PI3K/AKT和MAPK/ERK1/2信号通路对胰腺癌PANC-1细胞VEGF表达的影响

目的:探讨PI3K/AKT和MAPK/ERK1/2信号通路对人胰腺癌PANC-1血管内皮生长因子(VEGF)表达的影响。方法:抑制剂LY294002和PD98095分别处理人胰腺癌PANC-1细胞,Western blotting检测细胞VEGF蛋白表达。结果:分析表明LY294002和PD98095处理后的PANC-1细胞的磷酸化AKT、磷酸化ERK1/2及VEGF蛋白表达水平均明显低于对照组VEGF(P<0.05)。结论:抑制PI3K/AKT和MAPK/ERK1/2细胞信号通路能够下调VEGF蛋白表达,进而抑制肿瘤新生血管的生成及浸润转移能力。

潞党参对光老化小鼠皮肤组织中ERK1/2、AKT表达的实验研究

目的研究潞党参对光老化小鼠皮肤组织中ERK1/2、AKT蛋白含量的影响。方法选择75只小鼠随机分为5组,分别为空白对照组、模型对照组、MAPK抑制剂组、PI3K抑制剂组、中药剂量组。空白对照组小鼠正常饲养,对模型对照组、MAPK抑制剂组、PI3K抑制剂组和中药剂量组小鼠进行皮肤光老化模型制备。在造模前30 min,给空白对照组和模型对照组小鼠灌胃生理盐水,MAPK抑制剂组灌胃MAPK抑制剂,PI3K抑制剂组灌胃PI3K抑制剂,中药剂量组小鼠灌胃相应剂量潞党参药液。造模完成后,采用Western-blot方法检查皮肤组织中ERK1/2、AKT蛋白含量的表达水平。结果与空白对照组比较,模型对照组小鼠皮肤组织中ERK1/2、AKT蛋白含量的表达水平显著升高,差异具有统计学意义(P<0.01),与模型对照组相比,中药剂量组小鼠皮肤组织中ERK1/2、AKT蛋白含量的表达水平均显著降低(P<0.01),分别与MAPK抑制剂组、PI3K抑制剂组比较,中药剂量组小鼠皮肤组织中ERK1/2、AKT蛋白含量的表达水平显著升高(P<0.01)。结论潞党参对皮肤光老化具有一定的保护作用。

老年大鼠阴茎海绵体中P-Erk1/2和P-Akt1激酶的表达

目的:一氧化氮(NO)是阴茎勃起的关键因子,其生成主要由一氧化氮合酶(NOS)调节,而磷酸化Erk1/2(P-Erk1/2)和磷酸化Akt1(P-Akt1)均能调节一氧化氮合酶(NOS)的表达及活性从而影响阴茎勃起。本实验研究P-Erk1/2和P-Akt1激酶在老年大鼠阴茎海绵体中的表达,探讨其在老年大鼠勃起功能障碍(ED)发生中的可能作用。方法:A组(2月龄)和B组(18月龄)雄性SD大鼠各10只,测其血清睾酮(T),免疫组化和RT-PCR方法检测大鼠阴茎海绵体中P-Erk1/2和P-Akt1的表达水平。结果:血清T值在B组[(4.73±0.94)nmol/L]较A组[(9.57±1.57)nmol/L]显著下降(P<0.05)。P-Erk1、P-Erk2的mRNA和P-Erk1/2蛋白的相对表达量(积分光密度值IA)在B组(0.95±0.06、0.92±0.05、32.09±8.45)较A组(0.47±0.09、0.61±0.11、7.50±1.81)显著升高(P<0.05);P-Akt1的mRNA和P-Akt1蛋白的相对表达量在B组(0.94±0.05、10.93±3.06)与A组(0.97±0.04、11.67±5.61)无显著差异(P>0.05)。结论:P-Erk1/2的过表达可能是老年性ED发生的机制之一。

