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[实验性自身免疫性神经炎中免疫细胞糖酵解基因的表达及相关免疫细胞的变化]

[Expression of glycolytic genes in immune cells and changes of related immune cells in experimental autoimmune neuritis].

作者信息

Liu S P, Ma L Z, Pan S J, Gong Q Y, Cao Q, Xiao Z M, Lu Z N

机构信息

Department of Neurology, Renmin Hospital of Wuhan University, Wuhan 430061, China.

出版信息

Zhonghua Yi Xue Za Zhi. 2023 May 9;103(17):1334-1339. doi: 10.3760/cma.j.cn112137-20220904-01869.

Abstract

To investigate the expression of glycolytic genes in immune cells and the changes of related immune cells in experimental autoimmune neuritis (EAN), and deepen the understanding of pathogenesis of EAN. Twenty-four male C57BL/6 mice (6-8 weeks old, 18-20 g) were divided into four groups according to the random number table method: control group (P0 was replaced by PBS during modeling and mice were sacrificed on the 16th day), EAN mice were sacrificed on the 8th day after the end of modeling (EAN 8 d), EAN mice were sacrificed on the 16th day after the end of modeling (EAN 16 d), and EAN mice received drug intervention and were sacrificed on the 16 day after the end of modeling (2-DG was intraperitoneally injected since the day of the first immunization, 550 mg/kg; EAN 16 d+2-DG), with 6 rats in each group. The clinical symptoms and clinical scores were observed and recorded daily. At the end of the experiment, the mice were sacrificed under chloral hydrate anesthesia, and the serum, spleen, sciatic nerve and other tissues of each group were collected. The degree of inflammatory cell infiltration and demyelination of sciatic nerve were observed by hematoxylin and eosin (HE) staining and luxol fast blue (LFB) staining. Flow cytometry was used to detect the proportion of M1 macrophages, Th17 cells and Tregs cells. The mRNA expression levels of glycolysis-related genes (mTORC1, HIF1α, GLUT1 and LDHA) were detected by RT-PCR. Western blotting was used to detect the level of pan-lysine lactate in macrophages and sciatic nerve tissue. The expression of glycolysis-related genes (mTORC1, HIF1α, GLUT1 and LDHA) in spleen M1 macrophages and sciatic nerve was significantly up-regulated in EAN 16 d group, compared with control, EAN 8 d and EAN 16 d+2-DG groups (all <0.05). The relative pan-lysine lactate (pankla) expression level of spleen M1 macrophages (1.25±0.02) and sciatic nerve tissue (1.23±0.26) significantly increased in EAN 16 d group, compared with control, EAN 8 d and EAN 16 d+2-DG groups (M1 macrophages: 0.12±0.10, 1.07±0.12 and 0.42±0.07; sciatic nerve: 0.10±0.12, 0.87±0.20 and 0.36±0.05) (all <0.05). The expression of glycolytic genes in splenic CD4+T cells showed an increasing trend, but there were no statistically significant differences among the groups, and the expression of glycolytic genes did not decrease significantly after 2-DG treatment (all >0.05). The proportion of spleen M1 macrophages in the control group, EAN 8 d group, EAN 16 d group and EAN 16 d+2-DG group was 4.28±0.13, 7.54±0.25, 13.16±0.33 and 4.13±0.38 respectively, which was significantly higher in the EAN 16 d group (all <0.05). The proportion of spleen Th17 cells in the four groups was 3.78±0.03, 8.24±0.55, 12.30±1.34 and 4.83±0.01, respectively, which was significantly higher in the EAN 16 d group (all <0.05). The proportion of spleen Tregs cells in the four groups was 10.01±1.05, 7.54±0.70, 3.82±0.47 and 8.22±1.21, respectively, which was significantly lower in the EAN 16 d group (all <0.05). The expression of glycolytic genes in splenic macrophages significantly increases during EAN, but not in CD4+T cells. The proportion of M1 macrophages and Th17 cells in spleen gradually increases, while the proportion of Tregs cells gradually decreases.

摘要

为研究糖酵解基因在免疫细胞中的表达及实验性自身免疫性神经炎(EAN)中相关免疫细胞的变化,加深对EAN发病机制的认识。将24只雄性C57BL/6小鼠(6 - 8周龄,18 - 20 g)按随机数字表法分为四组:对照组(建模期间用PBS代替P0,于第16天处死小鼠),EAN小鼠在建模结束后第8天处死(EAN 8 d),EAN小鼠在建模结束后第16天处死(EAN 16 d),EAN小鼠接受药物干预并在建模结束后第16天处死(自首次免疫当天起腹腔注射2 - DG,550 mg/kg;EAN 16 d + 2 - DG),每组6只大鼠。每天观察并记录临床症状和临床评分。实验结束时,在水合氯醛麻醉下处死小鼠,收集每组的血清、脾脏、坐骨神经等组织。采用苏木精 - 伊红(HE)染色和Luxol固蓝(LFB)染色观察坐骨神经的炎性细胞浸润程度和脱髓鞘情况。采用流式细胞术检测M1巨噬细胞、Th17细胞和Tregs细胞的比例。采用RT - PCR检测糖酵解相关基因(mTORC1、HIF1α、GLUT1和LDHA)的mRNA表达水平。采用蛋白质免疫印迹法检测巨噬细胞和坐骨神经组织中泛赖氨酸乳酸水平。与对照组、EAN 8 d组和EAN 16 d + 2 - DG组相比,EAN 16 d组脾脏M1巨噬细胞和坐骨神经中糖酵解相关基因(mTORC1、HIF1α、GLUT1和LDHA)的表达显著上调(均<0.05)。与对照组、EAN 8 d组和EAN 16 d + 2 - DG组相比,EAN 16 d组脾脏M1巨噬细胞(1.25±0.02)和坐骨神经组织(1.23±0.26)中泛赖氨酸乳酸(pankla)相对表达水平显著升高(M1巨噬细胞:0.12±0.10、1.07±0.12和0.42±0.07;坐骨神经:0.10±0.12、0.87±0.20和0.36±0.05)(均<0.05)。脾脏CD4 + T细胞中糖酵解基因的表达呈上升趋势,但各组间差异无统计学意义,2 - DG处理后糖酵解基因表达未显著降低(均>0.05)。对照组、EAN 8 d组、EAN 16 d组和EAN 16 d + 2 - DG组脾脏M1巨噬细胞比例分别为4.28±0.13、7.54±0.25、13.16±0.33和4.13±0.38,EAN 16 d组显著升高(均<0.05)。四组脾脏Th17细胞比例分别为3.78±0.03、8.24±0.55、12.30±1.34和4.83±0.01,EAN 16 d组显著升高(均<0.05)。四组脾脏Tregs细胞比例分别为10.01±1.05、7.54±0.70、3.82±0.47和8.22±1.21,EAN 16 d组显著降低(均<0.05)。EAN期间脾脏巨噬细胞中糖酵解基因表达显著增加,但CD4 + T细胞中未增加。脾脏中M1巨噬细胞和Th17细胞比例逐渐升高,而Tregs细胞比例逐渐降低。

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