Article Text
Abstract
Objective Aberrant lipid metabolism is a hallmark of colorectal cancer (CRC). Squalene epoxidase (SQLE), a rate-limiting enzyme in cholesterol biosynthesis, is upregulated in CRC. Here, we aim to determine oncogenic function of SQLE and its interplay with gut microbiota in promoting colorectal tumourigenesis.
Design Paired adjacent normal tissues and CRC from two cohorts were analysed (n=202). Colon-specific Sqle transgenic (Sqle tg) mice were generated by crossing Rosa26-lsl-Sqle mice to Cdx2-Cre mice. Stools were collected for metagenomic and metabolomic analyses.
Results SQLE messenger RNA and protein expression was upregulated in CRC (p<0.01) and predict poor survival of patients with CRC. SQLE promoted CRC cell proliferation by inducing cell cycle progression and suppressing apoptosis. In azoxymethane-induced CRC model, Sqle tg mice showed increased tumourigenesis compared with wild-type mice (p<0.01). Integrative metagenomic and metabolomic analyses unveiled gut dysbiosis in Sqle tg mice with enriched pathogenic bacteria, which was correlated to increased secondary bile acids. Consistent with detrimental effect of secondary bile acids, gut barrier function was impaired in Sqle tg mice, with reduced tight junction proteins Jam-c and occludin. Transplantation of Sqle tg mice stool to germ-free mice impaired gut barrier function and stimulated cell proliferation compared with control mice stool. Finally, we demonstrated that terbinafine, a SQLE inhibitor, could be repurposed for CRC by synergising with oxaliplatin and 5-fluorouracil to inhibit CRC growth.
Conclusion This study demonstrates that SQLE mediates oncogenesis via cell intrinsic effects and modulation of gut microbiota-metabolite axis. SQLE represents a therapeutic target and prognostic marker in CRC.
- colorectal cancer
- colorectal neoplasm
- colonic microflora
Data availability statement
Data are available on reasonable request. All data are available from the corresponding author on request.
This is an open access article distributed in accordance with the Creative Commons Attribution Non Commercial (CC BY-NC 4.0) license, which permits others to distribute, remix, adapt, build upon this work non-commercially, and license their derivative works on different terms, provided the original work is properly cited, appropriate credit is given, any changes made indicated, and the use is non-commercial. See: http://creativecommons.org/licenses/by-nc/4.0/.
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Significance of this study
What is already known on this subject?
Aberrant lipid metabolism is a hallmark in colorectal cancer (CRC).
Cholesterol metabolism is frequently upregulated in CRC, but its function and potential interaction with gut microbiome remains unknown.
What are the new findings?
Squalene epoxidase (SQLE) is overexpressed in CRC and its high expression predicts poor survival.
Colon-specific Sqle transgenic expression in mice promotes colorectal tumourigenesis in azoxymethane-induced CRC.
Integrative metagenomic and metabolomic analyses demonstrate that colon-specific Sqle transgenic mice harbours a dysregulated microbiome with enriched pathogenic bacteria, which is correlated to increased secondary bile acids production.
Gut barrier function is disrupted in Sqle transgenic mice with suppressed tight junction proteins Jam-c and occludin.
Faecal transplantation of Sqle transgenic mice stool into germ-free mice promotes colonic cell proliferation and gut barrier disruption.
SQLE inhibitor terbinafine synergises with chemotherapy to inhibit CRC growth in vitro and in vivo.
How might it impact on clinical practice in the foreseeable future?
Targeting of SQLE-gut microbiome axis is a potential strategy for CRC prevention and treatment.
Introduction
Colorectal cancer (CRC) is the third most common cancer and ranks the second in terms of cancer mortality worldwide. Both the incidence and mortality of CRC are still increasing in young people, especially in low-income and middle-income countries. Patients with advanced CRC with metastasis still suffer from poor prognosis and drug resistance severely diminishes the therapeutic efficacy of chemotherapy. Hence, it is important to identify novel genes involved in the pathogenesis of CRC in order to develop effective treatments, either alone or in combination with chemotherapy.
Aberrant lipid metabolism is increasingly considered a hallmark characteristic of many cancers, including CRC. Both obesity and serum lipids are risk factors for CRC.1 2 Epidemiological studies also suggest a high dietary fat intake to increased risk of CRC.3 Lipid accumulation promotes CRC through increased reactive oxygen species and MAPK signalling.4 Fatty acids,5 6 cholesterol7 8 and bile acids9 have been implicated in CRC pathogenesis. Nevertheless, lipid metabolism-dependent molecular mechanisms involved in CRC remains poorly understood.
