Endothelial-derived small extracellular vesicles support B-cell acute lymphoblastic leukemia development.

IF 4.9 2区 医学 Q2 CELL BIOLOGY
Cellular Oncology Pub Date : 2024-02-01 Epub Date: 2023-09-26 DOI:10.1007/s13402-023-00855-0
Dan Huang, Yamin Yuan, Liyuan Cao, Difan Zhang, Yu Jiang, Yaping Zhang, Chiqi Chen, Zhuo Yu, Li Xie, Yujuan Wei, Jiangbo Wan, Junke Zheng
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引用次数: 0

Abstract

Purpose: The bone marrow niche plays an important role in leukemia development. However, the contributions of different niche components to leukemia development and their underlying mechanisms remain largely unclear.

Method: Cre/LoxP-based conditional knockout technology was used to delete VPS33B or ANGPTL2 gene in niche cells. Murine B-ALL model was established by overexpressing the N-Myc oncogene in hematopoietic stem progenitor cells. The frequency of leukemia cells and immunophenotypic B220+ CD43+ LICs was detected by flow cytometry. SEVs was isolated by sequential centrifugation and mass spectrometry was performed to analyze the different components of SEVs. Immunoprecipitation and western blot were used to measure the interaction of VPS33B and ANGPTL2.

Results: Here, we showed that specific knockout of vascular protein sorting 33b (Vps33b) in endothelial cells (ECs), but not megakaryocytes or mesenchymal stem cells, resulted in a significant decrease in the secretion of small extracellular vesicles (SEVs) and a delay in the development of B-cell lymphoblastic leukemia (B-ALL). Vps33b knockdown endothelial cells contained much lower levels of SEVs that contained angiopoietin-like protein 2 (ANGPTL2) than the control cells. Importantly, conditional knockout of Angptl2 in ECs significantly delayed B-ALL progression. Moreover, C-terminal region of ANGPTL2 (aa247-471) could directly interact with Sec1-like domain 1 of VPS33B (aa1-aa146). We further demonstrated that the point mutations R399H and G402S in ANGPTL2 led to a dramatic decrease in the secretion of ANGPTL2-SEVs. We also showed that wild-type ANGPTL2-containing SEVs, but not mutant ANGPTL2-containing SEVs, significantly enhanced B-ALL development.

Conclusion: In summary, our findings indicate that the secretion of ANGPTL2-containing SEVs in ECs sustains the leukemogenic activities of B-ALL cells, which is fine-tuned by the direct interaction of VPS33B and ANGPTL2. These findings reveal that niche-specific SEVs play an important role in B-ALL development.

Abstract Image

内皮细胞衍生的细胞外小泡支持B细胞急性淋巴细胞白血病的发展。
目的:骨髓生态位在白血病的发生发展中起着重要作用。然而,不同生态位成分对白血病发展的贡献及其潜在机制在很大程度上仍不清楚。方法:采用基于Cre/LoxP的条件敲除技术,对小生境细胞中的VPS33B或ANGPTL2基因进行敲除。通过在造血干祖细胞中过表达N-Myc癌基因建立小鼠B-ALL模型。流式细胞仪检测白血病细胞和免疫表型B220+CD43+LICs的频率。通过顺序离心分离SEV,并进行质谱分析来分析SEV的不同成分。免疫沉淀和蛋白质印迹法检测了VPS33B和ANGPTL2的相互作用。结果:我们发现,血管蛋白分选33b(VPS33B)在内皮细胞(EC)中的特异性敲除,而在巨核细胞或间充质干细胞中没有,导致细胞外小泡(SEVs)的分泌显著减少,并延迟B细胞淋巴细胞白血病(B-ALL)的发展。Vps33b敲低的内皮细胞含有比对照细胞低得多的含有血管生成素样蛋白2(ANGPTL2)的SEV水平。重要的是,ECs中Angptl2的条件性敲除显著延迟了B-ALL的进展。此外,ANGPTL2的C末端区域(aa247-471)可以直接与VPS33B的Sec1样结构域1(aa1-aa146)相互作用。我们进一步证明,ANGPTL2中的点突变R399H和G402S导致ANGPTL2 SEVs的分泌显著减少。我们还发现,含有SEVs的野生型ANGPTL2,而不是含有SEVss的突变体ANGPTL2显著增强了B-ALL的发育。结论:总之,我们的研究结果表明,内皮细胞中含有ANGPTL2的SEVs的分泌维持了B-ALL细胞的致白血病活性,而VPS33B和ANGPTL2之间的直接相互作用对其进行了微调。这些发现表明,小众特异性SEV在B-ALL的发展中起着重要作用。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
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来源期刊
Cellular Oncology
Cellular Oncology ONCOLOGY-CELL BIOLOGY
CiteScore
10.30
自引率
1.50%
发文量
86
审稿时长
12 months
期刊介绍: The Official Journal of the International Society for Cellular Oncology Focuses on translational research Addresses the conversion of cell biology to clinical applications Cellular Oncology publishes scientific contributions from various biomedical and clinical disciplines involved in basic and translational cancer research on the cell and tissue level, technical and bioinformatics developments in this area, and clinical applications. This includes a variety of fields like genome technology, micro-arrays and other high-throughput techniques, genomic instability, SNP, DNA methylation, signaling pathways, DNA organization, (sub)microscopic imaging, proteomics, bioinformatics, functional effects of genomics, drug design and development, molecular diagnostics and targeted cancer therapies, genotype-phenotype interactions. A major goal is to translate the latest developments in these fields from the research laboratory into routine patient management. To this end Cellular Oncology forms a platform of scientific information exchange between molecular biologists and geneticists, technical developers, pathologists, (medical) oncologists and other clinicians involved in the management of cancer patients. In vitro studies are preferentially supported by validations in tumor tissue with clinicopathological associations.
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