Your search keyword '"protein A"' showing total 1,447 results

1. Fast quantitative determination of monoclonal antibody in infusion bags using protein A nano liquid chromatography.

Author

Andre, Claire and Guillaume, Yves Claude

Subjects

*ANIMAL genetic engineering, *CAPILLARY columns, *IMMUNOGLOBULIN G, *LIQUID chromatography, *STAPHYLOCOCCUS aureus

Abstract

Staphylococcus aureus Protein A was immobilized on an in‐house made neutravidin poly (glycidyl methacrylate‐co‐ethylene dimethacrylate) capillary column with a 25 µm internal diameter, a length of 30 mm and a mass loadability of 60 ng. The immobilized quantity of protein A on the organic monolith was very low, in the pico mole range (1.80 pmol). This was of significance importance when working with less available or expensive purified enzyme. This capillary column was integrated into a nano liquid chromatographic system and used for the fast determination without dilution of the doses of therapeutic monoclonal antibodies (mAbs) in standardized infusion bags prepared in advance in a pharmacy department. This chromatographic method was linear in the studied concentration range with good precision and accuracy. Heat stressed studies indicated that the protein A affinity capillary column was able to monitor degraded mAbs. As well, the high specificity of this column to capture immunoglobulin G2 in cell culture supernatant was visualized. As the mAbs are produced through genetic engineering of animal cells this last result demonstrated that this novel protein A column could be used in the feature for rapid screening of immunoglobulin G concentration in cell culture. [ABSTRACT FROM AUTHOR]

Published

2024

2. Harnessing the combined effect of antivirulence agent trans-chalcone with bactericidal curcumin against sortase A enzyme to tackle Gram-positive bacterial infections.

Author

Kumari, Poonam, Banerjee, Sanjay K., Murty, Upadhyayula Surayanarayana, Ravichandiran, Velayutham, and Mohan, Utpal

Abstract

Gram-positive bacteria are responsible for a wide range of infections in humans. In most Gram-positive bacteria, sortase A plays a significant role in attaching virulence factors to the bacteria's cell wall. These cell surface proteins play a significant role in virulence and pathogenesis. Even though antibiotics are available to treat these infections, there is a continuous search for an alternative strategy due to an increase in antibiotic resistance. Thus, using anti-sortase drugs to combat these bacterial infections may be a promising approach. Here, we describe a method for targeting Gram-positive bacterial infection by combining curcumin and trans-chalcone as sortase A inhibitors. We have used curcumin and trans-chalcone alone and in combination as a sortase A inhibitor. We have seen ~78%, ~43%, and ~94% inhibition when treated with curcumin, trans-chalcone, and a combination of both compounds, respectively. The compounds have also shown a significant effect on biofilm formation, IgG binding, protein A recruitment, and IgG deposition. We discovered that combining curcumin and trans-chalcone is more effective against Gram-positive bacteria than either compound alone. The present work demonstrated that a combination of these natural compounds could be used as an antivirulence therapy against Gram-positive bacterial infection. [ABSTRACT FROM AUTHOR]

Published

2024

3. Staphylococcus aureus foldase PrsA contributes to the folding and secretion of protein A

Author

Mei-Hui Lin, Chao-Chin Liu, Chiao-Wen Lu, and Jwu-Ching Shu

Subjects

Staphylococcus aureus, Foldase, PrsA, Protein A, Microbiology, QR1-502

Abstract

Abstract Background Staphylococcus aureus secretes a variety of proteins including virulence factors that cause diseases. PrsA, encoded by many Gram-positive bacteria, is a membrane-anchored lipoprotein that functions as a foldase to assist in post-translocational folding and helps maintain the stability of secreted proteins. Our earlier proteomic studies found that PrsA is required for the secretion of protein A, an immunoglobulin-binding protein that contributes to host immune evasion. This study aims to investigate how PrsA influences protein A secretion. Results We found that in comparison with the parental strain HG001, the prsA-deletion mutant HG001ΔprsA secreted less protein A. Deleting prsA also decreased the stability of exported protein A. Pulldown assays indicated that PrsA interacts with protein A in vivo. The domains in PrsA that interact with protein A are mapped to both the N- and C-terminal regions (NC domains). Additionally, the NC domains are essential for promoting PrsA dimerization. Furthermore, an immunoglobulin-binding assay revealed that, compared to the parental strain HG001, fewer immunoglobulins bound to the surface of the mutant strain HG001ΔprsA. Conclusions This study demonstrates that PrsA is critical for the folding and secretion of protein A. The information derived from this study provides a better understanding of virulent protein export pathways that are crucial to the pathogenicity of S. aureus.

Published

2024

4. Host cell protein networks as a novel co‐elution mechanism during protein A chromatography.

Author

Panikulam, Sherin, Hanke, Alexander, Kroener, Frieder, Karle, Anette, Anderka, Oliver, Villiger, Thomas K., and Lebesgue, Nicolas

Abstract

Host cell proteins (HCPs) are process‐related impurities of therapeutic proteins produced in for example, Chinese hamster ovary (CHO) cells. Protein A affinity chromatography is the initial capture step to purify monoclonal antibodies or Fc‐based proteins and is most effective for HCP removal. Previously proposed mechanisms that contribute to co‐purification of HCPs with the therapeutic protein are either HCP‐drug association or leaching from chromatin heteroaggregates. In this study, we analyzed protein A eluates of 23 Fc‐based proteins by LC‐MS/MS to determine their HCP content. The analysis revealed a high degree of heterogeneity in the number of HCPs identified in the different protein A eluates. Among all identified HCPs, the majority co‐eluted with less than three Fc‐based proteins indicating a drug‐specific co‐purification for most HCPs. Only ten HCPs co‐purified with over 50% of the 23 Fc‐based proteins. A correlation analysis of HCPs identified across multiple protein A eluates revealed their co‐elution as HCP groups. Functional annotation and protein interaction analysis confirmed that some HCP groups are associated with protein‐protein interaction networks. Here, we propose an additional mechanism for HCP co‐elution involving protein‐protein interactions within functional networks. Our findings may help to guide cell line development and to refine downstream purification strategies. [ABSTRACT FROM AUTHOR]

Published

2024

5. A Multifunctionalized Potyvirus-Derived Nanoparticle That Targets and Internalizes into Cancer Cells.

Author

Truchado, Daniel A., Juárez-Molina, María, Rincón, Sara, Zurita, Lucía, Tomé-Amat, Jaime, Lorz, Corina, and Ponz, Fernando

Subjects

*TURNIP mosaic virus, *STAPHYLOCOCCAL protein A, *CANCER cells, *NANOPARTICLES, *SQUAMOUS cell carcinoma, *FC receptors

Abstract

Plant viral nanoparticles (VNPs) are attractive to nanomedicine researchers because of their safety, ease of production, resistance, and straightforward functionalization. In this paper, we developed and successfully purified a VNP derived from turnip mosaic virus (TuMV), a well-known plant pathogen, that exhibits a high affinity for immunoglobulins G (IgG) thanks to its functionalization with the Z domain of staphylococcal Protein A via gene fusion. We selected cetuximab as a model IgG to demonstrate the versatility of this novel TuMV VNP by developing a fluorescent nanoplatform to mark tumoral cells from the Cal33 line of a tongue squamous cell carcinoma. Using confocal microscopy, we observed that fluorescent VNP–cetuximab bound selectively to Cal33 and was internalized, revealing the potential of this nanotool in cancer research. [ABSTRACT FROM AUTHOR]

Published

2024

6. Staphylococcus aureus foldase PrsA contributes to the folding and secretion of protein A.

Author

Lin, Mei-Hui, Liu, Chao-Chin, Lu, Chiao-Wen, and Shu, Jwu-Ching

Subjects

*PROTEIN folding, *PROTEIN stability, *GRAM-positive bacteria, *SURFACE strains, *PROTEOMICS

Abstract

Background: Staphylococcus aureus secretes a variety of proteins including virulence factors that cause diseases. PrsA, encoded by many Gram-positive bacteria, is a membrane-anchored lipoprotein that functions as a foldase to assist in post-translocational folding and helps maintain the stability of secreted proteins. Our earlier proteomic studies found that PrsA is required for the secretion of protein A, an immunoglobulin-binding protein that contributes to host immune evasion. This study aims to investigate how PrsA influences protein A secretion. Results: We found that in comparison with the parental strain HG001, the prsA-deletion mutant HG001ΔprsA secreted less protein A. Deleting prsA also decreased the stability of exported protein A. Pulldown assays indicated that PrsA interacts with protein A in vivo. The domains in PrsA that interact with protein A are mapped to both the N- and C-terminal regions (NC domains). Additionally, the NC domains are essential for promoting PrsA dimerization. Furthermore, an immunoglobulin-binding assay revealed that, compared to the parental strain HG001, fewer immunoglobulins bound to the surface of the mutant strain HG001ΔprsA. Conclusions: This study demonstrates that PrsA is critical for the folding and secretion of protein A. The information derived from this study provides a better understanding of virulent protein export pathways that are crucial to the pathogenicity of S. aureus. [ABSTRACT FROM AUTHOR]

