The effects of leptin on the senescence of bone marrow-derived mesenchymal stem cells, frequencies of immune cells and lupus disease in MRL/lpr mice

Chen Haifeng; Zou Yaohong; Sun Lingyun

doi:10.3760/cma.j.issn.1007-7480.2018.08.003

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瘦素对骨髓间充质干细胞及免疫细胞亚群的调控作用及其对狼疮鼠病情的影响

中华风湿病学杂志, 2018,22(8) : 516-521. DOI: 10.3760/cma.j.issn.1007-7480.2018.08.003

摘要

目的

探讨重组瘦素作用于MRL/lpr鼠等动物模型，对其骨髓MSCs衰老、免疫细胞亚群及狼疮病情的影响。

方法

重组瘦素（1 μg/g，每日2次，3 d）或PBS，腹腔注射C57BL/6（B6）鼠、ob/ob鼠及MRL/lpr鼠（每组6只）。考马斯亮蓝法进行尿蛋白定量检测；ELISA法测定血清瘦素水平、自身抗体（ANA、抗dsDNA抗体）、总IgG；直接贴壁法分离培养MSCs，β-半乳糖苷酶染色计数阳性细胞比例，实时荧光定量PCR和蛋白质印迹法分别检测p53、p21的mRNA和蛋白水平，联合评估MSCs衰老情况；流式细胞术检测调节性T细胞及辅助性T细胞（Th）17细胞亚群。采用t检验、方差分析进行统计分析。

结果

狼疮鼠血清瘦素水平（4.5±0.8）ng/ml高于B6鼠（2.3±0.5）ng/ml（t=2.38，P<0.05）。瘦素体内作用均可促进小鼠骨髓MSCs衰老，表现为β-半乳糖苷酶阳性细胞比例增加[（20.6±0.6）%与（15.4±1.6）%，t=8.09，P<0.05]，p53、p21 mRNA和蛋白水平增高。瘦素作用于狼疮鼠致脾细胞数增多，且调节性T细胞降低[（2.77 ±0.23）%与（5.01±0.18）%，t=3.91，P<0.01]，Th17细胞增加[（2.24±0.11）%与（1.74±0.07）%，t=5.013，P<0.01]。瘦素作用致狼疮鼠血清ANA水平进一步增高[（288±69）U/ml与（190±90）U/ml，t=2.84，P<0.05]。瘦素作用组血清抗dsDNA抗体水平均较PBS对照组升高[（12 399±1 237）U/ml与（6 217±1 304）U/ml，t=3.44，P<0.01]。瘦素也可升高狼疮鼠血清IgG浓度[（27.2±2.9）mg/ml与（25.0±3.3）mg/ml，t=3.07，P<0.05]。瘦素体内作用致狼疮鼠尿蛋白浓度较前增加[（1.00±0.10）mg/ml与（0.81±0.06）mg/ml，t=3.31，P<0.05]。

结论

瘦素体内作用不仅加剧狼疮鼠骨髓MSCs的衰老，减弱其免疫调控功能，同时可直接作用引起Th17/调节性T细胞免疫失衡，从而加重狼疮病情。

引用本文: 陈海凤, 邹耀红, 孙凌云. 瘦素对骨髓间充质干细胞及免疫细胞亚群的调控作用及其对狼疮鼠病情的影响 [J] . 中华风湿病学杂志,2018,22 (8): 516-521. DOI: 10.3760/cma.j.issn.1007-7480.2018.08.003

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SLE是一种自身免疫病，伴多种促炎因子、自身抗体的产生及T、B细胞等异常活化等^[1]。SLE患者血清瘦素（leptin）水平升高^[2,3,4]，且与SLE疾病活动度相关^[5]。瘦素属于Ⅰ型细胞因子，发挥代谢、促炎、调节免疫反应等作用。有报道禁食或限制能量摄入缓解狼疮动物模型的病情，而禁食期间脂肪细胞分泌的瘦素则显著降低^[6]，因此瘦素对狼疮疾病的作用得到较多关注。近年来发现瘦素缺乏可缓解狼疮鼠病情，如促炎因子及自身抗体降低、肾脏病理改善等^[7,8]，在狼疮动物模型研究中，瘦素缺陷可致调节性T细胞、辅助性T细胞（Th）17细胞异常改变^[9,10]，提示瘦素可能在狼疮疾病中起到重要的作用，但具体作用及机制目前尚不清楚。

