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Multiplexed quantification of proteins adsorbed to surface-modified and non-modified microdialysis membranes

机译:吸附在表面修饰的和未修饰的微透析膜上的蛋白质的多重定量

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摘要

A simple and straightforward method for discovery and quantification of proteins adsorbed onto delicate and sensitive membrane surfaces is presented. The adsorbed proteins were enzymatically cleaved while still adsorbed onto the membranes using an on-surface enzymatic digestion (oSED). This was followed by isobaric tagging, nanoliquid chromatography, and tandem mass spectrometry. Protein adsorption on tri-block copolymer Poloxamer 407 surface-modified microdialysis (MD) membranes were compared with protein adsorption on unmodified MD membranes. Ventricular cerebrospinal fluid (vCSF) kept at 37 °C was used as sample matrix. In total, 19 proteins were quantified in two biological replicates. The surface-modified membranes adsorbed 33% less proteins than control membranes and the most abundant proteins were subunits of hemoglobin and clusterin. The adsorption of clusterin on the modified membranes was on average 36% compared to control membranes. The most common protein in vCSF, Albumin, was not identified adsorbed to the surface at all. It was also experimentally verified that oSED, in conjunction with tandem mass spectrometry can be used to quantify femtomole amounts of proteins adsorbed on limited and delicate surfaces, such as MD membranes. The method has great potential and can be used to study much more complex protein adsorption systems than previously reported.
机译:提出了一种简单直接的方法,用于发现和定量吸附在脆弱而敏感的膜表面上的蛋白质。酶解吸附的蛋白质,同时仍使用表面酶消化(oSED)吸附在膜上。然后进行等压标记,纳米液相色谱和串联质谱分析。比较了三嵌段共聚物Poloxamer 407表面修饰的微透析(MD)膜上的蛋白质吸附与未修饰的MD膜上的蛋白质吸附。保持在37°C的心室脑脊液(vCSF)作为样品基质。总共在两个生物学重复中定量了19种蛋白质。经表面修饰的膜比对照膜吸附的蛋白质少33%,并且最丰富的蛋白质是血红蛋白和簇蛋白的亚基。与对照膜相比,簇蛋白在改性膜上的吸附平均为36%。根本没有确定vCSF中最常见的蛋白白蛋白完全吸附在表面。还通过实验证明,oSED与串联质谱联用可用于量化吸附在有限且脆弱的表面(例如MD膜)上的fe的量。该方法具有巨大的潜力,可用于研究比以前报道的复杂得多的蛋白质吸附系统。

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