Published

2024

7. Rapid and sensitive detection of glucocorticoids using engineered magnetosomes functionalized protein A conjugated broad-spectrum monoclonal antibody

Author

Jinxin He, Yuan Wang, Yaqing Hou, Fang Tang, and Jiesheng Tian

Subjects

Engineered Magnetosome, Protein A, Broad-spectrum monoclonal antibody, Immunomagnetic assay, Glucocorticoids, Nutrition. Foods and food supply, TX341-641, Food processing and manufacture, TP368-456

Abstract

Engineered bacterial magnetic nanoparticles (BMPs) fused with protein A (BMP-PA) can bind antibodies, creating immunomagnetic beads that offer an attractive tool for targets screening. In the study, BMP-PA-IgG was formed by attaching broad-spectrum monoclonal antibodies against glucocorticoids (GCs) to BMP-PA. Immunomagnetic assay was developed for analysis of GCs, using the BMP-PA-IgG and hydrocortisone-horseradish peroxidase. The developed assay exhibited broad specificity for GCs, including hydrocortisone (HCS), betamethasone (BMS), dexamethasone (DMS), prednisolone (PNS), beclomethasone (BCMS), cortisone (CS), 6-α-methylprednisone (6-α-MPNS), and fludrocortisone acetate (HFCS), with half inhibitory concentrations (IC50) ranging from 0.88 to 6.57 ng/mL. The proposed assay showed average recoveries of HCS and DMS ranging from 75.6% to 105.2% in chicken and pork samples, which were correlated well with those obtained by LC-MS/MS. This study indicated that the integration of engineered immunomagnetic beads into immunoassay systems offer possibilities for the sensitive and selective detection of GCs.

Published

2024

8. Generation and Evaluation of Gold-binding Peptide Fused Protein A.

Author

Thuy-Dung Doan-Tran, Thanh-Tan Nguyen, and Hieu Tran-Van

Subjects

*PEPTIDES, *GOLD nanoparticles, *PROTEINS, *DETECTION limit, *POUND sterling, *IMMUNOGLOBULINS

Abstract

Immobilizing antibodies onto the surface of gold nanoparticles (AuNPs) in an oriented manneris essential to achieve high sensitivity and detection limits in immunoassays and biosensors. In this research, the two-domain protein proAx1-Au-binding was generated as the result of the fusion between staphylococcalprotein A and a gold-binding peptide (GBP). This novel protein allows the fragment antigen-binding (Fab) region of captured antibodies to be exposed while binding stably to the gold surface. In this present study, we successfully constructed the recombinant pET22b-proAx1-Au-binding plasmid. The expression of proAx1-Au-binding was induced by Isopropyl β-d-1-thiogalactopyranoside (IPTG) and then confirmed by Tricine-SDS-PAGE and Western Blot.The gold-binding ability of this novel protein was evaluated and the result showed that proAx1-Au-binding had a higher affinity for AuNPs than protein A alone, thereby enhancing antibody immobilization onto AuNPs. This study laid the groundwork for facilely preparing any target-specific antibody-AuNPs. [ABSTRACT FROM AUTHOR]

Published

2023

9. Orange-spotted grouper nervous necrosis virus-encoded protein A induces interferon expression via RIG-I/MDA5-MAVS-TBK1-IRF3 signaling in fish cells

Author

Siyou Huang, Yi Huang, Taowen Su, Runqing Huang, Lianpan Su, Yujia Wu, Shaoping Weng, Jianguo He, and Junfeng Xie

Subjects

nervous necrosis virus, protein A, channel catfish, interferons, RLR signaling, RIG-I, Microbiology, QR1-502

Abstract

ABSTRACT Nervous necrosis virus (NNV), a highly contagious fish virus, has caused huge economic losses to the global aquaculture industry. A previous study showed that protein A (ProA) encoded by orange-spotted grouper NNV triggers type I interferon (IFN) production in fish cells, but the activation and modulation of correlative signal pathways remain unclear. Here, we proved that ProA induces fish cell-specific IFN promoter activation in a dose-dependent manner. In channel catfish ovary (CCO, an NNV-permissive cell), ProA evoked expression and secretion of functional IFN with anti-DNA virus activity, suggesting a good model for IFN signaling research. A contrastive study of signaling in CCO and fathead minnow (FHM, an NNV-nonpermissive cell) using RNAi knockdown or dominant negative mutant overexpression verified that ProA-mediated IFN activation went through retinoic acid-inducible gene I (RIG-I)-like receptor (RLR) pathway (RIG-I/MDA5-MAVS-TRAF3-TBK1-IRF3) while NOD1-RIPK2-NFκB and TLR3-TRIF branches were unnecessary. As RNA receptors upregulated by ProA in FHM, RIG-I and MDA5 promoted ProA-mediated IFN activation to form a positive feedback loop, while LGP2, NOD1, and PKR inhibited this activation as negative modulators. In ProA-expressed, NNV-infected CCO, the transcription of RIG-I, MDA5, MAVS, TBK1, IRF3, and IFN was downregulated, but the expression of LGP2, TRAF3, and NOD1 remained unchanged, suggesting unknown IFN suppression mechanism by NNV infection. IFN inhibition by overexpressing mutated RIG-I greatly enhanced NNV replication in FHM, implying that RIG-I might be the main target for both ProA-mediated activation and NNV infection-induced inhibition. This study provides overviews and foundations for understanding the interaction between betanodavirus-encoded protein and fish innate immune signaling. IMPORTANCE As a major pathogen, nervous necrosis virus (NNV) infects more than 120 fish species worldwide and is virulent to larvae and juvenile fish, hampering the development of the fish fry industry. Understanding virus-host interaction and underlying mechanisms is an important but largely unknown issue in fish virus studies. Here, using channel catfish ovary and fathead minnow cells as models for the study of innate immunity signaling, we found that NNV-encoded ProA activated interferon signaling via the retinoic acid-inducible gene I (RIG-I)-like receptor (RLR) pathway which was still suppressed by the infection of wild-type NNV. This finding has important implications for the comprehension of NNV protein function and the immune response from different cells. First, RIG-I is the key node for anti-NNV innate immunity. Second, the response intensity of RLR signaling determines the degree of NNV proliferation. This study expands our knowledge regarding the overview of signal pathways affected by NNV-encoded protein and also highlights potential directions for the control of aquatic viruses.

Published

2024

10. High throughput purification of monoclonal recombinant antibodies using a Protein-A coated membrane plate system.

Author

Leal-Lopes, Camila, D'Angelo, Sara, Erasmus, M. Frank, Teixeira, Andre A.R., Temples, Graham, Zhou, Jinxiang, Bradbury, Andrew R.M., and Ferrara, Fortunato

Subjects

*MONOCLONAL antibodies, *RECOMBINANT antibodies, *SURFACE plasmon resonance

Abstract

The therapeutic use of monoclonal antibodies (mAbs) ranges from cancer treatment to immune-mediated conditions, covering infectious and cardiovascular disorders, among others. The development of improved methods for therapeutic antibody discovery has accelerated the identification of numerous mAbs: a discovery campaign can be deeply mined, resulting in hundreds, even thousands, of potential antibody leads for a given target of interest. High throughput mAb expression and purification methods are required for the rapid validation of those leads. In this work, we describe the implementation of a Protein-A coated membrane plate system, the Purexa™ AHT membrane plate, for robust preparative purification of hundreds of recombinant mAbs, without the need for automation. The high efficiency (>80%) recovery generated sufficient mAb for downstream screening analyses such as ELISA and surface plasmon resonance (SPR). This new system allows the functional validation of hundreds of lead antibodies from discovery campaigns in a timely manner regardless of operational size. • A membrane plate system was implemented for the rapid purification of hundreds of mAbs. • High recovery efficiency generates sufficient mass for mAbs functional screening. • Purification plate can be reused for at least 6 purification cycles. • Method is fast, affordable and does not require automation. [ABSTRACT FROM AUTHOR]

Published

2023

11. The immune evasion roles of Staphylococcus aureus protein A and impact on vaccine development.

Author

Bear, Alex, Locke, Thomas, Rowland-Jones, Sarah, Pecetta, Simone, Bagnoli, Fabio, and Darton, Thomas C.

