Introduction

MCO

Molecular and Clinical Oncology

2049-9450 2049-9469

D.A. Spandidos

10.3892/mco.2017.1528

MCO-0-0-1528

Articles

Knockdown of microRNA-29a regulates the expression of apoptosis-related genes in MCF-7 breast carcinoma cells

Khamisipour

Gholamreza

1 2 Mansourabadi

Elham

3 Naeimi

Behrouz

4 Moazzeni

Ali

1 Tahmasebi

Rahim

2 Hasanpour

Mojtaba

2 Mohammadi

Majid Mosahebi

5 Mansourabadi

Zahra

1 Shamsian

Shakib

1Department of Hematology, Faculty of Allied Medicine, Bushehr University of Medical Sciences, Bushehr 75189577, Iran 2The Persian Gulf Tropical Medicine Research Center, Bushehr University of Medical Sciences, Bushehr 75189577, Iran 3Student Research Committee, Vice-Chancellery Research and Technology Affairs, Bushehr University of Medical Sciences, Bushehr 75189577, Iran 4Department of Microbiology and Parasitology, Faculty of Medicine, Bushehr University of Medical Sciences, Bushehr 75189577, Iran 5Department of Hematology, Faculty of Medical Sciences, Tarbiat Modares University, Tehran 14115331, Iran

Correspondence to: Dr Gholamreza Khamisipour, Department of Hematology, Faculty of Allied Medicine, Bushehr University of Medical Sciences, 2 Sabzabad Street, Bushehr 75189577, Iran, E-mail: r.khamisipour@bpums.ac.ir

02 2018

08 12 2017

8 2 362 369 02022017 30112017

2018

MicroRNA (miR), as non-coding small RNA, are key regulators of cancer-related biological cell processes and contribute to tumor growth through regulation of groups of pro- and anti-apoptotic genes. The present study aimed to investigate the effects of miR-29a on the expression of genes involved in apoptosis, including p21, B-cell lymphoma 2 (BCL-2), p53 and survivin. The MCF-7 breast cancer cell line was transfected with anti-miR-29a and treated with Taxol in subdivided treatment groups including: Scramble; anti-miR-29a; anti-miR-29a + Taxol; Taxol; and control. Expression levels of p21, BCL-2, p53 and survivin were evaluated using reverse transcription-quantitative polymerase chain reaction. miR-29a knockdown resulted in p21 and p53 upregulation and a decrease in survivin expression. These results indicated that miR-29a inhibition regulates apoptosis. The present data suggested that miR-29a inhibition may be a promising strategy for the induction of apoptosis of tumor cells.

microRNA-29a breast carcinoma apoptosis Taxol MCF-7

Introduction

Breast cancer is the most common cancer and continues to be a major cause of morbidity and mortality among women worldwide (1). Global statistics show that >1.15 million women each year are diagnosed with breast cancer, which results in >502,000 mortalities (2–4). This multifactorial disease occurs as a result of several risk factors, including female gender, increasing age, familial history of breast cancer, diet, obesity and life behavior, such as smoking and alcohol consumption (5,6). Based on the increased incidence of breast cancer (2), early detection will improve treatment success. In this regard, investigating appropriate oncomarkers for early detection, monitoring and treatment appears to be crucial. Due to limited treatment options, resistances to current standard therapies, the short duration of response and rapid relapse (7,8), finding novel therapeutics is considered as extremely important. MicroRNA (miR) may be one of these therapeutic targets.

miR are class of endogenously expressed, single-stranded, non-protein coding small RNA that bind to target mRNA. miR have important roles in diverse biological and pathological processes via both transcriptional and post-transcriptional gene regulation, making them attractive biomarkers in cancer (9,10). Research has demonstrated that miR have important roles in regulating cell processes that are often deregulated in cancer, including proliferation, differentiation and apoptosis (11). The miR-29 family has three main members, including hsa-miR-29a, hsa-miR-29b and hsa-miR-29c (12). Research has indicated that miR-29a negatively regulates the expression of Myb-related protein B, resulting in inhibition of breast cancer growth and arrest of cells in the G0/G1 phase (13). Downregulation of myeloid cell leukemia 1, as an anti-apoptotic protein, by miR-29b in malignant KMCH cholangiocarcinoma cells has been reported (14). Although the mir-29 family is involved in regulating tumorigenesis and development of various types of cancer, the role and the underlying mechanism of miR-29a in breast cancer remains to be fully elucidated (15).

