The prognostic role of the Transducin-like Enhancer of split protein family in lung adenocarcinoma
Introduction
Lung cancer takes more lives each year than any other cancer worldwide. In 2018 alone, there were 2.1 million new lung cancer cases (1). Lung adenocarcinoma (LUAD) is the most common type of lung cancer (2). The outcomes of patients with LUAD are capricious and unpredictable (3,4). Therefore, reliable and predictive biomarkers are needed for the identification and stratification of patients.
Members of the Transducin-like Enhancer of split (TLE) family of proteins are involved in many developmental processes, including lateral inhibition, segmentation, sex determination, eye development, and pancreatic development (5). TLE family proteins repress the transcription process through multiple mechanisms (6). Instead of binding to DNA directly, TLE proteins are recruited to the template by DNA-bound repressor proteins (7,8). Seven TLE homologs have been found in humans, namely TLE 1–7. Four TLE proteins (TLE 1–4) are full length, while another two homologous proteins, TLE5 and TLE6, are expressed in truncated forms (9,10). All TLE proteins interact with Tcf1 and Lef1. They are also enriched in the Wnt signaling pathway, suggesting their involvement in T-cell development and function (11-13). TLE corepressors predominantly partner with Tcf1/Lef1 to form CD8+ T-cell identity and are physiologically required for T-cell development (14).
TLE1 and TLE4 have been found to function as tumor suppressors in myeloid leukemia (15). Overexpression of TLE1 was also detected in a subset of aggressive and advanced lung cancers, and might regulate lung cancer aggressiveness (16). Yao et al. reported that TLE1 promoted epithelial-mesenchymal transition in A549 lung cancer cells by suppressing E-cadherin. In human lung cancer cells, TLE1 promotes tumorigenicity and inhibits anoikis through ZEB1-mediated E-cadherin repression (17,18). Furthermore, TLE4 interacts with PU.1 and Pax5 transcription factor in blood lineage cells, indicating that it plays a role in B-cell function (19).
Lee JH reported that immunohistochemical expression of TLE1 in invasive breast cancer and its association with clinicopathological parameters, prognosis, and intrinsic subtype (20). Hu S provides new insights and evidence that TLE2 functions as a tumor suppressor gene and prognostic marker in pancreatic ductal adenocarcinoma (21). However, these two paper focus on only one member’ function. The novel idea in this paper is to analysis the whole TLE family members, and then select two family members (TLE1 and TLE2) according to the statistic significance. Furthermore, we combined these two members as one group. So, the combined biomarkers could be more precise and effective. More research is needed to ascertain the prognostic value of TLEs in LUAD. Therefore, we conducted a study of the correlation between TLE protein expression and survival outcomes in LUAD. We present the following article in accordance with the REMARK reporting checklist (available at https://dx.doi.org/10.21037/tlcr-21-582).
Methods
Patients
Gene expression data of LUAD tissues from The Cancer Genome Atlas (TCGA) were obtained via the Genomic Data Commons (GDC, available at: http://potal.gdc.cancer.gov/) data portal on November 6, 2019. The expression of TLE family members in 59 normal and 513 tumor samples in the TCGA dataset was quantified as fragments per kilobase of exon, per million reads mapped (FPKM). For paired analysis, 57 normal and 57 tumor paired tissues were selected. In accordance with the database policy, access to the de-identified linked dataset was obtained from TCGA.
Clinicopathological data for the patients in the TCGA dataset, including age, sex, pathologic stage, molecular data, and survival information, were also retrieved. Only patients with survival information and expression data available at that time point were included in the study. The study was conducted in accordance with the Declaration of Helsinki (as revised in 2013).
Gene Ontology (GO) term and Reactome pathway enrichment analyses of the TLE family members were performed. GO terms include biological processes (BPs), cellular components (CCs), and molecular functions (MFs). An adjusted P value <0.05 was considered to be statistically significant in both GO and Reactome pathway analysis.
Statistical analysis
Progression-free survival (PFS) and overall survival (OS) served as endpoints in this study. PFS refers to the length of time for which a patient lives with the disease without progression. OS is defined as the time from diagnosis to death from any cause or the last follow-up visit.
The Wilcoxon rank-sum test was employed for numerical data comparisons. Categorical data were compared using Fisher’s exact test. For survival analysis, the Kaplan-Meier method and log-rank test were applied. For the analysis of PFS and OS, univariate and multivariate Cox proportional hazard models were constructed, and 95% confidence intervals (95% CIs) were calculated. All statistical analyses were performed with R 3.6.0.
