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Rapid flip-flop of phospholipids in endoplasmic reticulum membranes studied by a stopped-flow approach.

机译:通过停止流方法研究内质网膜中磷脂的快速翻转。

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摘要

The transbilayer movement of short-chain spin-labeled and fluorescent 7-nitrobenz-2-oxa-1,3-diazol-4-yl (NBD) phospholipid analogs in rat liver microsomes is measured by stopped-flow mixing of labeled microsomes with bovine serum albumin (BSA) solution. Extraction of analogs from the outer leaflet of microsomes to BSA can be directly monitored in conjunction with electron paramagnetic resonance or fluorescence spectroscopy by taking advantage of the fact that the signal of spin-labeled or fluorescent analogs bound to BSA is different from that of the analogs inserted into membranes. From the signal kinetics, the transbilayer movement and the distribution of analogs in microsomal membranes can be derived provided the extraction of analogs by BSA is much faster in comparison to the transbilayer movement of analogs. Half-times of the back-exchange for spin-labeled and fluorescent analogs were <3.5 and <9.5 s, respectively. The unprecedented time resolution of the assay revealed that the transbilayer movement of spin-labeled analogs is much faster than previously reported. The half-time of the movement was about 16 s or even less at room temperature. Transmembrane movement of NBD-labeled analogs was six- to eightfold slower than that of spin-labeled analogs.
机译:短链自旋标记的和荧光的7-硝基苯-2-氧杂-1,3-二氮杂-4-基(NBD)磷脂类似物在大鼠肝微粒体中的跨双层运动是通过将标记微粒体与牛停流混合来测量的血清白蛋白(BSA)溶液。利用结合到BSA的自旋标记或荧光类似物的信号与类似物的信号不同的事实,可以结合电子顺磁共振或荧光光谱法直接监测从微粒体外小叶到BSA的类似物的提取。插入膜中。从信号动力学,可以得出透双层运动和类似物在微粒体膜中的分布,前提是与类似物的跨双层运动相比,BSA提取类似物要快得多。自旋标记和荧光类似物的反向交换的一半时间分别<3.5和<9.5 s。该测定方法史无前例的时间分辨率表明,自旋标记类似物的跨双层运动比以前报道的要快得多。在室温下,机芯的半衰期约为16 s或更短。 NBD标记类似物的跨膜运动比自旋标记类似物慢六到八倍。

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