Abstract
The IκB kinase (IKK)/NF-κB pathway has been shown to be a major regulator in cell survival. However, the mechanisms through which IKK mediates cell death are not clear. In this study, we showed that IKK-β contributed to hydrogen peroxide (H2O2)-induced cell death independent of the NF-κB pathway. Our results demonstrated that the pro-death function of IKK-β under oxidative stress was mediated by p85 S6K1 (S6 kinase 1), but not p70 S6K1 through a rapamycin-insensitive and mammalian target of rapamycin complex 1 kinase-independent mechanism. We found that IKK-β associated with p85, but not p70 S6K1, which was required for H2O2-induced activation of p85 S6K1. IKK-β and p85 S6K1 contributed to H2O2-induced phosphorylation of Mdm2 (S166) and p53 accumulation. p85 S6K1 is critical for IKK-β-mediated cell death. Thus, these findings established a novel oxidative stress-responsive pathway that involves IKK-β, p85 S6K1 and Mdm2, which is response for H2O2-induced cell death. Our results have important implications for IKK-β and p85 S6K1 as potential targets for the prevention of diseases involved in oxidative stress-induced aberrant cell death.
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Main
Reactive oxygen species (ROS), such as hydrogen peroxide (H2O2), are generated in cells as a consequence of oxidative metabolism. Although low levels of ROS are usually detoxified quickly by antioxidant enzymes, an excessive accumulation of ROS may result in oxidative stress. High and/or persistent levels of oxidative stress represent a major cause of cellular damage and aberrant death in a plethora of pathological conditions during the initiation and progression of a plethora of pathological conditions, including neurodegenerative diseases, cancer, autoimmune and the ageing process.1 While ROS may trigger cell death through multiple mechanisms,2 recent studies have established the nuclear factor-κB (NF-κB) pathway as a critical signaling pathway in mediating the action of ROS in cell survival/cell death.3
The NF-κB protein is a transcription factor composed of two subunits, and in many cell types the predominant form is the p65/p50 heterodimer complex. Inactive NF-κB exists in the cytoplasm in association with an inhibitor protein, IκBα. Canonical activation of NF-κB requires signaling events that activate IκB kinase (IKK) complexes, which are composed of catalytic subunits (IKK-α/IKK-1 and IKK-β/IKK-2) and a regulatory subunit IKK-γ/NEMO (NF-κB essential modulator). An activated IKK phosphorylates IκB-α and releases NF-κB for activation.4 Activation of IKK/NF-κB pathway by exogenous H2O2 has been found to be cell type-dependent. In some cell lines, H2O2 activates the pathway,5, 6, 7, 8 whereas in other cells, it has an opposite effect.9 The pro-survival role of NF-κB pathway has been extensively characterized.3 However, in some cell lines, NF-κB has been shown to possess pro-cell death function.10, 11 A recent study demonstrated that NF-κB sensitized MEF cells to oxidative stress via caspase-independent pathway.12 However, the pro-death role of IKK under oxidative stress has not been reported, and the mechanisms by which IKK/NF-κB pathway promotes cell death remain to be defined.
The mammalian target of rapamycin (mTOR) is a serine/threonine kinase and the catalytic subunit of two distinct complexes called mammalian target of rapamycin complex (mTORC)1 and mTORC2. Macrolides rapamycin allosterically inhibits the activity of mTORC1. The mTOR signaling pathway serves as a central regulator of cell metabolism, growth, proliferation, ageing and survival by integrating both intracellular and extracellular signals such as growth factors, nutrients, energy and stresses.13
One of the key effectors of the mTORC1 signaling pathway is S6 kinase 1 (S6K1), which has important roles in cell growth, cell survival and lifespan.14, 15 S6K1 exists in two isoforms, p70 and p85. The p85 form differs from p70 by an N-terminal addition of 23 amino acids, which has been shown to function as a nuclear localization signal for targeting p85 S6K1 to the nucleus. p70 S6K1, which lacks the sequence, is mainly cytoplasmic.16, 17 Phosphorylation at position T389 of p70 or the equivalent site in p85 (T412) is required for a full and sustained activation of S6K1. Consequently, the extent of S6K1 (T389/412) phosphorylation in cells is routinely used as a surrogate for mTORC1 signaling activity.18, 19 It has been shown that p70 and p85 S6K1 are concordantly activated by growth factors and nutrients in a rapamycin-sensitive manner;18 however, most of the previous studies focus on p70 S6K1, and little is known about p85 S6K1 regulation and function.
