丹参单体IH764-3对H2O2刺激肝星状细胞增殖和胶原合成的影响及其机制

目的：IH764－3对H2O2刺激的大鼠肝星状细胞（HSCs)增殖及胶原合成的抑制作用以及对粘着斑激酶（FAK）的影响,旨在为临床防治肝纤维化提供理论依据。方法：以不同剂量IH764－3干预H2O2刺激的HSCs,通过^3H-胸腺嘧啶（^3H-TdR)、^3H－脯氨酸（^3H-pro)掺入法测定HSCs增殖及胶原合成能力,应用逆转录聚合酶链反应（RT－PCR）方法检测FAK mRNA。结果：不同剂量IH764－3（10μg/ml,20μg/ml,30μg/ml,40μg/ml）作用于HSCs 48h及30μg/ml IH764－3作用于HSCs不同时间（12h,24h,48h),与单纯H2O2组相比,HSCs增殖明显被抑制（P＜0．05）;胶原合成能力降低（P＜0．05）;同时FAK mRNA表达下降。结论：丹参单体IH764－3能够抑制H2O2刺激的HSCs增殖及胶原合成,下调FAK是IH764－3抑制HSCs增殖及胶原合成的分子机制之一。     

丹参单体IH764-3通过下调H2O2刺激的肝星状细胞FAK水平影响MMP-13和TIMP-1的表达

目的：研究丹参单体IH764—3对H2O2刺激的肝星状细胞（HSC）基质金属蛋白酶-13（MMP-13）、基质金属蛋白酶组织抑制因子-1（TIMP-1）表达的影响以及此过程中粘着斑激酶（FAK）的变化。方法：应用RT-PCR方法检测MMP-13及FAKmRNA表达,原位杂交方法检测TIMP-1mRNA水平,Western blotting技术检测FAK及TIMP-1蛋白表达。结果：IH764—3干预组的MMP-13mRNA在2h的表达强度明显上调,而TIMP-1mRNA表达明显受抑,FAKmRNA表达强度明显下调;IH764—3干预24h组FAK及TIMP-1蛋白表达受抑制。结论：丹参单体IH764—3可以诱导MMP-13表达,抑制TIMP-1表达,下调FAK表达是其中的机制之一。     

丹参联合β-榄香烯对肝星形细胞LX-2增殖和凋亡的影响

目的：探讨丹参联合B-榄香烯对肝星形细胞LX-2增殖和凋亡的影响。方法：体外培养肝星形细胞LX-2,分别将丹参（浓度为1、2、4、6、8mg／ml）,β-榄香烯（浓度为25、50、100、150、200μg／ml）,单独作用于LX-2细胞后24h、48h用CCK-8（CellCountKit-8）法检测细胞的增殖情况,并选取合适的药物浓度（丹参3．6mg／ml,β-榄香烯125μg／ml）,然后进行联合用药,加药24h、48h后用CCK-8（Cell CountKit-8）法检测细胞的增殖情况,用流式细胞术检测细胞的凋亡率。结果：OCCK-8法显示丹参（浓度为1、2、4、6、8mg／ml）,8-榄香烯（浓度为25、50、100、150、200μg／ml）作用LX-2细胞24h、48h后,其增殖抑制率均明显高于正常对照组（P〈0．05）,并且呈浓度和时间依赖性。②联合用药（丹参3．6mg／ml,β-榄香烯125μg／ml）时,LX-2细胞的增殖抑制率和凋亡率均显著高于单独用药（P〈0．01）。结论：丹参、β-榄香烯单独或二者联合作用均能抑制LX-2细胞的增殖,且联合应用的作用显著高于单独用药,可协同促进LX-2细胞的凋亡。     

Cameleon测钙系统在H202诱导的A549细胞凋亡过程中的应用

观察Cameleon测钙系统在H202诱导的A549细胞凋亡过程中的应用,实时测定胞浆Ca2＋浓度（[Ca2＋]i）,并探讨[Ca2＋]I－与细胞凋亡和Pyk2磷酸化的关系。采用ca2＋指示器CameleonYC3．6转染A549细胞,24h后用50mmol／LH202刺激细胞。激光扫描共聚集显微镜实时测定选取细胞的[ca2＋]i变化。采用Westernblot检测H202刺激的细胞中Pyk2－tyr402磷酸化水平。采用DAPI染色试剂盒观察H2O2刺激后细胞凋亡情况。结果发现,在H2O2作用下,A549细胞胞浆内游离[Ca2＋]迅速升高,同时Pyk2－tyr402磷酸化水平显著升高俨〈O．05）,凋亡细胞百分比显著增加（Ｐ〈0．01）。因此,H202促进A549细胞内Ca02＋释放,可能通过活化Pvk2诱导细胞凋亡。     