SIRT1通过AKT通路和ERK1/2通路共同调节退变髓核细胞细胞外基质的合成

目的研究沉默信息调节因子2同源蛋白1(SIRT1/sirtuin 1)对已退变的人椎间盘髓核细胞(DNPCs)合成细胞外基质的影响。方法对人DNPCs进行分离、培养及其细胞鉴定,第一部分取P2代细胞用白藜芦醇(RES,SIRT1激动剂)、二甲双胍(MET,SIRT1激动剂)、尼克酰胺(NAM,SIRT1抑制剂)、SIRT1-siRNA进行相应处理,采用Western印迹检测Ⅱ型胶原(COLLA2α1)、聚蛋白多糖(Aggrecan)及其p-AKT、t-AKT、p-ERK1/2、t-EKR1/2。第二部分先RES与P2代细胞共培养后分别加入PI3K与ERK的特异性抑制剂LY294002、PD98059,观察COLLA2α1、Aggrecan的表达情况。结果用SIRT1激动剂刺激以后COLLA2α1、Aggrecan的表达显著提高,AKT及其ERK1/2的磷酸化水平也相应提高,用NAM及其SIRT1-siRNA处理后COLLA2α1、Aggrecan的表达显著降低,AKT及其ERK1/2的磷酸化水平也显著降低。用LY294002和PD98059分别处理后观察到COLLA2α1、Aggrecan的表达亦显著降低。结论 SIRT1可通过AKT及其ERK1/2两条通路上调人DNPCs细胞外基质的表达,抑制椎间盘的变性,为进一步研究椎间盘退变的机制、组织工程学、基因治疗等奠定了基础。

信号通路蛋白Akt1、ERK1/2与HIF-1α在肺癌组织中的表达及其临床意义

目的探讨信号通路蛋白Akt1、ERK1/2与HIF-1α在肺癌组织中的表达及其临床意义。方法采用免疫组化方法(Envision二步法),检测100例肺癌Akt1、ERK1/2和HIF-1α蛋白表达情况。结果 Akt1、ERK1/2及HIF-1α蛋白在肺癌组织中均呈不同程度表达,其阳性表达率分别为63.00%、68.00%和52.00%;Akt1与HIF-1α表达具有明显相关性(γ=0.673,P=0.000),ERK1/2与HIF-1α表达亦具有明显相关性(γ=0.568,P=0.000);Akt1、ERK1/2和HIF-1α表达均与肺癌分化程度、淋巴结转移及TNM分期有关(P<0.01)。结论 Akt1、ERK1/2和HIF-1α在肺癌中均呈高水平表达,Akt1、ERK1/2与HIF-1α表达具有明显相关性,三者均与肺癌分化程度、淋巴结转移及TNM分期有关,三者联合检测对肺癌诊断、治疗及预后具有重要意义。

Akt与ERK1/2在吡格列酮保护乳鼠心肌缺血再灌注损伤中的关系

目的：研究Akt与ERK1/2在吡格列酮保护乳鼠心肌缺血再灌注损伤作用中的关系.方法：体外培养1～3日龄的Wistar乳鼠心室肌细胞,通过缺氧3h,复氧3h,建立心肌细胞缺血再灌注损伤模型.实验分为空白对照组（C组）、缺血再灌注组（I/R组）、缺血再灌注＋吡格列酮组（I/R＋P组）、缺血再灌注＋吡格列酮＋Akt抑制剂mk2206组（I/R＋P＋MK组）、缺血再灌注＋吡格列酮＋ERK1/2抑制剂PD98059组（I/R＋P＋PD组）.应用免疫印迹和免疫荧光检测各组细胞p-Akt和p-ERK1/2的表达变化.结果：与I/R组比较,I/R＋P组p-Akt和p-ERK1/2均增加;I/R＋P＋MK组的p-Akt显著减少,而p-ERK1/2却明显增加;I/R＋P＋PD组的p-ERK1/2显著减少,而p-Akt却明显增加.各组间总Akt和ERK1/2的表达无明显变化.结论：吡格列酮可激活Akt和ERK1/2对缺血再灌注的心肌有保护作用,该过程中Akt和ERK1/2相互之间有影响.

