Predictive <i>In Vitro</i> Vitreous and Serum Models and Methods to Assess Thiol-Related Quality Attributes in Protein Therapeutics

Liu, Y. Diana; Chen, Yan; Tsui, George Kar; Wei, Bingchuan; Yang, Feng; Yu, Christopher; Cornell, Christopher

doi:10.1021/acs.analchem.9b05176

Cited by 5 publications

(3 citation statements)

References 39 publications

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“…Between them, Dilution Scheme 1, with a 3-fold dilution (before digestion), performed well, while the digestion efficiency was decreased when a 9-fold dilution was used (Dilution Scheme 2). After the dilution, the Lys-C digestion was carried out at pH 7 to minimize artificial deamidation occurring during protein digestion [ 38 ]. Lys-C enzyme to protein ratios (enzyme: protein w / w ) of 1:20 and 1:10 and digestion times were evaluated.…”

Section: Resultsmentioning

confidence: 99%

Expanding the Analytical Toolbox: Developing New Lys-C Peptide Mapping Methods with Minimized Assay-Induced Artifacts to Fully Characterize Antibodies

Liu,

Beardsley,

Yang

2023

Pharmaceuticals

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Peptide mapping is an important tool used to confirm that the correct sequence has been expressed for a protein and to evaluate protein post-translational modifications (PTMs) that may arise during the production, processing, or storage of protein drugs. Our new orally administered drug (Ab-1), a single-domain antibody, is highly stable and resistant to proteolysis. Analysis via the commonly used tryptic mapping method did not generate sufficient sequence coverage. Alternative methods were needed to study the Ab-1 drug substance (75 mg/mL) and drug product (3 mg/mL). To meet these analytical needs, we developed two new peptide mapping methods using lysyl endopeptidase (Lys-C) digestion. These newly developed protein digestion protocols do not require desalting/buffer-exchange steps, thereby reducing sample preparation time and improving method robustness. Additionally, the protein digestion is performed under neutral pH with methionine acting as a scavenger to minimize artifacts, such as deamidation and oxidation, which are induced during sample preparation. Further, the method for low-concentration samples performs comparably to the method for high-concentration samples. Both methods provide 100% sequence coverage for Ab-1, and, therefore, enable comprehensive characterization for its product quality attribute (PQA) assessment. Both methods can be used to study other antibody formats.

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Section: Resultsmentioning

confidence: 99%

Expanding the Analytical Toolbox: Developing New Lys-C Peptide Mapping Methods with Minimized Assay-Induced Artifacts to Fully Characterize Antibodies

Liu,

Beardsley,

Yang

2023

Pharmaceuticals

Self Cite

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“…Different in vitro models developed elsewhere, used static incubation 8,9,[35][36][37] or a dialysis setup. 7,10,11,13,27,38 Dialysis simulates a slow influx of the SC interstitial fluid 13,27 and allows to diffuse small molecules (excipients) across the membrane, whilst retaining the therapeutic protein locally. Such events have been argued to occur after SC administration.…”

Section: Discussionmentioning

confidence: 99%

“…Thus, a number of groups developed in vitro models simulating human in vivo conditions. For example using the desired biological fluid such as serum/plasma 7−9 (related to intravenous administration), vitreous humor 7,10,11 (related to intravitreal injections), artificial SC fluid, 12−15 or SC tissue homogenate 16 (related to SC administration). Simulating the SC tissue is particularly challenging as the SC interstitial fluid is not readily accessible.…”

Section: Introductionmentioning

confidence: 99%

Stability of monoclonal antibodies after simulated subcutaneous administration

Schuster

Mahler

Joerg

et al. 2021

Journal of Pharmaceutical Sciences

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Changes in the environment from the drug product to the human physiology might lead to physical and/or chemical modifications of the protein drug, such as in vivo aggregation and fragmentation. Although subcutaneous (SC) injection is a common route of administration for therapeutic proteins, knowledge on in vivo stability in the SC tissue is limited. In this study, we developed a physiologic in vitro model simulating the SC environment in patients. We assessed the stability of two monoclonal antibodies (mAbs) in four different protein-free fluids under physiologic conditions. We monitored protein stability over two weeks using a range of analytical methods, in analogy to testing purposes of a drug product. Both mAbs showed an increase of protein aggregates, fragments, and acidic species. mAb1 was consistently more stable in this in vitro model than mAb2, highlighting the importance of comparing the stability of different mAbs under physiologic conditions. Throughout the study, both mAbs were substantially less stable in bicarbonate buffers as compared to phosphate-buffered saline. In summary, our developed model was able to differentiate stability between molecules. Bicarbonate buffers were more suitable compared to phosphate-buffered saline in regards to simulating the in vivo conditions and evaluating protein liabilities.

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In Vivo Reoxidation Kinetics of Free Thiols in Multiple Domains of IgG1 Antibodies in Rats

Kim

Lechmann

Rajan³

et al. 2021

Journal of Pharmaceutical Sciences

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Predictive In Vitro Vitreous and Serum Models and Methods to Assess Thiol-Related Quality Attributes in Protein Therapeutics

Cited by 5 publications

References 39 publications

Expanding the Analytical Toolbox: Developing New Lys-C Peptide Mapping Methods with Minimized Assay-Induced Artifacts to Fully Characterize Antibodies

Expanding the Analytical Toolbox: Developing New Lys-C Peptide Mapping Methods with Minimized Assay-Induced Artifacts to Fully Characterize Antibodies

Stability of monoclonal antibodies after simulated subcutaneous administration

In Vivo Reoxidation Kinetics of Free Thiols in Multiple Domains of IgG1 Antibodies in Rats

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