miR-520b Promotes Breast Cancer Stemness Through Hippo/YAP Signaling Pathway.

INTRODUCTION: The breast cancer stem cells contribute to the initiation, progression, recurrence, metastasis as well as resistance of breast cancer. However, the mechanisms underlying the maintenance of breast cancer stemness have not been fully understood.
MATERIALS AND METHODS: TCGA and GEO data were used for measuring miR-520b expression in breast cancer tissues. Kaplan-meier analysis was used for determining the relationship between miR-520b expression level and the prognosis of patients. Genetic manipulation was performed by lentivirus system and miR-520b inhibitor was used for knockdown of miR-520b. qRT-PCR and Western blot were employed to determine the mRNA and protein levels, respectively. The stemness and EMT (Epithelial to mesenchymal transition) were assessed by sphere-formation and transwell assay as well as the expression of the related markers. The target genes of miR-520b were identified using the online database starBase V3.0.
RESULTS: miR-520b is upregulated in cancer tissues of breast cancer patients and predicts poor prognosis. Upregulation of miR-520b was found in breast cancer stem cells. Ectopic expression of miR-520b promotes the stemness of the breast cancer cells, conversely, depletion of miR-520b attenuates the stemness of these cells. miR-520b positively regulates Hippo/YAP signaling pathway and overexpression of LAST2 abolished the effect of miR-520b on the stemness of breast cancer cells.
CONCLUSION: miR-520b promotes the stemness of breast cancer patients by activating Hippo/YAP signaling via targeting LATS2.

Introduction

Breast cancer is recognized as one of the leading causes of cancer-related mortality in women worldwide.1 In spite of the development of aggressive interventions, the inevitability of relapse and metastasis result in severe mortality rate.2 While, the roots of breast cancer relapse and metastasis have remained elusive.

Cancer stem cells (CSCs) are a small but significant subpopulation of undifferentiated cells in tumor tissues.3–5 Accumulating evidences indicated that CSCs drive cancer initiation, progression, spread and resistance to chemo- or radiotherapy.6,7 CSCs were also identified in breast cancer tissues, called breast cancer stem cells (BCSCs). BCSCs were characterized with the ability of self-renewal, differentiation, tumor initiation, invasion and resistance of conventional therapy, which indicated that BCSCs should be an effective target for breast cancer therapy.8–12 However, our understanding of BCSCs still needs to be improved.

There are several signaling pathways that have been identified to be associated with the maintenance of breast cancer stemness, including Hippo/YAP, Notch, Hedgehog and Wnt pathways.13–18 In addition, numerous miRNAs are identified to be dysregulated in BCSCs population, such as miR-200c19, miR-205,20 miR-141,21 miR-1,22 miR-34a23, miR-221,24 miR-2125 and Let-7.26

miR-520b is a member of miR-302/372/373/520 family. Recently, several members in this family have been reported to be associated with cancers. For example, miR-373 and miR-520c/h have been reported with the role of oncogene in breast and esophageal cancer cells.27–29 While, miR-302, 372, 520a/b/e/h have been shown as a tumor suppressor in some types of cancers,30–34 which indicated that the function of the members of this family largely depends on the cellular context in specific tissue type.

In this study, we report that miR-520b promotes the stemness of breast cancer patients by activating Hippo/YAP signaling via targeting LATS2.

Materials and Methods

Cells, Clinical Samples and Cell Culture

MCF-7 and MDA-MB-231 breast cancer cells were purchased from Chinese Academy of Sciences (Shanghai, China). Both cells were cultured in Eagle’s Minimum Essential Medium (EMEM, Thermo Fisher, Waltham, MA, USA) supplemented with 10% fetal bovine serum (FBS, Thermo Fisher, Waltham, MA, USA). All tissues were obtained from Chongqing University Cancer Hospital, which was approved by ethics committee of Chongqing University Cancer Hospital. All patients provided written informed consent, and that this was conducted in accordance with the Declaration of Helsinki. The clinical information of the patients was provided in .

Stem Cell Isolation

The cells were digested, washed and re-seeded in stem cell medium (Thermo Fisher Scientific) in Ultra-low adherent plate (Corning) and cultured at 37°C in a 5% CO2 humidified incubator for 15–20 days.

Antibodies, Primers and Reagents

The detail information of antibodies and primers were provided in . miR-520b inhibitors were purchased Sigma-Aldrich (St. Louis, MO, USA). All other reagents were purchased from Sigma-Aldrich (St. Louis, MO, USA).

Plasmids

Lentivirus containing miR-520b (HLMIR0696) and miR-520b inhibitor (HSTUD0696) were purchased from Sigma Aldrich Merck (St. Louis, MO, USA). The coding sequence (CDs) region of LATS2 CDS was synthesized by PCR and was cloned into pCDH plasmids for virus package.

