Abstract
Targeting of extrinsic apoptosis pathway by TNF-related apoptosis-inducing ligand (TRAIL) is an attractive approach for cancer therapy. However, two TRAIL drug candidates failed in clinical trials due to lack of efficacy. We identified 17-hydroxy wortmannin (17-HW) in a drug repurposing screen that resensitized TRAIL's response in the resistant colon cancer cells. The deficiency of caspase-8 in drug-resistant cells along with defects in apoptotic cell death was corrected by 17-HW, an inhibitor of PIK3C3-beclin 1 (BECN1) complex and autophagy activity. Further study found that BECN1 significantly increased in the TRAIL-resistant cells, resulting in increased autophagosome formation and enhanced autophagy flux. The extracellular domain (ECD) of BECN1 directly bound to the caspase-8 catalytic subunit (p10), leading to sequestration of caspase-8 in the autophagosome and its subsequent degradation. Inhibition of BECN1 restored the caspase-8 level and TRAIL's apoptotic response in the resistant colon cancer cells. An analysis of 120 colon cancer patient tissues revealed a correlation of a subgroup of patients (30.8%, 37/120) who have high BECN1 level and low caspase-8 level with a poor survival rate. Our study demonstrates that the increased BECN1 accompanied by enhanced autophagy activity is responsible for the TRAIL resistance, and a combination of TRAIL with a PIK3C3-BECN1 inhibitor is a promising therapeutic approach for the treatment of colon cancer.
Introduction
Colorectal cancer is the third most common cancer in the United States. It is the second most common cause of cancer-related death in males and the third most common in females, with 135,430 new cancer cases and 50,260 deaths in both sexes estimated to have occurred in 2017 (1). While surgery is the main therapeutic approach, chemotherapy and targeted therapy are also used in more advanced stages of colorectal cancer. Although the overall survival rate of patients with colorectal cancer has been significantly improved in the last decade, drug resistance occurs in many patients. New therapies to overcome drug-resistant colorectal cancer is an unmet need.
Abnormality in apoptosis not only contributes significantly to tumorigenesis but also plays an important role in cancer drug resistance. Induction of tumor cell apoptosis is the basis of conventional chemotherapy. Apoptosis is initiated by either an intrinsic or an extrinsic pathway. The intrinsic pathway is controlled by the mitochondria through the pro- and antiapoptotic Bcl-2 family proteins, which can be triggered by cancer chemotherapies (2). The extrinsic pathway is initiated by binding of transmembrane death receptors (DR) with specific extracellular ligands, including tumor necrosis factor (TNF), Fas ligand (FASLG), and TNF-related apoptosis-inducing ligand (TRAIL), resulting in sequential activation of the caspase cascade (3).
TRAIL belongs to the TNF ligand family. The binding of TRAIL to the TNF receptor superfamily member 10a (TNFRSF10A) and TNFRSF10B, also known as DR4 and DR5, selectively activates caspase-8, initiating the apoptotic pathway leading to cell death (4). The TRAIL apoptotic pathway has been targeted for drug development in the last two decades since the discovery of the death receptors and ligands. Agonist antibodies and recombinant TRAIL proteins have been used to activate the TRAIL signaling pathway. This approach had been used in several clinical trials (5). However, the majority of human cancers were resistant to these TRAIL agonists, and no survival benefit was found in these clinical trials.
To identify the mechanism of TRAIL resistance and new therapeutics to restore TRAIL response, we employed a quantitative high-throughput screen (qHTS) with bioactive compound and approved drug collections in a TRAIL-resistant colon cancer cell line. We identified 17-hydroxywortmannin (17-HW) as a drug that resensitized TRAIL-resistant cancer cells. Further studies revealed an increased BECN1 protein level accompanied by a deficiency of caspase-8 protein in TRAIL-resistant colon cancer cells. The increased BECN1 directly binds to caspase-8 which is subsequently degraded by the enhanced autophagy in the TRAIL-resistant cells. The results indicated that BECN1 is a potential cotarget for development of the next generation of TRAIL therapies for colon cancer.
Materials and Methods
Compounds and antibodies
Recombinant human TRAIL protein was purchased from Thermo Fisher Scientific (PHC1634). FasL was purchased from Enzo Life Sciences (ALX-522-020). 17-HW and bafilomycin A1 (Baf.A1) were obtained from Cayman Chemical. The antibodies used in experiments are listed in Supplementary Table S1.