剪切应力环境下的内皮祖细胞对肝星状细胞增殖和生物功能的影响

目的：研究流体剪切应力条件下的内皮祖细胞（EPCs）对肝星状细胞（HSCs）增殖、粘附、迁移、凋亡等生物学功能以及成纤维化因子α-平滑肌肌动蛋白（α-SMA）、胶原I （Col-I）、胶原III （Col-III）表达的影响。方法：将HSCs与EPCs分别接种于共培养小室的上层和下层,共培养24 h后,给EPCs细胞施加12 dyne/cm²剪切应力,持续24 h。消化细胞,采用CCK-8法检测HSCs的增殖;流式细胞术检测HSCs的凋亡率;细胞贴壁法检测HSCs的粘附功能;Boyden小室检测HSCs的迁移;荧光定量PCR法及Western blot分别检测HSCs的α-SMA、Col-I、Col-III mRNA和蛋白质的表达情况。结果：在剪切应力条件下,EPCs生态小境能明显抑制HSCs的增殖、粘附和迁移能力,促进HSCs凋亡,下调HSCs中Col-I、Col-III mRNA和蛋白质的表达。结论：在剪切应力条件下,EPCs生态小境对HSCs纤维化的发展具有一定抑制作用。     

血管紧张素—（1—7）对大鼠血管平滑肌细胞PKC和ERK1／2的抑制作用

采用Western blot,氘－胸腺嘧啶（3H－TdR)和氘－亮氨酸（3H－Leu)掺入等技术和方法,用血管紧张素Ⅱ（AngⅡ)和血管紧张素－（1－7）[Ang-(1-7)]刺激大鼠血管平滑肌细胞（VSMCs),观察和分析Ang-(1-7)对VSMCs增殖及蛋白激酶C（PKC）和胞外调节蛋白激酶（ERK）表达的影响,Ang-(1-7)能明显抑制基础和AngⅡ刺激下的VSMCs PKC-Ⅱ和ERK1／2蛋白表达（P＜0．01或P＜0．05）,减少3H－TdR和3H－Leu掺入量（P＜0．01或P＜0．05）,结果提示,Ang-(1-7)对VSMCs增殖有抑制作用,这可能与影响PKC－ζ和ERK1／2蛋白表达有关。     

应用SYBR荧光实时定量RT-PCR法检测BMSCs诱导大鼠肝星状细胞中DR5mRNA表达

目的应用SYBR荧光实时定量RT-PCR法检测骨髓间充质干细胞（BMSCs）对大鼠肝星状细胞（HSCs）的死亡受体5（DR5）mRNA表达的影响,探讨BMSCs诱导HSCs凋亡及其机制。方法采用贴壁筛选法培养、纯化SD大鼠BMSCs,传至第4代使用;大鼠原代HSCs细胞及肝纤维原细胞系冻融后传代使用。应用6孔塑料培养板,建立上下双层细胞共培养体系,常规培养。实验分为3组：（1）实验组：BMSCs与HSCs共培养;（2）空白对照组：HSCs单独培养;（3）阴性对照组：大鼠肝纤维原细胞与HSCs共培养。以上培养体系动态观察24、48、72h,应用流式细胞仪检测HSCs细胞凋亡率,采用SYBRGreenI荧光实时定量RT-PCR法检测,以β-actin基因作为内参,计算各组DR5mRNA的相对表达量。结果在共培养组中,BMSCs促进了HSCs凋亡,与其他两组比较差异有显著统计学意义（P〈O．01）,空白对照组与阴性对照组比较无统计学意义（P〉0．05）。实验组BMSCs能明显上调HSCs中DR5mRNA的表达,与空白对照组和阴性对照组比较差异有显著统计学意义（P〈O．01）;空白对照组与阴性对照组DR5mRNA的表达比较无统计学意义（P〉O．05）。结论利用SYBR荧光实时定量RT-PCR法检测BMSCs诱导大鼠肝星状细胞中DR5mRNA表达,为进一步研究BMSCs通过死亡受体途径调控HSCs凋亡以及为BMSCs用于治疗肝纤维化的机制研究提供了理论基础。     