缺血后处理对脑缺血再灌注损伤后ERK1/2和Akt磷酸化及神经细胞凋亡的影响

目的:观察缺血后处理对大鼠局灶性脑缺血再灌注损伤后ERK1/2和Akt及神经细胞凋亡的影响。方法:成年健康SD大鼠72只,随机分为假手术(sham)组、缺血再灌注(I/R)组、缺血后处理(Postcond)组各24只,应用线栓法建立大脑中动脉闭塞(MCAO)再灌注模型。分别于再灌注10min、30min、6h、24h后留取大脑皮质。Western blot检测再灌注10min、30min、6h后ERK1/2和Akt活性变化;原位末端标记(TUNEL)检测再灌注后24h神经细胞凋亡。结果:Postcond组再灌注10min、30min、6h后ERK1/2和Akt活性高于I/R组(P<0.05);脑缺血再灌注24h后,Postcond组与I/R组比较,TUNEL阳性细胞减少(P<0.05)。结论:缺血后处理可提高大鼠脑缺血再灌注后皮质内ERK1/2和Akt活性,减少神经细胞凋亡。

抗ErbB2嵌合抗体chA21对SKBR3细胞的增殖抑制以及对PI3K/Akt和Erk1/2信号转导途径的影响

目的检测抗ErbB2嵌合抗体chA21对高表达ErbB2乳腺癌细胞SKBR3的增殖抑制作用,并分析抗体对细胞膜上ErbB2分布以及对细胞PI3K/Akt和Erk1/2信号转导途径的影响,探讨chA21的抑癌机制。方法采用MTT检测chA21对SKBR3的增殖抑制作用,流式细胞术检测经chA21处理后细胞膜上ErbB2抗原的分布变化,Western blot检测抗体作用后对细胞PI3K/Akt和Erk1/2信号转导途径的影响。结果chA21可抑制SKBR3细胞的增殖,其作用呈剂量和时间依赖性。抗体作用后可下调细胞膜上ErbB2含量,并不同程度下调细胞的PI3K/Akt和Erk1/2的活化水平。结论chA21可抑制SKBR3细胞增殖,可能通过下调细胞膜上ErbB2分布而减少其介导的PI3K/Akt和Erk1/2信号转导途径的活化来实现的。

氯化两面针碱调节AKT/ERK1/2磷酸化影响肺癌细胞生长、运动、微管形成以及免疫应答

目的:研究氯化两面针碱(NC)对肺癌细胞生长、运动及炎症因子的影响,并阐明其可能机制。方法:以肺癌细胞系A549和NCI-H661为体外研究模型,CCK-8测定不同浓度NC对细胞活力的影响。选择0、3、6、12 nmol/L 4个浓度处理细胞,EdU染色测定细胞增殖,Transwell测定细胞侵袭,微管形成实验测定细胞微管形成能力,RT-PCR检测炎症因子iNOS、TNF-α、IL-4和IL-10 mRNA表达,ELISA检测iNOS、TNF-α、IL-4和IL-10含量,Western blot检测VEGF、N-cadherin和E-cadherin蛋白水平及AKT/ERK1/2通路磷酸化。加入AKT激活剂SC79(4μg/ml)进行验证实验。12周龄雄性BALB/c小鼠作为体外研究对象,检测NC对肿瘤的影响。结果:与对照组比较,当NC浓度>6 nmol/L时,可显著降低细胞活力,减少EdU阳性细胞数量、促进凋亡,抑制细胞侵袭,降低微管形成能力并提高细胞抗炎能力。与NC 0μg组相比,NC可抑制肿瘤生长。结论:NC可抑制肺癌细胞生长、运动,提高其抗炎能力,其机制可能与AKT/ERK1/2通路激活有关。

