Wnt-C59

Inhibiting Wnt/beta‐catenin in CTNNB1‐mutated endometrial cancer

Marisa R. Moroney1 | Elizabeth Woodruff2 | Lubna Qamar2 |
Andrew P. Bradford2 | Rebecca Wolsky3 | Benjamin G. Bitler1,2 | Bradley R. Corr1

1Division of Gynecologic Oncology, Department of Obstetrics and Gynecology, University of Colorado School of Medicine, Aurora, Colorado, USA
2Division of Reproductive Sciences, Department of Obstetrics and Gynecology, University of Colorado School of Medicine, Aurora, Colorado, USA
3Department of Pathology, University of Colorado School of Medicine, Aurora, Colorado, USA

Correspondence
Benjamin G. Bitler and Bradley Corr, Department of Obstetrics and Gynecology, University of Colorado Anschutz Medical Campus, 12700 E. 19th Ave, MS 8613, Aurora, CO 80045.
Email: [email protected] and [email protected]

Funding information
The University of Colorado OB/GYN Academic Enrichment Fund; The American
Cancer Society, Grant/Award Number: 134106‐RSG‐19‐129‐01‐DDC; AAOGF/
ABOG; The University of Colorado Cancer
Center Developmental Therapeutics Program; University of Colorado Cancer Center Support Grant, Grant/Award Number: P30CA046934

Abstract
The role of β‐catenin/TCF transcriptional activity in endometrial cancer (EC) re- currence is not well understood. We assessed the impact of Wnt/β‐catenin inhibi- tion in EC models. In an analysis of the Cancer Genome Atlas, we confirmed that
CTNNB1 mutations are enriched in recurrent low‐risk EC and showed that aberrant Wnt/β‐catenin pathway activation is associated with recurrence. We studied CTNNB1‐wildtype (HEC1B, Ishikawa) and CTNNB1‐mutant (HEC108, HEC265, HEC1B‐S33Y, Ishikawa‐S33Y) EC cell lines. Dose response curves were determined for 5 Wnt/β‐catenin pathway inhibitors (Wnt‐C59, XAV‐939, PyrPam, PRI‐724, SM04690). XAV939, Wnt‐C59 and PyrPam inhibited function upstream of β‐catenin
transcriptional activity and were ineffective at inhibiting cell viability. In contrast, PRI724 and SM04690 indirectly inhibited β‐catenin transcriptional activity and
significantly reduced cell viability in CTNNB1‐mutant cell lines. Treatment with
SM04690 reduced cell viability (Licor Cell stain) in all EC cell lines, but viability was significantly lower in CTNNB1‐mutant cell lines (p < 0.01). Mechanistically, SM04690
significantly inhibited proliferation measured via 5′‐bromo‐2′‐deoxyuridine in-
corporation and reduced T cell factor (TCF) transcriptional activity. HEC1B, HEC1B‐ S33Y and HEC265 tumor‐bearing mice were treated with vehicle or SM04690. Tumors treated with SM04690 had smaller mean volumes than those treated with
vehicle (p < 0.001, p = 0.014, p = 0.06). In HEC1B‐S33Y and HEC265 tumors, SM04690 treatment significantly reduced Ki67 H‐scores compared to vehicle (p = 0.035, p = 0.024). Targeting the Wnt/β‐catenin pathway in CTNNB1‐mutant EC effectively inhibited proliferation and β‐catenin/TCF transcriptional activity and blunted tumor progression in in vivo models. These studies suggest β‐catenin transcriptional inhibitors are effective in EC and particularly in CTNNB1‐mutant EC, highlighting a potential therapeutic vulnerability for treatment of CTNNB1‐
mutant EC.

KEYWOR DS
CTNNB1, endometrial cancer, small molecule agents, tumor suppressor, Wnt/β‐Catenin

Molecular Carcinogenesis. 2021;1–13. wileyonlinelibrary.com/journal/nau © 2021 Wiley Periodicals LLC | 1

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⦁ | INTRODUCTION

Endometrial cancer (EC) is the most common gynecologic malignancy in the developed world, and both the incidence and mortality of EC are on the rise worldwide. Over the last decade in the United States, EC incidence rose from 42,190 new cases in 2009 to 61,880 new cases in 2019, while estimated annual deaths rose from 7780 to 12,160.1,2 EC is one of the only cancers to have a raising mortality rate, and with this increasing trajectory of both incidence and mor- tality, EC will likely soon be responsible for more annual deaths in the United States than ovarian cancer.1–5
Greater than 70% of ECs are diagnosed in early stages and have a generally favorable prognosis.6 However, when EC recurs, it can have a poor prognosis and be difficult to treat.7 Developing tools to prevent and predict EC recurrence is therefore of critical importance
for curbing the increasing EC mortality rates.3,8 Current clinical risk‐
stratification relies on tumor histopathologic features (histologic subtype and grade, myometrial invasion, lymphovascular space in- vasion [LVSI]) and disease stage in an attempt to identify ECs with a higher risk of recurrence and make treatment decisions accordingly.
Unfortunately, there is growing evidence that this risk‐stratification
system has low reproducibility and reliability and does not fully capture the clinical and molecular heterogeneity of EC.3,9–13 There-
fore, new methods for improving EC risk‐group stratification are
needed through molecular and genetic classifications. The Cancer Genome Atlas (TCGA) identified four subgroups of EC with distinct genetic profiles—polymerase epsilon ultramutated, microsatellite
instability hypermutated, copy‐number low (CNL), and copy‐number
high.13 Several groups independently reproduced the prognostic
significance of these subgroups, indicating the clinical potential for a molecular based risk‐group stratification system.11,12,14,14,15
CTNNB1 mutations have been identified as an important clinical
marker in EC.11–14,16CTNNB1 is a gene that codes for the β‐catenin protein, which is involved in the Wnt/β‐catenin pathway and is as-
sociated with multiple cancers.13,16–21 In normal cells in the absence of a Wnt ligand, a destruction complex consisting of adenomatous
polyposis coli (APC), axin, casein kinase I, and glycogen synthase kinase 3β binds to β‐catenin. GSK3β phosphorylates serine and
threonine residues on the N‐terminus of β‐catenin, which leads to
Beta‐Transducin Repeat Containing E3 mediated ubiquitination, and proteasomal degradation of β‐catenin. In contrast, when Wnt ligand is present, Wnt proteins bind to Frizzled and LDL (LRP 5/6) receptors
initiating a signaling cascade that prevents β‐catenin phosphoryla- tion. Without phosphorylation, β‐catenin is not degraded, accumu- lates in the cytosol, translocates to the nucleus and interacts with T cell factor (TCF)/lymphoid enhancing factor transcription factors and
co‐activators (e.g., cAMP response element binding protein [CREBBP]) to initiate transcription.16,17,19,19,20,22 CTNNB1 mutations associated with EC are mainly located in exon 3 of the CTNNB1 gene.
Exon 3 encodes the N‐terminus of β‐catenin, which contains the GSK3β phosphorylation sites. These mutations therefore disrupt phosphorylation of β‐catenin by the destruction complex, resulting in
unregulated accumulation of β‐catenin and subsequent transcrip- tional activation.12,16,23
Wnt/β‐catenin signaling is involved in the regulation of the normal endometrium, and aberrant Wnt/β‐catenin activity, like that
with CTNNB1 mutations, has been associated with the development of endometrial hyperplasia and malignancy.16,24–26 The crucial role of CTNNB1 mutations in the development of EC specifically is further supported by in vivo studies in which loss of CTNNB1 exon 3 resulted
in upregulation of the Wnt/β‐catenin pathway and development of
endometrial hyperplasia and endometrial adenocarcinoma.24,27 Multiple studies of ECs with otherwise low mutational burden report that tumors that contain CTNNB1 exon 3 mutations are more likely to recur, indicating that the CTNNB1 mutations are potential onco- genic drivers.12,13
CTNNB1‐mutant ECs tend to have low‐grade histology, low rates
of deep myometrial invasion and low rates of LVSI.23 In the current clinical risk‐stratification system, these histopathologic features would indicate a low risk of recurrence. However, CTNNB1 mutations
have been demonstrated to be associated with a significantly in-
creased rate of disease recurrence specifically in a low‐risk popula- tion of early stage, low grade ECs.28 In larger studies evaluating ECs of all grades, ECs with CTNNB1 exon 3 mutations have been found to have decreased recurrence‐free and overall survival.12,23,28,29
Due to the presumed oncogenic role of CTNNB1 mutations, the Wnt/β‐catenin pathway is a promising target for precision medicine‐ based approaches to improve EC outcomes. In this study, we ana-
lyzed the publicly available TCGA data set to further evaluate
CTNNB1 mutations and Wnt/β‐catenin signaling in EC. We in- vestigated targetable blockade of different aspects of the Wnt/β‐ catenin pathway in a panel of EC cell lines with different CTNNB1
mutations. In this panel of cells, we subsequently evaluated the ef- fect of β‐catenin inhibition on transcriptional activity, apoptosis, and cell proliferation. In vivo models were then utilized to further assess inhibition of the Wnt/β‐catenin pathways on tumor progression.

