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Glu-C,一种用于基于IgG的抗体生物治疗药物定量液相色谱-串联质谱分析的替代消化酶。

Glu-C, an alternative digestive enzyme for the quantitative LC-MS/MS analysis of an IgG-based antibody biotherapeutic.

作者信息

Hansen Kjetil, Szarka Szabolcs, Escoffier Emilie, Berthet Amandine, Venet Joris, Collet-Brose Justine, Hepburn Sophie, Wright Michael, Wheller Robert, Nelson Robert, Kay Richard G

机构信息

LGC, Newmarket Road, Fordham, Cambridgeshire, CB7 5WW, UK.

Novimmune SA, 1228 Plan-les-Ouates, Geneva, Switzerland.

出版信息

Bioanalysis. 2018 Jul 1;10(13):997-1007. doi: 10.4155/bio-2017-0259. Epub 2018 Jul 4.

Abstract

AIM

LC-MS/MS bottom-up quantitation of proteins has become increasingly popular with trypsin as the most commonly used protease. However, trypsin does not always yield suitable surrogate peptides. An alternative enzyme, Glu-C, was used to generate surrogate peptides for quantifying a bispecific IgG1 biotherapeutic antibody in preclinical matrices.  Materials and methods: IgG1 was quantified by pellet digestion using an Acquity UPLC coupled  with a Xevo TQ-S mass spectrometer.  Results: Two generic LC-MS/MS methods (heavy and light chain) were developed which afforded acceptable precision and accuracy, and an lower limit of quantitation of 1 μg/ml in three preclinical matrices. A small nonsignificant bias was observed when cynomolgus serum LC-MS/MS results were compared with electrochemiluminescent immunoassay data.

CONCLUSION

Glu-C was successfully used as an alternative digestion enzyme for bottom-up quantitation of an IgG1 in matrices from multiple preclinical species, with good agreement with electrochemiluminescent immunoassay data.

摘要

目的

液相色谱-串联质谱法(LC-MS/MS)自下而上的蛋白质定量分析越来越受欢迎,其中胰蛋白酶是最常用的蛋白酶。然而,胰蛋白酶并不总能产生合适的替代肽段。另一种酶,Glu-C,被用于生成替代肽段,以在临床前基质中定量一种双特异性IgG1生物治疗性抗体。材料和方法:使用Acquity超高效液相色谱仪与Xevo TQ-S质谱仪联用,通过沉淀消化法定量IgG1。结果:开发了两种通用的LC-MS/MS方法(重链和轻链),其在三种临床前基质中具有可接受的精密度和准确度,定量下限为1μg/ml。将食蟹猴血清LC-MS/MS结果与电化学发光免疫分析数据进行比较时,观察到一个小的无统计学意义的偏差。结论:Glu-C成功用作替代消化酶,用于在多种临床前物种的基质中自下而上定量IgG1,与电化学发光免疫分析数据具有良好的一致性。

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