黄连解毒汤合犀角地黄汤通过影响成纤维细胞活化介导的角质形成细胞增殖治疗银屑病的机制研究

doi:10.35541/cjd.20250033

中华皮肤科杂志 ›› 2025, Vol. 58 ›› Issue (11): 1064-1074.doi: 10.35541/cjd.20250033

黄连解毒汤合犀角地黄汤通过影响成纤维细胞活化介导的角质形成细胞增殖治疗银屑病的机制研究

彭友华¹ 高贵云¹ 刘超¹ 李婧琳² 张梦瑶² 戴婧² 陈瑶² 刘峻齐² 王旭东¹

¹湖南航天医院皮肤科，长沙 410205；²湖南中医药大学第二附属医院皮肤科，长沙 410005

收稿日期:2025-01-20 修回日期:2025-06-19 发布日期:2025-11-03
通讯作者: 王旭东 E-mail:Wjrd6@sina.com
基金资助:
湖南省自然科学基金（2024JJ5130）；湖南中医药管理局重点项目（C2022025）；湖南省卫生健康委科研项目（20232100）；长沙市自然科学基金项目（kq2403153）；航天医科重点项目（2024YK08）

Huanglian Jiedu decoction combined with Xijiao Dihuang decoction for the treatment of psoriasis via influencing fibroblast activation-mediated keratinocyte proliferation: a mechanistic study

Peng Youhua¹, Gao Guiyun¹, Liu Chao¹, Li Jinglin², Zhang Mengyao², Dai Jing², Chen Yao², Liu Junqi², Wang Xudong¹

¹Department of Dermatology, Hunan Aerospace Hospital, Changsha 410205, China; ²Department of Dermatology, the Second Affiliated Hospital of Hunan University of Chinese Medicine, Changsha 410005, China

Received:2025-01-20 Revised:2025-06-19 Published:2025-11-03
Contact: Wang Xudong E-mail:Wjrd6@sina.com
Supported by:
Hunan Provincial Natural Science Foundation （2024JJ5130）; Hunan Provincial Administration of Traditional Chinese Medicine Key Project （C2022025）; Hunan Provincial Health Commission Research Project （20232100）; Changsha Municipal Natural Science Foundation （kq2403153）; Aerospace Medical Key Project （2024YK08）

摘要/Abstract

摘要： 【摘要】目的探讨黄连解毒汤合犀角地黄汤调控成纤维细胞治疗银屑病的机制。方法采用5%咪喹莫特乳膏刺激小鼠背部构建银屑病小鼠模型，并采用不同剂量（7.7、30.6 g/kg）黄连解毒汤合犀角地黄汤进行灌胃干预，甲氨蝶呤（2 mg/kg）灌胃作为阳性对照组；7 d后记录并评估皮损情况，采用银屑病面积和严重程度指数（PASI）评分评估皮损严重程度，HE染色和Baker评分评估皮肤组织病理变化。体外实验中将成纤维细胞分为对照组、模型组、低剂量（5%含药血清）干预组、高剂量（20%含药血清）干预组；对照组细胞用20%正常大鼠血清培养24 h，模型组细胞采用20%正常大鼠血清加5 ng/ml肿瘤坏死因子α（TNF-α）和50 ng/ml白细胞介素17A（IL-17A）刺激24 h，以模拟银屑病发生过程中的成纤维细胞；低剂量干预组和高剂量组在模型组处理的基础上将20%正常大鼠血清分别换成5%和20%黄连解毒汤合犀角地黄汤含药血清培养24 h。成纤维细胞按照上述分组处理后，利用Transwell体系与角质形成细胞（HaCaT细胞）共培养。另外，在对照组的基础上，将成纤维细胞分为模型组、20%含药血清治疗组、20%含药血清治疗 + OE-SFRP2组，均以TNF-α、IL-17A刺激模拟银屑病状态，20%含药血清治疗组处理如前述，20%含药血清治疗 + OE-SFRP2组转染载体48 h构建过表达模型，后用20%含药血清培养24 h，不与HaCaT细胞共培养。采用细胞计数试剂盒8（CCK-8）检测细胞活性，流式细胞术检测细胞凋亡率，酶联免疫吸附试验（ELISA）检测小鼠血清或细胞培养基上清液TNF-α、IL-1β、IL-6、趋化因子配体（CXCL）1、CXCL12等炎症因子和趋化因子的蛋白含量；qPCR检测小鼠皮肤组织或细胞中炎症因子、趋化因子、细胞周期和增殖相关因子以及SFRP2的mRNA水平；Western印迹检测成纤维细胞中SFRP2、Wnt3a和β连环蛋白（catenin）的表达水平。多组间比较采用单因素方差分析，事后分析采用Tukey′s检验。结果小鼠体内实验显示，与正常组相比，模型组小鼠皮肤表现出典型的银屑病特征，皮肤组织炎性浸润、表皮增厚明显，TNF-α［（531.16 ± 28.27）比（239.58 ± 10.39） pg/ml］、IL-1β［（111.40 ± 5.16）比（80.35 ± 3.87） pg/ml］、IL-6［（109.17 ± 4.84）比（71.73 ± 2.04） pg/ml］含量和mRNA水平明显增加（均P < 0.001），而治疗组小鼠的银屑病表现减轻，炎症因子TNF-α［低剂量组、高剂量组和阳性对照组：（420.80 ± 29.30）、（322.33 ± 9.40）、（322.97 ± 12.16） pg/ml］、IL-1β［（98.69 ± 4.49）、（89.02 ± 1.56）、（88.88 ± 2.08） pg/ml］、IL-6［（94.07 ± 3.76）、（80.54 ± 3.30）、（83.21 ± 3.18） pg/ml］的含量和mRNA水平均较模型组显著下降（均P < 0.001）；在体外成纤维细胞实验中，相较于对照组，模型组中炎症因子IL-1β［（126.42 ± 3.56）比（34.81 ± 0.44） pg/ml］、IL-6［（459.44 ± 9.35）比（115.51 ± 7.26） pg/ml］和趋化因子CXCL1［（2 434.88 ± 127.63）比（762.85 ± 30.60）pg/ml］和CXCL12［（3 542.14 ± 35.86）比（2 095.86 ± 45.12） pg/ml］的含量和mRNA水平显著升高（均P < 0.001），SFRP2、Wnt3a、β-catenin蛋白的表达显著上升，采用黄连解毒汤合犀角地黄汤含药血清进行干预后，上述指标均显著下降（均P < 0.001）；然而同时给以20%含药血清干预，SFRP2过表达组的成纤维细胞中炎症因子和趋化因子表达均高于非过表达组（均P < 0.01）。将成纤维细胞与角质形成细胞共培养时，模型组中HaCaT细胞活性高于对照组且凋亡率低于对照组，而低剂量和高剂量组中HaCaT细胞活性低于模型组且凋亡率高于模型组（均P < 0.05）。结论黄连解毒汤合犀角地黄汤可能通过下调SFRP2/Wnt/β-catenin信号通路抑制成纤维细胞的活化和炎症进程，进而抑制角质形成细胞增殖和炎症细胞活化，发挥治疗银屑病的功效。