⦁ | METHODS

⦁ | TCGA database analysis

TCGA data was accessed on the cBioPortal for Cancer Genomics (http://www.cbioportal.org), and the TCGA PanCancer Atlas da- tabase of uterine corpus endometrial carcinomas (UCEC) was
utilized.30,31 We evaluated the Copy‐Number Low subgroup,
“UCEC_CN_LOW,” for CTNNB1 mutational status, patient demographics, histopathology, other gene mutations, treatments,
disease recurrence and survival outcomes. Independent of copy‐
number status, comparing RNA‐sequencing data from CTNNB1‐
mutant and wildtype ECs a list of differentially expressed genes (DEG) (p < 0.05, adj. p < 0.05) was identified. An overlap analysis between the DEGs and KEGG gene sets was conducted through the Broad Institute.32

⦁ | Cell culture

Ishikawa (CVCL_2529), HEC1B (CVCL_0294), HEC108
(CVCL_2923), and HEC265 (CVCL_2928) are human endometrial cancer cell lines (Table 1). Ishikawa and HEC1B are CTNNB1‐ wildtype, while HEC108 and HEC265 are CTNNB1‐mutant
(CTNNB1 Exon 3 base substitutions S37P and D32V, respec- tively). All four cell lines were authenticated using small tandem repeat analysis (The University of Arizona Genetics Core), and the CTNNB1 status of each cell line was confirmed through Sanger Sequencing. The HEC1B, HEC108, and HEC265 cells were cultured in Minimum Essential Medium (MEM) medium supple-
mented with 1% penicillin‐streptomycin, and 15% fetal bovine
serum, and Ishikawa cells were culture in MEM medium supple- mented with 1% penicillin‐streptomycin, 1% non‐essential amino acids, 1% glutamine, and 5% fetal bovine serum. All cells were
maintained in 5% CO2 at 37°C, were routinely tested for myco- plasma with MycoLookOut (Sigma‐Aldrich) and were last tested on November 21st, 2020.

⦁ | Retroviral packaging

Retrovirus production and transduction were performed as de- scribed previously33 under the University of Colorado Institu- tional Biosafety Protocol (IBC‐00001221). Phoenix cells were
used to package the viruses (a gift of Dr. Gary Nolan, Stanford University). pBabe‐CTNNB1‐S33Y plasmid was obtained from Addgene (#19286). The S33Y CTNNB1 mutation is an exon
⦁ mutation, which results in a structural alteration of the N‐terminus of β‐catenin, ultimately preventing phosphorylation
and degradation of β‐catenin by the destruction complex, as
described above. Two stable CTNNB1‐mutant cell lines (Ishikawa‐ S33Y and HEC1B‐S33Y) were created from the Ishikawa and HEC1B native CTNNB1‐wildtype cell lines. Retroviral transduc- tion of the S33Y‐mutant CTNNB1 gene (pBabe‐CTNNB1‐S33Y)
into the Ishikawa and HEC1B cell lines was performed. The presence of the mutant CTNNB1 gene in these cell lines was confirmed using Sanger Sequencing (Figure S2A). The comparison
of these newly produced CTNNB1‐mutant cell lines to their na-
tive CTNNB1‐wildtype counterparts allowed for evaluation of the direct impact of a CTNNB1 mutation on an EC cell line.

