RESEARCH
Liver X receptor inhibition potentiates mitotane-induced adrenotoxicity in ACC
Kate M Warde1, Erik Schoenmakers2, Eduardo Ribes Martinez1, Yi Jan Lim1, Maeve Leonard1, Sarah J Lawless1, Paula O’Shea3, Krishna V Chatterjee2, Mark Gurnell2, Constanze Hantel4,5 and Michael Conall Dennedy1
1Discipline of Pharmacology and Therapeutics, School of Medicine, National University of Ireland, Galway, Ireland 2Metabolic Research Laboratories, Wellcome Trust-MRC Institute of Metabolic Science-Metabolic Research Laboratories, University of Cambridge and National Institute for Health Research Cambridge Biomedical Research Centre, Addenbrooke’s Hospital, Cambridge, UK 3Department of Clinical Biochemistry, Galway University Hospitals, Saolta Hospitals Group, Galway, Ireland 4Department of Endocrinology, Diabetes, and Clinical Nutrition, University Hospital Zurich, Zurich, Switzerland 5Medizinische Klinik und Poliklinik III, University Hospital Carl Gustav Carus Dresden, Dresden, Germany
Correspondence should be addressed to M C Dennedy: michael.dennedy@nuigalway.ie
Abstract
Adrenocortical carcinoma (ACC) is a rare aggressive malignancy with a poor outcome largely due to limited treatment options. Here, we propose a novel therapeutic approach through modulating intracellular free cholesterol via the liver X receptor alpha (LXRx) in combination with current first-line pharmacotherapy, mitotane. H295R and MUC-1 ACC cell lines were pretreated with LXRx inhibitors in combination with mitotane. In H295R, mitotane (20, 40 and 50 uM) induced dose-dependent cell death; however, in MUC-1, this only occurred at a supratherapeutic concentration (200 uM). LXRx inhibition potentiated mitotane-induced cytotoxicity in both cell lines. This was confirmed through use of the CompuSyn model which showed moderate pharmacological synergism and was indicative of apoptotic cell death via an increase in annexinV and cleaved-caspase 3 expression. Inhibition of LXRa was confirmed through downregulation of cholesterol efflux pumps ABCA1 and ABCG1; however, combination treatment with mitotane attenuated this effect. Intracellular free-cholesterol levels were associated with increased cytotoxicity in H295R (r2 = 0.5210) and MUC-1 (r2 = 0.9299) cells. While both cell lines exhibited similar levels of free cholesterol at baseline, H295R were cholesterol ester rich, whereas MUC-1 were cholesterol ester poor. We highlight the importance of LXRa mediated cholesterol metabolism in the management of ACC, drawing attention to its role in the therapeutics of mitotane sensitive tumours. We also demonstrate significant differences in cholesterol storage between mitotane sensitive and resistant disease.
Key Words
adrenocortical carcinoma
liver X receptor alpha
mitotane
cholesterol
adrenal
Endocrine-Related Cancer (2020) 27, 361-373
Introduction
Adrenocortical carcinoma (ACC) is a rare, aggressive malignancy with an incidence of 2-5 per million and which carries a poor prognosis due to local invasion or distant metastases at the time of diagnosis in the majority of cases (Fassnacht et al. 2013, Libe 2019). Complete surgical resection (R0) is the only curative therapy
(de Reynies et al. 2009, Kerkhofs et al. 2013). Yet, for those on whom R0 resection is achieved, disease recurs in 50-85% (Pommier & Brennan 1992, Terzolo et al. 2007). Mitotane is the only currently licensed pharmacotherapy for adjuvant use or for recurrent disease and remains the most effective drug (alone or in combination with
@ 2020 The authors Published by Bioscientifica Ltd. Printed in Great Britain
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platinum based chemotherapy regimens) in preventing and treating recurrence (Haak et al. 1994, Terzolo et al. 2007, 2013, Fassnacht et al. 2018). Mitotane’s use is limited by its narrow therapeutic window, whereby at serum concentrations below 14 mg/L, it demonstrates poor efficacy, while at concentrations >20 mg/L, it is associated with unacceptable toxic effects (Hermsen et al. 2011, Terzolo et al. 2013). There is significant clinical need to improve the therapeutic options in managing persistent or recurrent ACC, and in this context, the current study investigates therapeutic strategies to enhance the efficacy and tolerability of mitotane.
Mitotane has been used for 50 years in the management of adrenocortical neoplasm (Montgomery & Welbourn 1965), yet its adrenotoxic mechanism remains incompletely understood (Hescot et al. 2013, Lehmann et al. 2013, Poli et al. 2013). Sbiera et al. demonstrated that mitotane-induced adrenotoxicity is associated with intracellular free-cholesterol (FC) accumulation causing endoplasmic reticulum (ER) stress (Sbiera et al. 2015). The authors also demonstrated that mitotane-induced FC accumulation is associated with inhibition of sterol- O-acyltransferase-1 (SOAT1) which usually converts FC to inert cholesteryl esters (CE) for intracellular storage. The adrenal-cytotoxic effects of SOAT1 inhibition have also been demonstrated by LaPensee et al. through the use of the selective inhibitor ATR-101 (LaPensee et al. 2016). Consequently, this lipotoxic mechanism mediated by intracellular FC accumulation is considered significant or even predominant in terms of mitotane-induced adrenotoxicity.