In the present study, through investigating the roles of IKK and mTORC1-S6K1 in the cell death induced by chronic H2O2 insult, we have identified IKK-β as a mediator of cell death independent of the canonical NF-κB pathway during oxidative stress and uncovered a novel signaling mechanism that is responsible for H2O2-induced phosphorylation of Mdm2 (S166), p53 stabilization and cell death. The unexpected function of IKK-β-p85 S6K1 not only presents a mechanism for aberrant cell death induced by chronic insult with high levels of ROS under pathological conditions, but also links two of the major pathways that control cell growth/proliferation and cell death/survival.
Results
IKK- β contributes to hydrogen peroxide-induced cell death via a NF- κ B-independent pathway
To determine the function of IKK in ROS-induced cell death, we examined the effects of IKK inhibition and overexpression on cell death, following H2O2 exposure. We found that H2O2 treatment caused breast cancer MCF-7 cell death in a dose- and time-dependent manner (Figures 1a and b). H2O2 at a concentration of 1 mM was used in the subsequent experiments, which induced significant (51.9%) cell death within 36 h (Figure 1a). Interestingly, knockdown of IKK-β, but not IKK-α remarkably prevented MCF-7 cells from H2O2-induced cell death (Figures 1c and d). Moreover, pretreatment of MCF-7 cells with IKK-specific inhibitors, Bay 11-7082 or wedelolactone, significantly (P<0.05) attenuated H2O2-induced MCF-7 cell death (Figure 1e). To further confirm the pro-death role of IKK-β, we expressed HA-IKK-α or HA-IKK-β in MCF-7 cells and found that IKK-β, but not IKK-α, overexpression sensitized MCF-7 cells to H2O2-induced cell death (Figure 1f). The preventive effect of IKK-β knockdown for H2O2-induced cell death was also observed in other cell lines such as HeLa and HCT-116 cells (Supplementary Figure 1). These results suggest that IKK-β is critical for H2O2-induced cell death.
As NF-κB functions downstream of IKK-β, we then tested whether NF-κB mediated the effect of IKK-β on H2O2-induced cell death. Surprisingly, proteasome inhibitor MG132, which inhibits NF-κB translocation and activation by preventing the degradation of IκB-α,20 did not decrease H2O2-induced cell death (Figure 1g). Moreover, p65 siRNA, was also unable to impair H2O2-induced MCF-7 cell death (Figure 1h). Downregulation of IKK-α/β or p65 by siRNA and inhibitors (1 or 3 μM of Bay 11-7082, 5 or 10 μM of wedelolactone and 250 or 500 nM of MG132) did not induce significant cell death in the absence of H2O2 (Figure 1c and Supplementary Figure 2). These observations suggest that classical NF-κB pathway is not required for IKK-β-mediated cell death during oxidative stress.
Taken together, these findings indicate that IKK-β mediates H2O2-induced cell death independent of the canonical NF-κB-pathway.
p85 S6K1 potentiates hydrogen peroxide-induced cell death via a rapamycin-insensitive mechanism
The mechanisms through which IKK-β mediates H2O2-induced cell death were further investigated. Recent reports show that multiple proteins distinct from IκB proteins are phosphorylated by IKK-α or IKK-β.21 IKK-β has been found to mediate tumor necrosis factor-α (TNF-α)-stimulated mTORC1-S6K1 signaling activity by phosphorylating tuberous sclerosis complex 1.22 Although the pro-survival role of mTORC1-S6K1 has been well established,23, 24 a few recent studies reported a pro-cell death function of mTORC1-S6K1 in response to endoplasmic reticulum stress or genotoxic agents (doxorubicin)-induced DNA damage in MEFs.25, 26, 27
To investigate the possible role of mTORC1-S6K1 in IKK-mediated cell death under oxidative stress, the effect of mTORC1 inhibition on H2O2-induced cell death was examined in MCF-7 cells. Unexpectedly, rapamycin treatment failed to prevent the cell death induced by either H2O2 or HA-IKK-β overexpression (Figure 2a). Similarly, mTORC1 downregulation by mTOR or Raptor siRNA (Figure 2b) was also unable to inhibit the H2O2-induced cell death, suggesting that mTORC1 is not required for IKK-β-mediated cell death under oxidative stress. Moreover, depletion of ras homolog-enriched brain (Rheb), a key upstream activator of mTORC1, strongly decreased P-S6 (S235/236) levels, but exerted no significant effect on H2O2-induced cell death (Figure 2c). In contrast, S6K1 siRNA dramatically repressed H2O2-induced cell death (Figures 2d and e). The protective effect of S6K1 knockdown on H2O2-induced cell death was also observed in HeLa and HCT-116 cells (Supplementary Figure 3). As S6K1 siRNA could reduce the levels of both p70 S6K1 and p85 S6K1, we surmised that p85, but not p70 S6K1, might have a role in the H2O2-induced cell death. Accordingly, we examined the effects of p70 S6K1 or p85 S6K1 overexpression on H2O2-induced cell death. Overexpression of p85, but not of p70 S6K1, drastically enhanced H2O2-induced cell death (Figure 2f). This observation demonstrates a distinct function of p85 S6K1 in oxidative stress-induced cell death, and suggests that p85, but not p70 S6K1, promotes cell death via a rapamycin-insensitive and mTORC1-independent mechanism under oxidative stress.
