STF-083010对肾脏缺血-再灌注损伤的保护作用

目的 观察STF083010对急性肾缺血-再灌注损伤的作用,探讨其损伤保护作用的机制.方法 选择健康雄性SD大鼠30只,随机分为假手术组(打开腹腔)、I-R组(建立大鼠肾I-R损伤模型)与STF083010组.分别在缺血-再灌注24h后处死大鼠,取血液和肾组织.全自动生化仪检测各组血清尿素氮(BUN)及肌酐(Scr)水平.PAS染色观察大鼠肾组织病理变化,免疫组化检测肾脏组织中XBP1、GRP78蛋白的表达.Quantitative real-time PCR(QPCR)测定大鼠肾组织标本中XBP1、GRP78 mRNA水平.结果 I-R组肌酐、尿素氮水平与假手术组相比差异均有统计学意义(P＜0.05).STF-083010组与I-R组相比,差异亦有统计学意义(P＜0.05).PAS病理图片可见STF-083010组肾小管损伤较I-R组明显减轻(P＜0.05);免疫组化检测显示STF-083010组XBP1的表达较I-R组明显降低(P＜0.05),STF-083010组GRP78蛋白的表达较I/R组明显升高;QPCR结果显示STF-083010组XBP1 mRNA水平较I-R组明显降低(P＜0.05),STF-083010组GRP78 mRNA较I-R组明显升高(P＜0.05).结论 STF-083010可以对大鼠肾脏缺血-再灌注损伤性保护作用.     

大鼠肺早期缺血再灌注损伤时线粒体DNA的表达及意义

目的 探讨线粒体DNA(mtDNA)在大鼠肺缺血再灌注损伤过程中的表达变化及意义.方法 32只雄性SD大鼠,分为4组:缺血再灌注1组(IR1组)大鼠按照原位缺血再灌注模型的制作方法缺血1h,再灌注0.5 h;缺血再灌注2组(IR2组),采用相同方法,缺血1h,再灌注1h;假手术对照1组(Con1组),开胸1.5h;假手术对照2组(Con2组),开胸2h.实验结束时分别处死各组大鼠,心脏采血,完整取下左肺.行HE染色,观察各组肺组织病理变化;测量肺湿重/干重,计算肺含水量;提取外周血DNA,荧光定量实时聚合酶链法测定各组大鼠外周血循环mtDNA表达量;酶联免疫吸附法测定各组大鼠肺组织中基质金属蛋白酶9(MMP-9)和单核细胞趋化蛋白1(MCP-1)含量.结果 与Con1组和Con2组相比较,IR1组和IR2组大鼠肺组织损伤加重,炎症细胞浸润、肺泡腔内渗出显著增多,肺水含量也升高(P＜0.01).IR1组大鼠外周血中mtDNA含量高于Con1组,IR2组大鼠外周血中mtDNA含量高于Con2组,差异均有统计学意义(P＜0.01,P＜0.01).与Con1组相比较,IR1组大鼠肺组织MMP-9和MCP-1的表达的差异无统计学意义(P＞0.05);而与Con2组相比较,IR2组大鼠肺组织MMP-9和MCP-1的表达升高(P＜0.01).结论 大鼠原位肺缺血再灌注损伤早期,循环中mtDNA明显升高,其表达与肺组织中MMP-9、MCP-1的表达具有相关性.     