磷酸化STAT3和磷酸化Akt及磷酸化ERK1/2与鳞状细胞癌大小及转移的关系

目的:了解磷酸化细胞信号传导与转录活化因子3(p-STAT3)和磷酸化Akt(p-Akt)及磷酸化细胞外信号调节激酶(p-ERK1/2)在鳞状细胞癌(SCC)中的表达及与肿瘤大小及转移的关系。方法:将50例SCC按肿瘤大小及是否转移分组,采用免疫组化法检测其中p-STAT3,p-Akt及p-ERK1/2的表达,评估其与SCC大小及转移的关系。结果:p-STAT3、p-Akt及p-ERK1/2在SCC中均有较高的阳性表达率。p-STAT3和p-Akt的阳性表达在有转移的SCC中高于无转移的SCC(P<0.05),而与肿瘤的大小无关(P>0.05)。p-ERK1/2的阳性表达与SCC的转移无关(P>0.05),而与肿瘤的大小有密切关系(P<0.05)。结论:p-STAT3,p-AKt和p-ERK1/2在SCC的发病机制中起重要作用。p-STAT3和p-AKt在SCC的转移机制中起重要作用,而p-ERK1/2则在肿瘤生长中起重要作用。

虫草素通过ERK1/2、Ezrin和Akt信号通路抑制胆囊癌细胞SNU-308的增殖和迁移

目的:探讨虫草素对胆囊癌细胞SNU-308增殖和迁移的影响及其分子机制。方法:MTT法和平板集落形成实验检测不同浓度虫草素对胆囊癌SNU-308细胞活力和集落形成能力的影响;Annexin V/PI双染法检测细胞凋亡率;Western blot法检测细胞凋亡和自噬相关蛋白以及Akt、ERK1/2和Ezrin蛋白的磷酸化水平;免疫荧光染色法检测细胞内LC3的表达水平;划痕愈合实验和Transwell实验检测虫草素对胆囊癌细胞迁移能力的影响;划痕实验检测Akt抑制剂和ERK1/2抑制剂及Ezrin基因沉默对细胞迁移能力的影响。结果:虫草素可显著抑制胆囊癌细胞的活力和集落形成能力(P<0.05)。流式细胞术结果显示,虫草素可诱导胆囊癌细胞凋亡(P<0.05)。Western blot结果显示,虫草素处理后Bcl-2表达降低,Bax、细胞色素C(Cyto C)、Fas、Fas L和cleaved caspase-3蛋白水平升高,自噬标识蛋白LC3-II/I比例和beclin 1表达上调(P<0.05)。免疫荧光染色结果显示,虫草素处理后SNU-308细胞胞浆中LC3荧光颗粒的数量明显增多。划痕实验和Transwell实验结果显示虫草素可抑制细胞迁移(P<0.05)。虫草素明显抑制Akt、ERK1/2和Ezrin蛋白的磷酸化水平(P<0.05)。Ezrin基因沉默及Akti-1/2和GDC-0994均可抑制胆囊癌细胞的迁移作用(P<0.05)。结论:虫草素通过诱导凋亡和自噬抑制胆囊癌细胞的增殖和迁移,其机制可能与调控ERK1/2,Ezrin和Akt信号通路有关。