Hydrogen peroxide activates p85 S6K1 through a rapamycin-insensitive mechanism
Different roles of p70 and p85 S6K1 in H2O2-induced cell death indicates that these two isoforms may be differentially regulated. We hence examined the activation of p70 and p85 S6K1 in response to various signals that are known to simulate mTORC1 activity. Consistent with the previous findings, nutrients (amino acids) or insulin strongly stimulated the phosphorylation of T389 on p70 and T412 on p85 S6K1 in MCF-7 cells starved for amino acids or serum. The insulin and nutrient-stimulated phosphorylation was completely blocked by pre-treating the cells with rapamycin (Figure 3a). Treating the cells with inflammatory factor TNF-α also induced the phosphorylation. However, while the TNF-α-stimulated phosphorylation at T389 of p70 was inhibited by rapamycin, the phosphorylation on T412 of p85 was insensitive to the drug (Figure 3b). Similarly, H2O2 stimulated the phosphorylation on T412 of p85, but not T389 of p70 S6K1. The H2O2-induced phosphorylation was also insensitive to rapamycin and Pp242, which is an ATP site-specific inhibitor of mTOR that inhibits both mTORC1 and mTORC2 (Figures 3b and c). These findings suggest that activation of p85 S6K1 by H2O2 is independent of mTOR kinase. As mitogen-stimulated mTORC1 and S6K1 activation requires the presence of nutrient, we further examined whether H2O2 was able to stimulate phosphorylation of p85 at T412 in cells starved for amino acids or treated with rapamycin. As shown in Figure 3d and Supplementary Figure 4, H2O2 increased phosphorylation of p85 (T412), but not that of p70 S6K1 (T389) in amino acids-starved or rapamycin-treated MCF-7, HeLa and HCT116 cells (Figure 3d and Supplementary Figure 4). 4E-BP1, another downstream target of mTORC1, had similar response to that of p70 S6K1 (Supplementary Figure 5).
S6 is the first identified and the most important p70/p85 S6K1 substrate. It has been well established that phosphorylation of S6 on S235/236 correlates with its function in protein synthesis and cell-size control.28 We further determined whether H2O2 was able to stimulate phosphorylation of S6 (S235/236) in the presence of rapamycin. We found that H2O2 dose- and time-dependently increased the phosphorylation in rapamycin-treated MCF-7 and HCT-116 cells (Figures 3b and c and Supplementary Figure 6). An in vitro S6K kinase assay revealed that ectopically expressed p85, but not p70, S6K1 purified from rapamycin-pretreated and H2O2-stimulated MCF-7 cells phosphorylated GST-S6 (S235/236) in vitro (Figure 3e). Consistent with this result, overexpressing p85, but not p70 S6K1, enhanced the H2O2-stimulated phosphorylation of S6 (S235/236) in cells (Figure 3f). Taken together, these results suggest that H2O2 activates p85, but not p70 S6K1, through an mTOR kinase-independent mechanism.
IKK- β is required for the rapamycin-insensitive activation of p85 S6K1 under oxidative stress
We further investigated the mechanisms of H2O2-induced rapamycin-insensitive activation of p85 S6K1. IKK is a major downstream kinase in the H2O2 and TNF-α signaling pathway,6 and has been shown to regulate mTORC1-S6K1.22, 29, 30, 31 Indeed, H2O2 stimulated the phosphorylation of IKK-α/β (S176/180) and degradation of IκB-α in MCF-7 cells (Figure 4a). To determine the role of IKK in H2O2-stimulated p85 S6K1 activation, we used chemical inhibitors or siRNA to block IKK activity. We found that IKK-specific inhibitor wedelolactone, but not PI-3K inhibitor Ly294002, decreased H2O2-stimulated p85 S6K1 (T412) and S6 (S235/236) phosphorylation in the presence of rapamycin (Figure 4b and Supplementary Figure 7). Furthermore, downregulation of IKK-β, but not IKK-α, prevented H2O2-stimulated phosphorylation of p85 S6K1 (T412) (Figure 4c). These results suggest that IKK-β is required for the rapamycin-insensitive activation of p85 S6K1.
