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自噬溶酶体途径参与大鼠肝脏的脂质降解。

Autophagy-lysosomal pathway is involved in lipid degradation in rat liver.

机构信息

Department of Biochemistry, Institute of Chemical Technology, Prague, Czech Republic.

出版信息

Physiol Res. 2012;61(3):287-97. doi: 10.33549/physiolres.932285. Epub 2012 Apr 5.

DOI:10.33549/physiolres.932285
PMID:22480422
Abstract

We present data supporting the hypothesis that the lysosomal-autophagy pathway is involved in the degradation of intracellular triacylglycerols in the liver. In primary hepatocytes cultivated in the absence of exogenous fatty acids (FFA), both inhibition of autophagy flux (asparagine) or lysosomal activity (chloroquine) decreased secretion of VLDL (very low density lipoproteins) and formation of FFA oxidative products while the stimulation of autophagy by rapamycine increased some of these parameters. Effect of rapamycine was completely abolished by inactivation of lysosomes. Similarly, when autophagic activity was influenced by cultivating the hepatocytes in "starving" (amino-acid poor medium) or "fed" (serum-supplemented medium) conditions, VLDL secretion and FFA oxidation mirrored the changes in autophagy being higher in starvation and lower in fed state. Autophagy inhibition as well as lysosomal inactivation depressed FFA and DAG (diacylglycerol) formation in liver slices in vitro. In vivo, intensity of lysosomal lipid degradation depends on the formation of autophagolysosomes, i.e. structures bringing the substrate for degradation and lysosomal enzymes into contact. We demonstrated that lysosomal lipase (LAL) activity in liver autophagolysosomal fraction was up-regulated in fasting and down-regulated in fed state together with the increased translocation of LAL and LAMP2 proteins from lysosomal pool to this fraction. Changes in autophagy intensity (LC3-II/LC3-I ratio) followed a similar pattern.

摘要

我们提供的数据支持这样一种假设,即溶酶体-自噬途径参与了肝脏内细胞内三酰基甘油的降解。在不存在外源脂肪酸(FFA)的情况下培养的原代肝细胞中,自噬流(天冬酰胺)或溶酶体活性(氯喹)的抑制均降低了 VLDL(极低密度脂蛋白)的分泌和 FFA 氧化产物的形成,而雷帕霉素刺激自噬则增加了其中一些参数。雷帕霉素的作用被溶酶体失活完全消除。同样,当通过在“饥饿”(氨基酸贫乏的培养基)或“喂养”(补充血清的培养基)条件下培养肝细胞来影响自噬活性时,VLDL 分泌和 FFA 氧化反映了自噬的变化,饥饿状态下自噬活性更高,而喂养状态下自噬活性更低。自噬抑制和溶酶体失活均可抑制肝切片中 FFA 和 DAG(二酰基甘油)的形成。在体内,溶酶体脂质降解的强度取决于自噬溶酶体的形成,即将底物带入降解并将溶酶体酶带入接触的结构。我们证明,在禁食和喂养状态下,肝自噬溶酶体部分中的溶酶体脂肪酶(LAL)活性上调,LAL 和 LAMP2 蛋白从溶酶体池向该部分的易位增加。自噬强度的变化(LC3-II/LC3-I 比值)也呈现出相似的模式。

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