Subjects

VACCINE development, COMPLEMENT activation, MONOCLONAL antibodies, OPPORTUNISTIC infections, PROTEINS, IMMUNE response

Abstract

While Staphylococcus aureus (S. aureus) bacteria are part of the human commensal flora, opportunistic invasion following breach of the epithelial layers can lead to a wide array of infection syndromes at both local and distant sites. Despite ubiquitous exposure from early infancy, the life-long risk of opportunistic infection is facilitated by a broad repertoire of S. aureus virulence proteins. These proteins play a key role in inhibiting development of a long-term protective immune response by mechanisms ranging from dysregulation of the complement cascade to the disruption of leukocyte migration. In this review we describe the recent progress made in dissecting S. aureus immune evasion, focusing on the role of the superantigen, staphylococcal protein A (SpA). Evasion of the normal human immune response drives the ability of S. aureus to cause infection, often recurrently, and is also thought to be a major hindrance in the development of effective vaccination strategies. Understanding the role of S. aureus virulence protein and determining methods overcoming or subverting these mechanisms could lead to much-needed breakthroughs in vaccine and monoclonal antibody development. [ABSTRACT FROM AUTHOR]

Published

2023

12. Different Strategies for Bio-Conjugation of Anti-CD4 Monoclonal Antibodies to Silica-Coated Magnetic Nanoparticles and Their Application for the Positive Selection of CD4+ Lymphocytes.

Author

Khorrami, M., Mahmoudi, M., Shobeiri, S. S., Moghadam, M., and Sankian, M.

Subjects

*MONONUCLEAR leukocytes, *MAGNETIC nanoparticles, *MONOCLONAL antibodies, *MAGNETICS, *LYMPHOCYTES, *T cells, *CHO cell

Abstract

Efficient cell separation techniques are required for the isolation of various cellular populations in fundamental research. In the present study, five types of magnetic nanoparticles (MNPs) have been designed to isolate CD4+ T cells from peripheral blood mononuclear cells. MNPs were synthesized by a modified solvothermal method and subsequently coated by a silica shell through the sol-gel process. Then, the anti-CD4 antibody was conjugated on the surface of different groups of MNPs, which were functionalized with various cross-linkers (including the carboxylic and aldehyde groups) and proteins (such as protein A and streptavidin). The performance of prepared MNPs for the separation of CD4+ lymphocytes was investigated by optical microscopy and flow-cytometry. This study revealed that the cell isolation rates by different functionalized groups, including aldehyde, carboxyl, CHO-protein A, COOH-protein A, and streptavidin conjugated with nanoparticles, were 32 ± 3, 32 ± 1, 80 ± 4, 70 ± 1, and 71 ± 2%, respectively. Based on such data, the CHO-protein A-functionalized MNPs have been considered a practical choice to separate CD4+ T cells with over 92 ± 3% purity. MNPs obtained in the study provide an adequate tool for the cell isolation method and further present the dramatic potential to be applied to several fields of biomedical purpose. [ABSTRACT FROM AUTHOR]

Published

2023

13. Performance of a new family of modular, bed‐supported, chromatography devices.

Author

Platteau, Gerald, Stroehlein, Guido, Alstine, James Van, and Nagaya, Masayoshi

Abstract

Prepacked chromatography columns and cassette filtration units offer many advantages in bioprocessing. These include reduced labor costs and processing times, ease of storage, and enhanced process flexibility. Rectangular formats are particularly attractive as they can be easily stacked and multiplexed together for continuous processing. Cylindrical chromatography beds have dominated bioprocessing even though their bed support and pressure‐flow performance vary with bed dimensions. This work presents the performance of novel, rhombohedral chromatography devices with internally supported beds. They are compatible with existing chromatography workstations and can be packed with any standard commercial resin. The devices offer pressure‐flow characteristics independent of container‐volume, simple multiplexing, and separation performance comparable to cylindrical columns. Their bi‐planar, internal bed support allows mechanically less‐rigid resins to be used at up to four times higher maximal linear velocities, and productivities approaching 200 g/L/h for affinity resins, compared to the 20 g/L/h typical of many column‐based devices. Three 5 L devices should allow processing of up to 3 kg of monoclonal antibody per hour. [ABSTRACT FROM AUTHOR]

Published

2023

14. Facile Purification and Use of Tobamoviral Nanocarriers for Antibody-Mediated Display of a Two-Enzyme System.

Author

Wendlandt, Tim, Koch, Claudia, Britz, Beate, Liedek, Anke, Schmidt, Nora, Werner, Stefan, Gleba, Yuri, Vahidpour, Farnoosh, Welden, Melanie, Poghossian, Arshak, Schöning, Michael J., Eber, Fabian J., Jeske, Holger, and Wege, Christina

Subjects

*SURFACE plasmon resonance, *MULTIENZYME complexes, *DISPLAY systems, *GLUCOSE oxidase, *HORSERADISH peroxidase, *NANOCARRIERS

Abstract

Immunosorbent turnip vein clearing virus (TVCV) particles displaying the IgG-binding domains D and E of Staphylococcus aureus protein A (PA) on every coat protein (CP) subunit (TVCVPA) were purified from plants via optimized and new protocols. The latter used polyethylene glycol (PEG) raw precipitates, from which virions were selectively re-solubilized in reverse PEG concentration gradients. This procedure improved the integrity of both TVCVPA and the wild-type subgroup 3 tobamovirus. TVCVPA could be loaded with more than 500 IgGs per virion, which mediated the immunocapture of fluorescent dyes, GFP, and active enzymes. Bi-enzyme ensembles of cooperating glucose oxidase and horseradish peroxidase were tethered together on the TVCVPA carriers via a single antibody type, with one enzyme conjugated chemically to its Fc region, and the other one bound as a target, yielding synthetic multi-enzyme complexes. In microtiter plates, the TVCVPA-displayed sugar-sensing system possessed a considerably increased reusability upon repeated testing, compared to the IgG-bound enzyme pair in the absence of the virus. A high coverage of the viral adapters was also achieved on Ta2O5 sensor chip surfaces coated with a polyelectrolyte interlayer, as a prerequisite for durable TVCVPA-assisted electrochemical biosensing via modularly IgG-assembled sensor enzymes. [ABSTRACT FROM AUTHOR]

Published

2023

15. A Multifunctionalized Potyvirus-Derived Nanoparticle That Targets and Internalizes into Cancer Cells

Author

Daniel A. Truchado, María Juárez-Molina, Sara Rincón, Lucía Zurita, Jaime Tomé-Amat, Corina Lorz, and Fernando Ponz

Subjects

turnip mosaic virus, VLP, protein A, Z domain, cetuximab, squamous cell carcinoma, Biology (General), QH301-705.5, Chemistry, QD1-999

Abstract

Plant viral nanoparticles (VNPs) are attractive to nanomedicine researchers because of their safety, ease of production, resistance, and straightforward functionalization. In this paper, we developed and successfully purified a VNP derived from turnip mosaic virus (TuMV), a well-known plant pathogen, that exhibits a high affinity for immunoglobulins G (IgG) thanks to its functionalization with the Z domain of staphylococcal Protein A via gene fusion. We selected cetuximab as a model IgG to demonstrate the versatility of this novel TuMV VNP by developing a fluorescent nanoplatform to mark tumoral cells from the Cal33 line of a tongue squamous cell carcinoma. Using confocal microscopy, we observed that fluorescent VNP–cetuximab bound selectively to Cal33 and was internalized, revealing the potential of this nanotool in cancer research.

Published

2024

16. The immune evasion roles of Staphylococcus aureus protein A and impact on vaccine development

Author

Alex Bear, Thomas Locke, Sarah Rowland-Jones, Simone Pecetta, Fabio Bagnoli, and Thomas C. Darton

Subjects

Staphylococcus aureus, Protein A, immune evasion, super antigen, vaccine development, B cells, Microbiology, QR1-502

Abstract

While Staphylococcus aureus (S. aureus) bacteria are part of the human commensal flora, opportunistic invasion following breach of the epithelial layers can lead to a wide array of infection syndromes at both local and distant sites. Despite ubiquitous exposure from early infancy, the life-long risk of opportunistic infection is facilitated by a broad repertoire of S. aureus virulence proteins. These proteins play a key role in inhibiting development of a long-term protective immune response by mechanisms ranging from dysregulation of the complement cascade to the disruption of leukocyte migration. In this review we describe the recent progress made in dissecting S. aureus immune evasion, focusing on the role of the superantigen, staphylococcal protein A (SpA). Evasion of the normal human immune response drives the ability of S. aureus to cause infection, often recurrently, and is also thought to be a major hindrance in the development of effective vaccination strategies. Understanding the role of S. aureus virulence protein and determining methods overcoming or subverting these mechanisms could lead to much-needed breakthroughs in vaccine and monoclonal antibody development.

