GSK2334470

Characterization of GSK2334470, a novel and highly specific inhibitor of PDK1

PDK1 (3-phosphoinositide-dependent protein kinase 1) activates a group of protein kinases belonging to the AGC [PKA (protein kinase A)/PKG (protein kinase G)/PKC (protein kinase C)]- kinase family that play important roles in mediating diverse biological processes. Many cancer-driving mutations induce activation of PDK1 targets including Akt, S6K (p70 ribosomal S6 kinase) and SGK (serum- and glucocorticoid-induced protein kinase). In the present paper, we describe the small molecule GSK2334470, which inhibits PDK1 with an IC50 of 10 nM, but does not suppress the activity of 93 other protein kinases including 13 AGC-kinases most related to PDK1 at 500- fold higher concentrations.

Addition of GSK2334470 to HEK (human embryonic kidney)-293, U87 or MEF (mouse embryonic fibroblast) cells ablated T-loop residue phosphorylation and activation of SGK isoforms and S6K1 induced by serum or IGF1 (insulin-like growth factor 1). GSK2334470 also inhibited T-loop phosphorylation and activation of Akt, but was more efficient at inhibiting Akt in response to stimuli such as serum that activated the PI3K (phosphoinositide 3-kinase) pathway weakly. GSK2334470 inhibited activation of an Akt1 mutant lacking the PH domain (pleckstrin homology domain) more potently than full-length Akt1, suggesting that GSK2334470 is more effective at inhibiting PDK1 substrates that are activated in the cytosol rather than at the plasma membrane. Consistent with this, GSK2334470 inhibited Akt activation in knock-in embryonic stem cells expressing a mutant of PDK1 that is unable to interact with phosphoinositides more potently than in wild-type cells. GSK2334470 also suppressed T-loop phosphorylation and activation of RSK2 (p90 ribosomal S6 kinase 2), another PDK1 target activated by the ERK (extracellular-signal-regulated kinase) pathway. However, prolonged treatment of cells with inhibitor was required to observe inhibition of RSK2, indicating that PDK1 substrates possess distinct T-loop dephosphorylation kinetics. Our data define how PDK1 inhibitors affect AGC signalling pathways and suggest that GSK2334470 will be a useful tool for delineating the roles of PDK1 in biological processes.

Key words: Akt/Akt1, cancer, kinase inhibitor, 3-phospho- inositide-dependent protein kinase, (PDK1), phosphoinositide 3-kinase (PI3K), p90 ribosomal S6 kinase (RSK), p70 ribosomal S6 kinase (S6K), serum- and glucocorticoid-induced protein kinase (SGK).

INTRODUCTION

PDK1 (3-phosphoinositide-dependent protein kinase 1) plays an important role in growth factor signalling cascades by phosphorylating and activating a group of protein kinases belonging to the AGC [PKA (protein kinase A)/PKG (protein kinase G)/PKC (protein kinase C)]-kinase family [1,2]. These enzymes co-ordinately regulate the cellular machinery controlling protein synthesis, metabolism, survival and proliferation. Kinases activated by PDK1 include isoforms of Akt [3], S6K1 (p70 ribosomal S6 kinase 1) [4], SGK (serum- and glucocorticoid- induced protein kinase) [5], RSK (p90 ribosomal S6 kinase) [6] and PKC [7]. The significance of the PDK1 pathway in pathological conditions is highlighted by the findings that the majority of human tumours have mutations in genes such as PTEN (phosphatase and tensin homologue deleted on chromosome 10), resulting in overactivation of PDK1 targets that promote proliferation and growth of tumour cells [2]. PDK1 is also frequently overexpressed in a variety of tumours including breast cancer [8,9]. Reduction in PDK1 expression protects mice from developing tumours resulting from the loss of the PTEN tumour suppressor [10]. These observations indicate that PDK1 inhibitors might have therapeutic utility for the treatment of cancer, a hypothesis that has been difficult to evaluate due to the lack of specific PDK1 inhibitors. Recent work has also suggested that inhibitors of PDK1 might have other benefits, such as counteracting resistance of cancer cells to drugs such as tamoxifen [11,12]. A number of PDK1 inhibitors, such as UCN-01 [13,14], BX-795 [15], dibenzo[c,f ][2,7]naphthyridine 1 derivatives [16] and celecoxib derivatives [17], have been described to date that are poorly specific and/or ineffective at inhibiting PDK1-dependent pathways in vivo (reviewed in [18]).

PDK1 activates 23 AGC kinases by phosphorylating a specific threonine or serine residue located within the T-loop of the kinase domain [1]. Maximal activation also necessitates phosphorylation of a serine/threonine residue located C-terminal to the catalytic domain, within a region known as the hydrophobic motif. Previous work has established that mTORC1 [mTOR (mammalian target of rapamycin) complex 1] phosphorylates the hydrophobic motif of S6K1, whereas a distinct mTORC2 complex phosphorylates the hydrophobic motif of Akt and SGK isoforms [19,20]. In the case of RSK, a second kinase domain, located C-terminal to the AGC catalytic domain, is activated by the ERK (extracellular-signal- regulated kinase)1/2 pathway phosphorylating the hydrophobic motif [21].

