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胆囊收缩素对脂多糖刺激大鼠肺泡巨噬细胞的影响被引量：1: 2006年; 孟爱宏凌亦凌阎锡新; 关键词：八肽胆囊收缩素肺泡巨噬细胞促炎性细胞因子内毒素休克 CCK

c-fos在CCK-8抗LPS所致的肺动脉平滑肌细胞损伤中的变化被引量：3: 2003年; 目的 :观察c -fos在八肽胆囊收缩素 (CCK - 8)减轻脂多糖 (LPS)所致的肺动脉平滑肌细胞 (PASMC)损伤中的变化。方法 :贴块法培养大鼠PASMC。应用电镜技术和生化方法 ,观察细胞形态和测定细胞丙二醛 (MDA)含量及乳酸脱氢酶 (LDH)释放率 ;台盼蓝染色法记录PASMC蓝染率的变化 ;免疫细胞化学技术检测细胞内c -fos蛋白的表达情况。结果 :CCK - 8可减轻LPS引起的细胞超微结构损伤 ;CCK - 8可降低LPS引起的细胞台盼蓝摄取率、MDA含量与LDH释放率的增高 ;LPS可轻微上调PASMC内c-fos蛋白表达 ,CCK - 8可使该上调作用显著上升。结论 :CCK - 8可减轻LPS所致的PASMC损伤 ;CCK - 8可能通过使c -fos蛋白表达上调来发挥其抗损伤作用。; 黄新莉凌亦凌鲁平刘岩王建钦艾洁; 关键词：脂多糖类八肽胆囊收缩素原癌基因蛋白质C-FOS CCK-8 内毒素休克

p38 MAPK和STAT3参与CCK-8抑制LPS诱导的大鼠促炎症细胞因子生成被引量：8: 2013年; 目的:观察八肽胆囊收缩素(CCK-8)是否改善脂多糖(LPS)引起的大鼠细胞因子的变化,并探讨p38丝裂原活化蛋白激酶(p38 MAPK)和信号转导子及转录激活子3(STAT3)的信号转导作用,以及CCK受体(CCK-R)的作用。方法:4组大鼠尾静脉分别注入生理盐水(对照)、LPS(8 mg/kg)、CCK-8(40μg/kg)和CCK-8(40μg/kg)+LPS(8 mg/kg),酶联免疫吸附法(ELISA)检测血清、肺脏及脾脏中肿瘤坏死因子α(TNF-α)、白细胞介素1β(IL-1β)和IL-6的变化,Western blotting和免疫荧光双标激光共聚焦显微镜检测肺脏和脾脏磷酸化p38MAPK和磷酸化STAT3的表达,RT-PCR检测脾脏CCK-R亚型的mRNA表达。结果:CCK-8可显著抑制LPS诱导的TNF-α、IL-1β和IL-6的增加。CCK-8可增加LPS诱导的大鼠肺脏和脾脏磷酸化p38 MAPK和磷酸化STAT3的表达。LPS有诱导CCK-AR及CCK-BR mRNA表达量增加的作用。结论:CCK-8对LPS刺激的大鼠促炎症细胞因子过量产生有抑制作用,p38 MAPK和STAT3可能参与了其信号转导机制。LPS刺激时,CCK-R受体发生正向调节,CCK-8有可能用于治疗全身性感染及其它的炎症性疾病。; 孟爱宏凌亦凌张霄鹏; 关键词：胆囊收缩素脂多糖类细胞因子

CCK-8 inhibits expression of TNF-α in the spleen of endotoxic shock rats and sigual transduction mechanism of p38 MAPK被引量：19: 2002年; AIM:To study the effect of sulfated cholecystokinin-octapeptide(CCK-8)on systemic hypotension,gene andprotein expression of TNF-α in spleen of lipopolysaccharide(LPS)-induced endotoxic shock(ES)rats,and furtherinvestigate the signal transduction mechanism of p38mitogen-activated protein kinase(MAPK).METHODS:The changes of blood pressure were observedusing physiological record instrument in four groups of rats:LPS(S mg·kg^(-1),iv),CCK-8(40μg·kg^(-1),iv)pretreatment10 rain before LPS(8 mg·kg^(-1)),CCK-8(40μg·kg^(-1),iv)ornormal saline(control)group.The content of TNF-αinspleen was assayed 2 h after LPS administration usingELISA kit and the expression of TNF-α mRNA was examined30 min,2 h and 6 h after LPS administration by reversetranscribed polymerase chain reaction(RT-PCR).Activationof p3S MAPK was detected with Western blot 30 min afterLPS administration.RESULTS:CCK-8 reversed LPS-induced decrease of meanarterial pressure(MAP)in rats.The content of TNF-α inspleen was(282±30)ng·L^(-1)in control group,while itincreased to(941±149)ng·L^(-1)in LPS group,P<0.01.CCK-8 significantly inhibited the LPS-induced increase ofTNF-α content in spleen.It decreased to(462±87)ng·L^(-1)inCCK-8+LPS group,P<0.01.The expression of TNF-αmRNA 30 min and 2 h after treatment was stronger in LPSgroup,while it was lowered after CCK-8 pretreatment.Thep38 MAPK expression increased significantly in LPS group(5.84 times of control)and CCK-8 increased the activationof p38 MAPK in ES rats(10.74 times of control).CONCLUSION:CCK-8 reverses the decrease of MAP in ESrats and has inhibitory effect on the gene and proteinexpression of TNF-α in spleen,and p38 MAPK may beinvolved in its signal transduction mechanisms.; Ai-Hong Meng Yi-Ling Ling Xiao-Yun Zhao Jun-Lan Zhang Department of Pathophysiology,Hebei Medical University,Shijiazhuang 050017,Hebei Province,China Xiao-Peng Zhang Department of Chest Sugery of Hebei Provincial People’s Hospital,Shijiazhuang 050000,China; 关键词：CCK-8 TNF-Α 内毒素休克

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