ABSTRACT
Desmoplastic small round cell tumor (DSRCT) is an aggressive, usually incurable sarcoma subtype that predominantly occurs in post-pubertal young males. Recent evidence suggests that the androgen receptor (AR) can promote tumor progression in DSRCTs. However, the mechanism of AR-induced oncogenic stimulation remains undetermined. Herein, we demonstrate that enzalutamide and AR-directed antisense oligonucleotides (AR-ASO) block 5α-dihydrotestosterone (DHT)-induced DSRCT cell proliferation and reduce xenograft tumor burden. Gene expression analysis and chromatin immunoprecipitation sequencing (ChIP-seq) were performed to elucidate how AR signaling regulates cellular epigenetic programs. Remarkably, ChIP-seq revealed novel DSRCT-specific AR DNA binding sites adjacent to key oncogenic regulators, including WT1 (the C-terminal partner of the pathognomonic fusion protein) and FOXF1. Additionally, AR occupied enhancer sites that regulate the Wnt pathway, neural differentiation, and embryonic organ development, implicating AR in dysfunctional cell lineage commitment. Our findings have immediate clinical implications given the widespread availability of FDA-approved androgen-targeted agents used for prostate cancer.
ONE SENTENCE SUMMARY We demonstrate that DSRCT, an aggressive pediatric cancer, is an AR-driven malignancy capable of responding to androgen deprivation therapy.
INTRODUCTION
Desmoplastic small round cell tumor (DSRCT) is an aggressive soft-tissue malignancy that usually presents in post-pubertal adolescents and young adults as a large intra-abdominal mass together with widespread coating of serosal and subdiaphragmatic surfaces by hundreds to thousands of malignant nodules. Given the inconspicuous tumor location, nearly all patients present in an advanced-stage with symptoms of abdominal pain or distention, nausea, constipation, and weight loss1.
DSRCT’s cell of origin is unknown, and these tumors universally exhibit a high-grade, poorly differentiated state characterized by cellular nests of unclear lineage, seeming to show epithelial, muscular, mesenchymal, and neural differentiation admixed with prominent desmoplastic stroma2–4. Given its rarity, with an age-adjusted incidence peak incidence of 0.3-0.74 cases per million,5 it wasn’t until 1989 that Gerald and Rosai first described DSRCT as a unique clinicopathologic disease6. Shortly thereafter, cytogenetic analyses demonstrated that DSRCT tumors harbor a pathognomonic t(11;22)(p13:q12) chromosomal translocation that pairs the Ewing sarcoma (ES) gene (EWSR1) with the Wilms tumor suppressor gene (WT1)6–9. The resulting chimeric 59 kDa fusion protein (FP), in concert with the heterozygous functional loss of the WT1 tumor suppressor protein, promotes an oncogenic effect that reinforces tumor survival and growth10.
The PI3K/AKT and androgen receptor (AR) signaling cascades are among the most frequently activated in cancer11,12. Given the striking observation that 90% of DSRCT cases occur in post-pubertal males (with an average age at diagnosis of 21.4 years), we investigated how AR contributes to tumorigenesis and survival4,13,14. A potential connection between the AR and DSRCT, first reported by Fine et al. in 2006, studied a series of twenty-seven advanced-stage DSRCT patients who had progressed through at least two chemotherapy regimens15. In that retrospective multi-center analysis, 37% of the samples were ≥2+ by immunohistochemistry, and surprisingly, three of six AR+ patients transiently benefited from 1st-generation combined androgen blockade (CAB) using Lupron and bicalutamide. Despite that promising signal of activity, AR-targeting has not been pursued further in the clinic, and at the time of this writing, no additional studies were reported in the literature.
In the present work, we use DSRCT xenografts and patient-derived tumor explants (PDXs) to extend the findings by Fine et al. to modern-day AR-targeted therapies, such as enzalutamide, that form the backbone of prostate cancer treatment16. Additionally, we present promising efficacy data using an experimental AR-targeted antisense oligonucleotide (ASO) that significantly delayed tumor growth by suppressing AR expression. Finally, we present chromatin immunoprecipitation sequencing (ChIP-seq) results that suggest a new mechanistic understanding of AR’s role in DSRCT tumorgenicity. Our research findings substantiate DSRCT as a second AR-driven malignancy, have direct implications for DSRCT treatment, and implicitly suggest a path towards clinical trials that center on AR-directed treatment options for this otherwise intractable pediatric cancer.
RESULTS
Protein expression in DSRCT differs substantially from ES
Given the differences in clinical presentation, tumor biology, and response to biologically targeted therapies, we conducted a reverse-phase protein lysate array (RPPA) to identify proteins enriched in DSRCT. To determine tumor-specific proteins, we compared protein lysates from DSRCT nodules and paired adjacent normalappearing mesenteric tissue from the same patients using a well-described RPPA platform enriched for known oncoproteins (Fig. S1)17–19. Unsupervised double hierarchical clustering correctly separated normal mesenteric tissues from DSRCT, which over-expressed Akt, Syk, PKC-α, and other proteins. Next, we identified proteins enriched in DSRCT compared to another malignancy, using ES as the closest molecular cousin that shares an N-terminus EWSR1 fusion partner. Interestingly, AR and Syk proteins were upregulated in most DSRCT specimens but nearly undetectable in ES (Fig 1A-B). The RPPA data, validated by Western blots, provides the first screen of proteins enriched in DSRCT (Fig. 1C-D).
