Abstract
It is intriguing that some pan-caspase inhibitors such as zVAD-fmk (zVAD) are capable of inducing necrotic cell death in a selected group of cells. As earlier reports from our laboratory have ruled out the original notion that zVAD-induced necrosis in mouse fibrosarcoma L929 cells was autophagic cell death, the main objective of this study was thus to determine the underlying mechanism of this form of cell death. In this study, we provided clear evidence that zVAD-induced necroptosis in L929 cells and such cell death is dependent on autocrine production of tumor necrosis factor-α (TNFα) at the transcriptional level. More importantly, we identified that activating protein-1 (AP-1), but not nuclear factor κ-B, is the transcription factor controlling zVAD-induced TNFα transcription. Moreover, zVAD is able to activate AP-1 through activation of two upstream mitogen-activated kinases (MAPKs), c-Jun N-terminal kinase and extracellular signal-regulated kinase. Finally, we found that protein kinase C is the important upstream signaling molecule in mediating zVAD-induced activation of MAPKs and AP-1, and subsequent autocrine production of TNFα and cell death. Data from this study reveal the molecular mechanisms underlying zVAD-induced necroptosis, an important form of programmed necrotic cell death with increasing understanding of its biological significance in health and diseases.
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Main
On the basis of the morphological and biochemical features, programmed cell death (PCD) can be classified into three categories: apoptosis, autophagic cell death, and necrosis.1 The autophagic cell death has been described as a non-apoptotic cell death that is caused by excessive induction of autophagy2, 3 On the other hand, there are several types of programmed necrosis described in the literature, including necrosis induced by ATP depletion,4 and necroptosis initiated by engagement of death receptors with their corresponding ligands, such as tumor necrosis factor-α (TNFα).5
TNFα is a pleiotropic proinflammatory cytokine that is capable of triggering multiple signaling pathways to regulate various physiological and pathological cellular processes. One important biological function of TNFα is to induce apoptosis by the extrinsic pathway.6 On the other hand, TNFα has also been demonstrated to trigger programmed necrosis, or necroptosis, in a number of cell types.7, 8, 9, 10 The execution of necroptosis requires the kinase activity of receptor-interacting protein 1 (RIP1) and can be blocked by the RIP1 kinase inhibitor, necrostatin-1.9, 10, 11 At present, how RIP1 controls necroptosis is largely unknown. One possibility is that RIP1 may promote intracellular ROS production and c-Jun N-terminal kinase (JNK) activation by the activation of Nox1 NADPH oxidase.12 Recently, RIP3 has been identified as another crucial factor in TNFα-induced necrotic cell death by interacting with RIP1.8, 13, 14 In TNFα-mediated necroptosis, there is one intriguing observation: blockage of caspase cascade by either chemical inhibitors or overexpression of a viral caspase inhibitor (CrmA) greatly promotes the cell death.15, 16 The exact mechanisms underlying such a sensitization effect are not known. As caspase 8 has been shown to cleave RIP1 in TNFα signaling,17 one possibility is that suppression of the caspase cascade would enhance the RIP1 protein stability and then promote RIP1-mediated necroptosis.
Among many types of caspase inhibitors, zVAD-fmk (zVAD) is probably the most commonly used pan-caspase inhibitor. Interestingly, although zVAD has been demonstrated to be of low cytotoxicity to most of cell lines in vitro,18 it can induce robust necrotic cell death in certain cell lines, particularly in L929 cells.19, 20 Such necrosis was originally recognized as an autophagic cell death evidenced by a massive accumulation of the autophagic markers in the dying cells.19 However, our earlier works have provided compelling evidence that zVAD-induced cell death in L929 cells is not autophagy-dependent; instead, autophagy has a protective function for cell survival.20, 21 Therefore, the pro-death mechanism in zVAD-mediated necroptosis remains to be examined.
