滋肾活血方对血管性痴呆大鼠分裂与融合蛋白Mfn1、Mfn2、Drp1、Fis1的影响

目的观察滋肾活血方对血管性痴呆(vascular dementia,VD)大鼠海马组织线粒体融合蛋白1(mitofusin 1,Mfn1)、线粒体融合蛋白2(mitofusin 2,Mfn2)、线粒体动力蛋白相关蛋白1(dynamin-related protein 1,Drp1)、线粒体分裂蛋白1(fission mitochondrial 1,Fis1)表达的影响。方法选用雄性SD大鼠60只,随机均分为假手术组、模型组、滋肾活血高剂量组、滋肾活血中剂量组、滋肾活血低剂量组、西药组。除假手术组外,其余各组均采用改良2-VO法建立VD大鼠模型。每组大鼠按9 mL/(kg·d)剂量灌胃相应药物。模型组、假手术组给予蒸馏水,滋肾活血低剂量组、滋肾活血中剂量组、滋肾活血高剂量组予以滋肾活血方溶液[9.8、17.8、35.6 g/(kg·d)]灌胃,西药组以多奈哌齐溶液[150 mg/(kg·d)]灌胃。连续喂药2周后,采用水迷宫实验评估大鼠学习记忆功能;取海马组织,采用免疫组化法检测实验大鼠海马组织中的Mfn1、Mfn2、Drp1、Fis1蛋白表达量。结果与假手术组比较,模型组大鼠逃避潜伏期(escape latency,EL)延长(P<0.05),Mfn1、Mfn2、Drp1蛋白的表达量降低(P<0.05)。与模型组对比,滋肾活血中、高剂量组大鼠EL缩短(P<0.05),Mfn1、Mfn2、Drp1蛋白表达量升高(P<0.05)。与滋肾活血低剂量组比较,滋肾活血中、高剂量组大鼠EL缩短(P<0.05),Mfn1、Drp1蛋白表达量升高(P<0.05)。结论滋肾活血方可能通过调节细胞内线粒体分裂与融合,上调Mfn1、Mfn2、Drp1蛋白的表达,从而改善认知功能。

FIS1 mRNA、HPV E6/E7 mRNA表达水平与宫颈病变严重程度的关系研究

目的 研究线粒体分裂蛋白1(FIS1)mRNA、人乳头瘤病毒(HPV)E6/E7 mRNA表达水平与宫颈病变严重程度的关系。方法 收集张家口市妇幼保健院2021年1月-2021年7月行宫颈癌筛查的5666例标本,经宫颈液基薄层细胞学检查(TCT)诊断285例不典型鳞状细胞(ASC)、183例鳞状上皮内低度病变(LSIL)、98例鳞状上皮内高度病变(HSIL)、10例宫颈癌;经病理活检诊断356例未明确诊断意义的不典型鳞状上皮细胞(ASCUS)、218例宫颈上皮内瘤样病变(CIN)Ⅰ级、42例CINⅡ级、24例CINⅢ级、15例宫颈鳞状细胞癌。分别参考TCT、病理活检诊断结果分析不同宫颈病变程度的FIS1 mRNA、HPV E6/E7 mRNA阳性检出率与表达量。通过Pearson分析FIS1 mRNA与HPV E6/E7 mRNA阳性表达与宫颈病变严重程度的相关性。结果 以TCT不同诊断级别为参考,FIS1 mRNA、HPV E6/E7 mRNA表达对LSIL、HSIL、宫颈鳞状细胞癌的阳性检出率高于ASC(P<0.05)。FIS1 mRNA、HPV E6/E7 mRNA表达对宫颈鳞状细胞癌的阳性检出率高于LSIL(P<0.05)。FIS1 mRNA拷贝数:宫颈癌、HSIL<LSIL<ASC(P<0.05);HPV E6/E7 mRNA拷贝数:宫颈癌>HSIL>LSIL>ASC(P<0.05)。以病理活检结果为诊断标准,FIS1 mRNA、HPV E6/E7 mRNA表达对CINⅡ级、CINⅢ级、宫颈鳞状细胞癌的阳性检出率高于ASCUS、CINⅠ级(P<0.05);FIS1 mRNA拷贝数:宫颈鳞状细胞癌、CINⅢ级<CINⅡ级<CINⅠ级<ASCUS(P<0.05);HPV E6/E7 mRNA拷贝数:宫颈鳞状细胞癌>CINⅢ级>CINⅡ级>CINⅠ级、ASCUS(P<0.05)。Pearson相关性分析结果显示,宫颈病变严重程度与FIS1 mRNA表达量呈显著负相关性(r=-0.881,P<0.05),与HPV E6/E7 mRNA表达量呈显著正相关性(r=0.903,P<0.05)。结论 FIS1 mRNA、HPV E6/E7 mRNA表达水平与宫颈病变程度存在显著相关性,宫颈病变程度越严重,FIS1mRNA表达量呈降低趋势,而HPV E6/E7 mRNA表达量呈上升趋势。