Expression of AR in DSRCT primary tumors
Since AR activity requires androgen-mediated nuclear translocation, we created a DSRCT-specific tissue microarray (TMA) from sixty cases treated at MD Anderson Cancer Center (MDACC) to determine the prevalence and cellular distribution of AR staining in patients treated at a single institution. Seventy-five percent of the cores available for analysis were positive for nuclear AR by immunohistochemistry (Fig. 2A-B and Fig. S2A-C), usually more prominently in the epithelioid cells rather than the desmoplastic stromal cells. Of the AR-positive samples, 7% showed focal AR expression in 10-50% rare, scattered cells and could be of any intensity (low positive AR expression), 3.3% had low AR expression where only 1-10% of cells are positive for AR expression (focal expression), and 25% demonstrated negative AR expression (where only 0-1% of cells are positive). 65% showed high AR expression, defined by AR-positivity in >50% of a sample’s cells (Fig. 2B and Fig. S2C). High-intensity staining was defined as completely obscuring the nuclear hematoxylin counterstain, while moderate staining allowed visualization of the stain. Weak staining required examination of the cells at least 200X to detect staining reliably. As an additional metric of AR expression, we evaluated an additional 12 DSRCT patient tumors for AR expression by Western blotting: 42% of the tumors showed high AR expression, 33% had moderate AR expression, and 25% were AR-negative (Fig. 2C & 2D). As IHC and Western blotting revealed moderate to high AR expression in ~three-quarters of the DSRCT cases assessed, this seemed to substantiate the RPPA results.
Genomic profiling of DSRCT, PC, and other sarcoma primary tumor samples
Given the male predominance of DSRCT, new AR protein expression data, and known abundance of AR-targeted therapies used for prostate cancer, we elected to pursue AR as a potential therapeutic target in DSRCT. The case report by Fine et al. hinted that DSRCT patients can respond briefly to a 1st-generation CAB, which heightened our enthusiasm to investigate how AR signaling contributes to DSRCT biology15.
Given the AR’s central role in prostate cancer (PC) growth and survival, and deep mechanistic understanding in that malignancy20–23, we performed a gene expression analysis comparing 22 DSRCT samples to 12 PC samples and a group of other diverse sarcoma subtypes, including 7 chondrosarcomas, 7 well-differentiated liposarcomas (WDLPS), 10 dedifferentiated liposarcoma (DDLPS), and 47 osteosarcoma samples, which served as negative controls. As expected, DSRCT demonstrated significant AR upregulation compared to these other sarcoma samples from chondrosarcoma, well-differentiated and dedifferentiated liposarcoma, and osteosarcoma (p< 0.01 – p<0.0001) but did not surpass the levels observed in PC (Fig. 2E-F).
Compared to other sarcoma subtypes, most DSRCT samples clustered together based upon their expression of 89 genes associated with the androgen pathway, as defined by KEGG (Fig. S2D). Similarly, DSRCT samples clustered together by their expression of 55 genes linked to canonical androgen signaling (Supplemental Fig. 2F). Pathway analysis revealed other cancer pathways enriched in DSRCT compared to other sarcoma subtypes. This included the cell adhesion molecule (CAM) communication pathway that regulates cell invasion through a coordinated balance between adhesion and detachment of cells24,25 and the extracellular matrix (ECM) interaction pathway, known to initiate cell motility across the ECM barrier26.
Characterizing extranuclear partners of AR and its nuclear cofactors
AR splice variants (AR-Vs) have been implicated in PC tumor progression, an increased risk of biochemical relapse, and inferior overall survival outcomes27–29. To determine if variant forms of AR exist in DSRCT, we assessed AR-V7 expression within a cohort of twelve consecutive DSRCT patients. As none of the initial twelve samples expressed AR-V by IHC, we elected not to examine this further in the broader sample set.
As AR activity can be influenced by integrins and transcriptional co-regulators30,31, we evaluated these AR activators within the same cohort of 11 DSRCT tumors at the proteomic level using a western blotting analysis. Among three alpha integrin (ITGAV, ITGA4, and ITGA5) and beta integrin (ITGB1, ITGB3, and ITGB5) subunits commonly observed in mesenchymal tissues, protein expression varied considerably and did not correlate with AR expression (Fig. S3A).
Since the epigenetic effects of AR can be modified by cofactor binding and matrix metalloproteins, we assessed whether steroid receptor coactivators NCOA1/2/3 or MMP2/13 contribute to the development of DSRCT through AR-dependent mechanisms32–37. To accomplish this, we performed a Western blot of 11 primary DSRCT tumors and the JN-DSRCT and LNCaP PC cell lines. The three-NCOA biomarkers demonstrated heterogeneous expression in the DSRCT clinical samples proportional to their AR expression (Fig. S3B). However, the JN-DSRCT cells showed low expression of NCOA1/2 and equivalent expression of NCOA2 versus LNCaP PC cells (Fig. S3C). Further investigation with a larger sample set will be required to determine how the AR-dependent integrin/NCOA-dependent pathway impacts DSRCT cell migration and death.