白藜芦醇对人子宫内膜癌细胞系AN3CA增殖和凋亡效应及其机制探讨

目的：探讨白藜芦醇（resveratrol,Res）对人子宫内膜癌细胞AN3CA的增殖抑制和凋亡诱导效应及可能存在的机制。方法：应用噻唑蓝（MTT）法检测Res对AN3CA的增殖影响;流式细胞术检测Res对细胞周期分布和凋亡影响：荧光实时定量PCR检测Res对细胞Bcl-2、Bax和MMP-9mRNA表达水平的影响;WesternBlot方法检测Res对PCNA、Bcl-2、Bax及ERK1／2、P—ERK1／2蛋白表达水平的影响。结果：Res对子宫内膜癌细胞AN3CA具有显著的生长抑制作用（P〈0．01）,呈时间-剂量依赖性;不同浓度Res处理细胞G0／G1期比例显著增加伴随S期细胞数的减少;细胞凋亡率明显增高,200Dmol／lRes处理48h凋亡率可达30．96％±2．041％（P〈0．01）。与对照组相比,Res能抑制PCNA的蛋白表达量,增加Bax和降低Bcl-2转录和蛋白水平的表达量。Res在短时间内（0．5—1h）激活ERK1／2的磷酸化表达但随着作用时间延长（4—48h）其表现为抑制效应。结论：Res具有抑制AN3CA细胞增殖,诱导细胞G0／G1期阻滞和凋亡的效应。Res诱导凋亡可能是通过上调Bax,下调Bcl-2发挥作用,其抗癌作用机制可能与ERK1／2通路失调相关。     

TNF—α对哮喘模型大鼠气道平滑肌细胞增殖及ERK1／2活性的影响

目的探讨TNF—α对哮喘大鼠气道平滑肌细胞（ASMCs）增殖及对ASMCs上ERK1／2mRNA、p-ERK1／2表达水平的影响。方法通过对哮喘模型大鼠ASMCs培养,分别以0．2μg／L、1．0μg/L、20μg/L TNF-α干预ASMCs生长。采用流式细胞仪、MTT法检测ASMCs增殖情况,观察不同浓度TNF—α对ASMCs增殖的影响。RT-PCR检测ASMCs上ERK1／2mRNA表达,免疫细胞化学染色法检测磷酸化ERK1／2蛋白的表达及定位。结果哮喘组ASMCsS期比例、A值、ERK1／2mRNA、p-ERK1／2蛋白的表达量分别为（34．45±2．08）％、（0．550±0．010）、（0．995±0．118）、（130．77±4．16）,与对照组（11．17±0．96）％、（0．292±0．008）、（0．576±0．098）、（163．82±1．38）比较均显著增高（均P〈0．01）。各TNF—α干预组ASMCs的S期比例、A值、ERK1／2mRNA和p-ERK1／2蛋白表达量与哮喘组比较均显著降低（均P〈0．01）,0．2μg/L和1．0μg／LTN-α组p-ERK1／2蛋白表达量高于对照组（P〈0．01）,20μg／L TNF-α组p-ERK1／2蛋白表达量与对照组比较无差异（P〉0．05）。结论与正常鼠相比,慢性哮喘大鼠气道平滑肌细胞增殖明显,处于S期的细胞比例明显增高。经TNF—α干预后,慢性哮喘大鼠气道平滑肌细胞处于S期的细胞比例减少,增殖减弱,TNF-α可能抑制慢性哮喘大鼠气道平滑肌细胞增殖。TNF—α可下调慢性哮喘大鼠气道平滑肌细胞上ERK1／2mRNA及p-ERK1／2表达,TNF-α可能通过抑制ERK信号转导通道的活性对气道平滑肌细胞的增殖进行调控。     

