Intact Protein Mass Spectrometry for Therapeutic Protein Quantitation, Pharmacokinetics, and Biotransformation in Preclinical and Clinical Studies: An Industry Perspective

Kellie, John F.; Tran, John; Jian, Wenying; Jones, Barry R; Mehl, John T; Ge, Ying; Henion, Jack D.; Bateman, Kevin P.

doi:10.1021/jasms.0c00270

Cited by 24 publications

(21 citation statements)

References 104 publications

(220 reference statements)

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“…For intact protein LC-MS applied to biopharmaceutical in-life studies (and perhaps mAb analysis in general), the LC-MS/MS platform presented here adds extra flexibility and benefit to analytical LC-MS workflows already in use. 25 The ZenoTOF 7600 system was able to achieve good sequence coverage at the reduced mAb level, especially for the light chain. The GSKmAb light chain (25 kDa) was within size range for MS/MS ions to cover 100% of the protein sequence; however, thorough top-down sequencing coverage for the intact mAb (150 kDa) or heavy chain (50 kDa) is not achieved, partly due to higher mass.…”

Section: ■ Discussionmentioning

confidence: 99%

Top-Down Characterization and Intact Mass Quantitation of a Monoclonal Antibody Drug from Serum by Use of a Quadrupole TOF MS System Equipped with Electron-Activated Dissociation

Kellie

Schneck

Causon³

et al. 2022

J. Am. Soc. Mass Spectrom.

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Time-of-flight MS systems for biopharmaceutical and protein characterization applications may play an even more pivotal role in the future as biotherapeutics increase in drug pipelines and as top-down MS approaches increase in use. Here, a recently developed TOF MS system is examined for monoclonal antibody (mAb) characterization from serum samples. After immunocapture, purified drug material spiked into monkey serum or dosed for an in-life study is analyzed by top-down MS. While characterization aspects are a distinct advantage of the MS platform, MS system and software capabilities are also shown regarding intact protein quantitation. Such applications are demonstrated to help enable comprehensive protein molecule quantitation and characterization by use of TOF MS instrumentation.

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Section: ■ Discussionmentioning

confidence: 99%

Top-Down Characterization and Intact Mass Quantitation of a Monoclonal Antibody Drug from Serum by Use of a Quadrupole TOF MS System Equipped with Electron-Activated Dissociation

Kellie

Schneck

Causon³

et al. 2022

J. Am. Soc. Mass Spectrom.

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“…Prior initiatives such as those describing first drafts of the human proteome in 2014 ( 33 , 34 ) and ongoing work under the aegis of the Human Protein Atlas and the Human Proteome Project ( 35 ) have accomplished a great deal over the past several years, and the Human Proteome Organization has called for the community to “systematically map all human proteoforms” ( 36 ). There has also been an industry-led call from several pharmaceutical companies underscoring the need for major improvements in proteoform measurement ( 37 ).…”

Section: Synergy Of the Human Proteoform Project With Other Initiativesmentioning

confidence: 99%

The Human Proteoform Project: Defining the human proteome

et al. 2021

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“…Peak-sharpening algorithms are subsequently used on the deconvolved data to resolve remaining overlapped features in the zero-charge spectrum. PMI includes a “comb filter” to identify peak series equally spaced in m / z , such as those arising from polydisperse adduction of a subunit, which can greatly improve analysis of mass spectra representing samples of this type, including those of great interest in the biopharmaceutical industry , such as highly disperse antibody-drug conjugates. ,,,− PMI is coded and compiled in C++ for increased speed, has batch processing capabilities, allows the user to easily select different liquid chromatography-MS (LC-MS) retention data to analyze, and can be used to automatically assign peaks based on protein sequence data or other user-supplied information. It is also vendor-neutral and can produce user-friendly, customizable reports for non-MS users, features important for its use in industry .…”

Section: State-of-the-art Approaches To Heterogeneity In Native Mass ...mentioning

confidence: 99%

“…Although many online solution-phase separation approaches (such as online chromatography methods − and capillary zone electrophoresis − ) have been introduced to help solve this problem, our discussion is confined to instrumentation and techniques commonly available within mass spectrometers themselves or with small modifications. As this review is written from an academic viewpoint, we refer readers not only to recent native MS work on biotherapeutics ,− but also to many recent efforts and helpful perspectives on this topic from industry scientists representing a variety of biopharmaceutical companies, drawing upon these insights where possible. ,,,− Importantly, though implementation of the methods we describe below faces unique challenges in industry (namely, rigorous standardization and commercialization), we hold that educating potential users on the theoretical aspects of these approaches is important and beneficial to all who utilize native MS, regardless of background. We conclude by reflecting upon the progress of native MS with respect to the problem of heterogeneity, discussing remaining challenges and future strategies for the field, and providing our view of optimal approaches to facilitate analysis and interpretation of the complicated mass spectra of heterogeneous biomolecules, which is paramount for continued growth of this technique as a tool in structural biology.…”

Section: Introductionmentioning

confidence: 99%

Approaches to Heterogeneity in Native Mass Spectrometry

Rolland

Prell

2021

Chem. Rev.

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Native mass spectrometry (MS) is aimed at preserving and determining the native structure, composition, and stoichiometry of biomolecules and their complexes from solution after they are transferred into the gas phase. Major improvements in native MS instrumentation and experimental methods over the past few decades have led to a concomitant increase in the complexity and heterogeneity of samples that can be analyzed, including protein–ligand complexes, protein complexes with multiple coexisting stoichiometries, and membrane protein–lipid assemblies. Heterogeneous features of these biomolecular samples can be important for understanding structure and function. However, sample heterogeneity can make assignment of ion mass, charge, composition, and structure very challenging due to the overlap of tens or even hundreds of peaks in the mass spectrum. In this review, we cover data analysis, experimental, and instrumental advances and strategies aimed at solving this problem, with an in-depth discussion of theoretical and practical aspects of the use of available deconvolution algorithms and tools. We also reflect upon current challenges and provide a view of the future of this exciting field.

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Intact Protein Mass Spectrometry for Therapeutic Protein Quantitation, Pharmacokinetics, and Biotransformation in Preclinical and Clinical Studies: An Industry Perspective

Cited by 24 publications

References 104 publications

Top-Down Characterization and Intact Mass Quantitation of a Monoclonal Antibody Drug from Serum by Use of a Quadrupole TOF MS System Equipped with Electron-Activated Dissociation

Top-Down Characterization and Intact Mass Quantitation of a Monoclonal Antibody Drug from Serum by Use of a Quadrupole TOF MS System Equipped with Electron-Activated Dissociation

The Human Proteoform Project: Defining the human proteome

Approaches to Heterogeneity in Native Mass Spectrometry

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