B-cell lymphoma 2 (BCL-2) is a prototypical member of the BCL-2 family, which has been identified as a regulator of apoptosis (16). This molecule prevents the mitochondrial pathway of apoptosis (16,17). It has been reported that the miR-15a and miR-16-1 region is deleted in chronic lymphocytic leukemia, which leads to an aggressive state (18). These miR naturally induce apoptosis in normal cells through regulation of the anti-apoptotic, proto-oncogene BCL-2 (18). BCL-2 expression may be downregulated by miR-34, which is compatible with the role of miR-34 in apoptosis mediated by p53 expression (19). p53 is a pleiotropic regulator of cell fate, which may facilitate apoptosis (20,21). miR have been identified to regulate p53 expression by controlling the upstream regulation of p53 and its pro-apoptotic function, as research has demonstrated that miR-125 negatively regulates p53 (22). Research has indicated that the expression level of p53 protein was decreased and apoptosis was stopped in human neuroblastoma and in lung fibroblasts (22). p21 is induced by p53-dependent and -independent mechanisms implicated in both major functions of the tumor suppressor-cell cycle arrest and apoptosis (23).

Survivin is overexpressed in the majority of human malignancies and functions as a key regulator of mitosis and programmed cell death (24,25). Research has demonstrated that miR-218 is involved in breast cancer evasion of apoptosis by targeting survivin (26). This molecule has been targeted for therapy in cancer based on its selective expression in tumors, but not normal tissues (27,28). The present study aimed to evaluate miR-29a knockdown on the expression of important genes involved in cell apoptosis and proliferation of breast carcinoma. In particular, it was proposed that knockdown of miR-29a may alter the expression profile of p53, p21, BCL-2 and survivin genes.

Materials and methods <sec> <title>Cell line

The MCF-7 human breast cancer line was obtained from the Iranian Stem Cell Technology Research Center (Tehran, Iran) and cultured in RPMI-1640 culture medium supplemented with 10% fetal bovine serum and 1% penicillin and streptomycin (all Gibco; Thermo Fisher Scientific, Inc., Waltham, MA, USA) at 37°C in a 5% CO₂ humidified incubator. At ~80% confluence, adherent cultured cells were harvested following trypsin treatment at 37°C for 3 min and used for transfection.

Reverse transfection of MCF-7 cells with anti-miR-29a

Cells were transfected using Lipofectamine reagent (Invitrogen; Thermo Fisher Scientific, Inc.) with anti-miR-29a (MIMAT0000086; 5′-UAGCACCAUCUGAAAUCGGUUA-3′; Qiagen, Inc., Valencia, CA, USA), at a final concentration of 50 nM, and scramble at a final concentration of 5 nM in opti-MEM medium (Invitrogen; Thermo Fisher Scientific, Inc.), as described previously (29). Following transfection, MCF7 cells were treated with Taxol [1, 10 and 50 ng/ml; concentrations determined using MTT assay (data not shown)] to inhibit cell growth and trigger apoptosis. Taxol (Paclitaxel) was purchased from Sobhan Oncology Co., (Tehran, Iran). Cells were harvested after 24 h of incubation with Taxol at 37°C in a 5% CO₂ humidified incubator.

Viability assessment

Studied cells were categorized into the nine following groups: Non-treated; scramble; anti-miR-29a; anti-miR-29a + Taxol (1 ng/µl); anti-miR-29a + Taxol (10 ng/µl); anti-miR-29a + Taxol (50 ng/µl); Taxol (1 ng/µl); Taxol (10 ng/µl); and Taxol (50 ng/µl). A total of 72 h after anti-miR-29a and Taxol treatment in a 5% humidified CO₂ incubator, 100 µl MTT (5 mg/ml) was added to the cells. Optical absorbance of generated formazan was evaluated at a wavelength of 590 nm in each group 4 h following replacement of supernatant by dimethyl sulfoxide. All experiments were conducted three times.

RNA extraction and reverse transcription-quantitative polymerase chain reaction (RT-qPCR)

Total RNA was extracted from cultured cells in the different groups using an easy-BLUE TM Total RNA Extraction kit (iNtRON Biotechnology, Inc., Sungnam, Korea), according to the manufacturer's instructions, 72 h after transfection and treatment with Taxol. RNA quality and concentration were determined after extraction using a Nanodrop spectrophotometer (Thermo Fisher Scientific, Inc.) and electrophoresis on 2% agarose gel. cDNA was generated using a cDNA Synthesis H Minus First Strand Revert Aid kit (Thermo Fisher Scientific, Inc.), according to the manufacturer's instructions. Sequences of specific primers for stem loop RT-PCR cDNA synthesis of miR-29a (target gene) and U6 small nuclear (sn)RNA (reference gene) were 5′-GTCGTATCCAGTGCAGGGTCCGAGGTATTCGCACTGGATCAGACTAACCGAT-3′ and 5′-AAAATATGGAACGCTTCACGAATTTG-3′, respectively. Using general primers (random and oligo dT primers) and a Maxime RT premix cDNA synthesis (iNtRON Biotechnology, Inc.) the cDNA for quantifying p21, p53, BCL-2 and survivin were synthesized.

qPCR was performed using a 2X Real MOD Green PCR Master Mix kit (Takara Bio, Inc., Otsu, Japan), according to the manufacturer's instructions. Briefly, 2 µl cDNA product was diluted in a final volume of 20 µl, containing 10 pmol of each primer, 10 µl 2× reaction mixture of SYBR Green and 7.4 µl sterile deionized water. The cycling program was as follows: Initial denaturation at 95°C for 10 min, followed by 40 cycles of denaturation at 95°C for 10 sec, annealing and extension at 55°C for 40 sec. U6 snRNA and hypoxanthine-guanine phosphoribosyltransferase (HGPRT) were used as internal housekeeping controls. All reactions were performed in triplicate and relative quantity of gene expression was analyzed using the Pfaffl method (30). Sequences of primers used for quantification of the desired genes involved in apoptosis are presented in Table I.

