非诺贝特对培养的兔脂肪细胞表达凝血和纤溶因子的影响

目的探讨非诺贝特对培养的兔脂肪细胞表达组织因子(TF)和纤溶酶原激活物抑制剂1(PAI-1)的影响.方法取正常兔脂肪组织分离培养脂肪细胞,以不同浓度(分别为0,1,10和100μmol/L)非诺贝特孵育兔脂肪细胞24 h后收集细胞.RT-PCR测定脂肪细胞TF和PAI-1 mRNA表达.用ELISA方法测定TF和PAI-1浓度.结果不同浓度非诺贝特均可抑制兔脂肪组织细胞TF和PAI-1的表达和蛋白产生,其抑制作用呈浓度依赖性增强.在非诺贝特10μmol/L培养时兔脂肪细胞TF和PAI-1 mRNA分别为(0.504±0.016)和(1.500±0.096),明显低于对照[分别为(0.579±0.018)和(1.607±0.063),均P＜0.01].在非诺贝特100μmol/L培养时兔脂肪细胞TF和PAI-1 mRNA分别为(0.451±0.023)和(1.269±0.084),与对照比显著降低(均P＜0.001).结论非诺贝特能抑制兔脂肪细胞TF和PAI-1 mRNA和蛋白的表达,提示非诺贝特可能具有独立于降脂作用外的抗血栓作用.     

常温与低温体外循环心脏直视手术对细胞因子及补体的影响

目的探讨常温及低温体外循环心脏直视手术对细胞因子及补体的影响。方法选择先天性和风湿性心脏病患者40例,随机分为常温组及低温组各20例,分别于术晨、体外循环结束时及术后1、4、7、14 d抽取患者静脉血标本,测定血浆TNF、IL-2、C3、C4值。结果两组术前各项检查指标无显著差异。(1)两组术后1~4 d的IL-2水平较术前显著下降,至术后7 d恢复正常。体外循环结束至术后4 d,低温组IL-2显著低于常温组。(2)体外循环结束时以及术后1、4、7 d,常温组TNF水平显著低于低温组。两组体外循环结束时及术后1、4 d均高于术前,常温组至术后7 d、低温组术后14 d恢复正常。(3)体外循环结束时及术后1、7 d,常温组C3水平高于低温组,术后4 d两组无差别;常温组及低温组于体外循环结束时、术后1、4 d均低于术前,至术后7 d常温组恢复正常,低温组至术后14 d恢复至术前水平。(4)两组体外循环结束时及术后1、4 d C4水平均低于术前。体外循环结束时、术后1 d,常温组C4水平高于低温组。结论常温体外循环心脏直视手术对细胞因子及补体的影响显著轻于低温组,因而对术后机体的恢复优于低温方法。     

环氧合酶-2和血管内皮生长因子共表达与肝细胞癌血管形成的关系

目的　探讨环氧合酶 (COX) 2与肝细胞癌血管形成的关系。方法　利用免疫组织化学、Westernblot方法检测 48例肝癌组织中COX 2和血管内皮生长因子 (VEGF)蛋白及逆转录 聚合酶链反应法 (RT PCR)检测COX 2和VEGFmRNA的共表达 ,对共表达COX 2和VEGF蛋白和mRNA的肝癌组织进行微血管记数。结果　免疫组织化学检测中 ,48例肝癌组织 3 6例共表达COX 2和VEGF蛋白。类似结果见于蛋白电泳分析。RT PCR显示 ,48例肝癌组织 3 6例共表达COX 2mRNA和VEGFmRNA。两者之间的表达明显相关 (γ =0 .845 )。共表达COX 2和VEGF蛋白和mRNA的肝癌组织中 ,平均微血管数 (5 6.8± 17.5 )个 ,明显高于阴性表达组。结论　COX 2可能与肝细胞癌的血管形成有关 ,且其作用之一可能是通过上调VEGF通道来发挥的     