Published

2023

17. Non-Affinity Purification of Antibodies.

Author

Arakawa, Tsutomu, Tomioka, Yui, Nakagawa, Masataka, Sakuma, Chiaki, Kurosawa, Yasunori, Ejima, Daisuke, Tsumoto, Kouhei, and Akuta, Teruo

Subjects

*IMMUNOGLOBULINS, *COLUMN chromatography, *GEL electrophoresis, *AGAROSE

Abstract

Currently, purification of antibodies is mainly carried out using a platform technology composed primarily of Protein A chromatography as a capture step, regardless of the scale. However, Protein A chromatography has a number of drawbacks, which are summarized in this review. As an alternative, we propose a simple small-scale purification protocol without Protein A that uses novel agarose native gel electrophoresis and protein extraction. For large-scale antibody purification, we suggest mixed-mode chromatography that can in part mimic the properties of Protein A resin, focusing on 4-Mercapto-ethyl-pyridine (MEP) column chromatography. [ABSTRACT FROM AUTHOR]

Published

2023

18. Development of a New Affinity Gold Polymer Membrane with Immobilized Protein A

Author

Tobias Steegmüller, Tim Kratky, Lena Gollwitzer, Sebastian Patrick Schwaminger, and Sonja Berensmeier

Subjects

affinity membrane chromatography, protein A, antibody purification, protein immobilization, gold membrane, Chemical technology, TP1-1185, Chemical engineering, TP155-156

Abstract

New and highly selective stationary phases for affinity membrane chromatography have the potential to significantly enhance the efficiency and specificity of therapeutic protein purification by reduced mass transfer limitations. This work developed and compared different immobilization strategies for recombinant Protein A ligands to a gold-sputtered polymer membrane for antibody separation in terms of functionalization and immobilization success, protein load, and stability. Successful, functionalization was validated via X-ray photoelectron spectroscopy (XPS). Here, a recombinant Protein A ligand was coupled by N-hydroxysuccinimide (NHS)/N-(3-dimethylaminopropyl)-N′-ethylcarbodiimide (EDC) chemistry to carboxy-functionalized, gold-sputtered membranes. We achieved a binding capacity of up to 104 ± 17 mg of the protein ligand per gram of the gold-sputtered membrane. The developed membranes were able to successfully capture and release the monoclonal antibody (mAb) Trastuzumab, as well as antibodies from fresh frozen human blood plasma in both static and dynamic setups. Therefore, they demonstrated successful functionalization and immobilization strategies. The antibody load was tested using bicinchoninic acid (BCA), ultraviolet-visible spectroscopy (UV-vis) measurements, and sodium dodecyl sulfate polyacrylamide gel electrophoresis (SDS-PAGE). The outcome is a fully functional affinity membrane that can be implemented in a variety of different antibody purification processes, eliminating the need for creating individualized strategies for modifying the surface to suit different substrates or conditions.

Published

2024

19. Sortase-promoted synthesis of homooligomers from a monomeric protein.

Author

Melikhova, Tatiana D., Bovin, Nicolai V., Antipov, Aleksandr D., Tereshin, Mikhail N., Ziganshin, Rustam H., and Tuzikov, Alexander B.

Subjects

*RECOMBINANT proteins, *PROTEINS, *ANTENNAS (Electronics)

Abstract

[Display omitted] We demonstrated covalent cross-linking of two or three protein molecules specifically at the C-terminus by sortase-catalyzed conjugation of recombinant proteins with conformationally rigid-flexible tetraantennary templates, where structure of the antenna is [Gly-Gly-(N -CH 2 COOH)Gly] n CH 2 –. [ABSTRACT FROM AUTHOR]

Published

2023

20. TRIM21 chimeric protein as a new molecular tool for multispecies IgG detection

Author

Anelize Felicio Ramos, Leonardo Antônio Fernandes, Franciane Batista, Bianca de Souza Vieira, Mayerson Thompson, Jacó Joaquim Mattos, Maria Risoleta Freire Marques, Maria de Lourdes Borba Magalhães, and Gustavo Felippe da Silva

Subjects

Antibody, Protein A, Protein G, Immunoglobulin, Protein engineering, ELISA, Biotechnology, TP248.13-248.65, Genetics, QH426-470

Abstract

Abstract Background The production of monoclonal antibodies for immunoglobulin detection is not cost-effective, while polyclonal antibody production depends on laboratory animals, raising concerns on animal welfare. The widespread use of immunoglobulins in the pharmaceutical industry and the increasing number and variety of new antibodies entering the market require new detection and purification strategies. The Tripartite motif-containing protein 21 is a soluble intracellular immunoglobulin G receptor that binds to the constant region of immunoglobulin G from various species with high affinity. We hypothesized that using this protein as an antibody-binding module to create immunoglobulin detection probes will improve the portfolio of antibody affinity ligands for diagnostic or therapeutic purposes. Results We created a chimeric protein containing a mutated form of the C-terminal domain of mouse Tripartite motif-containing protein 21 linked to streptavidin to detect immunoglobulin G from various species of mammals. The protein is produced by heterologous expression and consists of an improved molecular tool, expanding the portfolio of antibody-affinity ligands for immunoassays. We also demonstrate that this affinity ligand may be used for purification purposes since imidazole elution of antibodies can be achieved instead of acidic elution conditions of current antibody purification methods. Conclusion Data reported here provides an additional and superior alternative to the use of secondary antibodies, expanding the portfolio of antibodies affinity ligands for detection and purification purposes.

Published

2022

21. Expression and Characterization of Intein-Cyclized Trimer of Staphylococcus aureus Protein A Domain Z.

Author

Nandy, Suman, Maranholkar, Vijay M., Crum, Mary, Wasden, Katherine, Patil, Ujwal, Goyal, Atul, Vu, Binh, Kourentzi, Katerina, Mo, William, Henrickson, Amy, Demeler, Borries, Sen, Mehmet, and Willson, Richard C.

Subjects

*PROTEIN domains, *SURFACE plasmon resonance, *ISOTHERMAL titration calorimetry, *STAPHYLOCOCCUS aureus, *PROTEIN engineering, *FC receptors, *TANDEM mass spectrometry, *MICROCOCCACEAE

Abstract

Staphylococcus aureus protein A (SpA) is an IgG Fc-binding virulence factor that is widely used in antibody purification and as a scaffold to develop affinity molecules. A cyclized SpA Z domain could offer exopeptidase resistance, reduced chromatographic ligand leaching after single-site endopeptidase cleavage, and enhanced IgG binding properties by preorganization, potentially reducing conformational entropy loss upon binding. In this work, a Z domain trimer (Z3) was cyclized using protein intein splicing. Interactions of cyclic and linear Z3 with human IgG1 were characterized by differential scanning fluorimetry (DSF), surface plasmon resonance (SPR), and isothermal titration calorimetry (ITC). DSF showed a 5 ℃ increase in IgG1 melting temperature when bound by each Z3 variant. SPR showed the dissociation constants of linear and cyclized Z3 with IgG1 to be 2.9 nM and 3.3 nM, respectively. ITC gave association enthalpies for linear and cyclic Z3 with IgG1 of −33.0 kcal/mol and −32.7 kcal/mol, and −T∆S of association 21.2 kcal/mol and 21.6 kcal/mol, respectively. The compact cyclic Z3 protein contains 2 functional binding sites and exhibits carboxypeptidase Y-resistance. The results suggest cyclization as a potential approach toward more stable SpA-based affinity ligands, and this analysis may advance our understanding of protein engineering for ligand and drug development. [ABSTRACT FROM AUTHOR]

Published

2023

22. TRIM21 chimeric protein as a new molecular tool for multispecies IgG detection.

Author

Ramos, Anelize Felicio, Fernandes, Leonardo Antônio, Batista, Franciane, de Souza Vieira, Bianca, Thompson, Mayerson, Mattos, Jacó Joaquim, Marques, Maria Risoleta Freire, de Lourdes Borba Magalhães, Maria, and da Silva, Gustavo Felippe

Abstract

Background: The production of monoclonal antibodies for immunoglobulin detection is not cost-effective, while polyclonal antibody production depends on laboratory animals, raising concerns on animal welfare. The widespread use of immunoglobulins in the pharmaceutical industry and the increasing number and variety of new antibodies entering the market require new detection and purification strategies. The Tripartite motif-containing protein 21 is a soluble intracellular immunoglobulin G receptor that binds to the constant region of immunoglobulin G from various species with high affinity. We hypothesized that using this protein as an antibody-binding module to create immunoglobulin detection probes will improve the portfolio of antibody affinity ligands for diagnostic or therapeutic purposes. Results: We created a chimeric protein containing a mutated form of the C-terminal domain of mouse Tripartite motif-containing protein 21 linked to streptavidin to detect immunoglobulin G from various species of mammals. The protein is produced by heterologous expression and consists of an improved molecular tool, expanding the portfolio of antibody-affinity ligands for immunoassays. We also demonstrate that this affinity ligand may be used for purification purposes since imidazole elution of antibodies can be achieved instead of acidic elution conditions of current antibody purification methods. Conclusion: Data reported here provides an additional and superior alternative to the use of secondary antibodies, expanding the portfolio of antibodies affinity ligands for detection and purification purposes. [ABSTRACT FROM AUTHOR]

Published

2022

23. Different Strategies for Bio-Conjugation of Anti-CD4 Monoclonal Antibodies to Silica-Coated Magnetic Nanoparticles and Their Application for the Positive Selection of CD4+ Lymphocytes

Author

Khorrami, M., Mahmoudi, M., Shobeiri, S. S., Moghadam, M., and Sankian, M.

