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使用基于电捕获分离的质谱法鉴定膜蛋白,作为二维分级分离系统的一部分。

Membrane protein identifications by mass spectrometry using electrocapture-based separation as part of a two-dimensional fractionation system.

作者信息

Astorga-Wells Juan, Tryggvason Sam, Vollmer Susanne, Alvelius Gunvor, Palmberg Carina, Jörnvall Hans

机构信息

Department of Medical Biochemistry and Biophysics, Karolinska Instituttet, SE-171 77 Stockholm, Sweden.

出版信息

Anal Biochem. 2008 Oct 1;381(1):33-42. doi: 10.1016/j.ab.2008.06.031. Epub 2008 Jun 27.

Abstract

A two-dimensional (2D) separation method was used to decrease sample complexity in analysis of tryptic peptides from glomerular membrane proteins by tandem mass spectrometry (MS/MS). The first dimension was carried out by electrocapture (EC), which fractionates peptides according to electrophoretic mobility. The second dimension was reverse-phase liquid chromatography (RP-LC), in which EC fractions were further separated and analyzed online by MS/MS. Using this methodology, we now identify 102 glomerular proteins (57 membrane proteins). Many peptides were possible to observe and select for MS/MS only using the 2D approach. Others were detectable in both one-dimensional (1D, without the EC step) and 2D experiments but were selectable for sequence analysis only from the 2D separations because the decrease in complexity then gives time for the mass analyzer to select the peptide and switch to the MS/MS mode. A minority of the peptides were detectable only in the 1D mode (presumably because of handling losses), but at the end this did not decrease the number of proteins identified by the 2D separation. After a database search, the combination of EC and RP-LC MS/MS versus a 1D RP-LC MS/MS separation resulted in a threefold increase in the number of proteins identified and improved the sequence coverage in the identifications, bringing our proteome-identified glomerular proteins to 282.

摘要

采用二维(2D)分离方法来降低通过串联质谱(MS/MS)分析肾小球膜蛋白胰蛋白酶肽段时的样品复杂性。第一维通过电捕获(EC)进行,它根据电泳迁移率对肽段进行分级分离。第二维是反相液相色谱(RP-LC),其中EC分级分离物通过MS/MS进一步在线分离和分析。使用这种方法,我们现在鉴定出102种肾小球蛋白(57种膜蛋白)。仅使用二维方法就可以观察到许多肽段并选择用于MS/MS。其他肽段在一维(1D,无EC步骤)和二维实验中均可检测到,但仅从二维分离中可选择用于序列分析,因为复杂性的降低为质量分析器选择肽段并切换到MS/MS模式提供了时间。少数肽段仅在一维模式下可检测到(可能是由于操作损失),但最终这并未减少通过二维分离鉴定出的蛋白数量。经过数据库搜索,EC和RP-LC MS/MS与一维RP-LC MS/MS分离相结合,使鉴定出的蛋白数量增加了三倍,并提高了鉴定中的序列覆盖率,使我们通过蛋白质组学鉴定出的肾小球蛋白达到282种。

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