We theorised that the lipotoxic effects of mitotane on ACC cells could be enhanced by targeting complementary mechanisms to that of SOAT1 inhibition, which would further increase intracellular FC. Liver X receptor alpha (LXRx/NR1H3) inhibition represents one such mechanism. LXRa is a nuclear receptor, sensitive to intracellular FC and represents the predominant transcriptional mechanism mediating reverse cholesterol transportation to the liver (Costet et al. 2000, Kennedy et al. 2005, Wang et al. 2007). At rest, LXRa is bound to its nuclear response element and held in an inactive state by co-repressor molecules. Upon ligand activation, it recruits co-activator proteins to dimerise with the retinoid X receptor (RXR), and in turn transcribes regulatory proteins for cholesterol efflux, namely ABCA1 and ABCG1. These deliver excessive intracellular FC to circulating apolipoprotein (Apo) A1 or high density lipoprotein (HDL1) (Janowski et al. 1996, Fu et al. 2001, Hu et al. 2003, Huuskonen et al. 2004, Phelan et al. 2008).
LXRa is highly expressed in liver, innate immune cells and adrenal cortex (Cummins et al. 2006) and its sensitivity to intracellular cholesterol is effected through endogenous ligand molecules, oxysterols, generated from precursor cholesterol. The common oxysterol, 27-hydroxycholesterol (27HC, also known as (25R)26-HC), is catalysed by CYP27A1 and highly expressed in the adrenal cortex (Chen et al. 1998, Fedorova et al. 2015). Higher intracellular FC results in increased oxysterol production, activating LXRa dependent transcription of cholesterol efflux pumps. The cholesterol regulatory function of LXRa is conserved across cell types, mediating reverse cholesterol transport as well as providing cellular protection against toxic FC accumulation (Cignarella et al. 2005, Engel et al. 2007).
In the adrenal, oxysterols and LXRa also have a tissue-specific role, whereby they increase steroidogenesis by upregulating steroidogenic acute regulatory (StAR) protein (Cummins et al. 2006, Nilsson et al. 2007). In breast and prostate cancer, LXRa stimulation facilitates cancer cell survival which is partially explained by its role to enhance aerobic glycolysis, while also hypothesised to reduce FC-induced cytotoxicity (Nelson et al. 2013, Flaveny et al. 2015, Kim et al. 2018).
We hypothesised that inhibition of LXRa-modulated cholesterol efflux pump expression could potentiate mitotane-induced lipotoxic adrenocortical cell death at usually subtherapeutic mitotane concentrations. We investigated the dose-dependent interactions of mitotane with pharmacological inhibition of LXRa and dominant- negative (DN) interference of LXRa activity in two human ACC cell lines (H295R and MUC-1). Using this strategy, we demonstrate an enhanced ability of mitotane in combination with LXRa inhibition to kill ACC cells at lower concentrations than for mitotane alone. We show that this effect is associated with higher intracellular FC accumulation.
Materials and methods
Cell culture and treatments
H295R human primary ACC cells (NCI-H295R, CRL-2182; (American Type Culture Collection)) (Rainey et al. 1994) were maintained in DMEM/F12 (Thermo Fisher), containing 2.5% Nu serum (Corning), 1% ITS+ (Corning), 1% penicillin/streptomycin. H295R cells were isolated from a primary adrenocortical tumour of a 48-year-old black female and are mitotane sensitive.
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MUC-1 human metastatic ACC cells were established by Hantel et al. (2016) and maintained in DMEM Advanced (Thermo Fisher) containing 5% fetal bovine serum (FBS) and 1% penicillin/streptomycin. Originally isolated from a neck metastasis of a 24-year-old male, MUC-1 cells are an aggressive, mitotane resistant model of ACC. HepG2 human hepatocellular carcinoma cells (HB-8065™M; (American Type Culture Collection)) were utilised as a comparator cell line and maintained in Eagle’s MEM (Thermo Fisher), containing 5% FBS, 1% penicillin/streptomycin (Di et al. 2012, Bruschi et al. 2019). Cells were grown in a humidified atmosphere containing 5%CO2 and 37°℃, used between passage 3-10 (H295R/HepG2) or passage 21-26 (MUC-1). H295Rs were obtained from ATCC (July 2017) and cells are routinely tested for steroid production, forskolin responsiveness and cell line characteristics.
Pharmacological treatments
Cells were treated at the indicated concentrations of GSK2033-LXRa antagonist (Bio-techne, Minneapolis, MN, USA) (Griffett & Burris 2016), SR9243-LXRa inverse agonist (Flaveny et al. 2015), 27-hydroxycholesterol-endogenous LXRa agonist (Enzo Life Sciences), T0901317-synthetic, non-steroidal LXRa agonist and mitotane (2,4’-DDD). Cells were cholesterol loaded by preparing supplemented media using 45 ug/mL water-soluble cholesterol methyl- B-cylodextrin. All drugs were prepared in DMSO and the vehicle control remained below 0.1% at all times. H295R cells were pretreated with GSK2033 (5 uM), SR9243 (1 uM) or 27HC (5 uM) for 18 h followed by mitotane (20, 40, 50 uM) for 6 h. MUC-1 cells were pretreated with SR9243 (5 uM) for 24 h followed by mitotane (50, 100 and 200 µM) for 24 h. Both cell lines were cholesterol loaded 1 h prior to mitotane treatment. Reagents were obtained from Sigma unless otherwise indicated.