Lentivirus Package, Transfection and Stable Cell Selection

HEK293T cells were co-transfected with reconstructed plasmids, VSV-G (envelop plasmid) and delta R8.2 (packaging plasmid) and were cultured for 7–14 days. The media were harvested for virus concentration using a 0.45 μm filter and Lenti-X Concentrator (Clontech, Mountain View, CA, USA). MCF-7 and MDA-MB-231 cells were infected with lentivirus, and two days after infection, the cells were cultured with complete media with puromycin. The stable cell lines were verified by Western blot assay.

Quantitative Real-Time Reverse-Transcription PCR

RNAzol RT reagent (Molecular Research Center, Cincinnati, OH, USA) was employed for Total RNA isolation. SuperScript III Platinum SYBR Green One-Step qRT-PCR Kit (Thermo Fisher, Waltham, MA, USA) was used for quantitative reverse transcriptase PCR (qRT-PCR) and GAPDH was used as an internal control.

Western Blot

The protein samples were fist separated by sodium dodecyl sulfate-polyacrylamide gel electrophoresis (SDS-PAGE) and blotted onto Immobilon-P membranes (Millipore-Sigma, St. Louis, MO, USA). The membranes were then incubated with the primary antibody at 4°C overnight. After incubation with relevant horseradish peroxidase (HRP)-conjugated secondary antibody, the Clarity™ Western ECL Substrate (BioRad, Hercules, CA, USA) was used to produce the signals.

Transwell Assay

About 2×103 cells in serum-free culture media were placed on the upper layer of the culture insert with permeable membrane (Thermo Fisher, Waltham, MA, USA). The complete culture medium was then added in the culture well (Thermo Fisher, Waltham, MA, USA). Following an incubation for 18 hrs, the cells that have migrated through the membrane are stained and counted.

Statistics

At least three replicates were performed for each experiment. Data are represented as mean ± s.d. and the significance was determined by Student’s t-test.

Results

miR-520b Is Upregulated in Breast Cancer Tissues, Predicts Poor Prognosis and Associates Breast Cancer Stem Cells

To investigate the role of miR-520b in breast cancer, we first analyzed the expression of miR-520b in breast cancer tissues. GSE57897 dataset was downloaded from GEO (Gene expression omnibus) database and we found that the expression of miR-520b was significantly upregulated in breast cancer tissues, compared with adjacent normal tissues (Figure 1A). In addition, the result from Kaplan–Meier analysis using TCGA (The cancer genome atlas) data downloaded from the Kaplan–Meier Plotter database showed that high expression of miR-520b is associated with poor prognosis of breast cancer patients (Figure 1B).

Figure 1

miR-520b is associated with breast cancer stemness. (A) miR-520b is upregulated in breast cancer tissues as indicated by bioinformatic analysis. (B) TCGA data showed that Aberrant upregulation of miR-520b is associated with poor prognosis of breast cancer patients. (C, D) miR-520b is upregulated in spheres (C) and cells expressed high level of cancer stem cell markers (D). The expression of miR-520b in indicated cells was analyzed by qRT-PCR. (E) The expression of miR-520b positively correlates to cancer stem cell markers. Student’s t-test (***P<0.001).

Next, we isolated BCSCs from MCF-7 and MDA-MB-231 breast cancer cells by suspension culture and analyzed the expression of miR-520b in suspension-cultured spheres and adherent or re-adherent cells by qRT-PCR. As shown in Figure 1C, the mRNA level of miR-520b is significantly upregulated in suspension-cultured spheres (MCF-7 and MDA-MD-231) compared with adherent cells and re-adherent cells, respectively. In addition, as shown in Figure 1D, the expression of miR-520b is upregulated in CD44+, CD133+, ALDH1+ MCF-7 and MDA-MD-231 cells compared with CD44-, CD133-, ALDH1- cells. Moreover, the correlation between the expression of miR-520b and CD44, CD133 and ALDH1 was analyzed by Spearman analysis. We found that the expression of miR-520b is positively correlated with CD44, CD133 and ALDH1 in breast cancer tissues (Figure 1E). The clinical information of the patients was shown in .

These results thus suggested that miR-520b may associate with the maintenance of breast cancer stemness.

