Targeted Capture of Chinese Hamster Ovary Host Cell Proteins: Peptide Ligand Discovery

Lavoie, R. Ashton; Fazio, Alice di; Blackburn, R. Kevin; Goshe, Michael B.; Carbonell, Ruben G.; Menegatti, Stefano

doi:10.3390/ijms20071729

Cited by 33 publications

(65 citation statements)

References 33 publications

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“…In comparison, benchmark anion exchange resin Capto Q yielded 60.7% (179 of 295) at 20 mM and 33.6% (71 of 211) at 150 mM. Lower HCPs binding by Capto Q at a high salt concentration was anticipated, given that this resin relies solely on electrostatic binding; further, increased binding of the mAb product (isoelectric point ~ 7.6) by Capto Q at pH 8 (64.8% ± 2.6% at 20 mM and 57.0% ± 2.9% at 150 mM) also reduces the number of binding sites available for HCP capture as shown in Table (Lavoie et al, ). The mixed‐mode resin Capto Adhere showed high overlap in bound HCPs (71.4%, 220 of 308) at low salt concentration; however, promiscuous binding of HCPs was also accompanied by significant loss of mAb product (>80% for all pH conditions; Lavoie et al, ).…”

Section: Resultsmentioning

confidence: 97%

“…The feed samples were prepared by diafiltration of the cell culture fluid against the different buffers, incubated for 1 hr with the equilibrated adsorbents, and the supernatants (unbound and wash fraction) were collected and pooled before analysis. The resulting performance of each resin as a function of buffer condition by total HCP and IgG bound as reported in Lavoie et al () is summarized in Table .…”

Section: Resultsmentioning

confidence: 99%

Section: Methodsmentioning

confidence: 99%

“…The synthesis procedure was performed according to a protocol adapted from Menegatti et al () and is described in detail in prior work (Lavoie et al, ). Individual ligand candidates previously identified were synthesized and pooled as described in previous work (Lavoie et al, ). Briefly, the peptides were individually synthesized directly on Toyopearl AF‐Amino‐650M resin, and the resulting adsorbents were pooled as follows: (a) hexameric hydrophobic positive (6HP) resin, comprising of the peptide sequences GSRYRYGSG, RYYYAIGSG, AAHIYYGSG, IYRIGRGSG, HSKIYKGSG; (b) hexameric multipolar (6MP) resin, comprising ADRYGHGSG, DRIYYYGSG, DKQRIIGSG, RYYDYGGSG, YRIDRYGSG; (c) tetrameric hydrophobic positive (4HP) resin, comprising HYAIGSG, FRYYGSG, HRRYGSG, RYFFGSG; and (d) tetrameric multipolar (4MP) resin, comprising DKSIGSG, DRNIGSG, HYFDGSG, and YRFDGSG.…”

Section: Methodsmentioning

confidence: 99%

“…Briefly, the peptides were individually synthesized directly on Toyopearl AF‐Amino‐650M resin, and the resulting adsorbents were pooled as follows: (a) hexameric hydrophobic positive (6HP) resin, comprising of the peptide sequences GSRYRYGSG, RYYYAIGSG, AAHIYYGSG, IYRIGRGSG, HSKIYKGSG; (b) hexameric multipolar (6MP) resin, comprising ADRYGHGSG, DRIYYYGSG, DKQRIIGSG, RYYDYGGSG, YRIDRYGSG; (c) tetrameric hydrophobic positive (4HP) resin, comprising HYAIGSG, FRYYGSG, HRRYGSG, RYFFGSG; and (d) tetrameric multipolar (4MP) resin, comprising DKSIGSG, DRNIGSG, HYFDGSG, and YRFDGSG. All ligands were synthesized using standard Fmoc‐amino acid coupling chemistry and deprotection procedures as described in prior work (Lavoie et al, ). Resins were washed three to five times first with DMF then 20% methanol and stored in 20% methanol at 2–8°C.…”

Section: Methodsmentioning

confidence: 99%

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Targeted capture of Chinese hamster ovary host cell proteins: Peptide ligand binding by proteomic analysis

