ANGPTL2-containing small extracellular vesicles from vascular endothelial cells accelerate leukemia progression

白血病 细胞生物学 细胞外 胞外囊泡 细胞外小泡 微泡 内皮干细胞 化学 癌症研究 生物 血管生成 内皮 小泡 脐静脉 微泡 肿瘤微环境
作者
Dan Huang,Guohuan Sun,Xiaoxin Hao,Xiaoxiao He,Zhaofeng Zheng,Chiqi Chen,Zhuo Yu,Li Xie,Shihui Ma,Ligen Liu,Bo O. Zhou,Hui Cheng,Junke Zheng,Tao Cheng
出处
期刊:Journal of Clinical Investigation [American Society for Clinical Investigation]
卷期号:131 (1) 被引量:7
标识
DOI:10.1172/jci138986
摘要

Small extracellular vesicles (SEVs) are functional messengers of certain cellular niches that permit noncontact cell communications. Whether niche-specific SEVs fulfill this role in cancer is unclear. Here, we used 7 cell type-specific mouse Cre lines to conditionally knock out Vps33b in Cdh5+ or Tie2+ endothelial cells (ECs), Lepr+ BM perivascular cells, Osx+ osteoprogenitor cells, Pf4+ megakaryocytes, and Tcf21+ spleen stromal cells. We then examined the effects of reduced SEV secretion on progression of MLL-AF9-induced acute myeloid leukemia (AML), as well as normal hematopoiesis. Blocking SEV secretion from ECs, but not perivascular cells, megakaryocytes, or spleen stromal cells, markedly delayed the leukemia progression. Notably, reducing SEV production from ECs had no effect on normal hematopoiesis. Protein analysis showed that EC-derived SEVs contained a high level of ANGPTL2, which accelerated leukemia progression via binding to the LILRB2 receptor. Moreover, ANGPTL2-SEVs released from ECs were governed by VPS33B. Importantly, ANGPTL2-SEVs were also required for primary human AML cell maintenance. These findings demonstrate a role of niche-specific SEVs in cancer development and suggest targeting of ANGPTL2-SEVs from ECs as a potential strategy to interfere with certain types of AML.
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