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1.
为研究心脏发育关键基因nkx2.5的功能及应用价值,构建Ad-Nkx2.5重组腺病毒,并检测nkx2.5过表达拮抗氧化应激损伤的效应及机制。采用AdEasy腺病毒表达系统构建Ad-Nkx2.5重组腺病毒,建立H2O2诱导H9c2心肌细胞凋亡模型,分别用Ad-Nkx2.5重组病毒或对照病毒感染细胞,采用Hoechst33342染色观察细胞形态变化、MTT法检测细胞存活率,免疫印迹检测caspase-3活化、细胞色素C的胞浆含量。并通过Real-timePCR检测凋亡相关基因bcl-2和bax表达。结果发现,nkx2.5过表达促进H9c2细胞存活,抑制H2O2诱导的caspase-3活化及线粒体细胞色素C的释放。Nkx2.5过表达上调bcl-2表达,显著下调H2O2诱导的bax表达。并发现H2O2对Nkx2.5核定位无明显影响。结果显示重组腺病毒介导的Nkx2.5过表达可通过调控凋亡相关基因表达,抑制线粒体凋亡途径,保护心肌细胞抗氧化损伤。 相似文献
2.
缺血再灌注产生的氧自由基会导致心肌细胞凋亡. 近年研究发现, α-硫辛酸(α-lipoic acid, LA)具有抗氧化作用, 但LA是否能够对抗心肌细胞凋亡, 保护心脏功能的作用尚未明确. 本研究利用H2O2诱导的心肌细胞H9c2氧化应激模型, 分别用CCK 8方法检测细胞存活率、Hoechst33342染色观察细胞核的形态变化、流式细胞术检测细胞凋亡率、real time PCR法检测Bcl 2/Bax基因表达变化, 评价LA是否具有对抗氧化损伤引起的心肌细胞凋亡能力. 结果显示, LA能提高H2O2损伤的H9c2细胞存活率, 降低心肌细胞凋亡, 而且LA通过上调Bcl 2的表达而发挥抑制细胞凋亡的作用. 研究结果证实, LA对氧化应激损伤的心肌细胞具有较好的保护作用. 该研究为LA在临床上用于治疗氧化应激引起的心肌细胞凋亡提供了实验依据. 相似文献
3.
目的:研究黄芪苷Ⅳ(AST)是否通过细胞外信号调节激酶1/2(ERK1/2)通路发挥对H2O2诱导的H9c2细胞氧化损伤的保护作用。方法:用200μmoL/L的H2O2处理细胞6h,采用MTT法检测细胞存活率,建立H2O2诱导的H9c2细胞氧化损伤模型;比色法测定细胞培养液中乳酸脱氢酶(LDH)活性、总超氧化物歧化酶(T—SOD)和锰超氧化物歧化酶(Mn—SOD)活力以及丙二醛(MDA)含量;Western blot检测H9c2细胞ERK1/2蛋白的磷酸化水平。结果:在H2O2浓度为200μmol/L作用6h条件下,细胞存活率降低程度适中,实验结果重复性好,确定后续实验采用200μmol/L H2O2作用6h建立模型。与H2O2组比较,10mg/L及20mg/L AST均显著提高细胞存活率(P〈0.01),使细胞培养液中LDH活性显著降低(P〈0.01),T—SOD及Mn—SOD活力显著提高(P〈0.01),MDA含量显著降低(P〈0.01)。10mg/L及20mg/L AST均显著增加H2O2损伤的H9c2细胞p—ERK1/2蛋白的表达(P〈0.01),当用PD98059(ERK1/2的抑制剂)预处理后,AST的作用则被取消。结论:黄芪苷Ⅳ可以通过ERK1/2通路发挥对H2O2诱导的H9c2细胞氧化损伤的保护作用。 相似文献
4.
