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壳聚糖载基因纳米粒子荧光标记的优化研究被引量：3: 2008年; 目的研究荧光素异硫氰酸酯(FITC)与壳聚糖反应的主要影响因素,观察荧光标记对纳米粒子表征和转染效率的影响,以期建立一种快速、稳定并且适宜壳聚糖纳米载体示踪的荧光标记方法。方法FITC与壳聚糖在不同反应物比例、溶液pH及温度条件下反应,纯化并收获产物,计算其标记效率。采用复凝聚法制备荧光标记的壳聚糖载基因纳米粒子,并检测其表征及对Hela细胞转染效率。结果在该实验中,标记效率随着pH增大而增加,弱碱性(pH7.5)时最佳;随着反应温度的升高,标记效率也随之上升;标记效率还随FITC添加的比例增大而升高。壳聚糖纳米粒子表征和转染效率实验显示最佳的壳聚糖标记条件是反应物壳聚糖与FITC的添加比例为25∶1,在pH7.5、室温25℃条件下反应4h。结论优化的壳聚糖荧光标记方案的标记率比以前文献报道的方法高近3倍,用标记的壳聚糖制备的基因纳米粒子粒径及细胞转染效率与未标记壳聚糖制备的纳米粒子相近,可以达到较好的示踪效果。; 张海玲朱敦皖董霞刘兰霞冷希岗; 关键词：壳聚糖荧光标记

壳聚糖纳米粒子介导TFPI基因转染的实验研究: 2007年; 目的:评价壳聚糖纳米粒子携带组织因子途径抑制因子(tissuefactorpathwayinhibitor,TFPI)基因转染的效率及其细胞毒性。方法:制备壳聚糖纳米粒子-TFPI基因复合物,检测其粒度,zeta电位,包埋效率。以Lipofectamine2000为对照,观察血管平滑肌细胞系A10对壳聚糖TFPI基因纳米复合物的摄入速度和数量;利用逆转录-聚合酶链反应(RT-PCR)检测体外转染效果;应用噻唑蓝(MTT)评价壳聚糖纳米粒子的体外细胞毒性。结果:壳聚糖TFPI基因纳米复合物的平均粒径约为141nm,zeta电位为6.8mV;其DNA包埋效率和DNA含量分别为(98.8±3.4)%和(38.1±2.3)%。A10细胞的摄入和转染实验显示其效率与商品化的细胞转染试剂Lipofectamine2000相近,但是其毒性远低于Lipofectamine2000。结论:壳聚糖纳米粒子可高效携带TFPI基因转染平滑肌细胞,而且对细胞基本无毒性。; 张海玲朱敦皖李大伟冷希岗; 关键词：壳多糖富勒烯转染

Enhancement of transfection efficiency for HeLa cells via incorporating arginine moiety into chitosan被引量：4: 2007年; Arginine-rich peptides have attracted considerable attention due to their distinct internalization mechanism. It was reported that arginine and guanidino moieties were able to translocate through cell membranes and played a critical role in the process of membrane permeation. In this work, arginine was conjugated to the backbone of chitosan to form a novel chitosan derivative, arginine modified chitosan (Arg-CS). Arg-CS/DNA complexes were prepared according to the method of coacervation process. The physicochemical properties of Arg-CS and Arg-CS/DNA complexes were characterized and the transfection activity and efficiency mediated by Arg-CS/DNA complexes were investigated taking HeLa cells as target cells. Arg-CS was characterized by FTIR and 13C NMR. Arg-CS/DNA polye- lectrolyte complexes were investigated by agarose gel retardation, dynamic light scattering (DLS) and atomic force microscopy (AFM). The results revealed that the Arg-CS/DNA complexes started to form at N/P ratio of 2:1, and the size of particles varied from 100 to 180 nm. The cytotoxicity of Arg-CS and their complexes with plasmid DNA were determined by MTT assay for HeLa cells, and the results suggested that Arg-CS/DNA complexes were slightly less toxic than Arg-CS. Moreover, the derivative alone and their complexes showed significantly lower toxicity than PEI and PEI/DNA complexes, respectively. Taking HeLa cells as target cells and using pGL3-control as reporter gene, the luciferase expression mediated by Arg-CS was greatly enhanced to about 100 folds compared with the luciferase expression mediated by chitosan at different pH media. These results suggest that Arg-CS is a promising candi- date as a safe and efficient vector for gene delivery and transfection.; ZHU DunWanZHANG HaiLingBAI JinGenLIU WenGuangLENG XiGangSONG CunXianYANG JianLI XiaoWeiJIN XuSONG LiPingLIU LanXiaLI XiuLanZHANG YangYAO KangDe; 关键词：精氨酸

