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长链非编码 RNA ARAP1-AS1 通过靶向 miR-516b-5p/PDE5A 轴促进甲状腺癌的进展。

LncRNA ARAP1-AS1 targets miR-516b-5p/PDE5A axis to facilitate the progression of thyroid cancer.

机构信息

Department of Thyroid and Breast Surgery.

Department of Oncology.

出版信息

Anticancer Drugs. 2023 Jul 1;34(6):735-746. doi: 10.1097/CAD.0000000000001438. Epub 2022 Nov 17.

DOI:10.1097/CAD.0000000000001438
PMID:36730555
Abstract

Thyroid cancer (TC) remains a prevalent public health concern. To further study the molecular mechanism of TC development, we explored the regulatory mechanism and function of lncRNA ARAP1-AS1 in TC progression. The verification of ARAP1-AS1, PDE5A and miR-516b-5p expression levels among the TC cell lines and tissues was fulfilled via RT-qPCR and western blot analyses. Cell Counting Kit-8 and colony formation experiments were executed to assess ARAP1-AS1's biological function in vitro. Western blotting was conducted to assess apoptosis through the expressions of apoptotic markers. A tumor xenograft experiment was conducted to evaluate whether ARAP1-AS1 affected TC tumor development in vivo . The interactions of miR-516b-5p with ARAP1-AS1 and PDE5A were explored through a dual-luciferase reporter and RNA Binding Protein Immunoprecipitation assays, as well as through Pearson's correlation analysis. ARAP1-AS1 and PDE5A were evidently upregulated in the TC cell lines and tissues whereas miR-516b-5p was poorly expressed. ARAP1-AS1 silencing in TC cells hampered cell proliferation, reduced their viability and boosted apoptosis. Moreover, it inhibited tumor growth in vivo . ARAP1-AS1 had been revealed to be correlated negatively to miR-516b-5p. Finally, we demonstrated that the miR-516b-5p inhibitor was capable of reversing ARAP1-AS1-knockdown's repressive effects on TC cell development by means of regulating PDE5A expression. ARAP1-AS1 partially facilitated TC cell development and survival through the modulation of miR-516b-5p/PDE5A axis. This contributes a novel biomarker and new perspectives for TC treatment.

摘要

甲状腺癌(TC)仍然是一个普遍存在的公共卫生问题。为了进一步研究 TC 发展的分子机制,我们探讨了 lncRNA ARAP1-AS1 在 TC 进展中的调控机制和功能。通过 RT-qPCR 和 Western blot 分析验证了 TC 细胞系和组织中 ARAP1-AS1、PDE5A 和 miR-516b-5p 的表达水平。通过细胞计数试剂盒-8 和集落形成实验评估了 ARAP1-AS1 在体外的生物学功能。通过凋亡标志物的表达评估了 Western blot 分析的细胞凋亡情况。进行肿瘤异种移植实验以评估 ARAP1-AS1 是否影响 TC 肿瘤在体内的发展。通过双荧光素酶报告和 RNA 结合蛋白免疫沉淀测定以及 Pearson 相关分析探讨了 miR-516b-5p 与 ARAP1-AS1 和 PDE5A 的相互作用。在 TC 细胞系和组织中,ARAP1-AS1 和 PDE5A 明显上调,而 miR-516b-5p 表达水平较低。在 TC 细胞中沉默 ARAP1-AS1 会阻碍细胞增殖,降低细胞活力并促进细胞凋亡。此外,它还抑制了体内肿瘤的生长。ARAP1-AS1 与 miR-516b-5p 呈负相关。最后,我们证明 miR-516b-5p 抑制剂能够通过调节 PDE5A 表达逆转 ARAP1-AS1 敲低对 TC 细胞发育的抑制作用。ARAP1-AS1 通过调节 miR-516b-5p/PDE5A 轴部分促进 TC 细胞的发育和存活。这为 TC 治疗提供了一个新的生物标志物和新视角。

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