In this study, we demonstrate that autocrine production of TNFα is required for zVAD-induced necrotic cell death in L929 cells. Furthermore, zVAD-mediated autocrine production of TNFα is achieved by the activation of the protein kinase C (PKC)–mitogen-activated protein kinases (MAPKs)–activating protein-1 (AP-1) signaling pathway. Data from this study thus provide new insights into the molecular mechanisms underlying zVAD-induced necroptosis, an important form of PCD with increasing understanding of its biological significance in health and diseases.
Results
zVAD-fmk and BocD-fmk, but not QVD-oph, induce necrosis in L929 cells
zVAD-fmk (zVAD) is a well-established general caspase inhibitor to block apoptosis. Intriguingly, zVAD is also capable of efficiently inducing necrotic cell death in a selected group of cell types, particularly in L929 cells.19, 20 In this study, we first asked whether other caspase inhibitors possess the similar activity as zVAD for induction of necrosis. As shown in Figure 1a, among the caspase inhibitors tested, only zVAD-fmk and BocD-fmk were able to induce evident cell death in L929 cells. Interestingly, QVD-oph, another pan-caspase inhibitor that has been reported to be more efficient and of broader-spectrum than zVAD-fmk and BocD-fmk for caspase inhibition,22 was unable to induce cell death (Figure 1a). The effectiveness of all these caspase inhibitors was confirmed by their inhibitory effects on TNF-related apoptosis-inducing ligand (TRAIL)-induced cleavage of caspase 8, caspase 3, and poly(ADP-ribose)polymerase-1 (PARP-1) in L929 cells (Figure 1b). Among the caspase inhibitors tested above, the fmk group has been demonstrated to be much more cytotoxic than oph.18 We thus tested whether it is the fmk group that confers zVAD-fmk and BocD-fmk the killing ability. First, we found that neither zFA-fmk (a non-caspase inhibitor carrying fmk group) alone nor zFA-fmk plus QVD-oph induces cell death (data not shown). Next, the two caspase 8 inhibitors with different tags, IETD-fmk and IETD-oph, were found to induce marginal necrosis in L929 cells (Figure 1a). Moreover, at the same concentration, IETD-oph was slightly more toxic than IETD-fmk (Figure 1a). These results therefore negate the possibility that it is the fmk group leading to the cell death.
In an earlier report, the killing ability of zVAD was attributed to its caspase 8 inhibition effect.19 In this study, we further examined this by overexpression of CrmA, a viral protein known to specifically inhibit caspase 8.23 As shown in Figure 1c, overexpression of CrmA (indicated by co-transfected GFP fluorescence) in L929 cells led to no cell death, whereas CrmA greatly enhanced cell death in the cells treated with exogenous TNFα, being consistent with earlier observations.16 Furthermore, knockdown of caspase 8 or fas-associated death domain (FADD) did not kill L929 cells (Supplementary Figure S1b), while effectively suppressed TRAIL-induced caspase 3 and PARP-1 cleavage, and apoptosis (Supplementary Figure S1a, S1b). Taken together, all these findings clearly suggest that inhibition of caspase 8 alone is not sufficient for zVAD to induce cell death in L929 cells.
zVAD-induced necrotic cell death requires de novo protein synthesis
To further understand the mechanisms underlying zVAD-induced cell death, we then tested whether de novo gene transcription and protein synthesis are required for such cell death. As shown in Figure 1d, actinomycin D (ActD) or cycloheximide (CHX) offered perfect protection against zVAD-induced cell death. In contrast, ActD or CHX markedly enhanced TNFα-induced cell death in L929 cells (data not shown), indicating that their protective effect is specific to zVAD-induced cell death. These results thus suggest that zVAD-induced necrotic cell death requires de novo gene transcription and protein synthesis.
