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Phospholipid order in gel- and fluid-phase cell-size liposomes measured by digitized video fluorescence polarization microscopy.

机译:通过数字化视频荧光偏振显微镜测量的凝胶和液相细胞大小脂质体中的磷脂顺序。

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摘要

Low-light digitized video fluorescence microscopy has been utilized to measure the steady-state polarized fluorescence from the membrane probe diphenylhexatriene (DPH) and its cationic and phosphatidylcholine derivatives 1-(4-trimethylammoniumphenyl)-6-phenyl-1,3,5-hexatriene (TMA-DPH) and 2-[3-(diphenylhexatrienyl)propanoyl]-3-palmitoyl-L-alpha-phosphati dylcholine (DPH-PC), respectively, in cell-size (10-70 microns) unilamellar vesicles composed of gel-or fluid-phase phospholipid. Using an inverted microscope with epi-illumination optics and an intensified silicon intensified target camera interfaced to a minicomputer, fluorescence images of single vesicles were obtained at emission polarizer orientations of 0 degrees, 45 degrees, 90 degrees, and 135 degrees relative to the excitation light polarization direction. Fluorescence intensity ratios F90 degrees/F0 degrees (= F perpendicular/F parallel) and F135 degrees/F45 degrees were calculated on a pixel-by-pixel basis from digitized image pairs. Theoretical expressions were derived for collected polarized fluorescence as a function of position on the membrane surface as well as the degree of lipid order, in terms of the fluorophore's maximum angular motional freedom in the bilayer (identical to theta max), using a modification of the method of D. Axelrod (1979. Biophys. J. 26:557-574) together with the "wobbling-in-a-cone" model of probe rotational diffusion. Comparison of experimental polarization ratios with theoretical ratios yielded the following results. In gel-phase dipalmitoyl-phosphatidylcholine, the data for all three probes correspond to a model in which the cone angle theta max = 17 +/- 2 degrees and there exists a collective tilt of the phospholipid acyl chains of 30 degrees relative to the bilayer normal. In addition, approximately 5% of DPH and TMA-DPH molecules are aligned parallel to the plane of the bilayer. In fluid-phase palmitoyloleoyl-phosphatidylcholine, the data are well fit by models in which theta max = 60 +/- 2 degrees for DPH and DPH-PC and 32 +/- 4 degrees for TMA-DPH, with approximately 20% of DPH molecules and 10% of TMA-DPH molecules aligned parallel to the bilayer plane, and a net phospholipid tilt at or near the headgroup region of approximately 30 degrees. The results demonstrate that lipid order can be measured with a spatial resolution of approximately 1 micron2 in cell-size vesicles even with high aperture observation through a microscope.
机译:低光数字化视频荧光显微镜已用于测量膜探针二苯基己三烯(DPH)及其阳离子和磷脂酰胆碱衍生物1-(4-三甲基铵苯基)-6-苯基-1,3,5-的稳态偏振荧光六三烯(TMA-DPH)和2- [3-(二苯基六三烯基)丙酰基] -3-棕榈酰-L-α-磷脂酰胆碱(DPH-PC),分别由细胞大小(10-70微米)的单层囊泡组成,凝胶或液相磷脂。使用带有落射照明光学系统的倒置显微镜和与微型计算机连接的增强硅增强目标相机,可以在相对于激发光的0度,45度,90度和135度的发射偏振器方向上获得单囊泡的荧光图像。极化方向。从数字化图像对逐像素计算荧光强度比F90度/ F0度(= F垂直/ F平行)和F135度/ F45度。根据荧光团在双层中的最大角运动自由度(与theta max相同),推导出收集的极化荧光与膜表面位置和脂质有序度的关系的理论表达式。 D.Axelrod(1979. Biophys。J. 26:557-574)的方法以及探针旋转扩散的“圆锥中摇动”模型。实验极化比与理论比的比较产生以下结果。在凝胶相二棕榈酰磷脂酰胆碱中,所有三个探针的数据均对应于一个模型,其中锥角θmax = 17 +/- 2度,并且磷脂酰基链相对于双层的集体倾斜度为30度正常。此外,大约5%的DPH和TMA-DPH分子与双层平面平行排列。在液相棕榈酰油酰-磷脂酰胆碱中,模型拟合的数据很好,其中DPH和DPH-PC的theta max = 60 +/- 2度,而TMA-DPH的theta max = 32 +/- 4度,其中DPH约为20%分子和10%的TMA-DPH分子平行于双层平面排列,并且净磷脂在大约30度的头基区域或附近倾斜。结果表明,即使通过显微镜进行高光圈观察,也可以在细胞大小的囊泡中以约1 micron2的空间分辨率测量脂质顺序。

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