Department of Anesthesiology, Perioperative and Pain Medicine, Center for Experimental Therapeutics and Reperfusion Injury, Mass General Brigham and Harvard Medical School, 60 Fenwood Rd., Hale Building for Transformative Medicine 3-016, Boston, MA, 02115, USA.
Mol Med. 2024 Sep 18;30(1):153. doi: 10.1186/s10020-024-00877-w.
Specialized pro-resolving mediators (SPMs) promote resolution of inflammation, clear infections and stimulate tissue regeneration. These include resolvins, protectins, and maresins. During self-resolving acute inflammation, SPMs are produced and have key functions activating endogenous resolution response for returning to homeostasis. Herein, we addressed whether infections initiated with ongoing inflammation alter resolution programs, and if low-dose repetitive SPM regimen re-programs the resolution response.
Inflammation was initiated with zymosan (1 mg/mouse) followed by E. coli (10 CFU/mouse) infections carried out in murine peritonitis, and exudates collected at 4-72 h. Leukocytes were enumerated using light microscopy, percentages of PMN, monocytes and macrophages were determined using flow cytometry, and resolution indices calculated. Lipid mediators and SPM profiles were established using mass spectrometry-based metabololipidomics. Repetitive dosing with a SPM panel consisting of RvD1, RvD2, RvD5, MaR1 and RvE2 (0.1 ng/mouse each, i.p.) was given to mice, followed by zymosan challenge. Leukocyte composition, resolution indices and RNA-sequencing were carried out for the repetitive SPM treatments.
E. coli infections initiated acute inflammation-resolution programs with temporal SPM production in the infectious exudates. Zymosan-induced inflammation prior to E. coli peritonitis shifted exudate resolution indices and delayed E. coli clearance. Lipid mediator metabololipidomics demonstrated that E. coli infection with ongoing zymosan-induced inflammation shifted the time course of exudate SPMs, activating a SPM cluster that included RvD1, RvD5 and MaR1 during the initiation phase of infectious inflammation (0-4 h); RvD5 and MaR1 were present also in the resolution phase (24-48 h). To emulate daily SPM regimens used in humans, a repetitive subthreshold dosing of the SPM panel RvD1, RvD2, RvD5, MaR1 and RvE2 each at 0.1 ng per mouse was administered. This low-dose SPM regimen accelerated exudate PMN clearance following zymosan-induced inflammation, and shortened the resolution interval by > 70%. These low-dose SPMs regulated genes and pathways related to immune response, chemokine clearance and tissue repair, as demonstrated by using RNA-sequencing.
Infections encountered during ongoing inflammation in mice reset the resolution mechanisms of inflammation via SPM clusters. Low-dose SPMs activate innate immune responses and pathways towards the resolution response that can be reprogrammed.
专门的促解决介质(SPM)可促进炎症消退、清除感染并刺激组织再生。这些包括 resolvins、protectins 和maresins。在自我解决的急性炎症中,会产生 SPM 并具有激活内源性解决反应以恢复平衡的关键功能。在此,我们研究了正在进行的炎症引发的感染是否会改变解决程序,以及低剂量重复 SPM 方案是否会重新编程解决反应。
使用酵母聚糖(1mg/只小鼠)引发炎症,随后用大肠杆菌(10 CFU/只小鼠)感染进行小鼠腹膜炎,并在 4-72 小时收集渗出物。使用相差显微镜计数白细胞,使用流式细胞术确定PMN、单核细胞和巨噬细胞的百分比,并计算解决指数。使用基于质谱的代谢脂质组学确定脂质介质和 SPM 谱。给小鼠重复给予由 RvD1、RvD2、RvD5、MaR1 和 RvE2 组成的 SPM 组(每只 0.1ng/只,腹腔内注射),然后用酵母聚糖进行挑战。进行白细胞组成、解决指数和 RNA 测序,以进行重复 SPM 治疗。
大肠杆菌感染引发了急性炎症-解决程序,在感染性渗出物中产生了时间依赖性的 SPM。在大肠杆菌腹膜炎之前用酵母聚糖引发的炎症改变了渗出物的解决指数并延迟了大肠杆菌的清除。脂质介质代谢脂质组学表明,大肠杆菌感染伴持续酵母聚糖诱导的炎症改变了渗出物 SPM 的时间过程,激活了 SPM 簇,包括 RvD1、RvD5 和 MaR1,在感染性炎症的启动阶段(0-4 小时);RvD5 和 MaR1 也存在于解决阶段(24-48 小时)。为了模拟人类每日 SPM 方案,以 0.1ng/只小鼠的剂量重复给予 SPM 组 RvD1、RvD2、RvD5、MaR1 和 RvE2。这种低剂量 SPM 方案加速了酵母聚糖诱导的炎症后渗出物 PMN 的清除,并将解决间隔缩短了超过 70%。这些低剂量 SPM 通过 RNA 测序调节了与免疫反应、趋化因子清除和组织修复相关的基因和途径。
在小鼠正在进行的炎症中遇到的感染通过 SPM 簇重置了炎症的解决机制。低剂量 SPM 激活了先天免疫反应和解决反应的途径,可以对其进行重新编程。
Zotero 插件