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Long-chain acyl-CoA synthetase isoforms differ in preferences for eicosanoid species and long-chain fatty acids

机译:长链酰基辅酶A合成酶同工型在类花生酸和长链脂肪酸的偏好上有所不同

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摘要

Because the signaling eicosanoids, epoxyeicosatrienoic acids (EETs) and HETEs, are esterified to membrane phospholipids, we asked which long-chain acyl-CoA synthetase (ACSL) isoforms would activate these molecules and whether the apparent FA substrate preferences of each ACSL isoform might differ depending on whether it was assayed in mammalian cell membranes or as a purified bacterial recombinant protein. We found that all five ACSL isoforms were able to use EETs and HETEs as substrates and showed by LC-MS/MS that ACSLs produce EET-CoAs. We found differences in substrate preference between ACS assays performed in COS7 cell membranes and recombinant purified proteins. Similarly, preferences and Michaelis-Menten kinetics for long-chain FAs were distinctive. Substrate preferences identified for the purified ACSLs did not correspond to those observed in ACSL-deficient mouse models. Taken together, these data support the concept that each ACSL isoform exhibits a distinct substrate preference, but apparent substrate specificities depend upon multiple factors including membrane character, coactivators, inhibitors, protein interactions, and posttranslational modification.
机译:由于信号类二十烷酸,环氧二十碳三烯酸(EET)和HETE被酯化为膜磷脂,我们询问哪种长链酰基辅酶A合成酶(ACSL)同工型会激活这些分子,以及每种ACSL同工型的表观FA底物偏好是否可能不同取决于是在哺乳动物细胞膜中进行检测还是作为纯化的细菌重组蛋白进行检测。我们发现所有五种ACSL同工型均能够使用EET和HETE作为底物,并通过LC-MS / MS表明ACSL产生EET-CoA。我们发现在COS7细胞膜中进行的ACS测定与重组纯化的蛋白之间在底物偏好方面存在差异。同样,长链FA的偏好和Michaelis-Menten动力学也很独特。为纯化的ACSL确定的底物偏好与在ACSL缺陷小鼠模型中观察到的底物偏好不符。综上所述,这些数据支持以下概念:每种ACSL同工型均表现出不同的底物偏好,但表观底物特异性取决于多种因素,包括膜特性,共激活剂,抑制剂,蛋白质相互作用和翻译后修饰。

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