Squalene epoxidase (SQLE) is a rate-limiting enzyme in cholesterol biosynthesis. Recent work has shown that SQLE is overexpressed in CRC8 10 11; nevertheless, the potential role of SQLE in CRC initiation and progression remains controversial. SQLE was suggested to be oncogenic factor by promoting cell growth,10 whereas Jun et al 8 showed that reduction of SQLE could accelerate CRC metastasis. In this study, we demonstrated that SQLE is upregulated in CRC compared with adjacent normal tissues in multiple CRC cohorts and predicts poor patient survival.
To comprehensively decipher the role of SQLE in CRC, we first established colon-specific SQLE transgenic (tg) mice and SQLE knockout (KO) mice, we demonstrated the role of SQLE as an oncogene in CRC in vivo. We revealed that colon-specific SQLE overexpression promoted gut dysbiosis and metabolic alterations, which contribute to impaired gut barrier and induced colonic cell proliferation. Finally, we showed terbinafine, a Food and Drug Administration (FDA)-approved inhibitor of SQLE, synergised with 5-fluorouracil (5-FU) or oxaliplatin to inhibit the growth of CRC cells in vitro and in vivo. These findings suggest SQLE as a targetable oncogenic factor in CRC.
Materials and methods
Human CRC samples
Patient samples (Hong Kong cohort) with histologically confirmed CRC were collected in Beijing University Cancer Hospital when patients underwent surgery (n=144). Both tumour and adjacent normal tissues were immediately snap-frozen in liquid nitrogen. Patient characteristics are summarised in online supplemental table S1. An additional tissue microarray (TMA) cohort consists of 207 patients with CRC who underwent surgery in Prince of Wales Hospital, Hong Kong. The patient characteristics are summarised in online supplemental table S2. A publicly available cohort (GSE17538) was used for validation, containing 232 patients with CRC (online supplemental table S3). The Cancer Genome Atlas (TCGA) cohort dataset was accessed from UCSC Xena browser (https://xenabrowser.net/), with 50 paired adjacent normal and tumour samples from RNA-sequencing. GDS4382 consists of 17 paired adjacent normal and tumour samples analysed by the Affymetrix Human Genome U133 Plus 2.0 Array (https://www.ncbi.nlm.nih.gov/sites/GDSbrowser?acc=GDS4382).
Supplemental material
Colon-specific Sqle transgenic mice model
Sqle tg mice (Rosa26-pCAG-loxp-stop-loxp-SQLE) were previously established by us.12 To drive the colon-specific expression of SQLE, Sqle tg mice were crossed to Cdx2-CreERT2 mice. To activate SQLE overexpression, tamoxifen (100 mg/kg, intraperitoneally) was first injected to Sqle tg mice aged 6 weeks for 4 times daily to activate CreERT2. To induce colorectal carcinogenesis in Sqle tg mice, we employed the chemically induced CRC model. Briefly, azoxymethane (AOM, 10 mg/kg, intraperitoneally) was administered into mice 6 times, once per week. Mice were then sacrificed at week 24 after the first AOM injection. The number and size of tumours were recorded. All tissues were immediately stored in 10% formalin or −80°C freezer. Histology was scored after H&E staining by a pathologist blinded to the nature of samples.
Sqle knockout mice model
Whole body Sqle KO mice were generated by CRISPR/Cas9 technology. Heterozygous Sqle KO mice (Sqle+/− mice) were employed for the AOM-Dextran sulfate sodium (DSS) model, as homozygous KO mice were not viable. To induce CRC, Sqle+/− and wild-type mice were injected once with AOM (10 mg/kg, intraperitoneally) at 6 weeks of age. One week after AOM injection, three cycles of DSS treatment (2% in drinking water for 5 days) were given, with 2 weeks of break between each cycle. Mice were sacrificed 80 days after the first AOM injection. The number and size of tumours were measured. All tissues were immediately stored in 10% formalin or −80°C freezer.