高半胱氨酸促THP-1巨噬细胞表达单核细胞趋化蛋白-1和辛伐他汀的调节作用

目的 :研究高半胱氨酸 (Hcy)对人单核细胞系 (THP 1)分化而来的巨噬细胞 (THP 1巨噬细胞 )表达单核细胞趋化蛋白 1(MCP 1)的影响及辛伐他汀可能存在的调节作用。方法 :在培养的THP 1中加入佛波脂(PMA) ,使终浓度为 2 0ng/ml,培养 4 8h ,细胞贴壁呈巨噬细胞样分化。他汀组和Hcy组分别加入含有辛伐他汀(10 μmol/L ,5 0 μmol/L)或不含辛伐他汀完全培养基 37℃培养 2 4h ,再加入含DL Hcy(0 1mmol/L)完全培养基 ,对照组只加完全培养基 ,培养 2～ 2 4h ,上清离心 5 0 0g ,10min ,- 2 0℃保存。用ELISA法检测上清中MCP 1蛋白的量。每孔重复 3次。结果 :与对照组比较 ,加入 0 1mmol/LHcy可使THP 1巨噬MCP 1蛋白表达升高 ,4h后显著升高 (P <0 0 5 ) ,6h达高峰 (P <0 0 1) ,12h后逐渐下降 (P <0 0 5 ) ,分别为对照组的 2 9倍、5 8倍和 2 6倍 ,2 4h与对照组无显著差异。 10 μmol/L、5 0 μmol/L辛伐他汀分别使与Hcy共孵育 6h(高峰时间 )MCP 1蛋白量下降至Hcy组的 5 7 11%、2 3 6 4 %。结论 :病理浓度的Hcy(0 1mmol/L)可时间依赖性促进THP 1巨噬细胞表达MCP 1蛋白 ,该作用可被辛伐他汀下调。     

丝裂素活化蛋白激酶磷酸酶-1对血管平滑肌细胞增殖的影响及其机制

目的 研究丝裂素活化蛋白激酶磷酸酶-1(MKP1)对血管平滑肌细胞增殖的影响及机制。方法 转染MKP1质粒72h后，收集培养的血管平滑肌细胞(VSMC)，利用P^42／P^44磷酸化抗MAPK抗体通过免疫印迹法测定MAPK活性，用流试细胞仪测定细胞周期、细胞周期素和P27蛋白的表达。结果 转染MKP1质粒后，MAPK活性明显下降，VSMC阻滞于G0-G1期，同时抑制了细胞周期素D、E的表达，P27蛋白表达却明显增加。结论 MKP1抑制VSMC增殖可能是通过降低MAPK活性，抑制细胞周期素表达和增加P27蛋白表达途径实现的。     

The severity of airways obstruction as a determinant of treatment response in COPD

Guidelines recommend that patients with COPD are stratified arbitrarily by baseline severity (FEV₁) to decide when to initiate combination treatment with a long-acting β₂-agonist and an inhaled corticosteroid. Assessment of baseline FEV₁ as a continuous variable may provide a more reliable prediction of treatment effects. Patients from a 1-year, parallel-group, randomized controlled trial comparing 50 μg salmeterol (Sal), 500 μg fluticasone propionate (FP), the combination (Sal/FP) and placebo, (bid), were categorized post hoc into FEV₁ <50% and FEV₁ ≥50% predicted subgroups (n=949/513 respectively). Treatment effects on clinical outcomes – lung function, exacerbations, health status, diary card symptoms, and adverse events – were investigated. Treatment responses based on a pre-specified analysis explored treatment differences by severity as a continuous variable. Lung function improved with active treatment irrespective of FEV₁; Sal/FP had greatest effect. This improvement appeared additive in milder disease; synergistic in severe disease. Active therapy significantly reduced exacerbation rate in patients with FEV₁ <50% predicted, not in milder disease. Health status and breathlessness improved with Sal/FP irrespective of baseline FEV₁; adverse events were similar across subgroups. The spirometric response to Sal/FP varied with baseline FEV₁, and clinical benefits were not restricted to patients with severe disease. These data have implications for COPD management decisions, suggesting that arbitrary stratifications of baseline severity are not necessarily indicative of treatment efficacy and that the benefits of assessing baseline severity as a continuous variable should be assessed in future trials.     

地塞米松对内毒素作用下人脐静脉内皮细胞表达组织因子、凝血酶调节蛋白和蛋白S的影响

目的观察地塞米松(DEX)对内毒素(LPS)作用于人脐静脉内皮细胞(HUVEC)后表达组织因子(TF)、凝血酶调节蛋白(TM)和蛋白S(PS)的影响.方法24孔板培养的第1～5代HUVEC,在含不同浓度LPS和DEX的无血清培养基中培养一定时间后裂解细胞,应用酶联免疫吸附法(ELISA)测定裂解液中的TF、TM和PS含量.结果在LPS刺激下,HUVEC表达TF的量呈剂量依赖性升高,在LPS0.1μg/ml下TF的表达量为对照组的4倍(P＜0.01),同时加入0.5 μg/ml和1.0 μg/ml DEX则可使TF的表达量由128.3±25.7 pg/105细胞分别降至94.9±19.4 pg/105细胞和98.8±7.8 pg/105细胞(P＜0.05);LPS(0.01～10μg/ml)可抑制HUVEC表达TM,在LPS 10 μg/ml下,TM表达量降至对照组的60%(P＜0.05).DEX可拮抗LPS抑制HUVEC表达TM的效应,0.1 μg/ml、0.5 μg/ml和1.0 μg/ml DEX可使LPS(10 μg/ml)作用下TM的表达量由0.282±0.014 ng/105细胞分别增至0.409±0.009、0.462±0.017和0.362±0.019 ng/105细胞(P＜0.05);LPS(0～10 μg/ml)可抑制HUVEC表达PS,在LPS浓度1.0 μg/ml及10 μg/ml时,PS的表达量分别为对照组的43%和38%(P＜0.01).DEX则拮抗LPS抑制HUVEC表达PS的效应,0.5 μg/ml DEX可使LPS刺激下PS的表达量由13.1±4.8%/2×105细胞增至48.5±10.2%/2×105细胞(P＜0.01).结论LPS促进HUVEC表达TF,抑制HUVEC表达TM和PS.DEX能部分拮抗上述作用,提示DEX可能纠正内毒素血症时的高凝状态.     

