Hyslop P A, Morel B, Sauerheber R D
Department of Central Nervous System Pharmacology, Lilly Research Laboratories, Indianapolis, Indiana 46285.
Biochemistry. 1990 Jan 30;29(4):1025-38. doi: 10.1021/bi00456a027.
The molecular organization of sterols in liposomes of 1-palmitoyl-2-oleoyl-sn-glycero-3-phosphocholine (POPC) at 37 degrees C is examined by utilizing the fluorescent analogue of cholesterol cholesta-5,7,9-trien-3 beta-ol (cholestatrienol). (1) Cholestatrienol is shown to be indistinguishable from native cholesterol in terms of its ability to condense POPC, as determined by (i) pressure/area studies of mixed-lipid monolayers and (ii) its ability to increase the order of POPC bilayers (determined by electron spin resonance studies) whether on its own or admixed with cholesterol at various ratios. (2) By analysis of the perturbation of the absorption spectra, cholestatrienol was found to be freely miscible in aggregates of cholesterol in buffer. In contrast, a lack of any detectable direct interaction of the sterol molecules in POPC bilayers was detected. (3) Fluorescence intensity and lifetime measurements of POPC/sterol (1:1 mol/mol) at various cholesterol/cholestratrienol molar ratios (0.5:1 up to 1:1 cholestatrienol/POPC) confirmed that sterol molecules in the membrane matrix were not associated to any great degree. (4) A quantitative estimate of how close sterol molecules approach each other in the membrane matrix was evaluated from the concentration dependence of the steady-state depolarization of fluorescence and was found to be 10.6 A. From geometrical considerations, the sterol/phospholipid phase at 1:1 mol/mol is depicted as each sterol having four POPC molecules as nearest neighbors. We term this arrangement of the lipid matrix an "ordered bimolecular mesomorphic lattice". (5) The concentration dependence of depolarization of fluorescence of cholestatrienol in POPC liposomes in the absence of cholesterol yielded results that were consistent with the cholestatrienol molecules being homogeneously dispersed throughout the phospholipid phase at sterol/POPC ratios of less than 1:1. (6) From qualitative calculations of the van der Walls' hydrophobic interactions of the lipid species, the phospholipid condensing effect of cholesterol is postulated to arise from increased interpenetration of the flexible methylene segments of the acyl chains, as a direct result of their greater mutual attraction compared to their attraction for neighboring sterol molecules. (7) The interdependence of the ordered bimolecular mesomorphic lattice and the acyl chain condensation is discussed in an effort to understand the ability of cholesterol to modulate the physical and mechanical properties of biological membranes.
利用胆固醇的荧光类似物胆甾-5,7,9-三烯-3β-醇(胆甾三烯醇),研究了1-棕榈酰-2-油酰基-sn-甘油-3-磷酸胆碱(POPC)脂质体中甾醇在37℃时的分子组织。(1)通过以下方法确定,胆甾三烯醇在凝聚POPC的能力方面与天然胆固醇没有区别:(i)混合脂质单层的压力/面积研究,以及(ii)其增加POPC双层有序性的能力(通过电子自旋共振研究确定),无论是其自身还是与胆固醇以各种比例混合时。(2)通过对吸收光谱扰动的分析,发现胆甾三烯醇在缓冲液中能与胆固醇聚集体自由混溶。相反,在POPC双层中未检测到甾醇分子之间有任何可检测到的直接相互作用。(3)在各种胆固醇/胆甾三烯醇摩尔比(0.5:1至1:1胆甾三烯醇/POPC)下,对POPC/甾醇(1:1摩尔/摩尔)的荧光强度和寿命测量证实,膜基质中的甾醇分子在很大程度上没有相互缔合。(4)根据荧光稳态去极化的浓度依赖性,对膜基质中甾醇分子彼此接近的程度进行了定量估计,结果为10.6埃。从几何角度考虑,1:1摩尔/摩尔时的甾醇/磷脂相被描述为每个甾醇有四个POPC分子作为最近邻。我们将这种脂质基质的排列称为“有序双分子介晶晶格”。(5)在不存在胆固醇的情况下,对POPC脂质体中胆甾三烯醇荧光去极化的浓度依赖性进行的研究结果表明,在甾醇/POPC比例小于1:1时,胆甾三烯醇分子均匀分散在整个磷脂相中。(6)通过对脂质种类范德华疏水相互作用的定性计算,推测胆固醇的磷脂凝聚作用源于酰基链柔性亚甲基段相互渗透的增加,这是由于它们彼此之间的吸引力大于它们对相邻甾醇分子的吸引力的直接结果。(7)讨论了有序双分子介晶晶格与酰基链凝聚的相互依赖性,以试图理解胆固醇调节生物膜物理和机械性质的能力。
