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首页> 外文期刊>Biochimica et biophysica acta. Biomembranes >Effects of inhibitors of the vacuolar proton pump on hepatic heterophagy and autophagy
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Effects of inhibitors of the vacuolar proton pump on hepatic heterophagy and autophagy

机译:液泡质子泵抑制剂对肝异相和自噬的影响。

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摘要

Bafilomycin A_1 (BAF) and concanamycin A (ConcA) are selective inhibitors of the H~+-ATPases of the vacuolar system. We have examined the effects of these inhibitors on different steps in endocytic pathways in rat hepatocytes, using [~(125)I]tyramine-cellobiose-labeled asialoorosomucoid ([~(125)I]TC-AOM) and [~(125)I]tyramine-cellobiose-labeled bovine serum albumin ([~(125)ITC-BSA) as probes for respectively receptor-mediated endocytosis and pinocytosis (here defined as fluid phase endocytosis). The effects of BAF and ConcA were in principle identical, although ConcA was more effective than BAF. The main findings were as follows. (1) BAF/ConcA reduced the rate of uptake of both [~(125)I]TC-AOM and [~(125)I]TC-BSA. The reduced uptake of [~(125)I]TC-AOM was partly due to a redistribution of the asialoglycoprotein receptors (ASGPR) such that the number of surface receptors was reduced ≈40% without a change in the total number of receptors. (2) BAF/ConcA at the same time increased retroendocytosis (recycling) of both probes. The increased recycling of the ligand ([~(125)I]TC-AOM) is partly a consequence of the enhanced pH in endosomes, which prevents dissociation of ligand. (3) It was furthermore found that the ligand remained bound to the receptor in presence of BAF/ConCA and that the total amount of ligand molecules internalized in BAF/ConcA-treated cells was only slightly in excess of the total number of receptors. These data indicate that reduced pH in endosomes is the prime cause of receptor inactivation and release of ligand in early endosomes. (4) Subcellular fractionation experiments showed that [~(125)I]TC-AOM remained in early endosomes, well separated from lysosomes in sucrose gradients. The fluid phase marker, [~(125)I]TC-BSA, on the other hand, seemed to reach a later endosome in the BAF/ConcA-treated cells. This organelle coincided with lysosomes in the gradient, but hypotonic medium was found to selectively release a lysosomal enzyme (β-acetylglucosaminidase), indicating that even [~(125)I]TC-BSA remained in a prelysosomal compartment in the BAF/ConcA-treated cells. (5) Electron microscopy using horseradish peroxidase (HRP) as a fluid phase marker verified that BAF/ConcA inhibited transfer of material from late endosomes ('multivesicular bodies'). (6) BAF/ConcA led to accumulation of lactate dehydrogenase (LDH) in autophagic vacuoles, but although the drugs partly inhibited fusion between autophagosomes and lysosomes a number of autolysosomes was formed in the presence of BAF/ConcA. This observation explains the reduced buoyant density of lysosomes (revealed in sucrose density gradients). In conclusion, BAF/ConcA inhibit transfer of endocytosed material from late endosomes to lysosomes, but do not at the same time prevent fusion between autophagosomes and lysosomes.
机译:Bafilomycin A_1(BAF)和conconanamycin A(ConcA)是液泡系统H〜+ -ATPase的选择性抑制剂。我们使用[〜(125)I]酪胺纤维二糖标记的去唾液酸类糖体([〜(125)I] TC-AOM)和[〜(125))检查了这些抑制剂对大鼠肝细胞内吞途径不同步骤的影响。 I]酪胺-纤维二糖标记的牛血清白蛋白([〜(125)ITC-BSA)分别作为受体介导的内吞作用和胞饮作用(此处定义为液相内吞作用)的探针。尽管ConcA比BAF更有效,但BAF和ConcA的作用原理上是相同的。主要发现如下。 (1)BAF / ConcA降低了[〜(125)I] TC-AOM和[〜(125)I] TC-BSA的摄取率。 [〜(125)I] TC-AOM的吸收减少部分是由于去唾液酸糖蛋白受体(ASGPR)的重新分布,使得表面受体的数量减少了约40%,而受体的总数却没有变化。 (2)同时,BAF / ConcA会增加两种探针的逆转录内吞作用(再循环)。配体([〜(125)I] TC-AOM)再循环的增加部分是内体pH升高的结果,这阻止了配体的解离。 (3)还发现,在BAF / ConCA存在下,配体仍然与受体结合,并且在BAF / ConcA处理的细胞中内在化的配体分子的总量仅略大于受体的总数。这些数据表明,内体pH降低是早期内体受体失活和配体释放的主要原因。 (4)亚细胞分级分离实验表明,[〜(125)I] TC-AOM保留在早期的内体中,并在蔗糖梯度中与溶酶体充分分离。另一方面,在BAF / ConcA处理的细胞中,液相标记[〜(125)I] TC-BSA似乎到达了较晚的内体。该细胞器与溶酶体在梯度中重合,但发现低渗介质选择性释放溶酶体酶(β-乙酰氨基葡萄糖苷酶),表明甚至[〜(125)I] TC-BSA仍保留在BAF / ConcA-处理过的细胞。 (5)使用辣根过氧化物酶(HRP)作为液相标记物的电子显微镜证实,BAF / ConcA抑制了来自晚期内体(“多囊泡体”)的物质转移。 (6)BAF / ConcA导致自噬泡中乳酸脱氢酶(LDH)的积累,但是尽管药物部分抑制自噬体和溶酶体之间的融合,但是在BAF / ConcA存在下会形成许多自溶体。该观察结果解释了溶酶体的浮力密度降低(在蔗糖密度梯度中显示)。总之,BAF / ConcA抑制了内吞材料从晚期内体向溶酶体的转移,但没有同时阻止自噬体与溶酶体之间的融合。

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