Abstract
Heat shock protein 90 (Hsp90) is widely overexpressed in cancer cells and believed to be essential for the maintenance of malignant phenotypes. Targeting Hsp90 by small molecules has shown promises in solid and hematological malignancies, which likely involves degradation of client oncoproteins in a cell-type specific manner. In this study, we found that structurally unrelated Hsp90 inhibitors induce DNA damage and apoptosis via p53-dependent induction of PUMA, which indirectly triggers Bax activation and mitochondrial dysfunction in colon cancer cells. Deficiency in PUMA, BAX, or p53 at lesser extent, abrogated 17AAG-induced apoptosis and mitochondrial dysfunction, and enhanced clonogenic cell survival. Furthermore, suppression of p53-dependent p21 induction or enhanced p53 activation synergized with 17AAG to induce PUMA-dependent apoptosis. Finally, PUMA was found to mediate apoptotic and therapeutic responses to the 17AAG analog 17DMAG in xenografts. These results demonstrate an important role of the p53/PUMA/Bax axis in Hsp90 inhibitor-induced killing of p53 WT cells, and have important implications for their clinical applications.
Keywords: Hsp90 inhibitors, PUMA, p53, apoptosis, colon cancer
Introduction
Heat shock protein 90 (Hsp90) is one of the most abundant molecular chaperones in eukaryotes and regulates many cellular processes including signal transduction, protein degradation, protein folding and maturation of client proteins (1). Over 200 proteins have been reported to be Hsp90 clients, including many oncogenic proteins, such as mutant p53, Raf-1, Akt (1-2), and others associated with hallmarks of cancer (3). Interestingly, Hsp90 is constitutively expressed at 2–10-fold higher levels in tumor cells than their normal counterparts (4), and appears to be required for malignant transformation (5), and a selective therapeutic target in cancer cells (1-2). Hsp90 targeting has attracted considerable attention since the late 1990s. Currently, over 17 Hsp90 inhibitors have entered clinical trials as potential anticancer agents (1, 5). These inhibitors, such as the natural product geldanamycin (GA) and its less toxic analog 17-allylamino-17-demethoxygeldanamycin (17AAG) inhibit the molecular chaperone function of Hsp90 by binding to its ATP/ADP pocket and causing destabilization of its complexes with client proteins (2). Treatment with GA and 17AAG can induce apoptosis, inhibit metastasis or angiogenesis in both cell and animal models (1, 5-6). 17AAG is one of the very first Hsp90 inhibitors to complete phase II clinical trials (1, 5). Other Hsp90 inhibitors with improved pharmaceutical properties, such as 17DMAG and NVPAUY922, can promote apoptosis in preclinical models and are currently in phase I/II clinical trials (1, 7). However, the mechanisms underlying Hsp90 inhibition-induced cell killing are currently not well understood, and may vary by cell type. Several mechanisms have been suggested, including Akt down-regulation (8), inhibition of NF-κB activation due to IKK destabilization (9), ER stress (10), and more recently p53 activation (11-12).
The Bcl-2 family proteins are the central regulators of mitochondria-mediated apoptosis (13-15). The BH3-only sub family members are proximal signaling molecules that respond to distinct as well as overlapping signals, and consist of at least 10 members. Several of BH3-only proteins, such as PUMA and Bim, activate Bax/Bak following the neutralization of all known anti-apoptotic Bcl-2 family members (13-15) to promote mitochondrial dysfunction and caspase activation (16-18). PUMA is a critical mediator of p53-dependent and -independent apoptosis in multiple tissues and cell types (18). Transcription of PUMA is mainly dependent on p53 activity in response to DNA-damaging agents such as γ-irradiation, common chemotherapeutic drugs (18-19), and even some kinase inhibitors (20). Upon exposure to non-genotoxic stimuli, PUMA is induced by other transcriptional factors such as p73 (21-22), NF-κB (23), and FoxO3a (24-25). Bim regulates apoptosis in immune cells, normal and malignant hematopoietic cells, and some epithelial cells generally following nongenotoxic stresses (13).
In this study, we investigated the mechanisms of apoptosis induced by Hsp90 inhibitors in colon cancer cells. We found that p53-mediated induction of PUMA and Bax is required for the apoptotic responses to Hsp90 inhibitors via the mitochondrial pathway in vitro and in vivo. In contrast, p53-mediated p21 induction suppresses 17AAG-induced apoptosis. Enhanced p53 activation or p21 inhibition sensitized p53 WT colon cancer cells to PUMA-dependent apoptosis following treatment with Hsp90 inhibitors. These results demonstrate an important role of the p53/PUMA/Bax axis in the therapeutic responses to Hsp90 inhibitors in p53 WT cancers, and have important implications for their future development and applications.
