Identification and characterization of a residual host cell protein hexosaminidase B associated with <i>N</i>‐glycan degradation during the stability study of a therapeutic recombinant monoclonal antibody product

Li, Xuanwen; An, Yan; Liao, Jing; Xiao, Li; Swanson, Meghan R.; Martinez‐Fonts, Kirby; Pavon, Jorge Alexander; Sherer, Edward C.; Jawa, Vibha; Wang, Fengqiang; Gao, Xinliu; Letarte, Simon; Richardson, Douglas D.

doi:10.1002/btpr.3128

Cited by 25 publications

(16 citation statements)

References 25 publications

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“…HCPs can copurify with the therapeutic protein via specific or nonspecific interactions. 10,11 Several lipases, such as PLBL2, LPL, and LPLA2, have been reported to degrade PS-80 or PS-20 in biotherapeutics. [4][5][6][7]9 Multiple analytical tools have been developed as part of an overall HCP control strategy.…”

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confidence: 99%

“…PS prevents agitation-induced aggregation, and minimizes surface adsorption. − Polysorbate-80 (PS-80) and polysorbate-20 (PS-20) are the two most widely used PSs in the biopharma industry. , The degradation of PS can result in turbidity and formation of subvisible particles, which impact product quality or shorten the shelf life of the drug product. , PS degradation is an industry-wide challenge for process and formulation development in biotherapeutics. − The challenge increases with higher cell density and titer in bioprocess as well as higher drug concentrations in formulation development. , There are multiple mechanisms for PS degradation which can be grouped into two main categories: oxidation and hydrolysis. , Enzymatic hydrolysis is the dominant mechanism for PS degradation, which results in cleavage of an ester bond in PS by lipases, esterases, or possibly other host cell proteins (HCPs) without known lipase activity. HCPs can copurify with the therapeutic protein via specific or nonspecific interactions. , Several lipases, such as PLBL2, LPL, and LPLA2, have been reported to degrade PS-80 or PS-20 in biotherapeutics. − , …”

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confidence: 99%

“…ELISA provides one summed value for total HCP content. In some cases, specific antibodies were developed to known HCPs present in a sample. , Alternatively, liquid chromatography–mass spectrometry (LC-MS) based proteomics approaches are evolving rapidly as an orthogonal assay for HCP characterization, since proteomics can identify and quantify practically any individual HCP with certain abundance levels. ,− Absolute quantification of individual HCPs can be achieved by multiple reaction monitoring (MRM) or parallel reaction monitoring (PRM) targeted approaches with suitable internal standards. , However, current proteomics approaches have two main analytical challenges to overcome when investigating the cause of PS-80 degradation.…”

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confidence: 99%

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Profiling Active Enzymes for Polysorbate Degradation in Biotherapeutics by Activity-Based Protein Profiling

Chandra

Letarte

et al. 2021

Anal. Chem.

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Polysorbate is widely used to maintain stability of biotherapeutic proteins in pharmaceutical formulation development. Degradation of polysorbate can lead to particle formation in drug products, which is a major quality concern and potential patient risk factor. Enzymatic activity from residual host cell enzymes such as lipases and esterases plays a major role for polysorbate degradation. Their high activity, often at very low concentration, constitutes a major analytical challenge in the biopharmaceutical industry. In this study, we evaluated and optimized the activity-based protein profiling (ABPP) approach to identify active enzymes responsible for polysorbate degradation. Using an optimized chemical probe, we established the first global profile of active serine hydrolases in harvested cell culture fluid (HCCF) for monoclonal antibodies (mAbs) production from two Chinese hamster ovary (CHO) cell lines. A total of eight known lipases were identified by ABPP with enzyme activity information, while only five lipases were identified by a traditional abundance-based proteomics (TABP) approach. Interestingly, phospholipase B-like 2 (PLBL2), a well-known problematic HCP was not found to be active in process-intermediates from two different mAbs. In a proof-of-concept study with downstream samples, phospholipase A2 group VII (PLA2G7) was only identified by ABPP and confirmed to contribute to polysorbate-80 degradation for the first time. The established ABBP approach is approved to be able to identify low-abundance host cell enzymes and fills the gap between lipase abundance and activity, which enables more meaningful polysorbate degradation investigations for biotherapeutic development.