In vitro stimulation and inhibition of DSRCT proliferation via AR
Though AR activation by testosterone and DHT leads to brisk PC cell proliferation38, it was uncertain whether DSRCT cells similarly relied upon AR signaling for proliferation, growth, and survival. To evaluate this, we performed in vitro cell proliferation assays following DHT-mediated AR stimulation in JN-DSRCT; AR-expressing LNCaP PC cells, AR-non-expressing PC3 PC cells, and ES TC71 cells that were used as positive or negative controls. As hypothesized, DHT stimulation increased cell proliferation of JN-DSRCT and LNCaP cells compared to PC3 and ES cells (Fig. 3A). As measured by Western blotting, we confirmed strong AR expression by LNCaP and JN-DSRCT cell lines following DHT stimulation in contrast to its absence in the TC71 ES and PC3 prostate cancer cells (Fig. 3B). Next, we performed confocal immunofluorescence staining of these cells to determine if (and how quickly) DHT-mediated stimulation would facilitate AR transmigration from the cytoplasm into the cell nucleus. Our results suggest that AR-upregulation begins within 5 hours of DHT exposure and peaks in JN-DSRCT, or decreases in LNCaP cells at 24 hours (Fig. 3C-D).
Having shown that DHT stimulates DSRCT cells, we explored whether FDA-approved and experimental AR antagonists had an antiproliferative effect. Both enzalutamide (Fig. 3E) and the novel AR-ASO (IONIS 560131; formerly AZD5312) significantly slowed DSRCT cell proliferation at two weeks (Fig. 3F) and reduced AR expression (Fig. 3G). However, the in vitro antiproliferative effect was 4-fold more effective in the cells treated with the AR-targeted antisense blockade (Fig. 3E & 3F). Notably, this antineoplastic effect required 72-hours of DHT pretreatment (Fig. S4). Altogether, this data indicates a vital role for DHT-stimulated AR expression in DSRCT cell proliferation and conclusively demonstrates a potent antineoplastic effect of AR antagonists.
Preclinical efficacy of AR-based targeted therapy for the treatment of DSRCT
Since only one DSRCT cell line exists, we extended our evaluation of the AR antagonists to the in vivo setting using the JN-DSRCT xenograft and available DSRCT patient-derived tumor explants (PDXs). Immunocompromised NSG mice bearing JN-DSRCT xenograft tumors treated with enzalutamide or AR-ASO significantly reduced tumor burden and improved survival with the same efficacy, compared to placebo or control groups during the first two months of treatment (Fig. 4A-B). At two months, tumor growth began to accelerate in the enzalutamide-treated mice, whereas growth suppression continued in the mice treated with either 25 or 50 mg/kg of the AR-ASO (p<0.0001; Fig. 4A). Compared to enzalutamide, the AR-targeted ASO (25 and 50 mg/kg) demonstrated superior antineoplastic activity (Fig. 4A; p<0.0001 or p=0.006, respectively). The effects of AR-ASO and control ASOs were also assessed in NSG mice (5 mice/group) bearing a DSRCT PDX (Fig. 4D-F). As expected, tumor growth and Kaplan-Meier curves revealed that tumors treated with AR-ASO have significantly reduced tumor burden and improved survival compared to control ASO group (p=0.0097 & p<0.0001, respectively).
Though both agents delayed tumor growth, AR-ASOs were more effective than enzalutamide in both preclinical models. Therefore, our pharmacodynamic analysis focused primarily on the effect of AR-ASO treatment. Proteomic profiling by RPPA (Fig. 5A), Western blotting (Fig. 5B & C), immunofluorescence (Fig. 5D & E & Fig. S5A-C), and immunohistochemistry (Fig. 5F-H & Fig. S5D-F) validated the AR-ASO mediated knockdown of AR expression in the xenograft and PDX. To further characterize how the AR-ASO differed from enzalutamide mechanistically, we performed liquid chromatography tandem mass spectrometry (LC/MS/MS) analysis of 38 collected preclinical animal specimens shown in Figure 4. Consistent with prior literature in PC, loss of AR following AR-ASO treatment destabilized testosterone and reduced its intratumoral expression (Fig. S6)39,40. As a negative control, the corticosterone levels were unchanged by AR-blockade. Additionally, since the antineoplastic action of enzalutamide works by preventing ligand-AR binding, reducing AR shuttling to the nucleus, and impairing AR DNA binding affinity – instead of reducing AR levels (Fig. S7; panels A-E) – enzalutamide-treatment did not significantly lower intratumoral testosterone.
To gain a preliminary understanding of the short-term pharmacodynamic effects of AR suppression, a group of JN-DSRCT xenografts and DSRCT PDXs was collected 10 days into their AR-ASO treatment (Fig. 5A AR-ASO PD) for analysis by RPPA to assess early compensatory pharmacodynamic changes. pS6, Akt, ER, PD-1L, pAKT, and other proteins (Figure 5A and Supplemental Figure 7F-G) were upregulated. Others have reported that the PI3K-AKT pathway has pleiotropic effects in survival, proliferation, metabolism, and growth pathways of several malignancies41, and its blockade has long been of interest in managing PC, where a compensatory increase in AKT signaling can occur following AR inhibition42. Notably, the same AR-ASO (AZD5312) used in our preclinical experiments was well-tolerated when administered to PC patients (NCT03300505). Therefore, one could theoretically investigate this AR-ASO drug candidate in DSRCT-specific phase 2 trials without delay. Given the limited nature of our preclinical studies, future studies with enzalutamide is also of interest.