目的:研究黄芪苷Ⅳ(AST)是否通过细胞外信号调节激酶1/2(ERK1/2)通路发挥对H2O2诱导的H9c2细胞氧化损伤的保护作用。方法:用200μmol/L的H2O2处理细胞6 h,采用MTT法检测细胞存活率,建立H2O2诱导的H9c2细胞氧化损伤模型;比色法测定细胞培养液中乳酸脱氢酶(LDH)活性、总超氧化物歧化酶(T-SOD)和锰超氧化物歧化酶(Mn-SOD)活力以及丙二醛(MDA)含量;Western blot检测H9c2细胞ERK1/2蛋白的磷酸化水平。结果:在H2O2浓度为200μmol/L作用6 h条件下,细胞存活率降低程度适中,实验结果重复性好,确定后续实验采用200μmol/L H2O2作用6 h建立模型。与H2O2组比较,10 mg/L及20 mg/L AST均显著提高细胞存活率(P<0.01),使细胞培养液中LDH活性显著降低(P<0.01),T-SOD及Mn-SOD活力显著提高(P<0.01),MDA含量显著降低(P<0.01)。10 mg/L及20 mg/L AST均显著增加H2O2损伤的H9c2细胞p-ERK1/2蛋白的表达(P<0.01),当用PD98059(ERK1/2的抑制剂... 相似文献
5.
目的探讨硫化氢(H2S)对阿霉素(DOX)诱导的H9c2细胞损伤的影响及其作用机制。
方法H2S对DOX心肌毒性保护作用的实验分组为:对照组(Control组),5?μmol/?L DOX处理组(A组),5?μmol/L DOX和400?μmol/L NaHS共同处理组(B组),400?μmol/L NaHS单独处理组(C组),5?μmol/L DOX、400?μmol/L NaHS和15?μmol/L Sirtinol共同处理组(D组),15?μmol/L Sirtinol单独处理组(E组)。SIRT1是否参与H2S抗DOX心肌毒性作用机制的实验分组为:对照组(Control组),5?μmol/L DOX处理组(F组),5?μmol/L DOX和400?μmol/L NaHS共同处理组(G组),5?μmol/L DOX、400?μmol/L NaHS和15?μmol/L Sirtinol共同处理组(H组),15?μmol/L Sirtinol单独处理组(I组)。使用MTT法检测细胞活力;Elisa法检测细胞MDA以及SOD水平;DCFH-?DA荧光探针法检测ROS水平;采用Western Blot法检测SIRT1蛋白表达。使用单因素方差分析法进行统计学分析。
结果NaHS预处理可抑制DOX导致的H9c2细胞活力下降:Control组,A组、B组、C组细胞活力分别为100﹪、(54.58±1.58)﹪、(85.05±4.31)﹪、(100.22±4.46)﹪ (F = 134.9,P < 0.001)。NaHS预处理可减弱DOX引起的H9c2细胞ROS、MDA水平的增加以及SOD水平的降低:Control组的ROS、MDA和SOD水平分别是100﹪、(34.18±1.56) μmol/g、(53.69±1.44) U/?mg;A组的ROS、MDA和SOD水平分别是(174.90±12.65)﹪、(72.65±2.66) μmol/g、(31.80±2.05) U/?mg;B组的ROS、MDA和SOD水平分别是(126.08±6.25)﹪、(44.59±1.92) μmol/g、(48.06±1.56) U/mg;C组的ROS、MDA和SOD水平分别是(91.86±1.66)﹪、(32.93±1.56)?μmol/?g、(55.93±1.58)?U/?mg (F?= 83.26,P < 0.001;F = 271.4,P < 0.001;F = 127.0,P < 0.001)。F组(6、12、24?h)H9c2细胞SIRT1蛋白表达水平分别是(0.45±0.03)、(0.27±0.02)、(0.25±0.03),较Control组(1.00±0.00)降低(F = 611.1,P < 0.001)。本研究还发现,NaHS预处理H9c2细胞能阻止DOX引起的SIRT1蛋白表达下调:Control组、F组、G组、H组的SIRT1蛋白表达水平分别是(1.00±0.00)、(0.31±0.03)、(0.60±0.04)、(1.09±0.09)(F = 123.4,P?2S对DOX诱导的H9c2细胞活力降低的抑制作用:Control组,F组、G组、H组、I组细胞活力分别为100﹪、(54.58±1.58)﹪、(85.37±3.62)﹪、(71.11±2.11)﹪、(97.53±1.45)﹪ (F = 238.2,P < 0.001)。Sirtinol预处理可明显逆转H2S对DOX导致的H9c2细胞ROS和MDA含量增加及SOD水平降低的抑制作用:Control组的ROS、MDA和SOD水平分别是100﹪、(35.84±2.22)μmol/?g、(53.03±3.16) U/mg;F组的ROS、MDA和SOD水平分别是(184.6±11.33)﹪、(74.78±5.30)μmol/g、(29.26±0.85)U/mg;G组的ROS、MDA和SOD水平分别是(126.5±7.57)﹪、(41.95±3.43)μmol/g、(52.61±2.26)U/mg;H组的ROS、MDA和SOD水平分别是(174.7±5.50)﹪、(67.69±1.52) μmol/g、(35.33±1.95) U/mg,I组的ROS、MDA和SOD水平分别是(98.03±2.86)﹪、(37.66±2.49)μmol/g、51.14 U/mg(F = 112.0,P < 0.001;F = 93.73,P < 0.001;F = 84.92,P < 0.001)。
结论H2S通过调控SIRT1抑制DOX诱导的H9c2细胞损伤。 相似文献
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7.