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Profiling Active Enzymes for Polysorbate Degradation in Biotherapeutics by Activity-Based Protein Profiling

Chandra

Letarte

et al. 2021

Anal. Chem.

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“…The identification of individual HCPs is critical for Quality by Design-based process development (supports development of a control strategy) and risk assessment. Traditional abundance-based proteomics (TABP) has been demonstrated as a valuable tool to identify and track the clearance of PSDEs and other HCPs throughout a purification process, which supports process development efforts (both upstream and downstream) on key HCPs that can impact product quality and stability [ 5 , 24 ].…”

Section: Analytical Toolboxmentioning

confidence: 99%

The measurement and control of high-risk host cell proteins for polysorbate degradation in biologics formulation

Wang

et al. 2022

Antibody Therapeutics

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Non-ionic surfactant polysorbates (PS), including PS-80 and PS-20, are commonly used in the formulation of biotherapeutic products for both preventing surface adsorption and acting as stabilizer against protein aggregation. Trace levels of residual host cell proteins (HCPs) with lipase or esterase enzymatic activity have been shown to degrade polysorbates in biologics formulation. The measurement and control of these low-abundance, high-risk HCPs for polysorbate degradation is an industry-wide challenge to achieve desired shelf-life of biopharmaceuticals in liquid formulation, especially for high-concentration formulation product development. Here, we reviewed the challenges, recent advances and future opportunities of analytical method development, risk assessment and control strategies for polysorbate degradation during formulation development with a focus on enzymatic degradation. Continued efforts to advance our understanding of polysorbate degradation in biologics formulation will help develop high-quality medicines for patients.

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“…Host cell proteins (HCPs) present in the final drug product are a particular concern, due to the risk that a HCP could elicit an immune response in the patient or reduce efficacy (Hanania et al, 2015). In addition, the presence of proteolytic HCPs can degrade or affect the stability of the mAb (Li et al, 2021; Luo et al, 2019). Regulatory authorities consider the amount of HCP in the final product to be a critical quality attribute, and require that the total HCP concentration be < 100 ppm (Bracewell et al, 2015).…”

Section: Introductionmentioning

confidence: 99%

Annotation of the non-canonical translatome reveals that CHO cell microproteins are a new class of mAb drug product impurity

Rivadeneyra

Tzani

Kelly

et al. 2022

Preprint

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Mass spectrometry (MS) has emerged as a powerful approach for the detection of Chinese hamster ovary (CHO) cell protein impurities in antibody drug products. The incomplete annotation of the Chinese hamster genome, however, limits the coverage of MS-based host cell protein (HCP) analysis. In this study, we performed ribosome footprint profiling (Ribo-seq) of translation initiation and elongation to refine the Chinese hamster genome annotation. Analysis of these data resulted in the identification of thousands of previously uncharacterised non-canonical proteoforms in CHO cells, such as N-terminally extended proteins and short open reading frames (sORFs) predicted to encode for microproteins. MS-based HCP analysis of adalimumab with the extended protein sequence database, resulted in the detection of CHO cell microprotein impurities in a mAb drug product for the first time. Further analysis revealed that the CHO cell microprotein population is altered over the course of cell culture and in response to a change in cell culture temperature. The annotation of non-canonical Chinese hamster proteoforms permits a more comprehensive characterisation of HCPs in antibody drug products using MS.

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Identification and characterization of a residual host cell protein hexosaminidase B associated with N‐glycan degradation during the stability study of a therapeutic recombinant monoclonal antibody product

Cited by 25 publications

References 25 publications

Profiling Active Enzymes for Polysorbate Degradation in Biotherapeutics by Activity-Based Protein Profiling

Profiling Active Enzymes for Polysorbate Degradation in Biotherapeutics by Activity-Based Protein Profiling

The measurement and control of high-risk host cell proteins for polysorbate degradation in biologics formulation

Annotation of the non-canonical translatome reveals that CHO cell microproteins are a new class of mAb drug product impurity

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