贡献者信息

陈海凤

214023　南京医科大学附属无锡人民医院风湿免疫科

邹耀红

214023　南京医科大学附属无锡人民医院风湿免疫科

孙凌云

南京大学医学院附属鼓楼医院风湿免疫科

通信作者

孙凌云

南京大学医学院附属鼓楼医院风湿免疫科

Email：lingyunsun@nju.edu.cn

关键词

瘦素; 红斑狼疮，系统性; 细胞衰老; 间质干细胞; 免疫调控;

基金项目

国家自然科学基金青年基金（81501345）

江苏省青年医学人才项目（QNRC2016197）

历史

出版日期：2018-08-15

收稿日期：2017-09-11

本文编辑

臧长海

Original Article

The effects of leptin on the senescence of bone marrow-derived mesenchymal stem cells, frequencies of immune cells and lupus disease in MRL/lpr mice

Chen Haifeng, Zou Yaohong, Sun Lingyun

Published 2018-08-15

Cite as Chin J Rheumatol, 2018,22(8): 516-521. DOI: 10.3760/cma.j.issn.1007-7480.2018.08.003

Abstract

Objective

To explore the effects of leptin on the senescence of bone marrow-derived mesenchymal stem cells, frequencies of Treg and Th17 cells, and lupus disease in MRL/lpr mice, and to explore the pathogenesis of systemic lupus erythematosus (SLE).

Methods

Leptin (1 μg/g) or phosphate buffer saline (PBS) was injected into C57BL/6 (B6) mice, ob/ob mice and MRL/lpr mice intra-peritoneally. Urine protein was examined by Coomassie brilliant blue method. The levels of serum leptin, antinuclear antibody (ANA), anti-dsDNA antibody and immunoglobulin (Ig)G were detected by enzyme linked immunosorbent assay (ELISA). Bone marrow derived mesenchymal stem cells (MSCs) were isolated, and treated with or without leptin, then the senescence of MSCs were evaluated by SA-β-gal staining, the levels of p53 and p21 mRNA were measured by real time polymerase chain reaction (PCR), the protein levels of p53 and p21 were tested by Western blotting method. Data were analyzed with t test and ANOVA.

Results

The level of serum leptin was higher in MRL/lpr mice than that of B6 mice [(4.5±0.8) ng/ml vs (2.3±0.5) ng/ml, t=2.38, P<0.05]. Leptin treatment in vivo accelerated the senescence of bone marrow-derived MSCs from all B6 mice, lupus mice and ob/ob mice, manifestedas increased frequencies of SA-β-gal positive cells [(20.6±0.6)% vs (15.4±1.6)%, t=8.09, P<0.05], higher levels of mRNA and p53 and p21 protein. Leptin treatment in vivo also down-regulated the frequency of Treg cells [(2.77±0.23)% vs (5.01±0.18)% t=3.91, P<0.01], and up-regulated Th17 cells [(2.24±0.11)% vs (1.74±0.07)%, t=5.013, P<0.01]. The titer of ANA was further increased in leptin-treated MRL/lpr mice [(288±69) U/ml vs (190±90) U/ml, t=2.84, P<0.05]. The levels of serum anti-dsDNA antibody were also remarkably elevated [(12 399±1 237) U/ml vs (6 217±1 304) U/ml, t=3.44, P<0.01]. Leptin could increase the secretion of total IgG [MRL/lpr (27.2±2.9) mg/ml vs (25.0±3.3) mg/ml, t=3.07, P<0.05]. The proteinuria concentration was increased in lupus mice [(1.00±0.10) mg/ml vs (0.81±0.06) mg/ml, t=3.31, P<0.05], demonstrating that leptin accelerates lupus nephritis.

Conclusion

Leptin administr-ation in vivo enhances the senescence of bone marrow derived MSCs, dysregulate of Treg/Th17 cells from MRL/lpr mice, which impaires the role of immuno-modulation, and aggravates the progress of lupus disease.

Key words:

Leptin; Lupus erythematosus, systemic; Cell senescence; Mesenchymal stem cell; Immune regulation

Contributor Information

Chen Haifeng

Department of Rheumatology and Immunology, Wuxi People's Hospital Affiliated to Nanjing Medical University, Jiangsu 214023, China

Zou Yaohong

Sun Lingyun

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