Fast protein sequencing of monoclonal antibody by real-time digestion on emitter during nanoelectrospray

Growth in the pharmaceutical industry has led to an increasing demand for rapid characterization of therapeutic monoclonal antibodies. The current methods for antibody sequence confirmation (e.g., N-terminal Edman sequencing and traditional peptide mapping methods) are not sufficient; thus, we devel...

Descripción completa

Detalles Bibliográficos
Autores principales: Mao, Yuan, Zhang, Lichao, Kleinberg, Andrew, Xia, Qiangwei, Daly, Thomas J., Li, Ning
Formato: Online Artículo Texto
Lenguaje:English
Publicado: Taylor & Francis 2019
Materias:
Report
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC6601538/
https://www.ncbi.nlm.nih.gov/pubmed/30919719
http://dx.doi.org/10.1080/19420862.2019.1599633
_version_ 1783431308349800448
author Mao, Yuan
Zhang, Lichao
Kleinberg, Andrew
Xia, Qiangwei
Daly, Thomas J.
Li, Ning
author_facet Mao, Yuan
Zhang, Lichao
Kleinberg, Andrew
Xia, Qiangwei
Daly, Thomas J.
Li, Ning
author_sort Mao, Yuan
collection PubMed
description Growth in the pharmaceutical industry has led to an increasing demand for rapid characterization of therapeutic monoclonal antibodies. The current methods for antibody sequence confirmation (e.g., N-terminal Edman sequencing and traditional peptide mapping methods) are not sufficient; thus, we developed a fast method for sequencing recombinant monoclonal antibodies using a novel digestion-on-emitter technology. Using this method, a monoclonal antibody can be denatured, reduced, digested, and sequenced in less than an hour. High throughput and satisfactory protein sequence coverage were achieved by using a non-specific protease from Aspergillus saitoi, protease XIII, to digest the denatured and reduced monoclonal antibody on an electrospray emitter, while electrospray high voltage was applied to the digestion mixture through the emitter. Tandem mass spectrometry data was acquired over the course of enzyme digestion, generating similar information compared to standard peptide mapping experiments in much less time. We demonstrated that this fast protein sequencing method provided sufficient sequence information for bovine serum albumin and two commercially available monoclonal antibodies, mouse IgG1 MOPC21 and humanized IgG1 NISTmAb. For two monoclonal antibodies, we obtained sequence coverage of 90.5–95.1% for the heavy chains and 98.6–99.1% for the light chains. We found that on-emitter digestion by protease XIII generated peptides of various lengths during the digestion process, which was critical for achieving sufficient sequence coverage. Moreover, we discovered that the enzyme-to-substrate ratio was an important parameter that affects protein sequence coverage. Due to its highly automatable and efficient design, our method offers a major advantage over N-terminal Edman sequencing and traditional peptide mapping methods in the identification of protein sequence, and is capable of meeting an ever-increasing demand for monoclonal antibody sequence confirmation in the biopharmaceutical industry.
format Online
Article
Text
id pubmed-6601538
institution National Center for Biotechnology Information
language English
publishDate 2019
publisher Taylor & Francis
record_format MEDLINE/PubMed
spelling pubmed-66015382019-07-08 Fast protein sequencing of monoclonal antibody by real-time digestion on emitter during nanoelectrospray Mao, Yuan Zhang, Lichao Kleinberg, Andrew Xia, Qiangwei Daly, Thomas J. Li, Ning MAbs Report Growth in the pharmaceutical industry has led to an increasing demand for rapid characterization of therapeutic monoclonal antibodies. The current methods for antibody sequence confirmation (e.g., N-terminal Edman sequencing and traditional peptide mapping methods) are not sufficient; thus, we developed a fast method for sequencing recombinant monoclonal antibodies using a novel digestion-on-emitter technology. Using this method, a monoclonal antibody can be denatured, reduced, digested, and sequenced in less than an hour. High throughput and satisfactory protein sequence coverage were achieved by using a non-specific protease from Aspergillus saitoi, protease XIII, to digest the denatured and reduced monoclonal antibody on an electrospray emitter, while electrospray high voltage was applied to the digestion mixture through the emitter. Tandem mass spectrometry data was acquired over the course of enzyme digestion, generating similar information compared to standard peptide mapping experiments in much less time. We demonstrated that this fast protein sequencing method provided sufficient sequence information for bovine serum albumin and two commercially available monoclonal antibodies, mouse IgG1 MOPC21 and humanized IgG1 NISTmAb. For two monoclonal antibodies, we obtained sequence coverage of 90.5–95.1% for the heavy chains and 98.6–99.1% for the light chains. We found that on-emitter digestion by protease XIII generated peptides of various lengths during the digestion process, which was critical for achieving sufficient sequence coverage. Moreover, we discovered that the enzyme-to-substrate ratio was an important parameter that affects protein sequence coverage. Due to its highly automatable and efficient design, our method offers a major advantage over N-terminal Edman sequencing and traditional peptide mapping methods in the identification of protein sequence, and is capable of meeting an ever-increasing demand for monoclonal antibody sequence confirmation in the biopharmaceutical industry. Taylor & Francis 2019-05-07 /pmc/articles/PMC6601538/ /pubmed/30919719 http://dx.doi.org/10.1080/19420862.2019.1599633 Text en © 2019 The Author(s). Published with license by Taylor & Francis Group, LLC. http://creativecommons.org/licenses/by-nc-nd/4.0/ This is an Open Access article distributed under the terms of the Creative Commons Attribution-NonCommercial-NoDerivatives License (http://creativecommons.org/licenses/by-nc-nd/4.0/), which permits non-commercial re-use, distribution, and reproduction in any medium, provided the original work is properly cited, and is not altered, transformed, or built upon in any way.
spellingShingle Report
Mao, Yuan
Zhang, Lichao
Kleinberg, Andrew
Xia, Qiangwei
Daly, Thomas J.
Li, Ning
Fast protein sequencing of monoclonal antibody by real-time digestion on emitter during nanoelectrospray
title Fast protein sequencing of monoclonal antibody by real-time digestion on emitter during nanoelectrospray
title_full Fast protein sequencing of monoclonal antibody by real-time digestion on emitter during nanoelectrospray
title_fullStr Fast protein sequencing of monoclonal antibody by real-time digestion on emitter during nanoelectrospray
title_full_unstemmed Fast protein sequencing of monoclonal antibody by real-time digestion on emitter during nanoelectrospray
title_short Fast protein sequencing of monoclonal antibody by real-time digestion on emitter during nanoelectrospray
title_sort fast protein sequencing of monoclonal antibody by real-time digestion on emitter during nanoelectrospray
topic Report
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC6601538/
https://www.ncbi.nlm.nih.gov/pubmed/30919719
http://dx.doi.org/10.1080/19420862.2019.1599633
work_keys_str_mv AT maoyuan fastproteinsequencingofmonoclonalantibodybyrealtimedigestiononemitterduringnanoelectrospray
AT zhanglichao fastproteinsequencingofmonoclonalantibodybyrealtimedigestiononemitterduringnanoelectrospray
AT kleinbergandrew fastproteinsequencingofmonoclonalantibodybyrealtimedigestiononemitterduringnanoelectrospray
AT xiaqiangwei fastproteinsequencingofmonoclonalantibodybyrealtimedigestiononemitterduringnanoelectrospray
AT dalythomasj fastproteinsequencingofmonoclonalantibodybyrealtimedigestiononemitterduringnanoelectrospray
AT lining fastproteinsequencingofmonoclonalantibodybyrealtimedigestiononemitterduringnanoelectrospray

Ejemplares similares