Another interesting and accidental finding is that the volume of cell culture medium affects zVAD-induced cell death. As shown in Figure 1e, when L929 cells were cultured in different volume of medium containing the same final concentration of zVAD (10 μM), the cell death was found to be mitigated by increasing medium volume. In contrast, alterations of medium volume did not affect cell death induced by exogenously administered TNFα (Figure 1e). It is thus possible that some newly synthesized proteins are secreted into the medium to trigger the cell death signaling pathway.
zVAD-induced cell death is RIP1- and RIP3-dependent
It has been well-established that RIP1 has a critical function in TNFα-induced necroptosis and that necrostatin-1, a specific RIP1 kinase inhibitor, can suppress necroptosis.24 In this study, necrostatin-1 was found to be effective in suppressing cell death induced by zVAD, similar to that induced by TNFα, but not in MNNG-induced necrosis which has been reported to be mediated by PARP-1 overactivation (data not shown). On the other hand, RIP3 has recently been identified as a key modulator in TNFα-induced necroptosis.8, 13, 14 In this study, we also tested whether RIP3 is involved in zVAD-fmk-induced cell death. As shown in Supplementary Figure S2, knockdown of RIP3 significantly reduced cell death induced by zVAD or TNFα, while displayed no effect on TRAIL-induced apoptosis. It is thus believed that zVAD-induced cell death is similar to TNFα-induced necroptosis involving both RIP1 and RIP3.
zVAD promotes autocrine production of TNFα
L929 cells are well known to produce a variety of cytokines, including TNFα.25 Moreover, autocrine production of TNFα has been recently recognized as a critical signal for the induction of apoptosis in response to Smac-mimetics or IAP antagonists.26, 27, 28 In this study, we hypothesized that autocrine production of TNFα is involved in zVAD-induced necrotic cell death. A very low basal level of TNFα (around 3 pg/ml) was detected in the medium (Figure 2a), while the TNFα level was markedly increased upon zVAD treatment for 8 h (Figure 2b). The drop of TNFα concentration at 24 h-time point was probably due to cell death as shown earlier. Meanwhile, pretreatment with CHX totally abrogated the autocrine production of TNFα (Figure 2b). Next, we checked TNFα mRNA level using RT-PCR. As shown in Figure 2c, there was a higher level of TNFα mRNA in zVAD-treated cells than that in control cells. More importantly, both zVAD-fmk and BocD-fmk, but not QVD-oph, enhanced the transcription of TNFα (Figure 2c) and accordingly, autocrine production of TNFα in the medium (Figure 2d). Such findings are also consistent with the pattern of cell death induced by these caspase inhibitors as shown in Figure 1a.
Blockage of TNFα signaling suppresses zVAD-induced necroptosis
To test whether zVAD-induced autocrine production of TNFα, as shown above, is required for cell death, we first intercepted the TNFα signaling by blocking TNFα receptor 1 (TNFR1) using a TNFR1 blocking antibody. It is to be noted that this antibody dose-dependently suppressed zVAD-induced cell death (Supplementary Figure S3a). As expected, this antibody also prevented exogenous TNFα-induced cell death, without showing any protection against TRAIL-induced apoptosis in L929 cells (Supplementary Figure S3a). Moreover, a TNFα-neutralizing antibody that specifically neutralizes the TNFα ligand in culture medium also ablated zVAD-induced cell death dose-dependently (Supplementary Figure S3b). In an attempt to seek further supporting evidence, we next used XENP1595, a DN-TNF protein against soluble TNFα as reported previously.29 As shown in Supplementary Figure S3c, XENP1595 offered perfect protection against cell death induced by zVAD and exogenous TNFα. Collectively, these data clearly demonstrate that zVAD-induced necrotic cell death in L929 cells is necroptosis that depends on autocrine production of TNFα. Remarkably, such findings are consistent with a recent report in which autocrine production of TNFα was identified, through a genome-wide RNAi library screening, to be required for zVAD-induced cell death in L929 cells.30
Nuclear factor-κB (NF-κB) pathway is not involved in zVAD-induced autocrine production of TNFα, but has a protective function during zVAD-induced necroptosis. It is known that both canonical and non-canonical NF-κB pathways are implicated in autocrine production of TNFα in cancer cells.26, 28 In this study, we investigated whether NF-κB pathway is involved in zVAD-induced autocrine production of TNFα. We first silenced I-κB kinase (IKKβ) and IKKα, the two key upstream kinases of NF-κB. The IKKβ and IKKα knockdown efficiency was shown in Figure 3a. Disruption of the canonical NF-κB pathway by targeting IKKβ markedly sensitized L929 cells to zVAD-induced cell death, whereas silencing the non-canonical pathway by targeting IKKα did not significantly affect cell death (Figure 3b). We next disrupted the canonical and non-canonical NF-κB pathways by directly silencing their key components, RelA and RelB, respectively. The knockdown efficiency is shown in Figure 3c. Knockdown of RelA also greatly sensitized L929 cells to necroptosis induced by zVAD (Figure 3d), being consistent to the data from knockdown of IKKβ (Figure 3b). Finally, we found that knockdown of RelA or RelB failed to block the autocrine production of TNFα (Figure 3e). It is thus believed that neither the canonical nor the non-canonical NF-κB pathway contributes to zVAD-induced TNFα transcription, and the canonical NF-κB pathway acts as a prosurvival mechanism to ablate zVAD-induced cell death.