Agonists induce activation of AGC kinases by diverse mechanisms. In the case of S6K, SGK and RSK isoforms, which are activated in the cytosol, stimuli induce the phosphorylation of hydrophobic motifs by activating hydrophobic motif kinases. This phosphorylation promotes interaction, phosphorylation and activation by PDK1 [1,22]. Activation of Akt occurs at the plasma membrane and necessitates prior activation of PI3K (phosphoinositide 3-kinase) and generation of PtdIns(3,4,5)P3. PtdIns(3,4,5)P3 binds to the PH domain (pleckstrin homology domain) of Akt not only recruiting it to the cell membrane, but also inducing a conformational change that enables PDK1 to phosphorylate the T-loop residue of Akt (Thr308) [23–26]. PDK1 also contains a PH domain that binds with high affinity to PtdIns(3,4,5)P3 and PtdIns(3,4)P2, and more weakly to PtdIns(4,5)P2 [27,28]. The binding of PDK1 to phosphoinositides does not affect the catalytic activity, but functions to co-localize PDK1 and Akt at the plasma membrane thereby promoting Akt phosphorylation [29].

In the present paper, we report on the small molecule GSK2334470, which we establish is a highly specific and potent inhibitor of PDK1. We demonstrate that GSK2334470 can be employed in cells to ablate T-loop phosphorylation and activation of SGK, S6K1 and RSK as well also suppressing the activation of Akt. Our data indicate that GSK2334470 will be useful in probing biological processes controlled by PDK1.

MATERIALS AND METHODS

Materials

GSK2334470 was generated by GlaxoSmithKline [30] and detailed synthesis will be described elsewhere. GSK2334470 will be available from a commercial supplier in the near future. Protein G–Sepharose and glutathione–Sepharose were purchased from Amersham Biosciences. [γ -32P]ATP was from PerkinElmer. IGF1 (insulin-like growth factor 1) was from Cell Signaling Technology. DMSO, PMA and Tween 20 were from Sigma– Aldrich. CHAPS was from Calbiochem. PI-103 and GDC-0941 were synthesized by Dr Natalia Shpiro at the MRC Protein Phosphorylation Unit, University of Dundee, Dundee, Scotland, U.K. Recombinant full-length PDK1 was expressed in insect cells [31]. GST (glutathione transferase)–Akt1 and GST–∆PH- Akt1 (Akt1 lacking the PH domain) were purified from HEK (human embryonic kidney)-293 cells treated with 1 μM PI-103, a PI3K inhibitor, for 30 min as described previously [24]. Plasmids encoding SGK isoforms have been described previously [32,33]. Littermate wild-type PDK1 and homozygous PDK1K465E/K465E mouse ES (embryonic stem) cells were cultured as described previously [29].

Antibodies

The following antibodies were raised in sheep and affinity-purified on the indicated antigen: anti-Akt1 (S695B, third bleed; raised against residues 466–480 of human Akt1 RPHFPQFSYSASGTA, and used for immunoblotting and immunoprecipitation), anti- S6K (S417B, second bleed; raised against residues 25–44 of human S6K AGVFDIDLDQPEDAGSEDEL, and used for immunoblotting and immunoprecipitation), anti-PRAS40 (proline-rich Akt substrate of 40 kDa) (S115B, first bleed; raised against residues 238–256 of human PRAS40 DLPRPRLNTSD- FQKLKRKY, and used for immunoblotting), anti-phospho- PRAS40 Thr246 (S114B, second bleed, raised against residues 240–251 of human PRAS40 CRPRLNTpSDFQK, used for immunoblotting), anti-RSK2 (S382B, first bleed; residues 712– 734 of human RNQSPVLEPVGRSTLAQRRGIKK, and used for immunoblotting), anti-PDK1 (S682, third bleed; raised against residues 544–556 of human PDK1 RQRYQSHPDAAVQ, and used for immunoblotting and immunoprecipitation), anti- NDRG1 (N-myc downstream-regulated gene 1) (S276B third bleed; raised against full-length human NDRG1, and used for immunoblotting) and anti-phospho-NDRG1 Thr346/Thr356/Thr366 (S911B second bleed; raised against RSRSHTpSEG, a sequence common to all the three SGK1 phosphorylation sites on NDGR1, and used for immunoblotting). The following commercially available antibodies were used in the present study: phospho- RSK Ser227 (#sc-12445-R) and phospho-SGK1 Ser422 (#sc-16745) were purchased from Santa Cruz Biotechnology; phospho-Akt Ser473 (#9271), phospho-Akt Thr308 (#4056), phospho-S6K Thr389 (#9234), phospho-S6 ribosomal protein Ser235/Ser236 (#4856), phospho-S6 ribosomal protein Ser240/Ser244 (#4838), total S6 ribosomal protein (#2217), phospho-ERK Thr202/Tyr204 (#9101), total ERK (#9102), phospho-RSK Thr573 (#9346), phospho- GSK3 (glycogen synthase kinase 3)α/β Ser21/9 (#9331), phospho- PDK1 Ser241 (#3061) and phospho-NDRG1 Thr346 (#5482) were purchased from Cell Signaling Technology. For immunoblotting of the phosphorylated T-loop of S6K1, we employed the pan- PDK1 site antibody from Cell Signaling Technology (#9379) as described previously [34]. We have also found that this pan-PDK1 site antibody efficiently recognizes the phosphorylated T-loop of SGK isoforms (see Figure 2). The GSK3α/β antibody (#44- 610) was purchased from Biosource. Anti-GST–HRP (horseradish peroxidase) conjugate was purchased from Abcam (#ab58626). Secondary antibodies coupled to HRP used for immunoblotting were obtained from Thermo Scientific.