Plasmids, transfection and luciferase assay
H295R were transfected using Lipofectamine 3000 (Thermo Fisher) using either pCMX-hLXRa dominant-negative (LXR-DN) or WT (LXR-WT) expressing plasmids(Willy et al. 1995). Transfection efficiency was evaluated using green fluorescent protein co-expression (pmaxGFP, Lonza) using microscopy and flow cytometry (Supplementary Fig. 1I and J, see section on supplementary materials given at the end of this article). H295R were transfected in antibiotic free media for 24 h prior to drug treatments. Luciferase assay was carried out using firefly (pGL3-TK-LXRRE-Luc) and
renilla luciferase vectors (10:1). Activity were measured following 24-h stimulation with LXRx agonist T0901317 (1 uM) using the Dual-Glo Luciferase Assay System (Promega) according to the manufacturer’s guidelines. Luminescence was recorded on the Synergy HT Multi-Detection Microplate Reader (BioTek), normalised for renilla luciferase activity and represented as relative light units (RLU).
Gene expression
Following drug treatments, cells were washed with cold phosphate buffered saline (PBS) and total RNA was extracted from adherent cells using TRI Reagent®. Following spectrophotometric quantification, 1 µg of total RNA was reverse transcribed into cDNA using the Qiagen RT2 first strand kit. PCR assay was carried out using Go Taq® Green Master Mix (Promega), according to manufacturer’s guidelines. Amplified products were separated using a 4% agarose gel, visualized using SYBR Safe (Thermo Fisher) stain and imaged using the ChemiDoc™M XRS+ Imaging system (Bio-Rad Laboratories). Real-time quantitative PCR expression was assayed on Applied Biosystems StepOne Plus (Applied Biosystems) and carried out using SYBR green mastermix (Promega). Primer sequences are listed in Supplementary Table 1. Fold change was calculated using the 44CT method. Data is represented as fold change of mRNA relative to vehicle control.
Western blotting
Samples were harvested on ice and lysed using radio- immuno-precipitation (RIPA) buffer and 1X protease inhibitor cocktail (Calbiochem). Lysates were quantified by BCA assay, denatured at 95℃ and separated by SDS-PAGE using a 10% Tris-glycine gel. Proteins were transferred to PVDF membrane, blocked using 5% milk and incubated with relevant antibodies. Membranes were incubated with primary antibodies overnight at 4℃ followed by relevant HRP-linked secondary antibodies (Supplementary Table 2). Imaging was carried out using the ChemiDoc™M XRS+ Imaging system (Bio-Rad Laboratories) with SuperSignal™M HRP substrate (Thermo Fisher) and Image Lab™ Software (Bio-rad, V5.2.1). Semi-quantitative densitometry was carried out using ImageJ and normalised to the loading control (ß Actin).
Cell death and apoptosis
H295R were grown as described and stained with Calcein AM (Invitrogen) (1 µM) and propidium iodide
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(PI) (5 µg/mL) to assess viability via microscopy, all images (10x) were taken using the EVOS® Cell Imaging System (Thermo Scientific). For quantitative analysis, cells were trypsinised and resuspended in FACS buffer (PBS, 1% FBS, 0.05% sodium azide) following treatment. AnnexinV:FITC (Bio-Rad) staining was carried out at 10 µL/106 cells for 30 min, followed by 5-min PI staining. All fluorochromes were excited using a 488 nm laser followed by 530/30 (AnnexinV:FITC) and 585/35 (PI) bandpass filter. Compensated flow cytometry was performed on FACS CantoII® with FACS DiVa 6.0® acquisition software (BD Biosciences) and FlowJo® V10 analysis software (Tree Star Inc., Ashland, OR, USA). Gating strategy is described in Supplementary Fig. 2. AnnexinV and PI positive cells are represented as % cells relative to vehicle control.
Metabolic activity assay
MTT assay was carried out in 96 well plates, cells were seeded at 1 × 103 cells per well and grown for 3, 7, 10 and 14 days. Drug treatments GSK2033 (5 µM) and SR9243 (1 µM) were given at the indicated time points (day 0, 3, 7 and 10) for 24 h followed by mitotane (50 uM) for 24 h. Following incubation, MTT reagent (0.5 mg/mL) was added. The assay was terminated by solubilising MTT using DMSO and absorbance was read at 570 nm as described previously. Experimental conditions were carried out in replicates of six and the experiment was repeated four times. Data is represented as % metabolic activity adjusted to matched vehicle control (100%) for each individual time point.