PTEN-induced kinase 1-induced dynamin-related protein 1 Ser637 phosphorylation reduces mitochondrial fission and protects against intestinal ischemia reperfusion injury

BACKGROUND Intestinal ischemia reperfusion(I/R)occurs in various diseases,such as trauma and intestinal transplantation.Excessive reactive oxygen species(ROS)accumulation and subsequent apoptotic cell death in intestinal epithelia are important causes of I/R injury.PTEN-induced putative kinase 1(PINK1)and phosphorylation of dynamin-related protein 1(DRP1)are critical regulators of ROS and apoptosis.However,the correlation of PINK1 and DRP1 and their function in intestinal I/R injury have not been investigated.Thus,examining the PINK1/DRP1 pathway may help to identify a protective strategy and improve the patient prognosis.AIM To clarify the mechanism of the PINK1/DRP1 pathway in intestinal I/R injury.METHODS Male C57BL/6 mice were used to generate an intestinal I/R model via superior mesenteric artery occlusion followed by reperfusion.Chiu’s score was used to evaluate intestinal mucosa damage.The mitochondrial fission inhibitor mdivi-1 was administered by intraperitoneal injection.Caco-2 cells were incubated in vitro in hypoxia/reoxygenation conditions.Small interfering RNAs and overexpression plasmids were transfected to regulate PINK1 expression.The protein expression levels of PINK1,DRP1,p-DRP1 and cleaved caspase 3 were measured by Western blotting.Cell viability was evaluated using a Cell Counting Kit-8 assay and cell apoptosis was analyzed by TUNEL staining.Mitochondrial fission and ROS were tested by MitoTracker and MitoSOX respectively.RESULTS Intestinal I/R and Caco-2 cell hypoxia/reoxygenation decreased the expression of PINK1 and p-DRP1 Ser637.Pretreatment with mdivi-1 inhibited mitochondrial fission,ROS generation,and apoptosis and ameliorated cell injury in intestinal I/R.Upon PINK1 knockdown or overexpression in vitro,we found that p-DRP1 Ser637 expression and DRP1 recruitment to the mitochondria were associated with PINK1.Furthermore,we verified the physical combination of PINK1 and p-DRP1 Ser637.CONCLUSION PINK1 is correlated with mitochondrial fission and apoptosis by regulating DRP1 phosphorylation in intestinal I/R.These results suggest that the PINK1/DRP1 pathway is involved in intestinal I/R injury,and provide a new approach for prevention and treatment.

