Mechanism study of serum extracellular nano-vesicles miR-412-3p targeting regulation of TEAD1 in promoting malignant biological behavior of sub-centimeter lung nodules.

IF 4.6 Q2 MATERIALS SCIENCE, BIOMATERIALS

ACS Applied Bio Materials Pub Date : 2024-08-23 DOI:10.3233/cbm-240137

Yuxia Deng,Nishant Patel,Shuang Ding,Haijun Zhang

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Abstract

OBJECTIVE To investigate the impact and potential mechanisms of serum extracellular nano-vesicles (sEVs) miR-412-3p released from sub-centimeter lung nodules with a diameter of ⩽ 10 mm on the malignant biological function of micro-nodular lung cancer (mnLC). METHODS A total of 87 participants were included and divided into a mnLC group (n= 30), a benign lung nodule (BLN) group (n= 27), and a healthy people control group (n= 30). Transmission electron microscopy (TEM), nanoparticle tracking analysis (NTA) and Western blot (WB) were used to measure the morphological characteristics and surface markers of sEVs. In vitro analysis, real-time quantitative polymerase chain reaction (RT-qPCR), CCK-8 cell proliferation assay, clone formation assay, Transwell, stem cell sphere-forming assay, and WB assay were conducted to verify the effect of miR-412-3p/TEAD1 signaling axis on the biological function of lung cancer cells through, respectively. Further validation was conducted using the serum sEVs of the participants. RESULTS The expression level of sEVs-miR-412-3p in the mnLC group was significantly higher than that in the BLN and healthy groups (P< 0.01). In lung cancer cell lines, miR-412-3p can negatively regulate the targeted gene TEAD1. The miR-412-3p/TEAD1 signaling axis is involved in promoting the EMT signaling pathway and regulating the malignant biological functions of lung cancer cell proliferation, migration, and stemness (P< 0.05). In addition, sEVs in the mnLC group significantly promoted lung cancer cell proliferation, migration, and stemness compared to the BLN and healthy groups, inhibited the expression of E-cadherin and TEAD1 in lung cancer cells, and promoted the expression of N-cadherin and Vimentin (P< 0.05). CONCLUSION sEVs-miR-412-3p could promote the biological process of EMT, and lead to the occurrence of malignant biological behavior in sub-centimeter lung nodules. This provides evidence for the miR-412-3p/TEAD1 signaling axis as a potential therapeutic target for mnLC.

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血清细胞外纳米载体 miR-412-3p 靶向调控 TEAD1 促进厘米以下肺结节恶性生物学行为的机制研究

目的研究直径⩽ 10 mm的亚厘米肺结节释放的血清细胞外纳米载体（sEVs）miR-412-3p对微结节性肺癌（mnLC）恶性生物学功能的影响和潜在机制。方法共纳入 87 名参与者，分为微小结节肺癌组（30 人）、良性肺结节组（27 人）和健康人对照组（30 人）。透射电子显微镜（TEM）、纳米颗粒追踪分析（NTA）和 Western 印迹（WB）用于测量 sEVs 的形态特征和表面标记物。在体外分析中，通过实时定量聚合酶链反应（RT-qPCR）、CCK-8细胞增殖试验、克隆形成试验、Transwell、干细胞球形成试验和WB试验分别验证了miR-412-3p/TEAD1信号轴对肺癌细胞生物学功能的影响。结果mnLC组sEVs-miR-412-3p的表达水平明显高于BLN组和健康组（P< 0.01）。在肺癌细胞系中，miR-412-3p 能负向调节靶基因 TEAD1。miR-412-3p/TEAD1信号轴参与促进EMT信号通路，调控肺癌细胞增殖、迁移和干性等恶性生物学功能（P< 0.05）。此外，与 BLN 组和健康组相比，mnLC 组中的 sEVs 能显著促进肺癌细胞的增殖、迁移和干性，抑制肺癌细胞中 E-cadherin 和 TEAD1 的表达，促进 N-cadherin 和 Vimentin 的表达（P< 0.05）。这为 miR-412-3p/TEAD1 信号轴作为 mnLC 的潜在治疗靶点提供了证据。

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来源期刊

ACS Applied Bio Materials Chemistry-Chemistry (all)

CiteScore

9.40

自引率

2.10%

发文量

464