An optimised method to isotopically label pure synthetic peptides ‘in-house’ for absolute quantification in bottom-up proteomics

IF 1.8 3区 化学 Q4 BIOCHEMICAL RESEARCH METHODS Rapid Communications in Mass Spectrometry Pub Date : 2024-09-17 DOI:10.1002/rcm.9892
Nikita Bhakta, Colleen B. Maxwell, Shimon Atunde, Jatinderpal K. Sandhu, Oliver C. Slingsby, Emer M. Brady, Donald J. L. Jones, Leong L. Ng
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Abstract

Rationale

Heavy-labelled internal standards increasingly represent the gold standard for absolute quantitation in mass spectrometry (MS)-based bottom-up proteomics. The biggest drawbacks of using these standards are that they have high costs and lengthy lead times.

Methods

We describe an efficient, low-cost optimised method to enable ‘in-house’ heavy labelling of synthetic tryptic peptides for absolute quantification using tandem LC-MS/MS mass spectrometry. Our methodology uses 18O water in a trypsin-catalysed oxygen exchange reaction at the carboxyl terminus with the overall aim of reducing the costs and lead time associated with sourcing heavy standards from commercial vendors.

Results

Step-by-step instructions are provided on how to execute this protocol with high-throughput adaptations utilising a 96-well plate and a liquid-handling robot. Detailed notes on experimental setup, tips for troubleshooting and suggested improvements to maximise labelling efficiencies are highlighted to achieve the best results. Under optimum conditions, labelling efficiencies of peptides can reach from 95% to 100%.

Conclusions

The application of the ‘in-house’ labelled standards in generating calibration curves to quantify endogenous peptide concentrations is just as effective as using the synthetically sourced standards while also having great cost reduction implications as well as saving time spent waiting for peptides to arrive. The protocol is highly adaptable and can be customized to fit the specific setup of any laboratory, maximizing achievable labelling efficiencies.

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内部 "同位素标记纯合成肽的优化方法,用于自下而上蛋白质组学的绝对定量分析
理论依据 在基于质谱(MS)的自下而上蛋白质组学研究中,重标记内标日益成为绝对定量的黄金标准。使用这些标准的最大缺点是成本高、周期长。 方法 我们介绍了一种高效、低成本的优化方法,可对合成胰蛋白酶肽进行 "内部 "重标记,以便使用串联 LC-MS/MS 质谱进行绝对定量。我们的方法在羧基末端的胰蛋白酶催化的氧交换反应中使用 18O 水,总体目标是降低成本,缩短从商业供应商处采购重标准物质所需的时间。 结果 逐步说明了如何利用 96 孔板和液体处理机器人进行高通量调整来执行该方案。详细说明了实验设置、故障排除技巧和改进建议,以最大限度地提高标记效率,从而获得最佳结果。在最佳条件下,多肽的标记效率可达 95% 至 100%。 结论 应用 "内部 "标记的标准品生成校准曲线来量化内源性肽的浓度,与使用合成标准品一样有效,同时还能大大降低成本,节省等待肽到达的时间。该方案适应性强,可根据任何实验室的具体设置进行定制,最大限度地提高可实现的标记效率。
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来源期刊
CiteScore
4.10
自引率
5.00%
发文量
219
审稿时长
2.6 months
期刊介绍: Rapid Communications in Mass Spectrometry is a journal whose aim is the rapid publication of original research results and ideas on all aspects of the science of gas-phase ions; it covers all the associated scientific disciplines. There is no formal limit on paper length ("rapid" is not synonymous with "brief"), but papers should be of a length that is commensurate with the importance and complexity of the results being reported. Contributions may be theoretical or practical in nature; they may deal with methods, techniques and applications, or with the interpretation of results; they may cover any area in science that depends directly on measurements made upon gaseous ions or that is associated with such measurements.
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