朝向果蝇的膜蛋白质组学:质膜的一种分离方法。
Towards a membrane proteome in Drosophila: a method for the isolation of plasma membrane.
机构信息
Department of Biology, The Pennsylvania State University, University Park, PA 16802, USA.
出版信息
BMC Genomics. 2010 May 12;11:302. doi: 10.1186/1471-2164-11-302.
BACKGROUND
The plasma membrane (PM) is a compartment of significant interest because cell surface proteins influence the way in which a cell interacts with its neighbours and its extracellular environment. However, PM is hard to isolate because of its low abundance. Aqueous two-phase affinity purification (2PAP), based on PEG/Dextran two-phase fractionation and lectin affinity for PM-derived microsomes, is an emerging method for the isolation of high purity plasma membranes from several vertebrate sources. In contrast, PM isolation techniques in important invertebrate genetic model systems, such as Drosophila melanogaster, have relied upon enrichment by density gradient centrifugation. To facilitate genetic investigation of activities contributing to the content of the PM sub-proteome, we sought to adapt 2PAP to this invertebrate model to provide a robust PM isolation technique for Drosophila.
RESULTS
We show that 2PAP alone does not completely remove contaminating endoplasmic reticulum and mitochondrial membrane. However, a novel combination of density gradient centrifugation plus 2PAP results in a robust PM preparation. To demonstrate the utility of this technique we isolated PM from fly heads and successfully identified 432 proteins using MudPIT, of which 37% are integral membrane proteins from all compartments. Of the 432 proteins, 22% have been previously assigned to the PM compartment, and a further 34% are currently unassigned to any compartment and represent candidates for assignment to the PM. The remainder have previous assignments to other compartments.
CONCLUSION
A combination of density gradient centrifugation and 2PAP results in a robust, high purity PM preparation from Drosophila, something neither technique can achieve on its own. This novel preparation should lay the groundwork for the proteomic investigation of the PM in different genetic backgrounds in Drosophila. Our results also identify two key steps in this procedure: The optimization of membrane partitioning in the PEG/Dextran mixture, and careful choice of the correct lectin for the affinity purification step in light of variations in bulk membrane lipid composition and glycosylation patterns respectively. This points the way for further adaptations into other systems.
背景
质膜(PM)是一个备受关注的隔室,因为细胞表面蛋白会影响细胞与其相邻细胞和细胞外环境相互作用的方式。然而,由于其含量低,PM 很难分离。基于 PEG/Dextran 双相分级和对 PM 衍生微粒体的凝集素亲和力的水相双相亲和纯化(2PAP)是从几种脊椎动物来源中分离高纯度质膜的新兴方法。相比之下,在重要的无脊椎动物遗传模型系统中,如黑腹果蝇,PM 分离技术依赖于密度梯度离心的富集。为了促进对有助于质膜亚蛋白质组含量的活性的遗传研究,我们试图将 2PAP 适应于这种无脊椎动物模型,为果蝇提供一种稳健的 PM 分离技术。
结果
我们表明,2PAP 本身并不能完全去除污染的内质网和线粒体膜。然而,密度梯度离心加 2PAP 的新型组合可产生稳健的 PM 制剂。为了证明这种技术的实用性,我们从果蝇头部分离了 PM,并成功地使用 MudPIT 鉴定了 432 种蛋白质,其中 37%是来自所有隔室的完整膜蛋白。在 432 种蛋白质中,22%以前被分配到 PM 隔室,另外 34%目前未被分配到任何隔室,代表被分配到 PM 的候选物。其余的先前被分配到其他隔室。
结论
密度梯度离心和 2PAP 的组合可从果蝇中产生稳健、高纯度的 PM 制剂,这两种技术本身都无法实现。这种新的制剂应为在不同遗传背景下对果蝇 PM 的蛋白质组学研究奠定基础。我们的结果还确定了该程序中的两个关键步骤:在 PEG/Dextran 混合物中优化膜分配,以及根据大量膜脂质组成和糖基化模式的变化,为亲和纯化步骤仔细选择正确的凝集素。这为进一步适应其他系统指明了方向。
Zotero 插件