AR directly regulates important oncogenic regulators in DSRCT
To model the AR transcriptional program in a human JN-DSRCT cell line, we determined the genome-wide AR binding profiles using ChIP-Seq experiments in unstimulated or DHT-stimulated JN-DSRCT cells treated with control ASO or AR-ASO. As expected, DHT treatment enhanced AR binding to the chromatin as assessed by the average intensity plot on all significant peaks (p < 1e-7) and heat map (Fig. 6A). DHT stimulation led to ~4000 new peaks that were suppressed by treatment with AR ASO (Fig. 6B and Supplemental Table 1). These binding sites were enriched at known AR response elements (AREs) and in sites for FOXA1, a transcription factor known to open compacted DNA and cooperate with AR in prostate cancer43 (Fig. 6C and Supplemental Table 1). Consistent with DSRCT’s pathogenesis, we also noted enrichment of WT1 binding motifs within AR binding peaks (Fig. 6C) suggesting potential interactions between AR, FOXA1, and WT1 in JN-DSRCT cells. To further characterize the genes adjacent to AR binding site peaks, we performed a pathway analysis using 700 genes that are direct targets of AR. Upregulated pathways included the TNFa pathway, Hippo signaling, and pluripotency regulators (Fig. 6D and Supplemental Table 1), and key genes included WT1, CTNNB1, SOX2, GLI2, FOXF1 and GATA6 (Fig. 6E, Fig. S8D and Supplemental Table 1).
After evaluating the effects of androgen stimulation and withdrawal in JN-DSRCT cells, we next compared DSRCT to data from PC cells. Significant overlap existed at sites for AR binding at AREs (Fig. S8A), FOXA1 motifs (Fig. S8B), and sites that regulate key cancer pathways, including WNT, TGFβ, PI3K, MAPK, Hippo signaling, TNFα and epithelial-to-mesenchymal transformation (EMT) (Fig. S8C). To further evaluate the AR regulatory function in DSRCT tumor mouse models, we performed ChIP-seq on DSRCT-xenograft and PDX samples. Consistent with the cell line data, we observed suppressed AR binding to the chromatin by the treatment with AR ASO (Fig. S9A-B). Similarly, pathway analysis of the top 5000 lost AR binding sites targeted genes showed enrichment of MAPK pathway, Hippo signaling, Wnt signaling and pluripotency regulators (Fig. S9C-D). We also noted enrichment of AR and FOX family binding motifs within AR binding peaks in both DSRCT-xenograft and PDX samples (Fig. S9E). Genes adjacent to AR binding site peaks also showed high overlap with DSRCT specific genes in both models (Fig. S9F). Key genes from cell line data (Fig.6E) also showed AR signal reduction after AR-ASO treatment (Fig. S9G).
AR-dependent enhancer reprogramming activates oncogenic pathways in DSRCT
Several studies have shown that AR establishes a pro-tumorigenic transcriptome by reprogramming the active enhancer landscape (assessed by H3K27ac profiles) in prostate cancer progression44. Therefore, we asked if AR plays similar roles in DSRCT by examining genome-wide profiles for H3K27ac marks in unstimulated or DHT stimulated JN-DSRCT cells treated with control ASO or AR-ASO. We noted that unstimulated cells treated with AR-ASO showed a higher intensity and a higher number of H3K27ac peaks compared to control ASO treated cells (Fig. 7A-B, S10A, and Supplemental Table 2). Similarly, AR-ASO treatment in DHT-treated cells also increased the active enhancer peaks compared to control ASO treatment (Fig. 7A-B, S10A, and Supplemental Table 2). This observation is contrary to those in prostate cancers where active enhancer peaks are positively associated with higher AR activity44. It has been previously shown that AR recruits the MLL complex and CBP/p300, which is responsible for active enhancer marking in prostate cancer45. To identify which enhancers were likely derived by AR binding and potential recruitment of enhancer-marking proteins, we overlapped the AR and H3K27ac peaks in DHT treated cells (Fig. S10B and Supplemental Table 2). We then intersected these AR-targeted enhancer peaks with highly expressed genes in DSRCT (Fig. 7C and Supplemental Table 2) (FC> 1.5, adjusted p-value < 0.05 in comparison to other sarcoma subtypes). There, we identified WNT signaling and cell-adhesion as major drivers that are regulated at the chromatin level by AR-dependent active enhancer programs (Fig. 7D). The genes with direct AR binding and enhancer gains included important oncogenes such as AXIN2 and CDK6 (Fig. 7E). Additionally, we investigated alterations in super-enhancer (SE) regions that harbor a high-density of TF binding motifs46–48. SEs in control ASO treated cells marked important oncogenes such as AKT3 and GRHL2, whereas SEs in AR-ASO treated cells marked tumor suppressor genes such as RUNX1 and CUX1 (Fig. S10C-D and Supplemental Table 3), that potentially regulate the AR-driven transcriptome. Overall, our results suggest that AR activation reprograms typical enhancers and SE to regulate key oncogenic signaling pathways in DSRCT.
Interestingly, in preclinical tumor samples we also observed similar enhancer reprogramming. AR-ASO treatment of the DSRCT-xenograft significantly increased the active enhancer and promoter binding sites compared to control ASO treatment, whereas PDX samples showed a moderate increase (Fig. S11A-D). We also observed AR-dependent active enhancers regulating PI3K-AKT-mTOR, WNT signaling, cell-adhesion pathways (Fig. S11E-F), and key oncogenes (Fig. 7E), with direct AR binding and enhancer gains in both DSRCT-xenograft and PDX models (Fig. S11G).
