The EVE Biomarker Study was an exploratory, open‐label, single‐arm, multicentre study (ClinicalTrials.gov Identifier: NCT02109913; EudraCT number 2013‐004120‐11) to gain insight into tumour characteristics in order to predict which patients would have a high chance for a long PFS while using standard EVE/EXE. Eligible patients were ≥ 18‐year‐old postmenopausal women with ER‐positive, HER2‐negative (ER+/HER2‐) MBC and candidates for standard EVE/EXE. Their disease had to be refractory to a nonsteroidal aromatase inhibitor (NSAI) defined as a recurrence ≤ 12 months of adjuvant anastrozole or letrozole or having progressed while on or within 1 month of discontinuing NSAI treatment for metastatic disease. The NSAI did not have to be the last systemic treatment prior to enrolment. Previous treatment with mTOR inhibitors was not allowed. Patients receiving hormone replacement therapy, or those (zero)positive for HIV, hepatitis B or C or with inadequate bone marrow, liver or renal function, were excluded. All patients signed informed consent before enrolment. The study was approved by the Independent Ethics Committee of Amsterdam UMC and Institutional Review Boards at each participating site (Table S1). The study was performed in compliance with Good Clinical Practices, the Declaration of Helsinki, and carried out in keeping with applicable local law(s) and regulation(s).

Patients received EVE 10 mg and EXE 25 mg orally per day in cycles of 28 days. A starting dose of 5 mg daily for EVE was allowed to prevent stomatitis in frail patients, but in the absence of symptoms, this dose had to be increased to 10 mg in the next 2 weeks. Dose interruptions or modifications were allowed for adverse events (AEs) suspected to be related to EVE according to protocol guidelines. AEs were classified according to common terminology criteria for AEs (CTC‐AE) 4.03. AEs grade ≥ 2 were recorded in the electronic case‐record forms. Serious AEs were reported until 28 days after discontinuation of EVE unless related to progressive disease. Tumour measurements were performed with radiographic assessments to determine therapy efficacy preferably every 12 weeks.

Baseline blood samples were obtained immediately before dosing of EVE/EXE. Plasma from EDTA tubes was prepared within 30 min after blood collection by centrifugation at 1500 g for 10 min at room temperature. Plasma was stored at −20 °C at the local sites until it was shipped to the central laboratory. The workflow for the isolation and NGS evaluation of cfDNA is summarised in Fig. S1. cfDNA was isolated from 2 mL plasma with a customised Maxwell^® (MX) RSC ccfDNA Plasma Kit (Promega, Madison, WI, USA), an automatic magnetic beads‐based method. After plasma was defrosted, a second centrifugation at 12 000 g for 10 min at room temperature was performed. In all cases, cfDNA was isolated from a starting volume of 2 mL of plasma and eluted in 60 µL of the provided elution buffer. All cfDNA isolations were performed using the manufacturer’s protocol, including a third centrifugation step at 2000 g for 10 min at room temperature to eliminate residual white blood cells. Additionally, the custom Maxwell^® RSC ccfDNA Plasma Kit for large plasma volume protocol was used. In brief, equal amounts of plasma and binding buffer were added together with 140 µL of magnetic beads. This mix was shaken and incubated for 45 min at room temperature and subsequently centrifuged at 2000 g for 1 min at room temperature. The pelleted mix of beads and cfDNA were transferred to the cartridge and run further on the MX instrument following standard procedures.

