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椭偏测量法、激光扫描显微镜和Z扫描荧光相关光谱法相结合,阐明隐孢子虫防御素-4与支持的磷脂双层之间的相互作用。

Combination of ellipsometry, laser scanning microscopy and Z-scan fluorescence correlation spectroscopy elucidating interaction of cryptdin-4 with supported phospholipid bilayers.

作者信息

Miszta Adam, Machán Radek, Benda Ales, Ouellette Andre J, Hermens Wim Th, Hof Martin

机构信息

J. Heyrovský Institute of Physical Chemistry v.v.i., Academy of Sciences of the Czech Republic, Czech Republic.

出版信息

J Pept Sci. 2008 Apr;14(4):503-9. doi: 10.1002/psc.938.

Abstract

The present study has two main objectives. The first is to characterize antimicrobial peptide (AMP) cryptdin-4 (Crp-4) interactions with biological membranes and to compare those interactions with those of magainin 2. The second is to combine the complementary experimental approaches of laser scanning microscopy (LSM), ellipsometry, and Z-scan fluorescence correlation spectroscopy (FCS) to acquire comprehensive information on mechanisms of AMP interactions with supported phospholipid bilayers (SPBs)-a popular model of biological membranes. LSM shows appearance of inhomogeneities in spatial distribution of lipids in the bilayer after treatment with Crp-4. Ellipsometric measurements show that binding of Crp-4 does not significantly change the lipid structure of the bilayer (increase in adsorbed mass without a change in thickness of adsorbed layer). Furthermore, Crp-4 slows the lateral diffusion of lipids within the membrane as shown by Z-scan FCS. All changes of the bilayer induced by Crp-4 can be partially reversed by flushing the sample with excess of buffer. Bilayer interactions of magainin 2 are significantly different, causing large loss of lipids and extensive damage to the bilayer. It seems likely that differences in peptide mode of action, readily distinguished using these combined experimental methods, are related to the distinctive beta-sheet and alpha-helical structures of the respective peptides.

摘要

本研究有两个主要目标。第一个目标是表征抗菌肽(AMP)隐窝蛋白-4(Crp-4)与生物膜的相互作用,并将这些相互作用与蛙皮素2的相互作用进行比较。第二个目标是结合激光扫描显微镜(LSM)、椭偏仪和Z扫描荧光相关光谱(FCS)等互补的实验方法,以获取关于AMP与支持的磷脂双层(SPB,一种常用的生物膜模型)相互作用机制的全面信息。LSM显示,用Crp-4处理后,双层膜中脂质的空间分布出现不均匀性。椭偏测量表明,Crp-4的结合不会显著改变双层膜的脂质结构(吸附质量增加,而吸附层厚度不变)。此外,如Z扫描FCS所示,Crp-4减缓了膜内脂质的横向扩散。用过量缓冲液冲洗样品可部分逆转Crp-4引起的双层膜的所有变化。蛙皮素2的双层膜相互作用显著不同,导致脂质大量损失和双层膜广泛受损。使用这些组合实验方法很容易区分的肽作用模式差异,似乎与各肽独特的β折叠和α螺旋结构有关。

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