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The angiopoietin-like protein ANGPTL4 catalyzes unfolding of the hydrolase domain in lipoprotein lipase and the endothelial membrane protein GPIHBP1 counteracts this unfolding

机译:血管生成素样蛋白ANGPTL4催化脂蛋白脂肪酶中水解酶结构域的解折叠,内皮膜蛋白GPIHBP1抵消了这种解折叠

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摘要

Lipoprotein lipase (LPL) undergoes spontaneous inactivation via global unfolding and this unfolding is prevented by GPIHBP1 (Mysling et al., 2016). We now show: (1) that ANGPTL4 inactivates LPL by catalyzing the unfolding of its hydrolase domain; (2) that binding to GPIHBP1 renders LPL largely refractory to this inhibition; and (3) that both the LU domain and the intrinsically disordered acidic domain of GPIHBP1 are required for this protective effect. Genetic studies have found that a common polymorphic variant in ANGPTL4 results in lower plasma triglyceride levels. We now report: (1) that this ANGPTL4 variant is less efficient in catalyzing the unfolding of LPL; and (2) that its Glu-to-Lys substitution destabilizes its N-terminal alpha-helix. Our work elucidates the molecular basis for regulation of LPL activity by ANGPTL4, highlights the physiological relevance of the inherent instability of LPL, and sheds light on the molecular defects in a clinically relevant variant of ANGPTL4.
机译:脂蛋白脂肪酶(LPL)通过整体展开自发失活,这种展开被GPIHBP1阻止(Mysling等,2016)。我们现在显示:(1)ANGPTL4通过催化其水解酶结构域的展开而使LPL失活; (2)与GPIHBP1的结合使LPL在这种抑制作用下难以抵抗; (3)GPIHBP1的LU结构域和内在无序的酸性结构域都需要这种保护作用。遗传研究发现,ANGPTL4中常见的多态性变异导致血浆甘油三酯水平降低。我们现在报告:(1)该ANGPTL4变体在催化LPL的展开中效率较低; (2)其Glu-to-Lys取代会破坏其N-末端的α-螺旋。我们的工作阐明了ANGPTL4调节LPL活性的分子基础,强调了LPL固有不稳定性的生理相关性,并阐明了ANGPTL4临床相关变体中的分子缺陷。

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