The cfDNA of plasma from 10 healthy blood donors (HBDs) and from 171 MBC patients were analysed using the Ion Torrent™ Oncomine™ Breast cfDNA Assay in combination with the Ion Torrent S5XL Next Generation Sequencing (NGS) system, all according to protocols and consumables provided by the manufacturer (Life Technologies, Thermo Fisher Scientific, Waltham, MA, USA) (Vitale et al., ). The cfDNA input for our HBDs ranged from 4.86 to 10.41 ng, whereas for almost all MBC patients, 10 ng cfDNA could be used to generate targeted libraries following the manufacturer’s protocol. Firstly, concentrations of each Oncomine™ cfDNA library were determined by qPCR using the Ion Library TaqMan^® Quantitation Kit and then diluted to a final concentration of 50 pm. Next, sample barcoded libraries were pooled together for template preparation on the Ion Chef™ (Life Technologies) Instrument using the Ion 540™ (Life Technologies) Kit – Chef and loaded onto an Ion 540™ chip. The chip was sequenced on an Ion S5™ XL Sequencer Systems, and the data were analysed using the Ion Torrent Suite™ software 5.2.2 and Torrent Variant Caller 5.2.1.39 (Life Technologies) and applying default software settings for low mutation frequency detection. NGS data were checked using several quality control thresholds (Fig. S1). Median read depth, median molecular coverage and mean read lengths were reported as general NGS quality measure for each cfDNA sequenced (Table S2). Samples were sequenced at a median 20 000× read depth coverage. Those cfDNA specimens with median molecule coverage below 500 molecules were excluded from further NGS analyses. The NGS data included novel and hotspot variants and were quantified by read and molecule numbers for both total and variant sequences. For this study, hotspot mutations were further analysed only when the variant itself was identified in at least three independent molecules and in 10 reads or more, and when the amplicon of the variant was sequenced for at least 300 independent molecules covered by 5000 reads or more.

The Oncomine Breast Assay sequences 26 amplicons to detect 157 hotspots and indels for a panel of 10 breast cancer relevant genes (AKT1, EGFR, ERBB2, ERBB3, ESR1, FBXW7, KRAS, PIK3CA, SF3B1 and TP53; Fig. S1) as detected by Ion Torrent Suite™ 5.2.2 and Torrent Variant Caller 5.2.1.39 (Life Technologies). This NGS Assay applies molecular barcoding enabling the detection of mutations at allele frequencies as low as 0.1% with a recommended input of 20 ng cfDNA. Such a lower limit of detection is relevant due to the minute numbers of ctDNA molecules as demonstrated by several studies using digital PCR (Beije et al., ; Fribbens et al., ; Grasselli et al., ). Routine NGS settings use allele frequencies of 1% as threshold for positivity. In our cohort of patients, this threshold would result in ctDNA detection in only 92 (56%) instead of 125 (76%) patients. Multiplex NGS with molecular barcoding also enables us to simultaneously detect multiple hotspot mutations in the 10 genes most commonly affected in breast cancer and quantify multiple different mutant molecules within one cfDNA analysis. Furthermore, it is equally sensitive as digital PCR analysis which only detects a single genetic variant in the same amount of sample.

The NGS findings for each variant were expressed as mutant ctDNA molecule numbers per mL plasma (Fig. S1), next to variant allele frequencies (VAF). ctDNA‐positive patients were defined as those with at least two (≥ 2) mutant ctDNA molecules per mL plasma, while patients with less than two (< 2) ctDNA molecules per mL plasma were called ctDNA‐negative.

The genes with mutations in cfDNA were verified in cBioPortal for their occurrence in ER+/HER2− breast carcinomas using the datasets of MK, Molecular Taxonomy of Breast Cancer International Consortium (METABRIC) and The Cancer Genome Atlas (TCGA) separately and combined (see details in Table S3). In addition, our identified cfDNA hotspot mutations were explored in catalogue of somatic mutations in cancer (COSMIC; v90) and International Agency for Research on Cancer (IARC) TP53 (v20) databases (details in Table S4). Each mutation was verified in COSMIC whether it was reported as confirmed somatic and how often it was observed in breast cancer. The TP53 mutations were evaluated in IARC for the total somatic and germ‐line counts (Bouaoun et al., ).

Progression‐free survival was calculated as the time from the start of EVE/EXE until radiological progression of disease, clear clinical signs of progression or death by any cause. If there was no evidence of progression, but treatment was discontinued for whatever reason, patients were censored at time‐to‐treatment switch. Patients who were still on treatment at the data lock (1 March 2018) were censored at the last confirmed date of EVE/EXE exposure. OS was calculated as the time from the start of treatment until registered death; patients still alive or lost to follow‐up were censored at the last date of confirmed contact. Patients who stopped treatment with EVE/EXE within the first month were excluded from the PFS and OS analyses.