Materials and Methods
Cell culture and treatment
The human colorectal cancer cell lines, including HCT116, RKO, LoVo (wild-type (WT) p53, HT29 and DLD1 (mutant p53), were obtained from the American Type Culture Collection (Manassas, VA, USA). Isogenic HCT 116 knockout cell lines including p53-KO (26), PUMA-KO (27), BAX-KO (28), p21-KO (29), p21/PUMA- double KO (27) and PUMA-KO DLD1 cells (30) have been described. We examine loss of expression of targeted proteins by western blotting and conduct Mycoplasma testing by PCR during culture routinely. No additional authentication was done by the authors. Details on cell culture and drug treatments are found in the supplemental materials.
Western blotting
Western blotting was performed as previously described (16). More details on antibodies are found in the supplemental materials.
Real-time Reverse Transcriptase (RT) PCR
Total RNA was isolated from 17AAG-treated cells using the Mini RNA Isolation II Kit (Zymo Research, Orange, CA) according to the manufacturer's protocol. One μg of total RNA was used to generate cDNA using SuperScript II reverse transcriptase (Invitrogen, Carlsbad, CA, USA). Real-time PCR was carried out as before (24). Details on primers are found in the supplemental materials.
Small-interfering RNA knockdown
Transfection was performed 24 hours before 17AAG treatment using 400 pmol of siRNA in one well of a 12-well plate (20). All siRNA, including FoxO3a (ON-TARGETplus J-003007-10), PUMA (ACGTGTGACCACTGGCATTdTdT, and ACCTCAACGCACAGTACGAdTdT) (31), and Bim (GACCGAGAAGGUAGACAAUdTdT) (32) were synthesized by Dharmacon (Lafayette, CO, USA), and siRNAs were transfected with lipofectamine 2000 (Invitrogen, Carlsbad, CA, USA) according to the manufacturer's instructions.
Luciferase assays
PUMA luciferase reporter constructs (Fragments A-E) have been described previously (22). For reporter assays, cells were transfected with the fragment PUMA reporter along with the transfection control β-galactosidase reporter pCMVβ (Promega, Madison, WI, USA). Cell lysates were collected and luciferase activities were measured as previously described (33). All reporter experiments were performed in triplicate and repeated three times.
Analysis of apoptosis and cell death
Apoptosis was analyzed by nuclear staining with Hoechst 33258 (Invitrogen), and Annexin V/propidium iodide (PI) (Invitrogen) followed by flow cytometry as described (30). For colony formation assays, the same number of cells were treated and plated in 12-well plates at appropriate dilutions, and allowed to grow for 10–14 days before staining with crystal violet (Sigma, St. Louis, MO). For detection of mitochondrial membrane potential change, the treated cells were stained by JC-1 (30001, Biotium, Hayward, CA, USA) for 15 minutes according to the manufacturer's instruction, and then analyzed by flow cytometry.
Analysis of cytochrome c release and Bax multimerization, conformational change and interacting proteins
Cytoplasmic and mitochondrial fractions were separated by Mitochondrial Fractionation Kit (Active Motif, Carlsbad, CA, USA) according to the manufacturer's instructions. Cytochrome c in both cytoplasmic and mitochondrial fractions was detected by Western blotting. To detect Bax multimerization, purified mitochondrial fractions were cross-linked with 1mM of Dithiobis (succinimidyl) propionate (DSP) (Pierce, Rockford, IL, USA) as described (34-35), followed by Western blotting under non-denaturing conditions. Methods on detection of Bax conformational change (27) and interacting protein (16) have been described and details are found in the supplemental materials.
Xenograft studies
All animal experiments were approved by the University of Pittsburgh Institutional Animal Care and Use Committee. Female 5–6 week-old Nu/Nu mice (Charles River, Wilmington, MA) were housed in a sterile environment with micro isolator cages and allowed access to water and chow ad libitum. Mice were injected subcutaneously in both flanks with 4×106 WT or PUMA-KO HCT116 cells. After implantation, tumors were allowed to grow 7 days before treatment was initiated. Mice were randomized into two groups (n = 6 per group) receiving either vehicle (saline) or 17DMAG (15mg/kg/d) on days 1-4 and 7-11, respectively (36). Detailed methods on tumor measurements, harvests and histological analysis are found in the supplemental materials and as described (24, 31).
