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首页> 外文期刊>Analytical chemistry >Development of a Native Nanoelectrospray Mass Spectrometry Method for Determination of the Drug-to-Antibody Ratio of Antibody-Drug Conjugates
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Development of a Native Nanoelectrospray Mass Spectrometry Method for Determination of the Drug-to-Antibody Ratio of Antibody-Drug Conjugates

机译:测定抗体-药物缀合物的药物/抗体比率的天然纳米电喷雾质谱方法的开发

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Antibody-drug conjugates (ADCs), an increasingly important therapeutic modality for targeted cancer treatment, have been studied using many analytical methods. A class of ADCs that utilize the reduced interchain disulfide cysteine residues for drug attachment has attracted particular interest in drug development. One challenge in analytical characterization of this class of ADCs is that the intact mass information of the ADC molecule is not attainable using conventional reversed-phase liquid chromatography-mass spectrometry methods. In this paper, we report a mass spectrometry (MS) method engaging enzymatic digestion, nanoelectrospray ionization (nano-ESI), and native MS to achieve direct determination of the intact mass and, furthermore, to calculate the average drug-to-antibody ratio (DAR) of the cysteine-linked ADCs. The novel aspects of this method lie in the application of a nano-ESI technique and, more significantly, the utilization of limited enzymatic digestion with a cysteine protease as compared to the recently published method by Valliere-Douglass et al. In summary, this novel native nano-ESI MS method in combination with limited enzymatic digestion provides a sensitive method for direct DAR determination and possesses great potential in studying low-abundance ADC analytes such as those from animal or human in vivo investigations.
机译:抗体-药物偶联物(ADCs),一种针对靶向癌症治疗的日益重要的治疗方式,已使用许多分析方法进行了研究。利用减少的链间二硫半胱氨酸残基进行药物附着的一类ADC在药物开发中引起了特别的兴趣。这类ADC的分析表征中的一个挑战是,使用常规的反相液相色谱-质谱法无法获得ADC分子的完整质量信息。在本文中,我们报告了一种采用酶消化,纳米电喷雾电离(nano-ESI)和天然MS的质谱(MS)方法,以直接测定完整质量,并计算平均药物与抗体的比例半胱氨酸连接的ADC(DAR)。与Valliere-Douglass等人最近发表的方法相比,该方法的新颖之处在于应用了纳米ESI技术,更重要的是,利用半胱氨酸蛋白酶进行有限的酶消化。总之,这种新颖的天然纳米ESI MS方法与有限的酶消化相结合,为直接DAR测定提供了一种灵敏的方法,在研究低丰度ADC分析物(例如来自动物或人类体内研究的ADC分析物)方面具有巨大的潜力。

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