溶血性磷脂酸受体 3 缺乏可减少低氧小鼠肾脏中促红细胞生成素的产生。
Deficiency of lysophosphatidic acid receptor 3 decreases erythropoietin production in hypoxic mouse kidneys.
机构信息
The Key Laboratory of Cell Proliferation and Regulation Biology, Ministry of Education, Department of Biology, College of Life Sciences, Beijing Normal University, Beijing, 100875, China.
State Key Laboratory of Cardiovascular Disease, Fuwai Hospital, National Center for Cardiovascular Diseases, Chinese Academy of Medical Sciences and Peking Union Medical College, Beijing, China.
出版信息
Lipids Health Dis. 2024 Nov 18;23(1):381. doi: 10.1186/s12944-024-02367-8.
BACKGROUND
Lysophosphatidic acid (LPA) is a lipid mediator with diverse biological functions through its receptors on the cell membrane. As one of the six LPA receptors, LPA receptor 3 (LPAR3) is highly expressed in mouse kidneys, but its physiological function in the kidney has been poorly explored.
METHODS
Wild-type (WT) and Lpar3 mice were used to investigate the renal physiological function of LPAR3 under hypoxia. The expression levels of LPA receptors in the kidneys of WT mice with or without exposure to hypoxia (8% O) were detected by RT‒qPCR. RNA sequencing analysis was performed to identify differences in gene expression profiles between the hypoxic kidneys of WT and Lpar3 mice. The effects of LPAR3 deficiency and treatment with the LPAR1/3 inhibitor Ki16425 or the LPAR3 selective agonist 2S-OMPT on erythropoietin (EPO) production in the kidneys of hypoxic mice were determined by RT‒qPCR and ELISAs. The mechanism of LPAR3-mediated regulation of EPO expression was further studied in vivo with mouse models and in vitro with cultured human cells.
RESULTS
LPAR3 is the major LPA receptor in mouse kidneys, and its expression is significantly upregulated under hypoxic conditions. RNA sequencing analysis revealed that, compared with WT mice, Lpar3 mice presented a significant decrease in hypoxia-induced EPO expression in the kidney, together with reduced plasma EPO levels and lower hematocrit and hemoglobin levels. Hypoxic renal EPO expression in WT mice was diminished by the administration of the LPAR1/3 inhibitor Ki16425 and increased by 2S-OMPT, a selective agonist of LPAR3. Hypoxia-induced HIF-2α accumulation in mouse kidneys was impaired by LPAR3 deficiency. Further studies revealed that the PI3K/Akt pathway participated in the regulation of HIF-2α accumulation and EPO expression by LPAR3 under hypoxic conditions.
CONCLUSIONS
Our study revealed the role of LPAR3 in promoting the HIF-2α‒EPO axis in hypoxic mouse kidneys, suggesting that the LPA receptor may serve as a novel potential pharmaceutical target to regulate renal EPO production in hypoxia-related situations, such as chronic kidney disease and altitude disease.
背景
溶血磷脂酸 (LPA) 是一种通过细胞膜上的受体发挥多种生物学功能的脂质介质。作为六种 LPA 受体之一,LPA 受体 3 (LPAR3) 在小鼠肾脏中高度表达,但它在肾脏中的生理功能尚未得到充分探索。
方法
使用野生型 (WT) 和 Lpar3 小鼠研究 LPAR3 在缺氧下对肾脏的生理功能。通过 RT-qPCR 检测 WT 小鼠在缺氧(8% O2)暴露或不暴露时肾脏中 LPA 受体的表达水平。对 WT 和 Lpar3 小鼠缺氧肾脏的基因表达谱进行 RNA 测序分析,以确定差异。通过 RT-qPCR 和 ELISA 检测 LPAR3 缺失以及 LPAR1/3 抑制剂 Ki16425 或 LPAR3 选择性激动剂 2S-OMPT 处理对缺氧小鼠肾脏中促红细胞生成素 (EPO) 产生的影响。在体内小鼠模型和体外培养的人细胞中进一步研究 LPAR3 介导的 EPO 表达调控的机制。
结果
LPAR3 是小鼠肾脏中主要的 LPA 受体,其表达在缺氧条件下显著上调。RNA 测序分析显示,与 WT 小鼠相比,Lpar3 小鼠在肾脏中缺氧诱导的 EPO 表达显著减少,同时伴有血浆 EPO 水平降低、红细胞压积和血红蛋白水平降低。WT 小鼠给予 LPAR1/3 抑制剂 Ki16425 可减弱缺氧诱导的肾脏 EPO 表达,而 LPAR3 的选择性激动剂 2S-OMPT 则增加其表达。LPAR3 缺失可损害缺氧诱导的小鼠肾脏中 HIF-2α 的积累。进一步研究表明,PI3K/Akt 通路参与 LPAR3 调节缺氧条件下 HIF-2α 积累和 EPO 表达。
结论
本研究揭示了 LPAR3 在促进缺氧小鼠肾脏中 HIF-2α-EPO 轴中的作用,提示 LPA 受体可能成为一种新型潜在药物靶点,用于调节缺氧相关情况下(如慢性肾脏病和高原病)肾脏 EPO 的产生。
Zotero 插件