Cell culture
All the human colon cancer cell lines were purchased from ATCC. Cells were cultured in medium with 10% FBS and 100 U/mL penicillin–streptomycin at 37°C with 5% CO2 for less than 20 passages after thawing to conduct described experiments, tested negative for Mycoplasma contamination and validated for species and unique DNA profile by the provider. The DLD1 cell line (CCL-221) was cultured in RPMI1640 medium. The TRAIL-resistant subline (DLD1-R) was derived from the parental DLD1 cells with selection by gradual exposure to TRAIL as described previously (6, 7). HCT-116 (CCL-247) and HT-29 (HTB-38) were cultured in McCoy 5A medium; T84 (CCL-248) in DMEM: F-12 medium; LS180 (CL-187), LS174T (CL-188), Caco-2 (HTB-37), RKO (CRL-2577), and LS123 (CCL-255) in EMEM; SW403 (CCL-230), SW1417 (CCL-238) and SW620 (CCL-227) in Leibovitz L-15 medium; and SNU-C2B (CCL-250), HCT-15 (CCL-225), COLO320 (CCL-220) and NCI-H508 (CCL-253) in RPMI1640 medium.
Quantitative high-throughput screening
Caspase-8 assay (Caspase-Glo, Promega) was conducted according to the manufacturer's protocols. DLD1-R cells were plated at 3,000 cells/well in 5 μL of RPMI1640 medium with or without 10 ng/mL TRAIL with 10% FBS and 100 U/mL penicillin–streptomycin in 1,536-well, white, solid-bottom plates and incubated 4 hours at 37°C. Four concentrations of compounds from the library of pharmacologically active compounds (LOPAC, Sigma-Aldrich), the NIH Chemical Genomics Center Pharmaceutical collection (NPC; ref. 8), and Mechanism Interrogation Plate (MIPE) were added to the plates at 23 nL/well using a pintool station (WAKO Scientific Solutions). After 8-hour incubation at 37°C with 5% CO2, the caspase-8 assay reagents were added to the plates at 5 μL/well. After incubation for the indicated time, the luminescence signals were detected using a Viewlux plate reader (PerkinElmer). A total of 12 compounds were selected and confirmed as the primary hits from this screening (Supplementary Table S2).
Cell transfection and generation of stable cell lines
BECN1 short hairpin RNA (shRNA) lentiviral particles gene silencer system (sc-29797-V and sc-72578-V, Santa Cruz Biotechnology) was used to generate stable BECN1-silenced cell lines. Briefly, cells were seeded in 6-well plates (0.5 to 1.0 × 106 cells/well) and incubated overnight. Before infection, cells were treated with the medium containing 5 μg/mL polybrene (sc-134220, Santa Cruz Biotechnology). The lentiviral particles were added to each well at the multiplicity of infection (MOI) of 2 to 10. After 48-hour incubation, cells were washed and split at 1:3 ratio, then cultured for another 48 hours. Stable clones expressing BECN1 shRNA were selected by 8 μg/mL puromycin dihydrochloride (sc-108071, Santa Cruz Biotechnology).
Transfection of BECN1-truncated variants
All the BECN1-truncated variants plasmid, including pcDNA4-beclin1 (FL), pcDNA4-beclin1 1-242, pcDNA4-beclin1 243-450, pcDNA4-beclin1-(Δ151-241), pcDNA4-beclin1 1-150, and pcDNA4-beclin1 151-241 were gifts from professor Qing Zhong (Addgene plasmid # 24388, 24391, 24392, 24393, 24389, and 24390; ref. 9). Cell transfection was performed with TurboFectin 8.0 (Origene) according to the manufacturer's protocol. After 48-hour transfection, DLD1 cells were lysed in tandem affinity purification buffer containing 20 mmol/L Tris HCl (pH 7.5), 150 mmol/L NaCl, 0.5% Nonidet P-40, 1 mmol/L NaF, 1 mmol/L Na3VO4, 1 mmol/L EDTA, and protease and phosphatase inhibitor mixture (Roche). The whole-cell lysates were used for immunoprecipitation and immunoblotting as input sample control.
Caspase activity assays and ATP content cell viability assay
Caspase-8, caspase-3/7 activity assays (Caspase-Glo, Promega), and ATP content cell viability assay (CellTiter-Glo, Promega) were conducted according to the manufacturer's protocols. Cells were plated at 2,000 to 4,000 cells/well in 25 μL of complete culture medium in 384-well, solid white plates and incubated overnight at 37°C with 5% CO2. Compounds (25 μL/well) were added to each assay plate at indicated concentrations. After 8-hour (caspase-8 assay) or 16-hour (caspase 3/7 assay and ATP content cell viability assay) incubation, the assay reagents (50 μL/well) were added to the plates. After incubation of indicated time of each assay, the luminescence signals were detected in the ViewLux plate reader.