DISCUSSION
Ever since Ladanyi and Gerald discovered the EWSR1-WT1 chromosomal translocation8, DSRCT has been treated with the same chemotherapy regimens used for ES. The recent exceptions include ES-specific agents like TK-216 that target c-terminus ETS genes (e.g., FLI1 or ERG), or pazopanib, which demonstrates preferential activity in DSRCT and other soft-tissue sarcomas49. Phase II studies testing neoantigen targeted monoclonal antibodies (Abs), for example 8H9 in DSRCT, are also directed at unique sarcoma subtypes50.
As three-quarters of all DSRCT patients typically succumb to their malignancy within 5-years, our RPPA study intended to define new molecular targets for DSRCT and expand our therapeutic arsenal of biologically targeted therapies that engage them (Figure 1). Surprisingly, of 151 proteins assessed in the RPPA, SYK and AR were the most differentially expressed. The SYK protein – not previously reported in DSRCT – is a non-receptor tyrosine kinase (also known as spleen tyrosine kinase) commonly found in hematological tissues. Its constitutive activation has been shown to induce malignant transformation of B-cells to lymphomas or leukemias. As such, the oral SYK inhibitors cerdulatinib (Portola Pharmaceutical) and entospletinib (Gilead Sciences) are under active clinical investigation for the treatment of certain lymphomas, chronic lymphocytic leukemia, and acute myeloid leukemia (NCT01994382 and NCT02457598). An orally active SYK inhibitor, fostamatinib, has already received FDA-approval as a treatment for immune thrombocytopenia and continues to be investigated as an experimental therapy for hematological malignancies (NCT00446095). Though tantalizing to consider that SYK hyperactivation plays an oncogenic role in DSRCT, we have not yet had the opportunity to evaluate these relatively new drugs within our preclinical DSRCT models.
In contrast to SYK, numerous FDA-approved and experimental AR antagonists were available for immediate preclinical evaluation, and potentially available to patients via compassionate access or early-phase clinical trials. Though our RPPA data and 9:1 male-to-female ratio hinted that DSRCT is an AR-driven malignancy, to prove this explicitly we proposed several criteria, akin to Koch’s postulates: (a) tumors must adequately express AR, (b) DHT must stimulate DSRCT cell proliferation, and (c) AR antagonists should curtail the tumor-promoting effects of androgen stimulation. The inclusion of mechanistic studies, including those directly tying AR to androgen response elements (AREs), lends further credibility that DSRCT is a second AR-driven malignancy.
To date, the first criterion – requiring AR expression – has been reported by two prior teams that recognized the striking predilection of DSRCT for young males15,51. As discussed briefly in the Introduction, Fine et al. evaluated protein expression of AR, c-Kit, EGFR, and other proteins by Western blot and IHC, scored using a 5-point scale that ranged between 0 (no staining) to 4+ (highly positive)15. Ten of twenty-seven (37%) DSRCT patients in their case series scored 2+ or higher, but we highlight that fifteen demonstrated no AR expression (Figure 2), which suggests prospective studies may wish to stratify for response by AR-status to determine whether AR expression correlates with therapeutic efficacy. A more recent study published in 2018 by Bulbul et al. at U.C.S.D., used IHC and next-generation sequencing on tumors from thirty-five DSRCT patients (86% who were males); 59% were AR-positive using a dichotomous cut-off that required ≥1+ staining in ≥10% of the cells51. In the present study, we report the most extensive series of DSRCT patients to have undergone protein and transcriptomic profiling. Though enriched in oncoproteins, our RPPA array ranked AR as the most differentially expressed protein compared to ES, its closest molecular sarcoma subtype (Figure 1). Our subsequent confirmation of the RPPA results by Western blot, and later semi-quantitative analysis by IHC, is in agreement with earlier reports and appears to substantiate AR as a bona fide target in DSRCT.
Meeting the second of Koch’s postulates, a 72-hour cell proliferation assay demonstrated a significant increase in JN-DSRCT cell proliferation following exposure to physiological levels of DHT (Figure 3A), though lower than LNCaP PC cells. As one would expect in androgen-sensitive cells, DHT also promoted the nuclear shuttling of AR into the nucleus where it would function as a transcriptional regulator of its target genes (Figure 3C & 3D). As our results rely upon data from a single cell line (the only one in existence at the time), we remain vigilant to avoid over-interpreting them. Nevertheless, our results echo similar findings by Fine et al., where they reported a DHT-induced 2-fold increase in cell proliferation in a transient DSRCT cell line obtained from ascitic fluid18.
Fulfilling the third requirement that defines an AR-driven malignancy, our team again bolsters the work by Fine et al., which had taken a prescient step more than a decade ago to evaluate CAB – in that case using Lupron and bicalutamide in six DSRCT patients that were AR-positive (3+ or 4+ by IHC) 18. Interestingly, in their limited pilot trial, non-castrate level baseline testosterone levels were associated with modest responses lasting 3-4 months. Admittedly, having tested several DSRCT patients with the same drug combination between 2006-2015, well before the advent of modern-day androgen deprivation therapies (ADT) such as abiraterone and enzalutamide, our team observed limited clinical benefits lasting <3 months. Our renewed enthusiasm for AR targeting in DSRCT stemmed from the RPPA expression results, accompanied by the in vitro DHT stimulation studies and in vivo data using enzalutamide and the AR-ASO (Figure 4).
