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通过质谱法对乳糜泻免疫原性表位进行无标记靶向检测和定量分析。

Label free targeted detection and quantification of celiac disease immunogenic epitopes by mass spectrometry.

作者信息

van den Broeck Hetty C, Cordewener Jan H G, Nessen Merel A, America Antoine H P, van der Meer Ingrid M

机构信息

Wageningen UR, Plant Research International, PO Box 16, 6700 AA Wageningen, The Netherlands.

Wageningen UR, Plant Research International, PO Box 16, 6700 AA Wageningen, The Netherlands.

出版信息

J Chromatogr A. 2015 Apr 24;1391:60-71. doi: 10.1016/j.chroma.2015.02.070. Epub 2015 Mar 5.

Abstract

Celiac disease (CD) is a food-related disease caused by certain gluten peptides containing T-cell stimulating epitopes from wheat, rye, and barley. CD-patients have to maintain a gluten-free diet and are therefore dependent on reliable testing and labeling of gluten-free products. So far, the R5-ELISA is the approved method to detect if food products can be labeled gluten-free. Because the R5-ELISA detects gluten in general, there is a demand for an improved detection method that quantifies specifically CD-epitopes. Therefore, we developed a new method for detection and quantification of CD-epitopes, based on liquid chromatography (LC) coupled to mass spectrometry (MS) in multiple reaction monitoring (MRM) mode. This method enables targeted label free comparative analysis of the gluten proteins present in different wheat varieties and species, and in wheat-based food products. We have tested our method by analyzing several wheat varieties that vary in CD-epitope content, as was shown before using immunoblotting and specific monoclonal antibodies. The results showed that a modern bread wheat variety Toronto contained the highest amounts of CD immunogenic peptides compared with the older bread wheat variety Minaret and the tetraploid wheat variety Dibillik Sinde. Our developed method can detect quantitatively and simultaneously multiple specific CD-epitopes in a high throughput manner.

摘要

乳糜泻(CD)是一种与食物相关的疾病,由含有来自小麦、黑麦和大麦的T细胞刺激表位的某些麸质肽引起。CD患者必须保持无麸质饮食,因此依赖于无麸质产品的可靠检测和标签。到目前为止,R5-ELISA是检测食品是否可标注为无麸质的认可方法。由于R5-ELISA一般检测麸质,因此需要一种改进的检测方法来特异性定量CD表位。因此,我们开发了一种基于液相色谱(LC)与多反应监测(MRM)模式下的质谱(MS)联用的CD表位检测和定量新方法。该方法能够对不同小麦品种和物种以及小麦基食品中存在的麸质蛋白进行靶向无标记比较分析。我们通过分析几个CD表位含量不同的小麦品种测试了我们的方法,之前使用免疫印迹和特异性单克隆抗体已证明了这一点。结果表明,与较老的面包小麦品种尖塔和四倍体小麦品种迪比利克·辛德相比,现代面包小麦品种多伦多含有最高量的CD免疫原性肽。我们开发的方法能够以高通量方式同时定量检测多种特定的CD表位。

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