AP-1 activitation is required for zVAD-induced autocrine production of TNFα and cell death
In addition to NF-κB, another important transcription factor, AP-1, has been implicated in TNFα transcription.32 We thus attempted to elucidate the possible role of AP-1 in zVAD-mediated autocrine production of TNFα and subsequent necroptosis. As c-Jun is one of the essential components of AP-1, we first examined the effects of c-Jun knockdown on AP-1 activity, TNFα transcription, and cell death. The knockdown efficiency is shown in Figure 4a. Silencing of c-Jun significantly ablated AP-1 luciferase activity in the cells treated with zVAD (Figure 4b) and reduced TNFα mRNA transcription (Figure 4c). As expected, knockdown of c-Jun dramatically suppressed zVAD-induced cell death in L929 cells (Figure 4d). Therefore, this set of data strongly implies that AP-1 is responsible for zVAD-stimulated TNFα transcription.
zVAD-induced AP-1 activation is mediated by JNK and ERK
Next, we sought to explore the upstream signaling pathways mediating zVAD-induced AP-1 activation, by focusing on mitogen-activated protein kinases (MAPKs). First, zVAD treatment was found to activate c-Jun (Figure 5a). Second, zVAD was able to enhance the phosphorylation of JNK and extracellular signal-regulated kinase (ERK), the two important MAPKs upstream of AP-1 (Figure 5a). As TNFα is also known as a activator of MAPKs and c-Jun;33 it is thus possible that the activation of JNK, ERK, and c-Jun is triggered by autocrine production of TNFα, but not by zVAD per se. To exclude this possibility, we treated the cells with TNFα-neutralizing antibody to block the secreted TNFα function and found that zVAD was still capable of activating JNK, ERK, and c-Jun (Figure 5b), suggesting that zVAD-activated MAPKs is independent of autocrine production of TNFα. To further test whether JNK and ERK are the upstream molecules mediating AP-1 activation upon zVAD treatment, we next used two chemical inhibitors, SP600125 (SP) and PD98059 (PD), to inhibit JNK and ERK activation, respectively. As shown in Figure 5c, these two inhibitors almost completely abrogated zVAD-induced phosphorylation of JNK and ERK, as well as that of c-Jun. As a result, they blocked zVAD-induced AP-1 activation as determined by the AP-1 luciferase assay (Figure 5d). As expected, these inhibitors dramatically suppressed the autocrine production of TNFα (Figure 5e) and eventually offered perfect protection against zVAD-induced necroptosis in L929 cells (Figure 5f). Therefore, data from this part of the study clearly demonstrate that the MAPKs-mediated AP-1 activation is required for zVAD-induced autocrine production of TNFα and subsequent necroptosis.