In preparation for early-phase clinical trials now in development, our work takes the first step to advance our mechanistic understanding of AR signaling in DSRCT. As one of several steroid and nuclear hormone superfamily receptors that include the glucocorticoid receptor (GR), mineralocorticoid receptor (MR), progesterone and estrogen receptors (PR & ER), and the vitamin D receptor (VDR), AR retains a conserved 66-amino acid DNA-binding domain (DBD) able to join two (5’-AGAACA-3’) hexameric half-sites arranged as an inverted palindrome spaced 3-b.p. apart (IR3). Due to differences in local steroid metabolism, ligand abundance, chromatin accessibility, and cofactor occupancy, the DNA binding pattern of AR varies significantly in PC compared to other tissues52. Interestingly, among the pioneer factors that govern the lineage-specific binding of AR to specific genomic loci in PC53–55, and that control AR-mediated transcriptional regulation of prostate genes (such as PSA)56, FOXA1 was the most enriched MOTIF in JN-DSRCT cells (Figure 6C). Shared activation of the androgen signaling cascade in DSRCT and PC may explain the close transcriptomic clustering observed in Fig. 2E. Despite their similarities, ChIP-seq also identified notable differences in AR’s epigenetic regulation at enhancer (Figure 7) and super-enhancer (Figure S9C) binding sites.
Though the subject of future research, we suspect the heterotypic loss of WT1 or aberrant EWS-WT1 FP may recruit a specific set of chromatin modifiers at binding sites that differ from PC. Others have performed ChIP-seq in DSRCT patient specimens using WT1-specific antibodies, but the Santa Cruz antibody used in that publication57 has been discontinued. Lacking suitable ChIP-seq validated WT1-specific antibodies ATAC-seq might be used before and after WT1 RNA silencing, though interpretation of that experiment wouldn’t be as straightforward given the absence of selective antagonism of WT1 or EWS-WT1.
Interestingly, as occurs in castration-resistant PC11,58,59, our pharmacodynamic studies revealed an inverse relationship between AR and the Akt/PI3K/mTOR pathway. With numerous inhibitors of PI3K and mTOR already FDA-approved, an obvious next step would be to investigate whether co-targeting AR and either PI3K or mTOR results in synergistic anti-cancer activity. Though not explored in the present study, the estrogen receptor (ER) was also highly expressed following AR-ASO treatment. Given the shared binding DNA motifs that ER, AR, and other steroid hormone receptors have in common, this observation suggests that ER-targeted drugs might prove useful for patients with castrate-resistant DSRCT and, plausibly, the small minority of women that acquire this rare cancer type. Of course, further research in required to determine how AR and ER pathway switching affects tumor growth and survival, both in DSRCT and other hormonally-driven malignancies60.
Collectively, though morphologically and phenotypically distinct from PC, our data suggest that DSRCT is a second androgen-stimulated malignancy (third, if one considers the AR-positive molecular subset of triplenegative breast cancer). Shared dependence upon AR for tumor growth and survival provides an exciting opportunity to study AR signaling in a different cancer type and within a younger DSRCT-stricken patient population. Preclinical data using enzalutamide and AR-ASO raises the tantalizing possibility that AR-targeted drugs used for PC may also find utility to combat DSRCT.
PATIENTS AND METHODS
Patients
The collection of DSRCT tumor patients was approved by the Institutional Review Board of MDACC under the LAB08-0151 and LAB04-0890 protocols and conducted in compliance with the principals of the Declaration of Helsinki. The charts and electronic medical records of patients with a confirmed diagnosis of DSRCT were included for analysis and archived at the MDACC biospecimen bank or the collaborator PIs laboratories. We identified 60 DSRCT patients treated at MDACC from 1990 to 2019 to generate a TMA. Also, we collected 16 DSRCT and 6 Ewing sarcoma (ES) fresh frozen tumors, all of them were profiled by RPPA. Specialist pathologists used clinical information, immunohistochemistry, and cytogenic analysis for the EWSR1-WT1 or EWSR1-FLI1 fusions to confirm the DSRCT or ES diagnoses. Blood samples (EDTA) of 5 ml were collected from 17 DSRCT patients and 3 Ewing sarcoma patients (ES) to remove serum and assay PSA.
RPPA and Western blot analyses
The available snap-frozen DSRCT (n=16) and ES (n=6) specimens collected during a core-needle biopsy or surgical debulking procedures using clinical protocols approved by MDACC’s Institutional Review Board and specimens of normal-appearing mesenteric tissue adjacent to DSRCT obtained at the time of surgical debulking (n=8) were used for the proteomic analysis (Supplemental Table 4: Demographic information of DSRCT and ES patients). Lysates were created, protein concentrations were determined, and individual protein expression was measured using a well-validated reverse-phase protein array (RPPA) and Western blot (WB) technologies as previously described61–63. AR protein detection was performed using the CST antibody (#5153). Additional details about RPPA and WB analyses and normalized data are provided in the Supplementary Methods and Supplemental Table 5.
RNA Sequencing, gene expression analysis, and fusion detection
Total RNA from primary tumor samples was extracted and libraries made from cDNA using the NuGEN Ovation Ultralow Library System V2 (San Carlos, CA). RNA sequencing reads of the samples were mapped to the hg19 reference genome using the STAR aligner64. For calculation of gene expression, each gene’s raw count data were first obtained using HTSeq65, and are normalized by scaling the library size using calcNormFactors in the edgeR package 66. Then, Voom transformation was applied to normalized counts and a linear model fit to the data for differential expression analysis using the Limma package67. Pathway analyses of differentially expressed genes between two sample clusters were performed using Gene Set Enrichment Analysis (GSEA)68. Fusion transcripts were detected from RNA-seq data using MapSplice69.
