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糖蛋白的高效毛细管电泳:利用电渗流修饰剂分析微观异质性

High-performance capillary electrophoresis of glycoproteins: the use of modifiers of electroosmotic flow for analysis of microheterogeneity.

作者信息

Landers J P, Oda R P, Madden B J, Spelsberg T C

机构信息

Department of Biochemistry and Molecular Biology, Mayo Clinic/Foundation, Rochester, Minnesota 55905.

出版信息

Anal Biochem. 1992 Aug 15;205(1):115-24. doi: 10.1016/0003-2697(92)90587-w.

Abstract

High-performance capillary electrophoresis (HPCE) is rapidly gaining acceptance as an analytical tool for the study of biological macromolecules. In the present study, the utility of HPCE for separation of glycoproteins is highlighted using a pure ovalbumin preparation. Ovalbumin, the 43-kDa glycoprotein of avian egg white, is known to be heterogeneous in nature with at least nine different carbohydrate structures having been identified on the single Asn residue. HPCE separation in an 87-cm capillary containing borate buffer and 1 mM putrescine resolves five major protein peaks in less than 30 min under nondenaturing conditions. This effect appears to be specific to glycoproteins since analysis of the nonglycosylated protein carbonic anhydrase under the same conditions showed no enhanced separation. The sodium borate buffer is proposed to play a key role in the separation by preferentially complexing with the diols of specific carbohydrate moieties on ovalbumin. Addition of putrescine enhances resolution by slowing bulk flow through the capillary and allowing electrophoretic separation of what is deduced to be closely related glycoforms of ovalbumin. Dephosphorylation of the ovalbumin with either calf intestinal alkaline phosphatase or potato acid phosphatase results in a shift of all peaks to a more rapid migration time and is consistent with a loss of negative charge. This suggests that all major ovalbumin isoforms are phosphorylated to the same degree and that heterology among ovalbumin isoforms resides solely in the carbohydrate structure. The enhanced resolution obtained with the employment of longer capillaries and modifiers of endo-osmotic flow was not restricted to ovalbumin since partial resolution of pepsin isoforms was observed under the same conditions.

摘要

高效毛细管电泳(HPCE)作为一种用于研究生物大分子的分析工具正迅速得到认可。在本研究中,使用纯卵清蛋白制剂突出了HPCE在糖蛋白分离中的实用性。卵清蛋白是禽蛋清中的43 kDa糖蛋白,已知其本质上具有异质性,在单个天冬酰胺残基上已鉴定出至少九种不同的碳水化合物结构。在含有硼酸盐缓冲液和1 mM腐胺的87 cm毛细管中进行HPCE分离,在非变性条件下不到30分钟就能分离出五个主要蛋白峰。这种效应似乎对糖蛋白具有特异性,因为在相同条件下对非糖基化蛋白碳酸酐酶的分析显示没有增强的分离效果。有人提出硼酸钠缓冲液通过优先与卵清蛋白上特定碳水化合物部分的二醇络合在分离中起关键作用。添加腐胺通过减缓通过毛细管的总体流速并允许对推断为卵清蛋白密切相关糖型进行电泳分离来提高分辨率。用小牛肠碱性磷酸酶或马铃薯酸性磷酸酶对卵清蛋白进行去磷酸化会导致所有峰向更快的迁移时间移动,这与负电荷的丧失一致。这表明所有主要的卵清蛋白同工型磷酸化程度相同,并且卵清蛋白同工型之间的异质性仅存在于碳水化合物结构中。使用更长的毛细管和内渗流调节剂获得的分辨率提高并不限于卵清蛋白,因为在相同条件下观察到了胃蛋白酶同工型的部分分离。

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