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使用二氨基联苯胺诱导的密度转移分离外侧边界循环区室

Isolation of the lateral border recycling compartment using a diaminobenzidine-induced density shift.

作者信息

Sullivan David P, Rüffer Claas, Muller William A

机构信息

Department of Pathology, Feinberg School of Medicine, Northwestern University, Chicago, IL, 60611, USA.

出版信息

Traffic. 2014 Sep;15(9):1016-29. doi: 10.1111/tra.12184. Epub 2014 Jul 1.

Abstract

The migration of leukocytes across the endothelium and into tissue is critical to mounting an inflammatory response. The lateral border recycling compartment (LBRC), a complex vesicular-tubule invagination of the plasma membrane found at endothelial cell borders, plays an important role in this process. Although a few proteins have been shown to be present in the LBRC, no unique marker is known. Here, we detail methods that can be used to characterize a subcellular compartment that lacks an identifying marker. Initial characterization of the LBRC was performed using standard subcellular fractionation with sucrose gradients and took advantage of the observation that the compartment migrated at a lower density than other membrane compartments. To isolate larger quantities of the compartment, we modified a classic technique known as a diaminobenzidine (DAB)-induced density shift. The DAB-induced density shift allowed for specific isolation of membranes labeled with horseradish peroxidase-conjugated antibody. Because the LBRC could be differentially labeled at 4 °C and 37 °C, we were able to identify proteins that are enriched in the compartment, despite lacking a unique marker. These methods serve as a model to others studying poorly characterized compartments and organelles and are applicable to a wide variety of biological systems.

摘要

白细胞穿过内皮细胞迁移至组织对于引发炎症反应至关重要。侧向边界循环区室(LBRC)是在内皮细胞边界处发现的质膜复杂的囊泡 - 小管内陷结构,在此过程中发挥重要作用。尽管已证明有几种蛋白质存在于LBRC中,但尚无已知的独特标志物。在这里,我们详细介绍了可用于表征缺乏识别标志物的亚细胞区室的方法。LBRC的初步表征是使用蔗糖梯度进行标准亚细胞分级分离,并利用该区室比其他膜区室迁移密度更低这一观察结果。为了分离更多量的该区域,我们改进了一种称为二氨基联苯胺(DAB)诱导密度转移的经典技术。DAB诱导的密度转移允许特异性分离用辣根过氧化物酶偶联抗体标记的膜。由于LBRC在4°C和37°C时可被差异标记,因此尽管缺乏独特标志物,我们仍能够鉴定出在该区域富集的蛋白质。这些方法为其他研究特征不明的区室和细胞器的人提供了一个模型,并且适用于多种生物系统。

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