氟伐他汀对高脂血症兔心肌缺血再灌注损伤心肌局部细胞间粘附分子-1的影响

目的:研究氟伐他汀对高脂血症兔心肌缺血再灌注损伤心肌局部细胞间粘附分子-1(ICAM-1)表达的影响。方法:30只高脂喂养的日本大耳白兔随机分为3组(n=10):缺血再灌注组;氟伐他汀组,缺血再灌注前3 h,氟伐他汀10 mg·kg-1口服给药;假手术组。实验中监测心电图及心功能,实验完毕取心肌组织,Evans蓝及氯化三苯基四氮唑(TTC)染色测心肌梗死程度,逆转录聚合酶链反应法(RT-PCR)测心肌局部ICAM-1 mRNA表达。结果:缺血再灌注后,与缺血再灌注组相比,氟伐他汀组心肌局部ICAM-1mRNA表达降低(P<0.01),心肌梗死程度降低(P<0.01),心功能显著改善。结论:ICAM-1mRNA表达增高是心肌缺血再灌注损伤的重要因素,氟伐他汀短期预治疗可降低ICAM-1 mRNA表达,降低心肌梗死程度,改善心功能。

滋养层细胞促融合表位肽抗生育作用的初步研究

目的合成多价抗原肽,观察其体液免疫效果,并初步评估其抗生育潜力。方法选择人滋养层细胞促融合表位模拟肽与一种通用辅助T细胞表位(PADRE)作为骨架,合成多价抗原肽(MAP)结构的免疫原,与等量弗氏佐剂混悬后免疫雌性C57BL/6小鼠,观察体液免疫反应的特点及抗血清干扰滋养细胞融合的效果。结果在431A固相自动肽合成仪上成功地合成了MAP多肽,并经HPLC纯化、质谱鉴定证实其纯度达95%以上;其在小鼠血清中诱导出的特异性抗体的滴度最高达1:1024,且可以特异识别滋养层细胞相关抗原表位;在1:10稀释的抗血清存在时,forskolin诱导的人绒癌细胞(BeWo)间融合显著减少(P<0·01)。结论由含有人滋养层细胞促融合表位模拟肽、具有特异性氨基酸序列的新抗原所制备的抗血清可识别滋养层细胞相关天然抗原表位,并在小鼠体内激发出较理想的特异性体液免疫,同时,抗血清对BeWo细胞间融合具有一定抑制作用。

PDT/GR-ΔLBD融合蛋白的表达、纯化及穿膜特性的鉴定

目的构建穿膜肽(PDT)和缺失结合配体结构域的小鼠糖皮质激素受体(GR-ΔLBD)融合基因表达载体,经原核表达、纯化后,进行穿膜特性的鉴定。方法质粒pEGFP-GR-ΔLBD经双酶切,获得目的基因片段GR-ΔLBD,将该基因片段亚克隆入原核表达载体pGEX-PDT,获得pGEX-PDT/GR-ΔLBD融合基因表达载体。将表达载体转化大肠杆菌,经IPTG诱导表达、谷胱甘肽-琼脂糖树脂处理、谷胱甘肽洗脱液洗脱后,获得PDT/GR-ΔLBD融合蛋白,SDS-PAGE分析融合蛋白;采用荧光素FITC体外标记PDT/GR-ΔLBD融合蛋白(终浓度分别为0、500、1000nmol/L),与小鼠肺上皮细胞TC-1共培养2h,在荧光显微镜下观察其穿膜特性。结果成功构建了融合基因原核表达载体pPDT/GR-ΔLBD,并能表达蛋白产物,大小约78.6kD,与融合蛋白PDT/GR-ΔLBD的理论计算值(80kD)相符。随着PDT/GR-ΔLBD浓度的增加,进入TC-1上皮细胞的PDT/GR-ΔLBD明显增多,并可在胞核中浓聚。结论 PDT/GR-ΔLBD融合蛋白具有良好的可溶性和穿膜特性,为进一步研究PDT/GR-ΔLBD融合蛋白在抗炎过程中的作用奠定了基础。