中介素减轻大鼠肾脏缺血再灌注损伤

目的 探讨中介素(IMD)对大鼠肾脏缺血再灌注损伤(IRI)的影响,及其过程中一氧化氮合酶(NOS)的作用和机制.方法 将健康雄性Wistar大鼠分为4组:假手术组,行右肾切除术,1周后单纯分离左侧肾蒂及肾动脉,而不夹闭肾动脉；肾脏缺血再灌注(IR)组,行右肾切除术,1周后行左肾缺血再灌注手术；IMD基因转染组,右肾切除后左肾行超声微泡介导的IMD-pCDNA3.1(+)质粒转染术,饲养1周,再行左肾缺血再灌注手术；空质粒转染组,右肾切除后左肾行超声微泡介导的pCDNA3.1(+)质粒转染术,饲养1周,再行左肾缺血再灌注手术.大鼠于缺血再灌注术后24 h处死,用免疫组织化学方法检测肾组织IMD表达,取肾组织进行病理学观察,取血清测定尿素氮(BUN)和肌酐(Cr)浓度,检测肾组织中内皮型NOS(eNOS)、诱导型NOS(iNOS)以及神经型NOS(nNOS) mRNA及其蛋白的表达.结果 假手术组大鼠肾组织中IMD位于肾小管及间质细胞胞浆内,其表达灰度值为66±35;肾脏IR组大鼠肾小管上皮细胞和间质中IMD表达灰度值为176±48,高于假手术组(P＜0.01)；IMD基因转染组肾组织中IMD表达灰度值为262±68,高于肾脏IR组(P＜0.01)；空质粒转染组IMD表达灰度值为180±51,和肾脏IR组间表达的差异无统计学意义(P＞0.05).与肾脏IR组相比较,IMD基因转染组大鼠肾脏组织病理损伤程度较轻,血清BUN和Cr较低(P＜0.05),eNOS mRNA及eNOS表达升高(P＜0.05),iNOS mRNA及iNOS表达降低(P＜0.05),而两组间nNOSmRNA及nNOS表达的差异无统计学意义(P＞0.05).结论 中介素可能通过促进eNOS表达、抑制iNOS表达从而减轻大鼠肾脏IRI.     

内质网应激分子伴侣GRP78在大鼠缺血再灌注损伤肝脏中的表达

目的:观察内质网应激相关分子葡萄糖调节蛋白78(GRP78)在大鼠缺血再灌注损伤肝脏组织中的表达水平.方法:将24只健康雄性SD大鼠随机均分为假手术组,单纯肝缺血组(肝缺血30 min+再灌注0h),再灌注6h组(肝缺血30 min+再灌注6h)和再灌注12h组(肝缺血30 min+再灌注12h).分别检测各组血清丙氨酸转氨酶(ALT)和门冬氨酸转氨酶(AST)水平;肝组织病理学、凋亡情况及GRP78 mRNA表达水平.结果:与对照组比较,各实验组大鼠肝缺血后出现明显的肝组织损伤,且随着再灌注时间的延长损伤加重,表现为血清ALT和AST水平升高,明显的肝组织病理学改变,肝细胞凋亡率增加,各组间计量指标的差异均有统计学意义(均P＜0.05).大鼠肝组织GRP78 mRNA变化趋势与上述指标一致,缺血后表达明显上调,且随着再灌注时间延长而逐渐升高,各组间差异均有统计学意义(均P＜0.05).结论:缺血再灌注损伤肝脏组织中GRP78表达上调,但其具体作用还有待于探明.     

