Lu J Z, Hao Y H, Chen J W
National Laboratory of Biomacromolecules, Institute of Biophysics, Academia Sinica, Beijing 100101, China.
J Biochem. 2001 Jun;129(6):891-8. doi: 10.1093/oxfordjournals.jbchem.a002934.
We previously reported that 1,2-dipalmitoyl-sn-glycero-3-phosphocholine (DPPC) forms an interdigitated gel phase in the presence of 1-palmitoyl-sn-glycero-3-phosphocholine (16:0LPC) at concentrations below 30 mol%. In the present investigation, fluorescent probe 1,6-diphenyl-1,3,5-hexatriene (DPH), X-ray diffraction, and differential scanning calorimetry (DSC) were used to investigate the effect of cholesterol on the phase behavior of 16:0LPC/DPPC binary mixtures. At 25 degrees C, 30 mol% 16:0LPC significantly decreases the DPH fluorescence intensity during the transition of DPPC from the L(beta') phase to the L(betaI) phase. However, the addition of cholesterol to 16:0LPC/DPPC mixtures results in a substantial increase in fluorescence intensity. The changes in DPH fluorescence intensity reflect the probe's redistribution from an orientation parallel to the acyl chain to the center of the bilayer, suggesting a bilayer structure transition from interdigitation to noninterdigitation. The normal repeat period of small angle X-ray diffraction patterns can be restored and a reflection appears at 0.42 nm with a broad shoulder around 0.41 nm in wide angle X-ray diffraction patterns when 10 mol% cholesterol is incorporated into 30 mol% 16:0LPC/DPPC vesicles, indicating that the mixtures are in the gel phase (L(beta')). Moreover, DSC results demonstrate that 10 mol% cholesterol is sufficient to significantly decrease the main enthalpy, cooperativity and lipid chain melting of 30 mol% 16:0LPC/DPPC binary mixtures, which are L(betaI), indicating that the transition of the interdigitated phase is more sensitive to cholesterol than that of the noninterdigitated phase. Our data imply that the interdigitated gel phase induced by 16:0LPC is prevented in the presence of 10 mol% cholesterol, but unlike ethanol, an increasing concentration of 16:0LPC is not able to restore the interdigitation structure of the lipid mixtures.
我们之前报道过,在浓度低于30 mol%的1-棕榈酰-sn-甘油-3-磷酸胆碱(16:0LPC)存在下,1,2-二棕榈酰-sn-甘油-3-磷酸胆碱(DPPC)形成一种相互交错的凝胶相。在本研究中,使用荧光探针1,6-二苯基-1,3,5-己三烯(DPH)、X射线衍射和差示扫描量热法(DSC)来研究胆固醇对16:0LPC/DPPC二元混合物相行为的影响。在25摄氏度时,30 mol%的16:0LPC在DPPC从L(β')相转变为L(βI)相的过程中显著降低DPH荧光强度。然而,向16:0LPC/DPPC混合物中添加胆固醇会导致荧光强度大幅增加。DPH荧光强度的变化反映了探针从与酰基链平行的取向重新分布到双层中心,表明双层结构从相互交错转变为非相互交错。当将10 mol%的胆固醇加入到30 mol%的16:0LPC/DPPC囊泡中时,小角X射线衍射图谱的正常重复周期可以恢复,并且在广角X射线衍射图谱中在0.42 nm处出现一个反射峰,在0.41 nm附近有一个宽肩峰,这表明混合物处于凝胶相(L(β'))。此外,DSC结果表明,10 mol%的胆固醇足以显著降低30 mol%的16:0LPC/DPPC二元混合物(即L(βI))的主要焓、协同性和脂质链熔化,这表明相互交错相的转变比非相互交错相对胆固醇更敏感。我们的数据表明在存在10 mol%胆固醇的情况下,由16:0LPC诱导的相互交错凝胶相被阻止,但与乙醇不同,增加16:0LPC的浓度并不能恢复脂质混合物的相互交错结构。
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