α_(2)-肾上腺素能受体激动剂对心肌炎大鼠ERK1/2和AKT信号通路的影响研究

目的研究α_(2)-肾上腺素能受体(α_(2)-AR)激动剂对心肌炎大鼠ERK1/2和PI3K/AKT信号通路的影响。方法采用完全弗氏佐剂及猪心肌肌球蛋白感染易致敏的Lewis大鼠,构建实验性自身免疫性心肌炎(EAM)大鼠模型,将大鼠随机分为对照组、EAM模型组(EAM组)、α_(2)-AR激动剂组(EAM+α_(2)-AR组)、PI3K/AKT信号通路抑制剂组(EAM+α_(2)-AR+EAM-LY组)和ERK1/2信号通路抑制剂组(EAM+α_(2)-AR+U0126组),每组6只。超声心动图检查心率、EF、FS、LVEDD和LVEDS,HE染色检测大鼠心肌组织病理学情况,蛋白质免疫印迹法检测p-AKT、p-ERK1/2、Caspase-3、PARP蛋白的相对表达量,TUNEL染色检测大鼠心肌细胞凋亡情况。结果与对照组比较,EAM组大鼠的心率、LVEDD和LVEDS升高,EF和FS降低(P<0.01)。与EAM组比较,EAM+α_(2)-AR组大鼠心肌组织病变程度减轻;EAM+α_(2)-AR组大鼠炎性评分降低(P<0.01)。与EAM组比较,EAM+α_(2)-AR组大鼠心肌组织中p-AKT蛋白的相对表达量上调,p-ERK1/2、Caspase-3和PARP蛋白的相对表达量下调,ROS水平下降(P<0.01)。与EAM+α_(2)-AR组比较,EAM+α_(2)-AR+EAM-LY组大鼠心肌组织中p-AKT蛋白的相对表达量下调,细胞凋亡率升高(P<0.01);EAM+α_(2)-AR+U0126组大鼠心肌组织中p-ERK1/2蛋白相对表达量下调,细胞凋亡率降低(P<0.01)。结论α_(2)-AR激动剂可能通过激活PI3K/AKT信号通路和抑制ERK1/2信号通路的方式,下调Caspase-3和PARP蛋白的相对表达水平,降低ROS水平,从而缓解心肌炎大鼠的炎症反应、抑制其细胞凋亡,起到保护心肌的作用。

C5a激活Akt1-ERK1/2通路促进NSCLC细胞的增殖和迁移

目的:探讨C5a对非小细胞肺癌(non-small cell lung cancer,NSCLC)细胞增殖和迁移的影响及其潜在的分子机制。方法:RT-PCR和Western blot检测人正常支气管上皮细胞系BEAS-2B和3种NSCLC细胞系(H1703、PC9、H1299)中C5a受体(C5aR)的表达;CCK-8和划痕实验检测C5a对PC9细胞增殖和迁移的影响;Western blot检查C5a刺激PC9细胞后蛋白激酶Akt1、细胞外信号调节激酶1/2(extracellular signal-regulated kinase,ERK1/2)和蛋白激酶C-α(protein kinase C-α,PKC-α)表达及磷酸化水平;用Akt1抑制剂Perifosine和ERK1/2抑制剂U0126分别处理PC9细胞后再给予C5a刺激,Western blot检测Akt1和ERK1/2的表达和磷酸化及其上下游调控关系,CCK-8和划痕实验检测Perifosine和U0126对细胞增殖和迁移的影响。结果:PC9细胞C5aR的表达水平显著高于其他细胞;C5a可明显促进PC9细胞的增殖和迁移能力;C5a刺激PC9细胞后,可显著增强Akt1和ERK1/2的磷酸化;Akt1和ERK1/2抑制剂均能明显降低C5a刺激PC9细胞后引起的细胞增殖和迁移,且Akt1抑制剂不仅能减弱Akt1的磷酸化,还能减弱ERK1/2的磷酸化,而ERK1/2抑制剂则仅能阻断其自身的磷酸化。结论:C5a刺激NSCLC细胞后可能通过激活Akt1-ERK1/2通路促进细胞的增殖和迁移。

