Lipid loss and compositional change during preparation of simple two-component liposomes.

IF 2.4 Q3 BIOPHYSICS Biophysical reports Pub Date : 2024-09-11 Epub Date: 2024-08-21 DOI:10.1016/j.bpr.2024.100174
Eunice Kim, Olivia Graceffa, Rachel Broweleit, Ali Ladha, Andrew Boies, Sanyukta Prakash Mudakannavar, Robert J Rawle
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Abstract

Liposomes are used as model membranes in many scientific fields. Various methods exist to prepare liposomes, but common procedures include thin-film hydration followed by extrusion, freeze-thaw, and/or sonication. These procedures can produce liposomes at specific concentrations and lipid compositions, and researchers often assume that the concentration and composition of their liposomes are similar or identical to what would be expected if no lipid loss occurred. However, lipid loss and concomitant biasing of lipid composition can in principle occur at any preparation step due to nonideal mixing, lipid-surface interactions, etc. Here, we report a straightforward HPLC-ELSD method to quantify the lipid concentration and composition of liposomes and apply that method to study the preparation of simple cholesterol/POPC liposomes. We examine common liposome preparation steps, including vortexing during resuspension, lipid film hydration, extrusion, freeze-thaw, and sonication. We found that the resuspension step can play an outsized role in determining the lipid loss (up to ∼50% under seemingly rigorous procedures). The extrusion step yielded smaller lipid losses (∼10-20%). Freeze-thaw and sonication could both be employed to improve lipid yields. Hydration times up to 60 min and increasing cholesterol concentrations up to 50 mol % had little influence on lipid recovery. Fortunately, even conditions with large lipid loss did not substantially influence the target membrane composition, as long as the lipid mixture was below the cholesterol solubility limit. From our results, we identify best practices for producing maximum levels of lipid recovery and minimal changes to lipid composition during liposome preparation for cholesterol/POPC liposomes.

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制备简单双组分脂质体过程中的脂质损失和成分变化。
脂质体在许多科学领域被用作模型膜。制备脂质体的方法多种多样,但常见的程序包括薄膜水合后挤压、冻融和/或超声处理。这些程序可以制备出特定浓度和脂质成分的脂质体,研究人员通常会假设其脂质体的浓度和成分与不发生脂质损失时的预期相似或相同。然而,由于非理想混合、脂质表面相互作用等原因,脂质损失和随之而来的脂质成分偏差原则上可能发生在任何制备步骤中。在此,我们报告了一种直接的 HPLC-ELSD 方法来量化脂质体的脂质浓度和组成,并将该方法用于研究简单胆固醇/POPC 脂质体的制备。我们研究了常见的脂质体制备步骤,包括再悬浮过程中的涡旋、脂膜水合、挤压、冻融和超声。我们发现,再悬浮步骤在决定脂质损失方面起着非常重要的作用(在看似严格的程序下可高达 50%)。挤压步骤产生的脂质损失较小(10%-20%)。冻融和超声都可以提高脂质的产量。水合时间最长为 60 分钟,胆固醇浓度最高为 50 摩尔%,但这对脂质回收率影响不大。幸运的是,只要脂质混合物低于胆固醇溶解极限,即使在脂质大量流失的条件下,也不会对目标膜组成产生重大影响。根据我们的研究结果,我们确定了在胆固醇/POPC 脂质体的脂质体制备过程中实现最高水平的脂质回收和最小程度的脂质成分变化的最佳方法。
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来源期刊
Biophysical reports
Biophysical reports Biophysics
CiteScore
2.40
自引率
0.00%
发文量
0
审稿时长
75 days
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