首页> 外文学位 >Chemical composition of select pecan [Carya illinoinensis (Wangenh.) K. Koch] varieties and antigenic stability of pecan proteins.
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Chemical composition of select pecan [Carya illinoinensis (Wangenh.) K. Koch] varieties and antigenic stability of pecan proteins.

机译:精选山核桃[山核桃(Wangenh。)K. Koch]品种的化学组成和山核桃蛋白的抗原稳定性。

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摘要

Chemical composition of 25 pecan varieties revealed considerable differences in moisture (2.1--6.4%), protein (6.0--11.3%), lipid (65.9--78.0%), total soluble sugars (3.3--5.3%), ash (1.2--1.8%) and tannins (0.7--2.7%) when analyzed on an edible portion basis. Pecan varieties had similar protein polypeptide profiles as revealed by SDS-PAGE, IEF, and pecan pAb based Western blotting analysis.; Both pH and ionic strength were important for pecan protein solubilization. Borate Saline Buffer (pH 8.45) was an optimum solvent for extraction of pecan proteins among the mild buffers tested. Protein solubility was minimal in pH 3--7 range and increased significantly on either side of this pH range. Increasing ionic strength from 0 to 4 M NaCl significantly improved (∼8 fold) protein solubilization. Glutelin fraction (63.6%) accounted for the major portion of the total solubilized pecan proteins followed by globulin (31.5%), prolamin (3.4%) and albumin (1.5%) respectively. The majority of the pecan polypeptides were in the MW and pI range of 12,000--66,000 Da and pH 4.0--8.3 respectively. Pecan globulins contained the most glycoprotein polypeptides. Lysine was the first limiting essential amino acid in the defatted flour, globulin, prolamin and alkaline glutelin fractions. Leucine and tryptophan were the first limiting essential amino acid in albumin and acid glutelin fractions respectively. The minimum nitrogen solubility (5.9--7.5%) at 0.25--0.75 M TCA represented the non-protein nitrogen of pecan meal.; Pecan pAb-based inhibition ELISA could detect pecan proteins as low as 32 ng/ml. The assay, however, was not suitable for specific detection of pecan in foods as it showed cross-reactivity to various tree nut and seed proteins.; Pecan contained major allergenic polypeptides in the 50--66 kDa and 16--20 kDa range when tested with human sera IgE from 15 pecan allergic subjects. Pecan globulins contributed to the majority of 50--66 kDa allergens.; ELISAs and Western blotting assays indicated that pecan proteins subjected to various thermal treatments remained antigenically stable.; Complete proteolysis and loss of antigenicity was not observed in SGF and SIF in vitro digestion studies. Western blotting of SGF digested proteins displayed several low molecular weight antigenic peptides (16--20 kDa) that were either originally present in the pecan extract or were generated by pepsin under the digestion conditions.
机译:25个山核桃品种的化学成分显示出水分(2.1--6.4%),蛋白质(6.0--11.3%),脂质(65.9--78.0%),总可溶性糖(3.3--5.3%),灰分(按食用份量分析时,单宁含量为1.2--1.8%)和单宁酸含量为(0.7--2.7%)。山核桃品种具有相似的蛋白质多肽谱,如通过SDS-PAGE,IEF和基于山核桃pAb的蛋白质印迹分析所揭示。 pH和离子强度对山核桃蛋白的溶解都很重要。硼酸盐生理盐水(pH 8.45)是在所测试的温和缓冲液中提取山核桃蛋白的最佳溶剂。蛋白质溶解度在pH 3--7范围内最小,在此pH范围的任一侧均显着增加。将离子强度从0M NaCl增加到4 M NaCl可以显着改善(约8倍)蛋白质溶解。谷蛋白部分(63.6%)占可溶性山核桃蛋白总量的主要部分,其次是球蛋白(31.5%),谷醇溶蛋白(3.4%)和白蛋白(1.5%)。大多数山核桃多肽的MW和pI分别为12,000--66,000 Da和pH 4.0--8.3。山核桃球蛋白含有最多的糖蛋白多肽。赖氨酸是脱脂面粉,球蛋白,谷醇溶蛋白和碱性谷蛋白中的第一个限制性必需氨基酸。亮氨酸和色氨酸分别是白蛋白和酸性谷蛋白部分中的第一个限制性必需氨基酸。 TCA在0.25--0.75 M时的最低氮溶解度(5.9--7.5%)表示山核桃粉中的非蛋白质氮。基于山核桃pAb的抑制ELISA可以检测低至32 ng / ml的山核桃蛋白。然而,该测定法不适用于食品中的山核桃的特异性检测,因为它显示出与各种坚果和种子蛋白质的交叉反应性。当用来自15个山核桃过敏受试者的人血清IgE测试时,山核桃包含50--66 kDa和16--20 kDa范围内的主要过敏原多肽。山核桃球蛋白占50--66 kDa过敏原的大部分。 ELISA和Western blotting分析表明,经过各种热处理的山核桃蛋白在抗原上保持稳定。在SGF和SIF体外消化研究中未观察到完全蛋白水解和抗原性丧失。 SGF消化的蛋白质的蛋白质印迹显示了几种低分子量抗原肽(16--20 kDa),这些肽最初存在于山核桃提取物中,或由胃蛋白酶在消化条件下产生。

著录项

  • 作者

    Venkatachalam, Mahesh.;

  • 作者单位

    The Florida State University.;

  • 授予单位 The Florida State University.;
  • 学科 Agriculture Food Science and Technology.
  • 学位 Ph.D.
  • 年度 2004
  • 页码 105 p.
  • 总页数 105
  • 原文格式 PDF
  • 正文语种 eng
  • 中图分类 农产品收获、加工及贮藏;
  • 关键词

  • 入库时间 2022-08-17 11:43:22

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