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分离抗 CD22 免疫毒素荷质比变异体的过程。

Process scale separation of an anti-CD22 immunotoxin charge variant.

机构信息

MedImmune, One MedImmune Way, Gaithersburg, MD 20878, USA.

出版信息

J Chromatogr A. 2012 Oct 19;1260:120-5. doi: 10.1016/j.chroma.2012.08.061. Epub 2012 Aug 27.

Abstract

We describe the analytical characterization and process scale separation of a deamidated variant of an immunotoxin. The different charge variants of the immunotoxin were separated using analytical ion-exchange HPLC. These charge variants were analyzed by peptide mapping and LC-MS/MS to identify the site of modification, which was determined to reside in the toxin portion of the molecule. Using a cell-based bioassay it was also determined that deamidation led to reduced biological activity, requiring it be controlled during manufacturing. This was accomplished using process scale anion-exchange chromatography. The process was capable of reducing the deamidated form to a level low enough for the resulting product to maintain acceptable biological activity. Keys to the successful control of this impurity at process scale were a good understanding of structure-function relationship and the availability of an analytical HPLC assay to provide a surrogate for the cell-based bioassay.

摘要

我们描述了免疫毒素的脱酰胺变体的分析特性和工艺规模分离。使用分析离子交换 HPLC 分离免疫毒素的不同电荷变体。通过肽图分析和 LC-MS/MS 对这些电荷变体进行分析,以确定修饰的部位,结果确定位于分子的毒素部分。使用基于细胞的生物测定法还确定脱酰胺导致生物活性降低,因此在制造过程中需要对其进行控制。这是通过使用工艺规模的阴离子交换色谱法实现的。该工艺能够将脱酰胺形式降低到足够低的水平,使最终产品保持可接受的生物活性。在工艺规模上成功控制这种杂质的关键是对结构-功能关系有很好的理解,并且有分析 HPLC 测定法作为基于细胞的生物测定法的替代方法。

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