Mass Spectrometry of Putrescine, Spermidine, and Spermine Covalently Attached to Francisella tularensis Universal Stress Protein and Bovine Albumin.

IF 3.4 Q2 BIOCHEMICAL RESEARCH METHODS Biochemistry Research International Pub Date : 2024-02-05 eCollection Date: 2024-01-01 DOI:10.1155/2024/7120208
Lawrence M Schopfer, Benjamin Girardo, Oksana Lockridge, Marilynn A Larson
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Abstract

Bacterial and mammalian cells are rich in putrescine, spermidine, and spermine. Polyamines are required for optimum fitness, but the biological function of these small aliphatic compounds has only been partially revealed. Known functions of polyamines include interaction with nucleic acids that alters gene expression and with proteins that modulate activity. Although polyamines can be incorporated into proteins, very few naturally occurring polyaminated proteins have been identified, which is due in part to the difficulty in detecting these adducts. In the current study, bovine albumin and the recombinant universal stress protein from Francisella tularensis were used as models for mass spectrometry analysis of polyaminated proteins. The proteins were covalently bound to putrescine, spermidine, or spermine by the action of carbodiimide or microbial transglutaminase. Tryptic peptides, subjected to liquid chromatography tandem mass spectrometry (LC-MS/MS), were identified using Protein Prospector software. We describe the search parameters for identifying polyaminated peptides and show MS/MS spectra for adducts with putrescine, spermidine, and spermine. Manual evaluation led us to recognize signature ions for polyamine adducts on aspartate, glutamate, and glutamine, as well as neutral loss from putrescine, spermidine, and spermine during the fragmentation process. Mechanisms for the formation of signature ions and neutral loss are presented. Manual evaluation identified a false-positive adduct that had formed during trypsinolysis and resulted in peptide sequence rearrangement. Another false positive initially appeared to be a 71 kDa putrescine adduct on a cysteine residue. However, it was an acrylamide adduct on cysteine for a sample extracted from a polyacrylamide gel. The information presented in this report provides guidance and serves as a model for identifying naturally occurring polyaminated proteins.

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与土拉弗氏菌通用应激蛋白和牛白蛋白共价结合的普妥瑞辛、精胺和精胺的质谱分析。
细菌和哺乳动物细胞富含腐胺、亚精胺和精胺。多胺是达到最佳体能所必需的,但这些小型脂肪族化合物的生物功能仅被部分揭示。已知的多胺功能包括与核酸相互作用改变基因表达,以及与蛋白质相互作用调节活性。虽然多胺可以掺入蛋白质中,但很少有天然存在的多胺蛋白质被发现,部分原因是难以检测这些加合物。在本研究中,牛白蛋白和土拉弗氏菌重组通用应激蛋白被用作质谱分析多胺蛋白的模型。在碳化二亚胺或微生物转谷氨酰胺酶的作用下,蛋白质与腐胺、亚精胺或精胺共价结合。使用 Protein Prospector 软件对胰蛋白酶肽进行液相色谱串联质谱(LC-MS/MS)鉴定。我们描述了识别多氨基肽的搜索参数,并展示了与腐胺、亚精胺和精胺加合物的 MS/MS 图谱。通过人工评估,我们识别出了天冬氨酸、谷氨酸和谷氨酰胺上多胺加合物的特征离子,以及在碎片化过程中腐胺、亚精胺和精胺的中性损失。介绍了特征离子和中性损失的形成机制。人工评估发现了一个假阳性加合物,它是在胰蛋白酶溶解过程中形成的,并导致肽序列重排。另一个假阳性最初似乎是半胱氨酸残基上的 71 kDa 腐胺加合物。然而,从聚丙烯酰胺凝胶中提取的样本中,它是半胱氨酸上的丙烯酰胺加合物。本报告中提供的信息为鉴定天然存在的多胺蛋白提供了指导和模型。
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来源期刊
Biochemistry Research International
Biochemistry Research International BIOCHEMICAL RESEARCH METHODS-
CiteScore
6.30
自引率
0.00%
发文量
27
审稿时长
14 weeks
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