Association of IKK- β with p85 S6K1 is required for H2O2-induced p86 S6K1 activation
The requirement of IKK-β in H2O2-induced p85 S6K1 activation raised a possibility that IKK-β may interact with and phosphorylate p85 S6K1 directly. Indeed, we found that ectopically expressed IKK-β was able to co-immunoprecipitate with p85, but not p70, S6K1 (Figure 5a). Furthermore, the association between IKK-β and p85-S6K1 was enhanced upon H2O2 stimulation (Figure 5a). The association was further validated by Co-IP of endogenous IKK-β with p85 S6K1 (Figure 5b). In addition, immunofluoresence staining confirmed that these two proteins co-localized in the cytoplasm of the cells (Supplementary Figure 8). The cytoplasmic and nuclear localization of both p85 and p70 S6K1 was further confirmed by fluorescence analysis of exogenously expressed pEGFP-or flag-tagged p70 and p85 S6K1 and nuclear-cytoplasmic fractionation analysis of endogenous p70 and p85 S6K1 (Supplementary Figure 9).
We next performed IKK-β in vitro kinase assay to examine whether IKK-β was able to phosphorylate p85 S6K1 directly. Our result showed that although IKK-β purified from H2O2-treated MCF-7 cells phosphorylated GST-IκB-α (S32/36), it was ineffective for phosphorylation of bacterial-expressed and purified his-p85 S6K1 (T412) or his-p70 S6K1 (T389) in vitro (Figure 5c). This finding indicates that alternative kinase other than IKK-β may direct the H2O2-induced phsophorylation of p85 S6K1.
A recent study has shown that IKK-β acts as an adaptor protein for IκB-α degradation independently of its kinase activity in UV-induced NF-κB activation.32 IKK-β brings β-TrCP to IκB-α through interaction with β-TrCP via its N-terminal kinase domain and with IκB-α via C-terminal regulatory region, leading to IκB-α ubiquitinaiton and degradation.32 However, we found that neither the kinase-dead IKK-β mutant (IKK-β KD) nor the C-terminal regulatory region (291–756 aa) and the N-terminal kinase domain (1–308 aa) of IKK-β were able to associate with p85 S6K1 and stimulate p85 S6K1 phosphorylation upon H2O2 exposure (Figures 5d and e). Furthermore, knockdown of IKK-γ, a regulatory component of IKK complex essential for IKK-β kinase activity and activation of the classical IKK/NF-κB pathway, also repressed p85 S6K1 phosphorylation and MCF-7 cell death following H2O2 exposure (Supplementary Figure 10). These findings suggest that both the kinase activity of IKK-β and the association of p85 S6K1 with IKK-β are required for the activation of p85 S6K1 by H2O2.
IKK- β mediates hydrogen peroxide-induced cell death via activation of p85 S6K1-Mdm2-p53 pathway
Mdm2 is an E3 ligase, which mainly ubiquitinates p53 in the nucleus and promotes p53 nuclear export and degradation.33 It has been shown recently that mTORC1-S6K1 mediated MEF cell death in response to doxorubicin-induced DNA damage by phosphorylation of Mdm2 at S163 (mouse), and inhibited its nuclear entry, which prevented Mdm2-mediated p53 ubiquitination and inducing p53 accumulation.25 Interestingly, H2O2 also dose-dependently stimulated phosphorylation of Mdm2 on S166 (human) in MCF-7 cells, an equivalent site to S163 in mouse (Figure 6a). Even though the basal level of phosphorylated Mdm2 (S166) was slightly decreased by rapamycin treatment, the H2O2-induced phosphorylation was rapamycin-insensitive (Figure 6a). Moreover, knockdown of IKK-β or S6K1 by siRNA suppressed the phosphorylation (Figure 6b), suggesting critical roles of IKK-β and S6K1 in the H2O2-stimulated Mdm2 (S166) phosphorylation. This notion was further confirmed by the observation that overexpression of IKK-β and p85 S6K1, but not p70 S6K1, significantly increased the levels of phosphorylated Mdm2 (S166) (Figure 6c). These findings demonstrate a requirement of IKK-β and p85 S6K1 in H2O2-induced, rapamycin-insensitive phosphorylation of Mdm2 (S166).
We further examined the effect of H2O2 on p53 induction and possible roles of IKK-β and p85 S6K1 in regulation of p53. H2O2 treatment caused a time-dependent increase of p53 protein level (Figure 7a). The induction of p53 by H2O2 was suppressed in cells pre-treated with IKK-specific inhibitor wedelolactone, but not in those treated with rapamycin (Figure 7a). Consistently, IKK-β or S6K1 knockdown impaired the H2O2-induced p53 accumulation (Figure 7b). These observations suggest that IKK-β and p85 S6K1 are required for the H2O2-stimulated p53 induction.
