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磷脂酶D在没有去污剂的情况下可水解磷脂酰胆碱的短链类似物。

Phospholipase D hydrolyzes short-chain analogs of phosphatidylcholine in the absence of detergent.

作者信息

Davis L L, Maglio J J, Horwitz J

机构信息

MCP Hahnemann School of Medicine, Allegheny University of the Health Sciences, Philadelphia, Pennsylvania 19129, USA.

出版信息

Lipids. 1998 Feb;33(2):223-7. doi: 10.1007/s11745-998-0199-5.

Abstract

Phospholipase D is an important enzyme in signal transduction in neuronal tissue. A variety of assays have been used to measure phospholipase D activity in vitro. The most typical measure of phospholipase D activity is the production of phosphatidylethanol in the presence of ethanol. Phosphatidylethanol is a product of transphosphatidylation activity that is considered a unique property of phospholipase D. To support transphosphatidylation activity, high concentrations of ethanol may be required. Furthermore, most assays in the literature utilize a detergent. These extreme conditions, detergent and ethanol, may alter phospholipase D and hinder the study of its regulation. In this manuscript we describe an assay that eliminates these potentially confounding conditions. It utilizes high specific activity [3H]butanol as a nucleophilic receptor. This eliminates the need for high concentrations of alcohol. The substrate is an analog of phosphatidylcholine that contains short-chain fatty acids, 1,2-dioctanoyl-sn-glycero-3-phosphocholine. Phospholipase D readily hydrolyzes this substrate in the absence of detergent. This novel assay should be useful in the further characterization of phospholipase D.

摘要

磷脂酶D是神经组织信号转导中的一种重要酶。已使用多种测定方法在体外测量磷脂酶D的活性。磷脂酶D活性最典型的测量方法是在乙醇存在下产生磷脂酰乙醇。磷脂酰乙醇是转磷脂酰基化活性的产物,被认为是磷脂酶D的独特特性。为了支持转磷脂酰基化活性,可能需要高浓度的乙醇。此外,文献中的大多数测定方法都使用了去污剂。去污剂和乙醇这些极端条件可能会改变磷脂酶D并阻碍对其调节的研究。在本手稿中,我们描述了一种消除这些潜在混杂条件的测定方法。它利用高比活性的[3H]丁醇作为亲核受体。这消除了对高浓度酒精的需求。底物是含有短链脂肪酸的磷脂酰胆碱类似物,1,2-二辛酰基-sn-甘油-3-磷酸胆碱。磷脂酶D在没有去污剂的情况下很容易水解这种底物。这种新颖的测定方法应该有助于进一步表征磷脂酶D。

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