National Centre of Applied Human Genetics, School of Life Sciences, Jawaharlal Nehru University, New Mehrauli Road, Saraswatipuram, New Delhi 110 067, India.
Breast Cancer Res. 2011 Apr 4;13(2):R39. doi: 10.1186/bcr2861.
New levels of gene regulation with microRNA (miR) and gene copy number alterations (CNAs) have been identified as playing a role in various cancers. We have previously reported that sporadic breast cancer tissues exhibit significant alteration in H2AX gene copy number. However, how CNA affects gene expression and what is the role of miR, miR-24-2, known to regulate H2AX expression, in the background of the change in copy number, are not known. Further, many miRs, including miR-24-2, are implicated as playing a role in cell proliferation and apoptosis, but their specific target genes and the pathways contributing to them remain unexplored.
Changes in gene copy number and mRNA/miR expression were estimated using real-time polymerase chain reaction assays in two mammalian cell lines, MCF-7 and HeLa, and in a set of sporadic breast cancer tissues. In silico analysis was performed to find the putative target for miR-24-2. MCF-7 cells were transfected with precursor miR-24-2 oligonucleotides, and the gene expression levels of BRCA1, BRCA2, ATM, MDM2, TP53, CHEK2, CYT-C, BCL-2, H2AFX and P21 were examined using TaqMan gene expression assays. Apoptosis was measured by flow cytometric detection using annexin V dye. A luciferase assay was performed to confirm BCL-2 as a valid cellular target of miR-24-2.
It was observed that H2AX gene expression was negatively correlated with miR-24-2 expression and not in accordance with the gene copy number status, both in cell lines and in sporadic breast tumor tissues. Further, the cells overexpressing miR-24-2 were observed to be hypersensitive to DNA damaging drugs, undergoing apoptotic cell death, suggesting the potentiating effect of mir-24-2-mediated apoptotic induction in human cancer cell lines treated with anticancer drugs. BCL-2 was identified as a novel cellular target of miR-24-2.
mir-24-2 is capable of inducing apoptosis by modulating different apoptotic pathways and targeting BCL-2, an antiapoptotic gene. The study suggests that miR-24-2 is more effective in controlling H2AX gene expression, regardless of the change in gene copy number. Further, the study indicates that combination therapy with miR-24-2 along with an anticancer drug such as cisplatin could provide a new avenue in cancer therapy for patients with tumors otherwise resistant to drugs.
新的基因调控水平,包括 microRNA(miR)和基因拷贝数改变(CNAs),已被确定在各种癌症中发挥作用。我们之前曾报道过,散发性乳腺癌组织的 H2AX 基因拷贝数发生了显著改变。然而,CNA 如何影响基因表达,以及 miR-24-2 等已知调节 H2AX 表达的 miR 在拷贝数变化的背景下发挥作用,目前尚不清楚。此外,许多 miR,包括 miR-24-2,被认为在细胞增殖和凋亡中发挥作用,但它们的特定靶基因和促成它们的途径仍未得到探索。
使用实时聚合酶链反应(PCR)测定法在两种哺乳动物细胞系 MCF-7 和 HeLa 以及一组散发性乳腺癌组织中估计基因拷贝数和 mRNA/miR 表达的变化。通过计算机分析寻找 miR-24-2 的假定靶标。用 miR-24-2 前体寡核苷酸转染 MCF-7 细胞,使用 TaqMan 基因表达测定法检测 BRCA1、BRCA2、ATM、MDM2、TP53、CHEK2、CYT-C、BCL-2、H2AFX 和 P21 的基因表达水平。通过使用膜联蛋白 V 染料的流式细胞术检测测量细胞凋亡。进行荧光素酶测定以确认 BCL-2 是 miR-24-2 的有效细胞靶标。
观察到 H2AX 基因表达与 miR-24-2 表达呈负相关,而与基因拷贝数状态不一致,无论是在细胞系还是在散发性乳腺癌肿瘤组织中。此外,观察到过表达 miR-24-2 的细胞对 DNA 损伤药物敏感,发生凋亡性细胞死亡,表明在接受抗癌药物治疗的人癌细胞系中,miR-24-2 介导的凋亡诱导具有增强作用。BCL-2 被确定为 miR-24-2 的新型细胞靶标。
miR-24-2 能够通过调节不同的凋亡途径和靶向 BCL-2(一种抗凋亡基因)来诱导细胞凋亡。该研究表明,miR-24-2 可以更有效地控制 H2AX 基因表达,而与基因拷贝数的变化无关。此外,该研究表明,miR-24-2 联合顺铂等抗癌药物的联合治疗可能为对药物有抗性的肿瘤患者的癌症治疗提供新途径。
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