Quantitative PCR
Total RNA was extracted using RNeasy Plus kit (Qiagen). Total RNA (2 μg) was reverse transcribed into cDNA using High-Capacity RNA-to-cDNA Reverse Transcription Kit (Applied Biosystems). Messenger-RNAs of CASP8 and BECN1 were quantified using TaqMan PreAmp Master Mix Kit with ABI ViiA 7 System (Applied Biosystems). The qPCR reactions were performed in a final volume of 20 μL and with an initial incubation at 95°C for 10 minutes followed by 40 cycles of 95°C for 10 seconds and 60°C for 60 seconds. The relative expression level of each mRNA was normalized to the level of GAPDH mRNA and calculated using the ΔΔCt method. The CASP8 primer (Hs01018151_m1) and BECN1 primer (Hs00186838_m1) were purchased from Thermo Fisher Scientific.
Immunocytochemistry
Cells were grown and stained in black, clear-bottomed 96-well plates. Briefly, 4% paraformaldehyde was dispensed into each well and cells were fixed for 30 minutes, which was aspirated out and 50 μL 0.1% Triton X-100 was then added for cell permeabilization for 15 minutes, followed by 1-hour blocking. The cells were incubated overnight at 4°C with primary antibodies at the optimized concentration. After rinsing three times with PBS, secondary antibodies of correlated species were added. The nucleus was stained with Hoechst 33342 (H1399, Life Technologies) for 30 minutes. After rinsing with PBS three times, cells were imaged in the INCell2200 imaging system (GE Healthcare Life Sciences) with a 20 or 40 × objective lens. Image analysis was conducted using the INCell Analyzer software.
Western blotting and immunoprecipitation
The cell lysates were centrifuged at 16,000 rpm for 15 minutes, and the protein concentration was quantified with BCA Assay Kit (Pierce BCA Protein Assay Kit, Thermo Fisher Scientific). The protein was separated by Bis-Tris or Tris-Acetate gels and transferred to polyvinylidene difluoride membrane by dry transfer (iBlot 2 Gel Transfer Device, Thermo Fisher Scientific) or tank wet transfer. Immunoblot analysis was performed with an antibody, and the chemiluminescence signal was visualized with Luminata Forte Western HRP substrate (EMD Millipore) in the BioSpectrum system (UVP, LLC). The chemiluminescence intensities of the bands were quantified in the VisionWorks LS software (UVP, LLC).
For the immunoprecipitation, the Pierce direct magnetic IP/Co-IP kit (Thermo Fisher Scientific) was used. The antibodies were purified to remove BSA and gelatin, and preservative using the Pierce Antibody Clean-up Kit (Thermo Fisher Scientific), followed by coupling the purified antibodies to the activated N-hydroxysuccinimide magnetic beads. Cell lysates were subjected to immunoprecipitation by incubation with the antibody-coupled beads, followed by washing to remove nonbound proteins. The samples were then eluted in a low-pH elution buffer to dissociate the coprecipitated proteins that were analyzed by Western blotting. For the immunoprecipitation of FLAG-tagged BECN1-truncated variants, the FLAG Immunoprecipitation kit (Sigma) was used according to the manufacturer's instructions.
Human colon cancer tissue array and IHC
A human colon cancer tissue array, which had 120 cases of colon adenocarcinoma with tumor and normal adjacent tissue, as well as survival and tumor staging (TNM) information data, was purchased from US Biomax. The slides were stained with anti-caspase-8 and anti-BECN1 antibodies and then were scored by three independent pathologists.
Statistical analysis
The primary screen data were analyzed using customized software developed internally (10). All data from the cell-based assays were presented as the mean ± SEM. Half-maximal inhibitory (IC50) or activating (EC50) concentrations were calculated using Prism software (GraphPad Software). The cell lines with IC50 more than 200 ng/mL were defined as TRAIL-resistant. The two-tailed unpaired Student test of the mean was used for single comparisons of statistical significance between experimental groups. One-way ANOVA with the Bonferroni test was used for multiple comparisons. Bliss independence with Prism was used to define synergistic or additive effects.