Selective brain hypothermia-induced neuroprotection against focal cerebral ischemia/reperfusion injury is associated with Fis1 inhibition

Selective brain hypothermia is considered an effective treatment for neuronal injury after stroke,and avoids the complications of general hypothermia.However,the mechanisms by which selective brain hypothermia affects mitochondrial fission remain unknown.In this study,we investigated the effect of selective brain hypothermia on the expression of fission 1 (Fis1) protein,a key factor in the mitochondrial fission system,during focal cerebral ischemia/reperfusion injury.Sprague-Dawley rats were divided into four groups.In the sham group,the carotid arteries were exposed only.In the other three groups,middle cerebral artery occlusion was performed using the intraluminal filament technique.After 2 hours of occlusion,the filament was slowly removed to allow blood reperfusion in the ischemia/reperfusion group.Saline,at 4℃ and 37℃,were perfused through the carotid artery in the hypothermia and normothermia groups,respectively,followed by restoration of blood flow.Neurological function was assessed with the Zea Longa 5-point scoring method.Cerebral infarct volume was assessed by 2,3,5-triphenyltetrazolium chloride staining,and apoptosis was assessed by terminal deoxynucleotidyl transferase-mediated dUTP nick-end labeling staining.Fis1 and cytosolic cytochrome c levels were assessed by western blot assay.Fis1 mRNA expression was assessed by quantitative reverse transcription-polymerase chain reaction.Mitochondrial ultrastructure was evaluated by transmission electron microscopy.Compared with the sham group,apoptosis,Fis1 protein and mRNA expression and cytosolic cytochrome c levels in the cortical ischemic penumbra and cerebral infarct volume were increased after reperfusion in the other three groups.These changes caused by cerebral ischemia/reperfusion were inhibited in the hypothermia group compared with the normothermia group.These findings show that selective brain hypothermia inhibits Fis1 expression and reduces apoptosis,thereby ameliorating focal cerebral ischemia/reperfusion injury in rats.Experiments were authorized by the Ethics Committee of Qingdao Municipal Hospital of China (approval No.2019008).

黄芪多糖通过调节Drp1介导的线粒体分裂改善感染性心肌病

目的从线粒体动力相关蛋白1(Dp1)介导线粒体分裂平衡角度,解读黄芪多糖(APS)对感染性心肌病小鼠的心功能保护作用及机制。方法按随机数字表法将18只成年雄性C57BL/6J小鼠分为对照组、脂多糖(LPS)组和LPS+APS组,每组6只。采用LPS诱导制备感染性:心肌病模型。各组均于术后6h经尾静脉取外周血,采用酶联免疫吸附试验(ELISA)检测小鼠血清炎性因子水平;LPS处理后24 h行超声心动图检查心室功能,包括左室射血分数(LVEF)、左室短轴缩短率(LVFS)、左室舒张期末内径(LVEDD)和左室收缩期末内径(LVESD);检查后即刻处死小鼠取心肌组织,采用蛋白质印迹试验(Western bloting)检测肿瘤坏死因子-α(TNF-α)、白细胞介素-6(IL-6)、C3a、Drp1、线粒体分裂蛋白1(Fis1)、线粒体融合蛋白2(Mfn2)、视神经菱缩蛋白1(Opa1)蛋白表达。将购买的小鼠心房肌细胞株HL-1分为对照组、LPS组、LPS+APS组和LPS+APS+线粒体氧化磷酸化解偶联剂(FCCP)组。采用活性氧(ROS)检测试剂盒检测分离线粒体及HL-1细胞内的ROS含量:采用线粒体膜电位检测试剂盒(JC-1)检测线粒体膜电位(MMP);采用三磷酸腺背(ATP)检测试剂盒检测HL-1细胞内ATP含量。结果与对照组比较.LPS组小鼠心脏的LVEF、LNFS、LVEDD和LVESD均明显降低.线粒体内ROS含量明显升高,MMP和ATP含量均明显下降;而APS可改善感染性心肌病小鼠的心功能指标[LVEF:0.571±0.026比0.287±0.045.LVFS(%):33.13±2.11比21.22±0.99.LVEDD(mm):3.74±0.10比2.77±0.05.LVESD(mm):2.74±0.09比1.99±0.04.均P<0.05].明显降低心肌内ROS含量[ROS(%):138.39±9.28比260.97±19.22.P<0.05].明显抑制MMP和ATP含量下降[MMP(红色1绿色荧光强度比值):0.91±0.05比0.55±0.01,ATP(%):94.22±10.11比58.74±5.39.均P<0.05),且APS可明显抑制LPS处理后的Drp1和Fis1蛋白过表达以及MIn2和Opal蛋白低表达[Drp1/GAPDH(%):126.33±11.70比218.75±19.44,Fis1/CAPDH(%):105.71±15.77比194.39±5.27,Mfn2/CAPDH(%):92.75±10.44比41.88±3.95,0pa1/CAPDH(%):98.14±3.71比55.94±7.30.均P<0.05]。故进一步采用HL-1细胞构建感染性心肌病模型,HL-1细胞经FCCP处理后可明显抑制APS的保护效应。结论APS通过抑制Drp1过表达,抑制线粒体的过度分裂,减轻感染性心肌细胞的氧化应激和线粒体损伤,最终改善心脏功能,该机制的发现可为感染性心肌病的治疗提供新的理论依据和临床参考。

