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首页> 外文期刊>Biochimica et biophysica acta. Biomembranes >Monitoring glycolipid transfer protein activity and membrane interaction with the surface plasmon resonance technique.
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Monitoring glycolipid transfer protein activity and membrane interaction with the surface plasmon resonance technique.

机译:使用表面等离振子共振技术监测糖脂转移蛋白的活性和膜相互作用。

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The glycolipid transfer protein (GLTP) is a protein capable of binding and transferring glycolipids. GLTP is cytosolic and it can interact through its FFAT-like (two phenylalanines in an acidic tract) motif with proteins localized on the surface of the endoplasmic reticulum. Previous in vitro work with GLTP has focused mainly on the complete transfer reaction of the protein, that is, binding and subsequent removal of the glycolipid from the donor membrane, transfer through the aqueous environment, and the final release of the glycolipid to an acceptor membrane. Using bilayer vesicles and surface plasmon resonance spectroscopy, we have now, for the first time, analyzed the binding and lipid removal capacity of GLTP with a completely label-free technique. This technique is focused on the initial steps in GLTP-mediated transfer and the parameters affecting these steps can be more precisely determined. We used the new approach for detailed structure-function studies of GLTP by examining the glycolipid transfer capacity of specific GLTP tryptophan mutants. Tryptophan 96 is crucial for the transfer activity of the protein and tryptophan 142 is an important part of the proteins membrane interacting domain. Further, we varied the composition of the used lipid vesicles and gained information on the effect of membrane properties on GLTP activity. GLTP prefers to interact with more tightly packed membranes, although GLTP-mediated transfer is faster from more fluid membranes. This technique is very useful for the study of membrane-protein interactions and lipid-transfer rates and it can easily be adapted to other membrane-interacting proteins.
机译:糖脂转移蛋白(GLTP)是一种能够结合和转移糖脂的蛋白。 GLTP是胞质的,它可以通过其FFAT样(酸性区域中的两个苯丙氨酸)基序与内质网表面上的蛋白质相互作用。以前使用GLTP进行的体外研究主要集中在蛋白质的完全转移反应上,即结合和随后将糖脂从供体膜上去除,通过水环境转移以及糖脂最终释放到受体膜上。 。现在,我们使用双层囊泡和表面等离振子共振光谱,首次使用完全无标记的技术分析了GLTP的结合和脂质去除能力。该技术专注于GLTP介导的转移的初始步骤,可以更精确地确定影响这些步骤的参数。通过检查特定GLTP色氨酸突变体的糖脂转移能力,我们将新方法用于GLTP的详细结构功能研究。色氨酸96对于蛋白质的转移活性至关重要,而色氨酸142是蛋白质膜相互作用域的重要部分。此外,我们改变了所用脂质囊泡的组成,并获得了有关膜性质对GLTP活性影响的信息。 GLTP倾向于与更紧密堆积的膜相互作用,尽管GLTP介导的转移从更多的流体膜中更快。该技术对于研究膜蛋白相互作用和脂质转移速率非常有用,并且可以很容易地适应于其他与膜相互作用的蛋白。

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