血小板第4因子对辐射损伤小鼠免疫功能的保护作用

目的：探讨血小板第4因子（plateletfactor4，PF4）对辐射损伤小鼠免疫系统的影响。方法：雄性BALB／c小鼠随机分为3组，第1组（单纯照射组）、第Ⅱ组（PF4保护组）、第Ⅲ组（正常对照组），第Ⅱ组在照射前26h及20h腹腔注射PF440μg／kg，全身一次性5Gy60Co—γ射线照射后瑞氏染色法计数外周血淋巴细胞百分数。胸腺、脾脏制成细胞悬液计数后，MTT比色法测定胸腺及脾细胞增殖能力。结果：第Ⅱ组小鼠外周血淋巴细胞百分数下降趋势较第1组明显减慢。胸腺、脾细胞计数，第Ⅱ组明显高于第1组。淋巴细胞增殖试验，第Ⅱ组与第1组相比，小鼠胸腺及脾细胞的增殖能力明显增强。结论：PF4对免疫系统有辐射保护作用，可明显增强辐射损伤小鼠的免疫功能。     

靶向性蛋白激酶B1和环氧合酶-2 shRNA腺病毒载体的构建和在人胃癌细胞的表达

Objective To construct a short hairpin RNA (shRNA) adenovirus vector targeting protein kinase BI (PKB1/Akt1) and cyclooxygenase-2 (COX-2) and observe their expression in human gastric carcinoma cell line SGC-7901. Methods Akt1 and COX-2 shRNA expression frames were sub-cloned to pGSadeno adenovirus vector by homologous recombination technology to construct pGSadeno-Aktl + COX-2 ( pGSadeno-A + C) vector. Furthermore after screening and amplification,recombinant ade-novirus vector was digested with Pacl and transfected into HEK293 cells. The replication adenovirus rAd5-A + C was packed and amplified in the HEK293 cells, and its titer was detected. After human SGC-7901 cells in vitro were transfected by rAd5-A + C,Akt1 and COX-2 mRNA and protein expression levels were detected by real-time PCR and Western blot respectively. Compared with rAdS-A + C,SGC-7901 and gen-eral rAd5-HK were selected as the negative controls. Results The recombinant adenovirus rAd5-A + C was constructed successfully and its titer reached 1.0 ×1010 pfu/ml. Aktl and COX-2 mRNA expression was downregulated significantly, and their ACt values ( 12.26±0.05 and 5.41±0.09 respectively ) were higher than rAd5-HK group (10.63±0.02 and 3.75 +0.08 respectively) and control group (10.57± 0.02 and 3.73±0.08 respectively) (P <0.01 ). There was no significant difference between rAd5-HK and control groups (P >0.05). Aktl and COX-2 protein expression was downregulated by 70.5% and 63.7% respectively ( P < 0.01 ) in rAd5-HK group as compared with control group ( P > 0.05 ). Conclu-sion The shRNA aclenovirus vector targeting Akt1 and COX-2 can specifically inhibit Akt1 and COX-2 expression,and this may be a new strategy in gastric carcinoma gene therapy targeting Akt1 and COX-2.     

单纯性肥胖及2型糖尿病儿童胰岛素受体底物-1的研究

目的:探讨单纯性肥胖及2型糖尿病儿童胰岛素受体底物-1(IRS-1)表达的改变。方法:对20例单纯性肥胖儿童,20例2型糖尿病儿童及20例对照组儿童,采用细胞免疫技术进行白细胞染色,运用图像分析软件计算光密度值,从而定量分析白细胞中IRS-1的含量变化。结果:肥胖组、2型糖尿病组白细胞中IRS-1表达下降,且与对照组相比有统计学意义(P<0.05)。结论:肥胖组、2型糖尿病组白细胞中IRS-1表达下降,与对照组相比有统计学意义(P<0.05),提示肥胖组与2型糖尿病组儿童胰岛素信号传递中受体后作用的关键底物缺陷,影响了胰岛作用的发挥。提示IRS-1与胰岛素抵抗有关,有利于进一步理解2型糖尿病的发病机制,指导临床治疗。