Cholesterol analysis
Filipin complex III (Sigma) from Streptomyces filipinensis was used to assess free cholesterol (Hassall & Graham 1995). Filipin is a fluorescent marker of FC that is excited by a 405-nm laser followed by a 450/50 bandpass filter. Cells were treated as indicated, harvested via trypsinisation and fixed using fixation buffer (BioLegend, San Diego, CA, USA) according to manufacturer’s guidelines. Staining was carried out at 1 mg/mL for 1 h at 4℃ in darkness and analysed by microscopy and flow cytometry. CholEsteryl BODIPYTM FL C12 (cholesteryl 4,4-difluoro-5,7- dimethyl-4-bora-3a,4a-diaza-s-indacene-3-dodecanoate) (Invitrogen) was used to label cholesterol esters (Hsieh et al. 2012). Cells were grown to 60% confluence and media was supplemented with 5 uM CholEsteryl BODIPY™M FL C12 overnight. Cells were harvested via trypsinisation and analysed by flow cytometry on the BD FACSCantoII
(BD Bioscience). Sytox blue (Invitrogen) (1 µM) was used as a viability dye. Fluorescence was recorded using a 488-nm excitation laser followed by a 530/30 bandpass filter (CholEsteryl BODIPY™M FL C12) and a 405-nm laser followed by 450/50 bandpass filter (Sytox Blue). Single, live cells were gated according to Supplementary Fig. 6 and the resolution metric was calculated as described (Brando & Sommaruga 1993). Additionally, cells were analysed via imaging flow cytometry using the Amnis® ImageStream®xMk II (Luminex Corporation, Seattle, WA, USA). High sensitivity mode (60x) was used to record 3500 events per sample. Analysis was carried out using IDEAS® software (V6.2) and, briefly, focused cells were gated according to Gradient RMS_M01_Ch01 (<50). Single cells were gated using Area_M01 vs Aspect Ratio_M01 (size vs circularity). Live cells were gated by using Sytox Blue (Invitrogen) viability dye according to Intensity_MC_ Ch07. The population of live, single, focused cells was used for analysis of CholEsteryl BODIPYTM FL C12 according to Intensity_MC_Ch02. Image display properties were standardised as follows: X Range (37, 563), Midpoint (300, 127) and X-Axis Scale (32, 568).
Data analysis
Drug synergism was evaluated using CompuSyn (download from www.compusyn.com) according to the Chou-Talalay method (Chou 2008). Data were input as single agent and combined (non-constant ratio) agents as mean±s.E.M. Pharmacological synergism was interpreted according to the combination index (CI) model. CI plots and data tables are available in Supplementary Fig. 1K, L and M. Linear regression and statistical analyses were performed using GraphPad® Prism V 8.0 (GraphPad Software). Data is represented as mean±s.E.M. unless stated otherwise. Paired sample analyses were performed using a two-sided Student’s t-test. Multiple-group comparisons were carried out using an ANOVA followed by Tukey’s post-hoc test. Statistical significance for two-tailed analyses (P-value) was assigned for values <0.05.
Results
LXRa inhibition combined with mitotane enhances ACC cell death and significantly reduces ACC cell metabolic activity, when compared to mitotane alone
Mitotane produced dose-dependent cytotoxicity in H295R in line with previous findings (15, 27 and 28) (Fig. 1A
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| Endocrine-Related | K M Warde et al. | LXRa, a novel therapeutic | 27:6 | 365 |
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and Supplementary Fig. 1A) with maximally observed adrenocortical cell death occurring at the therapeutic concentration of 50 µM (16 mg/L) (Fig. 1A). For the mitotane-resistant ACC cell line MUC-1, significant cell death was observed only at the supratherapeutic concentration of 200 µM mitotane (64 mg/L) (Fig. 1C and Supplementary Fig. 1D). Consistent with previous findings, cell death in MUC-1 (49.1%, mitotane 200 µM) was significantly lower than that observed for H295R (66.2%, mitotane 50 µM) (Hantel et al. 2016).
Co-treatment of H295R with LXRa inhibitors (GSK2033 (5 µM) or SR9243 (1 µM)) and mitotane significantly increased cell death at subtherapeutic mitotane concentration of 20 µM (16% (mitotane) vs 39% (GSK2033+mitotane), P<0.0001; 27% (SR9243+mitotane), P=0.0308). This effect was also present for co-treatment of either agent with 40 uM mitotane (32% (mitotane) vs 52% (GSK2033 +mitotane), P<0.0001; vs 47% (SR9243+mitotane) P=0.0006) and with 50 µM mitotane co-treated with SR9243 (66% (mitotane), 76% (SR9243+mitotane); P=0.0194) (Fig. 1A and B).
For MUC-1, LXRa inhibition with SR9243 only increased ACC cell death at mitotane 200 µM (46% (mitotane) vs 69% (SR9243+mitotane), P<0.0001) (Fig. 1C).
A time-course experiment demonstrated significantly reduced cell metabolic activity of H295R and MUC-1 in the presence of 50 µM mitotane alone or in combination with LXRa inhibitors (Fig. 1D, E and Supplementary Table 3). This effect was greater in H295R and reached significance at day 3 in H295R (18% (mitotane), P<0.0001; 15% (GSK2033+mitotane), P<0.0001; 9% (SR9243+mitotane) P<0.0001) and at day 7 in MUC-1 (72% (mitotane), P<0.0001; 58% (GSK2033+mitotane), P<0.0016; 60% (SR9243+mitotane), P<0.0089).
