Formation of Pyroglutamic Acid from N-Terminal Glutamic Acid in Immunoglobulin Gamma Antibodies

Chelius, Dirk; Jing, Kay; Lueras, Alexis M. K.; Rehder, Douglas S.; Dillon, Thomas M.; Vizel, A. O.; Rajan, Rahul; Li, Tiansheng; Treuheit, Michael J.; Bondarenko, Pavel V.

doi:10.1021/ac051827k

Cited by 181 publications

(166 citation statements)

References 27 publications

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“…Glutamate conversion to pE does not result in a charge state difference, so this change might be missed using simple chromatography-based release assays. To monitor glutamate cyclization, more complex assays, such as peptide mapping, would be required (5,6). Whether pE is monitored and controlled for a given therapeutic antibody should be based on its impact to safety and efficacy.…”

Section: Discussionmentioning

confidence: 99%

“…To generate N-terminal pE for identification and quantification purposes, the purified mAbs were incubated in PBS, pH 7.4, at 37°C for up to 1 month. These conditions previously have been used to form pyroglutamate from N-terminal glutamate on selected antibodies (6). Pyroglutamate was identified by peptide mapping with protease Lys-C.…”

Section: Identification and Quantification Of Pe By Lc/ms/ms-mentioning

confidence: 99%

“…Pyroglutamate was identified by peptide mapping with protease Lys-C. The identification of the modification of the N-terminal peptide was based on the loss of 18 mass units that was specific for the N-terminal residue (MS/MS analysis; not shown) (6,7). Fig.…”

Section: Identification and Quantification Of Pe By Lc/ms/ms-mentioning

confidence: 99%

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N-terminal Glutamate to Pyroglutamate Conversion in Vivo for Human IgG2 Antibodies

Liu

Goetze

Bass

et al. 2011

Journal of Biological Chemistry

153

119

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Therapeutic proteins contain a large number of post-translational modifications, some of which could potentially impact their safety or efficacy. In one of these changes, pyroglutamate can form on the N terminus of the polypeptide chain. Both glutamine and glutamate at the N termini of recombinant monoclonal antibodies can cyclize spontaneously to pyroglutamate (pE) in vitro. Glutamate conversion to pyroglutamate occurs more slowly than from glutamine but has been observed under near physiological conditions. Here we investigated to what extent human IgG2 N-terminal glutamate converts to pE in vivo. Pyroglutamate levels increased over time after injection into humans, with the rate of formation differing between polypeptide chains. These changes were replicated for the same antibodies in vitro under physiological pH and temperature conditions, indicating that the changes observed in vivo were due to chemical conversion not differential clearance. Differences in the conversion rates between the light chain and heavy chain on an antibody were eliminated by denaturing the protein, revealing that structural elements affect pE formation rates. By enzymatically releasing pE from endogenous antibodies isolated from human serum, we could estimate the naturally occurring levels of this post-translational modification. Together, these techniques and results can be used to predict the exposure of pE for therapeutic antibodies and to guide criticality assessments for this attribute.

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Section: Discussionmentioning

confidence: 99%

Section: Identification and Quantification Of Pe By Lc/ms/ms-mentioning

confidence: 99%

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N-terminal Glutamate to Pyroglutamate Conversion in Vivo for Human IgG2 Antibodies

Liu

Goetze

Bass

et al. 2011

Journal of Biological Chemistry

153

119

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“…Further, there are disulfide bonds that hold the structure together: intradomain disulfide bonds, light chain to heavy chain disulfide bonds, and inter-heavy chain disulfide bonds. In addition to the complexity described above, antibodies undergo several post-translational modifications, such as pyroglutamic acid formation at the N-terminus, 14 Cterminal lysine removal, 15 and addition of polysaccharide chains. 16 The complexity of these molecules complicates our ability to study their mechanisms of aggregation.…”

Section: Introductionmentioning

confidence: 99%

Increased aggregation propensity of IgG2 subclass over IgG1: Role of conformational changes and covalent character in isolated aggregates

et al. 2010

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Aggregation of human therapeutic antibodies represents a significant hurdle to product development. In a test across multiple antibodies, it was observed that IgG1 antibodies aggregated less, on average, than IgG2 antibodies under physiological pH and mildly elevated temperature. This phenomenon was also observed for IgG1 and IgG2 subclasses of anti-streptavidin, which shared 95% sequence identity but varied in interchain disulfide connectivity. To investigate the structural and covalent changes associated with greater aggregation in IgG2 subclasses, soluble aggregates from the two forms of anti-streptavidin were isolated and characterized. Sedimentation velocity analytical ultracentrifugation (SV-AUC) measurements confirmed that the aggregates were present in solution, and revealed that the IgG1 aggregate was composed of a predominant species, whereas the IgG2 aggregate was heterogeneous. Tertiary structural changes accompanied antibody aggregation as evidenced by greater ANS (8-Anilino-1-naphthalene sulfonic acid) binding to the aggregates over monomer, and differences in disulfide character and tryptophan environments between monomer, oligomer and aggregate species, as observed by near-UV circular dichroism (CD). Differences between subclasses were observed in the secondary structural changes that accompanied aggregation, particularly in the intermolecular b-sheet and turn structures between the monomer and aggregate species. Free thiol determination showed 2.4-fold lower quantity of free cysteines in the IgG1 subclass, consistent with the 2.4-fold reduction in aggregation of the IgG1 form when compared with IgG2 under these conditions. These observations suggested an important role for disulfide bond formation, as well as secondary and tertiary structural transitions, during antibody aggregation. Such degradations may be minimized using appropriate formulation conditions.