General methods

Tissue culture, immunoblotting, restriction enzyme digests, DNA ligations and other recombinant DNA procedures were performed using standard protocols. DNA constructs used for transfection were purified from Escherichia coli DH5α using a Qiagen plasmid Mega or Maxi kit, according to the manufacturer’s protocol. All DNA constructs were verified by DNA sequencing, performed by DNA Sequencing & Services (MRC Protein Phosphorylation Unit, College of Life Sciences, University of Dundee, Scotland, U.K.; www.dnaseq.co.uk) using Applied Biosystems Big-Dye Ver 3.1 chemistry on an Applied Biosystems model 3730 automated capillary DNA sequencer. For transient transfections, ten 10- cm-diameter dishes of HEK-293 cells were cultured and each dish was transfected with 10 μg of the indicated plasmids using the polyethylenimine method [35]. Vesicles containing 100 μM PC (phosphatidylcholine), 100 μM PS (phosphatidylserine) and 10 μM PtdIns(3,4,5)P3 PtdIns(3,4,5)P3(diC16) [L-α-D-myo- phosphatidylinositol 3,4,5-triphosphate 3-O-phospho-linked, D( )-sn-1,2-di-O-hexadecanoylglyceryl] (#208; CellSignals) were prepared, and activation of Akt in the presence and absence of the PC/PS/PtdIns(3,4,5)P3 vesicles was undertaken as described previously [36]. Measurement of PDK1 activity employing the PDKtide peptide substrate (KT-FCGTPEYLAPEVRREPRILSEEEQEMFRDFDYIADWC) was undertaken as described previously [37].

Buffers

The following buffers were used: lysis buffer CHAPS-LB [40 mM Tris/HCl (pH 7.5), 0.3 % CHAPS, 120 mM NaCl, 0.27 mM sucrose, 1 mM EDTA, 50 mM NaF, 10 mM 2-glycerophosphate, 5 mM sodium pyrophosphate, 1 mM sodium orthovanadate (added prior to lysis), 1 mM benzamidine (added prior to lysis), 1 mM PMSF (added prior to lysis) and 0.1 % 2-mercaptoethanol (added prior to lysis)], TBS-Tween [50 mM Tris/HCl (pH 7.5),
0.15 M NaCl and 0.1 % Tween 20], kinase buffer [50 mM Tris/HCl (pH 7.5), 0.1 mM EGTA and 0.1 % 2-mercaptoethanol], wash buffer [50 mM Tris/HCl (pH 7.5), 0.1 mM EGTA, 0.1 % 2- mercaptoethanol, 0.27 M sucrose and 0.03 % Brij-35] and sample buffer [50 mM Tris/HCl (pH 6.8), 6.5 % (v/v) glycerol, 1 % (w/v) SDS and 1 % (v/v) 2-mercaptoethanol].

Cell treatments and lysis

Cells were cultured in 10 % (v/v) FBS (fetal bovine serum) in DMEM (Dulbecco’s modified Eagle’s medium) (high glucose) and treated with or without different inhibitors as described in the Figure legends. Following treatment, cells were rinsed with 5 ml of ice-cold PBS, lysed employing 0.5 ml of the lysis buffer, lysates were clarified by centrifugation (16 000 g at 4 ◦C for 20 min), and supernatants were snap frozen in liquid nitrogen and stored at 80 ◦C until required. The protein concentration was determined using Coomassie Protein Assay Reagent (cat# 1856209; Thermo Scientific).

Specificity kinase panel

All assays were performed at The National Centre for Protein Kinase Profiling (http://www.kinase-screen.mrc.ac.uk/) as described previously [38]. Briefly, all assays were carried out robotically at room temperature (21 ◦C), and were linear with respect to time and enzyme concentration under the conditions used. Assays were performed for 30 min using Multidrop Micro reagent dispensers (Thermo Electron) in a 96-well format. The abbreviations for each kinase are defined in the legend to Table 1. The concentration of magnesium acetate in the assays was 10 mM and [γ -32P]ATP ( 800 c.p.m./pmol) was used at 5 μM for Aurora A, CK2α, DYRK3, EF2K, ERK1, ERK8, GSK3β, HER4, HIPK2, IGF1R, IKKβ, IRR, MARK3, MKK1, p38γ MAPK, p38δ MAPK, PAK4, PIM2, Akt1 (S473D), PLK1, PKCζ and PRK; 20 μM for Aurora B, BRSK1, CaMKKβ, CDK2-cyclinA2, CHK1, CHK2, CK1δ, CSK, EPH-B3, ERK2, FGFR1, GCK, HIPK1, HIPK3, IR, IRAK4, JNK1α1, JNK2α2, JNK3α1, LKB1, MAPKAP-K2, MAPKAP-K3, MARK2, MLK1, MLK3, MSK1, MST2, MST4, NUAK1, p38βMAPK, PAK2 (T402E), PAK5, PAK6, PDK1, PIM1, PIM3, PKA, PKCα, PKCγ , PRAK, RIPK2, ROCKII, S6K1 (T412E), SGK1 (S422D), SYK, TTK and YES1; and 50 μM for BRSK2, BTK, CaMK1, DYRK1a, DYRK2, EPH- A2, IKKε, LCK, MARK4, MELK, MINK1, MNK1, MNK2α, NEK2A, NEK6, p38αMAPK, Akt2 (S474D), PKD1, RSK1, RSK2, Src, SRPK1 and TBK1, in order to be at or below the Km for ATP for each enzyme [38]. Lipid kinases were assayed as described previously [39].

