Huang Guodong, Liu Yuxia, Li Lisha, Li Bing, Jiang Ting, Cao Yufeng, Yang Xiaoping, Liu Xinning, Qu Honglin, Li Shitao, Zheng Xin
Central Laboratory, Qingdao Hiser Hospital Affiliated of Qingdao University (Qingdao Hospital of Traditional Chinese Medicine), Qingdao, Shandong, China.
Department of Respiration, Second Affiliated Hospital of Shandong University of Traditional Chinese Medicine, Jinan, Shandong, China.
Front Oncol. 2024 Dec 17;14:1508715. doi: 10.3389/fonc.2024.1508715. eCollection 2024.
Lung adenocarcinoma (LUAD) poses a significant therapeutic challenge, primarily due to delayed diagnosis and the limited efficacy of existing treatments.
To understand the pathogenesis and identify diagnostic biomarkers for LUAD in the early stage, we investigated differential miRNA expression in 33 stage I LUAD patients between tumor and matched paracancerous tissues by Illumina Sequencing. Target genes of differentially expressed miRNAs were predicted using TargetScan and miRDB databases and further analyzed by GO and KEGG pathway enrichment analysis. The miRNAs expression results were verified using qRT-PCR. Additionally, we evaluated the clinical significance of miRNAs by the TCGA database. miR-183-3p was chosen for subsequent biological functional studies by cell proliferation assays, cell migration and cell invasion assays, cell apoptosis and cell cycle assays in LUAD cells. The clinical relevance target genes of miR-183-3p were predicted by TargetScan databases and bioinformatics assays. Gene-specific experimental validation was performed using qRT-PCR, western blotting and luciferase reporter assays.
We identified 36 differentially expressed miRNAs between LUAD tissues and matched paracancerous tissues. Target genes for these miRNAs revealed associations with processes and pathways such as RNA biosynthesis, intracellular signaling, protein transport, and the Ras, MAPK, and PI3K-AKT pathways. The qRT-PCR results were in alignment with the sequencing data for 19 out of these 21 miRNAs which not yet implicated in LUAD, 13 were up-regulated, 6 were down-regulated. The clinical relevance assays showed that 5 up-regulated miRNAs have diagnostic value for LUAD. miR-183-3p showed significant advantages in the result of sequencing, qRT-PCR, and clinical relevance assay. Biological functional assays showed that miR-183-3p emerged as a key regulator, promoting LUAD cell proliferation, decreasing apoptosis, and augmenting migration and invasion capabilities. The clinical relevance assays and experimental validation showed SESN1 as a clinical significance target of miR-183-3p.
Our study lays the foundation for investigating miRNAs with diagnostic significance in early-stage LUAD, pointing out that inhibition of miR-183-3p may serve as a novel therapeutic in LUAD.
肺腺癌(LUAD)带来了重大的治疗挑战,主要是由于诊断延迟以及现有治疗方法疗效有限。
为了解LUAD的发病机制并鉴定早期诊断生物标志物,我们通过Illumina测序研究了33例I期LUAD患者肿瘤组织与配对癌旁组织中miRNA的差异表达。使用TargetScan和miRDB数据库预测差异表达miRNA的靶基因,并通过GO和KEGG通路富集分析进一步分析。使用qRT-PCR验证miRNA表达结果。此外,我们通过TCGA数据库评估了miRNA的临床意义。通过LUAD细胞的细胞增殖试验、细胞迁移和细胞侵袭试验、细胞凋亡和细胞周期试验,选择miR-183-3p进行后续生物学功能研究。通过TargetScan数据库和生物信息学分析预测miR-183-3p的临床相关靶基因。使用qRT-PCR、蛋白质免疫印迹和荧光素酶报告基因试验进行基因特异性实验验证。
我们鉴定出LUAD组织与配对癌旁组织之间有36种差异表达的miRNA。这些miRNA的靶基因显示与RNA生物合成、细胞内信号传导、蛋白质运输以及Ras、MAPK和PI3K-AKT通路等过程和途径相关。在这21种尚未与LUAD相关的miRNA中,qRT-PCR结果与19种的测序数据一致,其中13种上调,6种下调。临床相关性分析表明,5种上调的miRNA对LUAD具有诊断价值。miR-183-3p在测序、qRT-PCR和临床相关性分析结果中显示出显著优势。生物学功能分析表明,miR-183-3p是一个关键调节因子,可促进LUAD细胞增殖,减少细胞凋亡,并增强迁移和侵袭能力。临床相关性分析和实验验证表明SESN1是miR-183-3p的临床意义靶标。
我们的研究为研究早期LUAD中具有诊断意义的miRNA奠定了基础,指出抑制miR-183-3p可能成为LUAD的一种新治疗方法。