Ectopic Expression of miR-520b Promotes the Stemness of Breast Cancer Cells

To further confirm the role of miR-520b in the maintenance of breast cancer stemness, we overexpressed miR-520b in MCF-7 and MDA-MB-231 cells (). We first investigated the effect of miR-520b on the sphere-formation activities of breast cancer cells. As shown in Figure 2A, we found that miR-520b overexpression significantly increased the diameter and the number of the spheres, which demonstrated that miR-520b overexpression increased the sphere-formation activities of the breast cancer cells. As shown in Figure 2B, the results from transwell assay showed that the migration activity of the cells was significantly increased by miR-520b. In addition, the mRNA levels of the stem cell markers (CD44, CD133 and ALDH1) and mesenchymal markers (N-cadherin, Vimentin, Snail1 and ZEB1) were significantly upregulated in miR-520b-overexpressing cells (Figure 2C and D). Conversely, the mRNA levels of epithelial markers (E-cadherin and ZO-1) were significantly downregulated by miR-520b as identified by qRT-PCR (Figure 2E). The regulatory effects of miR-520b on CD44, E-cadherin, N-cadherin and Snail1 were also confirmed by Western blot assay (Figure 2F). Taken together, above results indicated that miR-520b promotes the stemness of breast cancer cells.

Figure 2

Ectopic expression of miR-520b promotes breast cancer stemness. (A) Ectopic expression of miR-520b increased both diameter and number of the breast cancer cell spheres. (B) miR-520b promoted the migration activity of the breast cancer cells as demonstrated by transwell assay. (C) The expression of cancer stem cell markers in indicated cells was tested by qRT-PCR. (D, E) The expression of EMT markers in indicated cells was tested by qRT-PCR. (F) The protein levels indicated markers in indicated cells were analyzed by Western blot. Student’s t-test (**P<0.01, ***P<0.001).

Knockdown of miR-520b Attenuates the Stemness of Breast Cancer Cells

Next, to confirm the stimulatory role of miR-520b in the maintenance of breast cancer stemness, miR-520b was inhibited by miR-520b inhibitor (). As we expected, the sphere-formation activity of the cells was inhibited by miR-520b inhibition (Figure 3A). miR-520b inhibition also attenuated the migration activity of the breast cancer cells (Figure 3B). The mRNA levels of cancer stem cell markers and the mesenchymal markers were significantly inhibited by miR-520b inhibition in the breast cancer cells (Figure 3C and D). While, the mRNA levels of epithelial markers were significantly upregulated in miR-520b-knockdown cells (Figure 3E). These results thus confirmed the conclusion that miR-520b promotes the stemness of breast cancer cells.

Figure 3

Knockdown of miR-520b attenuates the stemness of breast cancer cells. (A) Knockdown of miR-520b decreased both diameter and number of the breast cancer cell spheres. (B) Depletion of miR-520b attenuates the migration activity of the breast cancer cells as demonstrated by transwell assay. (C) The expression of cancer stem cell markers in indicated cells was tested by qRT-PCR. (D, E) The expression of EMT markers in indicated cells was tested by qRT-PCR. Student’s t-test (**P<0.01, ***P<0.001).

miR-520b Activates Hippo/YAP Signaling in Breast Cancer Cells

To investigate the mechanism underlying miR-520b promoting the stemness of breast cancer cells, we analyzed the potential target genes of miR-520b using the online database starBase V3.0. We found that a key component in Hippo/Yap signaling, LATS2, is the potential target of miR-520b (Figure 4A). In addition, bioinformatic analysis of GSE109169 dataset showed that the expression of LATS2 is significantly downregulated in breast cancer tissues (), which indicated that inhibition of LATS2 expression may be the cause of breast cancer development. As Hippo/YAP signaling pathway is largely associated with breast cancer stemness, we next investigated whether miR-520b regulates Hippo/YAP signaling in breast cancer cells. As shown in Figure 4B, the mRNA level of LATS2 was significantly inhibited by miR-520b in breast cancer cells. In addition, the mRNA levels of YAP target genes were significantly decreased in breast cancer cells (Figure 4C). Moreover, the phosphorylation level of YAP in breast cancer cells was significantly decreased by miR-520b (Figure 4D). Furthermore, the protein level of nuclear YAP was significantly upregulated by miR-520b in breast cancer cells (Figure 4E). These results demonstrated that miR-520b activates Hippo/YAP signaling in breast cancer cells.

Figure 4

miR-520b activates Hippo/YAP signaling pathway in breast cancer cells. (A) The binding site of miR-520b and LATS2. (B) miR-520b decreased the mRNA level of LATS2 in breast cancer cells as indicated by qRT-PCR. (C) miR-520b downregulated the mRNA levels of YAP target genes in breast cancer cells as analyzed by qRT-PCR. (D) miR-520b inhibits the phosphorylation of YAP in the breast cancer cells as identified by Western blot assay. (E) mIR-520b increased the protein level of nuclear YAP in breast cancer cells as identified by Western blot assay. Student’s t-test (**P<0.01, ***P<0.001).

