针刺“祛瘀”(LI11)和“血海”(SP10)预处理对荨麻疹大鼠肥大细胞和IL-33/ST2的影响[j]。

Si-Jia Liu, Jun-Tong Liu, Ji-Quan Li, Cheng-Cheng Wang, Miao Yu, Zhi-Qiang Guan, Lie Wang, Tie-Ming Ma
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引用次数: 0

摘要

目的:观察电针“祛瘀”(LI11)和“血海”(SP10)预处理对大鼠荨麻疹皮肤敏感区白细胞介素(IL)-33表达、致瘤性2 (ST2)抑制及肥大细胞脱粒的影响,探讨其预防荨麻疹的作用机制。方法:将32只雄性SD大鼠随机分为空白对照组、模型组、EA预处理组和给药组,每组8只。制备的抗卵清蛋白血清(外源血清,0.1 mL/点)沿背部脊柱两侧局部注射,48 h后经尾静脉注射卵清蛋白与0.5%埃文斯蓝、生理盐水混合溶液,建立荨麻疹模型。在建模前,对双侧LI11和SP10施加EA干预(2 Hz/15 Hz, 1 mA) 20 min,每天1次,持续7 d。从第5天开始进行背部致敏。给药组大鼠灌胃氯雷他定,模型组大鼠灌胃等量生理盐水。测量背部皮肤组织evans蓝斑直径;H.E.染色后光镜下观察蓝斑组织的病理变化。甲苯胺蓝染色观察皮下松散结缔组织肥大细胞的脱粒状态。ELISA法检测血清IgE和组胺含量,免疫组化法检测致敏斑(evans蓝色渗出斑)皮肤及皮下组织中IL-33和ST2的免疫活性。结果:与空白对照组比较,模型组evans蓝斑直径、肥大细胞脱粒率、血清IgE和组胺含量、evans蓝斑组织IL-33和ST2免疫活性均显著升高(ppp)。结论:EA预处理可预防大鼠荨麻疹(减小尺寸和敏感反应),可能与其通过抑制IL-33和ST2降低IgE水平的作用有关。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
[Effect of acupuncture pretreatment of "Quchi"(LI11) and "Xuehai" (SP10) on mast cells and IL-33/ST2 in rats with urticaria].

Objective: To observe the effect of electroacupuncture (EA) pretreatment at "Quchi "(LI11) and "Xuehai "(SP10) on expression of interleukin (IL)-33, suppression of tumorigenicity 2 (ST2) and mast cell degranulation in sensitive area of skin tissue in rats with urticaria, so as to explore its mechanisms underlying prevention of urticaria.

Methods: A total of 32 male SD rats were randomly divided into blank control, model, EA preconditioning and medication groups, with 8 rats in each group. The urticaria model was established by topical injection of the prepared anti-ovalbumin serum (foreign serum, 0.1 mL/spot) along the bilateral sides of the spinal column on the back, followed by injection of mixture solution of ovalbumin, 0.5% evans blue and normal saline via the tail vein 48 h later. EA intervention (2 Hz/15 Hz, 1 mA) was applied to bilateral LI11 and SP10 for 20 min, once daily for 7 d before modeling.Back sensitization was started from the 5th day on. Rats of the medication group received gavage of loratadine, and those of the model group received gavage of the same volume of normal saline. The diameter of evans blue spots at the back skin tissue was measured; the histopathological changes of the blue spot tissues were observed by light microscope after H.E. staining. The state of degranulation of mast cells in the subcutaneous loose connective tissue was observed by using toluidine blue staining. Serum IgE and histamine contents were detected by ELISA, and the immunoactivity of IL-33 and ST2 in the skin and subcutaneous tissues of the sensitized spots (evans blue exudation spots) was observed by immunohistochemistry.

Results: Compared with the blank control group, the diameter of evans blue spot, degranulation rate of mast cells, serum IgE and histamine contents, and the immunoactivity of IL-33 and ST2 in the evans blue exudation spot tissues were significantly increased in the model group (P<0.01). In comparison with the model group, the increase of the above-mentioned indexes was reversed in both EA and medication groups (P<0.01,P<0.05). No significant differences were found between the EA and medication groups in down-regulating the levels of the 6 indexes. H.E. staining of the blue spot tissues of rats in the model group showed incomplete structure of the epidermal layer of the skin, unclear interface of tissues, incomplete keratinization, chaotic epidermal cells, disorderly arrangement of fibers in the dermis, and infiltration of inflammatory cells and edema, which was relatively milder in the EA and medication groups.

Conclusion: EA preconditioning can prevent urticaria (reduce size and sensitive reactions) in rats, which may be associated with its functions in lowering the level of IgE through inhibiting IL-33 and ST2.

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