PKC has a critical function in zVAD-mediated MAPKs-AP1 activation, autocrine production of TNFα, and cell death
After establishing the role of MAPKs (JNK and ERK) in zVAD-induced TNFα transcription, here we sought to find the upstream mechanism mediating zVAD-induced MAPKs activation. It has been well established that PKC is one of the important signals upstream of MAPKs.34 Therefore, we examined whether zVAD is able to activate MAPKs by PKC. First, zVAD was found to evidently activate PKC, similar to the effect of 12-O-tetradecanoylphorbol-13-acetate (TPA), as determined by phosphorylation of the total PKC substrate (Figure 6a). A PKC inhibitor (PKCi, bisindolylmaleimide I) was able to completely inhibit both reactions. Importantly, TPA enhanced, whereas PKCi effectively suppressed, zVAD-induced phosphorylation of JNK, ERK, and c-Jun (Figure 6b), suggesting that PKC acts upstream of JNK and ERK, leading to AP-1 activation. Consistently, TPA was found to promote TNFα transcription and secretion (Figure 6c and d). Moreover, TPA further enhanced, whereas PKCi almost completely blocked, zVAD-induced TNFα autocrine production (Figure 6c and d). As expected, TPA markedly increased, whereas PKCi perfectly protected against, zVAD-induced cell death. Interestingly, TPA and PKCi modulated exogenously administered TNFα-induced necroptosis in an opposite pattern to their effects on zVAD-induced necroptosis (Figure 6e). These results suggest that activation of PKC can enhance zVAD-induced necroptosis by promoting autocrine production of TNFα, without affecting the downstream TNFα signaling pathways.
To further understand the involvement of PKC in zVAD-induced necroptosis as demonstrated above, we compared the effects of different pan-caspase inhibitors on PKC activation. As anticipated, zVAD-fmk and BocD-fmk, but not QVD-oph, were capable of activating PKC, as well as JNK, ERK, and c-Jun (Figure 7a). This result prompted us to test whether activation of PKC would affect the effect of QVD-oph on L929 cells. Interestingly, TPA indeed effectively turned QVD-oph into a cell killer (Figure 7b), while it has no effect on DEVD-cho (caspase 3 inhibitor) (Figure 7b), indicating that inhibition of certain caspases by QVD-oph, but not by DEVD-cho, is critical for such cell death. Similarly, TPA was also effective for induction of necroptosis in cells with knockdown of caspase 8 (Figure 7c), whereas knockdown of caspase 8 per se is not cytotoxic (Supplementary Figure S1). Such observations thus suggest that both autocrine production of TNFα and inhibition of the caspase cascade are required for necroptosis induced by zVAD-fmk and BocD-fmk.
Discussion
In recent years, necrotic cell death has been increasingly appreciated as an important form of PCD. In contrast to apoptosis, the molecular mechanisms underlying necrosis is much less understood. Necrosis usually occurs in cells when the apoptosis machinery is suppressed or absent. zVAD-induced necrotic cell death is among several necrosis models established so far. In this study, we identified autocrine production of TNFα as the missing pro-death signal in zVAD-induced necrotic cell death or necroptosis. Such results are indeed consistent with a recent report in which TNFR1 and autocrine production of TNFα were found to be crucial for zVAD-induced necrosis in L929 cells.30 It is known that endogenously produced TNFα can be secreted into the extracellular environments or exists as a membrane-bound form, both of which are able to trigger downstream signaling, leading to cell death.35 It is to be noted that our data suggest that zVAD-fmk-induced necroptosis in L929 cells is predominantly executed by the secreted soluble TNFα, on the basis of the following observations: (i) the TNFα-neutralizing antibody, which can only neutralize the soluble TNFα in medium, attenuated zVAD-fmk-induced cell death (Supplementary Figure S3b) and (ii) blocking the soluble TNFα by the DN-TNF protein offered perfect protection against zVAD-fmk-induced cell death (Supplementary Figure S3c).