Xenograft models
SW1116 and LOVO cells expressing empty vector or SQLE plasmid (1×107 cells in 0.1 mL phosphate-buffered saline (PBS)) were injected subcutaneously into the left dorsal flank of Balb/c nude mice aged 4 weeks. Subcutaneous tumour size was measured with a digital calliper. After 4 weeks, mice were sacrificed and examined. For drug treatment study, HT29 cells (1×107 cells in 0.1 mL PBS) were injected subcutaneously to dorsal flank of nude mice. The mice were randomised and received: (1) vehicle; (2) terbinafine (80 mg/kg, orally, daily); (3) 5-FU (30 mg/kg, intraperitoneally, 2 times per week); (4) oxaliplatin (10 mg/kg, intraperitoneally, once per week); (5) terbinafine+5-FU and (6) terbinafine+oxaliplatin. Tumour size was monitored and mice were sacrificed after 4 weeks.
In vivo intestinal permeability assay
To determine in vivo intestinal permeability, mice were starved overnight and fluorescein isothiocyanate (FITC)-dextran (Sigma) was administered by oral gavage (44 mg/100 g body weight). After 4 hours, mice were anaesthetised, blood was collected by cardiac puncture and mice were sacrificed. The serum was separated from whole blood, diluted and FITC fluorescence was then determined by spectrophotofluorometry (BioTek), with an excitation and emission of 485 nm and 528 nm, respectively. Serially diluted FITC-dextran was used as standard.
Shot-gun metagenome sequencing
Stool was collected from Sqle tg mice and wild-type littermates, and extracted using PowerFecal DNA isolation kit. Nextera XT adapter was used to generate amplified library, and sequencing was performed to obtain DNA (125 bp) paired end reads to a depth of 10G base pairs per sample using HiSeq Illuminex 2500. The same annotation pipeline was used for all faecal metagenomes in this study. For data analysis, host DNA removal and reads quality filtering were performed by BWA and SAM tools.13 14 After that, high-quality reads were used to obtain species-level taxonomic profiling by Kraken2 and Bracken.15 16 The differential abundance of species-level bacteria was performed by R package DESeq2.17 Bacteria species with adjusted p<0.05 and log2(fold change) >1 were considered statistically significant. Principal coordinate analysis was conducted using R packages phyloseq and vegan.18
Statistical analysis
All statistical tests were performed using SPSS (Version 19.0) or GraphPad Software. Data are presented as mean±SD. Cell viability assay and tumour growth rate evaluation was analysed with repeated-measures analysis of variance. The effect of clinical characteristics on SQLE messenger RNA (mRNA) expression and comparison between two groups was analysed with paired two-tailed Student’s t-test. The effect of clinical characteristics on SQLE protein expression was analysed with Pearson’s χ2 test or Fisher’s exact test. To evaluate the correlation between SQLE and prognosis, overall survival (OS) was defined as the duration from the date of surgery to the date of death. Using the Kaplan-Meier analysis, OS curve was formulated. Multivariate analysis for OS was performed with Cox proportional hazard regression analysis. To determine the significance SQLE on OS, log-rank test was used. P values <0.05 were considered statistically significant.
Additional methods are provided in online supplemental information.
Results
SQLE is overexpressed in patients with CRC
We analysed mRNA expression of SQLE in three independent CRC cohorts (in-house Hong Kong cohort, TCGA and GDS4382). The clinical characteristics of Hong Kong cohort are shown in online supplemental table S1. SQLE mRNA was highly upregulated in primary CRC as compared with adjacent normal tissues (n=141, p<0.0001), as determined by quantitative PCR (qPCR) (figure 1A). SQLE mRNA expression demonstrated significant correlation with advanced tumour, node, metastases stage (p<0.05) and distant metastasis (p<0.05) (online supplemental table S1). Its overexpression was validated in TCGA (n=50; p<0.0001) and GDS4382 cohorts (n=17; p<0.001) (figure 1A). At protein level, immunohistochemistry (IHC) validated overexpression of SQLE protein in CRC tumours compared with adjacent normal tissues (p<0.01) (figure 1B). Hence, SQLE overexpression is a frequent event in CRC.
SQLE overexpression is associated with poor prognosis in patients with CRC
Given its frequent overexpression in CRC, we then assessed the clinical significance of SQLE in human CRC. In Hong Kong cohort, Kaplan-Meier curve showed that high SQLE mRNA levels were associated with poor survival in patients with CRC (p<0.05) (figure 1C). Consistently, multivariate Cox proportional hazards regression analysis revealed that high SQLE mRNA expression was an independent prognostic factor associated with poor disease-specific survival in patients with CRC (p<0.05; HR 1.832; 95% CI 1.113 to 3.113) (figure 1C). We validated the prognostic significance of SQLE mRNA in GSE17538 cohort (n=232) (online supplemental table S3) using Kaplan-Meier curve (p<0.05) and univariate Cox proportional hazards regression analysis (p<0.05) (figure 1D).