Statistical analysis

Results were expressed as the mean ± standard deviation and analyzed using SPSS v. 16.0 software (SPSS, Inc., Chicago, IL, USA). Differences between groups was evaluated by Kruskal-Wallis tests, and comparison of studied groups for the expression of the desired genes was assessed by Mann-Whitney U tests. P<0.05 was considered to indicate a statistically significant difference.

Results <sec> <title>Knockdown of the miR-29a gene in the MCF-7 cell line

Downregulating the expression of miR-29a was the initial aim of the present experiment. In order to achieve this, cells were treated with anti-miR-29a and scramble. The cycle threshold of miR-29a was normalized with U6 snRNA as a reference gene and compared with the non-treated group as a calibrator. As demonstrated in Fig. 1, a significant reduction of miR-29a expression was observed following anti-miR-29a treatment compared with the scramble treatment (P<0.05). In cells transfected with anti-miR-29a, the expression of miR-29a was decreased by up to 75% compared with the scramble-treated group.

Effect of miR-29a suppression on cell viability

The viability of MCF-7 cells following knockdown of miR-29a was evaluated 72 h post-transfection with anti-miR-29a. As demonstrated in Fig. 2, the viability of cells transfected with anti-miR-29a was reduced compared with the scramble and negative control groups; however, this difference was not significant (P>0.05). According to MTT assay, 10 ng/ml Taxol was selected as the optimal concentration. With increasing concentrations of Taxol, cell viability of MCF-7 cells decreased; however, transfection with anti-miR-29a and treatment with Taxol simultaneously resulted in significant increases in the viability of cells compared to treatment with Taxol alone (P<0.05). Therefore, anti-miR-29a induces modification of cell viability following treatment with Taxol.

BCL-2 gene expression decreases following knockdown of miR-29a

Fold changes in the expression levels of genes, including p21, p53, BCL-2 and survivin, are represented in Table II. The cycle threshold of target genes was normalized against HGPRT as a reference gene. Fold changes were obtained by dividing the cycle threshold of each treatment group by the cycle threshold of the non-treated group. Nine groups of MCF-7 cells for each gene were treated: Non-treated (calibrator); treated by scramble; anti-miR-29a; anti-miR-29a + Taxol 1 ng/ml; anti-miR-29a + Taxol 10 ng/ml; anti-miR-29a + Taxol 50 ng/ml; Taxol 1 ng/ml; Taxol 10 ng/ml; and Taxol 50 ng/ml. Kruskal-Wallis and Mann-Whitney U non-parametric tests were used for evaluating the differences in expression levels of the desired genes between the experimental groups.

Results demonstrated that BCL-2 gene expression decreased following knockdown of miR-29a. It has been indicated that BCL-2 has a critical role in the pathogenesis of various types of cancer by regulating apoptosis (31). Thus, the expression of BCL-2 was measured in the different treatment groups. Based on RT-qPCR, it was observed that in cells transfected with anti-miR-29a, the gene expression of BCL-2 was downregulated by ~36% compared with the scramble; however, this difference was not significant (P>0.05). As demonstrated in Fig. 3, transfection with anti-miR-29a + Taxol and Taxol alone caused 50 and 87% reduction, respectively, in expression levels of BCL-2 compared with the non-treated group; however, these differences were not statistically significant. Thus, treatment with anti-miR-29a + Taxol could reduce the expression of BCL-2; however, it could not reduce the level to as low as that observed following treatment with Taxol alone, which was significantly lower than the expression level in the anti-miR-29a group (P<0.05).

p53 gene expression increases in anti-miR-29a-treated cells

To further understand the role of miR-29a in the apoptosis of cancer cells, the expression of p53 as a regulatory gene of apoptosis was analyzed by suppressing miR-29a with anti-miR-29a. Based on RT-qPCR, expression levels of p53 increased by ~40% in cells transfected with anti-miR-29a and scramble treatment induced a ~1.9-fold increase in p53 gene expression compared with the non-treated control group. Treatment with anti-miR-29a + Taxol and Taxol alone caused a reduction of 46 and 70%, respectively, in p53 expression compared with the non-treated group (Fig. 4). These results also indicated that p53 gene expression in the anti-miR-29a-treated group was significantly upregulated (5.8-fold higher) compared with the Taxol-treated group (P<0.05).

