Isolation of a Calcium-binding Peptide from Chlorella Protein Hydrolysates

S. Jeon, Ji‐hye Lee, K. Song
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引用次数: 13

Abstract

To isolate a calcium-binding peptide from chlorella protein hydrolysates, chlorella protein was extracted and hydrolyzed using Flavourzyme, a commercial protease. The degree of hydrolysis and calcium-binding capacity were determined using trinitrobenzenesulfonic acid and orthophenanthroline methods, respectively. The enzymatic hydrolysis of chlorella protein for 6 hr was sufficient for the preparation of chlorella protein hydrolysates. The hydrolysates of chlorella protein were then ultra-filtered under 5 kDa as molecular weight. The membrane-filtered solution was fractionated using ion exchange, reverse phase, normal phase chromatography, and fast protein liquid chromatography to identify a calcium-binding peptide. The purified calcium-binding peptide had a calcium binding activity of 0.166 mM and was determined to be 700.48 Da as molecular weight, and partially identified as a peptide containing Asn-Ser-Gly-Cys based on liquid chromatography/electrospray ionization tandem mass spectrum.
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从小球藻蛋白水解物中分离一种钙结合肽
为了从小球藻蛋白水解物中分离钙结合肽,利用商业蛋白酶Flavourzyme对小球藻蛋白进行了提取和水解。分别用三硝基苯磺酸法和正邻菲罗啉法测定水解度和钙结合能力。酶解小球藻蛋白6小时足以制备小球藻蛋白水解产物。将小球藻蛋白水解产物以5 kDa的分子量进行超滤。通过离子交换、反相色谱、正相色谱和快速蛋白液相色谱对膜过滤后的溶液进行分离,鉴定钙结合肽。纯化的钙结合肽的钙结合活性为0.166 mM,分子量为700.48 Da,通过液相色谱/电喷雾串联质谱分析,部分鉴定为含有Asn-Ser-Gly-Cys的肽。
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