To investigate differences in ctDNA characteristics among patients with and without benefit from EXE/EVE, we divided the group into tertiles based on the duration of PFS. Each subgroup contains a third of the patients: PFS‐T1 (PFS of 2.5 months), PFS‐T2 (PFS of 5.1 months) and PFS‐T3 (PFS of 11.5 months; Table ). To test whether the sum of specific mutations was able to distinguish survival differences in patients on treatment with EVE/EXE, an exploratory analysis was performed using cut‐off points with various numbers of mutations. A binary score of less than three (< 3) and three or more (≥ 3) specific mutations showed the clearest difference in PFS and was used in further analyses under the definition ‘number of mutations’. The median tumour load of 54 molecules per mL plasma in ctDNA‐positive patients was used as conservative threshold to distinguish patients with high ctDNA load (> 54 molecules) from those with no or low ctDNA load (0–54 molecules).

Tests for trends, Kruskal–Wallis and chi‐square were performed for nonparametric analyses of continuous or categorical variables and used as indicated in Tables. To analyse which ctDNA characteristics related with PFS or OS, multivariate step‐down analyses were performed for ctDNA characteristics with at least 10% patient cases per characteristic. Uni‐ and multivariate Cox regression analyses were used to calculate HR, 95% confidence intervals (95% CI) and P‐values. Clinicopathological factors included in the multivariate analyses were age, disease‐free interval (DFI), visceral metastasis, (neo)adjuvant therapy, number of treatment lines for metastatic disease, progesterone receptor (PR) and Eastern Cooperative Oncology Group (ECOG) screening visit status. P‐values were two‐sided and significance was defined at < 0.05. Survival time analyses were visualised by Kaplan–Meier curves; log‐rank test was applied to test for differences between survival curves. The study complied with reporting recommendations for tumour marker prognostic studies (REMARK) criteria (McShane et al., ). Statistical analyses were generated with spss 22.0 (IBM SPSS, Armonk, NY,USA) and STATA 14 (StataCorp LLC, College Station, TX, USA).

A total of 178 patients signed informed consent between March 2014 and February 2017 in 28 participating hospitals in the Netherlands (Table S1). Two patients were excluded who did not meet the inclusion and exclusion criteria, and one patient was excluded who never started treatment (Fig. S2; Table S5). Median PFS was 5.3 months (95% CI: 4.77–5.87) ranging from 0.46 to > 36.8 months.

At the data lock on 1 March 2018, five patients were still on treatment. Reasons for discontinuation other than progressive disease were as follows: toxicity (N = 13), physician’s decision (N = 2) and one at request of the patient. Median age of the study participants was 63 years. Most patients had metastases involving two or more sites (82%); 26 patients (15%) had bone only disease. At the time of the primary diagnosis, 128 (73%) tumours were PR positive. Thirty‐six patients (21%) presented with advanced disease as first breast cancer diagnosis. Most patients received prior systemic treatment for their metastatic disease; for 17 patients (10%), EVE/EXE was given as first‐line therapy in the metastatic setting.

In total, 383 AEs grade ≥ 2 occurred, which were possibly, probably or definitely related to EVE. The most common AEs grade ≥ 2, either possibly, probably or definitely related to EVE are listed in Table S6. There were three on treatment deaths not related to EVE/EXE. One patient died from pneumonitis related to EVE in the follow‐up period of 28 days.

Next‐generation sequencing data could be generated for 164 out of 175 patients (Figs S1 and S2; Table S5). Reasons for exclusion were as follows: no baseline plasma available (N = 5), insufficient NGS quality (N = 2) and discontinuation of treatment within cycle 1 due to toxicity (N = 4). Clinicopathological characteristics of the 164 patients are shown in Table S5.