Published

2023

24. Safety assessment of protein A and derivation of a parenteral health-based exposure limit.

Author

Graham, Jessica C., Anand, Sathanandam S., Bercu, Joel, Besenhofer, Lauren, de Zafra, Christina, Feng, Yu, Fisher, Craig, Hillegass, Jedd, Hutchinson, Richard, Jolly, Robert, Moudgal, Chandrika, Nicholas, Tyler, Olszova, Daniela, Schmitz, Matthew, and Semmelmann, Florian

Subjects

*BACTERIAL cell walls, *IMMUNOGLOBULIN G, *STAPHYLOCOCCUS aureus, *DATABASES, *CELL anatomy

Abstract

Protein A (PA) is a bacterial cell wall component of Staphylococcus aureus whose function is to bind to Immunoglobulin G (IgG). Given its ability to bind IgG as well as its stability and resistance to harsh acidic and basic cleaning conditions, it is commonly used in the affinity chromotography purification of biotherapeutics. This use can result in levels of PA being present in a drug product and subsequent patient exposure. Interestingly, PA was previously evaluated in clinical trials as well as supporting nonclinical studies, resulting in a database that enables the derivation of a health-based exposure limit (HBEL). Given the widespread use of PA in the pharmaceutical industry, the IQ DruSafe Impurities Safety Working Group (WG) evaluated the available information with the purpose of establishing a harmonized parenteral HBEL for PA. Based on this thorough, collaborative evaluation of nonclinical and clinical data available for PA, a parenteral HBEL of 1.2 μg/kg/dose (60 μg/dose for a 50 kg individual) is expected to be health protective for patients when it is present as an impurity in a biotherapeutic. [Display omitted] • PA is used in the purification of biotherapeutics and can be an impurity in a DP. • PA has been evaluated in nonclinical studies and clinical trials. • The parenteral HBEL for PA based on available nonclinical data is 3 μg/kg. • The parenteral HBEL for PA based on available clinical data is 1.2 μg/kg. • A conservative parenteral HBEL for PA is 1.2 μg/kg/dose. [ABSTRACT FROM AUTHOR]

Published

2024

25. The effects of Staphylococcus aureus protein a (SpA) on the expression of inflammatory cytokines in autoimmune patients and their probable immune response modulation mechanisms.

Author

Rigi, Garshasb, Kardar, Gholamali, Hajizade, Abbas, Zamani, Javad, and Ahmadian, Gholamreza

Subjects

*MONONUCLEAR leukocytes, *ESCHERICHIA coli, *RECOMBINANT proteins, *RECOMBINANT drugs, *IMMUNOREGULATION

Abstract

• The recombinant truncated SpA significantly reduced the expression of the cytokines. • The truncated SpA reduced the cytokines secretion more than full-length SpA and Enbrel. • In the truncated form of SpA the IgG-binding domains find a more exposed to IgG. The recombinant Staphylococcal protein A (SpA) is widely used in biotechnology to purify polyclonal and monoclonal IgG antibodies. At very low concentrations, the highly-purified form of the protein A can down-regulate the activation of human B-lymphocytes and macrophages which are the key cells in determining autoimmune diseases. In the present study, the efficiency of three different forms of protein A, including native full-length SpA, the recombinant full-length SpA, and a recombinant truncated form of SpA on the reduction of 4 inflammatory cytokines, including IL-8, IL-1β, TNF-α, and IL-6 by peripheral blood mononuclear cell (PBMCs) were studied and compared to an anti-rheumatoid arthritis commercial drug, Enbrel. The recombinant proteins were expressed in E. coli and the native form of SpA was commercially provided. PBMCs were obtained from adult patients with active rheumatoid arthritis (RA) and healthy control donors. Then, the effect of different doses of the three pure forms of SpA in comparison with Enbrel was investigated by analyzing the expression of selected cytokines using ELISA. The results showed that the truncated form of recombinant SpA significantly reduced the expression of cytokines more effectively than the other full-length formulations as well as the commercial drug Enbrel. In silico analysis shows that in the truncated protein, as the radius of gyration increases, the structure of IgG-binding domains become more open and more exposed to IgG. To summarize, our findings indicate that the truncated form of protein A is the most efficient form of SpA as it significantly decreases the secretion of evaluated cytokines from PBMCs in vitro. [ABSTRACT FROM AUTHOR]

Published

2024

26. Preparation of Protein A Membrane Adsorbers Using Strain-Promoted, Copper-Free Dibenzocyclooctyne (DBCO)-Azide Click Chemistry

Author

Joshua Osuofa and Scott M. Husson

Subjects

Protein A, membrane chromatography, alkyne–azide, copper-free click chemistry, antibody purification, Chemical technology, TP1-1185, Chemical engineering, TP155-156

Abstract

Protein A chromatography is the preferred unit operation for purifying Fc-based proteins. Convective chromatography technologies, like membrane adsorbers, can perform the purification rapidly and improve throughput dramatically. While the literature reports the preparation of Protein A membrane adsorbers utilizing traditional coupling chemistries that target lysine or thiol groups on the Protein A ligand, this study demonstrates a new approach utilizing copper-free dibenzocyclooctyne (DBCO)-azide click chemistry. The synthetic pathway consists of three main steps: bioconjugation of Protein A with a DBCO-polyethylene glycol (PEG) linker, preparation of an azide-functionalized membrane surface, and click reaction of DBCO-Protein A onto the membrane surface. Using polyclonal human immunoglobulins (hIgG) as the target molecule, Protein A membranes prepared by this synthetic pathway showed a flowrate-independent dynamic binding capacity of ~10 mg/mL membrane at 10% breakthrough. Fitting of static binding capacity measurements to the Langmuir adsorption isotherm showed a maximum binding (qmax) of 27.48 ± 1.31 mg/mL and an apparent equilibrium dissociation constant (Kd) of value of 1.72 × 10−1 ± 4.03 × 10−2 mg/mL. This work represents a new application for copper-less click chemistry in the membrane chromatography space and outlines a synthetic pathway that can be followed for immobilization of other ligands.

Published

2023

27. Scalability of Sartobind® Rapid A Membrane for High Productivity Monoclonal Antibody Capture

Author

Sabrina Yang, Ryszard Braczkowski, Shih-Hsun Chen, Ricarda Busse, Yudhi Li, Louis Fabri, and Innocent Berbelle Bekard

Subjects

monoclonal antibody, protein A, membrane chromatography, bioprocessing, rapid cycling, process intensification, Chemical technology, TP1-1185, Chemical engineering, TP155-156

Abstract

Improved upstream titres in therapeutic monoclonal antibody (mAb) production have shifted capacity constraints to the downstream process. The consideration of membrane-based chromatographic devices as a debottlenecking option is gaining increasing attention with the recent introduction of high-capacity bind and elute membranes. We have evaluated the performance and scalability of the Sartobind® Rapid A affinity membrane (1 mL) for high-productivity mAb capture. For scalability assessment, a 75 mL prototype device was used to process 100 L of clarified cell culture harvest (CH) on a novel multi-use rapid cycling chromatography system (MU-RCC). MabSelect™ PrismA (4.7 mL) was used as a benchmark comparator for Protein A (ProtA) resin studies. Results show that in addition to a productivity gain of >10×, process and product quality attributes were either improved or comparable to the benchmark. Concentrations of eluate pools were 7.5× less than that of the benchmark, with the comparatively higher bulk volume likely to cause handling challenges at process scale. The MU-RCC system is capable of membrane operation at pilot scale with comparable product quality profile to the 1 mL device. The Sartobind® Rapid A membrane is a scalable alternative to conventional ProtA resin chromatography for the isolation and purification of mAbs from harvested cell culture media.

Published

2023

28. Facile Purification and Use of Tobamoviral Nanocarriers for Antibody-Mediated Display of a Two-Enzyme System

Author

Tim Wendlandt, Claudia Koch, Beate Britz, Anke Liedek, Nora Schmidt, Stefan Werner, Yuri Gleba, Farnoosh Vahidpour, Melanie Welden, Arshak Poghossian, Michael J. Schöning, Fabian J. Eber, Holger Jeske, and Christina Wege

Subjects

turnip vein clearing virus (TVCV), tobacco mosaic virus (TMV), tobamovirus, enzyme nanocarrier, protein A, antibody, Microbiology, QR1-502

Abstract

Immunosorbent turnip vein clearing virus (TVCV) particles displaying the IgG-binding domains D and E of Staphylococcus aureus protein A (PA) on every coat protein (CP) subunit (TVCVPA) were purified from plants via optimized and new protocols. The latter used polyethylene glycol (PEG) raw precipitates, from which virions were selectively re-solubilized in reverse PEG concentration gradients. This procedure improved the integrity of both TVCVPA and the wild-type subgroup 3 tobamovirus. TVCVPA could be loaded with more than 500 IgGs per virion, which mediated the immunocapture of fluorescent dyes, GFP, and active enzymes. Bi-enzyme ensembles of cooperating glucose oxidase and horseradish peroxidase were tethered together on the TVCVPA carriers via a single antibody type, with one enzyme conjugated chemically to its Fc region, and the other one bound as a target, yielding synthetic multi-enzyme complexes. In microtiter plates, the TVCVPA-displayed sugar-sensing system possessed a considerably increased reusability upon repeated testing, compared to the IgG-bound enzyme pair in the absence of the virus. A high coverage of the viral adapters was also achieved on Ta2O5 sensor chip surfaces coated with a polyelectrolyte interlayer, as a prerequisite for durable TVCVPA-assisted electrochemical biosensing via modularly IgG-assembled sensor enzymes.

