自分泌小细胞外囊泡通过miR-21-5p诱导糖尿病肾病中的肾小管表型转化。

Autocrine small extracellular vesicles induce tubular phenotypic transformation in diabetic nephropathy via miR-21-5p.

作者信息

Zhang Mengting, Lu Yukang, Wang Lanfeng, Mao Yiping, Hu Xinyi, Chen Zhiping

机构信息

Laboratory Medicine, Wuhu Hospital of Traditional Chinese Medicine, Wuhu, Anhui Province 241000, China.

Laboratory Medicine, First Affiliated Hospital of Gannan Medical University, Ganzhou, Jiangxi Province 341000, China; The First School of Clinical Medicine, Gannan Medical University, Ganzhou, Jiangxi Province 341000, China.

出版信息

Gene. 2025 Feb 20;938:149156. doi: 10.1016/j.gene.2024.149156. Epub 2024 Dec 7.

DOI:10.1016/j.gene.2024.149156

PMID:39653091

Abstract

BACKGROUND

Diabetic nephropathy (DN) is one of the most common and serious microvascular complications associated with diabetes. DN is the leading contributor to the majority of cases of end-stage renal disease (ESRD). Small extracellular vesicles (sEVs) can transport various genetic materials to recipient cells. The objective of this study was to explore how sEVs released from HK-2 cells when stimulated by high glucose levels influence renal tubular phenotypic transformation through miR-21-5p.

METHODS

Both human and cell studies were utilized to explore the crosstalk between proximal renal tubules in DN. sEVs from plasma and cells were isolated using ultracentrifugation, and the differential expression of miR-21-5p in plasma sEVs from DN patients versus healthy controls was quantified using Quantitative Real-time PCR (RT-qPCR). A DN model was constructed by stimulating HK-2 cells with glucose. The expression of epithelial-mesenchymal transition (EMT) proteins in each cell group was analyzed by Western Blot (WB), while miR-21-5p levels in both cells and their sEVs were quantified using RT-qPCR. A stable transfected HK-2 cell line was constructed. The CCK8 assay, scratch assay, and WB were employed to detect EMT proteins, aiming to explore how autocrine sEVs affect tubular phenotypic transformation in diabetic nephropathy (DN).

RESULTS

The expression of miR-21-5p in plasma sEVs was significantly elevated in the DN group compared to the healthy control group. High glucose (HG) stimulation of HK-2 cells resulted in higher miR-21-5p expression in both cells and their sEVs, leading to enhanced proliferation, migration, and EMT capacities in these cells. Co-incubation of HK-2 cells with HG-sEVs significantly enhanced the proliferation, migration, and EMT capabilities of the recipient cells, but miR-21-5p knockdown reversed these effects.

CONCLUSION

These results indicate that high glucose stimulates HK-2 cells to secrete sEVs, which promote DN proliferation, migration, and EMT through miR-21-5p, thereby offering new insights into the treatment of DN.

摘要

背景

糖尿病肾病（DN）是糖尿病最常见且严重的微血管并发症之一。DN是大多数终末期肾病（ESRD）病例的主要病因。小细胞外囊泡（sEVs）可将各种遗传物质转运至受体细胞。本研究的目的是探讨高糖水平刺激下HK-2细胞释放的sEVs如何通过miR-21-5p影响肾小管表型转化。

方法

采用人体和细胞研究来探究DN中近端肾小管之间的相互作用。通过超速离心法分离血浆和细胞中的sEVs，并使用定量实时聚合酶链反应（RT-qPCR）对DN患者与健康对照者血浆sEVs中miR-21-5p的差异表达进行定量。通过用葡萄糖刺激HK-2细胞构建DN模型。采用蛋白质免疫印迹法（WB）分析各细胞组中上皮-间质转化（EMT）蛋白的表达，同时使用RT-qPCR对细胞及其sEVs中的miR-21-5p水平进行定量。构建稳定转染的HK-2细胞系。采用CCK8检测法、划痕实验和WB检测EMT蛋白，旨在探究自分泌sEVs如何影响糖尿病肾病（DN）中的肾小管表型转化。

结果

与健康对照组相比，DN组血浆sEVs中miR-21-5p的表达显著升高。高糖（HG）刺激HK-2细胞导致细胞及其sEVs中miR-21-5p表达升高，从而增强这些细胞的增殖、迁移和EMT能力。HK-2细胞与HG-sEVs共同孵育显著增强了受体细胞的增殖、迁移和EMT能力，但miR-21-5p敲低可逆转这些作用。