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通过高压液相色谱法分析人免疫球蛋白D的蛋白水解裂解机制、速率和位点。

Analysis of the mechanism, rate, and sites of proteolytic cleavage of human immunoglobulin D by high-pressure liquid chromatography.

作者信息

Ishioka N, Takahashi N, Putnam F W

出版信息

Proc Natl Acad Sci U S A. 1987 Jan;84(1):61-5. doi: 10.1073/pnas.84.1.61.

Abstract

The high susceptibility of human immunoglobulin D to proteolytic degradation affects its biological function, metabolism, and immunoassay. High-pressure liquid chromatography was used to investigate the mechanism and rate of limited proteolytic cleavage of IgD and also to identify, isolate, and quantify the reaction products. Within 1 to 5 min, tryptic digestion of native IgD almost quantitatively yields a labile Fab fragment, a stable Fc fragment, and a highly charged peptide derived from the hinge region. A galactosamine-rich glycopeptide from the hinge region increases inversely as the Fab is largely degraded to a series of peptides within 1 hr. In contrast, the Fc and the high-charge peptide resist proteolysis for more than 24 hr. The initial sites of cleavage of IgD occur in the hinge region at exposed secondary structures predicted to be beta-turns. Concomitant with removal of the galactosamine-rich glycopeptide at its carboxyl terminus, the Fd fragment is rapidly and rather randomly degraded, but the light chain is somewhat more resistant than the Fd section of the delta heavy chain. This study of the rapid rate of proteolysis of IgD explains the rarity with which intact IgD is found in human sera. It also raises questions about immunoassay of IgD, which is usually measured with antisera against Fc. In vivo, proteolytic cleavage initiates the catabolism of circulating IgD and also affects the role and fate of IgD as an antigen receptor on the B-cell membrane.

摘要

人免疫球蛋白D(IgD)对蛋白水解降解的高敏感性影响其生物学功能、代谢及免疫测定。采用高压液相色谱法研究IgD有限蛋白水解切割的机制和速率,并鉴定、分离和定量反应产物。在1至5分钟内,天然IgD经胰蛋白酶消化几乎定量产生一个不稳定的Fab片段、一个稳定的Fc片段以及一个源自铰链区的高电荷肽段。来自铰链区的富含半乳糖胺的糖肽随着Fab在1小时内大量降解为一系列肽段而呈反比增加。相比之下,Fc和高电荷肽段在超过24小时内抵抗蛋白水解。IgD的初始切割位点发生在铰链区预测为β-转角的暴露二级结构处。随着富含半乳糖胺的糖肽在其羧基末端被去除,Fd片段迅速且相当随机地降解,但轻链比δ重链的Fd部分更具抗性。对IgD蛋白水解快速速率的这项研究解释了在人血清中完整IgD罕见的原因。它还对通常用抗Fc抗血清进行测量的IgD免疫测定提出了疑问。在体内,蛋白水解切割启动循环IgD的分解代谢,也影响IgD作为B细胞膜上抗原受体的作用和命运。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/39a6/304141/04baf279e6b5/pnas00266-0079-a.jpg

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