目的:研究氯化钴(CoCl2)对大鼠胚胎心脏来源的H9c2心肌细胞中新基因Mipu1表达的影响。方法:利用不同浓度的CoCl2(0、100、200、300、400、500μmol/L)处理H9c2细胞9h,及200μmol/L CoCl2处理H9c2细胞不同的时间(0、6、9、12、24h)后,用RT-PCR和Western Blot分别观察H9c2细胞Mipu1 mRNA和蛋白的表达情况。结果:CoCl2可以诱导H9c2细胞中Mipu1 mRNA和蛋白表达升高,200μM CoCl2处理组的Mipu1的表达水平高于100μM CoCl2处理组,但是更高浓度的CoCl2(>200μM)不能使Mipu1的表达进一步升高。随着CoCl2作用时间的延长,Mipu1的表达逐步升高,在12h达到高峰,但是在24h后下降。结论:CoCl2能够促进H9c2细胞新基因Mipu1的表达,并且具有一定的剂量和时间依赖性。 相似文献
8.
目的:研究氯化钴(CoCl2)对大鼠胚胎心脏来源的H9c2心肌细胞中新基因Mipu1表达的影响。方法:利用不同浓度的CoCl2(0、100、200、300、400、500μmol/L)处理H9c2细胞9h,及200μmol/L CoCl2处理H9c2细胞不同的时间(0、6、9、12、24h)后,用RT-PCR和Western Blot分别观察H9c2细胞Mipu1 mRNA和蛋白的表达情况。结果:CoCl2可以诱导H9c2细胞中Mipu1 mRNA和蛋白表达升高,200μM CoCl2处理组的Mipu1的表达水平高于100μM CoCl2处理组,但是更高浓度的CoCl2(〉200μM)不能使Mipu1的表达进一步升高。随着CoCl2作用时间的延长,Mipu1的表达逐步升高,在12h达到高峰,但是在24h后下降。结论:CoCl2能够促进H9c2细胞新基因Mipu1的表达,并且具有一定的剂量和时间依赖性。 相似文献
9.
为了探讨LncRNA RMST对过氧化氢(H2O2)诱导的心肌细胞损伤的影响及其可能的作用机制,该研究采用H2O2诱导大鼠心肌细胞H9C2建立细胞氧化损伤模型,随机分组:si-NC+200 μmol/L H2O2组(即培养基中加入200 μmol/L H2O2干预2 h)、si-LncRNA RMST+200 μmol... 相似文献
10.