Kinase activity assays

Endogenous Akt, S6K and RSK were immunoprecipitated from 0.1 to 1 mg of cell lysate for 2 h at 4 ◦C on a vibrating platform using 3–5 μg of the indicated antibodies. For the SGK activity assays, 150 μg of transfected lysate was incubated with 5 μg of glutathione–Sepharose for 3 h at 4 ◦C.

The immunoprecipitates were washed twice with lysis buffer containing 0.5 mM NaCl, followed by two washes with kinase buffer. Kinase reactions were initiated by a reaction mixture to bring the final concentrations of the reaction components to 0.1 mM [γ -32P]ATP ( 200 c.p.m./pmol), 5 mM magnesium acetate, 0.1 % 2-mercaptoethanol and 30 mM Crosstide peptide (GRPRTSSFAEGKK), as described previously [40]. Reactions were carried out for 20 min at 30 ◦C on a vibrating platform and stopped by spotting the reactions on to P81 phosphocellulose paper. Cerenkov counting was done after washing the papers in phosphoric acid, rinsing in acetone and air-drying. One unit of activity was defined as that which catalysed the incorporation of 1 nmol of [32P]phosphate into the substrate over 1 h.

Purification of GST–Akt1 and GST–ΔPH-Akt1 from HEK-293 cells

Proteins were batch-purified as described previously with slight modifications [36]. Briefly, at 50 % confluency, HEK-293 cells in 10-cm-diameter dishes were transfected with 10 μg of plasmids encoding either GST–Akt or GST–∆PH-Akt using the polyethylenimine method [35]. After 24 h, cells were treated with 1 μM PI-103, a PI3K inhibitor, to induce dephosphorylation of Akt1 for 30 min and lysed as described above. The pooled supernatants were then incubated with glutathione–Sepharose (10 μl of beads/10-cm-diameter dish) for 1 h at 4 ◦C. The beads were washed twice with 10 vol. of lysis buffer containing 0.5 mM NaCl and 10 times with 10 vol. of wash buffer [in order to remove Triton X-100, which interferes with the PtdIns(3,4,5)P3 vesicle experiments]. Proteins were eluted from the beads by resuspension in an equal amount of wash buffer containing 20 mM glutathione (pH 7.5) for 1 h on ice. Supernatants were filtered through a 0.22-μm-spin column and aliquots were snap-frozen and stored at − 80 ◦C.

Immunoblotting

Total cell lysate (20 μg) or immunoprecipitated samples were heated at 95 ◦C for 5 min in sample buffer, and were subjected to PAGE (10 % gel) and electrotransfer on to nitrocellulose membranes. Membranes were blocked for 1 h in TBS-Tween containing 5 % (w/v) skimmed milk. The membranes were probed with the indicated antibodies in TBS-Tween containing 5 % (w/v) skimmed milk or 5 % (w/v) BSA for 16 h at 4 ◦C. Detection was performed using HRP-conjugated secon- dary antibodies and the ECL (enhanced chemiluminescence) reagent.

RESULTS

GSK2334470 suppresses SGK isoform T-loop phosphorylation and activity

To determine whether GSK2334470 could inhibit PDK1 activity in cells, we evaluated its impact on phosphorylation and activation of SGK isoforms induced by IGF1. We first monitored the effect that increasing concentrations of GSK2334470 had on the activity of endogenous SGK isoforms induced by IGF1 stimulation by analysing phosphorylation of the physiological SGK-specific substrate NDRG1 [41]. GSK2334470 induced significant dose- dependent inhibition of endogenous NDRG1 with over 50 % reduction in phosphorylation observed at doses of 0.1–0.3 μM (Figure 2A). As endogenous levels of SGK isoforms in HEK-293 cells are too low to study their phosphorylation state and activity [20], we overexpressed SGK1 (Figure 2B), SGK2 (Figure 2C) or SGK3 (Figure 2D) in HEK-293 cells and analysed the impact of GSK2334470 on IGF1-induced phosphorylation of the T-loop (PDK1 site) as well as intrinsic kinase activity. Stimulation of serum-starved HEK-293 cells with IGF1 in the absence of GSK2334470 induced marked T-loop phosphorylation of each isoform of SGK that was accompanied by increased kinase activity measured after immunoprecipitation (Figure 2). GSK2334470 induced a significant dose-dependent inhibition of the T-loop phosphorylation of each SGK isoform. Significant inhibition of T-loop phosphorylation was observed at low concentrations of 30 nM and was almost abolished at 0.1 μM inhibitor (Figure 2). GSK2334470 similarly inhibited SGK isoform activity and, at 0.1 μM, kinase activity was reduced to below levels observed in non-stimulated cells. Consistent with GSK2334470 inhibiting SGK isoform activity in cells, the drug suppressed phosphorylation of NDRG1 at similar doses to which it inhibited T-loop phosphorylation and kinase activity (Figure 2).

GSK2334470 suppresses S6K1 phosphorylation and activity

We investigated the effect of adding increasing amounts of GSK2334470 on endogenous S6K1 activity as well as T- loop and hydrophobic motif phosphorylation in HEK-293 cells cultured in the presence of serum (Figure 3A). Under these conditions, 1 μM GSK2334470 ablated S6K1 activity and phosphorylation of the T-loop (Thr229). Consistent with previous work showing that inhibition of S6K1 T-loop phosphorylation inhibits phosphorylation of the hydrophobic motif [42–44], GSK2334470 inhibited hydrophobic motif phosphorylation of S6K1 to a similar extent as T-loop phosphorylation (Figure 3A). GSK2334470 also inhibited phosphorylation of S6, an S6K substrate [4] (Figure 3A). The ability of GSK2334470 to suppress S6K1 activity and phosphorylation was rapid, with near maximal inhibition observed within 10 min and sustained for at least 2 h, the longest time point examined (Figure 3B). GSK2334470 also suppressed S6K1 activity and phosphorylation induced by IGF1 stimulation of serum-starved HEK-293 cells, although 3- fold higher concentrations were required to fully inhibit S6K1, compared with cells cultured in serum (compare Figure 3A with 3C). This is likely to be explained by the significantly higher degree of activation of the PI3K pathway and hence higher S6K1 activity induced by IGF1 compared with serum. Similar results have been observed for other signal transduction inhibitors such as Ku-0063794 [45] and PF-4708671 [39], where an 3-fold higher dose of these drugs are required to inhibit signalling responses in IGF1-treated HEK-293 cells compared with serum.