To determine whether SQLE predicts patient prognosis at protein level, we performed TMA analysis of 207 CRC cases by IHC (figure 1E). Evaluation of clinical characteristics with respect to SQLE protein levels revealed significant associations with The American Joint Committee on Cancer stage (p<0.01), lymph node metastasis (p<0.01) and distant metastasis (p<0.001) (online supplemental table S2), implying that SQLE may be involved in tumour progression. Indeed, high SQLE protein expression was associated with poor survival in patients with CRC by Kaplan-Meier curve (p<0.001) analysis (figure 1E) and by multivariate Cox proportional hazards regression analysis (p<0.05; HR 1.951; 95% CI 1.225 to 2.391) (figure 1E). Our data collectively indicate that SQLE mRNA and protein expression are independent prognostic factors for predicting poor survival of patients with CRC.
SQLE promotes CRC cell growth
To determine the oncogenic effect of SQLE in human CRC, we overexpressed SQLE in CRC cells LOVO and SW1116 (figure 2A) with low endogenous SQLE levels (online supplemental figure S1). SQLE expression promoted cell growth, as evidenced by both cell growth curve (p<0.01) (figure 2A) and colony formation assay (p<0.01) (figure 2B). Conversely, we performed SQLE knockdown in CRC cells HT29 and DLD1 (online supplemental figure S1), with high endogenous SQLE expression (figure 2C). SQLE short hairpin (sh) RNA suppressed cell viability (p<0.01) (figure 2C) and colony formation (p<0.01) (figure 2D) compared with shControl cells. Next, tumourigenic effect of SQLE were investigated in nude mice model. LOVO and SW1116 cells stably expressing empty vector or SQLE were injected subcutaneously into left and right dorsal flanks of nude mice, respectively. As shown in figure 2E, SQLE overexpression markedly increased tumour volume of LOVO (p<0.01) and SW1116 (p<0.01) xenografts. SQLE depletion also suppressed proliferation of primary CRC-derived organoids (figure 2F). Together, SQLE promotes CRC cell growth in vitro and in vivo.
Supplemental material
SQLE suppresses apoptosis and promotes cell cycle progression in CRC cell lines
We next determined the cytokinetic effect of SQLE in CRC cell lines. Overexpression of SQLE in LOVO and SW1116 cells suppressed apoptosis, as determined by annexin V/7-aminoactinomycin D assay (figure 3A). Inhibition of apoptosis by SQLE was further evidenced by reduced protein expression of cleaved (active) forms of caspase-3, caspase-7 and poly ADP-ribose polymerase (PARP) in SQLE-expressing SW1116 and LOVO cells (figure 3B). Conversely, SQLE knockdown promoted the induction of apoptosis in HT29 and DLD1 cells (figure 3C), together with increased cleaved caspase-3, caspase-7 and PARP (figure 3D). We analysed cell cycle distribution by flow cytometry, and showed that SQLE overexpression LOVO and SW1116 cells increased S phase population, with a concomitant decrease in cells in G1 phase (figure 3E). Consistent with this observation, SQLE overexpression increased the protein expression of proliferating cell nuclear antigen (PCNA), cyclin D1 and CDK4, but suppressed expression of cell cycle inhibitors p21Cip1, p27 Kip1 and p53 (figure 3F). In contrast, SQLE knockdown in HT29 and DLD1 cells induced G1 cell cycle arrest (figure 3G), implying that SQLE accelerated G1-S progression. SQLE knockdown suppressed PCNA, cyclin D1 and CDK4, while promoting the expression of cell cycle inhibitors (figure 3H). Collectively, SQLE promotes CRC growth by inhibiting apoptosis and activating cell cycle progression.