TMA Preparation and Immunohistochemistry Analyses
A tissue microarray (TMA) was constructed from archival surgical pathology materials comprising 60 formalin-fixed, paraffin-embedded tissues from 60 DSRCT patients. Areas of the viable tumor were selected by pathologist review of whole slide H&E-stained sections. Selected areas were punched and transferred, in duplicate, to a recipient block using an ATA-100 Advanced Tissue Arrayer (Chemicon International). All human specimens were utilized under an Institutional Review Board-approved research protocol (LAB04-0890) allowing for the retrospective sampling and analysis of existing archival materials collected in the course of standard patient care. Immunohistochemical studies were performed using an autostainer (Bond-Max; Leica Microsystems, Buffalo Grove, IL, USA) with anti-AR (1:30; clone AR441, Dako#M3562) antibody. Additional details about TMA slides preparation and IHC analyses are provided in the Supplementary Methods.
WST1 Cell Proliferation Assays
The JN-DSRCT, LNCaP, and TC71 cells tested for their proliferation capacity In vitro using a colorimetric assay in 96-Well plates with WST-1 reagent (Roche). The cells seeded at 3000 cells/well in triplicates with 10% FBS DMEM (JN-DSRCT) or RPMI (TC71 and LNCaP) complete media. Additional details about WST1 cell proliferation assays are provided in the Supplementary Methods.
Immunostaining of JN-DSRCT cells and xenograft animal tumors
JN-DSRCT cell line exhibiting a pathognomonic t(11;22)(p13;q12) translocation was generously provided from Dr. M Kikuchi’s laboratory (Fukuoka University, Fukuoka, Japan). In addition, PC3, LnCaP, and TC71 cell lines are provided by the MDA cell lines core facility. All available cell lines in Dr. Ludwig’s lab are registered within the MDA characterized cell line core (CCLC). Each cell line identity is validated twice per year in MDA CCLC using short-tandem repeat (STR) fingerprinting with an AmpFLSTR Identifier kit. Furthermore, according to the manufacturer’s protocol, all our cell lines are tested twice per year for mycoplasma contamination using the MycoAlert Detection Kit (Lonza Group Ltd.). Additionally, cell lines are sent for 3rd-party mycoplasma testing using a sensitive PCR testing approach any time a collection of cells are cryopreserved.
Monolayer JN-DSRCT cell culture in 8 chamber slides were fixed for 10 min at room temperature with 4% paraformaldehyde in phosphate-buffered saline (PBS). The primary JN-DSRCT xenograft and PDX tumors were harvested, fixed in 10% formalin, embedded in paraffin (formalin-fixed, paraffin-embedded: FFPE), and then sliced in 5 μm sections before processing them for antigen retrieval using 0.1M citrate buffer for 20 minutes and in a vegetable steamer. Altogether, monolayer and primary tumor slides were permeabilized and blocked with superblock buffer (Thermo Fisher Scientific, #37535) for 1 hour at room temperature. Slides were then incubated consecutively with primary antibodies to AR (Cell Signaling Technologies, #5153), (overnight at 4°C) and Alexa Fluor 488-labeled Goat-anti Rabbit (Thermo Fisher Scientific, #A11037) (for 1hr at room temperature). The nuclei were visualized using Hoechst (Thermo Fisher Scientific, #H357), and the immunofluorescence was acquired after subtracting the background intensities using the Nikon A1-Rsi confocal microscope (Nikon). Fluorescentdetection of proteins in the nuclei and cytosolic regions was quantified using the Imaris software (Bitplane) and its Cell module that use validated algorithms to define the segmentation by permitting the recognition of selected protein fluorescence in both nuclear and cytosolic regions.
Generation of DSRCT Xenograft/PDX mouse models and Drug Evaluation
All experiments were conducted per protocols and conditions approved by the University of Texas MD Anderson Cancer Center (MDACC; Houston, TX) Institutional Animal Care and Use Committee (eACUF Protocols #00000712-RN03). Male NOD (SCID)-IL-2Rgnull mice (The Jackson Laboratory; Farmington, CT) were subcutaneously injected with JN-DSRCT cells (5X106 cells/animal) or received PDX explants (2 mm) to generate DSRCT xenograft and PDX mouse models. The histologic and genetic analyses of DSRCT patient and PDX tumors are available on Supplemental Figure 12. All mice were maintained under barrier conditions and treated using protocols approved by The University of Texas MD Anderson Cancer Center’s Institutional Animal Care and Use Committee. Once their tumors reached a volume of 150 mm3, 5 mice per group received enzalutamide (25 mg/kg IP daily, 5 times per week), or AR ASOs (25 or 50 mg/kg subcutaneously daily, 5 times per week), or control ASOs (50 mg/kg subcutaneously daily, 5 times per week), or a placebo control (sterile vehicle buffer). Tumor volumes were measured using digital calipers at study initiation and 2–5 times per week after that for up to 85 days, or until their tumors reached 1500 mm3, whichever came first. A Kaplan-Meier analysis was performed to assess drug efficacy. Statistical analyses between control and treated group or between different treated groups were performed with the log-rank (Mantel-Cox) test using Graph-Pad Prism 8.0.