⦁ | Reagents and antibodies

Five inhibitors known to target the Wnt/β‐catenin pathway with variant mechanism were utilized: Wnt‐C59, XAV‐939, PyrPam, PRI‐724, and SM04690. All five inhibitors were obtained from
Selleckchem. The following antibodies from the indicated suppliers
were utilized: anti‐β‐catenin (Cat#8480S; 1:1000; Cell Signaling Technology), anti‐Lamin A/C (Cat#4777S, 1:1000; Cell Signaling Technology).
⦁ | Immunoblotting

Nuclear and cytoplasmic proteins were fractionated. Cell pellets were suspended in a buffer mix of 10 mM HEPES, 1.5 mmol/L MgCl2,
10 mmol/L KCl, 0.5 mmol/L DTT, 0.05% NP40 pH 7.9, Complete EDTA‐free protease inhibitors (Cat #11873580001; Roche), 10 mM NaF and 1 mM Na3VO4. The suspension was incubated at 4°C for 10 min, aspirated through a 27‐gauge needle, and then centrifuged at 3000 RPM for 10 min. The supernatant was collected as the cyto-
plasmic protein. The pellet was then resuspended in RIPA buffer (150 mmol/L NaCl, 1% TritonX‐100, 0.5% sodium deoxycholate, 0.1% sodium dodecyl sulfate (SDS) (50 mmol/L Tris pH 8.0), Complete EDTA‐free protease inhibitors, 10 mM NaF and 1 mM Na3VO4. Protein concentrations were quantified using a ThermoFisher BCA
protein assay kit (Cat. #23225; Thermo Fisher Scientific). Protein was then separated by SDS polyacrylamide gel electrophoresis and transferred to polyvinylidene fluoride membrane. Primary antibody incubation was performed overnight at 4°C. Secondary antibodies
(goat anti‐rabbit, IRDye 680RD or IRDye 800CW, LI‐COR, Cat #
92568071 or Cat #926‐3221, 1:20,000; goat anti‐mouse, IRDye 680RD or IRDye 800CW, LI‐COR, Cat # 926‐68070 or Cat #925‐
32210, 1:20,000) were applied for 1 h at room temperature. Blots were visualized and imaged using the Licor Odyssey Imaging System and densitometry was calculated using ImageStudio.

⦁ | 3D cell culture

The HEC1B, HEC108, HEC265 and Ishikawa cell lines were cultured in 3D conditions using Matrigel. The 3D culture procedure was adapted from previously published methods34 and utilized Matrigel
(Corning, Cat #354230) in combination with the previously de- scribed cell medium.33 A single cell suspension was plated in eight‐ well chambers and covered with 3% Matrigel/complete media.
Matrigel with complete media was changed every 4 days, and the cells were grown for 12 days. The cultured cells in spheroid forma- tion were then examined and photographed using Inverted Olympus microscope (model: FV1000). Cell diameter was measured using ImageJ (NIH) and used as a surrogate for cell growth, a method which was previously published and verified.33

⦁ | Dose curves

The effect of the Wnt/β‐catenin pathway inhibitors on cell viability was evaluated in the EC cell lines via Licor Cell Staining. Each cell line was plated in a 96‐well plate with 10,000 cells per well. The cells were incubated for 48 h following treatment. Dose ranges for each
inhibitor were determined based on prior studies of all five in- hibitors.35–40 Licor Cell Staining was then performed to measure cell viability with %cell confluency being the measure for cell viability. The accuracy of Licor Cell Staining in measuring a known cell con- fluency was confirmed previously (Figure S1A,B).

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TABLE 1 Cell line characteristics

Biological Histologic POLE
Cell line source grade CTNNB1 PTEN KRAS TP53 Hotspot MLH1 MLH3 MSH2 MSH6 PMS2 PR ER Source
Ishikawa human 1 wildtype Frameshift wildtype Missense Missense wildtype wildtype wildtype Missense Missense High High University of
uterus fram- fram- fFram- Colorado
shift shift shift GTFB
Ishikawa‐ human 1 S33Y Frameshift wildtype Missense Missense wildtype wildtype wildtype Missense Missense High High Viral
S33Y uterus trans- fram- fram- fram- Trans-
duction shift shift shift duction
HEC1B human 2 wildtype wildtype Missense Missense wildtype wildtype wildtype wildtype Frameshift Nonsense Low Low University of
uterus Colorado
GTFB
HEC1B‐
S33Y human
uterus 2 S33Y
trans- wildtype Missense Missense wildtype wildtype wildtype wildtype Frameshift Nonsense Low Low Viral
Trans-
duction duction
HEC108 human 3 Missense Frameshift wildtype Missense Missense wildtype Missense Missense Missense wildtype Unknown Negative Japanese
uterus S37P fram- fram- fram- Collection
Substi- shift shift shift of Researcg
tution non- Bioresour-
sense ces
Cell Bank
HEC265 human unknown Missense Frameshift wildtype Missense Missense Frameshift wildtype wildtype Frameshift wildtype High High Japanese
uterus D32V Collection
Substi- of Researcg
tution Bioresour-
ces
Cell Bank
Note: The cell lines' name, biologic source, histologic grade, PR and ER receptor expression status, and mutational status of ten well known endometrial cancer mutations are listed. The source by which the cell line was obtained is also listed.
MORONEY ET AL.
Abbreviations: ER, estrogen receptor; PR, progesterone receptor.

⦁ | Apoptosis assays

Cells were plated in a six‐well culture dish and allowed to attach for
24 h. The cells were then treated with vehicle or SM04690. After 48 h of treatment, the cells were stated with Alexa Fluor 488 an- nexin V (Cat A13201; Invitrogen) and propidium iodide according to the manufacturer's protocol. The cells were then analyzed using a Gallios Flow Cytometer at the University of Colorado Cancer Center Flow Cytometry Facility. FlowJo (v10) was used to analyze data.

⦁ | TCF transcriptional reporter

TCF transcriptional activity was evaluated using a Luciferase Assay System (Cat. E1501; Promega) and TOP‐FLASH, FOP‐FLASH plas- mids.41 Using FuGENE6 reagent (Cat. E2692; Promega), populations were transfected with TOP‐FLASH or FOP‐FLASH plasmid. M50 Super 8x TOPFlash and FOPFlash were provided by Randall Moon
(Cad #12456/12457; Addgene). Cells were incubated for 24 h, then moved to a 96‐well plate and treated with serial doses of SM04690. Following treatment, the cells were incubated for another 48 h. Cells
were then lysed and analyzed using the Luciferase Assay system with luminescence measured by a Promega GloMax.
To normalize this assay for transfection efficiency and cell count, FOP‐FLASH luciferase activity and crystal violet were performed on
each cell line. For FOP‐FLASH transfected cells, luminescence was
also quantified as a measure of transfection efficiency. For crystal violet, the cells were seeded, incubated and treated in the same way as the cells in the Luciferase Assay System. Then, 48 h after treat- ment, the cells were fixed (10% methanol, 10% acetic acid) and stained with 0.4% crystal violet. Crystal violet was dissolved in fixative and absorbance was measured at 570 nm.