Drp1在高糖诱导的大鼠心肌细胞肥大中的作用研究

目的:探讨发动蛋白相关蛋白1(Drp1)在高糖诱导的心肌细胞肥大模型中的表达及其作用机制。方法:原代乳大鼠心肌细胞培养,用高糖诱导建立心肌细胞损伤模型,将细胞分为对照组、高渗透压组、DMSO组、高糖组和高糖+线粒体分裂抑制剂1(Mdivi-1)组。用麦胚凝集素荧光染色检测单个心肌细胞表面积;用线粒体膜电位(MMP)检测试剂盒(JC-1)检测心肌细胞MMP水平;Western blot检测心肌细胞肥大标志物心房钠尿肽(ANP)及Drp1和Drp1在Ser616/Ser637位点的磷酸化蛋白[p-Drp1(Ser616/Ser637)]的蛋白水平。结果:与对照组相比,高渗透压组各检测结果均无显著差异(P>0.05)。与对照组和高渗透压组相比,高糖组心肌细胞的表面积均显著增大(P<0.01),MMP显著降低(P<0.01),而Drp1总蛋白表达无显著变化(P>0.05);心肌细胞ANP表达显著增加(P<0.01),p-Drp1(Ser616)水平显著升高(P<0.05),而p-Drp1(Ser637)水平显著降低(P<0.05)。与高糖组相比,高糖+Mdivi-1组ANP和p-Drp1(Ser616)蛋白水平显著降低(P<0.05),而p-Drp1(Ser637)的水平显著升高(P<0.05)。结论:高糖诱导心肌细胞肥大的机制,与Drp1在Ser616位点磷酸化水平升高、Ser637位点磷酸化水平降低导致的线粒体分裂增加有关。

动力相关蛋白1抑制剂减轻糖尿病小鼠心肌缺血/再灌注损伤

目的探究动力相关蛋白(Dynamin-related protein,Drp)1抑制剂Mdivi-1对糖尿病小鼠心肌缺血/再灌注(Myocardial ischemia/reperfusion,MI/R)损伤的作用及其机制。方法高脂饮食加小剂量链脲佐菌素(STZ)诱导建立糖尿病小鼠模型。造模成功的糖尿病小鼠进行MI/R处理,再灌注前15 min腹腔注射Mdivi-1(1.2 mg/kg)或其溶剂二甲基亚砜。主要评价指标包括线粒体形态、心脏功能、心肌损伤及凋亡,蛋白免疫印迹检测Drp1表达。结果糖尿病MI/R后线粒体分裂增加(P<0.01),线粒体Drp1转位明显增加(P<0.01),Mdivi-1可抑制缺血/再灌注心肌的Drp1线粒体转位及线粒体分裂,减少心肌梗死面积和心肌细胞凋亡(P<0.01),减轻氧化应激(P<0.05)。结论 Drp1介导的线粒体分裂增加参与了糖尿病MI/R损伤,Drp1抑制剂Mdivi-1可抑制线粒体分裂,减轻糖尿病MI/R损伤。

