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双重不对称离心法(DAC)——一种制备脂质体的新技术。

Dual asymmetric centrifugation (DAC)--a new technique for liposome preparation.

作者信息

Massing Ulrich, Cicko Sanja, Ziroli Vittorio

机构信息

Tumor Biology Center, Department of Clinical Research, Breisacher Strasse 117, D-79106 Freiburg, Germany.

出版信息

J Control Release. 2008 Jan 4;125(1):16-24. doi: 10.1016/j.jconrel.2007.09.010. Epub 2007 Oct 10.

Abstract

This is the first report on the use of a "dual asymmetric centrifuge (DAC)" for preparing liposomes. DAC differs from conventional centrifugation by an additional rotation of the sample around its own vertical axis: While the conventional centrifugation constantly pushes the sample material outwards, this additional rotation constantly forces the sample material towards the center of the centrifuge. This unique combination of two contra rotating movements results in shear forces and thus, in efficient homogenization. We demonstrated that it is possible to prepare liposomes by DAC, by homogenizing a rather concentrated blend of hydrogenated phosphatidylcholine and cholesterol (55:45 mol%) and 0.9% NaCl-solution, which results in a viscous vesicular phospholipid gel (VPG). The resulting VPG can subsequently be diluted to a conventional liposome dispersion. Since DAC is intended to make sterile preparations of liposomes, or to entrap toxic/radioactive compounds, the process was performed within a sealed vial. It could be shown that the DAC speed, the lipid concentration, the homogenization time and the addition of a mixing aid (glass beads) are all critical for the size of the liposomes. Optimized conditions resulted in liposomes of 60+/-5 nm and a trapping efficacy of 56+/-3.3% for the model compound calcein.

摘要

这是关于使用“双不对称离心机(DAC)”制备脂质体的首份报告。DAC与传统离心法的不同之处在于,样品会绕自身垂直轴进行额外旋转:传统离心法会持续将样品物质向外推,而这种额外旋转会持续迫使样品物质朝向离心机中心。这两种反向旋转运动的独特组合会产生剪切力,从而实现高效均质化。我们证明了通过DAC制备脂质体是可行的,方法是将氢化磷脂酰胆碱和胆固醇(55:45摩尔%)与0.9%氯化钠溶液的相当浓缩的混合物进行均质化,这会形成粘性囊泡磷脂凝胶(VPG)。随后可将所得的VPG稀释成常规脂质体分散液。由于DAC旨在制备脂质体的无菌制剂,或包封有毒/放射性化合物,该过程在密封小瓶内进行。结果表明,DAC速度、脂质浓度、均质化时间以及添加混合助剂(玻璃珠)对脂质体大小均至关重要。优化条件下得到的脂质体大小为60±5纳米,模型化合物钙黄绿素的包封率为56±3.3%。

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