纤维蛋白肽Bβ15～42对大鼠缺血再灌注损伤肾脏局部炎性反应的影响

目的 观察纤维蛋白肽Bβ15～42(the fibrin-derived peptide Bβ15-42,FgBβ15～42肽)对大鼠肾脏缺血再灌注损伤(IRI)后肾脏局部炎性反应的影响并探讨其机制.方法 将SD大鼠随机分成假手术组(Sham组)、IRI组、阴性治疗组和FgBβ15 ～ 42肽治疗组.Sham组:分离肾动脉后关闭腹腔;IRI组:采用双侧肾动脉夹闭的方法制作肾脏IRI模型;阴性治疗组:于肾脏再灌注后立即尾静脉注射随机肽段3.6 mg/kg; FgBβ15～42肽治疗组:于肾脏再灌注后立即尾静脉注射FgBβ15～ 42肽3.6 mg/kg.后3组按照再灌注24h、48 h分为两个亚组,Sham组与各亚组均为8只大鼠.常规生化法检测肾功能;HE、PAS染色观察肾脏组织学改变;免疫组化、实时荧光定量PCR法及Western印迹检测肾组织白细胞介素1β(IL-1β)、细胞间黏附分子1(ICAM-1)的mRNA及蛋白表达.结果 与Sham组相比,IRI组的Scr和BUN水平均显著增加(均P ＜0.05),肾小管及间质病理损伤显著,以再灌注48 h更为明显;与IRI组相比,FgBβ15～ 42肽治疗组Scr和BUN显著下降(均P＜0.05),小管间质损伤程度明显减轻(P＜0.05).与Sham组相比,IRI组IL-1β和ICA M-1的mRNA和蛋白水平于再灌注24h显著上升,48 h稍微下降,但仍维持在较高水平;FgBβ15～ 42肽治疗组大鼠肾组织IL-1β和ICAM-1的表达于再灌注24h、48 h显著低于同时间点的IRI组(均P＜0.05),但仍明显高于Sham组.上述各指标在阴性治疗组和IRI组之间的表达差异无统计学意义.结论 FgBβ15～42肽对肾脏IRI具有保护作用,其作用机制可能与其减少炎性因子IL-1β、黏附分子ICAM-1的表达有关.     

肾缺血再灌注损伤后miR-210及其靶基因的变化

目的 观察缺血再灌注损伤(IRI)对小鼠肾脏mir-210及其靶基因Ephrin-A3表达的影响.方法 将10只成年昆明雌鼠随机分为缺血再灌注组(IR)、假手术组(Sham),每组5只.IR组完全阻断双肾蒂40 min后恢复血流,Sham组暴露左右双肾40 min后关闭腹腔.每组在手术4 h后取肾组织标本,采用实时定量聚合酶链反应(PCR)检测mir-210表达水平;RT-PCR和酶标免疫组织化学染色法检测Ephrin-A3基因和蛋白的表达情况.结果 IR组miR-210表达水平明显上升(P<0.05).因miR-210对靶基因Ephrin-A3的负向调节作用,PCR结果显示IR组Ephrin-A3基因表达水平明显高于Sham组(P<0.01).Ephrin-A3蛋白主要表达在肾小管上皮细胞胞质中,Sham组Ephrin-A3蛋白表达水平较IR组明显升高(P<0.01).结论 肾缺血再灌注损伤明显影响miR-210及其靶基因Ephrin-A3的表达,miR-210表达的变化可能与肾缺血再灌注损伤的修复有关.     

硝苯地平对大鼠肾缺血再灌注损伤的影响

目的 探讨硝苯地平对大鼠肾缺血再灌注损伤的影响.方法 健康雄性SD大鼠42只,体重220～250 g,随机分为3组(n=14):假手术组(S组)、缺血再灌注组(IR组)和硝苯地平组(N组).IR组和N组采用夹闭双侧肾动、静脉45 min后恢复灌注的方法制备大鼠肾缺血再灌注模型,S组不夹闭双侧肾动、静脉.N组于夹闭前15 min和再灌注前15 min分别尾静脉注射硝苯地平0.1 mg/kg,IR组分别尾静脉注射等量溶剂.于再灌注6和24 h时留尿,测定尿N-乙酰-β-D-氨基葡萄糖苷酶(NAG)活性;抽取腹主动脉血,测定血清肌酐(Cr)、MDA和一氧化氮(NO)浓度,然后处死大鼠取肾,采用流式细胞仪检测肾皮质细胞凋亡情况、热休克蛋白70(HSP70)的表达,免疫组化法测定内皮素-1(ET-1)的表达.结果 与S组比较,IR组血清Cr和MDA浓度、尿NAG活性、HSP70和ET-1表达水平及肾皮质细胞凋亡率均升高(P＜0.05),血清NO浓度差异无统计学意义(P＞0.05);与IR组比较,N组血清Cr和MDA浓度、尿NAG活性、ET-1表达水平及肾皮质细胞凋亡率降低,血清NO浓度升高(P＜0.05),HSP70表达水平差异无统计学意义(P＞0.05).结论 硝苯地平可减轻大鼠肾缺血再灌注损伤,可能与其抑制ET-1表达有关.     