Inhibition of miR-29a has no effect on the expression level of p21

The role of miR-29a in apoptosis of cancer cells was explored through investigating the gene expression of p21 in MCF-7 cells. There were no significant differences between p21 gene expression levels in cells transfected with anti-miR-29a and the non-treated controls. As demonstrated in Fig. 5, transfection with scramble, anti-miR-29a + Taxol and Taxol alone resulted in significant reductions of 80, 60 and 90%, respectively, in gene expression of p21 compared with cells transfected with anti-miR-29a (P<0.05). The expression of p21 in Taxol-treated cells decreased by 10.5-fold compared with cells treated with anti-miR-29a (P<0.05).

Survivin gene expression is reduced in cells transfected with anti-miR-29a

Transfection of MCF-7 cells with anti-miR-29a caused reduction of survivin expression by 17% compared with the non-treated control group. However, there was no significant difference in expression of survivin in cells transfected with scramble and the non-treatment group. The present results demonstrated that transfection with anti-miR-29a significantly reduced the expression of survivin 1.43-fold lower than the Taxol-treated group (P<0.05). As indicated in Fig. 6, survivin gene expression increased significantly, by 1.7- and 1.2-fold, in cells transfected with anti-miR29a + Taxol and Taxol alone compared with the scramble, respectively (P<0.05).

Expression of target genes following transfection with anti-miR-29a

The present experiment demonstrated that inhibition of miR-29a could alter the expression profiles of target genes. As indicated in Fig. 7, following transfection with anti-miR-29a, the expression of BCL-2 increased 2.6-fold higher and 2-fold higher than survivin and p21, respectively. The difference between the expression levels of BCL-2 and survivin were significant (P<0.05). Also, the expression of p21 and survivin decreased 1.3- and 1.7-fold lower than p53 expression, respectively; however, these differences were not significant (P>0.05). Thus, transfection with anti-miR-29a resulted in increases of p53 and BCL-2 gene expression compared to p21 and survivin.

Anti-miR-29a transfection combined with treatment with various concentrations of Taxol results in different expression of target genes

To further analyze the expression of target genes (p21, p53, BCL-2 and survivin), in anti-miR-29a + Taxol-treated cells, it was hypothesized that various concentrations of Taxol would have different effects on gene expression. Therefore, transfection with anti-miR-29a was conducted, along with treatment with 1, 10 or 50 ng/ml Taxol. Results demonstrated that treatment with 1 ng/ml Taxol and anti-miR-29a transfection resulted in increased expression of target genes p21, p53 and BCL-2, compared with the other Taxol concentrations. As demonstrated in Fig. 8, cells treated with anti-miR-29a + Taxol 1 ng/ml showed a significant 3.6-, 1.9- and 4.7-fold increase in p21, p53 and BCL-2 expression, respectively, compared with cells treated with anti-miR-29a + Taxol 10 ng/ml (P<0.05). p21, p53 and BCL-2 levels were also significantly lower in the anti-miR-29a + Taxol 50 ng/ml groups compared with the anti-miR-29a + Taxol 1 ng/ml (P<0.05). Also, in cells treated with anti-miR-29a + Taxol 1 ng/ml, the expression of survivin was reduced by 1.5-fold compared with the expression levels in cells treated with anti-miR-29a + Taxol 10 ng/ml; however, this difference was not significant.

Discussion

Cellular expression of p21, p53, BCL-2 and survivin, which are involved in apoptosis and proliferation, is tightly regulated by miR-29a (32). High expression of miR-29a in the MCF-7 human adenocarcinoma breast cancer cell line and sera of patients with breast cancer disease has been reported (33). As described earlier, miR are key regulators in expression of genes involved in the control of tumor development, proliferation, apoptosis and the stress response (34). Aberrant expression of miR in various types of cancer have been demonstrated; however, the molecular mechanisms by which miR modulate the process of tumor genesis and the behavior of cancer cells remains controversial (35). In present study, it was demonstrated that the inhibition of miR-29a could efficiently alter the expression profile of genes that are regulators of apoptosis in MCF-7 cells. First, miR-29a expression was successfully downregulated using anti-miR-29a. The viability of cells treated with Taxol and anti-miR-29a simultaneously increased compared with treatment of Taxol alone, suggesting the interference role of anti-miR-29a in cancer cell apoptosis. Results indicated that miR-29a expression was reduced by up to 75% in cells transfected with anti-miR-29a compared with the non-treated control group.

miR-29 family members have been identified as regulators of p53, leading to upregulation of p53 and apoptosis induction (32). The effect of miR-29a on breast cancer cell growth is largely dependent on upregulation of p53, and the present study shed new insight on the regulation of breast cancer cell apoptosis by miR-29a. The expression of p53 as a tumor suppressor gene was upregulated by 50% in absence of miR-29a, although Taxol treatment caused a 70% reduction in p53 expression compared with non-treated controls. This undesirable reduction in p53 was also observed following treatment with anti-miR-29a + Taxol, with a 46% reduction compared with that seen in cells transfected with the scramble control. p53 expression in anti-miR-29a-treated cells was 5.8-fold higher compared with the Taxol-treated group. Therefore, inhibition of miR-29a alone could increase p53 expression and result in cancer cell cycle arrest and apoptosis.

