升麻素调控巨噬细胞极化在牙周炎中的作用

doi:10.13591/j.cnki.kqyx.2026.04.002

摘要/Abstract

摘要：

目的研究升麻素(cimifugin)调控巨噬细胞极化在牙周炎中的作用。方法 CCK-8和活/死细胞染色检测不同浓度(0、20.4、40.8、81.6、163.2、326.5、653.0、1 306.0 μmol/L)升麻素对RAW264.7细胞活性的影响,并确定后续实验最佳浓度;免疫荧光染色观察升麻素对M1型、M2型巨噬细胞极化表型CD86、CD206表达的影响;RT-qPCR分析升麻素处理后巨噬细胞诱导型一氧化氮合酶(inducible nitric oxide synthase,iNOS)、白细胞介素(interleukin,IL)-1β、CD86、IL-6、肿瘤坏死因子-α(tumor necrosis factor-α,TNF-α)及CD206、精氨酸酶-1(arginase-1,Arg-1)表达水平变化。构建小鼠牙周炎症模型,根据是否给药分为牙周炎组(PD组)和牙周炎+升麻素组(PD+Cimifugin组),假手术组作为空白对照组,Micro-CT扫描重建,CTAn测量各组釉牙骨质界到牙槽嵴顶距离(CEJ-ABC)、骨矿物质密度(bone mineral densitys,BMD)、相对骨体积分数(bone volume/total volume,BV/TV)、骨小梁分离度(trabecular separation,Tb.Sp),HE染色观察小鼠牙周组织变化,TRAP染色检测破骨细胞数量,免疫组化(immunohistochemistry,IHC)染色分析IL-1β、IL-10表达。结果浓度≤326.5 μmol/L时,升麻素对巨噬细胞的增殖及活性无明显影响(P>0.05)。326.5 μmol/L升麻素可抑制M1型巨噬细胞iNOS、IL-1β、CD86、IL-6、TNF-α表达,促进M2型巨噬细胞CD206、Arg-1表达(P<0.000 1)。与PD组相比,PD+Cimifugin组CEJ-ABC、Tb.Sp明显减小,BMD、BV/TV明显增加(P<0.01),小鼠牙周组织炎症细胞浸润减少、破骨细胞数量降低(P<0.05),IL-10表达显著升高(P<0.000 1),IL-1β表达明显降低(P<0.01)。结论升麻素通过抑制巨噬细胞M1型极化、促进M2型极化,减轻牙周组织炎症并减少骨缺损。

关键词: 牙周炎, 升麻素, 巨噬细胞极化

Abstract:

Objective To investigate the role of cimifugin in regulating macrophage polarization in periodontitis. Methods The effects of cimifugin at various concentrations (0, 20.4, 40.8, 81.6, 163.2, 326.5, 653.0, 1 306.0 μmol/L) on the viability of RAW264.7 cells were assessed using the CCK-8 and live/dead cell staining to determine the optimal concentration for subsequent experiments. Immunofluorescence staining was employed to observe the impact of cimifugin on M1 and M2 macrophage polarization phenotypes (CD86 and CD206). RT-qPCR was utilized to analyze changes in the expression levels of inducible nitric oxide synthase (iNOS), interleukin (IL)-1β, CD86, IL-6, tumor necrosis factor-α (TNF-α), CD206, and arginase-1 (Arg-1) in macrophages treated with cimifugin. A murine periodontal inflammation model was established, and the animals were divided into a periodontitis group (PD group), a periodontitis + cimifugin group (PD+Cimifugin group), and a sham surgery control group (Control group). Micro-CT was used for scanning and reconstruction, and CTAn software was employed to measure the cemento enamel junction-alveolar bone crest distance (CEJ-ABC), bone mineral density (BMD), relative bone volume/total volume (BV/TV), and trabecular separation (Tb.Sp). HE staining was performed to observe changes in periodontal tissues, while TRAP staining was used to quantify osteoclasts. Immunohistochemistry (IHC) was conducted to analyze the expression of IL-1β and IL-10. Results Cimifugin concentrations≤326.5 μmol/L did not significantly affect macrophage proliferation and viability (P>0.05). Cimifugin at 326.5 μmol/L inhibited the expression of M1 macrophage markers iNOS, IL-1β, CD86, IL-6, and TNF-α, while promoting the expression of M2 macrophage markers CD206 and Arg-1 (P<0.000 1). Compared to the PD group, the PD+Cimifugin group exhibited significant improvements in CEJ-ABC, BMD, BV/TV, and Tb.Sp (P<0.01), reduced inflammatory cell infiltration and osteoclast numbers in periodontal tissues (P<0.05), significantly elevated IL-10 expression (P<0.000 1), and markedly decreased IL-1β expression (P<0.01). Conclusion Cimifugin alleviates periodontal inflammation and reduces bone defects by inhibiting M1 macrophage polarization and promoting M2 macrophage polarization.

Key words: periodontitis, cimifugin, macrophage polarization

中图分类号:

R781.4

韩东, 杨舒涵, 于昕弘, 谢伟丽. 升麻素调控巨噬细胞极化在牙周炎中的作用[J]. 口腔医学, 2026, 46(4): 246-252.

HAN Dong, YANG Shuhan, YU Xinhong, XIE Weili. The role of cimifugin in regulating macrophage polarization in periodontitis[J]. Stomatology, 2026, 46(4): 246-252.

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基因	引物序列(5'—3')
GAPDH	F:GGTGAAGGTCGGTGTGACCG R:CTCGCTCCTGGAAGATGGT
CD86	F:CAGCACGGACTTGAACAACC R:CTCCACGGAAACAGCATCTGA
IL-1β	F:AAGAAGAGCCCATCCTCTGTG R:TGTTCATCTCGGAGCCTGTAG
IL-6	F:TTGGGACTGATGCTGGTGAC R:GTGGTATAGACAGGTCTGTTGGG
iNOS	F:GAGCGAGTTGTGGATTGT R:GCAGCCTCTTGTCTTTGA
TNF-α	F:CCCTCCTGGCCAACGGCATG R:TCGGGGCAGCCTTGTCCCTT
CD206	F:ACCCAAGGGCTCTTCTAA R:TGGCCTCTTGAGGTATGT
Arg-1	F:AGACAGCAGAGGAGGTGAAGAGTAC R:GGTAGTCAGTCCCTGGCTTATGGT