小檗胺诱导K562细胞凋亡及其与bcr/ablgene及P210表达的关系

目的:探讨小檗胺(BER)诱导K562细胞凋亡及其可能的机制。方法:以流式细胞仪(FCM)分析、电镜观察细胞微结构变化及基因组DNA电泳等方法检测细胞凋亡。以RT-PCR及Westernblot方法检测K562细胞BCR/ABLmRNA和蛋白质水平表达。结果:FCM检测见到典型的凋亡峰,8.0mg/LBER作用24-72h,随药物作用时间延长,细胞凋亡率由(29.20±3.82)%上升至(61.77±4.35)%(P＜0.01);以2.0-8.0mg/LBER作用24h,随药物浓度增加,K562细胞的凋亡率也增加。电镜下可见明确的细胞凋亡的形态学改变。DNA电泳呈现典型的梯形条带。16.0mg/LBER处理24h,K562细胞bcr/ablmRNA相对表达量及BCR/ABL融合蛋白质P210水平均明显低于对照组,分别为0.73±0.02vs1.19±0.02(P＜0.01)和0.63±0.01vs1.04±0.02(P＜0.01),呈时间-浓度依赖效应。经BER作用后,K562细胞bcr/ablmRNA表达强度与P210水平呈正相关(r=0.928,P＜0.05),且细胞凋亡率与bcr/ablmRNA表达呈负相关(r=-0.997,P＜0.01)。结论:在体外BER对K562细胞有明显的促凋亡作用,抑制bcr/ablmRNA表达及其蛋白质水平可能是其作用的重要机制之一。     

大学生感觉寻求人格特征与脑电诱发电位的关系

目的:研究大学生感觉寻求人格特征与脑电诱发电位的相关性.方法:测试大学生感觉寻求及MMPI人格特征,分析长潜伏期听觉诱发电位与感觉寻求人格特征的相关性,寻找感觉寻求人格特征的生物学标志,并进一步探讨感觉寻求人格特征的生物学基础.结果:1.高、低感觉寻求组轻躁狂(t=3.1)以及抑郁(t=3.62)分量表得分具有显著性差异(P均＜0.01),高感觉寻求组的抑郁得分较低,轻躁狂得分较高,而低感觉寻求组则与之相反.2.高感觉寻求者具有快速习惯化的特点(tc2=2.4,tc3=2.6,tc4=2.5,P均＜0.05).结论:1.感觉寻求人格特征呈现极端形式者(低或高)可能容易出现与抑郁、轻躁狂相关的精神问题.2.与强度依赖性相比,快速习惯化现象可能是高感觉寻求者的一个更加显著的电生理标志.     

体外分化胚胎干细胞为造血干细胞重建造血功能的研究

目的：探讨体外定向分化胚胎干细胞（ESCs）为造血干细胞（HSCs）对体内造血功能的重建作用。方法：将小鼠E14.1胚胎干细胞采用“三步诱导法”在体外分化发育为HSCs，造血克隆形成(CFU)实验观察其体外造血集落形成情况，免疫磁珠分选纯化HSCs移植给经亚致死剂量γ射线照射的雌性SCID小鼠，观察其植入及小鼠造血功能恢复情况。结果: 经过分阶段诱导，多种造血刺激因子联合应用能有效促进ESCs定向分化发育为HSCs,流式细胞仪检测HSCs特异性表面标志物CD34+/Sca-1+表达最高为（58.64±4.20）%，CFU培养能形成较多的红系、粒系/巨噬细胞系及混合细胞集落, Wright-Giemsa 染色显示为原始的造血细胞。此阶段的HSCs经分选纯化后移植给经γ射线照射后的小鼠，移植组小鼠+10 d造血功能开始恢复，观察40 d后除血小板恢复较慢外，白细胞、红细胞、血红蛋白等指标已接近正常，植入率为71.4%，存活率为43.0%，染色体检测证实已由受体鼠的XX转为供体鼠的XY。结论: 采用分阶段诱导的方法，可在体外定向诱导小鼠ESCs分化发育为HSCs，此来源的HSCs可以有效重建体内造血功能。     

