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表面活性剂对从头蛋白质组分析中累积胰蛋白酶活性的影响。

Impact of Surfactants on Cumulative Trypsin Activity in Bottom-Up Proteome Analysis.

机构信息

Department of Chemistry, Dalhousie University, Halifax, Nova Scotia B3H 4R2, Canada.

Allumiqs Corporation, Halifax, Nova Scotia B3H 0A8, Canada.

出版信息

J Proteome Res. 2024 Aug 2;23(8):3542-3551. doi: 10.1021/acs.jproteome.4c00162. Epub 2024 Jul 7.

Abstract

Trypsin digestion plays a pivotal role in successful bottom-up peptide characterization and quantitation. While denaturants are often incorporated to enhance protein solubility, surfactants are recognized to inhibit enzyme activity. However, several reports have suggested that incorporating surfactants or other solvent additives may enhance digestion and MS detection. Here, we assess the impacts of ionic surfactants on cumulative trypsin activity and subsequently evaluate the total digestion efficiency of a proteome mixture by quantitative MS. Although low surfactant concentrations, such as 0.01% SDS or 0.2% SDC, significantly enhanced the initial trypsin activity (by 14 or 42%, respectively), time course assays revealed accelerated enzyme deactivation, evident by 10- or 40-fold reductions in trypsin activity half-life at these respective surfactant concentrations. Despite enhanced initial tryptic activity, quantitative MS analysis of a common liver proteome extract, digested with various surfactants (0.01 or 0.1% SDS, 0.5% SDC), consistently revealed decreased peptide counts and signal intensity, indicative of a lower digestion efficiency compared to a nonsurfactant control. Furthermore, including detergents for digestion did not improve the detection of membrane proteins, nor hydrophobic peptides. These results stress the importance of assessing cumulative enzyme activity when optimizing the digestion of a proteome mixture, particularly in the presence of denaturants.

摘要

胰蛋白酶消化在成功进行自上而下的肽特征分析和定量中起着关键作用。虽然经常加入变性剂来提高蛋白质的溶解度,但表面活性剂被认为会抑制酶的活性。然而,有几项报道表明,加入表面活性剂或其他溶剂添加剂可能会增强消化和 MS 检测。在这里,我们评估了离子型表面活性剂对胰蛋白酶累积活性的影响,然后通过定量 MS 评估蛋白质混合物的总消化效率。虽然低浓度的表面活性剂,如 0.01% SDS 或 0.2% SDC,显著增强了初始胰蛋白酶活性(分别提高了 14%或 42%),但时程测定显示,酶的失活加速,在这些相应的表面活性剂浓度下,胰蛋白酶活性半衰期分别降低了 10 倍或 40 倍。尽管初始胰蛋白酶活性增强,但对不同表面活性剂(0.01 或 0.1% SDS、0.5% SDC)消化的常见肝蛋白质组提取物进行定量 MS 分析,发现肽计数和信号强度降低,表明与非表面活性剂对照相比,消化效率较低。此外,在消化中加入去污剂并不能改善膜蛋白或疏水性肽的检测。这些结果强调了在优化蛋白质混合物消化时评估累积酶活性的重要性,特别是在存在变性剂的情况下。

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