Colon-specific transgenic SQLE expression in mice accelerates colorectal tumourigenesis
To determine the relevance of SQLE in colorectal tumourigenesis in vivo, we constructed colon-specific Sqle tg mice by crossing Rosa26-Sqle tg mice to Cdx2-CreERT2 mice (figure 4A). Colon-specific overexpression of Sqle was activated with tamoxifen injection, which allows the activation of Cre the in colon epithelium (figure 4B). To initiate colorectal tumourigenesis, we injected wild-type and Sqle tg mice with 10 mg/kg AOM once a week for a total of 6 weeks (figure 4B). At 180 days after the first AOM injection, mice were sacrificed and the colon was analysed. As shown in figure 4C, Sqle tg mice demonstrated increased tumour incidence (10/10 vs 6/10), tumour number (p<0.01) and tumour burden (p<0.01) as compared with wild-type mice, implying an oncogenic role of SQLE in CRC tumourigenesis. Histological examination by H&E staining confirmed CRC formation in the colon of Sqle tg mice, together with the increased proportion of mice with colon dysplasia and high-grade dysplasia (figure 4D). In concordance with these findings, the oncogenic function of SQLE in CRC was evidenced by increased cell proliferation evidenced by Ki-67 score (figure 4E) but decreased cell apoptosis by terminal deoxynucleotidyl transferase dUTP nick end labeling (TUNEL) score (figure 4F) in Sqle tg mice as compared with wild-type mice. To identify differentially expressed genes in Sqle tg mice, we performed Cancer Pathway PCR analysis of colon tissues from Sqle tg mice and their wild-type littermates. Cell cycle progression markers including Mki67, Ccnd2 and E2f4 are top upregulated genes, whereas pro-apoptotic genes Casp9 and Casp2 were downregulated, confirming the role of Sqle in promoting cell proliferation and suppressing apoptosis in CRC tumourigenesis (figure 4G).
SQLE knockout in mice suppressed colorectal tumourigenesis
Next, the effect of SQLE on CRC development was determined in CRISPR/Cas9-based whole body Sqle KO mice. We generated heterozygous Sqle mice (figure 4H), and performed the AOM-DSS chemical carcinogenesis model (figure 4I). As shown in figure 4I, Sqle KO mice showed decreased tumour number (p<0.05) in the colon as compared with wild-type littermates. Collectively, our findings in Sqle tg mice and Sqle KO mice both confirmed the oncogenic function of Sqle in colorectal tumourigenesis in vivo.
SQLE promotes de novo cholesterol biosynthesis
SQLE is the second rate-limiting enzyme for cholesterol biosynthesis. We hence evaluated its effect on cholesterol biosynthesis pathway. In LOVO and SW1116 cells, SQLE overexpression increased the mRNA expression of cholesterol biosynthesis genes (HMGCS1, HMGCR, MVK, PMVK, MVD, IDI1, FDPS and FDFT1) (online supplemental figure S2), whereas SQLE knockdown exerted an opposite effect (online supplemental figure S3). Western blot analysis demonstrated that SQLE overexpressing cells or Sqle tg mice have elevated HMGCR, FDFT1 and FDPS protein levels, while SQLE knockdown or Sqle+/− mice have downregulated protein levels of these genes (online supplemental figures S2 and S3). These data suggest that SQLE promotes de novo cholesterol biosynthesis pathway, which contributes to increased cell proliferation in CRC cells.
Sqle transgenic mice displayed gut dysbiosis
Besides CRC cell intrinsic effects of SQLE, we asked if SQLE have an impact on the colonic microenvironment. Gut microbiota dysbiosis is an emerging aetiological factor in colorectal tumourigenesis.19 We therefore asked if gut dysbiosis, at least in part, mediates the oncogenic effect of Sqle in vivo. Shotgun metagenome analysis was performed on stools collected from Sqle tg and wild-type mice at 3 months of age. Beta-diversity analysis did not show separate clusters for Sqle tg mice versus wild-type mice (figure 5A), while the alpha diversity index revealed a decreased trend in Sqle tg (p=0.093) (figure 5A). We determined alterations in the bacterial composition of Sqle tg and wild-type mice at the species level, and unravelled outlier bacterial species with significant differential abundance among the two groups (fold change >2; p<0.05) (figure 5B). Interestingly, we observed significant enrichment of pathogenic bacterial species such as Desulfovibrio fairfieldensis, Rhodococcus erythropolis, Brucella abortus and Chlamydia muridarum were enriched in Sqle tg mice, while protective bacteria were depleted, including Streptomyces violaceusniger and Pseudomonas sp Leaf58 (figure 5C). The changes in these key bacterial species were confirmed by qPCR (figure 5D). These results suggest that Sqle overexpression in vivo promotes gut dysbiosis.
Sqle transgenic mice showed altered gut metabolomics
Since some of the enriched pathogenic bacterial species are known to possess various metabolic activities, we next performed non-targeted metabolomic profiling on the same stool samples. Principal component analysis showed that the metabolome of the Sqle tg can be separated from that of wild-type mice (figure 5E). Focusing on differentially abundant metabolites (figure 5F,G), we found that secondary bile acids, such as lithocholic acid, chenodeoxycholic acid, taurodeoxycholic acid and deoxycholic acid were enriched in the stools from Sqle tg mice as compared with wild-type mice (figure 5G). Increased levels of secondary bile acids including lithocholic acid, isolithocholic acid, isoallolithocholic acid and deoxycholic acid in the Sqle tg mice were validated by targeted metabolomic analysis (figure 5H).