肝再生增强因子对缺血再灌注损伤肾脏局部炎性反应的影响

目的 探讨重组人肝再生增强因子( rhALR)对缺血再灌注(IR)肾损伤大鼠模型肾脏局部炎性细胞浸润及炎性因子表达的影响.方法 将SD大鼠按随机数字表法分成假手术组、IR组、rhALR低剂量(100 μg/kg)组及rhALR高剂量(200 μg/kg)组.采用双侧肾蒂夹闭60 min后再灌注建立IR肾损伤动物模型.常规生化法检测血肌酐、尿素氮的水平,HE染色观察肾脏组织学改变,比色法检测肾组织髓过氧化物酶( MPO)的活性,Western印迹法检测肾组织肿瘤坏死因子α(TNF-α)、细胞间黏附分子1(ICAM-1)、单核细胞趋化蛋白1(MCP-1)的蛋白表达.结果 rhALR组的血肌酐和尿素氮显著低于IR组(均P＜ 0.05),肾组织病理损害减轻,rhALR高剂量组较rhALR低剂量组肾功能及肾脏病理改善更明显.IR组大鼠肾组织的MPO活性、TNF-α、ICAM-1、MCP-1的蛋白表达在术后12 h较假手术组显著上升,术后24h有所下降,但仍维持在较高水平(均P＜0.05);rhALR组肾组织MPO活性、肾组织TNF-α、ICAM-1、MCP-1的蛋白表达较IR组显著下降(均P＜0.05),且rhALR高剂量组4者较rhALR低剂量组下降更显著(均P＜0.05).结论 rhALR对IR肾损伤具有保护作用,其作用机制可能与其减少肾脏局部的炎性细胞浸润、抑制炎性因子MCP-1、ICAM-1、TNF-α的表达有关.     

党参皂甙减轻大鼠移植肾缺血再灌注损伤中细胞凋亡的作用及其机制

目的 探讨党参提取物皂甙减轻移植肾缺血再灌注损伤中细胞凋亡的作用及其机制.方法 将雌、雄各半SD大鼠随机分成三组,每组20只,即假手术组、缺血再灌注组和皂甙干预组.假手术组不进行肾移植,仅切除右肾,游离左肾动静脉,暴露左肾1 h后关闭腹腔.缺血再灌注组和皂甙干预组建立大鼠移植肾缺血再灌注损伤模型.皂甙干预组分别于肾移植前48、24和0.5 h经腹腔注入皂甙溶液(每千克体重80 mg).移植肾再灌注后24 h,取大鼠外周血和移植肾组织待测.检测各组血尿素氮(BUN)和肌酐(Cr)水平;采用脱氧核糖核苷酸末端转移酶介导的缺口末端标记(TUNEL)法检测各组肾组织原位细胞凋亡指数(AI);采用逆转录聚合酶链反应(RT-PCR)检测与细胞凋亡有关的基因Bcl-2和Bax mRNA在各组肾组织中的相对表达量.结果 与假手术组相比,缺血再灌注组和皂甙干预组血BUN和Cr水平都显著升高(P＜0.05);移植肾细胞凋亡指数也显著增高(P＜0.05);移植肾组织中Bcl-2 mRNA表达显著降低,Bax mRNA表达显著增高(P＜0.05).与缺血再灌注组比较,皂甙干预组血BUN和Cr值明显下降(P＜0.05);移植肾细胞凋亡指数明显下降(P＜0.05);移植肾组织中Bcl-2 mRNA表达显著增加,Bax mRNA表达明显下降(P＜0.05).结论 党参皂甙在移植肾缺血再灌注损伤中能显著减轻细胞凋亡.其机制可能是通过对Bcl-2基因表达的上调和对Bax基因表达的下调,从而抑制细胞的凋亡.     