Results
The expression of TLEs in normal and LUAD tissue samples
In this study, we examined the expression levels of TLEs in LUAD tissue samples in a TCGA dataset. We observed remarkable differences in the expression levels of TLEs in tumor samples compared with normal tissues (Figure 1). The same trends were also validated in the paired samples (Figure S1). The results suggested that the expression levels of TLEs might be related to LUAD progression.
The prognostic value of TLE expression levels in LUAD
The patients in the TCGA dataset were divided into two groups according to the median expression level of each TLE family member. Table 1 shows the differences between the high and low expression groups. A high expression of TLE1 (Figure 2A) and a low expression of TLE2 were found to have an adverse affect on both PFS and OS (Figure 2B) (PFS: P<0.001, P=0.003; OS: P<0.0001, P=0.004, respectively).
Full table
The expression of TLE family members in LUAD
The correlations between the expression levels of TLE members in LUAD were analyzed. As shown in Figure 3, the expression levels of the TLE family members were interrelated (all |RPearson| >0.1, Figure 3A), especially those of TLE3/TLE1, TLE4/TLE1, TLE6/TLE1, TLE3/TLE2, TLE5/TLE2, TLE6/TLE2, TLE6/TLE4, and TLE6/TLE5 (all |RPearson| >0.1, Figure 3B,C,D,E,F,G,H,I). These results suggest that the TLEs might be transcriptionally co-regulated together. Previous research has shown that TLE1, TLE2, and TLE5 work as a complex to regulate DNA transcription. A protein-protein interaction (PPI) network was constructed for the TLE family members and revealed interactions between TLE 1–6 (Figure 3J).
Clinical and molecular characteristics
The clinical and molecular characteristics of 513 LUAD patients in TCGA are shown in Table 2. Compared to those in the TLE1low group, patients in the TLE1high group were more likely to have received radiation therapy (P=0.021). Furthermore, high TLE1 expression showed a trend toward pathologic T1 stage (P=0.060). The TLE1high group also had a lower proportion of patients with RET (rearranged during transfection) mutation (48.25% vs. 51.95%, P=0.029).
Full table
Compared to the TLE2low group, high TLE2 expression was correlated with stage (P=0.011) and pathologic T stage (P=0.001). Moreover, high TLE2 expression showed a trend toward more pharmaceutical therapy (P=0.057). In the TLE2high group, lower proportions of patients had PIK3CA mutation (46.3% vs. 53.91%, P<0.001) and KRAS mutation (46.69% vs. 53.52%, P=0.011), but a higher proportion of patients had BRAF mutation (54.86% vs. 45.31%, P<0.001), compared with the TLE2low group.
Univariate and multivariate analysis of PFS and OS
To further assess the prognostic significance of TLE1/2, the expression levels of TLE 1–7 (high vs. low), age (≥60 vs. <60 years), sex, and common genetic mutations (ALK, BRAF, EGFR, ERBB2, KRAS, NRAS, PIK3CA, RET, and ROS1) were enrolled in univariate and multivariate analysis (Table 3). The univariate analysis identified three independent risk factors for PFS. They were high expression levels of TLE1, TLE2, and TLE5 (P<0.001, P=0.004, and P=0.035). While, the univariate analysis identified five independent risk factors for OS. They were high expression levels of TLE1, TLE2, and TLE5, ALK mutation, and NRAS mutation (P<0.0001, P=0.003, P=0.024, P=0.036, and P=0.045). The multivariate analysis identified high TLE1 and TLE2 expression as independent risk factors for both PFS and OS (PFS: P<0.001, P=0.020; OS: P<0.0001, P=0.047, respectively).
Full table
The combined prognostic effect of TLE1 and TLE2 in LUAD
The effects of TLE1 and TLE2 on PFS and OS were subsequently examined. The results showed that the subgroup with both TLE1high and TLE2low had significantly shorter PFS and OS than the other subgroups (TLE1low/TLE2low, TLE1low/TLE2high, TLE1high/TLE2high) (P<0.0001 and P<0.0001, respectively, Figure 4).