The major aim of this study is to understand the molecular mechanisms underlying zVAD-induced autocrine production of TNFα. It is known that the TNFα promoter region contains both NF-κB and AP-1 responsive elements.36 In cancer cells treated with the IAP antagonists, autocrine TNFα is produced by both the canonical and non-canonical NF-κB pathways.26, 28 In this study, we show that zVAD mainly uses the AP-1 pathway, but not the NF-κB pathway, to promote TNFα transcription (Figures 3 and 4). It is to be noted that such a notion is also supported by the finding in which, by using genome-wide RNAi library screening, Jun, but not NF-κB components, was identified as one of the critical functions involved in zVAD-induced necrosis.30 Moreover, we demonstrate that zVAD-induced AP-1 activation in L929 cells is mediated by the activation of MAPKs including JNK and ERK (Figure 5). These data are indeed consistent with recent reports that TNFα expression was regulated by JNK32 or ERK.37 Therefore, it appears that the transcriptional machinery for TNFα expression is cell type and stimulus specific.
One important finding in this study is that PKC acts upstream of MAPKs to promote autocrine production of TNFα in response to zVAD. The PKC family is an important group of proteins with diverse functions in many cellular processes such as cell proliferation, differentiation, and cell death.38 Among the three pan-caspase inhibitors tested in this study (zVAD-fmk, BocD-fmk, and QVD-oph), their effects on PKC activation, autocrine production of TNFα, and induction of cell death are highly correlated (Figures 1a, 2c, d, and 7a). Moreover, when combining with caspase inhibition, the typical PKC activator, TPA, was found to induce necroptosis in L929 cells (Figure 7b and c). Among the three groups of PKC, TPA is able to activate both the conventional (α, β, and γ) and novel (δ, ɛ, θ, and η) isoforms of PKC.39 Therefore, future work should include the identification of the exact isoforms of PKC involved in zVAD-induced autocrine production of TNFα and cell death. Another important and intriguing question would be how zVAD activates PKC. It appears that the activation of PKC is not related to caspase inhibition as QVD-oph fails to activate PKC. On the other hand, zVAD-fmk and BocD-fmk have been reported to possess nonspecific inhibitory effect toward other proteases such as cathepsins, while QVD-oph does not.22 It is thus possible that PKC activation might be due to the off-target effect of zVAD-fmk and BocD-fmk.
Although zVAD has been shown in this study to promote TNFα transcription and production, the autocrine level is still very low (around 10 pg/ml) (Figure 2b). Exogenous TNFα of such a concentration was found not cytotoxic (data not shown). Remarkably, when combining with zVAD, exogenous TNFα could induce necroptosis in L929 cells with a much faster kinetics and at a much lower concentration (data not shown). Therefore, it is believed that zVAD performs a dual function to induce necroptosis in L929 cells: (i) to promote autocrine production of TNFα, and (ii) to sensitize L929 cells to TNFα-induced necroptosis, most probably by suppression of the caspase cascade. At present, there is some evidence linking caspase suppression with promotion of necroptosis, on the basis of an earlier report that RIP1, the key kinase in TNFα-mediated necroptosis, is cleaved by caspase 8.17 This notion is also supported and strengthened by the following observations from this study: (i) although TPA alone and QVD-oph alone were not cytotoxic, combined treatment of TPA and QVD-oph was able to kill the cells efficiently (Figure 7b); and (ii) TPA alone was capable of inducing necroptosis when caspase 8 is silenced (Figure 7c). Thus far, the detailed mechanism underlying this sensitization effect requires further investigations.
Targeting caspase has been developed as a therapeutic approach to inhibit pathological apoptosis in vivo. However, the success of antiapoptotic therapies has been limited in mammalian cells and one possible reason is that the cells may undergo necrosis in the absence of apoptotic pathway.5, 15 Such a hypothesis is underscored by two very recent studies: the programmed necrosis in vivo was shown to implicate in the defense against vaccinia virus infection,13 and cerulein-induced acute pancreatitis is resulted from massive necrosis in vivo.8 Interestingly, in both models, the necrosis was triggered by endogenous TNFα. As a potent pan-caspase inhibitor, zVAD has been applied to various animal models to suppress the apoptotic responses. Recently, zVAD was reported to improve the therapeutic outcomes of radiation on tumor xenograft.40 It remains to be further determined whether the observed therapeutic effect of zVAD in vivo is due to caspase inhibition and suppression of apoptosis or due to promotion of autocrine production of TNFα and induction of necroptosis.