Results
17-HW restores the apoptotic response to TRAIL-resistant colon cancer cells
A drug repurposing screen was performed in a TRAIL-resistant DLD1-R cell line using a cell viability assay that identified 17-HW as a lead compound to overcome TRAIL resistance in DLD1-R (Supplementary Table S2). The DLD1-R cells were highly resistant to TRAIL that did not activate caspase-8, caspase-3, and caspase-7, nor cell death at concentrations up to 1 mg/mL. In the sensitive parental DLD1 cells, TRAIL concentration-dependently activated caspase-8 (EC50 of 2.6 ng/mL) and caspase 3/7 (EC50 of 3.0 ng/mL), and caused apoptotic cell death with IC50 of 2.3 ng/mL (Fig. 1A–C). Treatment of the resistant DLD1-R cells with 0.5 μmol/L 17-HW restored TRAIL's apoptotic response as evidenced by the activation of caspases and induction of apoptotic cell death (Fig. 1A–C). The EC50 of TRAIL for caspase-8 and caspase-3/7 were 8.31 and 2.47 ng/mL, respectively, and the IC50 for cell death was 2.57 ng/mL, similar to those observed in the sensitive DLD1 cells. The results indicated that 17-HW treatment restored the apoptotic response to TRAIL in the resistant DLD1-R cells.
Restoration of full-length caspase-8 in DLD1-R cells by 17-HW in TRAIL-resistant cells
We then examined the protein levels of caspases-8, -3, and -7 in the resistant DLD1-R cells with and without 17-HW. Consistent with the previous report (11), the full-length caspase-8 level was dramatically reduced in the resistant cells (Fig. 1D; Supplementary Fig. S1). Caspase-8 is the first enzyme activated by TRAIL in the extrinsic apoptotic pathway in which the full-length caspase-8 is cleaved to form an activated caspase-8. In addition to the absence of the full-length caspase-8 protein, the cleaved caspases-8, -3, and -7 (the active forms of these caspases) were all absent in the drug-resistant cells compared with the drug-sensitive DLD1 cells (Fig. 1D). The ubiquitinated caspase-8 level in the resistant DLD1-R cells was not changed (Supplementary Fig. S1), eliminating the possibility of ubiquitinated caspase-8 as a cause of decreased full-length caspase-8 proteins (12). The CASP8 transcription level did not change after 17-HW treatment in these cells, suggesting a posttranslational regulation of caspase-8 protein (Fig. 1E; Supplementary Fig. S1). Expression of TNFRSF10A, TNFRSF10B, and CFLAR in the TRAIL-resistant cells did not change either (Supplementary Fig. S1). In the extrinsic apoptosis pathway, TRAIL binds to death receptors that then sequentially activates caspase-8, -3, and -7. Thus, the absences of active (cleaved) caspase-3 and -7 in the TRAIL-resistant cells should be caused by the loss of caspase-8 and its activation in the DLD1-R cells.
Treatment of DLD1-R cells with 17-HW restored full-length caspase-8 protein level (Fig. 1D), and cleaved caspase-8, -3, -7, and PARP in response to TRAIL treatment were also recovered in DLD1-R cells (Fig. 1D). In the sensitive DLD1 cells, 17-HW did not significantly affect caspases and PARP protein expression (Fig. 1D). The CASP8 gene transcription did not change after 17-HW treatment in both cell lines (Fig. 1E). Together, the results demonstrate that the reduced full-length caspase-8 protein in the TRAIL-resistant DLD1-R cells can be restored by 17-HW resulting in restoration of TRAIL's apoptotic response.
Overexpression of BECN1 significantly enhances autophagy and autophagy flux in TRAIL-resistant cells
17-HW has been reported to inhibit autophagy induction and autophagosome formation through inhibition of the BECN1–PIK3C3 complex (13). To determine whether the autophagy inhibition by 17-HW is responsible for resensitization of resistant cells to TRAIL, two autophagy markers, the microtubule-associated protein 1 light chain 3 beta (MAP1LC3B) and sequestosome 1 (SQSTM1)/p62, were measured. The MAP1LC3 has two forms including MAP1LC3B-I in the cytosol and MAP1LC3B-II conjugated with phosphatidylethanolamine predominantly in autophagosomes and autolysosomes (14). We found that the levels of MAP1LC3B-I, MAP1LC3B-II, and SQSTM1 were extremely low in the DLD1-R cells compared with DLD1 cells (Fig. 2A), which were increased dramatically upon Baf.A1 treatment (vacuolar H+-ATPase inhibitor that increases autophagosomes due to an inhibition of autophagosome–lysosome fusion resulting in retardation of autophagy flux; Fig. 2A) (14). The results revealed the overactive autophagy and enhanced autophagy flux in TRAIL-resistant cells that can be ameliorated by 17-HW (Fig. 2A; Supplementary Fig. S2).