线粒体分裂蛋白1在人宫颈癌细胞中过表达能促进线粒体裂变并降低细胞的增殖和迁移能力

线粒体是持续进行分裂和融合的动态细胞器。近年来,除了线粒体代谢作用相关的研究之外,线粒体动力学也开始逐渐引起研究的关注。越来越多的研究表明,线粒体动力学与肿瘤细胞生物学行为具有相关性。线粒体分裂蛋白1(mitochondrial fission protein 1,FIS1)介导线粒体分裂复合物的组装,参与线粒体分裂,是线粒体融合分裂过程中重要的蛋白质。然而,鲜有研究揭示FIS1在人宫颈癌中的表达及其作用。本研究对比了宫颈癌组织以及癌旁组织的转录物组数据,结果显示,与癌旁组织相比,人宫颈癌组织中的FIS1 mRNA水平明显降低(P<0.01)。进一步进行宫颈癌组织FIS1高表达组与低表达组的差异基因分析,发现差异基因主要与线粒体功能相关。随后,进行FIS1过表达后HeLa细胞增殖、迁移、线粒体裂变以及ROS水平的相关分析。结果显示,过表达FIS1基因,HeLa细胞增殖及迁移能力显著降低,细胞内线粒体裂变程度加剧并且细胞内ROS水平升高。综合以上结果,FIS1在人宫颈癌细胞中表达水平较低,而过表达FIS1可促使宫颈癌细胞因线粒体动力学失衡而发生一系列生物学功能异常。因此,本研究为进一步研究FIS1在宫颈癌治疗中的作用奠定了重要基础。

杨梅素通过促进DRP1依赖性线粒体分裂诱导人卵巢癌SKOV3细胞凋亡

目的:观察杨梅素与mdivi-1分别或联合作用于人卵巢癌SKOV3细胞后细胞凋亡和线粒体分裂情况,探讨杨梅素诱导SKOV3细胞凋亡的机制。方法:体外培养SKOV3细胞,随机分为对照组、mdivi-1组、杨梅素组和联合给药组,mdivi-1组以50μmol·L^(-1) mdivi-1作用1h后更换普通细胞培养液继续培养23h,杨梅素组以50g·L^(-1)杨梅素作用24h,联合给药组以50μmol·L^(-1) mdivi-1作用1h后更换含50g·L^(-1)杨梅素的细胞培养液继续培养23h。MTT法检测各组细胞存活率;Muse~凋亡检测试剂盒检测各组细胞凋亡率;蛋白免疫印迹法(Western blotting)观察细胞色素C(Cyt C)、半胱氨酸天冬氨酸蛋白酶3(caspase3)、动力相关蛋白1(DRP1)和分裂蛋白1(FIS1)表达水平;MitoTracker~ Red荧光探针特异性标记线粒体观察各组细胞线粒体分裂情况。结果:与对照组比较,杨梅素组细胞存活率明显降低(P<0.05);与杨梅素组比较,联合给药组细胞存活率明显升高(P<0.05)。与对照组比较,杨梅素组细胞凋亡率升高(P<0.05);与杨梅素组比较,联合用药组细胞凋亡率明显降低(P<0.05)。与对照组比较,杨梅素组细胞中Cyt C和caspase3蛋白表达水平明显升高(P<0.05);与杨梅素组比较,联合用药组Cyt C和caspase3蛋白表达水平明显降低(P<0.05)。与对照组比较,杨梅素组细胞线粒体分裂程度增强;与杨梅素组比较,联合用药组线粒体分裂程度下降。与对照组比较,杨梅素组细胞中DRP1和FIS1蛋白表达水平升高(P<0.05);与杨梅素组比较,联合用药组DRP1和FIS1蛋白表达水平降低(P<0.05)。结论:杨梅素可通过促进DRP1依赖性线粒体分裂诱导人卵巢癌SKOV3细胞凋亡。