To determine whether activation of p85 S6K1 and induction of p53 is required for IKK-β-mediated cell death, we next examined the effect of p85 S6K1 knockdown or overexpression on IKK-β-mediated cell death. As expected, downregulation of S6K1 prevented the cell death induced by IKK-β overexpression (Figure 7c), whereas overexpression of p85 S6K1, but not p70 S6K1, reversed the protective effect of the IKK-β knockdown (Figure 7d). Most importantly, p53 siRNA inhibited cell death induced by H2O2, but repressed the protective effects of IKK-β or S6K1 knockdown (Figure 7e), suggesting an important role for p53 in IKK-β- and S6K1-mediated cell death under oxidative stress.
Collectively, these results support a model that IKK-β mediates H2O2-induced cell death via activation of p85 S6K1-Mdm2-p53 signaling pathway.
Discussion
Activation of IKK-β has been generally viewed as a major contributor to cell survival and proliferation. However, in the present study, we show that IKK-β also possesses a pro-death function that is independent of its role in regulation of NF-κB. Our findings suggest that the pro-death function of IKK is mediated by p85 S6K1, which in response to oxidative stress, phosphorylates Mdm2 (S166) and induces p53 accumulation.
Activation of the mTORC1 pathway is generally involved in cell survival and proliferation.23, 33, 34 However, several recent studies demonstrate a pro-apoptotic role of the pathway.25, 26, 27 In primary neuron and HeLa cells, mTORC1 was found to promote apoptosis induced by various toxic stimuli.27 Similarly, in MEF cells, a reduced mTORC1 activity by expression of tuberous sclerosis complex was able to protect the cells from endoplasmic reticulum stress-induced apoptosis. Interestingly, in the latter case, the protective effect of mTORC1 appeared to be insensitive to rapamycin.26 A recent study into the mechanism underlying the pro-apoptotic role of mTORC1 identified Mdm2 as a direct target of S6K1, which interacts with and phosphorylates Mdm2 at S163, causing Mdm2 cytoplasmic retention and p53 accumulation in response to genotoxic stress in MEFs.25 Although some studies showed that phosphorylation of Mdm2 at S163 promoted Mdm2 nuclear import, others failed to observe such a phenomenon.35, 36, 37, 38, 39 This mTORC1-enhanced S6K1–Mdm2 complex formation and S6K1-mediated Mdm2 phosphorylation are hence believed to be responsible for the pro-apoptotic role of mTORC1 under genotoxic stress conditions. However, the pro-death effect of mTORC1 appeared to be cell specific, as it was not observed in some cancer cell lines, including HeLa and HCT116.25, 40, 41 In the present study, we found that S6K1 knockdown protected the cells from H2O2-induced cell death in MCF-7, HeLa and HCT116. The pro-death effect of S6K1 in MCF-7 cells was independent of mTORC1, because neither rapamycin treatment nor knockdown of mTOR, Raptor and Rheb protected the cells from oxidative stress-induced cell death. Instead, we found that activation of p85, but not p70 S6K1, was responsible for the H2O2-induced cell death. Our results demonstrate that p85 S6K1, upon activation, phosphorylates Mdm2 at S163 and promotes p53 accumulation. This p53-dependent mechanism is likely to underlie the pro-death role of p85 S6K1 during oxidative stress and may help to explain the mTORC1-independent role of S6K1 in doxorubicin-induced cell death observed in previous studies.25, 40, 41
Both p70 and p85 S6K1 are downstream effectors of mTORC1. Previous studies have demonstrated that the two isoforms are concordantly activated in an mTORC1-dependent manner.42, 43 But a recent report has demonstrated that p85 S6K1, but not p70 S6K1, could be activated by phosphatidic acid in an mTORC1/rapamycin-independent way.44 p85 S6K1 was also previously found to primarily localize to the nucleus.17, 45 However, recent studies have shown that this kinase also functions in the cytoplasm.46, 47 Consistent with these recent observations, we found that p85 S6K1 exists predominantly in the cytoplasm. In addition, our results also indicate that the two isoforms can be differentially activated by TNF-α and H2O2 in an mTORC1-independent manner. Taken together, it is implicated that p70 and p85 S6K1 differ not only in localization, but also in regulation and function.