关键词: 银屑病, 黄连解毒汤, 犀角地黄汤, 成纤维细胞, HaCaT细胞, β连环素, 疾病模型, 动物

Abstract: 【Abstract】 Objective To explore the mechanisms of action of Huanglian Jiedu decoction combined with Xijiao Dihuang decoction （HLJDT-XJDH） in regulating fibroblasts in the treatment of psoriasis. Methods A mouse model of psoriasis was established by topical application of imiquimod 5% cream on the shaved back; HLJDT-XJDH at different doses of 7.7 and 30.6 g/kg was administered via gavage for intervention, and methotrexate （2 mg/kg） served as a positive control; after 7 days, the severity of skin lesions was assessed using the psoriasis area and severity index （PASI）, while histopathological changes of skin tissues were evaluated using hematoxylin-eosin （HE） staining and Baker scoring. For in vitro experiments, fibroblasts were divided into a control group, a model group, a low-dose （5% drug-containing serum） intervention group, and a high-dose （20% drug-containing serum） intervention group; cells in the control group were cultured with 20% normal rat serum for 24 hours; in the model group, cells cultured with 20% normal rat serum were stimulated with 5 ng/ml tumor necrosis factor （TNF）-α and 50 ng/ml interleukin （IL）-17A for 24 hours to mimic fibroblasts during the occurrence of psoriasis; cells in the low- and high-dose intervention groups received the same stimulation as the model group, and were cultured for 24 hours with 5% and 20% HLJDT-XJDH-containing serum, respectively, but not with the 20% normal rat serum. After the above treatment, these cells were co-cultured with keratinocytes （HaCaT cells） using a Transwell system. In addition, on the basis of the control group, fibroblasts were divided into the model group, 20% drug-containing serum intervention group, and 20% drug-containing serum intervention + OE-SFRP2 group; TNF-α and IL-17A were used to stimulate the cells to simulate the psoriatic state; the treatment in the 20% drug-containing serum intervention group was carried out as previously described; in the 20% drug-containing serum intervention + OE-SFRP2 group, cells were transfected with the vector for 48 hours to establish an overexpression model, followed by culture with 20% drug-containing serum for 24 hours, without co-culture with HaCaT cells.. Cell counting kit-8 （CCK-8） assay was performed to assess cell viability, flow cytometry to measure apoptosis rates, enzyme-linked immunosorbent assay （ELISA） to detect levels of inflammatory cytokines （TNF-α, IL-1β, IL-6） as well as chemokine ligand （CXCL） 1 and CXCL12 in mouse serum or cell culture supernatant, qPCR to determine the mRNA expression of inflammatory cytokines, chemokines, cell cycle- and proliferation-related factors, as well as SFRP2 in mouse skin tissues or cells, and Western blot analysis to determine the protein expression of SFRP2, Wnt3a, and β-catenin in fibroblasts. One-way analysis of variance was employed for intergroup comparisons, and post-hoc analysis was conducted using Tukey′s test. Results In vivo mouse experiments showed that compared with the normal control group, the model group exhibited typical psoriatic characteristics in skin morphology, including significant inflammatory infiltration in skin tissues and marked epidermal thickening; compared with the normal control group, the serum levels of TNF-α （531.16 ± 28.27 