Lavoie

Fazio

Williams

et al. 2019

Biotech & Bioengineering

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The clearance of host cell proteins (HCPs) is of crucial importance in biomanufacturing, given their diversity in composition, structure, abundance, and occasional structural homology with the product. The current approach to HCP clearance in the manufacturing of monoclonal antibodies (mAbs) relies on product capture with Protein A followed by removal of residual HCPs in flow‐through mode using ion exchange or mixed‐mode chromatography. Recent studies have highlighted the presence of “problematic HCP” species, which are either difficult to remove (Group I), can degrade the mAb product (Group II), or trigger immunogenic reactions (Group III). To improve the clearance of these species, we developed a family of synthetic peptides that target HCPs and exhibit low binding to IgG product. In this study, these peptides were conjugated onto chromatographic resins and evaluated in terms of HCP clearance and mAb yield, using an industrial mAb‐producing CHO harvest as model supernatant. To gather detailed knowledge on the binding of individual HCPs, the unbound fractions were subjected to shotgun proteomic analysis by mass spectrometry. It was found that these peptide ligands exhibit superior HCP binding capability compared to those of the benchmark commercial resins commonly used in mAb purification. In addition, some peptide‐based resins resulted in much lower losses of product yield compared to these commercial supports. The proteomic analysis showed effective capture of many “problematic HCPs” by the peptide ligands, especially some that are weakly bound by commercial media. Collectively, these results indicate that these peptides show great promise toward the development of next‐generation adsorbents for safer and cost‐effective manufacturing of biologics.

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Section: Resultsmentioning

confidence: 97%

Section: Resultsmentioning

confidence: 99%

Section: Methodsmentioning

confidence: 99%

Section: Methodsmentioning

confidence: 99%

Section: Methodsmentioning

confidence: 99%

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Targeted capture of Chinese hamster ovary host cell proteins: Peptide ligand binding by proteomic analysis

Lavoie

Fazio

Williams

et al. 2019

Biotech & Bioengineering

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Molecular Engineering of Cyclic Azobenzene‐Peptide Hybrid Ligands for the Purification of Human Blood Factor VIII via Photo‐Affinity Chromatography

Prodromou

Moore

Chu

et al. 2023

Adv Funct Materials

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The use of benign stimuli to control the binding and release of labile biologics for their isolation from complex feedstocks is a key goal of modern biopharmaceutical technology. This study introduces cyclic azobenzene‐peptide (CAP) ligands for the rapid and discrete photo‐responsive capture and release of blood coagulation factor VIII (FVIII). A predictive method—based on amino acid sequence and molecular architecture of CAPs—is developed to correlate the conformation of cis/trans‐CAP photo‐isomers to FVIII binding and release. Combined in silico ‐ in vitro analysis of FVIII:peptide interactions guide the design of a rational approach to optimize isomerization kinetics and biorecognition of CAPs. A photoaffinity adsorbent, prepared by conjugating selected CAP G‐cycloAZOB[Lys‐YYKHLYN‐Lys]‐G on translucent chromatographic beads, features high binding capacity (>6 mg of FVIII per mL of resin) and rapid photo‐isomerization kinetics (τ < 30 s) when exposed to 420–450 nm light at the intensity of 0.1 W cm−2. The adsorbent purifies FVIII from a recombinant harvest using a single mobile phase, affording high product yield (>90%), purity (>95%), and blood clotting activity. The CAPs introduced in this report demonstrate a novel route integrating gentle operational conditions in a rapid and efficient bioprocess for the purification of life‐saving biotherapeutics.

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Purification of polyclonal immunoglobulin G from human serum using peptide‐based adsorbents

et al. 2021

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This study presents the chromatographic purification of immunoglobulin G (IgG) from human plasma using a two‐column process integrating the peptide‐based adsorbents LigaGuard™, which captures non‐Ig plasma proteins in flow‐through mode, and LigaTrap™, which isolates IgG in bind‐and‐elute. Buffer composition and column loading were optimized for both adsorbents. Two process configurations were evaluated. In the first design, plasma was fed to a LigaGuard™ column to capture plasma proteins, the effluent was loaded on the LigaTrap™ column, and the bound IgG was eluted with 63.8% global recovery and 99.7% purity; in comparison, Protein G agarose afforded approximately 67% recovery and 97.2% purity. In the alternative design, the LigaGuard™ column was utilized to polish the LigaTrap™ elution stream, affording 82.3% global recovery and 98.8% purity. Collectively, these results demonstrate the potential of a fully chromatographic process for purifying polyclonal IgG from plasma feedstocks.

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Targeted Capture of Chinese Hamster Ovary Host Cell Proteins: Peptide Ligand Discovery

Cited by 33 publications

References 33 publications

Targeted capture of Chinese hamster ovary host cell proteins: Peptide ligand binding by proteomic analysis

Targeted capture of Chinese hamster ovary host cell proteins: Peptide ligand binding by proteomic analysis

Molecular Engineering of Cyclic Azobenzene‐Peptide Hybrid Ligands for the Purification of Human Blood Factor VIII via Photo‐Affinity Chromatography

Purification of polyclonal immunoglobulin G from human serum using peptide‐based adsorbents

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