Figure 2 Effect of GSK2334470 on SGK activity in HEK-293 cells (A) HEK-293 cells were serum-starved overnight and treated with the indicated concentrations of GSK2334470 for 30 min and stimulated with 50 ng/ml IGF1 for 30 min. Cells were lysed and lysates immunoblotted with the indicated antibodies. (B–D) HEK-293 cells were transfected with constructs encoding GST–∆N-SGK1 (which lacks residues 1–60) (B), GST–SGK2 (C) or GST–SGK3 (D). At 24 h post-transfection, cells were deprived of serum overnight and treated with the indicated concentration of GSK2334470 prior to stimulation with IGF1 as in (A). SGK isoforms were affinity-purified on glutathione–Sepharose and their catalytic activities were assayed using Crosstide as a substrate peptide. Each bar represents the mean + S.D specific activity from two different samples, with each sample assayed in duplicate. Affinity-purified SGK1 was also subjected to immunoblotting with an anti-GST antibody. Cell lysates were also analysed by immunoblotting with the other indicated antibodies. Similar results were obtained in two separate experiments.

GSK2334470 partially suppresses Akt1 phosphorylation and activity

We next studied the effect of adding increasing doses of GSK2334470 on the activity and T-loop (Thr308) as well as hydro- phobic motif phosphorylation (Ser473) of Akt1 in HEK-293 cells cultured in the presence of serum (Figure 4A). Similar to S6K1, GSK2334470 inhibited Thr308 phosphorylation as well as kinase activity. Although GSK2334470 did not suppress Akt1 activity to the same extent as treatment of cells with the PI3K inhibitor PI-103, 1 and 3 μM GSK2334470 markedly inhibited the phos- phorylation of several Akt substrates [FoxO (forkhead box O), GSK3 and PRAS40]. GSK2334470 did not significantly inhibit Ser473 hydrophobic motif phosphorylation of Akt1. GSK2334470 also induced near maximal inhibition of Akt1 activity and phosphorylation within 5 min, and Akt substrate phosphorylation (FoxO, GSK3 and PRAS40) was inhibited at a slightly later time point (10 min), as might be expected (Figure 4B).

When cells were stimulated with IGF1, Akt1 was activated to 20-fold higher levels than in cells cultured in serum [ 18 mU (milli-units)/mg of protein compared with 0.8 mU/mg of protein] (Figure 4). Following IGF1 stimulation, GSK2334470 even when deployed at high concentrations of 3 μM did not significantly inhibit Akt activation or phosphorylation of Thr308 or Ser473 (Figure 4C).

To study whether the ability of Akt to be activated by PDK1 at the plasma membrane might account for the reduced sensitivity to GSK2334470, we compared the effects that GSK2334470 had on overexpressed full-length Akt or a mutant of Akt lacking the PH domain (∆PH-Akt1) in serum- (Figure 5A) and IGF1- (Figure 5B) stimulated HEK-293 cells. This revealed that GSK2334470 suppressed T-loop phosphorylation of ∆PH-Akt1 with similar potency to that observed for SGK isoforms (Figure 2) and S6K1 (Figure 3). However, in the case of full-length overexpressed Akt1, GSK2334470 was much less efficient at inducing T-loop dephosphorylation compared with ∆PH-Akt1 (Figure 5).

We also investigated the ability of GSK2334470 to inhibit Akt phosphorylation in the previously described homozygous PDK1K465E/K465E knock-in ES cells expressing a mutant of PDK1 incapable of binding phosphoinositides [29] (Figure 5C). These studies revealed that GSK2334470 inhibited phosphorylation of Thr308 and Akt substrates (PRAS40 and GSK3) more potently in PDK1K465E/K465E knock-in cells compared with control littermate PDK1+/+ ES cells (Figure 5C). We observed that 0.3 μM GSK2334470 significantly inhibited phosphorylation of Akt or PRAS40/GSK3 in PDK1K465E/K465E knock-in but not wild-type ES cells (Figure 5C).

Figure 3 Effect of GSK2334470 on S6K1 activity in HEK-293 cells (A) HEK-293 cells cultured in medium containing 10 % (v/v) FBS were treated with the indicated concentrations of GSK2334470 for 30 min. Cells were lysed, endogenous S6K1 was immunoprecipitated and catalytic activity was assessed by employing the Crosstide substrate. Cell lysates were also analysed by immunoblotting using the indicated antibodies. Each bar represents the mean + S.D. specific activity from three separate samples. (B) As in (A), except cells were treated with 3 μM GSK2334470 for the indicated time points. (C) As in (A), except cells were serum-starved overnight and treated with the indicated concentrations of GSK2334470 for 30 min prior to stimulation with 50 ng/ml IGF1 for 30 min. Similar results were obtained in three separate experiments.