GO and Reactome pathway enrichment analysis of the TLE family members
Reactome pathway enrichment analysis of the TLE family members showed that they are related to the repression of WNT target genes, TCF-dependent signaling in response to WNT, and deactivation of the beta-catenin transactivating complex (Figure 5). GO term enrichment analysis revealed that the TLE family members were related to repressing transcription factor binding, beta-catenin-TCF-complex, transcription factor complex, negative regulation of canonical WNT signaling pathway, and cell-cell signaling by WNT (Figure 5). A model illustrating the relationship between the TLE family members and Wnt pathway is shown in Figure S2.
Discussion
This study found an increasing trend in TLE1 expression and a decreasing trend in TLE2 expression in LUAD. Furthermore, a high TLE1 level and a low TLE2 level were poor prognostic factors in patients with LUAD. Co-expression analysis confirmed that TLE1 and TLE2 were strongly correlated in LUAD. Based on multivariate analysis, TLE1 and TLE2 were also found to be independent risk factors for PFS and OS. Compared with the use of a single marker, the combined application of biomarkers seems to have higher value in the assessment of tumor prognosis.
The relationships between TLE family members and cancers have been studied recently. TLE1 has been shown to bind to Runx1, which is essential for the maintenance and generation of hematopoietic stem/progenitor cells (HSPCs) (22,23). TLE1 is related to chromatin through its interactions with the amino-terminal tail of histone H3 (24). The silencing function of the TLE1 gene is dependent on recruitment of the histone deacetylase (HDAC) protein. In a study by Chen et al., acetyl groups were removed from nearby DNA bound histones (25). TLE1 is highly expressed in diseased metaplastic and neoplastic transformed states as well as in proliferative epithelial tissues (26). TLE1 is also involved in the pathogenesis of cancers. For instance, it is abnormally expressed in various human cancers including synovial sarcoma (27), breast cancer (28), and lung cancer (16).
There were function differences of TLE proteins in different types of tumors. Seo et al. found that inhibition of TLE1 altered cancer cell proliferation and apoptosis through suppression of Bcl-2 expression (27). TLE1 is selectively over-expressed in invasive breast tumors compared to non-invasive ductal carcinoma in situ and normal mammary epithelial tissue (28). Allen et al. found that transgenic mice carrying the human TLE1 homolog developed LUAD. TLE1 was found to be overexpressed in approximately 11% of patients with lung squamous cell carcinomas and 20% of patients with LUADs. It is a putative lung-specific oncogene that positively regulates Bcl2 expression and ErbB1/ErbB2 signaling to promote cancer progression (16). Yao et al. found that the ZEB1/TLE1/E-cadherin transcriptional mechanism was a pathway that promoted the oncogenicity of lung cancer cells (18). TLE1 was also found to be an effector of epithelial-mesenchymal transition via transcriptional silencing of the epithelial marker E-cadherin in lung cancer cells (17). The TLE1 gene functions as a tumor suppressor in myeloid leukemia. Epigenetic inactivation of the TLE1 gene was shown to promote myeloid cell proliferation and survival (15). Elevated expression of TLE1 is frequently observed in glioblastoma, and is associated with poor OS (29). TLE1 expression is a good prognostic indicator in gastric cancer and that it exerts oncogenic effects (30). TLE1 may act as a tumor suppressor in hepatocellular carcinoma (31).
TLE1, which is a negative regulator of apoptosis, has been observed to inhibit low potassium-induced neuronal apoptosis (32), and to exhibit anti-neurogenic activity in mammalian forebrain development. Furthermore, Yao et al. reported that upregulation of TLE1 in transgenic mice inhibited neuronal development in vivo (33). In their study, Nuthall et al. observed that ectopic TLE1 expression in neural progenitor cells promoted their un-differentiation status with concomitant increased proliferation ability (34). In conjunction with Forkhead box protein G1 (FoxG1), TLE1 promoted survival in post-mitotic neurons in Zhang et al.’s study (32). It has also been observed to inhibit caspase-independent cell death induced by Bit1 (Bcl2-inhibitor of transcription 1) (35), and to positively regulate Bcl2 expression and ErbB1 and ErbB2 signaling (16). Furthermore, downregulation of TLE1 can result in excess inflammatory cytokine production (36). Also, Sonderegger et al. observed that exogenous TLE1 expression stimulated anchorage-independent growth in chicken embryo fibroblasts (37). These findings show that TLE1 play an important role in the BP.