To further explore the overactive autophagy in the TRAIL-resistant cells, we measured the inhibitory effect of 17-HW on BECN1 and PIK3C3 complex. BECN1 expression and phosphorylation at Ser15 and Ser93 significantly increased in DLD1-R cells at both the mRNA and protein levels (Fig. 2B and C; Supplementary Fig. S2). Although PIK3C3 levels were similar in both cell types, the BECN1–PIK3C3 complex markedly increased in the DLD1-R cells (Fig. 2D; Supplementary Fig. S2). However, the amount of total and phosphorylated ULK1 and MTOR, two upstream kinases of BECN1, did not change in the resistant cells (Supplementary Fig. S2). Together, these results suggested that the overexpression of BECN1 in TRAIL-resistant DLD1-R cells augmented binding of BECN1 to the PIK3C3 complex, contributing to enhanced autophagy that was inhibited by 17-HW.
Increased BECN1 level sequestrates full-length caspase-8 in autophagosomes for degradation in TRAIL-resistant cells
To determine the role of enhanced autophagy induced by increased BECN1 on the degradation of full-length caspase-8 in TRAIL-resistant DLD1-R cells (15), the turnover of full-length caspase-8 was studied. After treatment with 17-HW or Baf.A1, the level of full-length caspase-8 was restored in the resistant DLD1-R cells (Figs. 2E–G and 3A–C). However, after Baf.A1 treatment, the increased caspase-8 colocalized with the MAP1LC3 puncta (Fig. 2F–H), indicating that the full-length caspase-8 proteins were sequestered in the autophagosomes in the resistant cells. However, Baf.A1 could not sensitize DLD1-R cells to TRAIL (Supplementary Fig. S2) due to the unavailability of full-length caspase-8 proteins in the cytosol. In 17-HW–treated-cells, the increased caspase-8 did not colocalize with the MAP1LC3 puncta, suggesting that caspase-8 proteins, not sequestered in autophagosomes, can be activated by TRAIL (Fig. 2F–H). Hence, the full-length caspase-8 proteins increased by 17-HW restored the apoptotic response in the DLD1-R cells. After a combination treatment of 17-HW with TRAIL, the level of BECN1 protein was remarkably reduced in the resistant cells because the BECN1 was cleaved by the activated caspases (Fig. 3D; ref. 16). Together, the results indicated that the increased BECN1 proteins in the TRAIL-resistant cells led to the sequestration of full-length caspase-8 proteins in autophagosomes that were subsequently degraded by the overactive autophagy flux. Treatment of the TRAIL-resistant cells with 17-HW decreased the overactive autophagy, restored full-length caspase-8 level, and resensitized the apoptotic response of TRAIL in the resistant colon cancer cells.
Direct binding of BECN1 to full-length caspase-8
We hypothesized that increased BECN1 might bind to caspase-8 triggering its autophagic degradation in the TRAIL-resistant cells. To examine the direct binding of BECN1 to full-length caspase-8, a specific antibody recognizing the carboxyl terminus of full-length caspase-8 was used to detect the binding with BECN1 and its truncated variants. We found that after treatment with 17-HW, the restored full-length caspase-8 remained in the cytosol and its interactions with BECN1 were inhibited (Fig. 3A–C). In addition, the interaction of BECN1 with the small catalytic subunit (p10) of caspase-8 was detected upon treatment with TRAIL (Fig. 3D). However, this interaction was not found after the treatment with Baf.A1, which sequestrated caspase-8 to autophagosomes (Fig. 3A–C). Using truncated variants of BECN1, we then determined the domain of BECN1 responsible for binding with full-length caspase-8. We found that the evolutionarily conserved domain (ECD) of BECN1 mediated its interaction with full-length caspase-8 (Fig. 4A).