Published

2023

29. Rapid Point-of-Care Tests Using Staphylococcal Protein A Can Detect Early IgM Responses in HIV-1 and Treponema pallidum Infections

Author

Valentina A. Schmidt, Victoria Rose Stevens, Javan Esfandiari, and Konstantin P. Lyashchenko

Subjects

antibody, IgM, protein A, HIV, syphilis, serodiagnosis, Microbiology, QR1-502

Abstract

ABSTRACT Serological assays detecting IgM antibodies in addition to IgG antibodies have a diagnostic advantage in finding early infections. Staphylococcal protein A (SpA), widely used as an antibody-detecting reagent in various immunoassays, is considered to have a high binding affinity mainly to IgG, although its interaction with other classes of immunoglobulins has also been documented. Using 28 samples from 22 HIV-1 seroconversion panels, the present study demonstrated detection of early IgM antibodies by SpA-based rapid point-of-care tests, including DPP HIV 1/2, DPP HIV-Syphilis, STAT-PAK HIV 1/2, and Sure Check HIV 1/2. Samples with predominant IgM antibodies were identified by in-house IgM assays and confirmed by pretreatment with 0.1 M 2-mercaptoethanol. Likewise, the detection of treponemal IgM antibodies was shown by DPP HIV-Syphilis assay in eight samples collected at early syphilis infection. Direct interaction between IgM and SpA immobilized in solid phase or in solution was demonstrated with purified human polyclonal IgM. A strong correlation was found between the antibody levels detected by SpA and anti-IgM reagent in the early seroconversion samples, thus supporting the evidence for IgM binding by SpA. These assays demonstrated the ability to detect IgM antibodies, which may increase test sensitivity in early infections due to a reduced serodiagnostic window. IMPORTANCE Sexually transmitted infections, including HIV and syphilis, remain a global public health concern. The main laboratory testing approach for HIV and syphilis relies on serological assays. Detection of the IgM class of antibodies may have a diagnostic advantage in finding early infections. The present study using well-characterized HIV-1 and syphilis samples has demonstrated that staphylococcal protein A employed for antibody detection in rapid point-of-care tests, including DPP HIV 1/2, DPP HIV-Syphilis, STAT-PAK HIV 1/2, and Sure Check HIV 1/2, can capture IgM antibodies in addition to IgG antibodies. The findings strongly suggest that the ability to detect IgM antibodies by these immunoassays may facilitate the identification of acute-stage HIV and syphilis infections.

Published

2022

30. Development of solid support using protein A for the measurement of free thyroxine in human serum.

Author

Gnanasekar, Rani, Murhekar, Vishwas, and Kadwad, V B

Subjects

*IMMOBILIZED proteins, *RADIOIMMUNOASSAY, *THYROXINE, *PROTEINS, *STAPHYLOCOCCUS aureus, *CELL anatomy

Abstract

Protein A is a 56 kDa cell wall component of Staphylococcus aureus. It binds to the Fc part of the antibody with high affinity. Therefore, it can be used for the purification of antibodies in a plethora of applications. Additionally, it was applied for the immobilization of antibodies to solid supports. Herein, the development of free thyroxine radioimmunoassay (FT4 RIA) using protein A for immobilizing anti-T4 antibodies in the polystyrene tubes is described. 250µL of 5 µg/mL solution was sufficient to yield maximum coating efficiency with uniform and stable antibody-coated tubes with very less nonspecific binding. This approach was economical with respect to the consumption of antibodies and the time required for the preparation of antibody-coated tubes. This resulted in a FT4 assay with a sensitivity of 1pg/mL, with intra and inter-assay variation of less than 9.6 and 11.5% respectively, analyzed at three different FT4 concentrations. The developed system correlated well with the established FT4 RIA kit with a correlation coefficient of 0.985. [ABSTRACT FROM AUTHOR]

Published

2022

31. Mechanistic modeling of continuous capture step purification of biosimilar monoclonal antibody therapeutic.

Author

Deulgaonkar, Prashant, Bhambure, Rahul, Prasad, Bhaskarjyoti, Mishra, Ashok, Tiwari, Sanjay, and Mody, Rustom

Subjects

STANDARD deviations, AFFINITY chromatography, MONOCLONAL antibodies, ECCENTRIC loads

Abstract

BACKGROUND Continuous multicolumn Protein A chromatography offers various advantages for capture stage purification of monoclonal antibody therapeutics, like higher productivity and resin capacity utilization, lower buffer consumption, small footprint, etc. Due to the complexity of the continuous process, experimental optimization is time‐consuming and cost‐intensive. This investigation proposes a hybrid process development approach integrating experimental and mechanistic modeling for time‐ and cost‐effective development and optimization of continuous Protein A affinity chromatography. RESULTS: Productivity and capacity utilization of the continuous CaptureSMB process under varying operating conditions were predicted using the Chromatography Analysis and Design Toolkit (CADET) framework and validated with experimental results. Effects of critical process parameters like feed concentration (c0), loading breakthrough (s) and residence time (RT) on productivity and capacity utilization were evaluated. Model predictions were validated using the experimental results proving the reliability and feasibility of the modeling approach. At 15.00 ± 0.20 mg mL–1 feed model mAb concentration, the model‐based approach predicted the best performance giving 27.56 g L–1 h–1 productivity (RT = 2 min, s = 80%) using MabSelect™ PrismA resin. This productivity prediction was validated by performing the continuous CaptureSMB experiment at the same operating conditions and was found to be 25.59 g L–1 h–1 with a root mean square error of 1.96. CONCLUSIONS: The hybrid process development and optimization approach for CaptureSMB purification of biosimilar mAb purification is demonstrated and validated using the experimental and model‐based framework. The observed results showcase the effectiveness of the proposed hybrid process development approach, enabling a better understanding of the chromatography process and parameters affecting the CaptureSMB process. © 2021 Society of Chemical Industry (SCI). [ABSTRACT FROM AUTHOR]

Published

2022

32. Glycan-specific IgM is critical for human immunity to Staphylococcus aureus.

Author

Hendriks A, Kerkman PF, Varkila MRJ, Haitsma Mulier JLG, Ali S, Ten Doesschate T, van der Vaart TW, de Haas CJC, Aerts PC, Cremer OL, Bonten MJM, Nizet V, Liu GY, Codée JDC, Rooijakkers SHM, van Strijp JAG, and van Sorge NM

Subjects

Humans, Teichoic Acids immunology, Animals, Female, Male, Phagocytosis immunology, Bacteremia immunology, Bacteremia microbiology, Mice, Adult, Middle Aged, Opsonization immunology, Staphylococcus aureus immunology, Immunoglobulin M immunology, Immunoglobulin M blood, Staphylococcal Infections immunology, Staphylococcal Infections microbiology, Immunoglobulin G immunology, Immunoglobulin G blood, Antibodies, Bacterial immunology, Antibodies, Bacterial blood, Polysaccharides immunology

Abstract

Staphylococcus aureus is a major human pathogen, yet the immune factors that protect against infection remain elusive. High titers of opsonic IgG antibodies, achieved in preclinical animal immunization studies, have consistently failed to provide protection in humans. Here, we investigate antibody responses to the conserved S. aureus surface glycan wall teichoic acid (WTA) and detect the presence of WTA-specific IgM and IgG antibodies in the plasma of healthy individuals. Functionally, WTA-specific IgM outperforms IgG in opsonophagocytic killing of S. aureus and protects against disseminated S. aureus bacteremia through passive immunization. In a clinical setting, patients with S. aureus bacteremia have significantly lower WTA-specific IgM but similar IgG levels compared to healthy controls. Importantly, low WTA-IgM levels correlate with disease mortality and impaired bacterial opsonization. Our findings may guide risk stratification of hospitalized patients and inform future design of antibody-based therapies and vaccines against serious S. aureus infection., Competing Interests: Declaration of interests The authors declare no competing interests., (Copyright © 2024 The Author(s). Published by Elsevier Inc. All rights reserved.)

