公共文化服务平台

共 4 条记录，以下是 1-4

全选清除导出

排序方式：

高剂量O-糖基化修饰抑制剂Benzyl-α-GalNAc诱导体外培养肝细胞脂肪变: 2013年; 目的初步探讨蛋白质O-糖基化抑制剂Benzyl-α-GalNAc对肝细胞的影响。方法取雌性Balb／c小鼠（8～10周）20只随机分为正常组（n=10），Benzyl—d—GalNAc药物组（n=10），给Benzyl-α-GalNAc药物（5mg／kg，1次／d）灌胃。第2周末取小鼠血清及肝脏进行血清生化指标AIJT及AlJP测定及肝组织HE染色。培养HepG2细胞．Benzyl-α-GalNAc分别以0．5、1及5mg／ml与HepG2细胞共孵育。24h后进行油红O染液染色。5mg／ml药物组完全未贴壁，去除处理因素，继续培养12h观察细胞。Benzyl-α-Gal—NAc以3mg／ml处理HepG2细胞12h及24h观察细胞贴壁情况。培养L02细胞，Benzyl-α-GalNAc分别以0．1及0．5mg／ml与L02细胞共孵育。24h后进行油红O染液染色。结果药物组与正常对照组比较，肝组织切片显示轻微脂肪变。油红O染色显示药物处理组HepG2及L02细胞内的脂滴积聚。高浓度组细胞完全没有贴壁，24h后更换无药物培养基，去除处理因素12h后，可见HepG2开始贴壁生长。结论高浓度O-糖基化抑制剂Benzyl-α-GalNAc抑制体外肝细胞的黏附，并诱导轻微肝细胞脂肪变。; 张晓静张仁雯郝晓花任慧李红敏刘燃王智强魏红山; 关键词：肝细胞脂肪变

Role of C6ORF120, an N-glycosylated protein, is implicated in apoptosis of CD4＋ T lymphocytes被引量：9: 2011年; Background Although CD4＋ T cell apoptosis and CD8＋ T cell responses have been extensively studied during HIV infection, how apoptosis signals being initiated in CD4＋ T cells still need to be elucidated. The present study was designed to characterize the function-unknown gene, C6orf120, and elucidates its primary role in tunicamycin-induced CD4＋ T apoptosis. Methods The C6orf120 coding sequence was amplified from peripheral blood mononuclear cells （PBMCs） total RNA of AIDS patients. The DNA fragment was inserted into the pET-32a expression system, transformed into Escherichia coli, and preparation of C6ORF120 recombinant protein. The magnetic cell separation technology was used to prepare primary CD4＋ T cells and CD8＋T cells. The primary T cells were cultured at 1×10^6 cells/ml, treated with 0, 0.1,1, 10, 100 and 200 ng/ml of C6orf120 recombinant protein for 48 hours, then harvested for cell cycle and apoptosis analysis. Tunicamycin （0.5 μmol/L） was used to induce endoplasmic reticulum stress in Jurkat cells. The biomarker 78 KDa glucose-regulated protein （GRp78） and growth arrest and DNA damage （GADD） were used to evaluate endoplasmic reticulum stress of Jurkat cells. Results We prepared C6ORF120 recombinant protein and its polyclonal antibody. Immunohistochemical analysis showed that C6orf120 mainly expressed in hepatocytes and cells in germinal center of lymph node. At concentration of 0.1, 1, 10, 100, and 200 ng/ml, C6orf120 recombinant protein could induce apoptosis of Jurkat cells and primary CD4＊T cells, and promoting G2 phase of its cell cycle. Western blotting analysis showed that C6ORF120 recombinant protein increased the expression of GRp78 and GADD in Jurkat cells in vitro. Conclusion Our results suggested that C6ORF120 could induce apoptosis of CD4＋ T cells, at least in part, mediated with endoplasmic reticulum stress.; LI XinQIAO YongCHANG Lu-siXIAO FanLU Lian-heHAO Xiao-huaZHANG Ren-wenWU HaoWEI Hong-shan; 关键词：HIV/AIDS APOPTOSIS

分泌蛋白编码基因THEM6克隆表达及组织细胞分布: 2013年; 目的体外克隆表达THEM6，诱导重组蛋白，制备多克隆抗体，明确在不同组织细胞的表达特征。方法以外周血单核细胞总RNA反转录得到的cDNA为模板，扩增THEM6基因片段，诱导剂IFrG诱导THEM6重组蛋白表达，制备多克隆抗体，分析特异性、检测效价。用CCK-8检测试剂盒，分析THEM6重组蛋白对Jurkat细胞增殖的影响；观察该蛋白的组织、细胞系表达分布。结果成功体外克隆THEM6．获得重组蛋白及抗THEM6的多克隆抗体，ELISA （enzyme-linked immuno sorbent assay）酶联免疫吸附测定检测效价〉1280000；低浓度THEM6重组蛋白对Jurkat细胞增殖有影响，THEM6蛋白在Jurkat细胞等多种细胞及淋巴、肝脏等多种组织中表达。，结论THEM6基因在多种组织细胞中有广泛表达。; 李红敏任慧乔雍郝晓花刘燃王智强魏红山; 关键词：乙型肝炎病毒重组蛋白多克隆抗体

糖基化修饰在包膜病毒感染过程中的作用: 2021年; 包膜病毒感染过程中,劫持宿主细胞的糖基化修饰系统对自身抗原进行修饰,籍此逃脱宿主的免疫监视,是病毒感染的重要机制。而且,包膜蛋白的糖基化修饰,一方面发挥抗原屏蔽效应,导致疫苗研发更为困难;另一方面,修饰的聚糖对抗原表位结构也具有空间重构效应。因此,包膜病毒的中和抗体与修饰聚糖的结构有关。除此之外,抗原蛋白的糖基化修饰也与病毒识别、黏附,组织嗜性,病毒颗粒组装的质量控制以及毒性与侵袭力有关。本文对该领域的研究现状做一综述。; 何玲玲张成周蓉蓉魏红山; 关键词：病毒抗原

全选清除导出

共1页<1>

国家自然科学基金(81071411)

文献类型

领域

主题

机构

作者

传媒

年份

用户反馈

国家自然科学基金(81071411)

文献类型

领域

主题

机构

作者

传媒

年份

用户登录

用户反馈