核糖体蛋白L36介导的微小RNA-4432选择性装载到细胞外囊泡中,导致静脉畸形中血管周围细胞功能障碍。
Ribosomal protein L36-mediated selective loading of microRNA-4432 into extracellular vesicles contributes to perivascular cell dysfunction in venous malformations.
作者信息
Chen Gao-Hong, Ren Jian-Gang, Xia Hou-Fu, Zhang He-Jing, Wang Kui-Ming, Zhang Lin-Zhou, Chen Gang
机构信息
State Key Laboratory of Oral and Maxillofacial Reconstruction and Regeneration, Key Laboratory of Oral Biomedicine Ministry of Education, Hubei Key Laboratory of Stomatology, School and Hospital of Stomatology, Wuhan University, Wuhan, China.
Department of Oral and Maxillofacial Surgery, School and Hospital of Stomatology, Wuhan University, Wuhan, China.
出版信息
Br J Dermatol. 2025 Mar 18;192(4):717-727. doi: 10.1093/bjd/ljae492.
BACKGROUND
Venous malformations (VMs), predominantly arising from activating mutations of TIE2 in endothelial cells (ECs), are characterized by dilated and tortuous vessels with a paucity of perivascular cells (PCs). The mechanisms of interaction between mutant ECs and PCs remain largely elusive.
OBJECTIVES
To investigate the characteristics of extracellular vesicles (EVs) from VM ECs, especially the microRNAs (miRNAs) carried and their roles in crosstalk between ECs and PCs in VM pathogenesis.
METHODS
miRNA profiles of human umbilical vein endothelial cells overexpressing TIE2L914F (L914F cells) and TIE2WT [wildtype (WT) cells], along with their EVs, were analysed by RNA sequencing. In vitro studies using umbilical cord stem cells (UCSCs) were done to carry out functional assays of VM EVs and their enriched miRNA-4432 (miR-4432). miRNA pulldown and RNA interference techniques were used to identify the sorting regulator of miR-4432 into VM EVs.
RESULTS
RNA secretion was upregulated in L914F EVs vs. WT EVs. miRNA sequencing revealed a distinct profile of L914F EVs vs. L914F cells, WT cells and WT EVs, identifying miR-4432 as being preferentially encapsulated in EVs from L914F cells. Functional assays demonstrated that VM EVs and EV-carried miR-4432 inhibited the differentiation, adhesion and proliferation of UCSCs. Furthermore, ribosomal protein L36 (RPL36) was identified as an RNA binding protein and sorting regulator of miR-4432 during the EV secretion process in L914F cells.
CONCLUSIONS
This study, for the first time, identified an interaction between VM ECs and PCs via EVs, and offers valuable data on the miRNA profiles of VM ECs and normal ECs, along with their EVs. Our findings suggest that the RPL36-mediated selective loading of miR-4432 into EVs may contribute to the aberrant PC coverage in VMs, providing novel insights into VM pathogenesis and potential treatment strategies.
背景
静脉畸形(VMs)主要由内皮细胞(ECs)中TIE2的激活突变引起,其特征为血管扩张和迂曲,周围血管细胞(PCs)稀少。突变ECs与PCs之间的相互作用机制仍不清楚。
目的
研究VM ECs来源的细胞外囊泡(EVs)的特征,特别是其中携带的微小RNA(miRNAs)及其在VM发病机制中ECs与PCs相互作用中的作用。
方法
通过RNA测序分析过表达TIE2L914F(L914F细胞)和TIE2WT[野生型(WT)细胞]的人脐静脉内皮细胞及其EVs的miRNA谱。利用脐带干细胞(UCSCs)进行体外研究,以对VM EVs及其富集的miRNA-4432(miR-4432)进行功能分析。采用miRNA下拉和RNA干扰技术鉴定miR-4432进入VM EVs的分选调节因子。
结果
与WT EVs相比,L914F EVs中的RNA分泌上调。miRNA测序揭示了L914F EVs与L914F细胞、WT细胞和WT EVs的不同谱,确定miR-4432优先包裹在L914F细胞来源的EVs中。功能分析表明,VM EVs和EV携带的miR-4432抑制UCSCs的分化、黏附和增殖。此外核糖体蛋白L36(RPL36)被鉴定为L914F细胞EV分泌过程中miR-4432的RNA结合蛋白和分选调节因子。
结论
本研究首次确定了VM ECs与PCs通过EVs相互作用,并提供了有关VM ECs和正常ECs及其EVs的miRNA谱的有价值数据。我们的研究结果表明,RPL36介导的miR-4432选择性加载到EVs中可能导致VM中PC覆盖异常,为VM发病机制和潜在治疗策略提供了新见解。
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