⦁ | Anti‐BrdU FITC cell staining and flow cytometry

Cells were plated in 6‐well culture dishes and incubated in the ap- propriate growth media for 24 h at 37°C and 5% CO2. The cells were
then treated with either vehicle or SM04690 (64 nmol/L or 128 nmol/L) for 48 h. 5′‐bromo‐2′‐deoxyuridine (BrdU) (Cat. #550891; BD Biosciences) was then added directly to the well culture media
(final concentration 10 µM), and the cells were incubated at 37°C for
60 min. After BrdU incorporation, cells were washed twice with phosphate‐buffered saline (PBS) and treated with 0.25% trypsin/ 0.1% EDTA for 7 min at 37°C followed by two washes with 1% bo-
vine serum albumin (BSA)/PBS and resuspension in cold PBS. Finally, cells were slowly added to ice cold 70% ethanol and incubated at
−20°C for 30 min.
Fixed cells were incubated for 30 min in 2 N HCl with 0.5% Triton X‐100 (vol/vol) followed by resuspension in 0.1 mol/L Na2B4O7∙10 H2O, pH 8.5. Cells were then suspended in 0.5%
Tween 20 (vol/vol) plus 1% BSA/PBS and incubated for 30 min at
room temperature with anti‐BrdU FITC (BD Biosciences, Cat. #347583) at a concentration of 0.5 µg/106 cells. Lastly, cells were washed once in 0.5% Tween 20 (vol/vol) plus 1% BSA/PBS and
resuspended in PBS.
The anti‐BrdU FITC cells were then analyzed using a Gallios Flow Cytometer at the University of Colorado Cancer Center Flow
Cytometry Facility. Laser excitation was set at 488 nm. FlowJo (v10) was used to analyze data.

⦁ | Mouse models

All mouse work was approved under a University of Colorado Institutional Animal Care and Use Committee (IACUC) protocol.
Athymic nude mice (Charles River Labs, Strain 553) were injected with 5 × 106 HEC1B cells on the left flank and 5 × 106 HEC1B‐S33Y cells on the right flank. Investigators were blinded to which flank each cell line was injected. HEC1B and HEC1B‐S33Y tumors were all subsequently genotyped to confirm S33Y mutation. In an in-
dependent experiment, another set of nude mice were injected with 5× 106 HEC265 cells on the right flank. Tumor progression was measured using calipers every 3 days. Measurements were used to determine tumor volume based on the formula a2 x b/2, with “a” being the smaller diameter and “b” being the larger diameter.42 Once a tumor in each flank population grew to over 50 mm3, treatment was initiated in all mice. Mice were treated by daily intraperitoneal injection with either SM04690 25 mg/kg or vehicle (10% cyclodex- trin). Tumor size continued to be evaluated throughout treatment using caliper measurements every 2–3 days. In the mice with HEC1B
left flank and HEC1B‐S33Y right flank tumors, the study had to be
halted after Day 19 due to IACUC limitations (ulcerating tumors). The mice were sacrificed according to IACUC protocol, and the tu- mors were surgically resected. Tumor burden was calculated based on the weight of resected tumors. Portions of each tumor specimen were then snap frozen, fixed in 10% buffered formalin or stored in RNAlater.

⦁ | Immunohistochemistry

Tumor tissue from each specimen of the mouse model was fixed in 10% buffered formalin and stored in 70% ethanol. The tumor tissue
was then paraffin‐embedded and sectioned for hematoxylin and
eosin staining and immunohistochemistry (IHC). IHC staining was
performed for β‐catenin (Cat. #9562, 1:500; Cell Signaling Technology), cleaved caspase‐3 (Cat. #9661, 1:500; Cell Signaling Technology), and Ki67 (Cat. #RM‐9106‐S, 1:200; Thermo Fisher
Scientific). This tissue preparation, sectioning and staining was per- formed by the Histopathology Core of The University of Colorado Cancer Center as previously described.43 All slides were then dei-
dentified and Histology scores (H‐score) were calculated.44 The H‐
score is calculated by measuring the intensity (0,1,2,3) and percen- tage of tissue with that intensity.

⦁ | Statistical analysis

All statistical analyses were performed in Prism GraphPad (v8). Dose curve calculations were performed using a nonlinear regression (variable slope) and the IC20 and IC50 of each inhibitor for each cell line was determined. Standard statistical analysis with χ2, Fisher's
exact and Mann–Whitney tests were employed. Survival outcomes were compared using Kaplan–Meier survival curves and log‐rank tests.

⦁ | RESULTS

⦁ | CTNNB1 mutations are associated with recurrence in low risk EC

Among the 529 ECs in the TCGA PanCancer Atlas, 133 (25.1%) had CTNNB1 mutations. There were 147 classified into the CNL sub- group, of which 69 (46.9%) were CTNNB1‐mutant and 78 (53.1%)
were CTNNB1‐wildtype. CTNNB1‐wildtype CNL ECs had higher rates of TP53 mutations (11.5% vs 0.0%, p = .004). None of the CTNNB1‐ mutant CNL ECs had deficiencies in mismatch repair genes (MLH1, MSH2, MSH6, PMS2); 2/78 (2.6%) of the CTNNB1‐wildtype CNL ECs
had loss of MSH6 (p = 0.499). Of the 147 CNL EC patients, 135 (91.8%) patients were living at time of data publication and 12 (8.2%) were deceased. 119 (81.0%) of these 147 patients were disease‐free,
11 (7.5%) had recurred and 17 (11.6%) had unknown disease status.
Median disease‐free survival was 28.5 months. Median follow‐up was
30.1 months (range: 0.0–185.8 months). Disease‐free survival for CTNNB1‐mutant and CTNNB1‐wildtype CNL ECs was 78.3% and 83.3%, respectively (hazard ratio [HR]: 1.61, 95% confidence interval
[CI]: 0.48–5.27, p = 0.433). Overall survival was 91.3% and 92.3%,
respectively (HR: 1.17, 95% CI: 0.38–3.66, p = 0.784]).
When looking specifically at grade 1 ECs within the CNL sub- group (n = 55), overall survival for patients with grade 1 CNL EC was 100.0% with a median follow‐up time of 36.4 months (range: 0.4–96.5 months). 50 (90.9%) patients were disease‐free, 4 (7.3%)
had recurred and 1 (1.8%) had unknown disease status (Figure 1A). Median disease‐free survival was 29.9 months. CTNNB1 mutation was present in 31/55 (56.4%) CNL grade 1 tumors. CTNNB1 was present in all 4 (100%) of the recurrent and 26/50 (52%) of the non‐ recurrent tumors (p = 0.120) (Figure 1B). No other genetic mutation
analyzed by TCGA was present in all 4 of these recurrent ECs, and no
single mutation had a statistically different frequency in recurrent versus non‐recurrent grade 1 CNL ECs. Disease‐free survival for CTNNB1‐mutant grade 1 CNL EC patients was 83.9% compared to
100.0% for CTNNB1‐wildtype grade 1 CNL EC patients (HR: 7.4, 95% CI: 1.04–52.74, p = 0.045). There was no difference in overall survival between CTNNB1‐mutant and ‐wildtype EC patients in the grade 1 CNL subgroup (100.0% for both) (Figure 1C,D).
Independent of CNL‐status, we next examined whether grade 1 CTNNB1‐mutant ECs had a unique transcriptome. Using TCGA RNA‐ sequencing from 54 CTNNB1‐wildtype tumors and 43 CTNNB1‐
mutant EC tumors, we observed that there were 1615 DEGs. KEGG