Most patients had mutations in PIK3CA [76/164 (46%)], ESR1 [65/164 (40%)], and TP53 [37/164 (23%)] (Fig. A, Table S3). Mutations were rare in SF3B1 [6/164 (4%)], AKT1 [5/164 (3%)], ERBB2 [3/164 (2%)], ERBB3 [3/164 (2%)], KRAS [2/164 (1%)] and were not detected in EGFR and FBXW7. The most frequently detected variants (Fig. B, Table S4) resulting in oncogenic amino acid changes in ESR1 were p.D538G (N = 38), p.Y537S (N = 27) and p.E380Q (N = 17). For PIK3CA, these were p.E545K (N = 25), p.H1047R (N = 24) and p.E542K (N = 15).

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Mutational landscape of this study. (A) Landscape plot summarising 125 patients with gene mutations (orange boxes) detected in cfDNA by the Oncomine NGS panel. Number of hotspot mutations is illustrated by the blue vertical bars and the number of patients with a gene mutation by the green bars. (B) Sunburst plots for gene hotspot mutations identified in patients grouped per PFS tertile. Genes and hotspot mutations are ordered clockwise from high to low incidence. ESR1 hotspot mutations, especially p.Y537S, are most frequent in patients with poor response to EVE/EXE (PFS‐T1). The SF3B1 mutations are mainly observed in patients with benefit from EVE/EXE (PFS‐T3). (C) In silico analyses of ER+/HER2− breast carcinomas using the cBioPortal datasets MSK, METABRIC, TCGA. The Oncomine cfDNA panel genes and the most frequently mutated genes of each dataset are shown. Only the ESR1 mutation frequency in our study is considerably higher than that within the other datasets.

The TCGA, METABRIC and Memorial Sloan Kettering (MSK) datasets were explored via cBioPortal for in silico analyses of the mutational landscape of primary or metastatic biopsies of ER+/HER2‐ breast carcinomas. Mutational frequencies of all 10 genes used in the Oncomine cfDNA panel and additional genes representing the most frequently mentioned genes in each dataset are shown in Fig. C and Table S5. Of the analysed genes, the mutation frequency of only ESR1 was considerably higher in our study than in the consulted datasets. The 26 TP53 mutations detected in our study were verified in the IARC TP53 (v20) and COSMIC (v90) database for germ‐line reports (Table S5). Of these, 22 TP53 mutations were mentioned as germ‐line and only four mutations (p.C238F, p.H179L, p.L194R and p.R249M) were not. The 22 mutations with germ‐line counts in IARC were reported as confirmed somatic mutations, and 17 of these have frequently been observed in breast cancer by COSMIC. Thus far, germ‐line mutations for PIK3CA have not yet been reported.

A total of 125 of 164 patients (76%) were considered ctDNA‐positive, because they had at least two mutant ctDNA molecules per mL plasma with one (N = 55) or more (N = 70) missense hotspot mutations (Fig. S3). The median tumour load in ctDNA‐positive patients was 54 molecules per mL plasma (range 2–2549; Table S7). This median was used as conservative threshold to distinguish patients with high ctDNA load of > 54 molecules (N = 62; 38%) and those with no or low ctDNA load (N = 102, 62%). Most patients discontinued treatment due to progression of disease, although some discontinued EVE earlier than EXE. Total duration of EVE exposure and PFS correlated strongly (R = 0.95, data not shown), because of which time of treatment will not change our findings. The total dose of EVE correlated strongly with PFS (R = 0.89) and Cox regression demonstrated that this depended on ctDNA load (HR = 0.99, 95% CI: 0.99–1.00, P < 0.001; data not shown).

Patient groups were discriminated having ≥ 3 (N = 29) or < 3 (N = 135) specific mutations. Within single patients with different mutations detected, the number of ctDNA molecules among specific mutations could vary considerably (Fig. B). Multivariate step‐down analysis (Table S8) revealed that patients with ctDNA containing ≥ 3 mutations (3.4 months, P = 0.033) or with high ctDNA load (4.4 months, P = 0.024) had significantly shorter median PFS than patients with fewer mutations or with no/low ctDNA load (5.4 months and 5.7 months, respectively; Fig. A). This was confirmed in uni‐ as well as multivariate analyses (Table , Table S9) and illustrated by Kaplan–Meier curves (Fig. A). Of interest, the number of mutations and ctDNA load combined correlated more strongly with PFS than each separate factor in both uni‐ and multivariate analysis as shown in Table .