TNF-α and H2O2 treatments activate p85 S6K1 by inducing its phosphorylation at T412. This phosphorylation is blocked by inhibition of IKK or specifically knockdown of IKK-β, suggesting that the phosphorylation is mediated mainly by IKK-β. Although IKK has been implicated in mTORC1 regulation through direct phosphorylation of tuberous sclerosis complex 1, we found that inhibition of mTOR by rapamycin or ATP-competitive kinase inhibitor has little effect on the TNF-α and H2O2-induced phosphorylation of p85 S6K1. This finding rules out the involvement of mTOR in the process. On the other hand, our finding that IKK-β associates with p85 S6K1 raises the possibility that IKK-β is able to directly phosphorylate p85 S6K1. Despite this finding, we are unable to detect a direct phosphorylation of p85 S6K1 (T412) by IKK-β in our in vitro kinase assay, which indicates that alternative kinases may direct the H2O2-induced phsophorylation of p85 S6K1. As a recent study has revealed IKK-β as an adaptor in UV-induced IκB-α ubiquitination,32 our results implicate that IKK-β may act as a scaffold protein to recruit other kinases that are responsible for phosphorylation of p85 S6K1 upon H2O2 stimulation. The kinase activity of IKK-β is required for its association with p85 S6K1 and the activation of p85 S6K1.
In summary, our study reveals a novel oxidative stress-responsive pathway that involves IKK-β, p85 S6K1, Mdm2 and p53. Through this novel pathway, the oxidative stimulus drives IKK-β to activate p85 S6K1 independent of mTORC1. The activated p85 S6K1 in turn induces cell death through a mechanism involving phosphorylation of Mdm2 and induction of p53. Our results demonstrating that IKK-β has a role in promoting cell death adds another level of complexity to IKK-β regulation and function, which should be taken into consideration when IKK inhibitors are used in therapeutic treatments.
Materials and Methods
Chemicals and antibodies
Chemicals used in the study include: Pp242 (Active Biochemicals, Hongkong, China); Bay 11-7082 and Wedelolactone (Calbiochem, Darmstadt, Germany); Rapamycin, MG132, insulin and human recombinant TNF-α (Sigma, St. Louis, MO, USA); LY294002 (Cell Signaling, Beverly, MA, USA).
The following antibodies were used: flag (cat# F1804) (Sigma); phospho-p70/85-S6K1 (T389/412) (cat# 9206), 4E-BP1 (cat# 9644), phospho-4E-BP1 (T37/46) (cat# 2855), phospho-S6 (S235/236) (cat# 4856), IKK-α (cat# 2682), IKK-β (cat# 2678), phospho-IKKα/β (S176/180) (cat# 2694), Raptor (cat# 2280) and P-Mdm2 (S166) (cat# 3521) (Cell Signaling); S6 (cat# 74459), actin (cat# 47778), mTOR (cat# 1549), p65 (cat# 71677), Mdm2 (cat# 965), p53 (cat# 74573), p70-S6K (cat# 8418) and GFP (cat# 101536) (Santa Cruz Biotechnology Inc., Santa Cruz, CA, USA); myc (cat# ALX-804-627) (Enzo Life Sciences, Farmingdale, NY, USA); Histone H2A.X (cat# BS2984) and β-tubulin (cat# BS1482) (Bioworld Technology Inc., Louis Park, MN, USA); Rheb (cat# 25873) (Abcam, Cambridge, UK); IKK-γ (cat# 18474-1-AP) (ProteinTech Group Inc., Chicago, IL, USA).
Plasmids and preparation of GST-S6 and His-P70/85 S6K1 proteins
HA-IKK-α, HA-IKK-β, myc-IKK-α, myc-IKK-β and IKK-β kinase-dead (IKK-β KD) vectors were kindly provided by Dr. Gutian Xiao (University of Pittsburgh School of Medicine, Pittsburgh, PA, USA). The sequences encoding the C-terminal (291–756 aa) and N-terminal (1–308 aa) of IKK-β were sub-cloned into pUSEamp(+) vector (myc-his tag).
To generate plasmids that express only p85 S6k1, the sequence for the N-terminal 23 amino acids of p85 S6K1 was added to rat p70-S6K1 cDNA (pRK-7-p70 S6K1) (Addgene, Cambridge, MA, USA) by PCR and the p70 S6K1 translation starting site (70–72th bp, ATG) was changed into TTG. Both p70 S6K1 and p85 S6K1 cDNAs were sub-cloned into pcDNA3.1-Flag, pEGFP-C1 and PET-28a vectors. Human 40S ribosomal protein S6 cDNA was obtained from HEK293 cells by RT-PCR and was sub-cloned into prokaryotic expression vector pGEX-6P-1(pGEX-6P-1-S6). GST-S6, His-p70 S6K1 and His-p85 S6K1 proteins were induced by isopropyl β-D-1-thiogalactopyranoside and purified using glutathoine-agarose or Ni-NAT agarose beads. Purified GST-S6 and His-p70/85 S6K1 proteins were used as substrates for S6K1 or mTORC1, IKK-β in vitro kinase assay.
