Monolith affinity chromatography for the rapid quantification of a single-chain variable fragment immunotoxin.

Peter Satzer,Johanna Paulsson,Alois Jungbauer,Romana Zehetner,Ralf Sommer,Christoph Klade,Agnes Rodler,Klaus Hofstädter

doi:10.1002/jssc.201800257

Abstract

We developed a novel analytical method for concentration determination of tandem single‐chain antibody diphtheria toxin (immunotoxin). The method is based on polymethacrylate monoliths with Protein L ligands as the binding moiety. Different buffers were tested for elution of the Protein L‐bound immunotoxin and 4.5 M guanidinium hydrochloride performed best. We optimized the elution conditions and the method sequence resulting in a fast and robust method with a runtime <10 min. Fast determination of immunotoxin is critical if any process decisions rely on this data. We determined method performance and a lower limit of detection of 27 μg/mL and a lower limit of quantification of 90 μg/mL was achieved. The validity of the method in terms of residual analysis, precision, and repeatability was proven in a range from 100 to 375 μg/mL. The short runtime and ease of use of a high‐performance liquid chromatography method is especially useful for a process analytical tool approach. Bioprocesses related to immunotoxin where fermentation or other process parameters can be adjusted in accordance to the immunotoxin levels will be benefited from this method to achieve the highest possible purity and productivity.

Highlights

Monoliths offer a way for the rapid determination of biomolecules such as immunotoxins
Sole bottleneck in the GMP production and process development of A-dmDT390-bisFv(UCHT1) is the time-consuming inprocess control during up- and downstream processing, which consists of a preparative fractionation by size exclusion and Article Related Abbreviations: DT, diphtheria toxin; High-performance monolith affinity chromatography (HPMAC), high-performance monolith affinity chromatography; scFv, single-chain antibody
A fast in-process control method for the determination of an immunotoxin was developed. This method is based on affinity chromatography with protein L immobilized on the CIM® disk

Summary

Introduction

Monoliths offer a way for the rapid determination of biomolecules such as immunotoxins. In this case a fast and robust method was developed for in-process control for an immunotoxin. A bivalent immunotoxin consisting of two tandem single-chain antibodies (scFv) and a truncated diphtheria toxin (DT) intended for the treatment of CD3-positive peripheral T-cell lymphoma (leukemic, nodal, and extranodal) and the treatment of cutaneous T-cell lymphoma [1,2]. Sole bottleneck in the GMP production and process development of A-dmDT390-bisFv(UCHT1) is the time-consuming inprocess control during up- and downstream processing, which consists of a preparative fractionation by size exclusion and Article Related Abbreviations: DT, diphtheria toxin; HPMAC, high-performance monolith affinity chromatography; scFv, single-chain antibody

Methods

Results

Conclusion