羊栖菜多糖诱导lovo细胞凋亡及其机理探讨

本课题研究羊栖菜多糖（Sargassum Fusforme Polysaccharides．SFPS）诱导人大肠癌lovo细胞凋亡及凋亡过程中Caspase-3的变化及其意义。MTT法检测SFPS对大肠癌细胞增殖的抑制率：通过电镜、琼脂糖凝胶电泳、流式细胞术鉴定细胞凋亡：应用Westernblot法测定Caspase-3酶原的变化：RT—PCR检测Caspase-3mRNA表达。结果显示：SFPS作用lovo细胞24,36,48和72h的IC50分别为375,355,178和60mg／L,表明对lovo细胞具有显著生长抑制作用。在电镜下,可见明显的细胞凋亡特征：细胞膜表面微绒毛减少、染色质固缩、边集,凋亡小体形成。在琼脂糖凝胶电泳中,药物浓度为5—300mg／L作用24h后,显示有凋亡细胞特有的DNA梯状条带：而500mg／L处理后梯状条带模糊,开始出现“涂片状”,表明在高药物浓度的作用下,细胞有坏死。流式细胞仪测得细胞凋亡率有剂量的依赖性;DNA直方图出现亚G1峰,但细胞周期时相的分布无明显改变。SFPS处理lovo细胞后,发现Caspase-3酶原蛋白表达降低,Caspase-3的mRNA高表达,并具有剂量和时间的依赖性。实验结果提示,SFPS在体外能够诱导lovo细胞凋亡,这可能是SFPS抑制肿瘤增殖的机制之一．而Caspase-3的活化参与了SFPS诱导lovo细胞凋亡的调控。     

Haemin attenuates intermittent hypoxia‐induced cardiac injury via inhibiting mitochondrial fission

Obstructive sleep apnoea (OSA) characterized by intermittent hypoxia (IH) is closely associated with cardiovascular diseases. IH confers cardiac injury via accelerating cardiomyocyte apoptosis, whereas the underlying mechanism has remained largely enigmatic. This study aimed to explore the potential mechanisms involved in the IH‐induced cardiac damage performed with the IH‐exposed cell and animal models and to investigate the protective effects of haemin, a potent haeme oxygenase‐1 (HO‐1) activator, on the cardiac injury induced by IH. Neonatal rat cardiomyocyte (NRC) was treated with or without haemin before IH exposure. Eighteen male Sprague‐Dawley (SD) rats were randomized into three groups: control group, IH group (PBS, ip) and IH + haemin group (haemin, 4 mg/kg, ip). The cardiac function was determined by echocardiography. Mitochondrial fission was evaluated by Mitotracker staining. The mitochondrial dynamics‐related proteins (mitochondrial fusion protein, Mfn2; mitochondrial fission protein, Drp1) were determined by Western blot. The apoptosis of cardiomyocytes and heart sections was examined by TUNEL. IH regulated mitochondrial dynamics‐related proteins (decreased Mfn2 and increased Drp1 expressions, respectively), thereby leading to mitochondrial fragmentation and cell apoptosis in cardiomyocytes in vitro and in vivo, while haemin‐induced HO‐1 up‐regulation attenuated IH‐induced mitochondrial fragmentation and cell apoptosis. Moreover, IH resulted in left ventricular hypertrophy and impaired contractile function in vivo, while haemin ameliorated IH‐induced cardiac dysfunction. This study demonstrates that pharmacological activation of HO‐1 pathway protects against IH‐induced cardiac dysfunction and myocardial fibrosis through the inhibition of mitochondrial fission and cell apoptosis.     