Figure 4 Effect of GSK2334470 on Akt activity in HEK-293 cells HEK-293 cells cultured in medium containing 10 % (v/v) FBS were treated with the indicated concentrations of GSK2334470 for 30 min. Cells were lysed, endogenous Akt1 was immunoprecipitated and catalytic activity was assessed by employing the Crosstide substrate. Each bar represents the mean + S.D. specific activity from three separate samples. Cell lysates were also analysed by immunoblotting using the indicated antibodies. (B) As in (A), except cells were treated with 3 μM GSK2334470 for the indicated time points. (C) As in (A), except cells were serum-starved overnight and treated with the indicated concentrations of GSK2334470 for 30 min prior to stimulation with 50 ng/ml IGF1 for 30 min. Similar results were obtained in three separate experiments.

Investigation of the effects of GSK2334470 in U87 cells and fibroblasts

We investigated the ability of GSK2334470 to inhibit Akt (Figure 6A) and S6K1 (Figure 6B) as well as SGK1 (Figure 6C) activation in U87 glioblastoma cells that lack PTEN expression.

Consistent with the idea that loss of PTEN would result in a reasonably potent activation of the Akt pathway, we found that a high dose of 3 μM GSK2334470 only partially suppressed Thr308 phosphorylation or Akt activation 3-fold. GSK2334470 almost reduced S6K1 activity to the basal levels observed in cells treated with 1 μM PI-103, a PI3K inhibitor (Figure 6B). In contrast, 1 μM GSK2334470 effectively suppressed SGK1 activity as judged by the inhibition of NDRG1 phosphorylation (Figure 6C).

In MEF (mouse embryonic fibroblast) cells cultured in serum, in which PI3K pathway activation would be expected to be moderately activated, 1 μM GSK2334470 suppressed Akt Thr308 phosphorylation and activity to the same extent as 1 μM PI-103 (Figure 7A). In MEF cells (Figure 7A), we observed that, in contrast with HEK-293 cells (Figure 4) and U87 cells (Figure 6A), GSK2334470 inhibited phosphorylation of Akt at its hydrophobic motif to a similar extent as T-loop phosphorylation. Moreover, 1 μM GSK2334470 also potently suppressed activation of S6K1 (Figure 7B) as well as SGK1 (Figure 7C).

Figure 5 Association of Akt with PtdIns(3,4,5)P 3 suppresses sensitivity to GSK2334470 (A) HEK-293 cells were transfected with constructs expressing either full-length GST–Akt1 or GST–∆PH-Akt. Cells were cultured in the presence of medium containing 10 % (v/v) FBS and, at 48 h post-transfection, cells were treated with the indicated concentrations of GSK2334470 for 30 min. Akt forms were affinity-purified on glutathione–Sepharose and their catalytic activities were assayed using Crosstide as a substrate peptide. Each bar represents the mean + S.D. specific activity from three separate samples. Purified Akt forms were also subjected to immunoblot analysis with the indicated antibodies. (B) As in (A), except cells serum-starved for 16 h prior to treatment with GSK2334470 and stimulated with 50 ng/ml IGF1 for 30 min. Similar results were obtained in three separate experiments. (C) Wild-type PDK1+/+ and homozygous knock-in PDK1K465E/K465E [29] were deprived of serum for 4 h and treated with the indicated concentrations of GSK2334470 for 30 min prior to stimulation with 50 ng/ml IGF1 for 30 min. Cells were lysed, endogenous Akt1 was immunoprecipitated and catalytic activity was assessed by employing the Crosstide substrate. Cell lysates were also analysed by immunoblotting using the indicated antibodies. WT, wild-type.

Figure 6 Effect of GSK2334470 on Akt and S6K activity in U87 cells (A) U87 cells cultured in medium containing 10 % (v/v) FBS were treated with the indicated concentrations of GSK2334470 for 30 min. Cells were lysed, endogenous Akt1 was immunoprecipitated and catalytic activity was assessed by employing the Crosstide substrate. Each bar represents the mean + S.D. specific activity from three separate samples. Cell lysates were also analysed by immunoblotting using the indicated antibodies. (B) As in (A), except that endogenous S6K1 was immunoprecipitated and assayed. (C) As in (A), except that lysates were immunoblotted with the total and phospho-NDRG1 antibody as a readout of endogenous SGK activity. Similar results were obtained in three separate experiments.

GSK2334470 inhibits RSK2 activity

To define whether GSK2334470 inhibited RSK2, we incubated HEK-293 cells cultured in serum with 3 μM GSK2334470 for up to 24 h and evaluated how this affected activity of endogenous RSK2 (Figure 8A). This revealed that incubation of cells with 3 μM GSK2334470 for 4 h induced 50 % inhibition of RSK2 activity that was accompanied by a partial dephosphorylation of the PDK1 T-loop residue (Ser227). After 8 and 24 h, RSK2 activity and T-loop phosphorylation was suppressed by over 90 %. As expected, GSK2334470 did not affect the phosphorylation of RSK2 at Thr573 (Figure 8A), which is phosphorylated independently of PDK1 by ERK1/2. We also incubated HEK-293 cells for 8 h with increasing concentrations of GSK2334470 and observed that 0.1 μM GSK2334470 induced 50 % inhibition of RSK2 activity, which was almost completely suppressed at 1 μM GSK233440 (Figure 8B). Similar observations were made in U87 cells (Figure 8C) as well as MEF cells (Figure 8D), where prolonged 8–24 h incubation with 3 μM GSK2334470 was required to substantially inhibit RSK2 activity and induce T-loop dephosphorylation.