Statistical Analysis
Statistical analyses were carried out using GraphPad Prism IV software. P values were calculated by the student's t-test and were considered significant if p <0.05. The means ± one standard deviation (s.d.) are displayed in the figures.
Results
p53-dependent induction of PUMA and Bax by 17AAG in colon cancer cells
To determine a potential role of the Bcl-2 family in Hsp90 inhibitor-induced apoptosis, we first examined protein levels of its major members following 17AAG treatment in HCT116 colon cancer cells (Fig. 1A). Among them, PUMA, Bim and Bax were significantly induced, and induction was detected as early as 24 hours after treatment (Fig 1A). The levels of PUMA, BIM and BAX transcripts were also elevated (Fig. 1B). The expression of other Bcl-2 family members such as Bid, Bcl-2, and Bcl-xL remained unchanged, while that of Noxa and Mcl-1 decreased (Fig. 1A). We then treated parental, and p53-KO HCT116 or RKO cells with 17AAG to determine whether p53 is involved in the induction of PUMA, Bim and Bax. Induction of PUMA and Bax, but not Bim, was largely blocked in p53-KO cells, compared to parental cells (Fig 1C). Furthermore, we used a series of PUMA promoter luciferase reporters (containing ~2 kb upstream from the transcriptional initiation site) (22) to determine whether p53 directly activates PUMA transcription. We found that the reporters containing the two p53 binding sites (Frag “A”and “E”) had much higher activities after 17AAG treatment in p53 WT cells than in p53-KO HCT 116 cells (Fig. 1D). Moreover, the induction of PUMA and other p53 targets Bax and p21 paralleled that of p53, p53S15 phosphorylation and γ-H2AX, a marker of DNA double-strand breaks (Fig. 1E). Consistent with reports in other systems (37-38), 17AAG treatment decreased AKT and p-ERK (Fig. S1.). These findings demonstrate that 17AAG treatment leads to p53-dependent induction of PUMA and Bax, besides modulation of survival pathways.
PUMA mediates Hsp90 inhibitor-induced apoptosis
To examine a potential role of PUMA in 17AAG-induced apoptosis, we compared the responses of parental HCT116 cells with isogenic PUMA knockout (PUMA-KO) cells (27). 17AAG treatment induced apoptosis in HCT116 cells as early as 24 hours, which increased to over 30% at 72 hours, while apoptosis and activation of caspase-3 and -9 were abolished in PUMA-KO cells (Fig. 2A). Annexin V/propidium iodide staining confirmed apoptotic resistance of PUMA-KO cells (Fig. S2A and S2B). PUMA-KO cells were also found to be significantly more resistant to 17AAG than WT cells in a long-term clonogenic assay (Fig. 2B). PUMA knockdown suppressed 17AAG-induced apoptosis in p53 WT cell lines LoVo and RKO (Fig. 2C). In contrast, BIM knockdown did not inhibit 17AAG-induced apoptosis (Figs. S2C, S2D). Furthermore, 17DMAG and NVPAUY922 induced significant apoptosis in HCT 116 cells, which was largely blocked in PUMA-KO cells (Figs. 2D and S3). Collectively, these results indicate that PUMA is required for Hsp90 inhibitor-induced apoptosis in colon cancer cells with WT p53.
PUMA mediates 17AAG-induced apoptosis via the mitochondrial pathway and Bax activation
17AAG-induced apoptosis in HCT 116 was associated with mitochondrial membrane depolarization and release of cytochrome c and SMAC, which was suppressed in PUMA-KO cells (Fig. 3A). 17AAG treatment also induced PUMA-dependent Bax conformational changes and oligomerization (Fig. 3B and 3C). BAX-KO HCT116 cells were found to be resistant to 17AAG-induced apoptosis, and activation of caspase-3 and -9 (Fig. 3D), consistent with PUMA acting upstream of Bax (13-15). We further probed interactions of Bax with several Bcl-2 family members. 17AAG treatment induced dissociation of Bax from Bcl-xL and Bcl-2, which was suppressed in PUMA KO cells (Fig. 3E). In contrast, Bmi binding to Bax was largely unaffected by PUMA status or 17AAG treatment. No interaction was detected between Bax and Mcl-1, PUMA or Noxa. Interestingly, levels of Mcl-1 and Noxa decreased significantly upon 17AAG treatment in HCT 116 cells, which was reduced in PUMA KO cells (Figs. 1A and Fig. 3E). These results demonstrate that PUMA functions upstream of Bax to induce Bax activation and mitochondrial dysfunction in17AAG-induced apoptosis. PUMA likely activates Bax indirectly by replacing it from Bcl-xL or Bcl-2 (16, 39), and altered interactions among Bcl-2 family might affect their stabilities.