利多卡因预先给药对肾脏缺血再灌注损伤大鼠肾组织CD44和TNF-α表达的影响

目的 评价利多卡因预先给药对肾脏缺血再灌注损伤大鼠肾组织CD44和TNF-α表达的影响.方法 健康雄性Wistar大鼠36只,体重300～350 g,随机分为3组(n=12):假手术组(S组)、肾脏缺血再灌注组(IR组)和利多卡因预先给药组(L组).采用无创动脉夹夹闭双侧肾动脉60min、恢复灌注4 h,建立大鼠肾脏缺血再灌注模型.L组于夹闭双侧肾动脉前5min时尾静脉注射利多卡因5 mg/kg;IR组于夹闭双侧肾动脉前5 min时尾静脉注射等容量生理盐水;S组不夹闭双侧肾动脉,于分离肾动脉后尾静脉注射等容量生理盐水.再灌注4 h时处死大鼠,取肾组织,光镜下观察病理学结果;采用免疫组化法测定肾组织CD44和TNF-α的表达水平.结果 与S组比较,IR组肾组织CD44和TNF-α的表达上调(P＜0.05),L组肾组织CD44和TNF-α的表达差异无统计学意义(P＞0.05);与IR组比较,L组肾组织CD44和TNF-α的表达下调(P＜0.05),肾组织损伤减轻.结论 利多卡因预先给药减轻大鼠肾脏缺血再灌注损伤与其抑制肾组织CD44和TNF-α的表达有关.     

Reduction of renal ischemia reperfusion injury by hydrogen sulfide preconditioning through inhibiting oxidative stress

Objective To investigate the possible role of oxidative stress in the protection of hydrogen sulfide during renal ischemia reperfusion. Methods Male Wistar rats were randomly divided into 3 groups: sham operation (Sham) group, renal ischemia reperfusion (IR) group subject to occlusion of left renal pedicle for 45 min then reperfusion for 24 h, and sodium hydrosulfide (NaHS) preconditioning group with continuous infusion of NaHS (450 nmol/min) by left renal artery for 10 min before ischemia reperfusion. Renal injuries were evaluated by PAS staining. The protein levels of NADPH oxidase (NOX) 4, NOX2 were analyzed by Western blotting. The reactive oxygen species (ROS) level of renal tissue was determined by dihydroethidium (DHE) staining assay. Renal superoxide dismutase (SOD), malonic dialdehyde (MDA) and Scr, BUN were evaluated by chromatometry assay. Cell apoptosis were evaluated by TdT-mediated dUTP nick end labeling (TUNEL) staining. Results Compared with Sham group, in IR group the renal NOX4 and NOX2 protein expressions, the existence of acute tubular necrosis and ROS expression were up-regulated (all P＜0.01); MDA, Scr, and BUN were increased and SOD was decreased significantly in IR-treated kidney (all P＜0.01); Moreover, more apoptotic cells presented in the risk zone of IR-treated kindey (P＜0.01). The effects induced by IR were inhibited by NaHS. Compared to that in IR group, NaHS precondition reversed IR-induced damages of renal function and renal tissue, increased SOD activity and decreased MDA expression (all P＜0.05), as well as reduced the expression of NOX4, NOX2 and ROS (all P＜0.05). Moreover, NaHS precondition reduced apoptosis after IR (P＜0.05). Conclusions NaHS alleviates renal ischemia reperfusion injury through inhibiting oxidative stress. Hydrogen sulfide can decrease ROS by inhibiting the activation of NOX, further inhibit the activation of NOD-like receptor, and alleviate kidney damage.     

