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首页> 外文期刊>The Journal of biological chemistry >Starvation-induced Hyperacetylation of Tubulin Is Required for the Stimulation of Autophagy by Nutrient Deprivation
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Starvation-induced Hyperacetylation of Tubulin Is Required for the Stimulation of Autophagy by Nutrient Deprivation

机译:通过营养剥夺刺激自噬刺激饥饿诱导的微管蛋白化

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The molecular mechanisms underlying microtubule participation in autophagy are not known. In this study, we show that starvation-induced autophagosome formation requires the most dynamic microtubule subset. Upon nutrient deprivation, labile microtubules specifically recruit markers of autophagosome formation like class III-phosphatidylinositol kinase, WIPI-1, the Atg12-Atg5 conjugate, and LC3-I, whereas mature autophagosomes may bind to stable microtubules. We further found that upon nutrient deprivation, tubulin acetylation increases both in labile and stable microtubules and is required to allow autophagy stimulation. Tubulin hyperacetylation on lysine 40 enhances kinesin-1 and JIP-1 recruitment on microtubules and allows JNK phosphorylation and activation. JNK, in turn, triggers the release of Beclin 1 from Bcl-2-Beclin 1 complexes and its recruitment on microtubules where it may initiate autophagosome formation. Finally, although kinesin-1 functions to carry autophagosomes in basal conditions, it is not involved in motoring autophagosomes after nutrient deprivation. Our results show that the dynamics of microtubules and tubulin post-translational modifications play a major role in the regulation of starvation-induced autophagy.
机译:潜在的微管参与自噬的分子机制尚不清楚。在这项研究中,我们表明饥饿诱导的自噬体形成需要最动态的微管子集。在营养剥夺时,不稳定的微管特异性募集自磷脂酰肌醇激酶,WIPI-1,ATG12-ATG5缀合物和LC3-1的自噬体形成标记物,而成熟的自噬体可以结合稳定的微管。我们进一步发现,在营养剥夺时,管蛋白乙酰化在不稳定和稳定的微管中增加,并且需要允许自噬刺激。赖氨酸40上的微管蛋白化学化增强了在微管上的kinesin-1和JIP-1募集,并允许JNK磷酸化和活化。反过来,JNK触发了BECLIN 1的释放来自BCL-2-BENLIN 1络合物及其在可以引发自噬体形成的微管中的募集。最后,尽管Kinesin-1用于在基础条件下携带自噬物质,但它不参与营养剥夺后的电动自噬体。我们的研究结果表明,微管和微管蛋白的动态翻译后修饰在饥饿诱导的自噬的调节中起主要作用。

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