DISCUSSION

In the present study, we have characterized GSK2334470, a novel small-molecule cell-permeant PDK1 inhibitor that does not significantly inhibit the activity of 93 other protein kinases tested, including 13 AGC kinases most closely related to PDK1. GSK2334470 is therefore much more specific than other reported PDK1 inhibitors, including the staurosporine analogue UCN-01 [13] or BX-795 [15], that inhibit several other kinases more potently than PDK1 [46,47]. At concentrations of 0.1–1.0 μM, GSK2334470 suppressed to basal levels the T-loop phosphorylation and activation of cytosolic PDK1 substrates SGK and S6K1 that do not bind PtdIns(3,4,5)P3. GSK2334470 also inhibited phosphorylation of NDRG1 and S6 protein, physiological substrates of SGK1 [41] and S6K1 [4] respectively. GSK2334470 also effectively suppressed RSK2 T- loop phosphorylation and activity in all of the three cell lines studied (Figure 8). Our data indicate that the turnover of the RSK2 T-loop phosphorylation site in serum-cultured cells is relatively slow, as approx. 8 h is required to induce substantial dephosphorylation of this residue in contrast with 10–30 min for other PDK1 substrates studied (Akt, S6K1 and SGK isoforms). Similar results have been obtained in ES cells expressing a gatekeeper mutant of PDK1 that is sensitive to the NM-PP1 inhibitor, where 24 h was required to inactivate RSK2, whereas other AGC kinases were inactivated within 1 h [48]. Overall, these studies reveal that PDK1 substrates display significant differences in the kinetics of T-loop dephosphorylation.

Figure 7 Effect of GSK2334470 on Akt and S6K activity in MEF cells (A) MEF cells cultured in medium containing 10 % (v/v) FBS were treated with the indicated concentrations of GSK2334470 for 30 min. Cells were lysed, endogenous Akt1 was immunoprecipitated and catalytic activity was assessed by employing the Crosstide substrate. Each bar represents the mean + S.D. specific activity from three separate samples. Cell lysates were also analysed by immunoblotting using the indicated antibodies. (B) As in (A), except for endogenous S6K. Similar results were obtained in three separate experiments. (C) As in (A), except that lysates were immunoblotted with total and phospho-NDRG1 antibodies as a readout of endogenous SGK activity.

A key observation that may be relevant to development of other PDK1 inhibitors is that GSK2334470 inhibits Akt1 activation less efficiently than S6K1 and SGK isoforms. Under conditions of low PI3K pathway activity (serum stimulation), GSK2334470 effectively inhibited Akt1 T-loop phosphorylation and activity as well as phosphorylation of Akt substrates (GSK3, FoxO and PRAS40) (Figures 4A and 7A). However, in response to IGF1, which induces strong activation of the PI3K pathway, GSK2334470 was ineffective at inhibiting T-loop phosphorylation of endogenous (Figure 4C) or overexpressed full-length (Figure 5) Akt. GSK2334470 also did not completely suppress Akt activation in glioblastoma U87 cells that lack PTEN, which would be expected to result in an intermediate activation of the Akt pathway (Figure 6A).

Previous biochemical analysis revealed that activation of full-length Akt by PDK1 undertaken in the presence of PtdIns(3,4,5)P3-containing lipid vesicles was remarkably efficient, requiring 100–1000-fold lower levels of PDK1 compared with substrates not possessing a PH domain [24,49]. The unusually high rate at which PDK1 can activate full-length Akt1 in the presence of lipid vesicles containing PtdIns(3,4,5)P3 is likely to be a result of both PDK1 and Akt possessing PtdIns(3,4,5)P3-binding PH domains enabling the co-localization of these enzymes on a two-dimensional membrane surface, thereby hugely enhancing the probability of interaction of PDK1 with Akt. As activation of Akt at the plasma membrane proceeds so efficiently, it is possible that only a very small fraction of endogenous PDK1 is actually required to activate Akt. In agreement with this notion, no inhibition of Akt activation was observed in ES cells or mice expressing 5–10-fold lower than normal expression of PDK1 [50,51]. Thus the inability of GSK2334470 to suppress Akt activation under conditions of high pathway activation could be explained by a small residual pool of non-inhibited PDK1 still capable of activating Akt at the membrane in inhibitor-treated cells. This would also explain why ∆PH-Akt, which is localized in the cytosol, was inhibited more potently than full-length Akt by GSK2334470 (Figures 5A and 5B). Moreover, the finding that GSK2334470 inhibited Akt phosphorylation in PDK1K465E/K465E ES cells, in which PDK1 can no longer interact with phosphoinositides, more potently than in wild-type cells is also consistent with the idea that it is harder to inhibit Akt activation by PDK1 associated with PtdIns(3,4,5)P3 on the membrane. It is also possible that PDK1 associated with the plasma membrane may not be as effectively exposed to GSK2334470 as cytosolic PDK1. However, at least in vitro, GSK2334470 effectively inhibited activation of Akt in the presence of PtdIns(3,4,5)P3-containing lipid vesicles (Figure 1B). Another possibility is that, in vivo, the pool of membrane- localized PDK1 is complexed to other protein(s) that influence kinase domain structure in a manner that renders it less potently inhibited by GSK2334470.

