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“δpH”探针9-氨基吖啶:响应时间、结合行为及在膜上的二聚化

The 'delta pH'-probe 9-aminoacridine: response time, binding behaviour and dimerization at the membrane.

作者信息

Grzesiek S, Dencher N A

机构信息

Department of Physics, Freie Universität Berlin, Germany.

出版信息

Biochim Biophys Acta. 1988 Mar 3;938(3):411-24. doi: 10.1016/0005-2736(88)90139-3.

Abstract

The fluorescence quenching of 9-aminoacridine (9-AA) after imposition of a transmembrane pH gradient (inside acidic) in liposomes has been investigated for a number of different lipid systems. The initial fluorescence decrease after a rapid pH jump, induced in the extravesicular medium by a stopped-flow mixing technique, was ascribed to a response of 9-AA to the imposed pH gradient and not to changes in the vesicular system itself. Time constants for this fluorescence quenching are in the range of several hundred milliseconds at 25 degrees C. Fluorescence recovery which should be correlated to the dissipation of the pH gradient occurs in the 100 s time range and is 10-30-times faster than the delta pH decay monitored with the entrapped hydrophilic pH-indicator dye pyranine. The quenching was severely hindered below the lipid phase transition of dipalmitoylphosphatidylglycerol. No delta pH-induced quenching was obtained in lipid vesicles containing only zwitterionic, net uncharged phosphatidylcholine headgroups. For the occurrence of quenching, the presence of negatively charged headgroups, i.e. phosphatidylglycerol or phosphatidylserine, was necessary. The extent of quenching, at a specific pH difference applied, had a cooperative dependency (Hill coefficient approximately 2) on the number of negative headgroups in the membrane and on the concentration of unquenched (unbound) 9-AA molecules. The concentration of quenched 9-AA molecules was furthermore proportional to the number of dimer-excimer complexes of 9-AA which are formed during the quenching process.

摘要

对于多种不同的脂质体系,研究了在脂质体中施加跨膜pH梯度(内部呈酸性)后9-氨基吖啶(9-AA)的荧光猝灭情况。通过停流混合技术在囊泡外介质中诱导快速pH跃变后,最初的荧光下降归因于9-AA对施加的pH梯度的响应,而非囊泡系统本身的变化。在25℃下,这种荧光猝灭的时间常数在几百毫秒范围内。与pH梯度消散相关的荧光恢复发生在100秒的时间范围内,并且比用包封的亲水性pH指示剂染料吡喃荧光素监测的ΔpH衰减快10 - 30倍。在二棕榈酰磷脂酰甘油的脂质相变温度以下,猝灭受到严重阻碍。在仅含有两性离子、净电荷为零的磷脂酰胆碱头部基团的脂质囊泡中未观察到ΔpH诱导的猝灭。为了发生猝灭,带负电荷的头部基团,即磷脂酰甘油或磷脂酰丝氨酸的存在是必要的。在施加特定pH差时,猝灭程度对膜中负电荷头部基团的数量以及未猝灭(未结合)的9-AA分子浓度具有协同依赖性(希尔系数约为2)。此外,猝灭的9-AA分子浓度与猝灭过程中形成的9-AA二聚体 - 准分子复合物的数量成正比。

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