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蛋白质对脂质双层中荧光团寿命异质性的影响。

Effect of proteins on fluorophore lifetime heterogeneity in lipid bilayers.

作者信息

Williams B W, Scotto A W, Stubbs C D

机构信息

Department of Pathology and Cell Biology, Thomas Jefferson University, Philadelphia, Pennsylvania 19107.

出版信息

Biochemistry. 1990 Apr 3;29(13):3248-55. doi: 10.1021/bi00465a016.

Abstract

The effect of three different membrane proteins on the fluorescence lifetime heterogeneity of 1,6-diphenyl-1,3,5-hexatriene (DPH) in phospholipid vesicle systems was investigated. For large unilamellar vesicles of dimyristoylphosphatidylcholine (DMPC) and 1-palmitoyl-2-oleoylphosphatidylcholine (POPC) at 37 degrees C, the fluorescence decay was essentially monoexponential (8.6 and 8.2 ns, respectively) except for a minor component typical of DPH. For gramicidin D reconstituted into DMPC vesicles at a protein/lipid molar ratio of 1/7, the most appropriate analysis of the data was found to be in the form of a bimodal Lorentzian distribution. Centers of the major lifetime components were almost identical with those recovered for vesicles without proteins, while broad distributional widths of some 4.0 ns were recovered. Variation of the protein/lipid molar ratio in sonicated POPC vesicles revealed an abrupt increase in distributional width at ratios approximating 1/15-1/20, which leveled off at about 2.5 ns. For bacteriorhodopsin in DMPC vesicles and cytochrome b5 in POPC, the most appropriate analysis of the data was again found to be in the form of a bimodal Lorentzian also with broad distributional widths in the major component. Lifetime centers were decreased for these proteins due to fluorescence energy transfer to the retinal of the bacteriorhodopsin and heme of the cytochrome b5. Fluorescence energy transfer is distance dependent, and since a range of donor-acceptor distances would be expected in a membrane, lifetime distributions should therefore be recovered independently of other effects for proteins possessing acceptor chromophores.(ABSTRACT TRUNCATED AT 250 WORDS)

摘要

研究了三种不同膜蛋白对磷脂囊泡系统中1,6 - 二苯基 - 1,3,5 - 己三烯(DPH)荧光寿命异质性的影响。对于37℃下的二肉豆蔻酰磷脂酰胆碱(DMPC)和1 - 棕榈酰 - 2 - 油酰磷脂酰胆碱(POPC)的大单层囊泡,除了DPH典型的次要成分外,荧光衰减基本上是单指数的(分别为8.6和8.2纳秒)。对于以蛋白质/脂质摩尔比1/7重构到DMPC囊泡中的短杆菌肽D,发现对数据最合适的分析形式是双峰洛伦兹分布。主要寿命成分的中心与未含蛋白质的囊泡所测得的几乎相同,而恢复得到约4.0纳秒的宽分布宽度。超声处理的POPC囊泡中蛋白质/脂质摩尔比的变化表明,在接近1/15 - 1/20的比例时分布宽度突然增加,在约2.5纳秒时趋于平稳。对于DMPC囊泡中的细菌视紫红质和POPC中的细胞色素b5,再次发现对数据最合适的分析形式也是双峰洛伦兹分布,主要成分也有宽分布宽度。由于荧光能量转移到细菌视紫红质的视黄醛和细胞色素b5的血红素上,这些蛋白质的寿命中心降低。荧光能量转移是距离依赖性的,并且由于在膜中预期存在一系列供体 - 受体距离,因此对于具有受体发色团的蛋白质,寿命分布应独立于其他效应而恢复。(摘要截短于250字)

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