FIGU RE 1 TCGA database analysis of low‐risk endometrial cancer (EC) population. (A) Disease‐free status of grade 1 copy‐number low (CNL) ECs. (B) Frequency of CTNNB1 mutations in recurrent and disease‐free grade 1 CNL ECs. (C) Overall survival and (D) Disease‐free survival for CTNNB1‐mutant (n = 31) versus wildtype (n = 24) grade 1 CNL ECs. (E) KEGG pathway analysis. Statistical test, hypergeometric distribution and Benjamini–Hochberg multi‐comparison test. (F) Scatter plot of the differentially expressed genes (DEG) between grade 1 CTNNB1‐mutant and ‐wildtype ECs. Red dots indicate Wnt pathway genes identified in (E). (G) Recurrence‐free survival for grade 1 ECs with
low versus high combined mean expression of 15 Wnt pathway gene. (H) Same as G, but with a subset of 11 Wnt pathway genes that were found by iterative modeling to be strongly and significantly associated with recurrence‐free survival. TCGA, The Cancer Genome Atlas [Color figure can be viewed at wileyonlinelibrary.com]

pathway analysis of the DEG showed significant enrichment of sev- eral pathways, including Pathways in Cancer, Wnt signaling, and MAPK signaling (Figure 1E). Given CTNNB1‐mutations are associated
with elevated risk for EC recurrence and the established oncogenic role of the Wnt/β‐catenin pathway, we observed that the individual expression of certain “Wnt Pathway” genes correlated to recurrence
free survival. Through iterative modeling (Figure S1C and S1D) we
identified a sub‐set of Wnt/β‐catenin target genes that demonstrate association with recurrence‐free survival (HR: 19.14, 95% CI: 3.37–108.80; Figure 1G,H). Examining TCGA, we compared CTNNB1
mutational status with increased expression of the 11 prognostic Wnt pathway genes from Figure 1H. CTNNB1 mutational status significantly co‐occurred with elevated gene expression for 7 of 11
genes (Figure S1D). These data reinforce the concepts that CTNNB1 mutations activate the Wnt/β‐catenin transcriptional program and an increase in expression of Wnt/β‐catenin target genes is closely
correlated with disease recurrence.

⦁ | EC cell lines have variable CTNNB1 expression and β‐catenin transcriptional activity
CTNNB1 mutations and Wnt/β‐catenin activation convey a poorer prognosis in EC; thus, we next wanted to examine the effect of Wnt/ β‐catenin pathway inhibition in in vitro EC models. A panel of
CTNNB1‐wildtype (Ishikawa and HEC1B) and CTNNB1‐mutant
(HEC108 and HEC265) EC cell lines was selected (Table 1). The messenger RNA (mRNA) expression of CTNNB1 varied among the parental cell lines with HEC108 having the lowest expression
(Figure 2A). The protein expression of β‐catenin reflected the vari-
able CTNNB1 mRNA expression (Figure 2B). The mRNA expression of β‐catenin transcriptional target genes MMP7, MYC, FOSL1, CCND1 was also variable among the parental EC cell lines (Figure S2B).
To determine whether there were any differences in the growth between the cell lines we used a more physiological 3D matrigel spheroid model.34 In 3D culture, the parental EC lines grew into
variable spheroid size and number: CTNNB1‐mutant cell lines grew
into larger spheroids than CTNNB1‐wildtype cell lines, but had fewer spheroids grow out overall. Specifically, HEC108 and HEC265 had
significantly larger mean spheroid size than HEC1B and Ishikawa (102.3 au, 91.8 au vs. 69.4 au, 54.4 au, respectively) (Figure 2C), but had a statistically lower spheroid count per 4× field (mean spheroid count 40.7, 48.7 versus 103.7 and 128.7, respectively) (Figure 2D).

⦁ | Downstream Wnt/β‐catenin inhibition reduces cell viability in CTNNB1‐mutant cell lines

We aimed to pharmacologically dissect the dependence of the
Wnt/β‐catenin pathway in the panel of EC cells (Figure 3A). We hypothesized that Wnt/β‐catenin pathway inhibition of effectors downstream of β‐catenin transcriptional activity would be more

FIGU RE 2 CTNNB1 mRNA expression, β‐catenin protein expression and spheroid growth of CTNNB1‐wildtype and CTNNB1‐mutant cell lines. (A) CTNNB1 mRNA expression by qPCR and (B) β‐catenin expression by immunoblot among CTNNB1 of CTNNB1‐wildtype (Ishikawa, HEC1B) and CTNNB1‐mutant (HEC108, HEC265) cell lines. (C) Representative images and spheroid diameter (au; scale bar = 50 au) and D) Representative images and spheroid count in a 4× field of CTNNB1‐wildtype (Ishikawa, HEC1B) and CTNNB1‐mutant (HEC108, HEC265) cell lines grown in 3D culture (au; scale bar = 500 au). Experiments conducted at least two independent times in triplicate. Statistical test, one‐way
ANOVA, Tukey multicomparison. *p < 0.05, **p < 0.01, ****p < 0.0001. Error bars, SEM. ANOVA, analysis of variance; mRNA, messenger RNA

