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Label-Free Proteomic Analysis of Wheat Gluten Proteins and Their Immunoreactivity to ELISA Antibodies

机译:小麦麸质蛋白的无标记蛋白质组学分析及其对ELISA抗体的免疫反应性

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摘要

Enzyme-linked immunosorbent assay (ELISA) methods are currently the most widely used for gluten quantification. However, the lack of comparable measurements among commercial kits has caused much concern. Here, we studied the immunoreactivity of five commercial ELISA kits to wheat gluten fractionated by reversed-phase high-performance liquid chromatography and identified the proteins and peptides in the resulting fractions by mass spectrometry to understand the extent to which these may be contributing to the lack of comparability. The investigated monoclonal antibodies clearly demonstrated divergent responses to the fractioned wheat gluten proteins and sometimes to their initial intended targets. To make comparable gluten measurements a reality, the analytical measurement community requires a set of agreed peptide markers, known conversion factors from these markers to total gluten content, and appropriately characterized (certified) reference materials representative of gluten.
机译:酶联免疫吸附测定(ELISA)方法目前是最广泛用于麸质量化。 然而,商业套件中缺乏可比性测量引起了很大的关注。 在这里,我们研究了五种商业ELISA试剂盒的免疫反应性,通过反相高效液相色谱法分馏出小麦蛋白质,并通过质谱法鉴定所得级分中所得级分中的蛋白质和肽,以了解这些可能导致缺乏的程度 可比性。 研究的单克隆抗体清楚地证明了对分馏的小麦麸质蛋白的发散反应,有时是其初始预期靶标。 为了使相当的麸质测量现实,分析测量界需要一组商定的肽标记物,从这些标志物中已知的转化因子与总谷蛋白含量的总含量,并且具有适当的(认证的)参考资料代表麸质。

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    《Cereal Chemistry》 |2017年第5期|共7页
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  • 正文语种 eng
  • 中图分类 农业化学;
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