As secondary bile acids are bio-transformed from primary bile acids via the action of gut microbiome,20 we investigated the correlation between gut bacterial species and metabolites showing differential abundances in Sqle tg mice (figure 6A). We observed the significant correlations between secondary bile acids and C. muridarum, implying its potential involvement in contributing to increased secondary bile acids. Moreover, all four pathogenic bacteria showed positive association with key altered metabolites (figure 6A). Sqle transgene expression thus modulates the gut microbiome and metabolites in CRC development in mice.
SQLE transgenic overexpression impairs the intestinal barrier function and promotes inflammation
Secondary bile acids are known lipotoxins, whose increased levels is an important risk factor for CRC.21 They are toxic to colonic epithelial cells and are known to disrupt the gut barrier function.22 Gut microbial dysbiosis is also closely associated with the disruption of the gut barrier.23 We therefore compared the barrier function of Sqle tg mice and wild-type littermates by FITC-dextran transepithelial permeability assay. After oral gavage of FITC-dextran, higher serum FITC-dextran was detected in Sqle tg mice as compared with wild-type mice (figure 6B). Electron microscopy (EM) confirmed the disruption of tight junctions in Sqle tg mice (figure 6C). Epithelial tight junctions are maintained by intercellular junctional protein complexes. We determined expression of key tight junction proteins by western blot analysis, and revealed that Jam-c and occludin were downregulated in the Sqle tg mice colon as compared with that of wild-type mice (figure 6D). Moreover, Muc2, a key component of inner mucus, was downregulated at mRNA level in Sqle tg mice (figure 6E). A major consequence of a ‘leaky’ gut is the induction of a pro-inflammatory response. In line with this notion, inflammatory pathway PCR array analysis of Sqle tg colon tissues showed the significant upregulation of pro-inflammatory factors such as Cxcl3, Crp and Cxcr2 (online supplemental figure S4). These findings indicate the gut dysbiosis-metabolite axis might contribute to gut barrier dysfunction in Sqle tg mice.
SQLE overexpression-induced gut microbiota dysbiosis promotes gut barrier dysfunction and colonic epithelium proliferation in germ-free mice
To address whether Sqle tg expression-induced gut dysbiosis has a direct effect on colon cell proliferation, stools collected from Sqle tg mice and wild-type mice from the AOM model was transplanted to germ-free (GF) mice. One month later, mice were sacrificed. The oral gavage of different stools had no impact on body weight. Prior to sacrifice, we performed FITC-dextran transepithelial permeability assay, showing that FITC-dextran in the serum of GF mice gavaged with stool of Sqle tg mice was significantly higher than those gavaged with stool of wild-type mice (figure 6F) and disruption of gut barrier was confirmed by EM (figure 6G). Consistently, junction adhesion protein Jam-c and occludin were downregulated in GF mice gavaged with Sqle tg stool compared with wild-type stool (figure 6H). Moreover, Ki-67 staining demonstrated that Sqle tg mice stool significantly promoted proliferation of colonic epithelial cells of GF mice compared with wild-type mice stool (figure 6I). These data underscore a functional role of SQLE-induced gut microbiota dysbiosis in impairing gut barrier function and promoting colonic cell growth.
Pharmacological inhibition of Sqle improves therapeutic efficacy of chemotherapy in CRC treatment
Given that SQLE possesses oncogenic function in CRC, we next investigated if SQLE can be therapeutically targeted in CRC cells. To test whether SQLE represents a viable therapeutic target for CRC, we treated HT29 and DLD1 cells with terbinafine, an FDA-approved fungal SQLE inhibitor. As shown in figure 7A, terbinafine dose-dependently suppressed the growth of HT29 and DLD1 cells in vitro. Apart from CRC cell lines, terbinafine significantly impaired the growth of primary CRC organoids (figure 7A). We next assessed the effect of terbinafine in combination with oxaliplatin or 5-FU, the common chemotherapeutic drugs used for the treatment of patients with CRC. We performed cell viability assay in the presence or absence of terbinafine, which showed that terbinafine sensitised HT29 and DLD1 cells to the growth inhibitory effects of both oxaliplatin and 5-FU (figure 7B). Quantitative assessment using combination index (CI) demonstrated that combination of terbinafine with oxaliplatin (CI: 0.39–0.63) or 5-FU (CI: 0.332–0.472) was synergistic (<1) (figure 7C). In addition, apoptosis assay showed that the combination of terbinafine with oxaliplatin and 5-FU synergistically induced apoptosis in vitro (figure 7D). Terbinafine also potentiated 5-FU-induced cell cycle arrest (online supplemental figure S5).