Of the four genes examined in the present study, p21 was the only gene for which expression was not altered following anti-miR-29a transfection compared with the non-treated control. p21 is a downstream target of p53 and has a role in apoptosis inhibition, which reflects the unwanted performance of this molecule in the cancer process (36). Research has indicated that p21 activity may be regulated by multiple signal transduction pathways, resulting in a stimulatory or inhibitory role of p21 in tumor genesis depending on cellular status (37). The present study demonstrated that treatment of miR-29a + Taxol reduced the p21 expression levels by up to 60% compared with cells transfected with anti-miR-29a. This reduction was 90% in treatment with Taxol alone. The negative effect of Taxol on the expression of p21 was therefore moderated by the use of anti-miR-29a and Taxol simultaneously. The expression of p21 in the Taxol-treated group was reduced by 10.5-fold compared with the anti-miR-29a group. Regarding the dual role of p21 in tumor genesis, using Taxol to reduce p21 expression and resulting in apoptosis of tumor cells appears to be useful; however, on the other hand, this could help tumor progression.

Furthermore, the present study characterized BCL-2 as a functional target of miR-29a. BCL-2 acts as an apoptosis regulator and it has been reported that BCL-2 expression is associated with a good prognosis in patients with breast cancer (38). It has been reported that in breast cancer cells, silencing miR-15a and miR-16 restore BCL-2 expression (39). Also, due to the activity of miR-15a and miR-16, BCL-2 downregulation results in apoptosis (18). Accordingly, the present results demonstrated that silencing miR-29a increased BCL-2 expression 2-fold higher than the control. Although, in Taxol and anti-miR-29a + Taxol-treated groups, BCL-2 decreased by 87 and 50%, respectively, compared with the non-treated control. It may be concluded that silencing miR-29a could not exert a beneficial effect against tumor genesis through BCL-2. On the other hand, Taxol treatment through reduction of BCL-2 would have a positive effect on apoptosis induction.

Survivin, a multi-functional protein, has an important role in cell cycle regulation, inhibition of apoptosis and stimulation the angiogenesis (40). Survivin expression is upregulated in malignancies, which is associated with upregulation of human epidermal growth factor receptor 2 and vascular endothelial growth factor resulting in angiogenesis (41). It has been demonstrated that survivin leads to resistance to chemotherapy (42). Therefore, inhibition of this molecule could be an important strategy to overcome resistance to chemotherapy and to remove the inhibitory effect of this molecule on apoptosis. It has been reported that survivin expression could be inhibited using deguelin, which results in restoration of the sensitivity of tumor cells to chemotherapy (43). The results of the present study demonstrated that inhibition of miR-29a resulted in the downregulation of survivin by up to 17% compared with the non-treated group. Expression of survivin as a unique inhibitor of apoptosis was upregulated in cells transfected with Taxol alone and in combination with anti-miR-29a compared with cells transfected with anti-miR-29a alone. These findings demonstrated that reduction of survivin expression was achieved through inhibition of miR-29a. This may have a positive impact on apoptosis induction. However, Taxol had negative effects in regards to the levels of survivin.

The anticancer agent, Taxol, is used in chemotherapy regimens against breast cancer and leads to cell cycle arrest and apoptotic cell death (44). However, its application is limited due to adverse effects on normal cells. In the present study, it was demonstrated that lower doses of Taxol in combination with anti-miR-29a treatment induced stronger effects on the expression of target genes. In cells transfected with anti-miR-29a + Taxol 1 ng/ml, the expression profile of p21, p53 and BCL-2 was upregulated significantly compared with anti-miR-29a treatment combined with 10 or 50 ng/ml Taxol. Therefore, anti-miR-29a transfection attracts much attention as an anticancer treatment in the manner of boosting the effect of Taxol.

In conclusion, regarding the important role of miR-29a inhibitors in regulating the apoptosis of breast cancer cells that express a high level of miR-29a, they may be candidates for chemotherapeutic agents. Unlike the adverse effects of Taxol on normal cells and its infilltration throughout the body, as it is not a specific agent, anti-miR-29a may be applied locally in the tumor site. Due to the low stability of miR, the time duration of their application should be considered important. Furthermore, improving the stability of these molecules would be an important research area. However, further investingation in cells and animal models is required to verify the results of the present study.

Acknowledgements

We are grateful to the Research Deputy at Bushehr University of Medical Sciences (Bushehr, Iran) for financially supporting the present study (grant no. 2307-2013.07.16). We wish to thank Bonyakhteh Research Center (Tehran, Iran).