p53-dependent p21 induction inhibits 17AAG-induced apoptosis
p21 also showed p53-dependent induction following 17AAG treatment, while p53-KO cells were less resistant than PUMA-KO to 17AAG-induced apoptosis (Figs. 1E, 4A, 4B and S4). We hypothesized that p21-induction might inhibit apoptosis induced by Hsp90 inhibitors, much like it inhibits apoptosis induced by DNA damage (40-41). Indeed, p21-KO HCT 116 cells were found to be more sensitive to 17AAG-induced apoptosis compared to parental cells. Apoptosis was significantly reduced in p21/PUMA double KO (DKO) cells that phenocopied p53-KO cells (Figs. 4B and S4). UCN-01 was shown to selectively block p53 phosphorylation on S20 but not S15 by targeting Chk1 after DNA damage (42-43). We found that UCN-01 eliminated p21 expression and significantly enhanced 17AAG-induced apoptosis (Fig. 4C). The apoptosis induced by 17AAG and UCN-01 combination was partially dependent on PUMA (Fig. 4D). Together, these data suggest that p53-dependent induction of p21 suppresses the apoptotic response to 17AAG, and selective inhibition of p21 while preserving PUMA induction enhances cell killing.
Enhanced p53 activity synergizes with 17AAG to induce PUMA-dependent apoptosis
Chemosensitization effects of 17AAG have been extensively documented (1, 7). We found that HCT116 cells were relatively resistant to Cisplatin-induced apoptosis or PUMA expression, while p53 stabilization and serine 15 (S15) phosphorylation were readily detected (Fig. 5A and 5B). The combination of 17AAG with Cisplatin synergistically induced apoptosis, caspase activation, and PUMA expression in HCT 116 cells (Fig. 5A and 5B). The combination of 17AAG with Nutlin-3, a p53 activator that disrupts MDM2/MDMX and p53 interactions, also synergistically induced apoptosis and PUMA induction (Fig. 5C and 5D). Remarkably, the combination treatment-induced apoptosis was almost completely abolished in PUMA-KO cells (Fig. 5A and 5C). PUMA induction was reduced in p53-KO cells compared to WT HCT 116 cells (Fig. 5B and 5D). Loss of p21 induction likely explains why p53-KO cells were more sensitive than PUMA-KO to apoptosis induced by these combinations (Figs. 5A and 5B and S5). In addition, p53-KO cells were also partially resistant to apoptosis induced by 17DMAG and NVP-AUY922, and showed significantly reduced induction of PUMA and Bax, but not Bim (Fig. S5). These data demonstrate a general role of the p53/PUMA/Bax axis in Hsp90 inhibitor-induced apoptosis and chemosensitization in colon cancer cells.
Anti-tumor activities of Hsp90 inhibitors is mediated by PUMA-dependent apoptosis in vivo
To determine whether PUMA-mediated apoptosis plays a critical role in the anti-tumor activities of Hsp90 inhibitors in vivo, we established WT and PUMA-KO HCT116 xenograft tumors in nude mice. Tumor bearing mice were then treated with 15 mg/kg 17DMAG, which is water-soluble, or the vehicle by i.p., and tumor volumes were monitored every two days for 3 weeks. The WT tumors, but not PUMA-KO HCT116 tumors, responded well to 17DMAG treatment and reached roughly 1/4 the size of the tumors in vehicle treated mice on day 21 (Fig. 6A). PUMA, Bax, Bim as well as p53 phosphorylation (S15) were significantly induced by 17DMAG treatment in WT tumors (Fig. 6B), consistent with our in vitro data. TUNEL and active caspase-3 staining revealed marked apoptosis in these tumors, which decreased by over 55% in the PUMA-KO tumors treated identically (Fig. 6C and 6D). These data demonstrated an important role of the p53/PUMA/Bax axis in the anti-tumor activities of 17DMAG in vivo.