Drp1在糖尿病心肌病中的作用机制研究进展

糖尿病心肌病是糖尿病患者严重的慢性不可逆心血管并发症之一。近年来研究发现,线粒体动力学平衡紊乱导致的线粒体功能障碍与糖尿病心肌病的发生密切相关。动力相关蛋白1(Drp1)是线粒体分裂的重要调节因子。研究表明,糖尿病心肌细胞中Drp1活性增强可导致线粒体分裂增加、融合减少,从而引起线粒体功能障碍。Drp1通过诱发心肌细胞氧化应激、能量代谢障碍、细胞凋亡、胰岛素抵抗和脂毒性,导致糖尿病心肌病的发生发展。此外,抑制Drp1的活性可改善糖尿病心肌病的心脏功能。本文对Drp1在糖尿病心肌病中的作用机制进行综述,以期为糖尿病心肌病的防治和药物研发提供新思路。

线粒体动态相关蛋白1在阿尔茨海默病线粒体动态学中的作用机制研究进展（英文）

线粒体动态在哺乳动物细胞内发挥重要作用。在健康细胞内,线粒体保持分裂与融合的动态平衡。线粒体动态相关蛋白1(Drp1)在神经细胞轴突和树突部位线粒体分裂动态调控中发挥枢纽作用。对阿尔茨海默症患者的研究证明,Drp1表达及功能变化会破坏线粒体分裂与融合的动态平衡并导致患者海马细胞的功能损坏或缺失。因此,Drp1具有成为以调节线粒体动态为机制的阿尔茨海默病治疗新方案中的全新药物靶点蛋白。

敲减抗增殖蛋白2促进非小细胞肺癌细胞系A549凋亡

目的探讨抑制抗增殖蛋白2(PHB2)表达对非小细胞肺癌细胞系A549凋亡的影响及机制。方法慢病毒感染非小细胞肺癌细胞系A549,建立敲减PHB2的稳转细胞株,用动力相关蛋白1(DRP1)抑制剂Mdivi-1处理敲减PHB2的A549细胞。Western blot检测PHB2、p-DRP1(Ser616)和DRP1蛋白表达水平;TUNEL染色和annexin V-FITC/PI双染检测细胞凋亡;MitoTracker染色评估线粒体分裂情况;用相应试剂盒检测线粒体含量、柠檬酸合酶活性和细胞色素c含量。结果与shCtrl组相比,shPHB2组A549细胞凋亡率增加(P<0.05),DRP1介导的线粒体分裂增加(P<0.05),ATP含量减少(P<0.05),柠檬酸合酶活性降低(P<0.05),线粒体内细胞色素c减少(P<0.05)。与shPHB2组相比,shPHB2+Mdivi-1组A549细胞凋亡率减少(P<0.05),DRP1介导的线粒体分裂减少(P<0.05),ATP含量增加(P<0.05),柠檬酸合酶活性增加(P<0.05),线粒体内细胞色素c增加(P<0.05)。结论抑制PHB2促进A549细胞凋亡,其机制可能与促进DRP1介导的线粒体分裂有关。

FISSION 1A and FISSION 1 B Proteins Mediate the Fission of Peroxisomes and Mitochondria in Arabidopsis

Peroxisomes and mitochondria are metabolically diverse organelles that act in concert in a number of pathways in eukaryotes, including photorespiration and lipid mobilization in plants. The division machineries of these two types of organelles also share several components such as dynamin-related proteins （DRPs） and their organelle anchor, the FISSION1 （FIS1） protein. In Arabidopsis, members of the DRP3 and FIS1 small protein families, namely DRP3A, DRP3B, FISIA, and FISIB, are each dual-targeted to peroxisomes and mitochondria and are required for the division of both organelles; DRP3A and DRP3B are partially redundant in function. To further determine the contribution of FISIA and FISIB to the division of peroxisomes and mitochondria, we analyzed plants overexpressing FISIA or FISIB and mutants in which the functions of both proteins were disrupted. Domains in FISIA and FISIB required for peroxisomal targeting were also dissected. Our results demonstrate that FISIA and FISIB play rate-limiting and partially overlapping roles in promoting the fission of peroxisomes and mitochondria. Furthermore, although the C-terminus of FIS1 is both necessary and sufficient for targeting to peroxisomes, the role of the short C-terminal segment adjacent to the transmembrane domain may differ among diverse species in peroxisomal targeting.