丹参活性成分的现代中药药理研究进展

对传统中药丹参中丹参酮、丹酚酸、丹参单体IH764-3三种主要活性成分及其近年来的中药药理学研究进展进行综述,为进一步开发利用这一传统中药提供理论依据。     

Locking Intracellular Helices 2 and 3 Together Inactivates Human P-glycoprotein

The P-glycoprotein (P-gp) drug pump (ABCB1) has two transmembrane domains and two nucleotide-binding domains (NBDs). Coupling of the drug-binding sites in the transmembrane domains to the NBDs occurs through interaction of the intracellular helices (IHs) with residues in the NBDs (IH1/IH4/NBD1 and IH2/IH3/NBD2). We showed previously that cross-linking of cysteines in IH3 and IH1 with a short cross-linker mimicked drug binding as it activated P-gp ATPase activity. Here we show that residue A259C(IH2) could be directly cross-linked to W803C(IH3). Cross-linking was inhibited by the presence of ATP and adenosine 5′-(β,γ-imino)triphosphate but not by ADP. Cross-linking of mutant A259C/W803C inhibited its verapamil-stimulated ATPase activity mutant, but activity was restored after addition of dithiothreitol. Because these residues are close to the ball-and-socket joint A266C(IH2)/Phe¹⁰⁸⁶(NBD2), we mutated the adjacent Tyr¹⁰⁸⁷(NBD2) close to IH3. Mutants Y1087A and Y1087L, but not Y1087F, were misprocessed, and all inhibited ATPase activity. Mutation of hydrophobic residues (F793A, L797A, L814A, and L818A) flanking IH3 also inhibited maturation. The results suggest that these residues, together with Trp⁸⁰³ and Phe⁸⁰⁴, form a large hydrophobic pocket. The results show that there is an important hydrophobic network at the IH2/IH3/NBD2 transmission interface that is critical for folding and activity of P-gp.     

The direct profibrotic and indirect immune antifibrotic balance of blocking the cannabinoid 2 receptor

Cannabinoid 2 (CB2) receptors expressed on immune cells are considered to be antifibrogenic. Hepatic stellate cells (HSCs) directly interact with phagocytosis lymphocytes, but the nature of this interaction is obscure. We aimed to study the effects of CB2 receptors on hepatic fibrosis via their role in mediating immunity. Hepatic fibrosis was induced by carbon-tetrachloride (CCl(4)) administration in C57BL/6 wild-type (WT) and CB2 knockout (CB2(-/-)) mice. Irradiated animals were reconstituted with WT or CB2(-/-) lymphocytes. Lymphocytes from na?ve/fibrotic WT animals and healthy/cirrhotic hepatitis C virus were preincubated in vitro with or without CB2 antagonist, evaluated for proliferation and apoptosis, and then cocultured with primary mouse HSCs or a human HSC line (LX2), respectively. Lymphocyte phagocytosis was then evaluated. Following CCl(4)-administration, CB2(-/-) mice developed significant hepatic fibrosis but less necroinflammation. WT mice harbored decreased liver CD4(+) and NK(+) cells but increased CD8(+) subsets. Na?ve CB2(-/-) mice had significantly decreased T cell subsets. Adoptive transfer of CB2(-/-) lymphocytes led to decreased fibrosis in the irradiated WT recipient compared with animals receiving WT lymphocytes. Moreover, necroinflammation also tended to decrease. In vitro, a CB2-antagonist directly increased human HSC activation and increased apoptosis and decreased proliferation of mice/human T cells (healthy/fibrotic) and their phagocytosis. We concluded that CB2(-/-) lymphocytes exert an antifibrotic activity, whereas lack of CB2 receptor in HSCs promotes fibrosis. These findings broaden our understanding of cannabinoid signaling in hepatic fibrosis beyond their activity solely in HSCs.     

N、P营养盐胁迫对两株布朗葡萄藻生长的影响

采用批次培养方法,在光照强度60、110mol/m2s下分别设置了7个不同的氮、磷浓度(N:0-3500g/L,P:15-775g/L),研究两株布朗葡萄藻(Botryococcus braunii)对氮、磷胁迫的敏感性差异,筛选高营养利用效率的优良藻株。结果表明:两株藻对氮磷营养胁迫的耐受性存在差异,B.braunii764株对氮胁迫具有较高耐受性,而B.braunii765株对磷胁迫具有较高耐受性。光照强度110mol/m2s,不同氮浓度下B.braunii764株其平均生长速率均显著高于其他各处理组;不同磷浓度下B.braunii765株其平均生长速率显著高于B.braunii764株。在试验设定的光照强度条件下,适当增加光照强度能够显著降低氮胁迫对布朗葡萄藻生长的抑制效应。在光照强度110mol/m2s下,氮浓度3500g/L时两株布朗葡萄藻平均生长速率与在正常Chu-10培养基条件下无显著差异。磷浓度775g/L时两株布朗葡萄藻的平均生长速率均显著低于正常Chu-10培养基条件,增加光照强度对磷胁迫下藻细胞的生长无显著作用。两株布朗葡萄藻在第2天时磷吸收与初始磷浓度呈正相关关系,氮吸收在3500g/L时出现饱和现象。布朗葡萄藻的生长更容易受到培养基中磷营养胁迫的影响。