Taken together, data from this study suggest that a group of caspase inhibitors represented by zVAD are capable of inducing programmed necrosis or necroptosis by the following two orchestrated pathways: (i) promotion of autocrine production of TNFα by PKC–MAPKs–AP-1 signaling pathway, and (ii) inhibition of the caspase cascade, as illustrated in Figure 7d. It is of interest to further examine whether zVAD or other caspase inhibitors possess similar effects on other cell types, especially in human cancer cells.
Materials and Methods
Reagents and antibodies
The zVAD-fmk and DEVD-cho were purchased from BioMol (Plymouth Meeting, PA, USA). The BocD-fmk, QVD-oph, IETD-fmk, IETD-oph, and bisindolylmaleimide I (PKCi) were purchased from Calbiochem (San Diego, CA, USA). The antibodies against caspase 8 (4927), caspase 3 (9662), PARP-1 (9542), c-Jun (9162), RelB (4922), phosphor-ERK (thr202/tyr204) (9101), phosphor-c-Jun (ser73) (9164), and phosphor-PKC substrate (2261) were obtained from Cell Signaling (Danvers, MA, USA). The anti-phosphor-JNK (Thr183/Tyr185) (44-682G) was obtained from Biosource (Camarillo, CA, USA). The anti-RelA (SC-8008) and anti-IKKα (SC-7218) antibodies were from Santa Cruz (Santa Cruz, CA, USA). The anti-RIP3 (2283) antibody was obtained from ProSci (San Diego, CA, USA). The anti-IKKβ (05-535) antibody was from Upstate (New York City, NY, USA). The TNFα-neutralizing antibody (AF-410-NA), and TNFR1-blocking antibody (AF-425-PB), mouse TNFα and TRAIL were purchased from R&D (Minneapolis, MN, USA). The TPA, ActD, CHX, SP600125, PD98059, and anti-α-tubulin antibody were purchased from Sigma-Aldrich (St Louis, MO, USA). XENP1595, the DN-TNF against soluble TNFα was kindly provided by Dr. Szymkowski DE (Xencor).
Cell culture
L929 cells were maintained in Dulbecco's modified Eagle's medium (Sigma-Aldrich) containing 10% fetal bovine serum (HyClone, Cramlington, UK) and 1% penicillin-streptomycin (Invitrogen, Carlsbad, CA, USA) in a 5% CO2 atmosphere at 37°C.
Detection of cell death
The cell death was detected by (i) morphological changes examined under a microscope and (ii) the propidium iodide (PI) exclusion assay coupled with flow cytometry to quantify the percentage of viable cells, as described previously.20 Briefly, cells were trypsinized and collected after designated treatments and were resuspended in PBS containing PI for incubation at 37°C for 10 min. Ten thousand cells from each sample were scanned and analyzed with FACSCalibur flow cytometer and CellQuest software (BD Biosciences, San Jose, CA, USA).
Small interfering RNA
The nonspecific small interfering RNA (siRNA) oligonucleotides and siRNA oligonucleotides targeting mouse caspase 8, FADD, RIP3, c-Jun, IKKα, IKKβ, RelA, and RelB (ON-TARGETplus SMARTpool) were all obtained from Dharmacon (Layfayette, CO, USA). All siRNA were transfected into L929 cells using the DharmaFECT 4 Transfection Reagent according to manufacturer's protocol.