To further understand how BECN1 interacts with full-length caspase-8, we performed computational modeling to probe the protein-protein interactions between the ECD domain of BECN1 and full-length caspase-8. The binding model was predicted from the existing crystal structure of the ECD domain of BECN1 (17) and caspase-8 (18) using a protein docking program ZDOCK, which utilizes a pairwise statistical potential energy to optimize a large ensemble of docking complexes and the best model is generated from the most energetically stable one (19). The predicted binding model analysis showed that BECN1 preferentially binds to the p10 subunit of caspase-8 by forming a trimeric complex together with the p18 domain of caspase-8 (Fig. 4B). A cluster of aromatic residues from BECN1 including Tyr333, Tyr352, Phe359, and Phe360 are involved in an extensive hydrophobic and aromatic stacking interaction with caspase-8 at the protein binding interface (Fig. 4C). A previously reported mutagenesis study showed that the aromatic finger residues Phe359 and Phe360 in BECN1 played an important role in protein–protein binding interaction (17). On the other hand, studies showed that caspase-8 binds to the regulatory protein CFLAR at the same binding interface of p10 subunit, which is an inhibitor of initiator caspase activation and cell death (20). Together, these findings suggested that ECD domain of BECN1 binds to the p10 subunit of full-length caspase-8, which led to the sequestration of the full-length caspase-8 in autophagosomes for subsequent autophagic degradation.
Knockdown of BECN1 expression prevents degradation of full-length caspase-8 and restores the response to TRAIL in resistant DLD1-R cells
To further confirm that increased BECN1 causes autophagic degradation of full-length caspase-8 resulting in TRAIL resistance, we carried out a BECN1 knockdown experiment. In the resistant DLD1-R cells, both BECN1 mRNA and BECN1 protein were significantly reduced by the BECN1 shRNA (Fig. 5A; Supplementary Fig. S3). The CASP8 mRNA level was increased by the BECN1 shRNA (Supplementary Fig. S3). Similar to the treatment with 17-HW, the BECN1 knockdown restored the levels of caspases-8, -3, and -7 and TRAIL's response (Fig. 5B–D; Supplementary Fig. S3; Supplementary Table S3). The potency of TRAIL in the resistant DLD1-R cells after the BECN1 knockdown was similar to that in the sensitive DLD1 cells. The BECN1 knockdown increased MAP1LC3B-I and SQSTM1 to the levels similar to the sensitive cells (Fig. 5A), an indication of reductions in autophagosome formation and autophagy flux. Similarly, the full-length caspase-8 level was recovered in the resistant cells after the BECN1 knockdown (Fig. 5A). The restored full-length caspase-8 protein remained in the cytosol, even after Baf.A1 treatment (Fig. 5E), due to the reduction of autophagosome formation and decreased autophagy flux after the BECN1 knockdown. Together, the results further confirmed that the increased BECN1 level in TRAIL-resistant cells is responsible for the deficiency of full-length caspase-8 and TRAIL resistance.
To determine whether this mechanism of increased BECN1 that subsequently decreased the full-length caspase-8 level was present in other colon cancer cell lines, a panel of 15 other colon cancer cell lines were examined (Supplementary Table S4; Supplementary Fig. S4). We found that 11 of these 15 cell lines (IC50 > 200 ng/mL) exhibited significant resistance to TRAIL (Supplementary Fig. S4). The TRAIL resistance was overcome by either 17-HW treatment or BECN1 knockdown in three of them (Caco-2, LS174T, and LS180 cell lines), similar to that in the DLD1-R cells described above (Fig. 5G–L; Supplementary Tables S5 and S6). The results indicated that TRAIL resistance is present in many colon cancer cell lines (11 of 15). However, only a portion (3 of 15) are mediated by the mechanism of increased BECN1 and enhanced autophagy among the 15 cell lines examined. It also suggests that the combination therapy of TRAIL with a BECN1–PIK3C3 complex inhibitor such as 17-HW may improve the therapeutic efficacy for a subpopulation of patients with colon cancer with this type of TRAIL resistance.
