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组氨酸化脂质修饰的仙台病毒包膜介导增强的膜融合并增强靶向基因递送。

Histidylated lipid-modified Sendai viral envelopes mediate enhanced membrane fusion and potentiate targeted gene delivery.

作者信息

Verma Santosh K, Mani Prashant, Sharma Nishi Raj, Krishnan Anuja, Kumar Valluripalli Vinod, Reddy Bathula Surendar, Chaudhuri Arabinda, Roy Rajendra P, Sarkar Debi P

机构信息

Department of Biochemistry, University of Delhi South Campus, Benito Juarez Road, New Delhi 110021, USA.

出版信息

J Biol Chem. 2005 Oct 21;280(42):35399-409. doi: 10.1074/jbc.M506615200. Epub 2005 Aug 5.

DOI:10.1074/jbc.M506615200
PMID:16085643
Abstract

Recent studies have demonstrated that covalent grafting of a single histidine residue into a twin-chain aliphatic hydrocarbon compound enhances its endosome-disrupting properties and thereby generates an excellent DNA transfection system. Significant increase in gene delivery efficiencies has thus been obtained by using endosome-disrupting multiple histidine functionalities in the molecular architecture of various cationic polymers. To take advantage of this unique feature, we have incorporated L-histidine (N,N-di-n-hexadecylamine) ethylamide (L(H)) in the membrane of hepatocyte-specific Sendai virosomes containing only the fusion protein (F-virosomes (Process for Producing a Targeted Gene (Sarkar, D. P., Ramani, K., Bora, R. S., Kumar, M., and Tyagi, S. K. (November 4, 1997) U. S. Patent 5,683,866))). Such L(H)-modified virosomal envelopes were four times more (p < 0.001) active in terms of fusion with its target cell membrane. On the other hand, the presence of L(H) in reconstituted influenza and vesicular stomatitis virus envelopes failed to enhance spike glycoprotein-induced membrane fusion with host cell membrane. Circular dichroism and limited proteolysis experiments with F-virosomes indicated that the presence of L(H) leads to conformational changes in the F protein. The molecular mechanism associated with the increased membrane fusion induced by L(H) has been addressed in the light of fusion-competent conformational change in F protein. Such enhancement of fusion resulted in a highly efficient gene delivery system specific for liver cells in culture and in whole animals.

摘要

最近的研究表明,将单个组氨酸残基共价接枝到双链脂肪烃化合物中可增强其破坏内体的特性,从而产生优异的DNA转染系统。因此,通过在各种阳离子聚合物的分子结构中使用破坏内体的多个组氨酸功能,基因传递效率得到了显著提高。为了利用这一独特特性,我们将L-组氨酸(N,N-二正十六烷基胺)乙酰胺(L(H))掺入仅含有融合蛋白的肝细胞特异性仙台病毒体膜中(F-病毒体(生产靶向基因的方法(萨卡尔,D.P.,拉马尼,K.,博拉,R.S.,库马尔,M.,和蒂亚吉,S.K.(1997年11月4日)美国专利5,683,866)))。这种L(H)修饰的病毒体包膜在与其靶细胞膜融合方面的活性提高了四倍(p<0.001)。另一方面,在重组流感病毒和水疱性口炎病毒包膜中存在L(H)未能增强刺突糖蛋白诱导的与宿主细胞膜的融合。对F-病毒体进行的圆二色性和有限蛋白酶解实验表明,L(H)的存在导致F蛋白发生构象变化。根据F蛋白中具有融合能力的构象变化,探讨了与L(H)诱导的膜融合增加相关的分子机制。这种融合增强导致了一种针对培养细胞和整个动物肝脏细胞的高效基因传递系统。

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