Impact of ischemic preconditioning on dynamics of homing of endothelial progenitor cells after renal ischemia reperfusion injury

Objectives To investigate the impact of ischemic preconditioning (IPC) on dynamics of homing of endothelial progenitor cells (EPCs) after renal ischemia reperfusion injury (IR). Methods Sixty male Sprague-Dawley rats were randomly divided into three groups after right-side kidney nephrectomy: for sham-operated rats, lumbotomy without vascular clamping was performed; IR rats were clamped renal blood vessels for 40 minutes while IPC rats were pre-treated with 15 min ischemia and 10 min reperfusion. At 3, 12, 24 h, and 3 days after reperfusion, the pool of circulating, kidneys, lungs and spleens were harvested. The extent of renal injury was assessed by biochemical and histological examination. The dynamics of homing of EPCs was observed by flow cytometry. Results The rats in IPC group exhibited significant improvements in renal function and morphology. Compared with IR group and sham group, the number of EPCs in blood was increased in the IPC group at 12 h and 24 h after reperfusion (P＜0.05). The number of EPCs in kidney was increased at all times point in the IPC group and IR group as compared to the sham group (P＜0.05. In addition, EPCs number was increased in IPC group compared with the IR group at 12 h and 24 h [(11.36±0.66)% vs (6.37±0.69)%, (6.31±0.70)% vs (4.40±0.60)%, all P＜0.05]. Compared with IR group and sham group, the number of EPCs in the lung was increased in the IPC groups at 12 h after reperfusion [(2.95±0.66)% vs (1.78±0.59)%, (1.66±0.61)%, all P＜0.05]. The number of EPCs in spleen was increased in the IPC group at 72 h as compared with the IR group and sham group [(0.55±0.06)% vs (0.34±0.07)%, (0.31±0.06)%, all P＜0.05]. Conclusions Endogenous EPCs may home to injured kidney after IPC. EPCs can also gather in the lungs and spleen.     

Effects of Transfusion of Stored Red Blood Cells on Renal Ischemia-Reperfusion–Induced Hepatic Injury in Rats

BackgroundRenal ischemia-reperfusion (IR) injures the liver as well as the kidneys. Transfusion of stored red blood cells (RBCs) triggers inflammatory responses, oxidative stress, and activation of innate immunity. In the present study, we investigated the effect of transfusion of stored RBCs on renal IR-induced hepatic injury.MethodsSprague–Dawley rats were randomly divided into 3 groups based on the following treatments: rats subjected to sham operation (sham group), rats subjected to the induction of renal IR only (RIR group), and rats transfused with stored RBCs 1 hour after the start of reperfusion (RIR-TF group). Renal ischemia was induced for 1 hour, and reperfusion was allowed for 24 hours. After reperfusion, blood and liver tissue samples were obtained.ResultsSerum levels of aspartate and alanine aminotransferase were increased in the RIR-TF group compared with those in the RIR and sham groups. The hepatic mRNA expression levels of heme oxygenase-1 and neutrophil gelatinase-associated lipocalin were increased in the RIR-TF group compared with those in the RIR and sham groups. The mRNA expression level of high mobility group box-1 was also increased in the RIR-TF group compared with that in the RIR group.ConclusionThe transfusion of stored RBCs exacerbates renal IR-induced liver damage. Oxidative stress may be responsible for hepatic injury.     

外源性硫化氢在大鼠肾脏缺血再灌注损伤中的保护作用

目的 观察不同剂量外源性硫化氢(H2S)供体硫氢化钠对大鼠肾脏缺血再灌注损伤( IRI)的保护作用.方法 健康雄性Wistar大鼠28只随机分为4组,即假手术组( Sham)、肾缺血再灌注(IR)组、硫氢化钠(NaHS)高剂量组、硫氢化钠低剂量组.大鼠右肾切除后,以NaHS作为硫化氢的供体,NaHS高、低剂量组分别经左肾动脉插管,按照1.5 μmol/min、300 nmol/min的剂量连续15 min给药,假手术组及IR组给予同体积生理盐水.停药5 min 后,NaHS组和IR组用无损伤微动脉夹夹闭左侧肾蒂45 min后解除阻断,建立大鼠急性IRI模型,假手术组不夹闭左肾动脉,其他操作同模型组.于肾脏恢复血流24h时留取血和肾组织标本,检测血清尿素氮(BUN)、血肌酐(Scr);半定量分析肾脏病理损伤;检测肾组织H2S生成率;采用实时定量PCR法检测胱硫醚-β-合成酶(CBS)、胱硫醚-γ-裂解酶(CSE )mRNA表达.结果 与假手术组相比,IR组H2S生成率显著降低(P＜0.01);CBS、CSE mRNA表达显著下降(P＜0.01 );Scr、BUN显著升高(P＜0.01);肾脏病理表现为急性肾小管坏死,且最严重.与IR组相比,NaHS预处理组H2S生成率升高(P＜0.05);CBS、CSE mRNA表达升高(P＜0.01 );Scr、BUN降低(P＜0.01);病理损伤明显减轻.NaHS两个剂量组之间差异无统计学意义.结论 外源性H2S对大鼠IRI具有保护作用.     