Published

2024

33. The first report on the sortase-mediated display of bioactive protein A from Staphylococcus aureus (SpA) on the surface of the vegetative form of Bacillus subtilis

Author

Samira Ghaedmohammadi and Gholamreza Ahmadian

Subjects

Surface display, Bacillus subtilis, Protein A, Microbiology, QR1-502

Abstract

Abstract Protein A (SpA) is one of the most important Staphylococcus aureus cell wall proteins. It includes five immunoglobulin (Ig)-binding domains which can bind to immune complexes through the Fc region of immunoglobulins. The binding of SpA to the polymeric supports can be used to prepare affinity chromatography resins, which are useful for immunoprecipitation (IP) of antibodies. Protein A is also used to purify many anti-cancer antibodies. In this study, SpA was displayed on the surface of Bacillus subtilis cells using a sortase-mediated system to display the target protein to the B. subtilis cell wall. A series of plasmids consisting of cassettes for cell wall-directed protein A as well as negative controls were constructed and transformed into B. subtilis WASD (wprA sigD) cells. SDS-PAGE, western blot, flow cytometry, functional IgG purification assay, and a modified ELISA assay were used to confirm the surface display of SpA and evaluate its function. Semi-quantitative ELISA results showed that the binding capacity of lyophilized Bs-SpA is 100 μg IgG from rabbit serum per 1 mg of cells under optimal experimental conditions. Low production costs, optimal performance, and the use of a harmless strain compared to a similar commercial product predict the possible use of SpA immobilization technology in the future.

Published

2021

34. Optimization of multi flow rate loading strategy for process intensification of Protein A chromatography

Author

Anjali Ramakrishna, Vijay Maranholkar, Sandeep Hadpe, Jyoti Iyer, and Anurag Rathore

Subjects

Affinity chromatography, Protein A, Resin utilization, Productivity, High capacity capture, Multi flow rate loading, Analytical chemistry, QD71-142

Abstract

Monoclonal antibody (mAb) is a widely used therapeutic modality that is being used for treatment of chronic diseases like cancer, psoriasis, and other auto immune diseases. The affordability of these therapeutics is presently low because of their high manufacturing cost. Protein A chromatography step is a major contributor to the cost of manufacturing of mAbs. The proposed study is an attempt to improve process performance of the protein A chromatography step using multi-flow loading strategy. Although continuous chromatography is an efficient tool to improve resin utilization and process productivity, implementation of continuous chromatography warrants additional capital investment. Use of dual flow rate or multi flow rate offers the potential of attaining similar benefit without this additional investment. For optimization of multi flow rate loading strategy, it is necessary to understand the range of operating flow rate, switch time for changing flow rate to next flow rate and the delta change in the flow rate. In the current study, an alternate, industrially feasible and scalable multi flow rate strategy has been developed, which optimizes the switch time for a given set of flow rates. The algorithm uses LDF (linear driving force) model to predict the breakthrough curve. Further, the method optimizes flow trajectory based on simulated breakthrough curves using estimated diffusion coefficients at specific residence times and suggests a switch time strategy leading to a multi-step loading of increasing residence times. It was observed that by operating the process at multiple flow rates, a near maxima of both adsorbent capacity and the productivity can be achieved. Although variable flow rate approaches have been proposed in literature in recent times, our method for multi-step loading is simpler, practical and has been demonstrated both at lab and pilot scales. The results showed that this simple multi-flow loading approach increased loading capacities by ∼20% and resin utilization by ∼15% as compared to regular batch process; with new generation protein A resin, mAb Select PrismATM, as capture chromatography. Approximately 60% reduction in $COGS/g has been demonstrated when compared to constant flow batch process, similar to the benefits obtained with multi-column continuous chromatography.

Published

2022

35. The Effect of Preconditioning Strategies on the Adsorption of Model Proteins onto Screen-Printed Carbon Electrodes.

Author

Romih, Tea, Konjević, Ivan, Žibret, Lea, Fazarinc, Ika, Beltram, Ajda, Majer, David, Finšgar, Matjaž, and Hočevar, Samo B.

Subjects

*PROTEIN models, *GLOW discharges, *ADSORPTION kinetics, *SERUM albumin, *ADSORPTION (Chemistry), *CARBON electrodes, *VOLTAMMETRY

Abstract

The preconditioning and modification of the supporting electrode surface is an essential step in every biosensor architecture. In particular, when using screen-printed carbon electrodes (SPEs) as inexpensive and convenient disposable sensor substrates, their somewhat lower electrochemical (surface) reproducibility might represent a complex hurdle. Herein, we investigated the effect of selected preconditioning strategies, such as cyclic voltammetric pretreatment, in H2SO4 and H2O2 and plasma pretreatment with a positive and negative glow discharge, which all improved the electrochemical stability of the unmodified SPEs. Furthermore, we studied the influence of preconditioning strategies on the adsorption kinetics of the two most commonly used building blocks for biosensor preparation, i.e., bovine serum albumin (BSA) and protein A. We observed an advantageous effect of all the examined preconditioning strategies for the modification of SPEs with protein A, being the most effective the negative glow discharge. On the other hand, BSA exhibited a more complex adsorption behavior, with the negative glow discharge as the only generally beneficial preconditioning strategy providing the highest electrochemical stability. Protein A revealed a more substantial impact on the electrochemical signal attenuation than BSA considering their same concentrations in the modification solutions. For both BSA and protein A, we showed that the concentrations of 5 and 10 μg mL−1 already suffice for an electrochemically satisfactorily stable electrode surface after 60 min of incubation time, except for BSA at the positive-plasma-treated electrode. [ABSTRACT FROM AUTHOR]

Published

2022

36. Comparative Evaluation of Commercial Protein A Membranes for the Rapid Purification of Antibodies

Author

Joshua Osuofa and Scott M. Husson

Subjects

Protein A, membrane chromatography, dynamic binding capacity, elution volume, permeability, bioprocessing industry, Chemical technology, TP1-1185, Chemical engineering, TP155-156

Abstract

Protein A chromatography is ubiquitous to antibody purification. The high specificity of Protein A for binding the Fc-region of antibodies and related products enables unmatched clearance of process impurities like host cell proteins, DNA, and virus particles. A recent development is the commercialization of research-scale Protein A membrane chromatography products that can perform capture step purification with short residence times (RT) on the order of seconds. This study investigates process-relevant performance and physical properties of four Protein A membranes: Purilogics Purexa™ PrA, Gore® Protein Capture Device, Cytiva HiTrap™ Fibro PrismA, and Sartorius Sartobind® Protein A. Performance metrics include dynamic binding capacity, equilibrium binding capacity, regeneration-reuse, impurity clearance, and elution volumes. Physical properties include permeability, pore diameter, specific surface area, and dead volume. Key results indicate that all membranes except the Gore® Protein Capture Device operate with flow rate-independent binding capacities; the Purilogics Purexa™ PrA and Cytiva HiTrap Fibro™ PrismA have binding capacities on par with resins, with orders of magnitude faster throughput; and dead volume and hydrodynamics play major roles in elution behavior. Results from this study will enable bioprocess scientists to understand the ways that Protein A membranes can fit into their antibody process development strategies.

Published

2023

37. All fiber Mach-Zehnder interferometer immunosensor based on rabbit anti-human IgG and protein a for human IgG detection.

Author

Momeni, Fatemeh, Ahmadi, Vahid, and Babashamsi, Mohammad

Subjects

*OPTICAL fibers, *RABBITS, *INTERFEROMETERS, *ELECTROMAGNETIC interference, *REFRACTIVE index, *GLOBIN

Abstract

[Display omitted] • Presenting Mach Zehnder immunosensor based on optical fiber with a simple and stable design. • Investigating the effect of using protein A in attachment of rabbit anti-human IgG on the fiber surface in sensor sensitivity. • Using rabbit anti-human IgG instead of the goat's one because of the higher protein A affinity for rabbit anti-human IgG. Antibodies produced by the immune system, including immunoglobin G (IgG), are among the important biological biomarkers. Optical fibers are ideal for fabricating biosensors because of their flexibility, weight, biocompatibility, electromagnetic interference immunity, etc. This study proposes a multimode-single mode-multimode (MSM) Mach-Zehnder interferometer immunosensor based on rabbit anti-human IgG and protein A (PA) for human IgG detection. When IgG is trapped by antibodies located on the surface of the fiber, the refractive index (RI) changes, and the wavelength redshift occurs in the transmission spectrum of the interference pattern. Here, for binding the antibody to the pre coated PA surface, a rabbit anti-human IgG has been used, which has stronger binding to PA and as a result higher stability than the goat anti-human IgG on the optical fiber surface. By optimizing the optical configuration and biolayer material, a limit of detection of 0.067 μg/ml and sensitivity of 0.14 nm.ml/μg could be achieved. [ABSTRACT FROM AUTHOR]

Published

2024

38. CaptureSelect FcXP affinity medium exhibits strong aggregate separation capability.

Author

Dong, Wanyuan, Zhang, Dan, and Li, Yifeng

Subjects

*BISPECIFIC antibodies, *GRADIENT elution (Chromatography), *CARRIER proteins, *BINDING sites, *PROTEIN binding, *ELUTION (Chromatography), *AFFINITY chromatography