目的:探讨外源性硫化氢(H2S)恢复缺氧后适应对衰老H9C2细胞的保护作用及相关机制。方法:H9C2细胞(心肌细胞系)用30 μmol/L过氧化氢(H2O2)处理2 h后再培养3 d,诱导生成衰老细胞。衰老H9C2细胞被随机分5组(n=8):正常组(Control)、缺氧/复氧组(H/R)、H/R+NaHS组、缺氧后适应(PC)组、PC+NaHS组。缺氧/复氧(H/R)模型:衰老H9C2细胞用缺氧液(无血清、无糖培养基,pH=6.8)培养3 h,然后正常培养6 h;缺氧后适应(PC)模型:方法同H/R模型,缺氧结束复氧前连续进行3次5 min间隔的复氧/再缺氧处理,随后复氧6 h。ELISA试剂盒分别检测大鼠晚期糖基化终末产物(AGEs)含量和caspase-3活性;CCK-8试剂盒检测细胞活力;DCFH-DA染色检测活性氧(ROS)水平;Hoechst 33342染色检测细胞凋亡率;Real-time PCR检测相关基因mRNA水平。结果:30 μmol/L H2O2可诱导H9C2细胞衰老但不会导致其凋亡;与Control组比较,H/R和PC均降低细胞活力,增加细胞凋亡率、ROS水平及caspase-3、caspase-9和Bcl-2 mRNA水平(P<0.01);且PC组与H/R组比较,上述指标变化无明显差异;在H/R和PC组加入NaHS,可显著提高细胞活力,降低细胞凋亡率和氧化应激;PC+NaHS对上述指标的作用明显强于H/R+NaHS。结论:外源性H2S能够恢复PC对衰老H9C2细胞的保护作用,其机制与抑制氧化应激和细胞凋亡有关。 相似文献
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目的:观察白藜芦醇(RSV)对过氧化氢(H2O2)所致的海马神经元HT22细胞损伤的保护作用,并探讨超氧化物歧化酶2(Mn-SOD)在其中的作用。方法:采用体外培养HT22小鼠海马神经元细胞系,H2O2作为损伤因素模拟氧化应激损伤。将细胞分为5组,分别为正常培养组(Control)、150μM H2O2损伤组(H2O2)、25μM白藜芦醇保护组(RSV+H2O2)、SOD2-si RNA干扰组(SOD2-si RNA+RSV+H2O2)和乱序RNA组(SC-si RNA+RSV+H2O2),药物暴露24 h后,应用MTT法检测HT22细胞活力、比色法检测乳酸脱氢酶(Lactate Dehydrogenase,LDH)释放量、相差显微镜观测细胞形态。结果:与对照组相比,H2O2组的活力显著下降(P0.05),LDH释放量明显增加(P0.05),细胞形态明显破坏;25μM的RSV显著恢复了HT22细胞的活力、减少了LDH释放、改善了细胞形态,而SOD2-si RNA显著逆转了RSV引起的上述保护作用,乱序RNA(SC-si RNA)未对上述保护作用产生明显影响。结论:白藜芦醇可能通过上调SOD2减轻H2O2对HT22细胞的氧化应激损伤。 相似文献
12.
Baohua Wang Jayant Shravah Honglin Luo David D.Y. Chen 《Biochemical and biophysical research communications》2009,389(1):105-448
Propofol is a widely used intravenous anesthetic agent with antioxidant properties secondary to its phenol based chemical structure. Treatment with propofol has been found to attenuate oxidative stress and prevent ischemia/reperfusion injury in rat heart. Here, we report that propofol protects cardiac H9c2 cells from hydrogen peroxide (H2O2)-induced injury by triggering the activation of Akt and a parallel up-regulation of Bcl-2. We show that pretreatment with propofol significantly protects against H2O2-induced injury. We further demonstrate that propofol activates the PI3K-Akt signaling pathway. The protective effect of propofol on H2O2-induced injury is reversed by PI3K inhibitor wortmannin, which effectively suppresses propofol-induced activation of Akt, up-regulation of Bcl-2, and protection from apoptosis. Collectively, our results reveal a new mechanism by which propofol inhibits H2O2-induced injury in cardiac H9c2 cells, supporting a potential application of propofol as a preemptive cardioprotectant in clinical settings such as coronary bypass surgery. 相似文献
13.
The aim of this study was to investigate the potential of quercetin and two of its "in vivo" metabolites, 3'-O-methyl quercetin and 4'-O-methyl quercetin, to protect H9c2 cardiomyoblasts against H(2)O(2)-induced oxidative stress. As limited data are available regarding the potential uptake and cellular effects of quercetin and its metabolites in cardiac cells, we have evaluated the cellular association/uptake of the three compounds and their involvement in the modulation of two pro-survival signalling pathways: ERK1/2 signalling cascade and PI3K/Akt pathway. The three flavonols associated with cells to differing extents. Quercetin and its two O-methylated metabolites were able to reduce intracellular ROS production but only quercetin was able to counteract H(2)O(2) cell damage, as measured by MTT reduction assay, caspase-3 activity and DNA fragmentation assays. Furthermore, only quercetin was observed to modulate pro-survival signalling through ERK1/2 and PI3K/Akt pathway. In conclusion we have demonstrated that quercetin, but not its O-methylated metabolites, exerts protective effects against H(2)O(2) cardiotoxicity and that the mechanism of its action involves the modulation of PI3K/Akt and ERK1/2 signalling pathways. 相似文献
14.