Overexpression of LATS2 Abolished the Effect of miR-520b on Breast Cancer Stemness

Next, we performed rescue experiment by overexpression of LATS2 in breast cancer cells () to confirm the role of Hippo/YAP signaling in the effect of LATS2 on breast cancer stemness. As shown in Figure 5A, we found that overexpression of LATS2 significantly restored the sphere-formation activity of miR-520b-overexpressing cells. Similarly, the miR-520b-induced increased migration activity of the cells was reduced by LATS2 overexpression (Figure 5B). Moreover, overexpression of LATS2 significantly abolished the effect of miR-520b on the expression of stem cell markers, mesenchymal markers as well as epithelial markers as indicated by qRT-PCR (Figure 5C–E). Thus, these results demonstrated that miR-520b promotes breast cancer stemness through Hippo/YAP signaling pathway by targeting LATS2.

Figure 5

Overexpression of LATS2 abolished the effect of miR-520b on the stemness of breast cancer cells. (A) LATS2 overexpression abolished the effect of miR-520b on the sphere-formation activities of breast cancer cells. (B) Overexpression of LATS2 abolished the effect of miR-520b on the migration activities of breast cancer cells. (C–E) Overexpression of LATS2 abolished the effect of miR-520b on the expression of stem cell markers (C), mesenchymal markers (D) and epithelial markers (E) in the breast cancer cells. Student’s t-test (**P<0.01, ***P<0.001).

Discussion

Breast cancer is one of the leading causes of tumor-related mortality worldwide.1 Recent studies indicated that BCSCs are the root of breast cancer initiation, progression, metastasis and resistance to conventional therapy.8–12 However, the mechanisms underlying the maintenance of the stemness of breast cancer cells have remained elusive. In this study, we found that miR-520b is an oncogene that promotes the stemness of BCSCs through Hippo/YAP signaling. Our finding thus improved our understanding of mechanisms underlying the maintenance of breast cancer stemness.

Through bioinformatic analysis, we first found that miR-520b is upregulated in breast cancer tissues compared with adjacent normal tissues (Figure 1A). In addition, subsequent analysis showed that upregulation of miR-520b is associated with poor prognosis of breast cancer patients (Figure 1B). Moreover, ectopic expression of miR-520b promotes the sphere-formation and migration activities (Figure 2A and B). Conversely, knockdown of miR-520b attenuates the sphere formation and migration activities (Figure 3A and B). These data thus demonstrated that miR-520b is an oncogene. Our finding is opposed to the finding of Zhang et al in which miR-520b showed as a tumor suppressor by targeting MEKK2 and cyclin D1 in hepatoma cells.32 This information indicates that the function of miR-520b and other members in this family largely depends on the cellular context and the further studies are needed for understanding of the switch of such regulation.

Furthermore, we found that the expression of miR-520b is positively correlated with stem cells markers (Figure 1E). In addition, the expression of miR-520b is upregulated in spheres and cells expressed a high level of cancer stem cell markers (CD44, CD133 and ALDH1) compared with adherent and re-adherent control cells and cancer stem cell markers negative cells (Figure 1C and D). Moreover, we found that overexpression of miR-520b promotes the stemness of cancer stem cells, including sphere-formation, migration activities as well as the expression of stem cell markers, mesenchymal markers and epithelial markers (Figure 2). Conversely, knockdown of miR-520b inhibits the stemness of breast cancer cells (Figure 3). These results thus demonstrated that miR-520b promotes the stemness of breast cancer cells.

Hippo/YAP signaling pathway plays a central role in organ size control, tissue development and stemness maintenance of both normal and cancer stem cells.35 In Hippo/YAP signaling, LATS2 is activated by MST1/2-induced phosphorylation and then phosphorylates and inhibits YAP-mediated gene transcription; most of YAP target genes positively regulates cell cycle and stemness maintenance.36,37 In this study, we found that LATS2, the potential target of miR-520b (Figure 4A), was downregulated by miR-520b overexpression (Figure 4B). Correspondingly, the target genes of Hippo/YAP signaling pathway were inhibited in miR-520b-overexpressing cells (Figure 4C). Moreover, the phosphorylation of YAP is downregulated by miR-520b overexpression (Figure 4D). Furthermore, the protein level of nuclear YAP was significantly upregulated by miR-520b (Figure 4E). These results demonstrated that Hippo/YAP signaling is positively regulated by miR-520b in breast cancer cells. Subsequent rescue experiments showed that inhibition of LATS2 is necessary for miR-520b promoting the stemness of BCSCs. Taken together, these results demonstrated that miR-520b promotes breast cancer stemness through Hippo/YAP signaling pathway by targeting LATS2.

Conclusion

In conclusion, our results demonstrated that miR-520b promotes the stemness of breast cancer cells by activating Hippo/YAP signaling pathway via targeting LATS2.