References 1

Montazeri

Vahdaninia

Harirchi

Sajadian

Khaleghi

Ebrahimi

Haghighat

Breast cancer in Iran: Need for greater women awareness of warning signs and effective screening methods

Asia Pac Fam Med762008

10.1186/1447-056X-7-6

19099595

Ferlay

Cancer IAfRo: GLOBOCAN 2000: Cancer incidence, mortality and prevalence worldwideIARC press2001

Parkin

Bray

Ferlay

Pisani

Global cancer statistics, 2002

CA Cancer J Clin55741082005

10.3322/canjclin.55.2.74

15761078

Stewart

Kleihues

World cancer reportGeneva

International Agency for Research on Cancer. World Health Organization

2003

Khatib

Modjtabai

Guidelines for the early detection and screening of breast cancer: World Health Organization

Regional Office for the Eastern Mediterranean2006

Network

NCC

NCCN clinical practice guidelines in oncology™ breast cancer: National Comprehensive Cancer Network2007

André

Zielinski

Optimal strategies for the treatment of metastatic triple-negative breast cancer with currently approved agents

Ann Oncol23suppl 6vi46vi512012

10.1093/annonc/mds195

23012302

Bauer

Hummon

Effects of the miR-143/-145 microRNA cluster on the colon cancer proteome and transcriptome

J Proteome Res11474447542012

10.1021/pr300600r

22897626

Bartel

MicroRNAs: Target recognition and regulatory functions

Cell1362152332009

10.1016/j.cell.2009.01.002

19167326

Chen

Rajewsky

The evolution of gene regulation by transcription factors and microRNAs

Nat Rev Genet8931032007

10.1038/nrg1990

17230196

Getz

Miska

Alvarez-Saavedra

Lamb

Peck

Sweet-Cordero

Ebert

Mak

Ferrando

MicroRNA expression profiles classify human cancers

nature4358348382005

10.1038/nature03702

15944708

Chang

Lee

Wentzel

Arking

West

Dang

Thomas-Tikhonenko

Mendell

Widespread microRNA repression by Myc contributes to tumorigenesis

Nat Genet4043502008

10.1038/ng.2007.30

18066065

Huang

Zou

Guo

The inhibitory role of Mir-29 in growth of breast cancer cells

J Exp Clin Cancer Res32982013

10.1186/1756-9966-32-98

24289849

Mott

Kobayashi

Bronk

Gores

mir-29 regulates Mcl-1 protein expression and apoptosis

Oncogene26613361402007

10.1038/sj.onc.1210436

17404574

Jiang

Zhang

Jiang

Diverse roles of miR-29 in cancer (review)

Oncol Rep31150915162014

10.3892/or.2014.3036

24573597

Letai

Pharmacological manipulation of Bcl-2 family members to control cell death

J Clin Invest115264826552005

10.1172/JCI26250

16200198

Plati

Bucur

Khosravi-Far

Dysregulation of apoptotic signaling in cancer: Molecular mechanisms and therapeutic opportunities

J Cell Biochem104112411492008

10.1002/jcb.21707

18459149

Cimmino

Calin

Fabbri

Iorio

Ferracin

Shimizu

Wojcik

Aqeilan

Zupo

Dono

miR-15 and miR-16 induce apoptosis by targeting BCL2

Proc Natl Acad Sci USA1021394413949

2005

10.1073/pnas.0506654102

16166262

Bommer

Gerin

Feng

Kaczorowski

Kuick

Love

Zhai

Giordano

Qin

Moore

p53-mediated activation of miRNA34 candidate tumor-suppressor genes

Curr Biol17129813072007

10.1016/j.cub.2007.06.068

17656095

Brown

Lain

Verma

Fersht

Lane

Awakening guardian angels: Drugging the p53 pathway

Nat Rev Cancer98628732009

10.1038/nrc2763

19935675

Junttila

Evan

p53-a Jack of all trades but master of none

Nat Rev Cancer98218292009

10.1038/nrc2728

19776747

Teh

Shyh-Chang

Xie

Zhou

Korzh

Lodish

Lim

MicroRNA-125b is a novel negative regulator of p53

Genes Dev238628762009

10.1101/gad.1767609

19293287

Xia

Knezevic

Vassilev

p21 does not protect cancer cells from apoptosis induced by nongenotoxic p53 activation

Oncogene303463552011

10.1038/onc.2010.413

20871630

Altieri

Survivin in apoptosis control and cell cycle regulation in cancer

Prog Cell Cycle Res54474522003

14593739

Mita

Nawrocki

Giles

Survivin: Key regulator of mitosis and apoptosis and novel target for cancer therapeutics

Clin Cancer Res14500050052008

10.1158/1078-0432.CCR-08-0746

18698017

Yagüe

miR-218 targets survivin and regulates resistance to chemotherapeutics in breast cancer

Breast Cancer Res Treat1512692802015

10.1007/s10549-015-3372-9

25900794

Altieri

Survivin, cancer networks and pathway-directed drug discovery

Nat Rev Cancer861702008

10.1038/nrc2293

18075512

Kanwar

Kamalapuram

Kanwar

Survivin signaling in clinical oncology: A multifaceted dragon

Med Res Rev337657892013

10.1002/med.21264

22688671

Choghaei

Khamisipour

Falahati

Naeimi

Mossahebi-Mohammadi

Tahmasebi

Hasanpour

Shamsian

Hashemi

Knockdown of microRNA-29a changes the expression of heat shock proteins in breast carcinoma MCF-7 cells