TLE2 can form a complex with the replication and transcription activator (RTA) to access the cognate DNA sequence of the RTA-responsive element at different promoters and subsequently inhibit replication and transactivation (38). TLE2 and β-catenin are physically associated with NDRG1 to affect the Wnt pathway in esophageal cancer cells (39). TLE2 is also associated with the survival and progression of bladder cancer. A low expression of TLE2 was associated with shorter OS and PFS, whereas a high expression of TLE2 was associated with favorable OS. This was consistent with Wu et al.’s analysis of a cohort from the TCGA (40). In our study, the results showed that the subgroup with both TLE1high and TLE2low had significantly shorter PFS and OS than the other subgroups. High TLE1 expression and low TLE2 are independent adverse prognostic factors in LUAD and can serve as prognostic biomarkers.
Regarding TLE3, Qian et al. found that it was highly expressed in slow-proliferating and -migrating breast cancer cell lines like MCF-7; however, it was downregulated in more malignant stromal cells like ZR-75-30. These results revealed TLE3 as the possible key factor in breast cancer cell proliferation and migration (41).
The transcriptional pathways of the TLE family include Wnt, Notch, Pax2, and Runx2 (19). Cell fate determination during embryogenesis in adults is mediated by Wnt growth factors. Co-repressors of TLEs are known to contribute to the repression of Wnt targets in the absence of signaling; however, inactivation or displacement of TLE by Wnt signaling is still poorly understood. Ramakrishnan et al. reviewed the prevalence and molecular mechanisms of the Wnt transcription switch, and found that the regulation of gene expression by the Wnt pathway is complex (42). Fu et al. revealed that loss of Lats1/2 mobilized a previously unrecognized TLE/YAP/TAZ-Groucho interaction to suppress Wnt/TCF-mediated transcription, which led to Wnt-uncoupled progenitor expansion and intestinal stem cell depletion (43). Wnt acts by stabilizing cellular levels of the transcriptional coactivator beta-catenin, which forms complexes with sequence-specific DNA-binding Tcf/Lef transcription factors. Tcf/Lefs acts as transcriptional repressors by binding to Groucho/TLE proteins in the absence of nuclear β-catenin. Hanson et al. revealed a mechanism by which XIAP-mediated removal of Gro/TLE from TCF/Lef allows assembly of β-catenin-TCF/Lef complexes that initiate a Wnt-specific transcriptional program (44). Daniels et al. confirmed that β-catenin displaced Groucho/TLE from Tcf/Lef by binding to a previously unidentified second, low-affinity binding site on Lef-1 that includes sequences just N-terminal to the DNA-binding domain, and that overlaps the Groucho/TLE-binding site (45). Wu et al. found that the removal of O-GlcNAc was important for gene activation via Wnt-responsive promoters and demonstrated how Groucho/TLEs repress gene transcription (46).
In conclusion, we found that the expression levels of TLEs shows a significantly different trend with the progression of LUAD. A high expression TLE1 and a low expression of TLE2 were associated with a poor prognosis. Furthermore, TLE1 and TLE2 were found to be independent prognostic factors for patients with LUAD, and might also be potential therapeutic targets. Moreover, the combined use of TLE1 and TLE2 was better than the use of a single biomarker. However, further studies of the molecular mechanism of TLEs in LUAD are needed.
Acknowledgments
Thank you Yue Wang and Jianyan Wen for providing professional writing services and materials.
Funding: This study is supported by the funding from the research and demonstration application of clinical diagnosis and treatment technology in Beijing capital city (Z191100006619008).
Footnote
Reporting Checklist: The authors have completed the REMARK reporting checklist. Available at https://dx.doi.org/10.21037/tlcr-21-582
Conflicts of Interest: All authors have completed the ICMJE uniform disclosure form (available at https://dx.doi.org/10.21037/tlcr-21-582). The authors have no conflicts of interest to declare.
Ethical Statement: The authors are accountable for all aspects of the work in ensuring that questions related to the accuracy or integrity of any part of the work are appropriately investigated and resolved. The study was conducted in accordance with the Declaration of Helsinki (as revised in 2013).
Open Access Statement: This is an Open Access article distributed in accordance with the Creative Commons Attribution-NonCommercial-NoDerivs 4.0 International License (CC BY-NC-ND 4.0), which permits the non-commercial replication and distribution of the article with the strict proviso that no changes or edits are made and the original work is properly cited (including links to both the formal publication through the relevant DOI and the license). See: https://creativecommons.org/licenses/by-nc-nd/4.0/.
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