Cell culture and transfection
MCF-7, HeLa, HEK293 and HCT116 cells were purchased from American Type Culture Collection (Manassas, VA, USA) and cultured in high glucose DMEM (Life Technologies Corporation, Carlsbad, CA, USA) supplemented with 10% FBS in a humidified atmosphere of 5% CO2. For transient transfection, HEK293 or MCF-7 cells were transfected with plasmid DNAs using lipofectamine 2000 (Invitrogen, Carlsbad, CA, USA) following the manufacturer’s instruction.
RNA interference
Negative control siRNAs, IKK-α, IKK-β, IKK-γ, mTOR, Raptor, Rheb, p53, p65 and p70/85 S6K1-specific siRNA were chemically synthesized by GenePharma Co., Ltd (Shanghai, China). The sequences of these siRNAs are the following:
IKK-α #1: 5′-GCAGGCUCUUUCAGGGACA-3′; IKK-α #2: 5′-CAAAGAAGCUGACAAUACU-3′;
IKK-β #1: 5′-CAGGUGAGCAGAUUGCCAU-3′; IKK-β #2: 5′-GGUGGAAGAGGUGGUGAGC-3′;
IKK-γ #1: 5′-ACAGGAGGUGAUCGAUAAG-3′; IKK-γ #2: 5′-AACAGGAGGUGAUCGAUAA-3′;
S6K1 #1: 5′-GGACUUCCGAGACAGGGAATT-3′; S6K #2: 5′-AAACACUCCUGCCAUGUCC-3′;
p53 #1: 5′-CAGTCTACCTCCCGCCATA-3′; p53 #2, 5′-GAAGAAACCACTGGATGGA-3′;
mTOR: 5′-GAGCCUUGUUGAUCCUUAATT-3′; Rheb: 5′-CGGGCAAGAUGAAUAUUCUTT-3′;
p65: 5′-GCCCUAUCCUUUACGUCA-3′.
Cells were transfected with the siRNAs at 60% confluence using lipofectamine 2000 (Invitrogen), following the manufacturer’s instructions.
Immunoprecipitation and western blot
To detect the association of endogenous IKK-β with p85 S6K1, MCF-7 cells grown in 6 cm dishes treated with rapamycin and H2O2 were rinsed twice with PBS, and lysed with 400 μl of ice-cold lysis buffer (40 mM HEPES, pH 7.5, 120 mM NaCl, 1 mM EDTA, 10 mM pyrophosphate, 10 mM glycerophosphate, 50 mM NaF, 1.5 mM Na3VO4, 1% Triton X-100, and 1 × EDTA-free protease inhibitors) on ice for 30 min, followed by centrifugation at 12 000 × g for 10 min. Supernatants were incubated with 4 μg of anti-IKK-β antibody overnight at 4 °C on a nutator, followed by addition of 30 μl of 50% slurry of protein G Sepharose (Amersham Phamacia, Cincinnati, OH, USA) beads for another 2 h. Beads were then washed four times with lysis buffer and used for immunoblotting analysis.
To detect the association of overexpressed myc-IKK-β with flag-p70/85 S6K1, HEK293 cells were grown in 6 cm dishes and co-transfected with myc-IKK-β wt, IKK-β KN, IKK-β (1–308) or IKK-β (291–756) and flag-p70/85 S6K1 plasmids. Twenty-four hours later, cells were treated and lysed, as described above, and lysates were precipitated with anti-myc antibody. Precipitated proteins were then analyzed by immunoblotting.
In vitro kinase assay for S6K1, mTORC1 and IKK- β
For S6K1 in vitro kinase assay, HEK293 cells transfected with flag-p70 or flag-p85 S6K1 were lysed with lysis buffer and lysates were incubated with anti-flag antibody for 3 h at 4 °C, followed by incubation with protein G Sepharose beads for another 2 h. Beads were washed four times with lysis buffer and once with kinase buffer (50 mM Tris-Cl, pH 7.4, 0.5 mM dithiothreitol, 10 mM MgCl2). Four micrograms of purified GST-S6 was added to a 20 μl kinase reaction mixture (10 mM ATP, 50 mM Tris-Cl, pH 7.4, 0.5 mM dithiothreitol, 10 mM MgCl2). After 30 min of incubation at room temperature, the reaction was stopped by the addition of 2 × SDS sample buffer followed by boiling for 5 min.