pg/ml vs. 239.58 ± 10.39 pg/ml）, IL-1β （111.40 ± 5.16 pg/ml vs. 80.35 ± 3.87 pg/ml）, and IL-6 （109.17 ± 4.84 pg/ml vs. 71.73 ± 2.04 pg/ml） significantly increased in the model group, along with their mRNA expression levels in mouse skin tissues （all P < 0.001）; compared with the model group, the treatment group showed alleviated psoriatic manifestations, and significant reductions in the levels of inflammatory factors TNF-α （low-dose, high-dose, and positive control groups: 420.80 ± 29.30 pg/ml, 322.33 ± 9.40 pg/ml, 322.97 ± 12.16 pg/ml, respectively）, IL-1β （98.69 ± 4.49 pg/ml, 89.02 ± 1.56 pg/ml, 88.88 ± 2.08 pg/ml, respectively）, and IL-6 （94.07 ± 3.76 pg/ml, 80.54 ± 3.30 pg/ml, 83.21 ± 3.18 pg/ml, respectively）, as well as in their mRNA expression levels （all P < 0.001）. In in vitro fibroblast experiments, compared with the control group, the model group exhibited a significant elevation in the supernatant levels of IL-1β （126.42 ± 3.56 pg/ml vs. 34.81 ± 0.44 pg/ml）, IL-6 （459.44 ± 9.35 pg/ml vs. 115.51 ± 7.26 pg/ml）, CXCL1 （2 434.88 ± 127.63 pg/ml vs. 762.85 ± 30.60 pg/ml） and CXCL12 （3 542.14 ± 35.86 pg/ml vs. 2 095.86 ± 45.12 pg/ml）, the expression levels of their mRNAs （all P < 0.001）, as well as the protein expression levels of SFRP2, Wnt3a, and β-catenin; after intervention with HLJDT-XJDH-containing serum, all the above indices significantly decreased （all P < 0.001）. However, when 20% drug-containing serum intervention was administered simultaneously, the expression of inflammatory factors and chemokines in fibroblasts was significantly higher in the SFRP2 overexpression group than in the non-overexpression group （all P < 0.01）. When fibroblasts were co-cultured with HaCaT cells, the model group showed significantly increased cell viability but a decreased apoptosis rate of HaCaT cells compared with the control group, while the low- and high-dose intervention groups showed significantly decreased cell viability but increased apoptosis rates of HaCaT cells compared with the model group （all P < 0.05）. Conclusion HLJDT-XJDH may exert therapeutic effects in psoriasis by downregulating the SFRP2/Wnt/β-catenin signaling pathway, thereby inhibiting fibroblast activation and inflammatory process, which subsequently suppresses the proliferation of keratinocytes and the activation of inflammatory cells.

Key words: Psoriasis, Huang Lian Jie Du Tang, Xi Jiao Di Huang Tang, Fibroblasts, HaCaT cells, beta Catenin, Disease models, animal

彭友华高贵云刘超李婧琳张梦瑶戴婧陈瑶刘峻齐王旭东. 黄连解毒汤合犀角地黄汤通过影响成纤维细胞活化介导的角质形成细胞增殖治疗银屑病的机制研究[J]. 中华皮肤科杂志, 2025,58(11):1064-1074. doi:10.35541/cjd.20250033

Peng Youhua, Gao Guiyun, Liu Chao, Li Jinglin, Zhang Mengyao, Dai Jing, Chen Yao, Liu Junqi, Wang Xudong. Huanglian Jiedu decoction combined with Xijiao Dihuang decoction for the treatment of psoriasis via influencing fibroblast activation-mediated keratinocyte proliferation: a mechanistic study[J]. Chinese Journal of Dermatology, 2025, 58(11): 1064-1074.doi:10.35541/cjd.20250033

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黄连解毒汤合犀角地黄汤通过影响成纤维细胞活化介导的角质形成细胞增殖治疗银屑病的机制研究

Huanglian Jiedu decoction combined with Xijiao Dihuang decoction for the treatment of psoriasis via influencing fibroblast activation-mediated keratinocyte proliferation: a mechanistic study

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