首页> 美国卫生研究院文献>Biochemical Journal >Comparison of the degradative fate of monoamine oxidase in endogenous and transplanted mitochondrial outer membrane in rat hepatocytes. Implications for the cytomorphological basis of protein catabolism.
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Comparison of the degradative fate of monoamine oxidase in endogenous and transplanted mitochondrial outer membrane in rat hepatocytes. Implications for the cytomorphological basis of protein catabolism.

机译:大鼠肝细胞内源性和线粒体外膜单胺氧化酶降解命运的比较。对蛋白质分解代谢的细胞形态学基础的影响。

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摘要

The degradative fate of monoamine oxidase in endogenous and transplanted mitochondrial outer membrane has been compared in rat hepatocyte monolayers. Monoamine oxidase was specifically irreversibly radiolabelled by the suicide inhibitor [3H]pargyline. Hepatocyte monolayers were cultured in conditions in which rates of protein catabolism like those in vivo are maintained [Evans & Mayer (1983) Biochem. J. 216, 151-161]. Incubation of hepatocyte monolayers for 17 h with [3H]pargyline specifically radiolabels mitochondrial monoamine oxidase, as shown by Percoll-gradient fractionation of broken hepatocytes. Monoamine oxidase is degraded at a similar rate to that observed in liver in vivo (t1/2 approx. 63 h). The effects of leupeptin, methylamine and colchicine on the degradation of endogenous radiolabelled enzyme has been studied over prolonged culture periods. Culture of hepatocytes for periods of up to 80 h with inhibitors was not cytotoxic, as demonstrated by measurements of several intrinsic biochemical parameters. Leupeptin, methylamine and colchicine inhibit the degradation of endogenous monoamine oxidase by 60, 38 and 18% respectively. Monoamine oxidase in mitochondrial-outer-membrane vesicles introduced into hepatocytes by poly(ethylene glycol)-mediated vesicle-cell transplantation is degraded at a similar rate (t1/2 55 h) to the endogenous mitochondrial enzyme. Whereas leupeptin inhibits the degradation of endogenous and transplanted enzyme to a similar extent, methylamine and colchicine inhibit the degradation of transplanted enzyme to a much greater extent (85 and 56% respectively). Fluorescence microscopy (with fluorescein isothiocyanate-conjugated mitochondrial outer membrane) shows that transplanted mitochondrial outer membrane undergoes internalization and translocation to a sided perinuclear site, as observed previously with whole mitochondria [Evans & Mayer (1983) Biochem. J. 216, 151-161]. The effects of the inhibitors on the distribution of transplanted membrane material in the cell and inhibition of proteolysis show the importance of cytomorphology for intracellular protein catabolism.
机译:已在大鼠肝细胞单层中比较了内源性和移植的线粒体外膜中单胺氧化酶的降解命运。自杀抑制剂[3H] pargyline特别不可逆地对单胺氧化酶进行了放射性标记。在维持蛋白质分解代谢速率如体内速率的条件下培养肝细胞单层[Evans&Mayer(1983)Biochem。 J. 216,151-161]。肝细胞单层与[3H] Pargyline一起孵育17小时后,会特异性地放射性标记线粒体单胺氧化酶,如破碎的肝细胞的Percoll梯度分级所示。单胺氧化酶的降解速率与体内肝脏观察到的速率相似(t1 / 2约63小时)。在延长的培养时间内,已经研究了亮肽素,甲胺和秋水仙碱对内源性放射性标记酶降解的影响。如通过几个固有生化参数的测量所证实,用抑制剂培养肝细胞长达80 h的时间没有细胞毒性。 Leupeptin,甲胺和秋水仙碱分别抑制内源性单胺氧化酶的降解60%,38%和18%。通过聚(乙二醇)介导的囊泡细胞移植引入肝细胞的线粒体外膜囊泡中的单胺氧化酶以与内源性线粒体酶相似的速率(t1 / 2 55 h)降解。亮肽素对内源和移植酶的降解具有相似的抑制作用,而甲胺和秋水仙碱对移植酶的降解具有更大的抑制作用(分别为85%和56%)。荧光显微镜(用异硫氰酸荧光素缀合的线粒体外膜)显示,移植的线粒体外膜经历了内在化和易位至侧核周位点,如先前在整个线粒体中所观察到的那样(Evans&Mayer(1983)Biochem。 J. 216,151-161]。抑制剂对细胞中膜材料分布的分布和蛋白水解的抑制作用表明细胞形态对细胞内蛋白质分解代谢的重要性。

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