Wei-Cheng Chen Shih-Rong Hsieh Chun-Hwei Chiu Ban-Dar Hsu Ying-Ming Liou 《Journal of biomedical science》2014,21(1):56
Background
Epigallocatechin-3-gallate (EGCG) has been documented for its beneficial effects protecting oxidative stress to cardiac cells. Previously, we have shown the EGCG-mediated cardiac protection by attenuating reactive oxygen species and cytosolic Ca2+ in cardiac cells during oxidative stress and myocardial ischemia. Here, we aimed to seek a deeper elucidation of the molecular anti-oxidative capabilities of EGCG in an H2O2-induced oxidative stress model of myocardial ischemia injury using H9c2 rat cardiomyoblasts.Results
Proteomics analysis was used to determine the differential expression of proteins in H9c2 cells cultured in the conditions of control, 400 μM H2O2 exposure for 30 min with and/or without 10 to 20 μM EGCG pre-treatment. In this model, eight proteins associated with energy metabolism, mitochondrial electron transfer, redox regulation, signal transduction, and RNA binding were identified to take part in EGCG-ameliorating H2O2-induced injury in H9c2 cells. H2O2 exposure increased oxidative stress evidenced by increases in reactive oxygen species and cytosolic Ca2+ overload, increases in glycolytic protein, α-enolase, decreases in antioxidant protein, peroxiredoxin-4, as well as decreases in mitochondrial proteins, including aldehyde dehydrogenase-2, ornithine aminotransferase, and succinate dehydrogenase ubiquinone flavoprotein subunit. All of these effects were reversed by EGCG pre-treatment. In addition, EGCG attenuated the H2O2-induced increases of Type II inositol 3, 4-bisphosphate 4-phosphatase and relieved its subsequent inhibition of the downstream signalling for Akt and glycogen synthase kinase-3β (GSK-3β)/cyclin D1 in H9c2 cells. Pre-treatment with EGCG or GSK-3β inhibitor (SB 216763) significantly improved the H2O2-induced suppression on cell viability, phosphorylation of pAkt (S473) and pGSK-3β (S9), and level of cyclin D1 in cells.Conclusions
Collectively, these findings suggest that EGCG blunts the H2O2-induced oxidative effect on the Akt activity through the modulation of PIP3 synthesis leading to the subsequent inactivation of GSK-3β mediated cardiac cell injury. 相似文献15.
The aim of this study was to investigate the activation of JNK1/2 signalling pathway and the respective cellular phenotype
of H9c2 cardiac myoblasts during two distinct types of oxidative insult. We examined the dose- and time-dependent activation
of JNK1/2 pathway by exogenous H2O2, both under transient and sustained stimulation. At 2 h of either sustained or transient treatment, maximal phosphorylation
of c-Jun was observed, coincidently with the activation of nuclear JNK1/2; under sustained stress, these phosphorylation levels
remained elevated above basal for up to 6 h, whereas under transient stress they declined to basal ones within 4 h of withdrawal.
Furthermore, the JNK1/2 selective inhibitor SP600125 abolished the c-jun phosphorylation induced by oxidative stress. Our
results using cell viability assays and light microscopy revealed that sustained H2O2 stimulation significantly and time-dependently decreased H9c2 viability, in contrast to transient stimulation; SP600125 (10 μM)
abolished cell death induced by sustained as well as cell survival induced by transient oxidative stress. Hoechst staining
showed an increase in DNA condensation during sustained, but not during transient stimulation. Moreover, from the antioxidants
tested, catalase and superoxide dismutase prevented oxidative stress-induced cell death. Flow cytometry studies reconfirmed
that sustained oxidative stress induced apoptosis, whereas transient resulted in the recovery of cardiac myoblasts within
24 h. We conclude that in H9c2 myoblasts, sustained activation of JNK1/2 signalling pathway during oxidative stimulation is
followed by an apoptotic phenotype, while transient JNK1/2 activation correlates well with cell survival, suggesting a dual
role of this signalling pathway in cell fate determination. 相似文献
16.
