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无唾液酸胎球蛋白修饰脂质体在小鼠体内的肝实质细胞靶向性研究 被引量:4
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作者 王黎 舒桂明 +2 位作者 王向涛 李沙 侯新朴 《北京大学学报(医学版)》 CAS CSCD 北大核心 2001年第3期251-254,共4页
目的 :研究经无唾液酸胎球蛋白 (asialofetuin ,AF)修饰后 ,脂质体达到小鼠肝实质细胞靶向的可能性。方法 :用放射性同位素标记的方法测定普通长循环脂质体 (stericallystabilizedliposomes,SSL)、AF 修饰普通脂质体(AF linkednormallip... 目的 :研究经无唾液酸胎球蛋白 (asialofetuin ,AF)修饰后 ,脂质体达到小鼠肝实质细胞靶向的可能性。方法 :用放射性同位素标记的方法测定普通长循环脂质体 (stericallystabilizedliposomes,SSL)、AF 修饰普通脂质体(AF linkednormalliposomes,AF NL)及AF 修饰长循环脂质体 (AF linkedstericallystabilizedliposomes,AF SSL)在小鼠血、心、肝、脾、肺、肾等各器官及肝内不同细胞中的分布。结果 :SSL、AF NL及AF SSL的血中半衰期分别为14.44、4.73、11.49h ;整个肝中的分布AF NL >AF SSL >SSL ,经t化极差 q法检验 ,三者之间差异均存在显著性 ;肝不同细胞 (即实质与非实质细胞 )中脂质体的浓度均为AF NL >AF SSL >SSL(P <0 .0 5 ) ,但实质细胞与非实质细胞的浓度比为AF NL≈AF SSL SSL(P <0 .0 5 )。结论 :经AF修饰后 ,无论是否长循环 。 展开更多
关键词 细胞靶向性 无唾液酸胎球蛋白 脂质体 代谢 肝代谢
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FITC标记无唾液酸胎球蛋白对人精子去唾液酸糖蛋白受体的定位
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作者 孙平楠 周小玲 +3 位作者 黄天华 谢庆东 陈惠芳 康祥锦 《癌变.畸变.突变》 CAS CSCD 2009年第2期132-134,共3页
背景与目的:采用FITC标记的无唾液酸胎球蛋白(FITC-ASF)对人精子去唾液酸糖蛋白受体(ASGP-R)进行定位和监测。材料与方法:采用FITC标记ASGP-R天然配体无唾液酸胎球蛋白得到FITC-ASF,进一步使用FITC-ASF对人精子表面ASGP-R标记,通过免疫... 背景与目的:采用FITC标记的无唾液酸胎球蛋白(FITC-ASF)对人精子去唾液酸糖蛋白受体(ASGP-R)进行定位和监测。材料与方法:采用FITC标记ASGP-R天然配体无唾液酸胎球蛋白得到FITC-ASF,进一步使用FITC-ASF对人精子表面ASGP-R标记,通过免疫荧光和流式细胞术检测其应用于外源ASF蛋白与该受体结合情况。结果:FITC-ASF能够较好的标记人精子表面ASGP-R,并成功应用于外源蛋白与该受体的结合。结论:本研究为获得一种适合临床广泛应用的新的简便易行的ASGP-R监测方法提供了实验基础。 展开更多
关键词 无唾液酸胎球蛋白 异硫氰酸荧光素 人精子 去唾液酸糖蛋白受体 定位
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Study on Hepatocyte-targeted Liposomes
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作者 For Ph. D. Degree: Wang Li Supervisor: Hou Xinpu Department of Pharmacy, School of Pharmaceutical Science, Peking University, Beijing 100083 《Journal of Chinese Pharmaceutical Sciences》 CAS 2001年第3期168-168,共1页
关键词 HEPATOCYTE Cell targeted Liposomes Asialoglyprotein receptor asialofetuin ADRIAMYCIN
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Isolation, purification and characterization of an N-acetyl-D-lactosamine binding mitogenic and anti-proliferative lectin from tubers of a cobra lily Arisaema utile Schott
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作者 Vikram Dhuna Kshitija Dhuna +3 位作者 Jatinder Singh Ajit Kumar Saxena Satyam Kumar Agrawal Sukhdev Singh Kamboj 《Advances in Bioscience and Biotechnology》 2010年第2期79-90,共12页
Lectins are the carbohydrate-binding proteins of non-immune origin which have been the subject of intense investigation over the last few decades owing to the variety of interesting biological properties. Most of the ... Lectins are the carbohydrate-binding proteins of non-immune origin which have been the subject of intense investigation over the last few decades owing to the variety of interesting biological properties. Most of the lectins which have been purified and characterized from plants have been obtained from dicotyledons. In the present study a lectin was purified from tubers of a monocot plant Arisaema utile (AUL) Schott by affinity chromatography on asialofetuin-linked amino activated silica beads. AUL gave a single band in SDS-PAGE at pH 8.3 corresponding to subunit Mr 13.5 kDa. The native molecular mass of AUL was 54 kDa suggesting a homotetrameric structure. AUL gave multiple bands in isoelectric focusing and in native PAGE at pH 8.3. AUL was inhibited by N-acetyl-D-lactosamine (Lac NAc), a disaccharide and asialofetuin, a complex desialylated serum glycoprotein. When treated with denaturing agents, the lectin was stable in the presence of urea (3 M), thiourea (4 M) and guanidine HCl (4 M). AUL was a glycoprotein with a carbohydrate content of 1.2%. Complete loss of activity was observed upon modification of tryptophan residues of the lectin. The activity was reduced to 25% after modification of tyrosine. Chemical modification of arginine, histidine, serine and cysteine residues of AUL did not affect its activity. Using Far UV CD spectra the estimated secondary structure was 37% α-helix, 25% β-sheet and 38% random contributions. The lectin showed potent mitogenic response towards human lymphocytes. In vitro anti-proliferative assay using 11 human cancer cell lines resulted in 50% inhibition of six cell lines viz. SW-620, HCT-15, SK-N-SH, IMR-32, Colo-205 and HT-29 at 38, 42, 43, 49, 50 and 89 &amp;#181;g/ml, respectively. 展开更多
关键词 N-acetyl-D-lactosamine ARISAEMA Utile Affinity Purification ANTI-PROLIFERATIVE asialofetuin Chemical Modification LECTIN Mitogenicity
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