Mass spectroscopy based determination of intratumoral hormone levels
Testosterone and corticosterone quantification were determined using Agilent’s Infinity II UHPLC in line with a 6495 triple quadrupole mass spectrometer and MassHunter workstation software (8.0.8.23.5). Briefly, DSRCT xenograft and PDX samples were homogenized using water containing internal standard (Cerilliant, T070) extracted with tert-butyl methyl ether (Sigma 34875), dried under nitrogen, and derivatized using hydroxylamine hydrochloride (Sigma 431362). The recovered ketoxime steroids were reconstituted in methanol/water (1:1 v/v) and injected into the Infinity II UHPLC. Ketoxime steroids were separated using a Chromolith reverse phase column (RP-18 endcapped 100-2mm, Sigma 152006) and introduced into a JetStream source (Agilent) for triple quadrupole analysis. Data were analyzed and quantified using MassHunter software (Agilent)39,40.
ChIP-Seq Assays
Chromatin immunoprecipitation was performed as described earlier70 with optimized shearing conditions and minor modifications for JN-DSRCT cells. The antibodies used were: H3K27ac (Abcam ab4729) and AR (CST#5153). Briefly, 3 million cells per sample were cross-linked using 1% formaldehyde for 10 min at 37 °C. After quenching with 150 mM glycine for 5 min at 37 °C, cells were washed twice with ice-cold PBS and frozen at −80 °C for further processing. Later, cells were thawed on ice and lysed with ChIP harvest buffer (12 mM Tris-HCl, 0.1 × PBS, 6 mM EDTA, 0.5% sodium dodecyl sulfate [SDS]) for 30 min on ice. Lysed cells were sonicated with Bioruptor (Diagenode) to obtain chromatin fragment. Antibody-dynabead mixtures were incubated for 1 hr at 4 °C and cellular extracts were then incubated overnight with these mixtures. After overnight incubation, immune complexes were washed five times with RIPA buffer, twice with RIPA-500 (RIPA with 500 mM NaCl) and twice with LiCl wash buffer (10 mM Tris-HCl pH8.0, 1 mM EDTA pH8.0, 250 mM LiCl, 0.5% NP-40, 0.1% deoxycholate). For reverse-crosslinking and elution, immune complexes were incubated overnight at 65 °C in elution buffer (10 mM Tris-HCl pH8.0, 5 mM EDTA, 300 mM NaCl, 0.5% SDS). Eluted DNA was then treated with proteinase K (20 mg/ml) and RNase A and DNA clean-up was done using SPRI beads (Beck-man-Coulter). ChIP libraries were amplified and barcoded with use of the NEBNext® Ultra™ II DNA library preparation kit (New England Biolabs). After library amplification, DNA fragments were size-selected (200 - 500 bp) using AMPure XP beads (Beckman Coulter) and assessed using high sensitivity D1000 screen tape on the Bioanalyzer (Agilent Technologies). Libraries were multiplexed together and sequenced in HiSeq2000 (Illumina).
ChIP-seq Data Processing
ChIP-seq data were quality controlled and processed by pyflow-ChIPseq71, a snakemake72 based ChIP-seq pipeline. Briefly, raw reads were mapped by bowtie173 to hg19. Duplicated reads were removed, and only uniquely mapped reads were retained. RPKM normalized bigwigs were generated by deep tools74, and tracks were visualized with IGV75. Peaks were called using macs1.476 with a p-value of 1e-9 for H3K27ac and 1e-7 for AR. Heatmaps were generated using R package EnrichedHeatmap. ChIP-seq peaks were annotated with the nearest genes using ChIPseeker77. Super-enhancers were identified using ROSE78 based on H3K27ac ChIP-seq data.
Differential Peaks Analysis
To identify variable AR or enhancer domains enriched in specific DSRCT samples, enhancer peaks that overlap with 2.5kb upstream and 2.5kb downstream of any known TSSs were removed. The unique and shared peaks within multiple groups were identified by Intervene79. The peaks were annotated with ChIPseeker R package 77, using addFlankGeneInfo function for enhancers.
Identification of AR and Enhancer Associated Pathways
Differential AR binding sites and enhancers associated genes in each sample were imported into the ClusterProfiler80 for pathway analysis, restricted to GO, KEGG, Hallmark, and WiKi gene sets. The Enrichplot package81 was used to generate dot plot and bar plot for gene sets enriched with a false discovery rate (FDR) cut-off of < 0.05.
Enrichment of Motifs in AR-Specific Peaks
To identify the motifs over-represented within AR-specific peak sets, we used the HOMER motif database and the coordinates of AR-specific peak sets82.
Data availability
All ChIP-seq data are available at GEO accession number GSE151380. All codes used to generate the ChIP-seq data are available at https://github.com/crazyhottommy/pyflow-ChIPseq. RNA-seq data for DSRCT are under EGAS00001004575, liposarcoma under EGAS00001002807, osteosarcoma under EGAS00001003247, chondrosarcoma under EGAS00001004585, and prostate cancer through Subudhi et al.83.
Footnotes
↵* Co-first authors
Financial Disclosures: Dr. MacLeod is an employee and shareholder of Ionis Pharmaceuticals.
Research Support: The University of Texas MD Anderson Cancer Center is supported by the National Institutes of Health through Cancer Center Support Grant CA016672. JAL and AHJ are funded through the generous philanthropy of the Cory Monzingo Foundation.