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神经节苷脂 GM1 在聚酰胺-胺树枝状高分子细胞内化机制中的作用。

The role of ganglioside GM1 in cellular internalization mechanisms of poly(amidoamine) dendrimers.

机构信息

Program in Macromolecular Science and Engineering and Biophysics, University of Michigan, Ann Arbor, Michigan 48109-1055, USA.

出版信息

Bioconjug Chem. 2009 Aug 19;20(8):1503-13. doi: 10.1021/bc900029k. Epub 2009 Jul 7.

Abstract

Generation 7 (G7) poly(amidoamine) (PAMAM) dendrimers with amine, acetamide, and carboxylate end groups were prepared to investigate polymer/cell membrane interactions in vitro. G7 PAMAM dendrimers were used in this study because higher-generation of dendrimers are more effective in permeabilization of cell plasma membranes and in the formation of nanoscale holes in supported lipid bilayers than smaller, lower-generation dendrimers. Dendrimer-based conjugates were characterized by (1)H NMR, UV/vis spectroscopy, GPC, HPLC, and CE. Positively charged amine-terminated G7 dendrimers (G7-NH(2)) were observed to internalize into KB, Rat2, and C6 cells at a 200 nM concentration. By way of contrast, neither negatively charged G7 carboxylate-terminated dendrimers (G7-COOH) nor neutral acetamide-terminated G7 dendrimers (G7-Ac) associated with the cell plasma membrane or internalized under similar conditions. A series of in vitro experiments employing endocytic markers cholera toxin subunit B (CTB), transferrin, and GM(1)-pyrene were performed to further investigate mechanisms of dendrimer internalization into cells. G7-NH(2) dendrimers colocalized with CTB; however, experiments with C6 cells indicated that internalization of G7-NH(2) was not ganglioside GM(1) dependent. The G7/CTB colocalization was thus ascribed to an artifact of direct interaction between the two species. The presence of GM(1) in the membrane also had no effect upon XTT assays of cell viability or lactate dehydrogenase (LDH) assays of membrane permeability.

摘要

制备了第七代(G7)聚酰胺-胺(PAMAM)树枝状聚合物,其末端基团分别为胺基、乙酰胺基和羧基,以研究体外聚合物/细胞膜相互作用。在这项研究中使用了第七代 G7 PAMAM 树枝状聚合物,因为与较小的、较低代的树枝状聚合物相比,更高代的树枝状聚合物更有效地使细胞质膜穿孔,并在支撑的脂质双层中形成纳米级孔。树枝状聚合物缀合物通过(1)H NMR、UV/vis 光谱、GPC、HPLC 和 CE 进行了表征。观察到带正电荷的胺端基 G7 树枝状聚合物(G7-NH2)在 200 nM 浓度下可内化到 KB、Rat2 和 C6 细胞中。相比之下,带负电荷的 G7 羧基端基树枝状聚合物(G7-COOH)和中性乙酰胺端基 G7 树枝状聚合物(G7-Ac)既不与细胞质膜结合也不内化。进行了一系列体外实验,使用内吞标记霍乱毒素亚单位 B(CTB)、转铁蛋白和 GM1-芘,以进一步研究树枝状聚合物内化到细胞中的机制。G7-NH2 树枝状聚合物与 CTB 共定位;然而,与 C6 细胞的实验表明,G7-NH2 的内化不依赖于神经节苷脂 GM1。因此,G7/CTB 共定位归因于两种物质之间直接相互作用的假象。GM1 存在于膜中也不会影响细胞活力的 XTT 测定或膜通透性的乳酸脱氢酶(LDH)测定。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/d13d/4641442/af887daafff0/nihms735137f1.jpg

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