Oncol Res2369782016

10.3727/096504015X14478843952906

Jolla

Quantification strategies in real-time PCR Michael W. Pfaffl11122004

Yip

Reed

Bcl-2 family proteins and cancer

Oncogene27639864062008

10.1038/onc.2008.307

18955968

Park

Lee

Nam

Kim

miR-29 miRNAs activate p53 by targeting p85 alpha and CDC42

Nat Struct Mol Biol1623292009

10.1038/nsmb.1533

19079265

Michael

O'Connor

van Holst Pellekaan

Young

James

Reduced accumulation of specific MicroRNAs in colorectal neoplasia11note: Susan M. O'Connor and Nicholas G. van holst pellekaan contributed equally to this work

Mol Cancer Res18828912003

14573789

MicroRNAs in human diseases: From cancer to cardiovascular disease

Immune Netw111354542011

10.4110/in.2011.11.3.135

21860607

Iorio

Croce

MicroRNA dysregulation in cancer: Diagnostics, monitoring and therapeutics. A comprehensive review

EMBO Mol Med41431592012

10.1002/emmm.201100209

22351564

Abbas

Dutta

p21 in cancer: Intricate networks and multiple activities

Nat Rev Cancer94004142009

10.1038/nrc2657

19440234

Warfel

El-Deiry

p21WAF1 and tumourigenesis: 20 years after

Curr Opin Oncol2552582013

10.1097/CCO.0b013e32835b639e

23159848

Redondo

Bcl-2, an antiapoptotic gene indicator of good prognosis in breast cancer: The paradox

J Carcinogene Mutagene41351392013

10.4172/2157-2518.1000134

Yang

Cao

Sun

Zhang

Curcumin reduces the expression of Bcl-2 by upregulating miR-15a and miR-16 in MCF-7 cells

Med Oncol27111411182010

10.1007/s12032-009-9344-3

19908170

Schmidt

Schag

Müller

Weck

Appel

Kanz

Grünebach

Brossart

Survivin is a shared tumor-associated antigen expressed in a broad variety of malignancies and recognized by specific cytotoxic T cells

Blood1025715762003

10.1182/blood-2002-08-2554

12576330

Asanuma

Torigoe

Kamiguchi

Hirohashi

Ohmura

Hirata

Sato

Survivin expression is regulated by coexpression of human epidermal growth factor receptor 2 and epidermal growth factor receptor via phosphatidylinositol 3-kinase/AKT signaling pathway in breast cancer cells

Cancer Res6511018110252005

10.1158/0008-5472.CAN-05-0491

16322251

Jha

Shukla

Pandey

Survivin expression and targeting in breast cancer

Surg Oncol211251312012

10.1016/j.suronc.2011.01.001

21334875

Ghanbari

Mohseni

Tabasinezhad

Yousefi

Saei

Sharifi

Rashidi

Samadi

Inhibition of survivin restores the sensitivity of breast cancer cells to docetaxel and vinblastine

Appl Biochem Biotechnol1746676812014

10.1007/s12010-014-1125-6

25086926

Ofir

Seidman

Rabinski

Krup

Yavelsky

Weinstein

Wolfson

Taxol-induced apoptosis in human SKOV3 ovarian and MCF7 breast carcinoma cells is caspase-3 and caspase-9 independent

Cell Death Differ96366422002

10.1038/sj.cdd.4401012

12032672

Figure 1.

miR-29a gene expression in MCF-7 cells. Cells transfected with anti-miR-29a demonstrated a 75% reduction in miR-29a expression compared with the scramble. Gene expression levels were evaluated relative to the non-treated group and calibrated by the hypoxanthine-guanine phosphoribosyltransferase control gene. Data are presented as the mean ± standard deviation. *P<0.05 vs. scramble. miR, microRNA.

Figure 2.

Viability of MCF-7 breast cancer cells following knockdown of miR-29a. Data demonstrate the ratio of obtained absorbance of formed formazan for treated groups and the non-treated group (calibrator). *P<0.05 vs. Taxol 1 ng/ml; **P<0.05 vs. Taxol 10 ng/ml; ***P<0.05 vs. Taxol 50 ng/ml. miR, microRNA.

Figure 3.

BCL-2 gene expression in MCF-7 cells. Cells were transfected with scramble, anti-miR-29a, anti-miR-29a + Taxol or Taxol alone. Transfection with anti-miR-29a resulted in a 17.5-fold increase in expression of BCL-2 compared with Taxol treatment alone. Data are presented as the mean ± standard deviation. *P<0.05 vs. anti-miR-29a. BCL-2, B-cell lymphoma 2; miR, microRNA.

