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多肽键及由此产生的结构特征作为洛瑞酚反应中强大的显色因子。对一种不含洛瑞酚反应性氨基酸的糖蛋白及其去唾液酸化和去糖基化产物的研究。

Polypeptide linkages and resulting structural features as powerful chromogenic factors in the Lowry phenol reaction. Studies on a glycoprotein containing no Lowry phenol-reactive amino acids and on its desialylated and deglycosylated products.

作者信息

Wu A M, Wu J C, Herp A

出版信息

Biochem J. 1978 Oct 1;175(1):47-51. doi: 10.1042/bj1750047.

Abstract

With bovine serum albumin as the reference standard, the armadillo salivary-gland glycoprotein, although containing no chromogenic amino acids and only small amounts of colour-yielding peptides [Chou & Goldstein (1960) Biochem. J. 75, 100-115], is highly reactive in the Lowry phenol protein assay [Wu & Pigman (1977) Biochem. J. 161, 37-47]. After desialylation and Smith degradation of the glycoprotein, the Lowry phenol value increased by 13 and 30% respectively, which suggests that both sialic acid and N-acetylhexosamine exert shielding effects in this reaction. Acid hydrolysis for 30 min decreased the Lowry phenol value by more than 45%, which indicates that the peptide linkages and steric features affect the Lowry phenol reactivity. After hydrolysis for up to 6h, the remaining Lowry phenol value of the partially hydrolysed core protein paralleled the amount of unhydrolysed peptides, inferring that both acid-sensitive and acid-resistant chromophoric peptides are fairly evenly distributed along the whole polypeptide chain. As with bovine serum albumin, more than 80% of the colour yield obtained in the Lowry phenol assay with this glycoprotein is Cu2+-dependent.

摘要

以牛血清白蛋白作为参比标准,犰狳唾液腺糖蛋白尽管不含生色氨基酸且仅含有少量呈色肽[Chou和Goldstein(1960年)《生物化学杂志》75卷,100 - 115页],但在洛瑞酚蛋白测定法[Wu和Pigman(1977年)《生物化学杂志》161卷,37 - 47页]中具有高反应性。对该糖蛋白进行脱唾液酸处理和史密斯降解后,洛瑞酚值分别增加了13%和30%,这表明唾液酸和N - 乙酰己糖胺在该反应中均发挥屏蔽作用。30分钟的酸水解使洛瑞酚值降低超过45%,这表明肽键和空间特征会影响洛瑞酚反应性。水解长达6小时后,部分水解的核心蛋白剩余的洛瑞酚值与未水解肽的量平行,这推断酸敏感和酸抗性发色肽在整个多肽链上分布相当均匀。与牛血清白蛋白一样,用该糖蛋白进行洛瑞酚测定所获得的颜色产量中超过80%依赖于Cu2 + 。

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On the chemical basis of the Lowry protein determination.基于洛瑞蛋白质测定法的化学原理。
Anal Biochem. 1985 Nov 1;150(2):278-87. doi: 10.1016/0003-2697(85)90511-1.

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