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Functional Compartmentation of the Golgi Apparatus of Plant Cells 1: Immunocytochemical Analysis of High-Pressure Frozen- and Freeze-Substituted Sycamore Maple Suspension Culture Cells

机译:高尔基体植物细胞的功能区划1:高压冷冻和冷冻替代的梧桐枫悬浮培养细胞的免疫细胞化学分析

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摘要

The Golgi apparatus of plant cells is engaged in both the processing of glycoproteins and the synthesis of complex polysaccharides. To investigate the compartmentalization of these functions within individual Golgi stacks, we have analyzed the ultrastructure and the immunolabeling patterns of high-pressure frozen and freeze-substituted suspension-cultured sycamore maple (Acer pseudoplatanus L.) cells. As a result of the improved structural preservation, three morphological types of Golgi cisternae, designated cis, medial, and trans, as well as the trans Golgi network, could be identified. The number of cis cisternae per Golgi stack was found to be fairly constant at approximately 1, whereas the number of medial and trans cisternae per stack was variable and accounted for the varying number of cisternae (3-10) among the many Golgi stacks examined. By using a battery of seven antibodies whose specific sugar epitopes on secreted polysaccharides and glycoproteins are known, we have been able to determine in which types of cisternae specific sugars are added to N-linked glycans, and to xyloglucan and polygalacturonic acid/rhamnogalacturonan-I, two complex polysaccharides. The findings are as follows. The β-1,4-linked d-glucosyl backbone of xyloglucan is synthesized in trans cisternae, and the terminal fucosyl residues on the trisaccharide side chains of xyloglucan are partly added in the trans cisternae, and partly in the trans Golgi network. In contrast, the polygalacturonic/rhamnogalacturonan-I backbone is assembled in cis and medial cisternae, methylesterification of the carboxyl groups of the galacturonic acid residues in the polygalacturonic acid domains occurs mostly in medial cisternae, and arabinose-containing side chains of the polygalacturonic acid domains are added to the nascent polygalacturonic acid/rhamnogalacturonan-I molecules in the trans cisternae. Double labeling experiments demonstrate that xyloglucan and polygalacturonic acid/rhamnogalacturonan-I can be synthesized concomitantly within the same Golgi stack. Finally, we show that the xylosyl residue-linked β-1,2 to the β-linked mannose of the core of N-linked glycans is added in medial cisternae. Taken together, our results indicate that in sycamore maple suspension-cultured cells, different types of Golgi cisternae contain different sets of glycosyl transferases, that the functional organization of the biosynthetic pathways of complex polysaccharides is consistent with these molecules being processed in a cis to trans direction like the N-linked glycans, and that the complex polysaccharide xyloglucan is assembled exclusively in trans Golgi cisternae and the trans Golgi network.
机译:植物细胞的高尔基体参与糖蛋白的加工和复杂多糖的合成。为了研究这些功能在单个高尔基体中的区室化,我们分析了高压冷冻和冷冻取代的悬浮培养的美国梧桐枫(Acer pseudoplatanus L.)细胞的超微结构和免疫标记模式。作为改善的结构保存的结果,可以识别出高尔基蓄水池的三种形态类型,称为顺式,中间和反式,以及反式高尔基体网络。发现每个高尔基堆栈的顺式水箱数量相当恒定,大约为1,而每个堆栈的内侧和反式水箱的数量是可变的,并说明了在所检查的许多高尔基堆栈中水箱的数量不一(3-10)。通过使用七种抗体的电池,这些抗体的分泌糖和糖蛋白上的特定糖表位是已知的,我们已经能够确定在哪种储罐中将特定糖添加到N-连接的聚糖,木葡聚糖和聚半乳糖醛酸/鼠李糖半乳糖醛酸-I中,两种复合多糖。调查结果如下。木葡聚糖的β-1,4-连接的d-葡萄糖基骨架是在反式池中合成的,木葡聚糖的三糖侧链上的末端岩藻糖基残基部分地添加在反式池中,部分地在反式高尔基体中。相反,聚半乳糖醛酸/鼠李半乳糖醛酸聚糖-I主链在顺式和内侧储水池中组装,聚半乳糖醛酸域中半乳糖醛酸残基的羧基的甲基酯化主要发生在内侧储水池中,并且聚半乳糖醛酸域的含阿拉伯糖的侧链将其加入反式水箱中的新生的聚半乳糖醛酸/鼠李半乳糖醛酸聚糖-I分子中。双重标记实验表明,木葡聚糖和聚半乳糖醛酸/鼠李半乳糖醛酸聚糖-I可以在同一高尔基体中同时合成。最后,我们显示了在内侧水箱中添加了木糖基残基连接的β-1,2至N-连接聚糖核心的β-连接甘露糖。两者合计,我们的结果表明,在美国梧桐枫悬浮培养的细胞中,不同类型的高尔基蓄水池含有不同的糖基转移酶组,复杂多糖的生物合成途径的功能组织与顺式加工成反式的这些分子是一致的方向像N-连接的聚糖一样,并且复杂的多糖木葡聚糖仅在反式高尔基蓄水池和反式高尔基体网络中组装。

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