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Combined Approach to the Analysis of Recombinant Protein Drugs Using Hollow-Fiber Flow Field-Flow Fractionation, Mass Spectrometry, and Chemiluminescence Detection

机译:中空纤维流场-流分离,质谱法和化学发光检测相结合的重组蛋白药物分析方法

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The impurities present in recombinant protein drugs produced by large-scale refolding processes can not only affect the product safety but also interact with the expressed protein. To relate the impurity profile to conformation and functionality of the protein drug, analytical methods able not to degrade the sample components should be preferred. In this work, an urate oxidase (uricase) drug from Aspergillus flavus expressed in Saccharomyces cerevisiae, and a reagent-grade uricase from Candida sphaerica expressed in Escherichia coli, are analyzed by combining hollow-fiber flow field-flow fractionation with matrix-assisted laser desorption-ionization time-of-flight mass spectrometry (MALDI/TOFMS) and with chemiluminescence enzyme activity assay. Preliminary detection and identification of sample impurities is performed by means of conventional methods such as RP HPLC with electrospray ionization quadrupole-TOF MS and MALDI/TOFMS with SDS PAGE and 2D SDS PAGE. Results show that the recombinant uricase samples obtained from different microorganisms have different impurities and different enzymatic activity and that different uricase oligomers are present in solution.
机译:通过大规模重折叠过程生产的重组蛋白药物中存在的杂质不仅会影响产品安全性,而且还会与表达的蛋白发生相互作用。为了将杂质分布与蛋白质药物的构象和功能相关联,应优先采用不能降解样品成分的分析方法。在这项工作中,通过将中空纤维流场流分馏与基质辅助激光相结合,分析了在酿酒酵母中表达的黄曲霉的尿酸氧化酶(尿酸酶)药物和在大肠杆菌中表达的球形假丝酵母的试剂级尿酸酶。解吸电离飞行时间质谱(MALDI / TOFMS)并采用化学发光酶活性测定。样品杂质的初步检测和鉴定是通过常规方法进行的,例如带电喷雾电离四极杆-TOF MS的RP HPLC和带SDS PAGE和2D SDS PAGE的MALDI / TOFMS。结果表明,从不同微生物获得的重组尿酸酶样品具有不同的杂质和不同的酶活性,并且溶液中存在不同的尿酸酶低聚物。

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