Figure 4.

Expression of p53 in MCF-7 cells transfected with scramble, anti-miR-29a, anti-miR-29a + Taxol or Taxol alone. There was an increase in p53 gene expression in anti-miR-29a-transfected MCF-7 cells compared with the non-treated control group; however, this difference was not significant. Data are presented as the mean ± standard deviation. *P<0.05 vs. scramble and anti-miR-29a groups. miR, microRNA.

Figure 5.

Results of reverse transcription-quantitative polymerase chain reaction for p21 gene expression in treated cells. Cells were transfected with scramble, anti-miR-29a, anti-miR-29a + Taxol and Taxol alone. There were no differences between P21 gene expression in cells transfected cells with anti-miR-29a compared with the non-treated control group. Data are presented as the mean ± standard deviation. *P<0.05 vs. anti-miR-29a. miR, microRNA.

Figure 6.

Results of reverse transcription-quantitative polymerase chain reaction for survivin gene transcript in MCF-7 cells transfected with scramble, anti-miR-29a, anti-miR-29a + Taxol or Taxol alone. Survivin gene expression significantly reduced in cells transfected with anti-mir-29a compared with those treated with anti-miR-29a + Taxol and Taxol alone. Data are presented as the mean ± standard deviation. *P<0.05 vs. anti-miR-29a + Taxol and Taxol alone; ^#P<0.05 vs. scramble. miR, microRNA.

Figure 7.

Comparison of the expression level of desired genes following transfection with anti-miR-29a. Following transfection with anti-miR-29a, the expression of BCL-2 and p53 increased compared with p21 and survivin in MCF-7 cells. Gene expression levels were evaluated relative to the non-treated group and calibrated by the hypoxanthine-guanine phosphoribosyltransferase control gene. Data are presented as the mean ± standard deviation. *P<0.05 vs. BCL-2. miR, microRNA; BCL-2, B-cell lymphoma 2.

Figure 8.

Expression level of p21, p53, BCL-2 and survivin in MCF-7 cells treated with anti-miR-29a and various doses of Taxol. Taxol 1 ng/ml in combination with anti-miR-29a resulted in significantly increased expression of p21, p53 and BCL-2 compared with the two other doses. Data are presented as the mean ± standard deviation. *P<0.05 vs. 1 ng/ml Taxol for the same gene. miR, microRNA; BCL-2, B-cell lymphoma 2.

Table I.

Primers used for reverse transcription-quantitative polymerase chain reaction.

Gene	Direction	Primer sequence
MicroRNA-29a	F	5′-TGCGCTAGCACCATCTGAAA-3′
	R	5′-CAGTGCAGGGTCCGAGGAT-3′
U6 small nuclear RNA	F	5′-CTCGCTTCGGCAGCACATATAC-3′
	R	5′-ACGCTTCACGAATTTGCGTGTC-3′
p21	F	5′-GAGGCCGGGATGAGTTGGGAGGAG-3′
	R	5′-CAGCCGGCGTTTGGAGTGGTAGAA-3′
p53	F	5′-TAACAGTTCCTGCATGGGCGGC-3′
	R	5′-AGGACAGGCACAAACACGCACC-3′
B-cell lymphoma 2	F	5′-GGTGGGGTCATGTGTGTGG-3′
	R	5′-CGGTTCAGGTACTCAGTCATCC-3′
Survivin	F	5′-AGAACTGGCCCTTCTTGGAGG-3′
	R	5′-CTTTTTATGTTCCTCTATGGGGT-3′
Hypoxanthine-guanine phosphoribosyltransferase	F	5′-GGACAGGACTGAACGTCTTG-3′
	R	5′-ATAGCCCCCCTTGAGCACAC-3′

F, forward; R, reverse.

Table II.

Fold changes in p21, p53, BCL-2 and survivin gene expression in the experimental groups.

	Gene

Group	p21	p53	BCL-2	Survivin
Scramble	0.32±0.070	1.9±0.080	3.27±0.701	0.97±0.021
Anti-miR-29a	1.06±0.030	1.4±0.051	2.1±0.070	0.8±0.020
Anti-miR-29a + Taxol 1 ng/ml	1.46±0.090	1.06±0.011	2.3±0.061	1.07±0.020
Anti-miR-29a + Taxol 10 ng/ml	0.4±0.005	0.5±0.003	0.49±0.030	1.6±0.061
Anti-miR-29a + Taxol 50 ng/ml	0.47±0.011	0.78±0.110	0.62±0.021	0.6±0.040
Taxol 1 ng/ml	0.2±0.006	0.42±0.070	0.16±0.003	1.2±0.090
Taxol 10 ng/ml	0.1±0.005	0.24±0.030	0.12±0.003	1.16±0.051
Taxol 50 ng/ml	0.19±0.020	0.14±0.011	0.43±0.008	1.28±0.010

Data are presented as the mean ± standard deviation. BCL-2, B-cell lymphoma 2; miR, microRNA.