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高尔基体复合体的剖析。II. 用莫能菌素处理的病毒感染细胞中特定高尔基体功能的密度分离

Dissection of the Golgi complex. II. Density separation of specific Golgi functions in virally infected cells treated with monensin.

作者信息

Quinn P, Griffiths G, Warren G

出版信息

J Cell Biol. 1983 Mar;96(3):851-6. doi: 10.1083/jcb.96.3.851.

Abstract

In the accompanying paper (Griffiths, G., P. Quinn, and G. Warren, 1983, J. Cell Biol., 96:835-850), we suggested that the Golgi stack could be divided into functionally distinct cis, medial, and trans compartments, each comprising one or two adjacent cisternae. These compartments were identified using Baby hamster kidney (BHK) cells infected with Semliki Forest virus (SFV) and treated with monensin. This drug blocked intracellular transport but not synthesis of the viral membrane proteins that were shown to accumulate in the medial cisternae. In consequence, these cisternae bound nucleocapsids. Here we show that this binding markedly increased the density of the medial cisternae and allowed us to separate them from cis and trans Golgi cisternae. A number of criteria were used to show that the intracellular capsid-binding membranes (ICBMs) observed in vivo were the same as those membranes sedimenting to a higher density in sucrose gradients in vitro, and this separation of cisternae was then used to investigate the distribution, within the Golgi stack, of some specific Golgi functions. After labeling for 2.5 min with [3H]palmitate, most of the fatty acid attached to viral membrane proteins was found in the ICBM fraction. Because the viral membrane proteins appear to move from cis to trans, this suggests that fatty acylation occurs in the cis or medial Golgi cisternae. In contrast, the distribution of alpha 1-2-mannosidase, an enzyme involved in trimming high-mannose oligosaccharides, and of galactosyl transferase, which is involved in the construction of complex oligosaccharides, was not affected by monensin treatment. Together with data in the accompanying paper, this would restrict these two Golgi functions to the trans cisternae. Our data strongly support the view that Golgi functions have specific and discrete locations within the Golgi stack.

摘要

在随附论文(格里菲思,G.,P. 奎因,和 G. 沃伦,1983 年,《细胞生物学杂志》,96:835 - 850)中,我们提出高尔基体堆叠可分为功能上不同的顺面、中间和反面区室,每个区室由一或两个相邻的扁平囊组成。这些区室是通过用辛德毕斯病毒(SFV)感染并经莫能菌素处理的幼仓鼠肾(BHK)细胞来鉴定的。这种药物阻断细胞内运输,但不阻断病毒膜蛋白的合成,结果显示这些膜蛋白在内侧扁平囊中积累。因此,这些扁平囊结合核衣壳。在这里我们表明这种结合显著增加了内侧扁平囊的密度,并使我们能够将它们与顺面和反面高尔基体扁平囊分离。我们使用了一些标准来表明在体内观察到的细胞内衣壳结合膜(ICBMs)与在体外蔗糖梯度中沉降到更高密度的那些膜相同,然后利用这种扁平囊的分离来研究某些特定高尔基体功能在高尔基体堆叠内的分布。在用[³H]棕榈酸标记 2.5 分钟后,发现附着在病毒膜蛋白上的大部分脂肪酸存在于 ICBM 组分中。由于病毒膜蛋白似乎从顺面移动到反面,这表明脂肪酸酰化发生在顺面或中间高尔基体扁平囊中。相比之下,参与修剪高甘露糖寡糖的α1 - 2 - 甘露糖苷酶以及参与复杂寡糖构建的半乳糖基转移酶的分布不受莫能菌素处理的影响。连同随附论文中的数据,这将把这两种高尔基体功能限制在反面扁平囊中。我们的数据有力地支持了这样一种观点,即高尔基体功能在高尔基体堆叠内具有特定且离散的位置。

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