We validated these findings of pharmacological LXRa inhibition by transfecting H295R cells with a LXRx dominant-negative construct (LXRa-DN, transfection efficiency: 40%) that blocks LXRa-WT functioning (Supplementary Fig. 1G, H, I and J). LXRa-DN-expressing cells reached significantly higher rates of mitotane- induced cytotoxicity for all mitotane concentrations, compared to LXRa-WT (11% (WT:mitotane 20 µM) vs
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24% (DN:mitotane 20 µM), P=0.0044; 27% (WT:mitotane 40 µM) vs 53% (DN:mitotane 40 µM), P<0.001; 55% (WT:mitotane 50 µM) vs 67% (DN:mitotane 50 M), P=0.0089)) (Fig. 1F). These findings suggest an LXRx- mediated mechanism of enhanced mitotane-induced cytotoxicity. We validated these results by stimulating LXRa activity using the endogenous ligand oxysterol 27HC. 27HC reduced mitotane-induced cytotoxicity in H295R at concentrations between 10 and 40 µM (32% (mitotane) vs 27% (mitotane+27HC 10 µM), P=0.265; vs 15% (mitotane+27HC 20 µM), P=0.0002; vs 8% (mitotane+27HC 40 M), P<0.0001) (Fig. 1G).
Pharmacological inhibition of LXRa alone with GSK2033 or SR9243 reduced cell metabolic activity in both cell lines and this effect was similar across all timepoints (Fig. 1D and E). LXRa inhibition using GSK2033 but not SR9243 had a moderately induced dose-dependent cell death in H295R but not MUC-1 (Supplementary Fig. 1B, C, E and F). We calculated the combination index (CI) using CompuSyn to investigate cytotoxic mechanistic synergy between mitotane and LXRa inhibition. SR9243 demonstrated CI values <1.0, indicative of modest synergy with mitotane for its cytotoxic effects in H295R across all doses (0.7 (SR9243+mitotane 20 µM); 0.95 (SR9243+mitotane 40 µM); 0.64 (SR9243+mitotane 50 M); 0.59 (GSK2033+mitotane 20 µM); 0.86 (GSK2033+mitotane 40 M); 0.84 (GSK2033+mitotane 50 µM)) and for MUC-1 at mitotane 200 µM only
(0.81 (SR9243+mitotane 200 µM)) (Supplementary Fig. 1K, L and M).
The early apoptosis marker AnnexinV increased dose- dependent for all mitotane concentrations in the presence and absence of GSK2033 or SR9243 in H295R (Fig. 2A). The combination of mitotane with GSK2033 resulted in higher AnnexinV expression vs 40 µM mitotane alone (32% (mitotane 40 µM) vs 50% (GSK2033+mitotane 40 µM), P=0.0004). Combination with SR9243 demonstrated higher AnnexinV expression vs all mitotane alone (10% (mitotane 20 µM) vs 26% (SR9243+mitotane 20 µM), P=0.0008; 32% (mitotane 40 µM) vs 53% (SR9243+mitotane 40 µM), P<0.0001; 52% (mitotane 50 „M) vs 67% (SR9243 +mitotane 50 µM), P=0.0008). The late apoptosis marker, cleaved caspase 3, was also increased for mitotane at doses of 40 µM and 50 µM, reflective of the higher cell death at these mitotane concentrations. Higher cleaved-caspase 3 expression was present for the combination with either LXRa inhibitor vs 40 µM or 50 uM mitotane alone (Fig. 2B and Supplementary Fig. 3A, B). There was also higher expression of the ER stress markers CHOP and XBP1s/u in mitotane-treated H295R across all concentrations, which increased in combination with either LXRa inhibitor (Fig. 2C).
For MUC-1, higher cell death at 200 µM mitotane was also reflected in higher expression of AnnexinV, which in turn was significantly higher with LXRa inhibition with SR9234 (3% (VehicleControl) vs 22.6% (mitotane 50 µM),
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P<0.0001; 22.6% (mitotane 50 µM) vs 39% (SR9243 mitotane 50 µM), P<0.0001)) (Fig. 2D).
LXRa inhibition reduces expression of cholesterol efflux pumps in H295R and MUC-1 ACC cells
In H295R and MUC-1, LXRa expression at baseline (Fig. 3A and B) was equivalent to expression in the positive control HepG2 hepatocellular carcinoma cells. Similarly, high expression levels of the oxysterol synthetic enzyme CYP27A1 were detected (Fig. 3A and B). Transfection with a luciferase construct under the control of an
LXRa-responsive element (TK-LXRRE-Luc) showed significant constitutive baseline activation of LXRx, which was increased by stimulation with the LXRx agonist T0901317 (1 µM) (Fig. 3C). These data indicate high activity of the LXRx/oxysterol pathway in adrenal cells, equivalent to that of hepatic tissue.
Expression of LXRa target genes, the FC efflux pumps, ABCA1 and ABCG1, were reduced by each LXRa inhibitor in H295R and MUC-1, respectively (Fig. 3D, E, F, G and Supplementary Fig. 4A, B, C, D). In line with these findings, expression of ABCA1 and ABCG1 increased in both cell lines when stimulated using the non-steroidal
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LXRa agonist T0901317 (Fig. 3D, E, F and G). Expression for ABCA1 and ABCG1 also decreased in the presence of the LXRa-DN construct (Fig. 3H), confirming direct involvement of LXRa in their expression.