FIGU RE 3 Dose response, apoptosis and proliferation in CTNNB1‐wildtype and CTNNB1‐mutant cell lines following treatment with Wnt/β‐ catenin signaling inhibitors. (A) Schematic of Wnt/β‐catenin signaling pathway and the points at which five inhibitors (Wnt‐C59, XAV939, PyrPam, PRI‐724, SM04690) act on the pathway. (B) Dose response curves for CTNNB1‐wildtype (Ishikawa, HEC1B) and CTNNB1‐mutant (HEC108, HEC265) cell lines performed by measuring %cell confluency with Licor cell stain following treatment with serial doses of Wnt‐C59 (µmol/L), XAV‐939 (µmol/L), and PyrPam (nmol/L) and (C) PRI‐724 (µmol/L) and SM04690 (nmol/L). (D) Apoptosis measured by %cells Annexin V/PI positive among CTNNB1‐wildtype (Ishikawa, HEC1B) and CTNNB1‐mutant (HEC108, HEC265) cell lines following serial dosing of SM04690 (0–128 nmol/L). (E) Cells treated with SM04690 for 48 h and incubated with BrdU for 1 h. (F) CTNNB1‐S33Y transduced into HEC1B
and Ishikawa cells. Control and S33Y cells were used for a SM04690 dose response assay, (G) Control and S33Y cells were treated with SM04690 for 48 h and Annexin V/PI positivity measured. (H) BrdU Incorporation control and S33Y cells treated with SM04690 for 48 h.
Experiments conducted at least two independent times in triplicate. Statistical tests, nonlinear regression (B, C); one‐way ANOVA, Tukey
multicomparison (D, E, G, H, I); and unpaired t test (F). *p < 0.05, **p < 0.01, ***p < 0.001. Error bars, SEM. ANOVA, analysis of variance; BrdU, 5′‐bromo‐2′‐deoxyuridine; PI, propidium iodide [Color figure can be viewed at wileyonlinelibrary.com]

detrimental in CTNNB1‐mutant cells compared to wildtype cells. Upstream targets included (1) Wnt‐C59, which inhibits Porcupine (PORCN) palmitoleoyltransferase activity and blunts the secretion of
Wnt ligands35; (2) XAV‐939, which stabilizes Axin in the destruction complex and therefore promotes degradation of β‐catenin40; and (3) PyrPam, which promotes GSK3 phosphorylation of β‐catenin,
thereby promoting its degradation.36 Downstream targets included
(1) PRI‐724, which blocks the interaction of β‐catenin with CREBBP, a co‐activator of β‐catenin transcriptional activity37,39; and (2) SM04690, which is a small molecule that indirectly inhibits
TCF/β‐catenin transcriptional activity by inhibiting intranuclear CDC‐like kinase 2 and thus disrupting alternative splicing.38
Dose escalation of Wnt‐C59, XAV‐939, and PyrPam in CTNNB1‐
mutant and ‐wildtype cell lines inclusive of Ishikawa, HEC1B, HEC108, and HEC265 demonstrated minimal activity as defined by
cell confluence greater than 50% measured by a fluorescence cell tag (Figure 3B, Figure S1 and S3). Of these upstream inhibitors, PyrPam only had a moderate effect on cell lines, irrespective of CTNNB1 mutational status, in particular HEC265 cell line, which may be a toxicity effect.

Downstream inhibition with PRI724 was effective broadly at doses ranging from 64 µmol/L to 256 µmol/L with less than 50% cell confluence achieved in all cell lines (Figure 3C). The two highest doses (PRI724 128 and 256 µmol/L) demonstrated significantly lower %cell confluence in HEC265 compared with HEC1B (p < 0.05). Moreover, Ishikawa cells demonstrated increased sensitivity to PRI724, possibly due to mutations within the target, CREBPP.45 SM04690 demonstrated activity at lower 50% cell confluence dose ranges from 256 nmol/L to 1024 nmol/L in the Ishikawa, HEC108 and HEC265 cell lines (Figure 3C). HEC1B %cell confluence was never below 50.0% when treated with SM04690.
Treatment with SM04690 demonstrated increased activity in the CTNNB1‐mutant cell lines compared to wildtype (Figure 3C,D). Beginning at an SM04690 dose of 64 nmol/L, HEC108 and HEC265 (CTNNB1‐mutant), had significantly lower % cell confluence than
HEC1B and Ishikawa (CTNNB1‐wildtype) (24.2%, 32.3% vs. 71.4%,
50.4%, p < 0.0001). This level of significance was maintained for all subsequent serial doses of SM04690.
Mechanistically, we examined SM04690's effect on apoptosis and proliferation via Annexin V/PI and BrdU incorporation, respec- tively. In Ishikawa and HEC265, SM04690 induced a mild apoptotic in a dose dependent fashion (Figure 3D; gating strategy Figure S3A). In these CTNNB1 wildtype cell lines, statistical significance in % Annexin V/PI positive cells were only reached at high doses of 128 nmol/L. In contrast, SM04690 induced a robust apoptotic re- sponse in HEC108 cells (Ctrl, 0.65% vs. 128 nmol/L 28.5% Annexin V/PI positive). With respect to proliferation, SM04690 significantly inhibited BrdU incorporation and an exceptional inhibition in the
HEC265 cell lines (Figure 3E; gating strategy Figure S3B). These data highlight that the CTNNB1‐mutant cells lines are more sensitive to SM04690. The source of this sensitivity does seem to vary among
cell lines, with HEC108 demonstrating a proapoptotic response and HEC265 demonstrating an antiproliferative response, likely due to each cell line's larger mutational profile.
We further examined the direct role of the CTNNB1 mutation on conveying sensitivity to SM04690 by transducing a serine 33 to
tyrosine (S33Y) CTNNB1‐mutant into wildtype cell lines (HEC1B and
Ishikawa). In both HEC1B and Ishikawa, the introduction of the S33Y CTNNB1‐mutant resulted in a slower proliferation rate (Figure S3C). Sensitivity to SM04690 and PRI724 was assessed in the HEC1B, HEC1B‐S33Y, Ishikawa, and Ishikawa‐S33Y cells via the dose re- sponse assay. Treatment with both SM04690 and PRI724 demon- strated increased activity in the CTNNB1‐mutant S33Y cell lines compared to wildtype parent cell lines (Figure 3F AND S3D).
Following treatment with SM04690 64 nmol/L, %cell confluence for HEC1B‐S33Y was significantly lower than HEC1B (44.4% and 71.4%, respectively, p < 0.05), and this difference was maintained with subsequent doses. Ishikawa‐S33Y had a significantly lower %cell confluence than the Ishikawa control starting at a SM04690 dose of
16 nmol/L (58.8% and 95.6%, respectively, p = 0.026), and this dif-
ference was also maintained with subsequent doses. When treated with PRI724, HEC1B‐S33Y had a significantly lower % cell con- fluence than HEC1B starting at 8.0 µmol/L (48.92% and 69.05%,
respectively, p < 0.01) and Ishikawa‐S33Y had a significantly lower % cell confluence than Ishikawa‐S33Y starting at 2.0 µmol/L (56.08% and 69.56%, respectively, p = 0.008). Again, these differences were
maintained at subsequent doses. Examining apoptosis and pro- liferation, we detected a small but significant increase in apoptosis in the HEC1B‐S33Y cells treated with SM04690 compared to the
HEC1B cells (Figure 3G). However, SM04690 did not induce apop- tosis in the Ishikawa‐S33Y cells (Figure 3G). In contrast to apoptosis, SM04690 significantly inhibited BrdU incorporation in both the HEC1B‐S33Y and Ishikawa‐S33Y cells (Figure 3H).

