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Preparation and Characterization of Avenin-Enriched Oat Protein by Chill Precipitation for Feeding Trials in Celiac Disease

机译:冷沉淀法制备乳糜丰富的燕麦蛋白的制备及表征

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摘要

The safety of oats for people with celiac disease remains unresolved. While oats have attractive nutritional properties that can improve the quality and palatability of the restrictive, low fiber gluten-free diet, rigorous feeding studies to address their safety in celiac disease are needed. Assessing the oat prolamin proteins (avenins) in isolation and controlling for gluten contamination and other oat components such as fiber that can cause non-specific effects and symptoms is crucial. Further, the avenin should contain all reported immunogenic T cell epitopes, and be deliverable at a dose that enables biological responses to be correlated with clinical effects. To date, isolation of a purified food-grade avenin in sufficient quantities for feeding studies has not been feasible. Here, we report a new gluten isolation technique that enabled 2 kg of avenin to be extracted from 400 kg of wheat-free oats under rigorous gluten-free and food grade conditions. The extract consisted of 85% protein of which 96% of the protein was avenin. The concentration of starch (1.8% dry weight), β-glucan (0.2% dry weight), and free sugars (1.8% dry weight) were all low in the final avenin preparation. Other sugars including oligosaccharides, small fructans, and other complex sugars were also low at 2.8% dry weight. Liquid chromatography tandem mass spectrometry (LC-MS/MS) analysis of the proteins in these preparations showed they consisted only of oat proteins and were uncontaminated by gluten containing cereals including wheat, barley or rye. Proteomic analysis of the avenin enriched samples detected more avenin subtypes and fewer other proteins compared to samples obtained using other extraction procedures. The identified proteins represented five main groups, four containing known immune-stimulatory avenin peptides. All five groups were identified in the 50% (v/v) ethanol extract however the group harboring the epitope DQ2.5-ave-1b was less represented. The avenin-enriched protein fractions were quantitatively collected by reversed phase HPLC and analyzed by MALDI-TOF mass spectrometry. Three reverse phase HPLC peaks, representing ~40% of the protein content, were enriched in proteins containing DQ2.5-ave-1a epitope. The resultant high quality avenin will facilitate controlled and definitive feeding studies to establish the safety of oat consumption by people with celiac disease.
机译:燕麦对腹腔疾病患者的安全性尚未得到解决。燕麦具有吸引人的营养特性,可以改善限制性低纤维无麸质饮食的质量和适口性,但需要进行严格的喂养研究以解决其在乳糜泻中的安全性。隔离评估燕麦谷醇溶蛋白(avenins)并控制面筋污染和其他燕麦成分(如纤维)会导致非特异性作用和症状至关重要。此外,阿维宁应包含所有已报告的免疫原性T细胞表位,并应以使生物学反应与临床疗效相关的剂量给药。迄今为止,分离足够数量的纯化食品级avenin用于喂养研究尚不可行。在这里,我们报告了一种新的面筋分离技术,该技术能够在严格的无面筋和食品级条件下,从400公斤无麦燕麦中提取2公斤avenin。提取物由85%的蛋白质组成,其中96%的蛋白质为avenin。在最终的avenin制剂中,淀粉(干重1.8%),β-葡聚糖(干重0.2%)和游离糖(干重1.8%)的浓度均较低。其他糖包括低聚糖,小果聚糖和其他复合糖也很低,干重为2.8%。液相色谱串联质谱(LC-MS / MS)对这些制剂中蛋白质的分析表明,它们仅由燕麦蛋白质组成,未受到含麸质谷物的污染,包括小麦,大麦或黑麦。与使用其他提取程序获得的样品相比,富含avenin的样品的蛋白质组学分析检测到更多的avenin亚型和更少的其他蛋白质。鉴定出的蛋白质代表五个主要组,其中四个包含已知的免疫刺激阿维宁肽。在50%(v / v)乙醇提取物中鉴定出所有五个组,但是带有表位DQ2.5-ave-1b的组的代表较少。通过反相HPLC定量收集富Avenin的蛋白质级分,并通过MALDI-TOF质谱分析。代表蛋白质含量约40%的三个反相HPLC峰富含含有DQ2.5-ave-1a表位的蛋白质。由此产生的高质量阿维宁将有助于进行控制性和确定性的喂养研究,以建立腹腔疾病患者食用燕麦的安全性。

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