Increased resistance to apoptosis during differentiation and syncytialization of BeWo choriocarcinoma cells

Transition from mononuclear villous cytotrophoblast into multinuclear syncytiotrophoblast in the human placenta is accompanied by changes in apoptosis-related proteins and an apparent increased resistance to induced apoptosis. We investigated the specific nature and timing of changes in Bcl-2, Bax, p53, and caspases 3 and 8 in forskolin-treated BeWo choriocarcinoma cells, a model for villous cytotrophoblast differentiation. BeWo cells were treated with forskolin or vehicle alone for up to 72 h and evaluated at 24 h intervals for syncytialization and quantitative expression specific apoptosis-related proteins and mRNAs. Syncytialization was quantified using fluorescent staining of intercellular membranes and enumeration of the percentage of nuclei in multinucleate cells, and differential localization of apoptosis-related proteins to multinuclear or mononuclear cells was determined by quantitative immunofluorescence. Forskolin treatment for up to 72 h resulted in 80% syncytialization, increased expression of Bcl-2 protein (P ) and mRNA (P ), and significantly decreased expression of protein and mRNA for Bax, p53, and caspases 3 and 8. Syncytialized cells expressed higher levels of Bcl-2 protein concurrent with increased resistance to cisplatin-induced apoptosis. Thus, syncytialization of BeWo cells was accompanied by altered transcription of apoptotic-related proteins characteristic of increased apoptosis resistance secondary to increased expression of the anti-apoptotic protein Bcl-2 and diminish expression of pro-apoptotic proteins.

原子力显微镜单分子力谱研究ICAM-1/CD11b相互作用及药物干预的影响

目的利用绿色荧光蛋白(GFP)标记人细胞间黏附分子-1(ICAM-1),观察GFP是否影响ICAM-1在细胞膜表面的定位,实现ICAM-1可视化。应用原子力显微镜(AFM)单分子力谱研究ICAM-1/CD11b相互作用,并探讨瑞舒伐他汀(RSV)及单抗类药物干预的影响。方法从人脐静脉内皮细胞(HUVEC)中提取总RNA,设计合成PCR引物(两端分别含有Bam HⅠ、HindⅢ特异性酶切位点),使用RT-PCR扩增获取ICAM-1cDNA编码区序列,经测序分析筛选正确序列,与pEGFP-N1表达载体相接,即得到基于GFP的重组质粒pICAM-1-GFP,脂质体介导转染COS-7细胞,通过荧光显微镜观察融合蛋白pICAM-1-GFP在COS-7上的定位。AFM单分子力谱测量该细胞模型上单对黏附分子ICAM-1/CD11b的相互作用力值,应用RSV及抗ICAM-1单克隆抗体干预,检测黏附力值是否有变化。结果序列分析RT-PCR扩增获得的片段为人ICAM-1的cDNA编码区,pICAM-1-GFP发出绿色荧光定位于COS-7细胞表面。单对黏附分子ICAM-1/CD11b的相互作用力值约为42pN,RSV干预对此值无明显影响,而抗ICAM-1单克隆抗体则有效降低了此单对黏附分子亲和力。结论荧光蛋白GFP能融合于ICAM-1的C端,且不影响ICAM-1在COS-7细胞膜表面的定位表达。RSV不能通过直接阻断单分子ICAM-1或CD11b影响其相互作用,可能是通过有效抑制ICAM-1表达量的增加从而发挥抗动脉粥样硬化炎症进程作用。抗ICAM-1单克隆抗体有效降低黏附分子亲和力,提示单抗类药物在抗炎治疗领域的应用前景。该研究建立的方法模型可作为活细胞体系探讨单对黏附分子亲和力及药物干预影响的重要研究手段。