The responses of ABCA1 and ABCG1 in the presence of increasing concentrations of mitotane did not significantly change (Fig. 3I and J). However, the efficacy of GSK2033 or SR9243 to reduce ABCA1 and ABCG1 expression were attenuated with mitotane treatment in a dose-dependent manner, which is unlikely to reflect a direct effect of mitotane on cholesterol efflux pumps. However, this may be explained by increasing intracellular FC accumulation at higher mitotane doses. We next investigated intracellular cholesterol within this model.
LXRa inhibition enhances mitotane-induced toxic accumulation of free cholesterol in H295R ACC cells
Mitotane exposure resulted in a dose-dependent increase in intracellular FC in H295R, reaching significance at all
mitotane concentrations (Fig. 4A) (15, 16). The inhibition of LXRx with GSK2033 and SR9243 significantly increased intracellular FC in H295R at baseline and in combination with mitotane, with higher levels for each dose of mitotane vs mitotane alone (Fig. 4A and Supplementary Fig. 5A). For MUC-1, only the cytotoxic 200-uM mitotane concentration resulted in a significant increase in intracellular FC, increased further with SR9243 (Fig. 4B). Cell death and intracellular cholesterol correlated for both cell lines: H295R (r2=0.5210, P=0.008) and MUC-1 (r2=0.9299; P=0.0001) (Supplementary Fig. 5B and C). While intracellular FC differed in response to mitotane and LXRa inhibition, baseline levels were similar for H295R and MUC-1 (Fig. 4C and D). Interestingly, intracellular lipid droplet storage of CE was undetectable in MUC-1, when compared to H295R (Fig. 4E, F, G and Supplementary Fig. 6A, B).
We next evaluated mitotane-induced cytotoxicity, in the presence and absence of LXRa inhibition, for each cell line under cholesterol-loaded cell culture conditions. Cholesterol
A
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MUC-1
C
D
E
2.0
Vehicle
2.0
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Free Cholesterol (Filipin Staining Metric)
GSK2033
Free Cholesterol (Filipin Staining Metric)
Vehicle
Free Cholesterol (Filipin)
SR9243
H295R
MUC-1
SR9243
UNSTAINED
400-UNSTAINED
Resolution Metric
H295R
MUC-1
1.5-
1UNSTAINED
1.5
=
1.5
STAINED
STAINED
STAINED
-
STAINED
Count
1.0-
Count
1.0
T
1.0
0.5-
UNSTAINED
0.0
405_450_50-A
H295R
MUC-1
488_530_30-A Cholesteryl Ester
0.5
0.5-
Free Cholesterol (Filipin)
0
20
40
50
0
50
100
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Mitotane (µM)
Mitotane (uM)
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G
H
H295R
I
MUC-1
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Bright field
Cholesterol Esters
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Vehicle + Cholesterol
1.5-
120
100
**
Vehicle + Cholesterçı
GSK2033 + Cholesterol
20-
SR9243 + Cholestery|
Ch01
Ch02
10-
SR9243 + Cholesterol
-
Cholesteryl Ester Resolution Metric
% Dead Cells
% Dead Cells
3022
80
10-
1.0-
H295R
% Dead cells
Cholesterol
80
% Dead cells
60
Cholesterol
**** 7 um
0.5-
Ch01
Ch02
1283
40
0.0-
MUC-1
40
H295R
MUC1
20
… 7 pm
0
0
0
20
40
50
0
50
100
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Mitotane (μM)
Mitotane (uM)
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loading alone induced a moderate but significant increase in percentage cell death for both H295R (2% (baseline) vs 15% (cholesterol loaded), P<0.001) and MUC-1 (3% (baseline) vs 20% (cholesterol loaded), P=0.0068) when compared to non-loaded cell culture conditions. Treatment with each LXRa inhibitor resulted in a two-fold increase in H295R cell death in cholesterol-loaded cells. When combined with mitotane, both pharmacological LXRx inhibitors demonstrated significantly higher cell death for subtherapeutic doses of mitotane, with maximally observed cell death at 40 µM (12.4 mg/L) (Fig. 4H). Cholesterol loading of MUC-1 resulted in an increased cell death at 100 µM and 200 µM mitotane (7% (baseline mitotane 100 µM) vs 19% (cholesterol-loaded mitotane 100 µM), P<0.011) and 200 µM (46% (baseline mitotane 200 µM) vs 62% (cholesterol-loaded mitotane 200 µM), P<0.003)). The LXRx inverse agonist SR9243 only significantly increased cell death when combined with mitotane at 200 uM (Fig. 4I).
SOAT1 expression was significantly reduced by mitotane at doses <40 uM in H295R (Supplementary Fig. 5D). However, SOAT1 expression was unaffected by LXRx inhibition alone in both cell lines (Supplementary Fig. 5E and F), suggesting that intracellular FC is increasing due to the alternative mechanism of reduced efflux pump expression (Fig. 3).