目的:观察番茄红素(lycopene,LYC)对于血管内皮细胞功能的作用,探讨其作用机制。方法:人脐静脉内皮细胞(HUVECs)处理实验分组:对照组,H2O2组,H2O2+LYC组(1、2、4、8μmolL-1)。MTT法检测HUVECs存活率;免疫印迹法(Western blot)检测p38MAPK蛋白磷酸化水平、抗凋亡蛋白B淋巴细胞/白血病-2(bcl-2)及线粒体凋亡通路相关蛋白bax的表达;细胞黏附能力测定和伤口愈合实验检测HUVECs粘附率和迁移率;TUNEL法检测HUVECs凋亡率;ELASA法测定HUVECs内活性氧(ROS),超氧化物歧化酶(SOD),乳酸盐脱氢酶(LDH)释放量和caspase-3的活性。结果:H2O2损伤后HUVECs存活率显著降低(P0.01),凋亡率显著增加(P0.01),黏附和迁移能力显著降低(P0.01),bax和p-p38MAPK的表达上调,bcl-2的表达下调,并且ROS、LDH的释放和caspase-3的活性增加(P0.01),SOD的释放减少。而LYC的预处理可以明显逆转H2O2以上作用。结论:H2O2氧化应激损伤中,LYC保护内皮细胞可能与其抗过氧化损伤细胞凋亡,抑制异常的p38MAPK信号通路有关。 相似文献
17.
The purpose of our study was to investigate underlying basic mechanisms of hypothermia-induced cardioprotection during oxidative stress in a cardiomyocyte cell culture model. For hypothermic treatment we cooled H9c2 cardiomyocytes to 20 °C, maintained 20 min at 20 °C during which short-term oxidative damage was inflicted with 2 mM H2O2, followed by rewarming to 37 °C. Later on, we analyzed lactate dehydrogenase (LDH), caspase-3 cleavage, reactive oxygen species (ROS), mitochondrial activity, intracellular ATP production, cytoprotective signal molecules as well as DNA damage. Hypothermia decreased H2O2 damage in cardiomyocytes as demonstrated in a lower LDH release, less caspase-3 cleavage and less M30 CytoDeath staining. After rewarming H2O2 damaged cells demonstrated a significantly higher reduction rate of intracellular ROS compared to normothermic H2O2 damaged cardiomyocytes. This was in line with a significantly greater mitochondrial dehydrogenase activity and higher intracellular ATP content in cooled and rewarmed cells. Moreover, hypothermia preserved cell viability by up-regulation of the anti-apoptotic protein Bcl-2 and a reduction of p53 phosphorylation. DNA damage, proven by PARP-1 cleavage and H2AX phosphorylation, was significantly reduced by hypothermia. In conclusion, we could demonstrate that hypothermia protects cardiomyocytes during oxidative stress by preventing apoptosis via inhibiting mitochondrial dysfunction and DNA damage. 相似文献
18.
Xuehua Zhang Yanyan Zhao Dong Bai Xiutai Yuan Shan Cong 《Journal of biochemical and molecular toxicology》2019,33(5)
Schizandrin is a major bioactive constituent of Schisandra chinensis (Turcz.) Baill with antioxidant and anti‐inflammatory properties. The objective of this study was to explore the potential effects of schizandrin on a cell model of myocarditis. The H9c2 cells were treated with schizandrin alone or in combination with lipopolysaccharide (LPS), after which, cell survival, migration, and the release of inflammatory cytokines were assessed. Moreover, downstream effectors and signaling pathways were studied to reveal the possible underlying mechanism. As a result, LPS stimulation induced significant cell damage as cell viability was repressed and the apoptosis was induced. In the meantime, LPS promoted the release of proinflammatory cytokines including interleukin 1β (IL‐1β), IL‐8, IL‐6, and tumor necrosis factor (TNF‐α) while repressing the release of the anti‐inflammatory cytokine IL‐10. Schizandrin could promote H9c2 cell migration and long‐term treatment (7 days) enhanced cell viability. More interestingly, pretreatment with schizandrin attenuated LPS‐induced cell loss and inflammatory response. Besides this, Smad3 was a downstream effector of schizandrin. The beneficial effects of schizandrin on the H9c2 cells were attenuated when Smad3 was overexpressed. Moreover, the silencing of Smad3 deactivated c‐Jun N‐terminal kinase (JNK) and nuclear factor κB (NF‐κB) pathways. This study preliminarily demonstrated that schizandrin prevented LPS‐induced injury in the H9c2 cells and promoted the recovery of myocardial tissues by enhancing cell viability and migration. Schizandrin conferred its beneficial effects possibly by downregulating Smad3 and inhibiting the activation of JNK and NF‐κB pathways. 相似文献