⦁ | SM04690 inhibits β‐catenin transcriptional activity

In the CTNNB1‐mutant cell lines, TCF transcriptional activity was measured using the TOP‐FLASH/FOP‐FLASH luciferase‐based re-
porter system. Using luminescence as readout of TCF transcriptional activity, in HEC108 and HEC265 cells SM04690 inhibited TCF transcriptional (Figure 4A,B). In HEC265 cells, 32 nmol/L SM04690 increased TCF transcriptional activity possibly through a compen- satory mechanism. The SM04690 inhibition of TCF transcriptional activity results are consistent with previous findings from a color- ectal cancer model.46 PRI724 also reduced TCF transcriptional ac- tivity, albeit at higher concentrations (Figure S4A–C). Using the matched HEC1B and Ishikawa wildtype and S33Y cell lines, we de- monstrated that the S33Y cells have increased TCF transcriptional activity compared to the wildtype cells (Figure 4C,D, Control bars). In HEC1B and Ishikawa, SM04690 treatment inhibited TCF transcrip- tional activity in both the wildtype and S33Y cells lines; however, in
HEC1B‐S33Y cells treated with 64 nmol/L of SM04690 showed a
significant decrease in luminescence compared to HEC1B control cells (Figure 4C). A similar trend was observed in Ishikawa
control and S33Y cells, the SM04690‐mediated reduction in tran-
scriptional activity was more potent in the S33Y cells compared to the control cells (Figure 4D). Both PRI724 and SM04690 significantly reduce TCF transcriptional activity.

⦁ | In vivo tumors have diminished growth when treated with SM04690

Xenograft models of CTNNB1‐mutant (HEC265 and HEC1B‐S33Y) and ‐wildtype (HEC1B) tumors were evaluated with SM04690 treatment. EC cells were injected subcutaneously and tumor bearing mice were treated daily with vehicle or SM04690 (25 mg/kg via IP
injection). The HEC265, HEC1B and HEC1B‐S33Y tumors all had similar volumes at the initiation of treatment (Figure S5A).
In the HEC265 xenograft model, SM04690 significantly inhibited tumor growth rate and tumor volume compared to vehicle was 336.2
and 979.7 mm3, respectively, p < 0.0001 (Figure 5A and Figure S5B). In wildtype and HEC1B‐S33Y tumor bearing mice, the tumors began to ulcer at Day 19 of treatment. Mice were treated until Day 25 at

FIGU RE 4 β‐Catenin/TCF transcriptional activity in CTNNB1‐wildtype and CTNNB1‐mutant cell lines following treatment with SM04690. TCF transcriptional activity measured via TOP‐FLASH luciferase‐based reporter system. (A) HEC108 and (B) HEC265 (CTNNB1‐mutant) cell lines were transfected with either TOP‐ or FOP‐FLASH and treated with increasing doses of SM04690 for 48 h. Luminescence was normalized to cell number and FOP‐FLASH signal (transfection control). (C) HEC1B (CTNNB1‐wildtype) and HEC1B‐S33Y (CTNNB1‐mutant) cell lines and
(D) Ishiskawa (CTNNB1‐wildtype) and Ishikawa‐S33Y (CTNNB1‐mutant) were transfected with either TOP‐ or FOP‐FLASH and treated with increasing doses of SM04690 for 48 h. Luminescence was normalized to cell number, FOP‐FLASH signal (transfection control), and parental cell line. Experiments conducted at least two independent times in triplicate. Statistical test, one‐way ANOVA, Tukey multicomparison. *p < 0.05,
**p < 0.01, ***p < 0.001, ****p < 0.0001. Error bars, SEM. ANOVA, analysis of varianc; TCF, T cell factor

which point the mice required euthanization. At both 19 and 25 days, SM04690 significantly inhibited tumor growth rate (Figure 5B,C and Figure S4C). At Day 19, the tumor volumes for the HEC1B tumors of
treatment versus vehicle were 146.4 and 335.4 mm3 (p < 0.0001) and for HEC1B‐S33Y tumors was 136.4 and 243.1 mm3, respectively (p = 0.014; Figure 5B,C).
Using IHC, we next assessed β‐catenin expression, apoptosis (cleaved caspase 3) and proliferation (Ki67). There was not a sig- nificant difference in total β‐catenin levels in the HEC1B‐S33Y compared to HEC1B tumors (Figure S5D). However, we also eval- uated whether final tumor volume was correlated with β‐catenin expression and, in two of three models (HEC265 and HEC1B), there was an inverse correlation with a higher β‐catenin expression being significantly correlated to a lower final tumor volume of treated mice
(Figure 5D–F). This inverse correlation suggests that increased β‐ catenin conveyed sensitivity to SM04690. Apoptosis was not in- creased in the HEC265, HEC1B or HEC1B‐S33Y SM04690 treated in
vivo tumors (Figure S5E,‐F). In HEC265 tumors, SM04690 sig-
nificantly inhibited proliferation (p = 0.0241; Figure 5G,H). With re- spect to growth, in the HEC1B tumors the S33Y vehicle treated tumors grew significantly slower compared to wildtype tumors
(Figure S4G). In HEC1B‐S33Y tumors, SM04690 reduces prolifera-
tion, as demonstrated by a significantly lower Ki67 score (Figure 5I,J). There appears to be a similar trend towards lower Ki67 score, or reduced proliferation, in HEC1B tumors treated with

SM04690, but this is not statistically significant (Figure 5I,J). Relating these in vivo findings to human tumors we examined the TCGA primary tumors with or without driver CTNNB1 mutations. The
CTNNB1‐mutant tumors have a significantly lower MKI67 expression
compared to CTNNB1‐wildtype tumors (Figure 5K). These data sug- gest that β‐catenin mutant tumors likely grow slower and that tar- geting β‐catenin transcriptional activity further slows tumor
progression via inhibiting proliferation.