Discussion
Adrenocortical carcinoma (ACC) has demonstrated resistance to most cytotoxic chemotherapeutic approaches, with mitotane representing the single best pharmacotherapeutic for disease control; however, with a limited therapeutic window. Recent work demonstrated the putative adrenotoxic mechanism of mitotane through inhibition of the enzyme SOAT1, resulting in intracellular FC accumulation and suggests SOAT1-specific inhibitors as stand-alone therapy or adjuncts to mitotane in the management of ACC (Sbiera et al. 2015, LaPensee et al. 2016). In the study presented herein, we explored LXRa/cholesterol efflux pathway and proposed this as a complementary mechanism to enhance toxic intracellular FC accumulation in ACC. We investigated these effects on two validated in vitro models of ACC: H295R cells which are mitotane-sensitive and MUC-1, a metastatic, mitotane-insensitive cell line (Hantel et al. 2016).
Transcellular cholesterol flux in steroidogenic cells, such as ACC, is central to cellular function and cholesterol provides the principle substrate for steroidogenesis. In steroidogenic cells intracellular cholesterol (1) is stored
within lipid droplets following conversion to cholesteryl esters by SOAT1 (Cignarella et al. 2005, Dove et al. 2006); (2) provides a substrate for steroidogenesis following transfer to the mitochondrion via the STAR protein (Stocco & Clark 1996) or (3) is removed from the cells by the cholesterol efflux pumps, ABCA1 or ABCG1 to circulating ApoA1 and HDL1, respectively (Kraemer 2007). Cholesterol efflux is tightly regulated by the oxysterol/LXRa system through conversion of surplus FC to oxysterols through the action of enzymes such as CYP27A1. In the adrenal, the role of LXRa and its ligand oxysterols are of key relevance in all of these processes. This was highlighted by Cummins et al. who demonstrated the contribution of oxysterol/LXRa to (1) regulate steroidogenesis, (2) control adrenocortical cholesterol metabolism and (3) act as a ‘safety valve’ through the ABCA1/ABCG1-mediated efflux pathway, to provide a basal protective mechanism in preventing free-cholesterol induced adrenal lipotoxicity (Cummins et al. 2006).
Our data show that pharmacological inhibition or functional blockade of LXRa significantly reduced cholesterol efflux pump expression (ABCA1 and ABCG1) and is accompanied by higher intracellular FC concentrations, ER stress, apoptosis and cell death markers. Using the combined therapeutic approach, the mitotane- sensitive H295R underwent apoptosis and cell death at subtherapeutic mitotane concentrations. However, MUC-1, while combined mitotane/LXRa inhibition considerably enhanced the cytotoxic effect of mitotane alone, retained their resistance to pharmacologically acceptable mitotane concentrations below 200 uM. In both cell lines, higher intracellular FC levels were associated with increased cell death and when challenged with a cholesterol- loaded extracellular environment, the cytotoxic effect of mitotane alone and in combination with LXRx inhibition was further enhanced. These findings support our overarching hypothesis and are also in line with the findings of other groups (Sbiera and La Pensee) who have investigated SOAT1 inhibition (Sbiera et al. 2015, LaPensee et al. 2016). While H295R were very sensitive to combined LXRa/mitotane treatment and MUC-1 demonstrated enhanced sensitivity to the combination at high mitotane doses, MUC-1 gave disappointing results in terms of a therapeutic strategy. However, when taken together, we believe our data convincingly support a role for LXRa and cholesterol storage/efflux in ACC cell adaptation and survival.
It is unclear why MUC-1 are insensitive to LXRx/ mitotane treatment. MUC-1 were derived from a metastatic neck lesion in a young, mitotane-resistant patient and
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for whom four cycles of combination chemotherapy were unsuccessful in limiting the extent disease spread. When we evaluated intracellular cholesterol in MUC-1, we demonstrated an almost complete absence of stored cholesteryl esters (CE) at baseline and even under cholesterol-loaded conditions (data not shown). In contrast, mitotane-sensitive H295R supported a rich CE store within their intracellular lipid droplets under baseline and cholesterol-loaded culture conditions. Yet, in spite of markedly different intracellular CE stores, intracellular FC was similar for both cell lines. The difference in intracellular cholesterol handling between MUC-1 and H295R is interesting, particularly in the context of the putative mechanism of mitotane activity through SOAT1. We did not perform a SOAT1 activity assay; however, the reduced storage of CE in MUC-1 in the presence of similar FC suggests low baseline SOAT1 activity, irrespective of the expression of this enzyme. This also suggests that, in contrast to H295R, MUC-1 favor alternative mechanism(s) of regulation and clearance of intracellular cholesterol, providing a possible escape mechanism from mitotane-induced lipotoxicity. Seidel et al. have described similar findings in relation to FC and CE handling in a strain of HAC15 with induced resistance to mitotane (Seidel et al. 2020). Detailed evaluation of lipid/cholesterol metabolism in ACC, using the full range of cell lines and banked tumour samples, is necessary to evaluate the significance for development of future therapeutic strategies.
In the presence of increasing FC accumulation, higher mitotane doses attenuated the inhibitory effect of LXRa blockade on cholesterol efflux pump expression in H295R. In our study, mitotane alone had no significant effect on either ABCA1 or ABCG1 expression. Sbeira et al. previously demonstrated a short-lived decrease in ABCG1 which quickly increased back to baseline with prolonged therapy (Sbiera et al. 2015). It is therefore unlikely that this is a direct pharmacodynamic effect of mitotane. It is a possible secondary effect of intracellular FC accumulation which is a substrate for catalysis to 27HC by CYP27A1 and will compete with the LXRa antagonists. In line with this observation, we have also demonstrated that stimulating LXRa with 27HC reduces the therapeutic efficacy of mitotane. Whether or not this represents a mechanism whereby ACC cells can overcome long-term susceptibility to mitotane needs more detailed investigation.