氯沙坦对大鼠肾脏缺血/再灌注损伤中STAT-1及ICAM-1蛋白表达的影响

目的：研究氯沙坦在肾缺血/再灌注损伤中对STAT-1和ICAM-1蛋白表达的影响及在损伤修复过程中的作用。方法：大鼠背部双侧切开找到肾蒂,行无创动脉夹夹闭造成急性肾缺血/再灌注损伤模型,以氯沙坦预处理灌胃,苦味酸法测血清肌酐,免疫组化测肾组织切片中的STAT-1蛋白和ICAM-1蛋白表达的水平。结果：假手术组在6h和24h肾组织的病理和血肌酐数值无明显变化;模型组在缺血再灌注6h和24h与假手术组对比血清肌酐数值明显升高,肾组织切片在6h时STAT-1和ICAM-1蛋白已有表达,24h时两指标表达均明显上调;氯沙坦预处理组在缺血再灌注损伤6h和24h时与模型组对比,血肌酐数值明显下降,同时肾组织中STAT-1和ICAM-1蛋白表达也明显下调。结论：氯沙坦在肾缺血再灌注损伤中起保护作用,机制可能通过下调STAT-1和ICAM-1蛋白表达有关。     

大鼠肝移植术后早期肝脏损害与Ref-1蛋白的表达

目的 观察大鼠肝移植术后早期肝组织内氧化还原因子1(redox factor-1,Ref-1)蛋白表达与肝脏损伤的关系.方法 将150只Wistar大鼠动物分为三个组,肝移植组、假手术组和空白对照组.分别于肝移植术后3、6、9、12、24 h取材,采用免疫组织化学方法检测移植后各时间肝组织Ref-1蛋白表达,同时通过血清生化指标、组织病理学分析研究Ref-1蛋白表达的意义.结果 血清学检查显示,肝移植术后3 h AST、ALT显著升高,术后6 h降低.病理学分析显示:术后24 h内,部分肝组织结构不清,肝细胞变性,肝窦扩张充血,炎细胞明显浸润.肝损伤较重.免疫组化检测显示,肝移植后早期肝实质细胞内Refl蛋白增高.9h达高峰,以后逐渐下降.结论 肝移植术后发生肝损伤以术后6 h为最重,之后损伤程度逐渐减轻,这是由于移植术后缺血再灌注损伤,激活Ref-1的表达明显增加,修复了由于缺血再灌注损伤导致的细胞凋亡.     

