Department of Pathophysiology, Anhui Medical University, Hefei 230000, China.
The First Clinical Medical College, Anhui Medical University, Hefei 230000, China.
J Immunol Res. 2021 Dec 30;2021:8356645. doi: 10.1155/2021/8356645. eCollection 2021.
Sepsis is an organ dysfunction caused by the dysregulated inflammatory response to infection. Lipopolysaccharide-binding protein (LBP) binds to lipopolysaccharide (LPS) and modulates the inflammatory response. A rare systematic study has been reported to detect the effect of LBP gene during LPS-induced sepsis. Herein, we explored the RNA sequencing technology to profile the transcriptomic changes in liver tissue between LBP-deficient rats and WT rats at multiple time points after LPS administration. We proceeded RNA sequencing of liver tissue to search differentially expressed genes (DEGs) and enriched biological processes and pathways between WT and LBP-deficient groups at 0 h, 6 h, and 24 h. In total, 168, 284, and 307 DEGs were identified at 0 h, 6 h, and 24 h, respectively, including , , , , , and , which are related to the inflammatory or lipid-related process. Functional enrichment analysis revealed that inflammatory response to LPS mediated by , , , and was enhanced at 6 h, while lipid-related metabolism associated with , , and was enriched at 24 h after LPS administration in the WT samples. The inflammatory process was not found when the LBP gene was knocked out; lipid-related metabolic process and peroxisome proliferator-activated receptor (PPAR) signaling pathway mediated by and were significantly activated in LBP-deficient samples. Our study suggested that the invading LPS may interplay with LBP to activate the nuclear factor kappa B (NF-B) signaling pathway and trigger uncontrolled inflammatory response. However, when inhibiting the activity of NF-B, lipid-related metabolism would make bacteria removal via the effect on the PPAR signaling pathway in the absence of LBP gene. We also compared the serum lactate dehydrogenase (LDH) and alkaline phosphatase (ALP) levels using the biochemistry analyzer and analyzed the expression of high mobility group box 1 (HMGB1) and cleaved-caspase 3 with immunohistochemistry, which further validated our conclusion.
脓毒症是一种器官功能障碍,由感染引起的炎症反应失调引起。脂多糖结合蛋白 (LBP) 与脂多糖 (LPS) 结合,调节炎症反应。据报道,一项罕见的系统研究检测了 LPS 诱导的脓毒症期间 LBP 基因的作用。在此,我们使用 RNA 测序技术来描绘 LPS 给药后多个时间点 LBP 缺陷型大鼠和 WT 大鼠肝组织的转录组变化。我们对肝组织进行 RNA 测序,以在 0 h、6 h 和 24 h 时搜索 WT 组和 LBP 缺陷组之间差异表达基因 (DEGs) 和富集的生物过程和途径。总共在 0 h、6 h 和 24 h 时鉴定出 168、284 和 307 个 DEGs,包括 、 、 、 、和 ,它们与炎症或脂质相关过程有关。功能富集分析表明,LPS 介导的炎症反应在 6 h 时通过 、 、 和 增强,而 LPS 给药后 24 h 时与脂质相关的代谢与 、 和 富集。当 LBP 基因被敲除时,未发现炎症过程;在 LBP 缺陷型样本中,脂质相关代谢过程和过氧化物酶体增殖物激活受体 (PPAR) 信号通路由 和 介导,显著激活。我们的研究表明,入侵的 LPS 可能与 LBP 相互作用,激活核因子 kappa B (NF-B) 信号通路并引发不受控制的炎症反应。然而,当抑制 NF-B 的活性时,在没有 LBP 基因的情况下,脂质相关的代谢会通过对 PPAR 信号通路的影响来清除细菌。我们还使用生化分析仪比较了血清乳酸脱氢酶 (LDH) 和碱性磷酸酶 (ALP) 水平,并通过免疫组织化学分析了高迁移率族框 1 (HMGB1) 和切割型半胱天冬酶 3 的表达,进一步验证了我们的结论。
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