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活细胞成像显示,在烟草 BY-2 细胞中,双标记的高尔基堆叠在运动和布雷菲德菌素 A 处理过程中表现出相似的行为。

Live-cell imaging of dual-labeled Golgi stacks in tobacco BY-2 cells reveals similar behaviors for different cisternae during movement and brefeldin A treatment.

机构信息

Department of Biochemistry and Cellular and Molecular Biology, University of Tennessee, Knoxville, TN 37996-0840, USA.

出版信息

Mol Plant. 2011 Sep;4(5):896-908. doi: 10.1093/mp/ssr067. Epub 2011 Aug 25.

DOI:10.1093/mp/ssr067
PMID:21873295
Abstract

In plant cells, the Golgi apparatus consists of numerous stacks that, in turn, are composed of several flattened cisternae with a clear cis-to-trans polarity. During normal functioning within living cells, this unusual organelle displays a wide range of dynamic behaviors such as whole stack motility, constant membrane flux through the cisternae, and Golgi enzyme recycling through the ER. In order to further investigate various aspects of Golgi stack dynamics and integrity, we co-expressed pairs of established Golgi markers in tobacco BY-2 cells to distinguish sub-compartments of the Golgi during monensin treatments, movement, and brefeldin A (BFA)-induced disassembly. A combination of cis and trans markers revealed that Golgi stacks remain intact as they move through the cytoplasm. The Golgi stack orientation during these movements showed a slight preference for the cis side moving ahead, but trans cisternae were also found at the leading edge. During BFA treatments, the different sub-compartments of about half of the observed stacks fused with the ER sequentially; however, no consistent order could be detected. In contrast, the ionophore monensin resulted in swelling of trans cisternae while medial and particularly cis cisternae were mostly unaffected. Our results thus demonstrate a remarkable equivalence of the different cisternae with respect to movement and BFA-induced fusion with the ER. In addition, we propose that a combination of dual-label fluorescence microscopy and drug treatments can provide a simple alternative approach to the determination of protein localization to specific Golgi sub-compartments.

摘要

在植物细胞中,高尔基体由许多堆叠组成,而这些堆叠又由几个扁平的潴泡组成,具有明确的 cis-to-trans 极性。在活细胞的正常功能中,这个不寻常的细胞器表现出广泛的动态行为,如整个堆栈的运动、内质网中通过潴泡的恒定膜通量以及高尔基体酶通过内质网的再循环。为了进一步研究高尔基体堆栈动力学和完整性的各个方面,我们在烟草 BY-2 细胞中共同表达了一对已建立的高尔基体标记物,以在莫能菌素处理、运动和布雷菲德菌素 A(BFA)诱导的解体过程中区分高尔基体的亚区室。顺式和反式标记物的组合表明,高尔基体堆栈在细胞质中移动时保持完整。在这些运动过程中,高尔基体堆栈的取向显示出 cis 侧略微领先的偏好,但也发现反式潴泡位于前沿。在 BFA 处理过程中,大约一半观察到的堆栈的不同亚区室依次与内质网融合;然而,无法检测到一致的顺序。相比之下,离子载体莫能菌素导致反式潴泡膨胀,而中间特别是 cis 潴泡大多不受影响。因此,我们的结果表明,不同潴泡在运动和 BFA 诱导与内质网融合方面具有显著的等效性。此外,我们提出,双重荧光显微镜和药物处理的组合可以为确定特定高尔基体亚区室的蛋白质定位提供一种简单的替代方法。

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