Transfection and luciferase reporter assay
For CrmA transfection, cells grown in 24-well plates were transfected with CrmA and EGFP plasmids (10 : 1) using Lipofectamine and Plus reagent (Invitrogen) according to manufacturer's instruction. For AP-1 luciferase assay, cells grown in 24-well plates first were transfected with AP-1-Luc and Renilla plasmids (100 : 1) using Lipofectamine and Plus reagent (Invitrogen) according to manufacturer's instruction. Twenty-four hours after transfection, cells were treated as indicated in each figure legend. The AP-1 luciferase activity was measured using a Dual-Luciferase(R) Reporter Assay kit (Promega, Madison, WI, USA) on a Glomax 96 Microplate Luminometer (Promega) according to manufacturer's protocol.
Reverse transcription-PCR
RNA was extracted using an RNeasy kit (Qiagen, Germantown, MD, USA). One microgram of total RNA from each sample was used as a template for cDNA synthesis by a QuantiTect Reverse Transcriptase Kit (Qiagen). An equal volume of cDNA product was used in the PCR performed using the TopTaq Master Mix Kit (Qiagen). The mouse TNFα and GAPDH primers were purchased from R&D. The PCR reaction conditions were set according to the protocol coming with primers (R&D). The PCR products were resolved using an agarose gel containing GelRed Nucleic Acid Gel Stain (Biotium, Hayward, CA, USA), and exposed on a Kodak Image Station 440CF (Kodak, Rochester, NY, USA). The band density was quantified using ImageJ image processing program (NIH, Bethesda, MD, USA) and normalized to that of the control group.
Measurement of autocrine production of TNFα in culturing medium by ELISA
Cells grown in a 10-cm dish were washed with PBS twice, then were incubated in fresh medium and treated as described in the figure legends. The culture medium was collected and the concentration of TNFα was determined by a Mouse TNF-alpha/TNFSF1A Quantikine ELISA Kit (R&D) following the instruction from the manufacturer.
Western blotting
Cells were lysed in M2 lysis buffer: 20 mM Tris at pH 7, 0.5% NP-40, 250 mM NaCl, 3 mM EDTA, 3 mM EGTA, 2 mM dithiothreitol, phosphatase inhibitor cocktail (Pierce, Rockford, IL, USA) and protease inhibitor cocktail (Roche, Indianapolis, IN, USA). Equal amount of protein was fractionated on SDS-PAGE and transferred onto PVDF membrane (Bio-Rad, Hercules, CA, USA). After blocking with 5% non-fat milk, the membrane was probed with designated first antibodies and second antibodies (Pierce) and developed with enhanced chemiluminescence reagents (Pierce) and visualized on a Kodak Image Station 440CF (Kodak).
Abbreviations
- TNFα:
-
tumor necrosis factor-α
- FADD:
-
fas-associated death domain
- TRAIL:
-
TNF-related apoptosis-inducing ligand
- RIP1:
-
receptor-interacting protein 1
- RIP3:
-
receptor-interacting protein-3
- AP-1:
-
activating protein-1
- JNK:
-
c-Jun N-terminal kinase
- MAPK:
-
mitogen-activated protein kinase
- IKK:
-
I-κB kinase
- TNFR1:
-
TNF receptor-1
- ERK:
-
extracellular signal-regulated kinase
- NF-κB:
-
nuclear factor κ-B
- PKC:
-
protein kinase C
- PARP-1:
-
poly(ADP-ribose)polymerase-1
- TPA:
-
12-O-tetradecanoylphorbol-13-acetate
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Acknowledgements
We thank Dr. Szymkowski for providing reagent. Y-T Wu is supported by an NUS research scholarship. This study is supported by grants from the NUS University Research Council (URC) and Singapore Biomedical Research Council (BMRC) to H-M Shen. This work is also supported in part by the Toxicology Program under the Life Science Institute, NUS.
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Wu, YT., Tan, HL., Huang, Q. et al. zVAD-induced necroptosis in L929 cells depends on autocrine production of TNFα mediated by the PKC–MAPKs–AP-1 pathway. Cell Death Differ 18, 26–37 (2011). https://doi.org/10.1038/cdd.2010.72
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DOI: https://doi.org/10.1038/cdd.2010.72
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