亚甲蓝通过增强ERK1/2和AKT磷酸化降低IL⁃1β水平改善糖尿病大鼠视网膜病变

目的探究亚甲蓝对糖尿病大鼠视网膜病变的神经保护作用。方法将30只SD大鼠随机分为空白组、对照组和实验组。对照组和实验组采用链脲佐菌素(STZ)腹腔注射构建糖尿病大鼠模型。造模成功6周后,在实验组动物玻璃体内按照[0.2 mg/(kg·d)]剂量注射亚甲蓝,对照组玻璃体内注射等量二甲基亚砜(DMSO),均连续处理7 d。采用ELISA检测大鼠的视网膜超氧化物歧化酶(SOD),8⁃异前列腺素F2α(iPF2α)和白细胞介素1β(IL⁃1β)的水平,Western blot法检测视网膜磷酸化的细胞外信号调节激酶1/2(p⁃ERK1/2)和磷酸化的蛋白激酶B(p⁃AKT)表达,过碘酸希夫(PAS)染色检测视网膜形态变化。结果与空白组大鼠相比,对照组和实验组大鼠中的视网膜SOD活性明显降低,iPF2α和IL⁃1β水平增加,p⁃ERK1/2水平增加、p⁃AKT磷酸化水平降低;与对照组相比,实验组大鼠SOD活性增加,iPF2α和IL⁃1β水平降低,p⁃ERK1/2、p⁃AKT水平明显升高,视网膜层的整体厚度和视网膜神经节细胞的数量显著减少。结论亚甲蓝通过降低视网膜氧化应激和增强ERK1/2和AKT磷酸化改善糖尿病大鼠视网膜病变。

去整合素echistatin对糖尿病兔后发性白内障形成中信号通路PI3-K/Akt和ERK1/2的影响

目的观察去整合素echistatin对糖尿病兔后发性白内障形成中信号通路PI3-K/Akt和ERK1/2的影响,从分子水平上探讨echistatin的作用。方法建立糖尿病兔模型(n=24),随机分组并行透明晶状体囊外摘出术,术毕前房分别注入0.2 m L灭菌蒸馏水(对照组,n=12)或0.2 m L 10.0 mg·L^(-1)echistatin溶液(echistatin干预组,n=12)。术后10 d及6周(每个时间点6眼),裂隙灯显微镜观察两组术眼PCO分级情况,同时摘取术眼应用RT-PCR法检测后囊膜上信号因子Akt和ERK1/2 mRNA表达情况。结果术后10 d对照组和echistatin干预组PCO分级比较差异无统计学意义(P=0.093),但echistatin干预组PCO1级眼数少于对照组;术后6周echistatin干预组PCO级别明显低于对照组(P=0.006)。对照组和echistatin干预组Akt mRNA相对表达量术后10 d分别为0.981 7±0.380 4、0.481 7±0.166 5,术后6周分别为0.651 7±0.204 7、0.401 7±0.151 3,echistatin干预组均明显低于对照组(P=0.015,0.037)。对照组和echistatin干预组ERK1/2 mRNA相对表达量术后10 d分别为0.948 3±0.227 5、0.610 0±0.280 6,术后6周分别为0.921 7±0.299 4、0.465 0±0.180 0,echistatin干预组均明显低于对照组(P=0.045,0.009)。结论去整合素echistatin对糖尿病兔后发性白内障的发生和发展有一定的抑制作用,其发生的机制可能与抑制信号因子Akt和ERK1/2表达,进而阻断信号通路PI3-K/Akt和ERK1/2的转导有关。

Estrogen up-regulates MMP2/9 expression in endometrial epithelial cell via VEGF-ERK1/2 pathway

Objective:To study the effect of estrogen on anovulatory dysfunctional uterine bleeding(ADUB).Methods:Primary endometrial epithelial cells of Hainan Lizu female was cultured and hydrolylic activity of gelalinase was determined by gelatin zymography analysis.Cellular mRNA and protein synthesis was blocked respectively to determine whether the increased expression of MMP-2/9 was induced by estrogen.The expression of VEGF was blocked by siRNA.After treatment with various factors.MMP-9,VEGF,total Erk and phosphorylated Erk expression in primary uterine epithelial cells was detected by Western blotting analysis.Cell MMP-2/9mRNA levels was measured by real-time RT-PCR.Results:The activity and expression of MMP2/9 was inereased in the endometrium of patients with ADUB.Estrogen could up-regulate the expression of VEGF and activate Erk 1/2-Elk1 signal path.After interference by siRNA,ERK1/2 pathway was blocked in cells,and the expression of MMP-2/9 was down-regulated.ERK1/2 specific blocker U0126 blocked ERK phosphorylation,and it could down-regulate the expression of MMP-2/9.Conclusions:The results showed that the estrogen can increase the expression of VEGF,and thus activate ERK1/2 pathway to induce MMP-2/9 expression.

