Label-Free Glycoprofiling with Multiplex Surface Plasmon Resonance: A Tool To Quantify Sialylation of Erythropoietin

被引:16
作者
Geuijen, Karin P. M. [1 ,2 ]
Halim, Liem A. [3 ]
Schellekens, Huub [3 ]
Schasfoort, Richard B. [4 ,5 ]
Wijffels, Rene H. [2 ,6 ]
Eppink, Michel H. [1 ,2 ]
机构
[1] Synthon Biopharmaceut BV, Downstream Proc, NL-6503 GN Nijmegen, Netherlands
[2] Wageningen Univ, Bioproc Engn, NL-6700 AA Wageningen, Netherlands
[3] Univ Utrecht, Utrecht Inst Pharmaceut Sci, Dept Pharmaceut, NL-3584 CG Utrecht, Netherlands
[4] IBIS Technol, NL-7521 PR Enschede, Netherlands
[5] Univ Twente, Fac Sci & Technol, MIRA Inst, Med Cell Biophys Grp, NL-7500 AE Enschede, Netherlands
[6] Univ Nordland, Fac Biosci & Aquaculture, N-8049 Bodo, Norway
关键词
LIQUID CHROMATOGRAPHY/MASS SPECTROMETRY; RECOMBINANT-HUMAN-ERYTHROPOIETIN; LECTIN MICROARRAY; BIOLOGICAL FUNCTION; REAL-TIME; CHO-CELLS; GLYCOSYLATION; CARBOHYDRATE; GLYCOPROTEINS; HEMOGLOBIN;
D O I
10.1021/acs.analchem.5b00870
中图分类号
O65 [分析化学];
学科分类号
070302 ; 081704 ;
摘要
Protein glycosylation is among the most common and well-defined post-translational modifications due to its vital role in protein function. Monitoring variation in glycosylation is necessary for producing more effective therapeutic proteins. Glycans attached to glycoproteins interact highly specific with lectins, natural carbohydrate-binding proteins, which property is used in the current label-free methodology. We have established a lectin microarray for label-free detection of lectin-carbohydrate interactions allowing us to study protein glycosylation directly on unmodified glycoproteins. The method enables simultaneous measurement of up to 96 lectin-carbohydrate interactions on a multiplex surface plasmon resonance imaging platform within 20 min. Specificity determination of lectins succeeded by analysis of neoglycoproteins and enzymatically remodeled glycoproteins to verify carbohydrate binding. We demonstrated the possibilities for glycosylation fingerprinting by comparing different Erythropoietin sources without the need for any sample pretreatment and we were able to accurately quantify relative sialylation levels of Erythropoietin.
引用
收藏
页码:8115 / 8122
页数:8
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