The pathogenesis of spinal cord involvement in dengue virus infection

To investigate the mechanisms of dengue (DEN) virus transmission within the spinal cord, severe combined immunodeficient mice were intracerebrally inoculated with DEN virus type 2. After inoculation, a high virus titer and antigens were detected in the brain and spinal cord. At early stages of the infection, ultrastructural examinations showed that a few virions were present in the cytoplasm of ependymal cells lining the central canal. As the infection progressed, virions were observed in the lumen of the rough endoplasmic reticulum (RER), RER-derived vesicles and the Golgi region of infected neurons. These data suggest that the inoculated DEN virus might spread to the neurons of the spinal cord via the cerebral spinal fluid and cause several neuronal pathological responses. Moreover, DEN virus was also observed in myelinated and unmyelinated nerve fibers and typical neuronal synapses. Some virion-containing vesicles appeared to be fused with the membrane of presynapses, indicating that neuron-to-neuron transport of DEN virus might occur in the spinal cord. Additionally, anterior, lateral and posterior horns of the spinal cord exhibited different numbers of the positive neurons and different staining intensities of the DEN antigen during the infection. This difference likely represents variation of susceptibility to the DEN virus among the neurons of the spinal cord.     

血清CA125测定对卵巢恶性肿瘤的诊断及随访复发的价值

本文采用放射免疫法对９８例６１５份血清进行糖类抗原ＣＡ１２５值的测定，其中正常对照３０例，卵巢良性肿瘤２５例，交界性肿瘤１例，卵巢恶性肿瘤４２例。对恶性肿瘤患者中２４例同时进行了阴道超声检查的随访监测，发现卵巢恶性是血清ＣＡ１２５值明显高于良性肿瘤和正常对照组（Ｐ〈０．０１）；良性肿瘤ＣＡ１２５值与正常对照组无显著性差异（Ｐ〉０．０５）。术前卵巢恶性肿瘤阳性检出率８５．１９％，其中卵巢上皮性癌阳性     

强力霉素影响基质金属蛋白酶活性和血管重构的实验研究

目的：观察强力霉素对损伤动脉组织中基质金属蛋白酶（MMP）活性的抑制作用，并探讨强力霉素对血管平滑肌细胞增殖、动脉内膜增生、管腔重构的影响。方法:球囊导管扩张动脉的方法建立大鼠颈总动脉损伤模型。治疗组用强力霉素30 mg·kg^-1·d^-1干预。明胶酶谱法测定损伤动脉组织中MMPs的活性。用HE染色、VVG染色、免疫组化标记α-actin和增殖细胞核抗原的方法观察损伤动脉内膜厚度、管腔重构及平滑肌细胞增殖的情况。结果:①强力霉素治疗组MMP-9活性在术后24 h、3 d分别比对照组低26.3％、34.5％（P<0.01）；MMP-2活性在术后7 d比对照组低40.0％（P<0.01）。②强力霉素治疗使术后7 d内膜平滑肌细胞增殖率（43.23％±1.06％）显著低于对照组（62.76％±1.02％）（P<0.01）；使术后14 d、28 d新生内膜厚度比对照组分别少32.0％、38.8％（P<0.01），而管腔面积比对照组多58.0％、90.4％（P<0.01） 。结论：强力霉素可以显著降低血管损伤后MMPs活性，抑制内膜平滑肌细胞的增殖、新生内膜增生以及管腔重构，提示它可能具有防治PTCA术后再狭窄的作用。     

Cx40和Cx43调节大鼠肠系膜上动脉收缩反应性与钙敏感性的机制

目的：研究连接蛋白Cx40/Cx43对大鼠肠系膜上动脉内膜依赖的血管收缩反应性与钙敏感性的调节作用机制。方法:以SD大鼠肠系膜上动脉（SMA）为研究对象，用Cx40或Cx43反义寡脱氧核苷酸（Cx40/Cx43AODN）阻断SMA Cx40或Cx43表达，观察缺氧处理后SMA的收缩反应性、钙敏感性、肌球蛋白轻链磷酸酶/激酶（MLCP/MLCK)的活性、20 kD的肌球蛋白轻链（MLC₂₀）磷酸化程度的变化。结果:Cx40AODN可以降低正常组、1 h和3 h缺氧组SMA MLCP活性，增加MLC₂₀磷酸化水平，改善血管的钙敏感性和内膜依赖的收缩反应性；Cx43AODN可以增加各组血管的MLCP活性，减少MLC₂₀磷酸化水平，降低血管的钙敏感性和内膜依赖的收缩反应性。Cx40和Cx43AODN对SMA MLCK活性无明显作用。结论:Cx40和Cx43主要通过调节血管平滑肌细胞的MLCP活性和MLC₂₀磷酸化水平调节血管的钙敏感性，从而调节休克后内膜依赖的血管收缩反应性。     