The role of LXRa in supporting the cancer microenvironment and promoting cancer cell survival is established in other human cancer models
(Kim et al. 2018, Wang et al. 2019). Higher tumour grade and enhanced metastasis in breast cancer have been associated with higher LXRa expression and activation (Nelson et al. 2013). Work by Flaveny et al. also demonstrated that the LXRa inverse agonist SR9243 induced apoptosis across models of lung, colon and prostate cancer (Flaveny et al. 2015). Other work has demonstrated the potential for LXRa inhibition to induce lipotoxicity through FC accumulation (Schuster et al. 2002, Bradley et al. 2007).
We propose that, based on our date, the use of LXRx inhibitors can be translated into a therapeutic strategy for mitotane-sensitive ACC by adopting a complementary approach to one of mitotane’s known mechanisms of action: intracellular FC-induced lipotoxicity. We show that enhanced FC accumulation within H295R in response to LXRa blockade increased the cytotoxicity of mitotane at half the usual minimum therapeutic dose. The main limitations to mitotane’s clinical use are (1) no significant improvements in progression or recurrence- free survival of disease below 14 mg/L (Terzolo et al. 2013, Berruti et al. 2017) and (2) poor patient tolerability, with significant impact on quality of life and inability to continue therapy above 20 mg/mL (Haak et al. 1994). Recent data have suggested that adjunctive mitotane should continue indefinitely even in individuals with R0 resection without tumour recurrence (Berruti et al. 2017). Therefore, the development of strategies to facilitate the long-term tolerability of this drug is an important clinical consideration. In relation to mitotane- resistant disease, we demonstrated increased cell death for MUC-1 in response to combined mitotane and LXRx inhibition, but show that mitotane-resistance was not overcome. Therefore, while adopting this combination strategy offers promise in mitotane-sensitive disease and to enhance adjuvant mitotane, it is unlikely to be of benefit in disease that is mitotane resistant. However, the differences in cholesterol handling between mitotane- sensitive and mitotane-resistant ACC cells demonstrate the merits of better understanding the adaptation of ACC cells to facilitate metastasis and cell survival. Finally, we propose that the selective induction of high cholesterol uptake or selective delivery of cholesterol to ACC cells as a combination therapy represents an interesting challenge for future translational research.
In summary, two cell lines representing some of the best validated human cell culture models of ACC, the mitotane-resistant metastatic MUC-1 cell line and the mitotane-sensitive H295R, representing the standard for early mechanistic/therapeutic investigation, were
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used to investigate LXRa inhibitors and mitotane’s effect to induce adrenal cytotoxicity (Rainey et al. 1994, Bird et al. 1995, Wang & Rainey 2012, Hantel et al. 2016). Our data suggest a complementary pathway to enhance mitotane-induced cytotoxicity by preventing FC efflux from ACC cells, mediated through blockade of the LXRa pathway and enhanced by cholesterol loading. Therefore, it is reasonable to conclude that the mitotane- LXRa inhibition combined therapeutic approach exploits separate but complementary and synergistic mechanisms to accumulate toxic levels of FC and to induce ACC cytotoxicity. The findings provide valuable mechanistic insights and an important backdrop to support further animal and pre-clinical studies of the effects of LXRx inhibition as a therapeutic target for ACC in mitotane- sensitive disease. Of the two pharmacological inhibitors chosen for investigation, the inverse agonist SR9243 is well tolerated in animals and has a favorable toxicity profile (Flaveny et al. 2015, Wu et al. 2019). This drug therefore presents good translational feasibility in future in vivo studies. We also highlight the ongoing challenge of approaching effective strategies for drug- resistant metastatic disease and the importance of better understanding cholesterol metabolism in ACC cells in this regard.
Supplementary materials
This is linked to the online version of the paper at https://doi.org/10.1530/ ERC-20-0031.
Declaration of interest
The authors declare that there is no conflict of interest that could be perceived as prejudicing the impartiality of the research reported.
Funding
K M W is supported by the Irish Research Council Government of Ireland Postgraduate Research Scholarship. K V C and E S are supported by the Wellcome Trust (210755/Z/18/Z) and K V C is supported by the NIHR Cambridge Biomedical Centre. E R M is supported by a EPRSC-SFI LifETIME CDT postgraduate PhD research scholarship. C H is supported by the Uniscientia Foundation (Keyword Tumor Model). This work is also supported by the Irish Endocrine Society Basic Science Research Grant and by the Postgraduate Scholarship Fund at the School of Medicine, NUI Galway.
Acknowledgements
The authors would like to thank Ms Coralie Mureau and Dr Mark Webber for their technical assistance at The Lambe Institute for Translational Research. The authors would also like to thank Dr Shirley Hanley, Dr Joana Cabral and Dr Dagmar Quandt at the NUI Galway Flow Cytometry Core Facility.
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Received in final form 4 April 2020 Accepted 9 April 2020 Accepted Manuscript published online 9 April 2020
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