wijkander,
V. Manganiello, and E. Degerman.
1998.
Insulin-induced translocation of protein kinase B to the plasma membrane in rat adipocytes.
Biophys. Biochem. Res. Commun.
246:249-254.
|
| 18.
|
Kohn, A. D.,
K. S. Kovacina, and R. A. Roth.
1995.
Insulin stimulates the kinase activity of RAC-PK, a pleckstrin homology domain containing Ser/thr kinase.
EMBO J.
14:4288-4295[Medline].
|
| 19.
|
Li, Z.,
M. Wahl,
A. Eguinoa,
L. Stephens,
P. Hawkins, and O. Witte.
1997.
Proc.
Natl. Acad. Sci. USA
94:13820-13825[Abstract/Free Full Text].
|
| 20.
|
Pullen, N.,
P. Dennis,
M. Andjelkovic,
A. Dufner,
S. Kozma,
B. Hemmings, and G. Thomas.
1998.
Phosphorylation and activation of p70s6k by PDK1.
Science
279:707-710[Abstract/Free Full Text].
|
| 21.
|
Sable, C. L.,
N. Filippa,
C. Filloux,
B. A. Hemmings, and E. Van Obberghen.
1998.
Involvement of the pleckstrin homology domain in the insulin-stimulated activation of protein kinase B.
J. Biol. Chem.
273:29600-29606[Abstract/Free Full Text].
|
| 22.
|
Stephens, L.,
K. Anderson,
D. Stokoe,
H. Erdjument-Bromage,
G. Painter,
A. Holmes,
P. Gaffney,
C. Reese,
F. McCormick,
P. Tempst,
J. Coadwell, and P. Hawkins.
1998.
Protein kinase B kinase that mediate phosphatidylinositol 3,4,5-trisphosphate-dependent activation of protein kinase B.
Science
279:710-714[Abstract/Free Full Text].
|
| 23.
|
Stokoe, D.,
L. R. Stephens,
T. Copeland,
P. R. J. Gaffney,
C. B. Reese,
G. F. Painter,
A. B. Holmes,
F. McCormick, and P. T. Hawkins.
1997.
Duel role of phosphatidylinositol-3,4,5,-trisphosphate in the activation of protein kinase B.
Science
277:567-570[Abstract/Free Full Text].
|
| 24.
|
Walker, K.,
M. Deak,
A. Paterson,
K. Hudson,
P. Cohen, and D. Alessi.
1998.
Activation of protein kinase B beta and gamma isoforms by insulin and by 3-phosphoinositide-dependent protein kinase-1 in vitro: comparison with protein kinase B.
Biochem. J.
331:299-308.
|
| 25.
|
Wijkander, J.,
L. Stenson-Holst,
T. Rahn,
S. Resjo,
I. Castan,
V. Manganiello,
P. Belfrage, and E. Degerman.
1997.
Regulation of protein kinase B in rat adipocytes by insulin, vanadate, and peroxyvanadate.
J. Biol. Chem.
272:21520-21526[Abstract/Free Full Text].
|
Molecular and Cellular Biology, August 2000, p. 5712-5721, Vol. 20, No. 15
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Copyright © 2000, American Society for Microbiology. All rights reserved.
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Abstract
Introduction