To confirm the synergistic effect of terbinafine plus 5-FU or oxaliplatin in suppressing CRC growth, we performed subcutaneous xenograft model in nude mice. HT29 cells (1×106) were implanted into the dorsal flanks of nude mice, and divided into six groups: (1) vehicle; (2) terbinafine; (3) 5-FU; (4) oxaliplatin; (5) terbinafine+5-FU and (6) terbinafine+oxaliplatin. As shown in figure 7E, single drug treatments inhibited tumour growth by approximately 50% (p<0.01). Importantly, either the combination of terbinafine+5-FU or terbinafine+oxaliplatin triggered complete growth arrest (p<0.001) as compared with vehicle and was significantly more effective than single drug treatments (p<0.01). Our data indicate that SQLE is an actionable target in CRC and that SQLE inhibition could improve the therapeutic efficacy of chemotherapy in CRC.
Discussion
In this study, we established SQLE as an oncogenic factor in CRC using cell lines, colon-specific Sqle tg mice and Sqle KO mice models. We revealed that SQLE mediates tumourigenesis via both cell intrinsic effects and the modulation of gut microbiota-metabolite axis, which respectively drives tumour cell proliferation and intestinal barrier dysfunction. We further demonstrated that SQLE inhibitor, terbinafine, could be re-purposed for the treatment of CRC by exerting synergistic effects in combination with chemotherapy. Corroborating our preclinical findings, SQLE is overexpressed in CRC and its expression predicts poor patient survival, implying SQLE as a therapeutic target and prognosification factor in CRC.
Our work clearly demonstrated that SQLE functions as a tumour cell-intrinsic oncogenic factor in CRC. Ectopic expression of SQLE in CRC cells promoted cell proliferation by accelerating cell cycle progression and suppressed cell apoptosis, whereas KO of SQLE exerted opposite effects. To validate the effect of SQLE in vivo, we established colon-specific Sqle tg mice and Sqle+/− mice to comprehensively evaluate the effect of Sqle gain-of-function and loss-of-function in colorectal carcinogenesis. Consistent with our notion that SQLE is an oncogene, colon-specific Sqle overexpression exacerbated AOM-induced CRC, both in terms of tumour incidence and disease severity, and tumours from Sqle tg mice exhibited significantly higher cell proliferation indices. In contrast, Sqle KO impaired AOM-DSS-induced CRC. The pro-tumourigenic effect of SQLE could be partly attributed to induction of cholesterol biosynthesis, which is critical for supporting increased cell proliferation. All these findings collectively show that SQLE functions as an oncogene in CRC tumourigenesis.
Accumulating evidence suggests that colorectal tumourigenesis involved a complex interaction of tumour cells and its microenvironment.24 In particular, the gut microbiota is increasingly recognised as causative agents for CRC. Previously, we have shown that GF mice orally gavaged with stools from patients with CRC had significantly induced colonic cell proliferation and tumourigenesis.19 However, it is unclear if the interplay between genetic alterations and gut dysbiosis plays a role in colorectal tumourigenesis. Here, we demonstrated that Sqle transgene expression in mice induces gut dysbiosis, characterised by the enrichment of several pathogenic bacteria including D. fairfieldensis, R. erythropolis, B. abortus and C. muridarum, that are associated with various pathologies25–27; while potential protective bacteria with anti-inflammatory and antitumour properties, S. violaceusniger and Pseudomonas sp Leaf58, were depleted.28–30 Transplantation of Sqle tg stool to GF mice significantly promoted the proliferation of the colonic epithelial cells as compared with wild-type mice, implying that Sqle-induced gut dysbiosis plays a casual role in CRC. These data imply that Sqle impacts the gut microbiome beyond its direct effect on tumour cell proliferation and survival.