4 | DISCUSSION

Clinically, CTNNB1 mutational status conveys an increased risk of EC recurrence in certain populations. Specifically, our TCGA analysis demonstrated that CTNNB1 mutations were associated with worse
disease‐free survival in low‐risk patients (Grade 1, CNL subgroup),
and all recurrent cases in this low‐risk population were CTNNB1‐ mutant. Our TCGA analysis also supports the idea that aberrant activation of the Wnt/β‐catenin pathway conveys a similar risk of disease recurrence. In vitro and in vivo analysis of EC in this manu- script elucidate the importance of the Wnt/β‐catenin pathway in cancer cell viability and tumor progression. We discovered that CTNNB1‐mutant cell lines have increased β‐catenin/TCF transcrip-
tional activity. Upstream blockade of the Wnt/β‐catenin pathway
through porcupine inhibition (Wnt‐C59), stabilization of APC (XAV‐

FIGU RE 5 Xenograft models of CTNNB1‐wildtype and CTNNB1‐mutant tumors treated with SM04690 versus vehicle. (A) Changes in mean tumor volume of HEC265 (CTNNB1‐mutant) tumors in mice treated with 28 days of daily intraperitoneal treatment with SM04690 25 mg/kg (Blue dots/lines) versus vehicle (Red dots/lines). (B) Changes in mean tumor volume of HEC1B tumors (CTNNB1‐wildtype) and (C) HEC1B‐S33Y (CTNNB1‐mutant) tumors, in mice treated with 19 days of daily intraperitoneal SM04690 25 mg/kg (Blue dots/lines) versus vehicle (Red dots/ lines). (D) Correlation between final tumor volume (mg) of SM04960‐treated mice and β‐catenin histological score (H‐score) determined by immunohistochemistry (IHC) analysis of HEC265, (E) HEC1B and (F) HEC1B‐S33Y tumors in mice treated with SM04690 25 mg/kg
intraperitoneally daily. (G) Representative images of IHC of Ki67 in HEC265 control and SM04690 treated tumors. Scale bar = 50 microns.
(H) Ki67 H‐score determined by IHC analysis of HEC265 control and SM04690 treated tumors. (I) Representative images of IHC of Ki67 in HEC1B (wildtype) and HEC1B‐S33Y tumors treated with control or SM04690. Scale bar = 50 microns. (J) Comparison of Ki67 H‐scores in HEC1B and HEC1B‐S33Y control and SM04690 treated tumors. (K) Comparison of MKI67 mRNA expression between endometrial cancer tumors with and without driver CTNNB1 mutations from the TCGA database. (A,B,C) Statistical tests, linear regression; (D,E,F) Pearson correlation; (G) unpaired t test; and (H, I) one‐way ANOVA, Tukey multi‐comparison; and (J) unpaired t test followed by Benjamini–Hochberg. *p < 0.05,
***p < 0.001. Error bars, SEM. mRNA, messenger RNA; TCGA, The Cancer Genome Atlas [Color figure can be viewed at wileyonlinelibrary.com]

939) and promotion of GSK3 phosphorylation (PyrPam) are not as effective in in vitro analysis compared to downstream direct
β‐catenin transcriptional blockade (PRI‐724 and SM04690). We
therefore focused our further analysis on downstream inhibitors of β‐catenin transcription. SM04690 was more promising for future development, as preclinical analyses demonstrated efficacy in the
low nanomolar range and early clinical studies have produced safety data in both animal and human studies.
Physiological doses of SM04690 (64 nmol/L and greater) in vitro inhibited viability and proliferation of EC cell lines irrespective of
CTNNB1 mutation, however demonstrated increased effectiveness on CTNNB1‐mutant cell lines. Introduction of the S33Y mutation in the HEC1B cells caused the tumors to grow more slowly than their
parent cell line confirming the relation of mutational status to this effect. The combined in vitro and in vivo data examining apoptosis and proliferation demonstrate that mechanistically SM04690, espe- cially in the setting of a CTNNB1 mutation, profoundly inhibits pro- liferation rather than induces apoptosis. These conclusions were further highlighted in primary tumors from the TCGA data set. This also explains rational in which transcriptional blockade Wnt in- hibitors are more effective at inhibiting tumor growth in CTNNB1
mutated tumors but are also effective in non‐mutated tumors as the
Wnt pathway can still be active in non‐mutated cells.
The cell lines utilized in this study represent EC tumors of a variety of histologic grades (Table 1). Although there is literature demonstrating an association between CTNNB1 mutations and low

grade EC histology,23 as well as an association between CTNNB1 mutations and risk of recurrence in low grade EC,12,23,28,29 it is also important to note that CTNNB1 mutations and the aberrant Wnt activation signature are present in EC of all grades, including the cell lines utilized in this study.13,45 In TCGA, 44.8% of Grade 1, 35.3% of Grade 2% and 16.3% of Grade 3 ECs had CTNNB1 mutations.13
Therefore, our results demonstrating β‐catenin/Wnt inhibition re-
sults in decreased EC viability and proliferation in in vitro and in vivo models indicate that CTNNB1 mutation and an aberrant Wnt acti- vation signature may be a targetable molecular marker in EC, no matter the grade.
Clinically, this data is promising for future drug development and leads to a hypothesis that transcriptional Wnt blockade may be a more effective maintenance therapy in EC rather than single agent or combination cytotoxic chemotherapies. Cytotoxic chemotherapies are most effective on rapidly dividing cells and therefore have less rational for combinatory therapy. For the same reason, there is less rational for these cytotoxic chemotherapies in slower growing tu- mors like those that are Grade 1 and CTNNB1 mutant. Historically, there has been concern regarding clinical use of Wnt inhibitors as they have been associated with significant side effects, such as bone loss.47 However, murine studies and Phase I and II human studies have demonstrated a tolerable safety profile for SM04690 and its bioequivalent.38,41,46 Also, while the bioavailability of SM04690 is not optimal for oral administration, the bioequivalent and next generation of compound, SM08502, has improved bioavailability and shows antitumor effect in gastrointestinal cancer models.41 SM08502 is currently in a phase I clinical trial for advanced solid tumors (NCT03355066); highlighting the possibility of translating the findings of this report into a targeted treatment option for pa- tients with EC. Overall, this report provides strong rationale for
targeting the Wnt/β‐catenin pathway in CTNNB1‐mutant EC at the
nuclear level.

ACKNOWLEDGMENTS
The authors would like to acknowledge funding from The University of Colorado OB/GYN Academic Enrichment Fund (MM), The
University of Colorado Cancer Center Developmental Therapeutics Program (BGB), The American Cancer Society (BGB; 134106‐RSG‐
19‐129‐01‐DDC), and ABOG/AAOGF (BC). Support of Core Facilities
was provided by the University of Colorado Cancer Center Support Grant (P30CA046934).

CONFLICT OF INTERESTS
The authors declare that there are no conflict of interests.

DATA AVAILABILITY STATEMENT
The data that support the findings of this study are available from the corresponding author upon reasonable request.

ORCID
Bradley R. Corr http://orcid.org/0000-0002-6608-2585
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