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ctDNA characteristics and survival. (A) The ctDNA load and number of mutations and their relation with PFS on EVE/EXE and with OS. (B) Samples (n = 29) with ctDNA containing ≥ 3 mutations showing heterogeneity in mutant ctDNA molecules per patient. It represents the sum of mutant ctDNA molecules per mL plasma for all gene mutations found in 29 patients with ≥ 3 hotspot mutations in their ctDNA. The figure shows the patients who have < 1000 (left, N = 18) or more than 1000 (right, N = 11) mutant ctDNA molecules per mL plasma. Some patients exhibit clearly large differences in the number of mutant ctDNA molecules among mutations. (C) Top 10 most frequent gene hotspot mutations observed in this study and relationship with PFS and OS. (D) Patients with ESR1 p.Y537S mutations (n = 27) have no other mutation (n = 4), additional mutations in ESR1 (n = 12), or mutations in other genes (n = 11).

We compared ctDNA characteristics among three subsets of patients grouped in tertiles based on PFS period. These three subsets were similar for clinicopathological factors (Table , Fig. B). Patients in PFS‐T3 had preferentially less ctDNA molecules (median 15) than patients in PFS‐T2 (median 26) and PFS‐T1 (median 54). SF3B1 mutations were preferentially observed in patients in PFS‐T3 (Table , Fig. B). Patients with shorter PFS from EVE/EXE had relatively more ctDNA containing ESR1 mutations compared to those with benefit (Fig. B). Specifically, ESR1 variants p.Y537S (P = 0.023), p.Y537N (P = 0.084), and p.Y537C (P = 0.088) were preferentially observed in patients in PFS‐T1 (Fig. B, Table S4). Univariate Cox regression analyses confirmed these findings (Fig. C, Table S10). Since ESR1 p.Y537S was one of the most frequently observed mutations (n = 27) and especially in patients with short PFS, it was investigated in more detail (Fig. D). In four patients, ESR1 p.Y537S was the only hotspot mutation identified. Twelve patients had additional ESR1 mutations, whereas the remaining eleven patients had one or more mutations in other genes.

Uni‐ and multivariate Cox regression analyses of clinicopathological factors, ctDNA load and number of hotspot mutations for PFS and OS are presented in Table . Clinicopathological factors associated with a worse PFS in the univariate analyses were age > 70 years (P = 0.047) and visceral metastases (P = 0.043). In the multivariate analyses, presence of visceral metastases and (neo)adjuvant therapy turned out to be significantly associated with a worse PFS, while longer DFI was associated with a better PFS. The only clinicopathological factor associated with longer OS was DFI in both univariate and multivariate analyses (both P < 0.001). Number of mutations and ctDNA load were both independently related with a worse PFS in uni‐ as well as multivariate analyses (Table ). With regard to OS, ctDNA load was significantly related with a worse survival (uni P < 0.001, multi P = 0.008).

Shorter OS was observed in patients with high ctDNA load compared to low ctDNA load patients (HR = 2.20, P < 0.001; Fig. A). Shorter OS was also found in patients with a PIK3CA mutation (HR = 1.80, P = 0.011) and especially in those with a p.H1047R mutation (HR = 1.98, P = 0.013; Fig. C, Table S10). Step‐down analyses revealed that only high ctDNA load remained associated with a shorter OS (Table S8) as illustrated by the Kaplan–Meier survival curve (Fig. E; P < 0.001). Uni‐ and multivariate Cox regression analyses for OS confirmed that only high ctDNA load was significantly associated with a worse survival (uni P < 0.001, multi P = 0.008, Table ). OS in patients with ≤ 54 ctDNA molecules was 124.8 months, while that in patients with > 54 ctDNA molecules was 107.7 months. As shown in Table , combining ctDNA load with number of mutations resulted in a stronger association with OS in both uni‐ and multivariate analysis.

All data are available in supplementary files.