Department of Microbiology and Immunology, University of British Columbia, Vancouver, BC, Canada.
Department of Cellular and Physiological Sciences, University of British Columbia, Vancouver, BC, Canada.
Front Immunol. 2020 Jan 30;11:29. doi: 10.3389/fimmu.2020.00029. eCollection 2020.
Alveolar macrophages (AMs) are CD44 expressing cells that reside in the alveolar space where they maintain lung homeostasis by serving critical roles in immunosurveillance and lipid surfactant catabolism. AMs lacking CD44 are unable to bind the glycosaminoglycan, hyaluronan, which compromises their survival and leads to reduced numbers of AMs in the lung. Using RNA sequencing, lipidomics and multiparameter flow cytometry, we demonstrate that CD44 mice have impaired AM lipid homeostasis and increased surfactant lipids in the lung. CD44 AMs had increased expression of CD36, a lipid scavenger receptor, as well as increased intracellular lipid droplets, giving them a foamy appearance. RNA sequencing revealed the differential expression of genes associated with lipid efflux and metabolism in CD44 AMs. Lipidomic analysis showed increased lipids in both the supernatant and cell pellet extracted from the bronchoalveolar lavage of CD44 mice. Phosphatidylcholine species, cholesterol, oxidized phospholipids and levels of reactive oxygen species (ROS) were increased in CD44 AMs. Oxidized phospholipids were more cytotoxic to CD44 AMs and induced greater lung inflammation in CD44 mice. Reconstitution of CD44 mice with CD44 bone marrow as well as adoptive transfer of CD44 AMs into CD44 mice showed that lipid accumulation in CD44 AMs occurred irrespective of the lung environment, suggesting a cell intrinsic defect. Administration of colony stimulating factor 2 (CSF-2), a critical factor in AM development and maintenance, increased AM numbers in CD44 mice and decreased phosphatidylcholine levels in the bronchoalveolar lavage, but was unable to decrease intracellular lipid accumulation in CD44 AMs. Peroxisome proliferator-activated receptor gamma (PPARγ), downstream of CSF-2 signaling and a regulator of lipid metabolism, was reduced in the nucleus of CD44 AMs, and PPARγ inhibition in normal AMs increased their lipid droplets. Thus, CD44 deficiency causes defects in AMs that lead to abnormal lipid accumulation and oxidation, which exacerbates oxidized lipid-induced lung inflammation. Collectively, these findings implicate CD44 as a regulator of lung homeostasis and inflammation.
肺泡巨噬细胞 (AMs) 是表达 CD44 的细胞,它们存在于肺泡空间中,通过在免疫监视和脂质表面活性剂代谢中发挥关键作用来维持肺内稳态。缺乏 CD44 的 AMs 无法结合糖胺聚糖透明质酸,从而影响其存活并导致肺部 AMs 数量减少。通过 RNA 测序、脂质组学和多参数流式细胞术,我们证明 CD44 敲除小鼠的 AM 脂质内稳态受损,肺表面活性剂脂质增加。CD44 AMs 表达上调了脂质清道夫受体 CD36,以及细胞内脂滴增加,使它们呈现泡沫状外观。RNA 测序揭示了 CD44 AMs 中与脂质外排和代谢相关的基因差异表达。脂质组学分析显示,CD44 敲除小鼠支气管肺泡灌洗液上清液和细胞沉淀中均有更多的脂质。CD44 AMs 中的磷酯酰胆碱种类、胆固醇、氧化型磷脂和活性氧 (ROS) 水平升高。氧化型磷脂对 CD44 AMs 的细胞毒性更大,并在 CD44 敲除小鼠中引起更大的肺部炎症。将 CD44 骨髓重新植入 CD44 敲除小鼠以及将 CD44 AMs 过继转移到 CD44 敲除小鼠中表明,CD44 AMs 中的脂质积累与肺部环境无关,提示存在细胞内在缺陷。集落刺激因子 2 (CSF-2) 是 AM 发育和维持的关键因子,CSF-2 给药可增加 CD44 敲除小鼠的 AM 数量并降低支气管肺泡灌洗液中的磷酯酰胆碱水平,但不能减少 CD44 AMs 中的细胞内脂质积累。CSF-2 信号下游的过氧化物酶体增殖物激活受体 γ (PPARγ) 是脂质代谢的调节因子,其在 CD44 AMs 的核内减少,而在正常 AMs 中抑制 PPARγ 则增加了它们的脂滴。因此,CD44 缺失导致 AMs 缺陷,导致异常脂质积累和氧化,从而加剧氧化脂质诱导的肺部炎症。综上所述,这些发现表明 CD44 是肺内稳态和炎症的调节因子。
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