Endogenous hydrogen sulfide and ERK1/2-STAT3 signaling pathway may participate in the association between homocysteine and hypertension

Background Homocysteine(Hcy)is a risk factor for hypertension,although the mechanisms are poorly understood.Methods We first explored the relationship between Hcy levels and blood pressure(BP)by analyzing the clinical data of primary hypertensive patients admitted to our hospital.Secondly,we explored a rat model to study the effect of Hcy on blood pressure and the role of H2S.An hyperhomocysteinemia(HHcy)rat model was induced to explore the effect of Hcy on blood pressure and the possible mechanism.We carried out tissue histology,extraction and examination of RNA and protein.Finally,we conducted cell experiments to determine a likely mechanism through renin-angiotensin-aldosterone system(RAAS)and extracellular signal-regulated kinase 1/2(ERK1/2)signaling pathway.Results In primary hypertensive inpatients with HHcy,blood pressure was significantly higher as compared with inpatient counterparts lacking HHcy.In the rat model,blood pressure of the Wistar rats was significantly increased with increases in serum Hcy levels and decreased after folate treatment.Angiotensin converting enzyme 1(ACE1)expression in the Wistar Hcy group was enhanced comparing to controls,but was decreased in the Wistar folate group.Angiotensin II receptor type 1(AGTR1)levels in the kidney tissue increased in the Wistar folate group.Both serum H2S and kidney cystathionineγ-lyase decreased with elevated levels of serum Hcy.In vitro,increased concentrations and treatment times for Hcy were associated with increased expression of collagen type 1 and AGTR1.This dose and time dependent response was also observed for p-STAT3 and p-ERK1/2 expression.Conclusion Endogenous H2S might mediate the process of altered blood pressure in response to changes in serum Hcy levels,in a process that is partly dependent on activated RAAS and ERK1/2-STAT3 signaling pathway.

1,2,3,4,6-penta-O-galloyl-β-D-glucose Protects PC12 Cells from MPP^+-mediated Cell Death by Inducing Heme Oxygenase-1 in an ERK- and Akt-dependent Manner

This study examined the ability of 1,2,3,4,6-penta-O-galloyl-β-D-glucose (β-PGG) to induce the expression of heme oxygenase-1 (HO-1) in the PC12 cells and its regulation in the PC12 cells.One week before treatment with the drug,nerve growth factor (NGF) was added to the cultures at a final concentration of 50 ng/mL to induce neuronal differentiation.After drug treatment,HO-1 gene transcription was analyzed by reverse transcription polymerase chain reaction (RT-PCR).Expression of HO-1 and NF-E2-related factor2 (Nrf2) and activation of extracellular signal-regulated kinase (ERK) and Akt were detected by Western blotting.The viability of the PC12 cells treated with different medicines was examined by MTT assay.The oxidative stress in the PC12 cells was evaluated qualitatively and quantitatively by DCFH-DA.The results showed that β-PGG up-regulated HO-1 expression and this increased expression provided neuroprotection against MPP+-induced oxidative injury.Moreover,β-PGG induced Nrf2 nuclear translocation,which was found to be upstream of β-PGG-induced HO-1 expression,and the activation of ERK and Akt,a pathway that is involved in β-PGG-induced Nrf2 nuclear translocation,HO-1 expression and neuroprotection.In conclusion,β-PGG up-regulates HO-1 expression by stimulating Nrf2 nuclear translocation in an ERK-and Akt-dependent manner,and HO-1 expression by β-PGG may provide the PC12 cells with an acquired antioxidant defense capacity to survive the oxidative stress.