intermedin预处理对大鼠肾脏缺血再灌注损伤修复和再生过程的作用

目的 探讨intermedin （IMD）预处理对大鼠肾脏缺血再灌注（IR）损伤修复和再生过程的作用。 方法 将Wistar大鼠按随机数字表法分为4组：假手术组（sham）、IR组、转空质粒组和转IMD组。在切除右肾后,转IMD组用超声微泡造影剂介导的基因转染方法将IMD真核质粒转染到大鼠肾组织,用RT-PCR和Western印迹法检测转染效率。转染成功后,制作肾脏IR损伤模型,分别于再灌注后1 d、2 d、3 d、4 d、7 d和14 d 6个时间点各取6只大鼠,留取血清及肾组织标本,常规检测血清BUN和Scr;HE和PAS染色观察肾组织的病理变化;免疫组化法观察肾小管上皮细胞的增殖程度。 结果 （1）转IMD组比转空质粒组的IMD蛋白和mRNA表达均增多（均P < 0.05）,且转IMD组7 d时表达最多,与转IMD组4 d时差异无统计学意义;（2）与sham组相比,IR组1 d和2 d时Scr和BUN均显著增高（P < 0.05）;与IR组相比,转IMD组显著下降（P < 0.05）;转空质粒组与IR组相比差异无统计学意义（P > 0.05）。（3）IR组、转空质粒组和转IMD组大鼠的肾小管均受损,但转IMD组的损伤较轻,均以2 d时病理损伤最重。（4）sham组肾小管和肾小球内几乎没有增殖细胞核抗原（PCNA）阳性细胞的表达;IR组和转空质粒组的PCNA阳性数在IR损伤1 d时开始增加,7 d时最多;转IMD组的PCNA阳性细胞数在IR损伤1 d时开始增加,3 d时最多。与IR组1~4 d相比,转IMD组的PCNA阳性细胞数显著增加（P < 0.05）;与IR组7 d相比,转IMD组7 d的PCNA阳性细胞数显著减少（P < 0.05）。 结论 IMD预处理可以促进肾小管上皮细胞增殖,加速肾脏IR损伤修复和再生。     

Expression and function of Erbin protein in renal ischemia-reperfusion injury

Objective To investigate the expression of ErbB2 interacting protein (Erbin) in renal ischemia-reperfusion injury (IRI) in vivo and in vivo, and the effect of Erbin over-expression on IRI. Methods (1) In vivo, the model of renal IRI was constructed in mice, and set up sham group and reperfusion 3, 6, 12, 24 and 48 h IRI group. BUN and Scr were detected and PAS staining was used to observe the pathology change of renal tissues. Cell apoptosis was detected by TUNEL staining. Erbin and NF-κB expression in renal tissue was detected by Western blotting, and immunohistochemistry was used to detect the distribution of Erbin. (2) In vivo, IRI model in HK2 cells was constructed and cells were harvested after culturing in normal medium for 3, 6, 12 and 24 h. Erbin expression was detected by Western blotting. Flow cytometry and ELISA were used to evaluate the level of cell apoptosis and inflammatory cytokine secretion respectively. HK2 cells were transiently transfected with Prk5-myc-Erbin plasmid via lipofectamine 2000, and were divided into control group, IRI group, Erbin group and Erbin+IRI group. The protein expression of Erbin and NF-κB, cell apoptosis and inflammatory cytokine secretion was detected. Results (1) Compared with sham group, serum BUN and Scr were dramatically increased in IRI model, especially in 24 h after reperfusion (P＜0.05). Moreover, PAS staining showed that a lot of renal tubular epithelial cells were necrosis and fell off, and many protein cast were formed, renal injury score and apoptotic index were higher in 6 h, 12 h, 24 h, 48 h IRI model than those in sham group (all P＜0.05). The expression of Erbin, which was expressed in renal tubules, and nuclear NF-κB in 24 h IRI model were significantly increased, as compared with sham group (all P＜0.05). (2) Compared to those in control group, nuclear NF-κB expression, apoptosis and inflammatory cytokine secretion were significantly increased in IRI group. Meanwhile, Erbin expression was also induced and peaked at 24 h (P＜0.05). Compared to those in IRI group, cell apoptosis, the expression of nuclear NF-κB, inflammatory cytokine IL-6 and TNF-α were decreased in Erbin+IRI group (all P＜0.05). Conclusions Erbin expression is up-regulated in renal IRI, and over-expression of Erbin can partly inhibit NF-κB activation, cell apoptosis and inflammatory cytokine secretion in IRI group, which indicates Erbin may playing a protective role in renal IRI.