首页|期刊导航|针刺研究|穴区外泌体在电针促进多裂肌损伤大鼠肌肉再生修复中的作用

穴区外泌体在电针促进多裂肌损伤大鼠肌肉再生修复中的作用OA

Exosomes in acupoint area involved in the effect of electroacupuncture on muscle regeneration and repair in rats with multifidus muscle injury

中文摘要英文摘要

目的:观察电针对多裂肌损伤模型大鼠肌肉再生修复的影响,探讨穴区外泌体在针刺调节中的作用.方法:将40只SD大鼠随机分为正常组、模型组、电针组、抑制剂组,每组10只.模型组、电针组和抑制剂组采用0.5%布比卡因肌肉注射制备多裂肌损伤模型.电针组和抑制剂组分别予以电针"委中"和"肾俞"治疗,疏密波,频率 2 Hz/10 Hz,1 mA,每次20 min,1次/d,连续干预7 d.抑制剂组在每次电针前1 h予双侧"委中"和"肾俞"穴位注射外泌体抑制剂GW4869(3 mg/mL,50 µL/穴).造模后第 7天取多裂肌,HE染色观察多裂肌组织形态变化,Masson染色观察多裂肌胶原纤维,免疫组织化学法观察配对盒转录因子 7(Pax7)、成肌分化抗原(MyoD)的阳性表达,提取各组大鼠血清外泌体并采用透射电子显微镜(TEM)、纳米颗粒追踪分析技术(NTA)进行鉴定,Western blot法检测各组大鼠多裂肌组织中肌细胞生成素(MyoG)、肌球蛋白重链(MyHC)及血清外泌体中CD63、程序性细胞死亡因子6相互作用蛋白(Alix)、肿瘤易感基因101蛋白(TSG101)的表达.结果:模型组大部分肌纤维变性坏死,肌纤维周围可见大量炎性细胞浸润,可见大片蓝染胶原纤维;电针组肌纤维形态较完整,新生肌纤维较多,损伤区炎性细胞减少,胶原纤维明显减少;抑制剂组肌纤维破坏及炎性细胞浸润仍较多,可见直径不均的新生肌纤维,胶原纤维较多.TEM、NTA及Western blot的结果均显示外泌体提取成功,电镜下其形态为典型茶托样,粒径范围集中分布在70~200 nm,标志蛋白CD63、Alix、TSG101均为阳性.与正常组比较,模型组多裂肌中Pax7的表达,血清外泌体Alix、CD63 表达升高(P<0.01,P<0.05,P<0.001).与模型组比较,电针组多裂肌中Pax7、MyoD、MyoG、MyHC表达,血清外泌体Alix、TSG101表达显著升高(P<0.01,P<0.05).与电针组比较,抑制剂组多裂肌中Pax7、MyoD、MyoG、MyHC表达,血清外泌体TSG101、CD63表达显著降低(P<0.01,P<0.05,P<0.001).结论:电针能显著上调损伤多裂肌Pax7、MyoD、MyoG和MyHC的表达,促进腰多裂肌再生修复,该作用可能与穴区外泌体释放有关.

Objective To observe the effect of electroacupuncture(EA)on the expressions of paired box transcription factor 7(Pax7),myogenic differentiation antigen(MyoD),myogenin(MyoG)and myosin heavy chain(MyHC)in the multifidus muscle,and CD63,programmed cell death protein 6 interacting protein(Alix)and tumor susceptibility gene 101(TSG101)proteins in the serum exosomes in rats with lumbar multifidus muscle injury(MFMI),so as to explore the effect of exosomes in acupoint areas on EA improvement of muscular regeneration and repair.Methods Forty male SD rats were randomly divided into normal control,model,EA and EA+exosome inhibitor(EA+inhibitor)groups,with 10 rats in each group.The MFMI model was established by injection of 0.5%bupivacaine(150 μL×4)into the 4 points of the multifidus muscle along the bilateral lumbar(L)4—L5 spinous processes.EA(2 Hz/10 Hz,1 mA)was applied to bilateral"Weizhong"(BL40)and"Shenshu"(BL23)for 20 min,once a day for 7 d.For rats of the EA+inhibitor group,exosome inhibitor GW4869(3 mg/mL,50 μL/acupoint)was injected into bilateral BL40 and BL23 1 h before each EA intervention.The morphological changes of the multifidus muscle were observed after H.E.staining and Masson staining.The immunoactivity of Pax7 and MyoD was observed by immunohistochemistry.The serum exosomes were extracted and identified by transmission electron microscope(TEM)and nanoparticle tracking analysis(NTA).The expression levels of MyoG and MyHC in the multifidus muscle tissue and CD63,Alix and TSG101 proteins in the serum exosomes were detected by Western blot.Results Morphological results showed that in the model group,most of the muscle fibers were degenerated and necrotic,a large number of inflammatory cells infiltrated around the muscle fibers and more blue-stained collagen fibers were observed.In the EA group,the morphology of muscle fibers was relatively complete,with more new muscle fibers and reduced inflammatory cells in the injured area,and the collagen fibers were significantly reduced.In the EA+inhibitor group,there were still more muscle fiber destruction and inflammatory cell infiltration,new muscle fibers with uneven diameter and more collagen fibers.Compared with the normal control group,the immunoactivity of Pax7 in the multifidus muscle,the expression of Alix and CD63 proteins in the serum exosomes were significantly increased in the model group(P<0.01,P<0.05,P<0.001).In comparison with the model group,the immunoactivity of Pax7 and MyoD,the expression levels of Alix and TSG101 in the serum exosomes and MyHC and MyoG proteins in the multifidus muscle were considerably up-regulated in the EA group(P<0.01,P<0.05).After local injection of GW4869 at BL40 and BL23,the immunoactivity of Pax7 and MyoD,the protein expression levels of TSG101,CD63,MyHC and MyoG were significantly lower in the EA+inhibitor group than those of the EA group(P<0.01,P<0.05,P<0.001).The results of TEM and NTA showed that the exosomes were successfully extracted.The morphology of the exosomes was typical saucer-like under electron microscope,and the particle size range was concentrated in 70-200 nm.Conclusion EA of BL40 and BL23 can significantly up-regulate the expressions of Pax7,MyoD,MyoG and MyHC in the injured multifidus muscle,and promote the regeneration and repair of lumbar multifidus muscle,which may be related to its functions in promoting the release of exosomes in the acupoint area.

吕宗泽;谢淼;陈颖;徐小琳;黄志宾;王迪霖;李文敏;温春娣;刘通

广州中医药大学第五临床医学院,广州 510095广州中医药大学第五临床医学院,广州 510095广州中医药大学第五临床医学院,广州 510095广州中医药大学第五临床医学院,广州 510095广州中医药大学第五临床医学院,广州 510095广东省第二中医院针灸康复科,广州 510095广东省第二中医院针灸康复科,广州 510095广东省第二中医院针灸康复科,广州 510095广州中医药大学第五临床医学院,广州 510095

电针多裂肌损伤穴位血清外泌体肌肉修复与再生

ElectroacupunctureMultifidus muscle injuryAcupointsSerum exosomesMuscle repair and regeneration

《针刺研究》 2026 (1)

1-10,10

国家自然科学基金面上项目(No.82174482)广东省特支计划青年拔尖人才项目(No.0720240248)广州地区中医药重大科技项目(No.2025CX001)广东省第二中医院青年培优项目广东省第二中医院院内基金项目(No.SEZYY2023B17)

10.13702/j.1000-0607.20241250

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