Figure 8 Effect of GSK2334470 on RSK2 activity in serum-cultured HEK-293 cells (A) HEK-293 cells cultured in medium containing 10 % (v/v) FBS were treated with 3 μM GSK2334470 for the indicated time points. Cells were lysed, endogenous RSK2 was immunoprecipitated and the catalytic activity was assessed by employing the Crosstide substrate. Each bar represents the mean + S.D. specific activity from three separate samples. Cell lysates were also analysed by immunoblotting using the indicated antibodies. Similar results were obtained in two separate experiments. (B) As in (A), except that cells were treated with the indicated concentrations of GSK2334470 for 8 h before lysis. (C and D) As in (A), except that U87 cells (C) or MEF cells (D) were employed.

The finding that GSK2334470 more efficiently suppresses Akt activity under conditions of weaker PI3K pathway stimulation has implications for the use of this drug. Our present data implies that different concentrations of PDK1 inhibitors may be required to inhibit Akt activity in cells dependent on the level of PI3K activation. If the aim is to inhibit the activity of RSK, then long (up to 8 h) exposure of cells with GSK2334470 is required to achieve substantial inhibition of this enzyme. Effects of GSK2334470 that are observed over shorter periods of time are unlikely to be due to inhibition of RSK isoforms. Our present data would suggest that other PDK1 inhibitors being developed would also suppress activation of the non-PtdIns(3,4,5)P3-binding cytosolic targets SGK or S6K more efficiently than Akt, especially in cells treated with agonists that induce a large activation of PI3K. If only a low percentage of cellular PDK1 is required to maximally activate Akt at the plasma membrane, this may indicate that it will be challenging to develop a drug that effectively suppresses Akt, especially in response to stimuli or mutations that induce large activation of the PI3K pathway.

Our present data suggest that GSK2334470 does not inhibit mTORC2, as this compound did not suppress hydrophobic motif phosphorylation endogenous Akt1 (Figure 4) or overexpressed Akt1 (Figure 5) or ∆PH-Akt1 (Figure 5). In contrast, GSK2334470 inhibited the hydrophobic motif phosphorylation of endogenous Akt in MEF cells exposed to serum to a similar extent as Thr308 phosphorylation (Figure 4). Structural analysis of Akt2 has established that T-loop phosphorylation and hydrophobic motif phosphorylation co-operate to stabilize the structure of the Akt kinase domain [52,53]. These studies indicate that inhibiting Thr308 phosphorylation by treatment with GSK2334470 would lead to a less stable Akt1 conformation, in which Ser473 would not interact with the kinase domain and would thus be exposed and accessible to becoming dephosphorylated by protein phosphatase(s). This may explain why GSK2334470 could lead to the loss of Akt Ser473 phosphorylation. However, further work is required to determine why GSK2334470 affects Ser473 phosphorylation in MEF cells, but not HEK-293 or U87 cells.
Although Akt is considered to be one of the key enzymes driving the growth and proliferation of cancer cells, there is increasing evidence that Akt-independent pathways, perhaps requiring SGK isoforms, may play a crucial role in driving expansion of a number of tumours [54]. Moreover, recent work carried out in Caenorhabditis elegans has disputed the widely believed opinion that Akt is the key mediator of signalling downstream of mTOR and at least in this species, with SGK rather than Akt being the key mediator of growth, fat metabolism, reproduction and life- span [55,56]. Akt has many other vital functions in cells and therefore an anticancer drug that potently inhibited Akt and other PDK1 substrates may have significant side effects. It will be very interesting to evaluate whether a compound such as GSK2334470, which inhibits S6K and SGK isoforms more potently than Akt, would be effective at suppressing the growth of various cancers and whether it would be better-tolerated than other PI3K pathway inhibitors being developed and/or evaluated in clinical trials. It would also be of interest to assess the effects of combining low doses of PDK1 and mTOR kinase inhibitors, as it might be envisaged that inhibiting both key upstream activators would be more effective at suppressing the actions of AGC kinases in cancer than employing PDK1 or mTOR inhibitors individually. Despite the complications of GSK2334470 not completely inhibiting Akt activity under conditions of high PI3K pathway activation, this compound will be a very useful research tool to probe signalling responses downstream of PDK1 and represents a useful addition to our armoury of effective signal transduction inhibitors to dissect biological roles of protein kinases.

AUTHOR CONTRIBUTION

Ayaz Najafov performed all of the experiments shown with the exception of the kinase profiling panels (Tables 1 and 2) and Figure 2. Eeva Sommer performed the experiments in Figure 2. Jeffrey Axten and Phillip DeYoung were involved in the discovery and development of GSK2334470. Ayaz Najafov and Dario Alessi planned the experiments, analysed the experimental data and wrote the manuscript.

ACKNOWLEDGEMENTS

We are grateful to Juan M. Garc´ıa-Mart´ınez, Stephan Wullschleger, Laura Pearce, Nick Leslie, Alexander Gray and Ian Batty for valuable discussions. We thank the staff at the National Centre for Protein Kinase Profiling (www.kinase-screen.mrc.ac.uk) for undertaking the kinase specificity screening, the Sequencing Service (School of Life Sciences, University of Dundee, Dundee, Scotland, U.K.) for DNA sequencing, and the protein production and antibody purification teams [Division of Signal Transduction Therapy (DSTT), University of Dundee, Dundee, Scotland, U.K.] co-ordinated by Hilary McLauchlan and James Hastie for expression and purification of antibodies.

FUNDING

This work was supported by the Medical Research Council, and the pharmaceutical companies supporting the Division of Signal Transduction Therapy Unit (AstraZeneca, Boehringer-Ingelheim, GlaxoSmithKline, Merck-Serono and Pfizer).

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