Increased BECN1 levels plus reduced caspase-8 levels in colon cancer patient tissues correlates with a poor patient survival rate
To determine the clinical relevance of our above finding, we next examined BECN1 and full-length caspase-8 levels in a human colon cancer tissue array with samples from 120 patients including 90 of them with matched adjacent normal colon tissue (Supplementary Table S7). All patients whose tumor samples were included in this array suffered from adenocarcinoma of the colon. Associations of BECN1 and caspase-8 with clinicopathologic features (including pathologic tumor stage, lymph node metastases, and histologic grade) were examined, respectively (Supplementary Table S8). Neither BECN1 nor caspase-8 protein levels, as a single factor, correlated with any of these clinicopathologic features (P > 0.05, χ2test). Examining two factors together, high BECN1 levels and low full-length caspase-8 levels, yielded a subpopulation with significant correlation to more advanced pathologic T stage (T3 and T4, P = 0.005, χ2 test), and poor histologic differentiation of the tumor (P = 0.023, χ2 test). In addition, BECN1 or full-length caspase-8 levels showed no significant association to survival rate in Kaplan–Meier survival curves individually (P = 0.2392 and P = 0.3054, respectively; Fig. 6A and B). After combining two factors (high BECN1 and low full-length caspase-8 levels), it showed a significant correlation with the low survival rate (P < 0.0001; Fig. 6C). In this cohort of patients, it revealed a statistically negative correlation between BECN1 and full-length caspase-8 in the Spearman' r coefficient test (Fig. 6D). Decreased levels of full-length caspase-8 tended to present in tumor tissues with increased BECN1 (Fig. 6E). These findings concord well with the model which predicted an increased BECN1 level leading to a decreased full-length caspase-8 level in a subgroup of patients (Fig. 6F). Taken together, the results showed that patients with high BECN1 level and low caspase-8 level clinically correlates with high cancer progression and low survival rate, implying the poor prognosis of the patients with potential TRAIL resistance.
Discussion
Development of resistance to therapeutics, either intrinsic or acquired, is a major challenge in colon cancer treatments. Abnormality in the apoptotic cell death signaling pathway has been implicated in colorectal cancer, which conduces to the survival of cancer cells and is a leading cause of resistance to current therapeutic approaches (21). Because the extrinsic pathway activates apoptosis independently, a potential therapeutic development for colorectal cancer has been explored by targeting FASLG and TRAIL. FASLG was shown to strongly induce apoptosis in a wide range of cancer cells including colorectal cancer (22), but it is not clinically useful due to its lethal hepatotoxicity (23). Similar to FASLG, TRAIL-induced apoptosis in cancer cells. In contrast to FASLG, TRAIL spared most normal cells with only marginal cytotoxicity (24), an attractive quality for cancer therapy. TRAIL has been shown to induce apoptosis in malignant cells both in vitro and in preclinical models of colorectal cancer (22, 25). However, a large number of patients with cancer including those with colorectal cancer became resistant to TRAIL treatment in phase II/III clinical trials (22, 25). Defects in the TRAIL signaling pathway have been reported that confer resistance to TRAIL in colorectal cancer including downregulation and/or impaired functionality of TNFRSF10A and TNFRSF10B, inhibition of caspase-8 activation, decrease of pro- or activated caspase-8 level, and increased level of antiapoptotic proteins, such as BCL2, Bcl-xL, and inhibitor of apoptosis proteins (IAP; refs. 11, 22).
Caspase-8 plays a central role in the extrinsic apoptosis pathway because it is the primary caspase that initiates the death signal transduction after the binding of TRAIL to DRs (26). It has been reported that caspase-8 protein expression was decreased in colorectal cancer (27). The loss of caspase-8 compromises extrinsic apoptotic cell death that has been reported in neuroendocrine tumors such as neuroblastoma (28) and small-cell lung carcinoma (29). Reduction of caspase-8 expression in about 10% of patients with colorectal cancer was reported (30). The silence of CASP8 expression has been linked to the promoter methylation or gene deletion (31). It has been reported that caspase-8 protein expression was absent in multiple lung and breast carcinoma cell lines without a significant change of CASP8 mRNA level (32). Despite these findings, the precise reasons for decreased caspase-8 protein expression have not been well elucidated (26).
Autophagy is a degradation pathway for long-lived proteins and organelles, which usually functions to maintain normal cell survival but can mediate cell death in certain conditions (15). Autophagy flux starts from autophagosome formation, moves to fusion with lysosomes to form autolysosomes, and ends in a sequential degradation of contents in autolysosomes (14). Although autophagy interplays with apoptosis, their crosstalk is complicated and many details remain unresolved (33). It has been reported that activated caspase-3, -7, and -8 can mediate cleavage of BECN1 or ATG13, resulting in autophagy inhibition and enhancing apoptosis (16). Conversely, inhibition of autophagy could block active caspase-3 or -8 by autophagic degradation of these proteins (34, 35). However, whether the full-length caspase-8 is reduced by autophagic degradation has not been reported previously.