Studies have shown that metabolites and microbiota can affect each other reciprocally in gut.31 Metabolomic profiling marked the induction of secondary bile acids in the stool of Sqle tg mice. Since secondary bile acids are products of microbial metabolism, we integratively analysed metagenome and metabolome datasets. Indeed, we identified that secondary bile acids positively correlated with C. muridarum, an outlier pathogenic bacteria in Sqle tg mice. Secondary bile acids are important lipotoxins that are known to induce DNA damage in colonic epithelium32 and promote colon cancer formation in mice.33 Consistent with this, we found that gut barrier function was impaired in Sqle tg mice, as shown by increased intestinal permeability, EM analysis and downregulation of tight junction proteins. Accompanying the compromised gut barrier integrity is an inflammatory response in Sqle tg mice, which further exacerbated colorectal tumourigenesis. These results indicate the gut dysbiosis-metabolite-gut barrier axis might contribute, at least in part, to the tumour promoting effect of SQLE in vivo.
Given the important role of SQLE in CRC development, we next evaluated its potential as a therapeutic target. We thus tested terbinafine, an FDA-approved drug for antifungal infection, as a novel treatment for CRC. In line with the oncogenic function of SQLE, its blockade by terbinafine exerted growth inhibitory effects on CRC cells. In particular, terbinafine in combination with 5-FU or oxaliplatin, chemotherapy commonly used in CRC, synergistically suppressed CRC growth in vitro and in vivo. Our results suggest that the re-purposing of terbinafine might be a strategy for the treatment of CRC in combination with chemotherapy.
Corroborating our experimental results, analysis of independent human CRC cohorts revealed that SQLE is overexpressed in CRC and its expression predicts poor survival in patients with CRC. In agreement with our data, Kim et al and He et al both reported that SQLE protein expression predicts poor survival of patients with CRC.10 11 On the contrary, Jun et al demonstrated that high SQLE predicts favourable outcomes specifically in patients with stage IV CRC, and that depletion of SQLE promotes metastasis phenotypes in CRC cells. SQLE may thus have disparate effects on CRC growth and metastasis. Studies on the role of SQLE in CRC metastasis using Sqle transgenic or KO mice are warranted in the future.
In conclusion, our work establishes an oncogenic role of SQLE in CRC. SQLE promotes CRC cell proliferation and survival, and exerts an influence on the tumour microenvironment by causing gut microbiota and gut barrier dysfunction. Targeting of SQLE by terbinafine significantly improved the efficacy of conventional chemotherapy, indicating its potential clinical application in CRC treatment in the future.
Data availability statement
Data are available on reasonable request. All data are available from the corresponding author on request.
Ethics statements
Patient consent for publication
Ethics approval
This study involves human participants and was approved by Human Ethics Committee of Beijing University Cancer Hospital and the Chinese University of Hong Kong (ID: CREC Ref. 2019.425). Participants gave informed consent to participate in the study before taking part. All animal studies were performed in accordance with guidelines approved by the Animal Experimentation Ethics Committee of the Chinese University of Hong Kong (AMUWEC-20192185).
References
Supplementary materials
Supplementary Data
This web only file has been produced by the BMJ Publishing Group from an electronic file supplied by the author(s) and has not been edited for content.
Supplementary Data
This web only file has been produced by the BMJ Publishing Group from an electronic file supplied by the author(s) and has not been edited for content.
Footnotes
CL and YW are joint first authors.
Correction notice This article has been corrected since it published Online First. Online supplemental file 1 has been replaced. Human SQLE qPCR primers in Table S4 are corrected as follow: Human SQLE qPCR Forward: 5’-GATGATGCAGCTATTTTCGAGGC-3’; Reverse: 5’-CCTGAGCAAGGATATTCACGACA-3.
Contributors Chuangen Li (CL) performed the experiments, analysed the data and drafted the manuscript; YW provided the facilities for the animal work; DL and YZ provided the transgenic mouse model and commented on the study; CCW commented on the study and revised manuscript; OOC and Changan Liu (CL) performed bioinformatics analyses; YL performed the organoid experiments; XZ and JJYS commented on the study; WK and KFT assisted for tissue microarray; JY designed, supervised the project and revised the manuscript. JY is the guarantor for this paper.
Funding This project was supported by National Key R&D Programme of China (No. 2020YFA0509200/2020YFA0509203), National Natural Science Foundation of China (NSFC; 81972576), RGC-CRF Hong Kong (C4039-19GF and C7065-18GF), RGC-GRF Hong Kong (14110819, 24100520 and 14108718), Health and Medical Research Fund (06170686 and 07181256) and Vice-Chancellor’s Discretionary Fund CUHK.
Competing interests None declared.
Provenance and peer review Not commissioned; externally peer reviewed.
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