Inhibitory effect of ketamine on phosphorylation of the extracellular signal-regulated kinase1/2 following brain ischemia and reperfusion in rats with hyperglycemia

To determine if the inhibitory effects of ketamine on the extracellular signal-regulated kinase (ERK) 1/2 are involved in reduction of the hyperglycemia-exaggerated cerebral ischemic lesion, rats with normoglycemia, hyperglycemia, or hyperglycemia supplemented with ketamine were subjected to 15 min of forebrain ischemia, and then, reperfusion for 0.5, 1, and 3h. Phosphorylation of ERK1/2 in the brain tissues was assessed by immunohistochemistry and Western blot analysis. In rats with normoglycemia, we demonstrated a moderate increase of the ERK1/2 phosphorylation in the cingulum cortex and hippocampus CA3 following an ischemic intervention. It quickly dropped to control levels after reperfusion for 0.5h. In rats with hyperglycemia, however, the increase of the ERK1/2 phosphorylation in these areas was significantly higher in all animals reperfused. The neuronal death, detected by the TdT-mediated-dUTP nick end labeling assays, was found in the cingulum cortex (5.23+/-2.34, per high power feild) and hippocampus CA3 areas (6.29+/-3.68, per 1mm(2)) in hyperglycemic group after reperfusion for 3h. With ketamine treatment, the ERK1/2 phosphorylation in cingulum cortex and hippocampus CA1 and CA3 areas was found to be the same as that in normoglycemia rats. Our results suggest that hyperglycemia may increase the ischemic insult through modulation of the signal transduction pathways involving ERK1/2. The inhibitory effects of ketamine on the hyperglycemia-activated ERK1/2 phosphorylation are probably through inhibition of the N-methyl d-aspartate-mediated calcium influx, which subsequently reduce the hyperglycemia-exaggerated cerebral damage.     

抗HER-2抗体chA21对人乳腺癌SKBR3细胞凋亡的诱导作用及其机制

目的探讨抗HER-2工程抗体chA21在体外对高表达HER-2的人乳腺癌SKBR3细胞凋亡的诱导作用及其分子机制。方法采用透射电镜和原位末端标记技术(TUNEL)观察和检测chA21对SKBR3细胞凋亡的诱导,采用免疫细胞化学技术检测凋亡相关基因bc l-2、bax、Fas及caspase-3表达的改变。结果chA21作用72 h,可见SKBR3细胞凋亡,chA21高浓度组(5.4mg/L)凋亡指数显著高于低浓度组(0.2 mg/L)(P<0.01);chA21处理组SKBR3细胞的bax、Fas及caspase-3表达增加,而bc l-2表达及bc l-2/bax比值降低,上述改变在chA21高、低两个浓度组间有显著差异(P<0.01)。结论chA21在体外可诱导SK-BR3细胞凋亡,其分子机制与调节凋亡相关基因bax、bc l-2、Fas及caspase-3的表达有关。     

NMDA受体在β-淀粉样蛋白引起海马神经元突触蛋白改变中的作用

为了研究NMDA受体活性对Aβ引发的海马神经元突触蛋白表达变化的影响,本文运用免疫细胞化学方法检测不同浓度NMDA受体激动剂以及拮抗剂对Aβ诱导的海马神经元突触蛋白变化的影响。结果显示:NMDA可浓度依赖性地缓解Aβ25-35引起的突触蛋白synaptophysin与PSD-95的减少。抑制突触内NMDA受体,NMDA缓解Aβ减少突触蛋白的作用减弱;抑制突触外NMDA受体,对抗Aβ的作用无显著变化。本研究结果提示NMDA受体活性改变影响Aβ诱导的突触蛋白减少,突触内NMDA受体激活可对抗Aβ的毒性作用。突触内NMDA受体活性减弱可能在谷氨酸兴奋毒性中发挥作用。