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“…Various modifications are determined by analyzing recombinant monoclonal antibodies at different levels, depending on the molecular weight differences of the modifications. Modifications, such as N-terminal glutamine and glutamate cyclization [3][4][5][6][7][8][9], different types of the conserved N-linked oligosaccharides [5,[7][8][9][10][11][12][13], amino acid truncation and insertion [8,11], cysteinylation [14], C-terminal lysine processing [5,7,11,15,16], fragmentation [12,15,17], glycation [18], oxidation [19,20], and nitration [21] can be directly determined by measurements of the molecular weights of intact antibodies, antibody light chain and heavy chain, and Fab and Fc fragments after papain or lys-C digestion [14]. On the other hand, analysis at the peptide level is normally required to determine the sites of modifications and modifications with small molecular weight differences, such as deamidation [22,23] and amidation [11], which results in a molecular weight difference of only 1 Da.…”

mentioning

confidence: 99%

Analysis of reduced monoclonal antibodies using size exclusion chromatography coupled with mass spectrometry

Liu

Gaza-Bulseco

Chumsae

2009

J. Am. Soc. Mass Spectrom.

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Size-exclusion chromatography (SEC) has been widely used to detect antibody aggregates, monomer, and fragments. SEC coupled to mass spectrometry has been reported to measure the molecular weights of antibody; antibody conjugates, and antibody light chain and heavy chain. In this study, separation of antibody light chain and heavy chain by SEC and direct coupling to a mass spectrometer was further studied. It was determined that employing mobile phases containing acetonitrile, trifluoroacetic acid, and formic acid allowed the separation of antibody light chain and heavy chain after reduction by SEC. In addition, this mobile phase allowed the coupling of SEC to a mass spectrometer to obtain a direct molecular weight measurement. The application of the SEC-MS method was demonstrated by the separation of the light chain and the heavy chain of multiple recombinant monoclonal antibodies. In addition, separation of a thioether linked light chain and heavy chain from the free light chain and the free heavy chain of a recombinant monoclonal antibody after reduction was also achieved. This optimized method provided a separation of antibody light chain and heavy chain based on size and allowed a direct measurement of molecular weights by mass spectrometry. In addition, this method may help to identify peaks eluting from SEC column directly. (J Am Soc Mass Spectrom 2009, 20, 2258 -2264) © 2009 Published by Elsevier Inc. on behalf of American Society for Mass Spectrometry M ass spectrometry is one of the most indispensable techniques for the characterization of recombinant monoclonal antibodies because most of the modifications that result in heterogeneity and degradation are involved in molecular weight differences [1,2]. Various modifications are determined by analyzing recombinant monoclonal antibodies at different levels, depending on the molecular weight differences of the modifications. Modifications, such as N-terminal glutamine and glutamate cyclization [3][4][5][6][7][8][9], different types of the conserved N-linked oligosaccharides [5,[7][8][9][10][11][12][13], amino acid truncation and insertion [8,11], cysteinylation [14], C-terminal lysine processing [5,7,11,15,16], fragmentation [12,15,17], glycation [18], oxidation [19,20], and nitration [21] can be directly determined by measurements of the molecular weights of intact antibodies, antibody light chain and heavy chain, and Fab and Fc fragments after papain or lys-C digestion [14]. On the other hand, analysis at the peptide level is normally required to determine the sites of modifications and modifications with small molecular weight differences, such as deamidation [22,23] and amidation [11], which results in a molecular weight difference of only 1 Da.Mass spectrometry is commonly coupled with reversedphase high-performance liquid chromatography (RP-HPLC), which desalts the samples and separates different components based on hydrophobicity. The molecular weights of intact antibodies [12,15] and their light chains and heavy chains can be readily measured by on...

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Formation of Pyroglutamic Acid from N-Terminal Glutamic Acid in Immunoglobulin Gamma Antibodies

Cited by 181 publications

References 27 publications

N-terminal Glutamate to Pyroglutamate Conversion in Vivo for Human IgG2 Antibodies

N-terminal Glutamate to Pyroglutamate Conversion in Vivo for Human IgG2 Antibodies

Increased aggregation propensity of IgG2 subclass over IgG1: Role of conformational changes and covalent character in isolated aggregates

Analysis of reduced monoclonal antibodies using size exclusion chromatography coupled with mass spectrometry

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