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通过质谱法进行碳水化合物图谱分析:一种鉴定糖蛋白中天冬酰胺连接糖的连接位点的新方法。

Carbohydrate mapping by mass spectrometry: a novel method for identifying attachment sites of Asn-linked sugars in glycoproteins.

作者信息

Carr S A, Roberts G D

出版信息

Anal Biochem. 1986 Sep;157(2):396-406. doi: 10.1016/0003-2697(86)90643-3.

Abstract

A new method is described for locating the specific sites of attachment of Asn-linked carbohydrates in glycoproteins. The molecular weights of peptides released from the glycoprotein with proteases of known specificity are determined by fast atom bombardment mass spectrometry and fitted to the known or DNA-derived sequence. Oligosaccharides attached to Asn are released either before or after proteolysis with a glycosidase, usually peptide: N-glycosidase F, an enzyme that cleaves the beta-aspartylglycosylamine linkage of all known types of Asn-linked sugars and converts the attachment-site Asn to Asp. New peaks appearing in the mass spectra after treatment with glycosidase correspond to formerly glycosylated sites. Conversely, signals which disappear after glycosidase treatment correspond to glycopeptides. The differences in mass between these sets of signals define the composition of the carbohydrate at the given site in terms of deoxyhexose, hexose, N-acetylhexosamine, and sialic acid content. The extent of glycosylation at a given site can be estimated from the ratio of the peak heights corresponding to the Asn- vs Asp-containing peptides which differ by 1 Da in mass. This rapid and sensitive (low nmol) technique is illustrated here for ribonuclease B and for tissue plasminogen activator, a multiply glycosylated glycoprotein.

摘要

本文描述了一种定位糖蛋白中天冬酰胺连接型碳水化合物特异性连接位点的新方法。用具有已知特异性的蛋白酶从糖蛋白释放的肽段,通过快原子轰击质谱法测定其分子量,并与已知序列或由DNA推导的序列进行比对。与天冬酰胺相连的寡糖在用糖苷酶进行蛋白水解之前或之后释放,通常使用肽:N-糖苷酶F,该酶能裂解所有已知类型天冬酰胺连接型糖的β-天冬氨酰糖胺键,并将连接位点的天冬酰胺转化为天冬氨酸。用糖苷酶处理后质谱中出现的新峰对应于先前糖基化的位点。相反,糖苷酶处理后消失的信号对应于糖肽。这些信号组之间的质量差异根据脱氧己糖、己糖、N-乙酰己糖胺和唾液酸含量确定给定位点碳水化合物的组成。给定位点的糖基化程度可根据质量相差1 Da的含天冬酰胺肽段与含天冬氨酸肽段的峰高比来估算。本文以核糖核酸酶B和组织纤溶酶原激活剂(一种多重糖基化的糖蛋白)为例说明了这种快速且灵敏(低纳摩尔级)的技术。

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