Discussion
Hsp90 helps mammalian cells and lower eukaryotes to cope with environmental stresses (44). Cancer cells are constantly under a variety of stresses (3) and Hsp90 is believed to help buffer such stresses for their survival, while different client proteins might be involved depending on cellular context (1, 7). Hsp90 inhibitors induce apoptosis in a variety of preclinical models through degradation of oncogenic client proteins including mutant p53, Raf-1, Akt, Her-2 and ALK fusion proteins (1, 7, 45). Using multiple cell lines and structurally unrelated compounds, we demonstrate a role of the p53/PUMA/Bax axis in Hsp90 inhibitor-induced apoptosis and chemosensitization in colon cancer cells using cell culture and xenograft models. p53-dependent PUMA expression directly activates Bax and the mitochondrial apoptotic pathway. Modulation of other Bcl-2 family members and survival pathways (37-38), and ER stress (Fig. S6) can also contribute to apoptosis or PUMA induction. However, the cell killing mechanisms by Hsp90 inhibitors are likely different in p53 WT and mutant cancer cells where mutant p53 is targeted for degradation (46-48).
Several recent studies showed that functional p53 is required for the induction of apoptosis by 17AAG (11-12), while the mechanism has not been well defined. We discovered distinct roles of p53-mediated PUMA and p21 induction in this process. In contrast to p53-mediated induction of PUMA/Bax, induction of p21 protected against 17AAG-induced apoptosis, consistent with the known antiapoptotic function of p21 in p53-dependent apoptosis (40-41). The induction of γ-H2AX further suggests a classical p53-dependent DNA damage response associated with double strand breaks (Fig 1E) (40-41, 49), while the precise cause of DNA damage upon Hsp90 inhibition remains to be defined. 17AAG is commonly used as a chemosensitizer and enhances cell killing when combined with a variety of cytotoxic agents, such as cisplatin, UCN-01, taxol, gemcitabine, cytarabine, or proteasome inhibitors and HDAC inhibitors (7). Our results provide mechanistic insights for such a synergy in p53 WT cells. For examples, Cisplatin or Nutlin-3 enhances 17AAG-induced cell killing via enhanced p53 activity and PUMA/Bax induction. On the other hand, UCN-01 enhances 17AAG-induced cell killing by blocking p21 expression. Therefore, selective modulation of p53-mediated apoptosis or cell cycle arrest can be exploited to enhance cancer cell killing.
The results of Hsp90 inhibitors in clinical trials are mixed (1, 5), likely reflecting lack of patient stratification or biomarkers. Improved response rates were observed in HER2-positive metastatic breast cancer patients treated with 17AAG and trastuzumab (50), as well as in ALK-rearranged non-small cell lung cancer (NSCLC) patients treated with Hsp90 inhibitor IPI-504 (51). This has been attributed to the degradation of the Hsp90 clients as driver oncoproteins. Our study together with others (11-12) would strongly suggests that this class of agents works differently in cancers with WT p53, and examining the modulation of PUMA, Bax, Bim, and p21 might help better distinguish responders from non-responders in these tumors. No mutation in the PUMA gene has been reported in human cancer while reduced PUMA expression has been reported in cutanous melanoma and Burkitt's lymphomas (18). Therefore reduced PUMA expression can potentially contribute to resistance to Hsp90 inhibitors. Toxicity to normal tissues is also a concern of Hsp90 inhibitors. It is tempting to speculate that blocking p53-dependent apoptosis might selectively reduce normal tissue toxicity without compromising efficacy in tumors harboring mutant p53.
In conclusion, we have shown that the p53/PUMA/Bax axis plays an important role in the therapeutic and apoptotic response to Hsp90 inhibitors in p53WT cancer cells. Loss of PUMA, BAX, or p53 leads to resistance at varying degrees, while loss of p21 leads to sensitization. These findings provide novel mechanistic insights for Hsp90 inhibitor-induced apoptosis, and can have important implications for their future development and application.
Supplementary Material
Acknowledgements
We thank Bert Vogelstein (Howard Hughes Medical Institute, Johns Hopkins University) for p53-KO, p21-KO HCT116 cells, and p53-KO RKO cells, and other members of Yu and Zhang laboratories for helpful discussions.
Financial information
This work is supported by NIH grant CA129829, American Cancer Society grant RGS-10-124-01-CCE, FAMRI (J. Yu), and by NIH grants CA106348, CA121105, and American Cancer Society grant RSG-07-156-01-CNE (L. Zhang). This project used shared facilities that were supported in part by UPCI CCSG award P30CA047904.
Footnotes
Disclosures: All authors disclosed no conflict of interest, and agreed on the submission.
Author contributions:
JY conceived and supervised the study. KH, XZ and JY designed experiments, analyzed and interpreted data, and wrote the paper. KH and XZ performed experiments. LZ designed experiments and analyzed data.
References
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