mTORC1 or IKK-β in vitro kinase assay were performed, as previously described.48 Endogenous mTORC1 was immunopurified from HEK293 cells. IKK-β was immunopurified from HEK293 cells transfected with myc-IKK-β. Cells were lysed in ice-cold buffer (40 mM HEPES (pH 7.4), 2 mM EDTA, 10 mM pyrophosphate, 10 mM glycerophosphate, 0.3% CHAPS, and one tablet of EDTA-free protease inhibitors (Roche, Basel, Switzerland) per 25 ml). Supernatants were incubated with anti-mTOR or myc antibody for 2 h at 4 °C, followed by addition of 30 μl of 50% slurry of protein G Sepharose beads for another 1 h. Beads were then washed four times with lysis buffer and once kinase buffer (mTORC1 kinase buffer: 25 mM HEPES (pH 7.4), 50 mM KCl, 10 mM MgCl2, 250 μM ATP; IKK-β kinase buffer: 20 mM HEPES (pH 7.7), 20 mM β-glycerophosphate, 10 mM MgCl2, 10 mM PNPP, 100 μM Na3VO4, 2 mM DTT, 1 mM ATP, 10 μg/ml approtonin, 50 mM NaCl). Four micrograms of purified His-p70 S6K1, p85 S6K1 or GST-IκB-α (Millipore, Billerica, MA, USA) were added to 30 μl kinase buffer. Kinase assays were performed for 30 min at 30 °C, and terminated by the addition of the 2 × SDS sample buffer.
Cell viability analysis
After each treatment, the number of viable cells was counted by trypan blue dye exclusion using a hemocytometer. The dead cell ratio=trypan blue-stained cells/total cells × 100%.
Nuclear-cytoplasmic fractionation
Nuclear and cytosolic fractions were isolated as described previously.25 Briefly cultured cells were washed twice with cold PBS, lysed with ice-cold lysis buffer containing 10 mM Tris, pH 7.9, 10 mM KCl, 2 mM MgCl2, 0.1 mM EDTA and 0.7% Nonidet P-40. After incubation on ice for 10 min, lysates were centrifuged at 500 × g for 5 min. The supernatant was collected as the cytosolic fraction, and the pellet was re-suspended in buffer containing 40 mM Tris, pH 7.9, 350 mM NaCl, 2 mM MgCl2, 1 mM EDTA, 0.2 mM EGTA, 20% glycerol, 1% Nonidet P-40, 1 mM phenylmethylsulfonyl fluoride, 2 mM dithiothreitol, 2 μg/ml leupeptin and 1 μg/ml aprotinin on ice for 20 min and harvested by centrifugation at 12 000 × g for 10 min at 4 °C. The purity of the nuclear and cytosolic fractions was assessed by immunoblotting extracts and the isolated fractions with antibodies against nuclear protein Histone H2A.X and cytosol protein β-tubulin.
Immunofluorescence and confocal microscopy
Cells plated on chamber slides were fixed with 4% paraformaldehyde, permeabilized with 0.2% Triton X-100, and incubated with the primary antibody at 4 °C overnight. Chamber slides were subsequently incubated with fluorescein isothiocyanate (FITC)- or (tetramethyl Rhodamine Iso-thiocyanate) TRITC-conjucated secondary antibody for 1 h at room temperature. The slides were mounted in ProLong Gold Antifade Reagent with 4, 6-diamidino- 2-phenylindole dihydrochloride (DAPI) (Invitrogen) and imaged with a Nikon Eclipse E400 fluorescent microscope (Nikon Corporation, Tokyo, Japan).
Abbreviations
- IKK:
-
IκB kinase
- mTORC1:
-
mammalian target of rapamycin complex 1
- Mdm2:
-
murine double minute-2
- ROS:
-
reactive oxygen species
- IκB:
-
inhibitor of κB
- NF-κB:
-
nuclear factor-κB
- mTOR:
-
mammalian target of rapamycin
- S6K1:
-
S6 kinase 1
- NLS:
-
nuclear localization signal
- TNF-α:
-
tumor necrosis factor-α
- TSC:
-
tuberous sclerosis complex
- Raptor:
-
regulatory associated protein of mTOR
- Rheb:
-
ras homolog enriched brain
- PA:
-
phosphatidic acid
- siRNA:
-
short interfering RNA
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Acknowledgements
We thank Dr. Jian Yang and Dr. Richard T Tran for critical review of the paper. The work was supported by National Natural Sciences Foundation of China (30900555, 31000633 and 91029727), Program for Changjiang Scholars and Innovative Research Team in University (IRT1142) and the State Key Development Program for Basic Research of China (2009CB 918904).
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Jia, CH., Li, M., Liu, J. et al. IKK-β mediates hydrogen peroxide induced cell death through p85 S6K1. Cell Death Differ 20, 248–258 (2013). https://doi.org/10.1038/cdd.2012.115
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DOI: https://doi.org/10.1038/cdd.2012.115
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