线粒体动力相关蛋白1在炎症性肺实质疾病中的作用机制及研究进展

线粒体动力相关蛋白1(Drp1)作为介导线粒体分裂的主要蛋白,对维持线粒体的形态、功能和完整性至关重要,并参与细胞的生理活动及疾病的发生、发展进程,尤其在炎症性肺实质疾病的能量代谢中发挥关键调节作用。文章探讨了Drp1的结构与功能,并对其在急性呼吸窘迫综合征、肺动脉高压、哮喘、慢性阻塞性肺疾病中的作用机制进行综述,为炎症性肺实质疾病的防治提供理论依据。

线粒体分裂相关蛋白高表达参与阿霉素大鼠肾病模型蛋白尿的发生

目的:探讨肾小球线粒体动力相关蛋白1(Drp1)、P-Drp1(Ser616)和线粒体分裂蛋白1(Fis1)表达与足细胞损伤及蛋白尿发生的关系。方法:建立阿霉素大鼠肾病模型,用免疫组化和western blot检测肾小球和肾皮质Drp1、P-Drp1(Ser616)及Fis1的表达,分析上述蛋白表达与蛋白尿及足细胞线粒体形态的相关性。在小鼠足细胞系MPC5过表达Drp1,分析对凋亡和线粒体形态的影响。结果:肾小球和肾皮质Drp1在阿霉素大鼠肾病模型4周和6周时表达增强,肾小球P-Drp1(Ser616)在6周时表达增强,肾小球Fis1在2周和6周时增强。肾小球和肾皮质Drp1、肾小球P-Drp1(Ser616)和Fis1表达与24h尿蛋白正相关。肾小球Drp1表达量与足细胞线粒体胞浆密度和线粒体细胞密度呈负相关。肾小球P-Drp1(Ser616)与足细胞线粒体最大长宽比呈负相关。肾小球Fis1与足细胞线粒体面积和周长呈负相关。过表达Drp1致小鼠足细胞凋亡显著增多,线粒体片段化。结论:肾小球Drp1、P-Drp1(Ser616)与Fis1高表达参与阿霉素大鼠肾病模型蛋白尿的发生,Drp1高表达致线粒体片段化和足细胞凋亡。

Dynamin-related protein 1在线粒体分裂和细胞凋亡中的作用

Dynamin-related protein 1属于动力蛋白GTP酶超家族,是线粒体分裂体系的组成成分,在线粒体分裂中具有重要作用。在不同物种中,dynamin-related protein 1在与多种分子相互作用后,可以定位于线粒体并组装成高级结构,引起膜的收缩和分裂。Dynamin-related protein 1功能的消失会增强线粒体的融合和线粒体之间的连通性。Dynamin-related protein 1在细胞凋亡等多种细胞功能中也具有重要作用。