没食子酸甲酯抑制胶质瘤细胞中Akt和ERK1/2活性发挥抗肿瘤作用

目的探讨没食子酸甲酯(methyl gallate,MG)对大鼠胶质瘤细胞C6和人胶质瘤细胞U373增殖和迁移的影响以及抗肿瘤活性和调控机制。方法 MG从簇毛槭茎皮中分离提取,通过MTT法检测MG对胶质瘤细胞活性的影响,BrdU法检测胶质瘤细胞的增殖,应用划痕实验分析MG对胶质瘤细胞迁移的影响。Western blot检测MG对Akt和ERK1/2活性的影响。免疫荧光染色实验观察黏着斑的形成。结果细胞划痕试验显示,对照组划痕基本愈合,MG(5μg·mL-1)处理组划痕愈合被抑制(P<0.05);外源性Glu可增加细胞的迁移速度和距离,MG预处理抑制Glu诱导的细胞活性和迁移(P均<0.05)。Western blot结果显示,在向C6和U373细胞中加入Glu(终浓度150μM)后,Akt的磷酸化水平无变化(P>0.05),ERK1/2磷酸化水平升高(P<0.05)。免疫荧光染色结果显示,对照组和Glu处理组中,鬼笔环肽染色无变化,FA的数量和规模增加(P<0.05)。NBQX可抑制细胞的存活和迁移(P<0.05)。终浓度50μM的钙离子螯合剂BAPTA-AM预处理后,Akt磷酸化水平降低,细胞死亡增加(P<0.05)。用5μg·mL-1MG处理细胞,20 min后加入Glu刺激,Western blot结果表明,MG不仅抑制了Akt的磷酸化水平,还抑制了Glu诱导ERK1/2磷酸化;MG抑制Glu诱导的桩蛋白Ser83磷酸化(P<0.05)。结论 MG可抑制大鼠胶质瘤细胞C6和人胶质瘤细胞U373增殖和迁移,可能与抑制Akt和ERK1/2信号通路有关。

The role of ERK1/2 signaling pathway in coronary microembolization-induced rat myocardial inflammation and injury

Objectives In this work,we explore the effect of atorvastatin on myocardial apoptosis and caspase-8 acti- vation after coronary microembolization(CME) in rats. Methods Fifty rats were randomly divided into five groups; the coronary microembolization(CME) group,the sham-operated (sham) control group,the gastric lavage control group, the atorvastatin lavage group,and the caspasse-8 inhibitor (N-acetyl-Ile-Glu-Thr-Asp-CHO,abbreviated as CHO) group,with 10 rats for each group.A microembolization ball was injected through the left ventricle for constructing the CME model.Animals in the sham control group were given an injection of physiological saline instead of the microembolization ball.Seven days before the operation,the atorvastatin group underwent gastric lavage with 20 mg/kg of atorvastatin once a day.Gastric lavage control animals underwent gastric lavage with an equivalent dose of physiological saline instead of the atorvastatin.Animals in the CHO group were given an intraperitoneal injection of 10 mg/kg of CHO 30 min before the operation.Six hours after the operation,cardiac ultrasonic detection was conducted on each group to measure the cardiac function indexes.TUNEL(Terminal-deoxynucleoitidyl transferase mediated dUTP nick end labeling) assays were used to measure myocardial apoptosis,and western blots were used to quantify the expression levels of activated caspase-3 and -8.Results(1) The echocardiographic parameters showed that,compared to the sham control animals,the left ventricular ejection fraction(LVEF) of the CME group was significantly decreased(P【0.05).In addition, cardiac sonography revealed a decrease in the left ventricular shortening fraction(FS) and cardiac output(CO), but an increase in the left ventricular end-diastolic dimension (LVEDd).Compared to the CME group,the atorvastatin and CHO groups exhibited significantly improved cardiac function (P【0.05).(2) When compared with the sham control,the myocardical apoptotic rate of the CME group,as well as the levels of activated caspase-3 and-8,increased significantly (P【0.05).The myocardial apoptotic rate,as well as the levels of activated caspase-3 and caspase-8 in the atorvastatin and CHO groups,decreased significandy(P【0.05) in comparison to the CME group.Conclusions The atorvastatin pretreatment clearly suppressed post-CME myocardial apoptosis and improved cardiac function.The most likely mechanism for these effects is the blockade of the myocardial death receptor -mediated apoptosis pathway.