Wortmannin was a pan-PI3K inhibitor, which forms a covalent bond with a conserved lysine residue involved in the phosphate-binding reaction to prevent its interaction with beclin 1 and the subsequent autophagy activation (36). 17-HW was an analogue of wortmannin with modification at position 17 remote from its furan ring and was the most potent inhibitor in its class (37, 38). Moreover, 17-HW was more stable than wortmannin in vivo that remained detectable after 30 minutes, and the pegylated 17-HW remained detectable after 60 minutes, whereas wortmannin had been reported to be undetectable after intravenous administration to mice (37, 39). In addition, PX-866, another structure-modified compound based on wortmannin, exhibits remarkable in vivo antitumor efficacy via both oral and intravenous administrations (39, 40). It has been evaluated for the treatment of recurrent glioblastoma and metastatic castration-resistant prostate cancer in phase II clinical trial.
The flux dual contrasting roles of autophagy flux have been linked to both tumor promotion and tumor suppression (41). A high level of autophagy activity has been considered as the resistance mechanism for drug-resistant mediated extrinsic apoptosis in several cancer types including colorectal cancer (34), breast cancer (42), leukemia (43), hepatocellular carcinoma (44), lung cancer (35), and prostate cancer (45). Inhibition of autophagy with small-molecule inhibitors or by silencing of autophagy-associated genes such as BECN1, ATG5, ATG7, or ATG12 has been shown to sensitize cancer cells to TRAIL (42–45). The autophagic degradation of active caspase-8 (34) or TNFRSF10A and TNFRSF10B (42) has been reported as possible mechanisms involved in TRAIL resistance. However, the activation of autophagy flux has been reported to enhance TRAIL-induced extrinsic apoptosis through downregulation of CFLAR (46), and upregulation of TNFRSF10B (47), which are very different from what we have observed in the subpopulation of cell lines and patient samples.
Downregulation of active caspase-8 has been linked to TRAIL resistance (34) and proteasome degradation (48). The degradation of full-length caspase-8 is unclear. In this study, we demonstrate that the increased BECN1 level in the TRAIL-resistant cells causes inclusion of full-length caspase-8 proteins into autophagosomes through the direct binding of BECN1 to full-length caspase-8 and the full-length caspase-8 proteins in autophagosomes are then degraded by the enhanced autophagy flux in the TRAIL-resistant cells. Overexpressed BECN1 levels were reported in 44.5% of colorectal cancer (49). In the tissue array of 120 colorectal cancer patient samples, we also found the increased BECN1 level plus reduced full-length caspase-8 level correlated with the poor patient survival rate in approximately 30.8% of patient tissues (37 of 120 patients). These data also implied a subpopulation of potential TRAIL-resistant patients would have the poor prognosis.
Colorectal cancer is a heterogeneous disease in accordance with its molecular profiles and clinical presentations (50). We found that the increased BECN1 level and BECN1-mediated autophagy degradation of full-length caspase-8 are present in a subgroup of colon cancer cell lines and patients. Therefore, a combination therapy of TRAIL with a BECN1–PIK3C3 complex inhibitor has potential as a new therapeutic approach for the subgroup of patients with colon cancer with an increased BECN1 level plus a reduced full-length caspase-8 level.
Disclosure of Potential Conflicts of Interest
No potential conflicts of interest were disclosed.
Authors' Contributions
Conception and design: S. Dai, W. Sun, A.D. Schimmer, C. He, H. Zhu, W. Zheng
Development of methodology: S. Dai, W. Sun, B. Fang, W. Zheng
Acquisition of data (provided animals, acquired and managed patients, provided facilities, etc.): S. Dai, S. Yang, B. Fang, H. Zhu
Analysis and interpretation of data (e.g., statistical analysis, biostatistics, computational analysis): S. Dai, S. Yang, X. Hu, W. Sun, G. Tawa, W. Zheng
Writing, review, and/or revision of the manuscript: S. Dai, S. Yang, X. Hu, W. Sun, W. Zhu, A.D. Schimmer, H. Zhu, W. Zheng
Administrative, technical, or material support (i.e., reporting or organizing data, constructing databases): S. Dai, A.D. Schimmer
Study supervision: W. Zheng
Acknowledgments
The authors thank the compound management group at NCATS, NIH for their professional support, and Dr. DeeAnn Visk, a medical writer and editor, for editing the manuscript. This work was supported by the Intramural Research Programs of the National Center for Advancing Translational Sciences, NIH (to W. Zheng), and a grant 81703076 from the National Natural Science Foundation of China (to D. Sheng).
The costs of publication of this article were defrayed in part by the payment of page charges. This article must therefore be hereby marked advertisement in accordance with 18 U.S.C. Section 1734 solely to indicate this fact.