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高尔基体从内质网进行生物合成的能力。

Capacity of the golgi apparatus for biogenesis from the endoplasmic reticulum.

作者信息

Puri Sapna, Linstedt Adam D

机构信息

Department of Biological Sciences, Carnegie Mellon University, Pittsburgh, Pennsylvania 15213, USA.

出版信息

Mol Biol Cell. 2003 Dec;14(12):5011-8. doi: 10.1091/mbc.e03-06-0437. Epub 2003 Oct 17.

Abstract

It is unclear whether the mammalian Golgi apparatus can form de novo from the ER or whether it requires a preassembled Golgi matrix. As a test, we assayed Golgi reassembly after forced redistribution of Golgi matrix proteins into the ER. Two conditions were used. In one, ER redistribution was achieved using a combination of brefeldin A (BFA) to cause Golgi collapse and H89 to block ER export. Unlike brefeldin A alone, which leaves matrix proteins in relatively large remnant structures outside the ER, the addition of H89 to BFA-treated cells caused ER accumulation of all Golgi markers tested. In the other, clofibrate treatment induced ER redistribution of matrix and nonmatrix proteins. Significantly, Golgi reassembly after either treatment was robust, implying that the Golgi has the capacity to form de novo from the ER. Furthermore, matrix proteins reemerged from the ER with faster ER exit rates. This, together with the sensitivity of BFA remnants to ER export blockade, suggests that presence of matrix proteins in BFA remnants is due to cycling via the ER and preferential ER export rather than their stable assembly in a matrix outside the ER. In summary, the Golgi apparatus appears capable of efficient self-assembly.

摘要

尚不清楚哺乳动物的高尔基体能否从内质网重新从头形成,还是需要一个预先组装好的高尔基体基质。作为一项测试,我们检测了高尔基体基质蛋白被迫重新分布到内质网后高尔基体的重新组装情况。使用了两种条件。其一,通过结合使用布雷菲德菌素A(BFA)导致高尔基体解体和H89阻断内质网输出,实现内质网重新分布。与单独使用布雷菲德菌素A不同,后者会使基质蛋白留在内质网外相对较大的残余结构中,向经BFA处理的细胞中添加H89会导致所有测试的高尔基体标记物在内质网中积累。其二,氯贝丁酯处理诱导基质和非基质蛋白在内质网中重新分布。重要的是,两种处理后高尔基体的重新组装都很稳健,这意味着高尔基体有能力从内质网重新从头形成。此外,基质蛋白从内质网中重新出现时内质网输出速率更快。这一点,连同BFA残余物对内质网输出阻断的敏感性,表明BFA残余物中基质蛋白的存在是由于通过内质网循环和优先内质网输出,而不是它们在质网外基质中的稳定组装。总之,高尔基体似乎能够进行高效的自我组装。

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