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Lipoprotein lipase activity and interactions studied in human plasma by isothermal titration calorimetry

机译:等温滴定热法研究人血浆中脂蛋白脂肪酶的活性和相互作用

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摘要

LPL hydrolyzes triglycerides in plasma lipoproteins. Due to the complex regulation mechanism, it has been difficult to mimic the physiological conditions under which LPL acts in vitro. We demonstrate that isothermal titration calorimetry (ITC), using human plasma as substrate, overcomes several limitations of previously used techniques. The high sensitivity of ITC allows continuous recording of the heat released during hydrolysis. Both initial rates and kinetics for complete hydrolysis of plasma lipids can be studied. The heat rate was shown to correspond to the release of fatty acids and was linearly related to the amount of added enzyme, either purified LPL or postheparin plasma. Addition of apoC-III reduced the initial rate of hydrolysis by LPL, but the inhibition became less prominent with time when the lipoproteins were triglyceride poor. Addition of angiopoietin-like protein (ANGPTL)3 or ANGPTL4 caused reduction of the activity of LPL via a two-step mechanism. We conclude that ITC can be used for quantitative measurements of LPL activity and interactions under in vivo-like conditions, for comparisons of the properties of plasma samples from patients and control subjects as substrates for LPL, as well as for testing of drug candidates developed with the aim to affect the LPL system.
机译:LPL水解血浆脂蛋白中的甘油三酸酯。由于复杂的调节机制,很难模仿LPL在体外起作用的生理条件。我们证明使用人血浆作为底物的等温滴定量热法(ITC)克服了以前使用的技术的一些局限性。 ITC的高灵敏度允许连续记录水解过程中释放的热量。可以研究血浆脂质完全水解的初始速率和动力学。加热速率显示出与脂肪酸的释放相对应,并且与添加的酶(纯化的LPL或肝素后血浆)的量线性相关。 apoC-III的添加降低了LPL的初始水解速率,但是当脂蛋白的甘油三酸酯含量较低时,抑制作用随时间的推移而减弱。血管生成素样蛋白(ANGPTL)3或ANGPTL4的添加通过两步机制导致LPL活性降低。我们得出的结论是,ITC可用于在类似体内的条件下定量测量LPL活性和相互作用,用于比较作为LPL底物的患者和对照组受试者的血浆样品的性质,以及用于测试使用目的是影响LPL系统。

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