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Quantitation of lysolipids fatty acids and phospholipase A2 activity and correlation with membrane polarity

机译:溶血脂脂肪酸和磷脂酶A2活性的定量及其与膜极性的关系

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摘要

Acrylodan-labeled rat-intestinal fatty acid binding protein, ADIFAB, binds both of lysophosphatidylcholines (LPC) and FA. Binding displaces Acrylodan and its fluorescence peak shifts from 432 to 505 nm. A fluorescence assay that relies on this shift is presented for quantitating LPC, FA, and phospholipase A2 (PLA2) activity in phospholipid bilayers in absolute units of μM/min/mg of enzyme. This is a development over an earlier assay that took into account only FA binding. Activities of bee venom PLA2 on dipalmitoylphosphatidylcholine (DPPC) and dioleylphosphatidylcholine (DOPC) bilayers were measured. Standard pH-Stat assays validated the present assay. Products increase linearly with time for about one minute in DOPC and five minutes in DPPC corresponding to completion of 5 to 8% hydrolysis in DOPC and 20% in DPPC. Membrane polarity and microviscosity measured using electron spin resonance (ESR) exhibited discontinuities at compositions that mimicked similar percentages of hydrolysis products in the respective bilayers. The observed hydrolysis rate decrease following the initial linear period thus correlates to changes in membrane polarity. The ability of the assay to yield actual product concentrations, reveal structure in the reaction progress curves, and interpretation in light of the ESR data bring insight into the shape of the reaction curve.
机译:Acrylodan标记的大鼠肠道脂肪酸结合蛋白ADIFAB结合溶血磷脂酰胆碱(LPC)和FA。结合取代了丙烯腈,其荧光峰从432 nm移至505 nm。提出了一种依赖于这种转变的荧光测定法,用于以绝对单位μM/ min / mg的酶定量磷脂双层中的LPC,FA和磷脂酶A2(PLA2)活性。这是对仅考虑FA结合的早期检测方法的改进。测量了蜂毒PLA2对二棕榈酰磷脂酰胆碱(DPPC)和二油酰磷脂酰胆碱(DOPC)双层的活性。标准pH-Stat测定法验证了本测定法。在DOPC中,产物随时间线性增加约1分钟,而在DPPC中则随时间线性增加5分钟,这对应于DOPC中5%至8%的水解完成和DPPC中20%的水解完成。使用电子自旋共振(ESR)测量的膜极性和微粘度在模仿相应双层中水解产物相似百分比的组合物中表现出不连续性。在初始线性周期之后观察到的水解速率降低,因此与膜极性的变化相关。该测定产生实际产物浓度,揭示反应进程曲线中结构的能力以及根据ESR数据进行解释的能力使您能够洞悉反应曲线的形状。

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