壳聚糖修饰对细胞摄入和细胞毒性的影响被引量：11: 2006年; 目的研究精氨酸或十六烷基修饰壳聚糖对其细胞摄入和细胞毒性的影响及作用机制。方法用α-^32P-dATP标记质粒DNA，分别与十六烷基化壳聚糖和精氨酸修饰的壳聚糖通过复凝聚方法形成壳聚糖DNA纳米复合物。采用血管平滑肌A10细胞进行摄入测试，并用β液闪计数仪检测结果。用MTT方法对壳聚糖DNA纳米复合物的细胞毒性进行评价。结果经^32P标记的DNA与不同修饰的壳聚糖复合所形成的纳米复合物粒径约为55．9—174．9nm，zeta电位约为1．8—10．8mV。细胞摄入实验显示通过精氨酸或十六烷基修饰的壳聚糖与DNA形成的纳米复合物更易于进入细胞。其中十六烷基化壳聚糖DNA纳米复合物（HCNC）在N／P为1：1时细胞摄入量最高，精氨酸修饰的壳聚糖DNA纳米复合物（ACNC）细胞摄人次之，与未经修饰的壳聚糖DNA纳米复合物（UCNC）相比，差异具有显著性（HCNC、ACNC比UCNC高1．3倍，P〈0．05）。细胞毒性实验显示，修饰后的壳聚糖纳米复合物的毒性远远小于商品化的细胞转染试剂Lipofectamine2000。结论两种修饰对壳聚糖DNA纳米复合物的血管平滑肌细胞摄入有明显促进作用，其作用机制各不相同；同时其细胞毒性远小于商品化的细胞转染试剂Lipofeetamine2000。; 张海玲朱敦皖杨健宋丽萍柏金根姚康德冷希岗; 关键词：壳聚糖化学修饰纳米复合物细胞毒性

壳聚糖修饰对细胞摄入和细胞毒性的影响: 目的将相对分子量50000的壳聚糖分别进行精氨酸和十六烷基修饰,生成壳聚糖衍生物,制备壳聚糖及其衍生物的载基因超微粒子,研究其对细胞摄入和细胞毒性的影响及作用机制。方法用P-dATP 标记质粒 DNA,分别与十六烷基化壳...; 张海玲朱敦皖柏金根冷希岗; 文献传递

壳聚糖基因纳米粒子的细胞摄入和体外毒性研究被引量：8: 2007年; 用分子量为50kDa和400kDa的壳聚糖分别和[α-32P]dATP标记的质粒DNA,在不同的N/P比下,通过复凝聚方法形成基因纳米粒子。对形成的壳聚糖基因纳米粒子(Chitosan gene nanoparticle,CGN)进行表征,评价CGN体外细胞毒性,研究两种壳聚糖形成的基因纳米粒子被A10和K562细胞摄入的量和速度。结果表明:(1)随着壳聚糖分子量和N/P比的增大,形成的基因纳米粒子更易于进入细胞,同时显示纳米粒子的zeta电位与细胞摄入量之间存在关联性;(2)壳聚糖基因纳米粒子的毒性远远小于商品化的细胞转染试剂Lipofectamine2000。; 张海玲王芹宋丽萍岳井银冷希岗; 关键词：质粒壳聚糖基因纳米粒子细胞毒性

Synthesis of N-methylene phosphonic chitosan(NMPCS)and its potential as gene carder被引量：3: 2007年; N-Methylene phosphoulc chitosan (NMPCS),an amphiphilic macromolecule with powerful chelating ability of Ca^(2+) ions,was synthesized and characterized.The physicochemical properties of NMPCS and the interactions between NMPCS and plasmid DNA were investigated by FTIR,^(13)C NMR,X-ray,agarose gel electrophorcsis retardation assay,atomic force microscopy (AFM) and circular dichroism (CD).The results suggest that at charge ratio 2:1 or above,DNA could be completely entrapped and spherical complexes with mean size of 80-210 nm were formed.Taking HeLa as host cell,luciferase expression mediated by NMPCS improved about 100 times compared to the expression mediated by chitosan.; Dun Wan ZhuJin Gen BoHai Ling ZhangWen Guang LiuXi Gang LengCun Xian SongYu Ji YinLi Ping SongLan Xia LiuLin MeiXiu Lan LiYang ZhangKang De Yao

精氨酸修饰壳聚糖提高基因转染效率的研究被引量：7: 2007年; 富精氨酸短肽由于其独特的内在化机理而受到了广泛的关注.研究结果表明,精氨酸和胍基能有效转运穿透细胞膜,在细胞穿膜过程中扮演非常重要的角色.本文将精氨酸接枝到壳聚糖上制备了一种新型的壳聚糖衍生物——精氨酸修饰的壳聚糖(Arg-CS),并用复凝聚的方法制备了Arg-CS/DNA纳米复合物.对Arg-CS及Arg-CS/DNA复合物的物理化学性质进行了表征,并以HeLa细胞为宿主细胞研究了Arg-CS/DNA复合物的转染行为和效率.Arg-CS介导的荧光素酶质粒的表达较壳聚糖介导的荧光素酶的表达提高了大约100倍,而MTT实验表明,Arg-CS及其与DNA复合物在整个实验浓度范围内细胞毒性均很小,Arg-CS有望成为一种高效、安全的壳聚糖基非病毒载体.; 朱敦皖张海玲柏金根刘文广冷希岗宋存先杨健李晓卫金旭宋丽萍刘兰霞李秀兰张杨姚康德; 关键词：壳聚糖非病毒载体

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