CORM-2通过p38MAPK信号通路对脂多糖刺激大鼠肺巨噬细胞中线粒体分裂蛋白Fis1的影响

目的探讨CORM-2通过p38分裂原激活蛋白激酶（p38MAPK）信号通路对脂多糖（LPS）刺激大鼠肺巨噬细胞中线粒体分裂蛋白Fisl的影响。方法将传代培养的大鼠肺泡巨噬细胞以2×105／mL密度接种于96孔板。培养24h后，采用随机数字表法将其分为4组：正常对照组（C组）、LPS组（L组）、CO释放剂CORM-2＋LPS组（LC组）、p38MAPK抑制剂SB203580＋CORM-2＋LPS组（LCS组）。细胞孵育24h时，应用试剂盒测定线粒体MDA含量及SOD活力，应用Westernblot测定HO-1、线粒体相关分裂蛋白Fisl和p38的表达。应用RT—PCR测定HO-1和FislmRNA含量的表达。结果与c组比较，L组MDA[2．43±0．12 vs．3．59±0．07]含量、HO-1[1．31±0．27 vs．1．65±0．41]、Fisl[1．27±0．23 vs．1．65±0．41]、p38[1．01±0．24 vs．1．36±0．17]表达水平升高，SOD[81．7±1．62 vs．54．7±1．62]活力降低（P〈0、05）；与L组比较，Lc组MDA[3．59±0．07 vs．3．08±0．52]含量、Fisl[2．01±0．35 vs．1．48±0．39]表达水平降低，SOD[54．7±1．62VS．67．4±1．32]活力、HO-1[1．65±0．41 vs．2．25±0．18]、p38[1．36±0．17 vs．1．78±0．23]表达水平升高（P〈0、05）；与LC组比较，LCS组MDA[3．08±0．52vs．4．16±0．19]含量、Fisl[1．48±0．39vs．1．96±0．31]表达水平升高，SOD[67．4±1．32vs．45．9±1．52]活力、HO-1[2．25±0．18 vs．1．78±0．19]、p38[1．78±0．23VS．1．12±0．29]表达水平降低（P〈0、05）。结论HO-1／CO抑制LPS刺激大鼠肺巨噬细胞中线粒体分裂蛋白Fisl表达机制与p38MAPK信号通路有关。

磷酸甘油酸变位酶5与坏死样凋亡

多年来人们认为细胞死亡方式主要包括坏死和凋亡。坏死是不受特定调控的被动死亡方式，表现为细胞器肿胀，细胞膜破裂，内容物渗出，有炎症反应[1]，而凋亡则是由细胞内胱天蛋白酶（caspase）调控的一种主动死亡方式，因caspase激活导致细胞内底物裂解，破坏胞膜囊泡形成凋亡小体，死亡过程中无内容物渗出，不引起炎症反应[2]。

线粒体动力学调控对肾缺血-再灌注损伤的影响

缺血-再灌注损伤(IRI)是肾移植术后早期移植肾功能障碍的主要原因之一。我国器官移植已经进入公民逝世后器官捐献时代,供者心肺复苏风险增加、低灌注时间和热缺血时间延长等可导致移植肾IRI,影响受者和移植肾的近期及远期临床结局。在IRI等应激状态下,以线粒体分裂和融合的动态调控为主要表现的线粒体动力学机制对线粒体的生物学功能具有重要影响,其损伤引发的细胞凋亡是导致急性肾损伤的关键环节,主要表现为线粒体动力学调控机制失调。本文综述了线粒体动力学调控对肾IRI影响机制的研究进展,以期为改善肾移植临床结局提供参考。

Rescue axonal defects by targeting mitochondrial dynamics in hereditary spastic paraplegias

Impaired axonal development and degeneration underlie debilitating neurodegenerative diseases including hereditary spastic paraplegia, a large group of inherited diseases. Hereditary spastic paraplegia is caused by retrograde degeneration of the long corticospinal tract axons, leading to progressive spasticity and weakness of leg and hip muscles. There are over 70 subtypes with various underlying pathophysiological processes, such as defective vesicular trafficking, lipid metabolism, organelle shaping, axonal transport, and mitochondrial dysfunction. Although hereditary spastic paraplegia consists of various subtypes with different pathological characteristics, defects in mitochondrial morphology and function emerge as one of the common cellular themes in hereditary spastic paraplegia. Mitochondrial morphology and function are remodeled by mitochondrial dynamics regulated by several key fission and fusion mediators. However, the role of mitochondrial dynamics in axonal defects of hereditary spastic paraplegia remains largely unknown. Recently, studies reported perturbed mitochondrial morphology in hereditary spastic paraplegia neurons. Moreover, downregulation of mitochondrial fission regulator dynamin-related protein 1, both pharmacologically and genetically, could rescue axonal outgrowth defects in hereditary spastic paraplegia neurons, providing a potential therapeutic target for treating these hereditary spastic paraplegia. This mini-review will describe the regulation of mitochondrial fission/fusion, the link between mitochondrial dynamics and axonal defects, and the recent progress on the role of mitochondrial dynamics in axonal defects of hereditary spastic paraplegia.