白细胞介素22和p38 MAPK信号通路抑制骨关节结核骨质破坏的作用机制研究

doi:10.19982/j.issn.1000-6621.20240568

中国防痨杂志 ›› 2025, Vol. 47 ›› Issue (4): 454-459.doi: 10.19982/j.issn.1000-6621.20240568

白细胞介素22和p38 MAPK信号通路抑制骨关节结核骨质破坏的作用机制研究

盛杰¹, 洪凯峰², 米尔扎提·艾沙¹, 唐伟¹(), 地里下提·阿不力孜¹()

¹新疆维吾尔自治区传染病医院骨科,乌鲁木齐 830000
²新疆维吾尔自治区乌鲁木齐市友谊医院骨科,乌鲁木齐 830049

收稿日期:2024-12-16 出版日期:2025-04-10 发布日期:2025-04-02
通信作者: 地里下提·阿不力孜,Email:xkyy2011@126.com; 唐伟,Email:Jncz211@163.com
作者简介:注:洪凯峰和盛杰对本文有同等贡献,为并列第一作者
基金资助:
新疆维吾尔自治区科技厅自然科学基金面上项目(2021D01A161);新疆维吾尔自治区“天山英才”医药卫生高层次人才培养计划(TSYC202301B087)

Study on the mechanism of IL-22 and p38 MAPK signaling pathways in inhibiting bone destruction in bone and joint tuberculosis

Sheng Jie¹, Hong Kaifeng², Mierzhati Aisha¹, Tang Wei¹(), Dilixiati Abulizi¹()

¹Department of Orthopedics, Xinjiang Uygur Autonomous Region Infectious Disease Hospital, Urumqi 830000, China
²Department of Orthopedics, Urumqi Friendship Hospital, Xinjiang Uygur Autonomous Region, Urumqi 830049, China

Received:2024-12-16 Online:2025-04-10 Published:2025-04-02
Contact: Dilixiati Abulizi, Email: xkyy2011@126.com; Tang Wei, Email:Jncz211@163.com
Supported by:
General Project of the Natural Science Foundation of the Science and Technology Department of Xinjiang Uygur Autonomous Region(2021D01A161);The “Tianshan Talents” High-Level Talent Training Program in Medicine and Health of Xinjiang Uygur Autonomous Region(TSYC202301B087)

摘要/Abstract

摘要：

目的: 探讨白细胞介素22(IL-22)通过p38 MAPK信号通路影响骨关节结核骨质破坏的作用机制。方法: (1)选取2021年1—12月在新疆维吾尔自治区传染病医院骨科接受手术治疗的骨关节结核患者作为病例组,共58例;选取相同时间段该医院接受手术治疗的骨折患者作为对照组,共51例。收集研究对象的血清样本,使用酶联免疫吸附试验检测IL-22水平;收集骨组织样本,应用Western blot检测p38、p-p38、CatK和MMP9蛋白表达水平。(2)将小鼠单核巨噬细胞白血病细胞(RAW264.7)诱导为破骨细胞模型,实验分为6组,分别为破骨细胞组、破骨细胞+H37Rv组、破骨细胞+H37Rv+阴性对照组、破骨细胞+H37Rv+IL-22-shRNA组、破骨细胞+H37Rv+p38抑制剂组、破骨细胞+H37Rv+p38抑制剂+IL-22-shRNA组。通过TRAP染色法观察破骨细胞的活性,使用qRT-PCR和Western blot检测p38、CatK和MMP9的基因和蛋白表达水平。结果: (1)临床研究结果显示,对照组血清中IL-22的表达水平[中位数(四分位数)]为34.61(28.29,76.92)pg/ml,明显低于病例组[102.74(56.12, 132.78)pg/ml],差异有统计学意义(Z=-3.840,P=0.001)。病例组p38、p-p38、CatK和MMP9蛋白表达水平分别为0.649±0.043、0.856±0.062、0.506±0.072,均明显高于对照组(分别为0.346±0.078、0.708±0.094、0.366±0.046),差异均有统计学意义(t值分别为-8.368、-3.203、-4.025,P值均<0.05)。(2)细胞实验结果显示,破骨细胞+H37Rv组每光镜视野(×100)TRAP染色阳性细胞个数为51.333±12.858,明显高于其他组,差异有统计学意义(F=26.270,P<0.001);破骨细胞+H37Rv组p-p38、CatK和MMP9蛋白表达水平明显升高,与之相比,在IL-22-shRNA和p38抑制剂干预后明显下调。结论: 敲减IL-22抑制p38 MAPK信号通路可减轻骨关节结核的骨质破坏。

关键词: 分枝杆菌, 结核, 结核, 骨关节, 破骨细胞, 白细胞介素类

Abstract:

Objective: o elucidate the mechanistic role of interleukin-22 (IL-22) in mediating bone destruction in bone and joint tuberculosis via the p38 mitogen-activated protein kinase (MAPK) signaling pathway. Methods: (1) A total of 58 patients diagnosed with bone and joint tuberculosis who underwent surgical intervention at the Department of Orthopedics, Xinjiang Uygur Autonomous Region Infectious Disease Hospital between January and December 2021 were enrolled as the case group. A control group comprising 51 patients with fractures who underwent surgical treatment at the same institution during the same period was also established. Peripheral blood serum samples were collected from all participants, and IL-22 levels were quantified using enzyme-linked immunosorbent assay (ELISA). Additionally, bone tissue specimens were obtained for protein expression analysis. The expression levels of p38 MAPK, phosphorylated p38 (p-p38), cathepsin K (CatK), and matrix metalloproteinase-9 (MMP9) were determined via Western blotting. (2) Mouse monocyte-macrophage leukemia cells (RAW264.7) were differentiated into osteoclast-like cells and subsequently divided into six experimental groups: osteoclast group, osteoclast+H37Rv group, osteoclast+H37Rv+negative control group, osteoclast+H37Rv+IL-22-shRNA group, osteoclast+H37Rv+p38 inhibitor group, and osteoclast+H37Rv+p38 inhibitor+IL-22-shRNA group. The osteoclastogenic activity was assessed using tartrate-resistant acid phosphatase (TRAP) staining, while gene and protein expression levels of p38 MAPK, CatK, and MMP9 were quantified using quantitative real-time polymerase chain reaction (qRT-PCR) and Western blotting. Results: (1) Clinical findings: The serum IL-22 levels in the control group (median (quartiles): 34.61 (28.29, 76.92) pg/ml) were significantly lower than those in the case group (102.74 (56.12, 132.78) pg/ml), with a statistically significant difference (Z=-3.840, P=0.001). The protein expression levels of p38, p-p38, CatK, and MMP9 in the case group were 0.649±0.043, 0.856±0.062, and 0.506±0.072, respectively, all of which were significantly higher than those in the control group (0.346±0.078, 0.708±0.094, and 0.366±0.046, respectively), with statistically significant differences (t=-8.368, -3.203, -4.025; all P<0.05). (2) Cellular experiment findings: The number of TRAP-positive osteoclasts per microscopic field (×100) was highest in the osteoclast+H37Rv group (51.333±12.858), significantly exceeding that of all other groups (F=26.270, P<0.001). The expression levels of p-p38, CatK, and MMP9 proteins were markedly upregulated in the osteoclast+H37Rv group but were significantly downregulated following intervention with IL-22 short hairpin RNA (shRNA) and a p38 MAPK inhibitor. Conclusion: Silencing IL-22 expression and inhibiting the p38 MAPK signaling pathway significantly mitigates bone destruction associated with bone and joint tuberculosis. These findings suggest that IL-22 and p38 MAPK play pivotal roles in osteoclastic activity and bone resorption in the pathogenesis of bone and joint tuberculosis, highlighting their potential as therapeutic targets for preventing disease-associated bone loss.

Key words: Mycobacterium tuberculosis, Tuberculosis, osteoarticular, Osteoclasts, Interleukins

中图分类号:

R529.2

盛杰, 洪凯峰, 米尔扎提·艾沙, 唐伟, 地里下提·阿不力孜. 白细胞介素22和p38 MAPK信号通路抑制骨关节结核骨质破坏的作用机制研究[J]. 中国防痨杂志, 2025, 47(4): 454-459. doi: 10.19982/j.issn.1000-6621.20240568

Sheng Jie, Hong Kaifeng, Mierzhati Aisha, Tang Wei, Dilixiati Abulizi. Study on the mechanism of IL-22 and p38 MAPK signaling pathways in inhibiting bone destruction in bone and joint tuberculosis[J]. Chinese Journal of Antituberculosis, 2025, 47(4): 454-459. doi: 10.19982/j.issn.1000-6621.20240568

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参考文献 14

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名称	序列(5'~3')	片段长度(bp)
CatK-F	AAAGCCCTGAAGAGAGCAGT	179
CatK-R	CAGTGCTTGCTTCCCTTCTG
MMP9-F	AAAACCTCCAACCTCACGGA	190
MMP9-R	GTGGTGTTCGAATGGCCTTT
mouse β-actin F	GTGACGTTGACATCCGTAAAGA	245
mouse β-actin R	GCCGGACTCATCGTACTCC

组别	CatK	MMP9
破骨细胞组	1.047±0.357	1.008±0.158
破骨细胞+H37Rv组	2.311±0.254	1.981±0.277
破骨细胞+H37Rv+阴性对照组	2.339±0.111	1.978±0.244
破骨细胞+H37Rv+IL-22-shRNA组	1.688±0.301	1.485±0.242
破骨细胞+H37Rv+p38抑制剂组	1.635±0.087	1.440±0.111
破骨细胞+H37Rv+p38抑制剂+IL-22-shRNA组	1.160±0.063	1.102±0.101
F值	17.634	12.819
P值	<0.001	<0.001

组别	p38	p-p38	CatK	MMP9
破骨细胞组	0.676±0.032	0.585±0.016	0.302±0.018	0.650±0.044
破骨细胞+H37Rv组	0.650±0.033	1.161±0.105	0.530±0.023	0.925±0.013
破骨细胞+H37Rv+阴性对照组	0.657±0.044	1.167±0.047	0.546±0.060	0.957±0.064
破骨细胞+H37Rv+IL-22-shRNA组	0.704±0.023	0.750±0.216	0.439±0.026	0.766±0.051
破骨细胞+H37Rv+p38抑制剂组	0.718±0.054	0.717±0.038	0.453±0.025	0.807±0.044
破骨细胞+H37Rv+p38抑制剂+IL-22-shRNA组	0.699±0.083	0.611±0.005	0.335±0.039	0.635±0.101
F值	0.944	82.237	24.416	15.733
P值	0.488	<0.01	<0.01	<0.01

白细胞介素22和p38 MAPK信号通路抑制骨关节结核骨质破坏的作用机制研究

Study on the mechanism of IL-22 and p38 MAPK signaling pathways in inhibiting bone destruction in bone and joint tuberculosis

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分组	例数	p38	p-p38	CatK	MMP9
对照组	51	0.559±0.089	0.346±0.078	0.708±0.094	0.366±0.046
病例组	58	0.575±0.089	0.649±0.043	0.856±0.062	0.506±0.072
t值		-0.308	-8.368	-3.203	-4.025
P值		0.764	<0.001	0.011	0.002

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