Abstract

Protein A affinity chromatography has been widely used for initial product capture in recombinant antibody/Fc-fusion purification. However, in general Protein A lacks the capability of separating aggregates (unless the aggregates are too large to enter the pores of resin beads or have their Protein A binding sites buried, in which case the aggregates do not bind). In the current work, we demonstrated that CaptureSelect FcXP affinity medium exhibited strong aggregate separation capability and effectively removed aggregates under pH or conductivity gradient elution in two bispecific antibody (bsAb) cases. For these two cases, aggregate contents were reduced from >16% and >22% (in the feed) to <1% and <5% (in the eluate) for the first and second bsAbs, respectively. While more case studies are required to further demonstrate FcXP's superiority in aggregate removal, findings from the current study suggest that FcXP can potentially be a better alternative than Protein A for product capture in cases where aggregate content is high. • In general, Protein A affinity chromatography lacks the capability of separating aggregates. • FcXP, a CH3-specific affinity medium, exhibits good aggregate separation potential under linear pH gradient elution. • Linear conductivity gradient, which enables improved resolution, facilitates convenient conversion into stepwise elution. • FcXP can potentially be a better alternative than Protein A for product capture in cases where aggregate content is high. [ABSTRACT FROM AUTHOR]

Published

2024

39. Label-free aptasensor targeting Staphylococcus aureus surface Protein A.

Author

Canciu, Alexandra, Tătaru, Ana-Maria, Bogdan, Diana, Barbu-Tudoran, Lucian, Olah, Diana, Tertiș, Mihaela, Cernat, Andreea, and Cristea, Cecilia

Subjects

*STAPHYLOCOCCUS aureus, *BACTERIAL colonies, *PROTEINS, *DRUG resistance in microorganisms, *DETECTION limit, *APTAMERS

Abstract

[Display omitted] • A label-free aptasensor was designed for Staphylococcus aureus protein A. • An LOD of 8.33 nM was determined for protein A detection. • A good correlation was obtained after incubation with S. aureus culture samples. • The aptasensor was succesfully assessed in human serum samples. The rapid detection of Staphylococcus aureus (S. aureus) is of major importance for the biomedical world in the context where the antimicrobial resistance (AMR), the "silent pandemic", is considered a global public health threat to humanity. There are various approaches to detect S. aureus either as a whole bacterium or via different biomarkers that indicate the presence of this microorganism. Herein, a label-free aptasensor was designed for the detection of a cellular bacterial wall component, protein A (PrA), as a biomarker for the bacteria presence. A rapid procedure, under 5 min, that involves the deposition of the aptamer at the surface of a gold-based screen-printed electrode was applied followed by a blocking step to prevent non-specific adsorption of the target. After the incubation with PrA, the electrochemical detection was achieved, the aptasensor exhibiting good sensitivity across a wide linear range from 25 nM to 1000 nM, with a limit of detection (LOD) of 8.33 nM in standard solutions of the target. S. aureus was detected in commercial human serum and culture samples displaying a good correlation of the signal and the number of bacteria colonies, in the latter case. [ABSTRACT FROM AUTHOR]

Published

2024

40. Staphylococcal Protein A with Engineered Cysteine: Comparison of Monomeric Content as a Critical Quality Attribute during Intracellular and Extracellular Expression.

Author

Choudhury, Lipsa, Shukla, Esha, Jena, Rajender, Yadav, Vishwanath, Ahmad, Aziz, Mishra, Rajesh, and Pandey, Gaurav

Subjects

STAPHYLOCOCCAL protein A, ESCHERICHIA coli, CYSTEINE, REDUCING agents, INDUSTRIAL costs

Abstract

Background: The introduction of engineered cysteine in staphylococcal protein A (SPA-cys) for site-specific conjugation results in a substantial amount of dimerized SPA due to spontaneous oxidation during its production, leading to inaccessibility and thus rendering it unusable. Monomers are usually recovered from dimers by using reducing agents before conjugation in subsequent steps. However, this leads to low conjugation efficiency and increases overall cost and production time. This study aims to systematically compare and quantify the monomeric and dimeric content of SPA when produced through intracellular and extracellular routes in E. coli. Methods: Purified SPAs with and without cysteine from both intracellular and extracellular processes are compared for their monomeric content and efficiency to conjugate on solid support matrix with and without an additional pre-step of reduction. Results: The monomeric form of SPA-cys, which is a desired key quality attribute, is less than 50% when produced extracellularly. SPA-cys produced through the intracellular production process has high monomeric content (≥85%) and shows higher binding to solid support. Conclusion: The study demonstrates that the intracellular route for production of SPA-cys should be the preferred method, and the release assays for SPA-cys products should include the amount of monomeric content as one of the quality attributes. The abundance of monomeric content enhances the site-specific conjugation efficiency and density of SPA on the resin matrix. [ABSTRACT FROM AUTHOR]

Published

2022

41. Binding characteristics of staphylococcal protein A and streptococcal protein G for fragment crystallizable portion of human immunoglobulin G

Author

Hae Gon Lee, Shinill Kang, and Joon Sang Lee

Subjects

Immunoglobulin G, Protein A, Protein G, Protein docking, Affinity chromatography, Molecular dynamics, Biotechnology, TP248.13-248.65

Abstract

In the wide array of physiological processes, protein–protein interactions and their binding are the most basal activities for achieving adequate biological metabolism. Among the studies on binding proteins, the examination of interactions between immunoglobulin G (IgG) and natural immunoglobulin-binding ligands, such as staphylococcal protein A (spA) and streptococcal protein G (spG), is essential in the development of pharmaceutical science, biotechnology, and affinity chromatography. The widespread utilization of IgG-spA/spG binding characteristics has allowed researchers to investigate these molecular interactions. However, the detailed binding strength of each ligand and the corresponding binding mechanisms have yet to be fully investigated. In this study, the authors analyzed the binding strengths of IgG–spA and IgG–spG complexes and identified the mechanisms enabling these bindings using molecular dynamics simulation, steered molecular dynamics, and advanced Poisson–Boltzmann Solver simulations. Based on the presented data, the binding strength of the spA ligand was found to significantly exceed that of the spG ligand. To find out which non-covalent interactions or amino acid sites have a dominant role in the tight binding of these ligands, further detailed analyses of electrostatic interactions, hydrophobic bonding, and binding free energies have been performed. In investigating their binding affinity, a relatively independent and different unbinding mechanism was found in each ligand. These distinctly different mechanisms were observed to be highly correlated to the protein secondary and tertiary structures of spA and spG ligands, as explicated from the perspective of hydrogen bonding.

Published

2021

42. Diagnostic validity of a marker model of first trimester in pregnancy in prediction of birth weight.

Author

Vujović, Slavica, Šćepanović, Andjelka, Terzić, Milan, and Djurović, Milena

Subjects

*FIRST trimester of pregnancy, *BIRTH weight, *LOW birth weight, *CHORIONIC gonadotropins, *FETAL growth retardation

Abstract

Background/Aim. Nowadays, low birth weight is considered to be one of the main causes of cardiovascular diseases or metabolic syndrome occurring later in life. Many studies have shown a strong impact of abnormal birth weight onto the future development, however, due to its stronger influence onto the development, a special emphasis is placed on low birth weight as compared to higher one. There is still no high-percentage accuracy test that will clearly classify expectant women under the risk of giving birth to a child too low or too big for gestational age. The aim of this paper was to set up a model that may indicate future low or high birth weight. Methods. This study included 191 expectant women who were divided into three groups, based on the birth weight (group 1: ˂ 3,000 g; group 2: 3,000-4,000 g; group 3: ˃ 4,000 g). The values of biochemical (pregnancy associated plasma protein A - PAPP-A, free β human chorionic gonadotropin) and ultrasonographic markers (nuchal translucency) as well as their multiple of the median (MoM) were determined and compared among groups. Results. It was shown that the values of PAPP-A MoM were considerably lower in groups of expectant women that had a fetus with low body weight (p = 0.003, p = 0.001). Statistically significant correlation between PAPP-A MoM and the newborn's weight (rs = 0.221, p = 0.001) was proven among the groups examined within this study. Conclusion. The usage of a combination of biochemical parameters, sonographic and demographic data in screening program increases the chances for early identification of fetuses that are under higher risk for growth restriction or increased growth. Also, the increase in the value of PAPP- A MoM causes the increase of fetus' body weight. [ABSTRACT FROM AUTHOR]

Published

2022

43. Functional Magnetic Microdroplets for Antibody Extraction.

Author

Al‐Terke, Hedar H., Latikka, Mika, Timonen, Jaakko V. I., Vékás, Ladislau, Paananen, Arja, Joensuu, Jussi, and Ras, Robin H. A.

Subjects

MICRODROPLETS, CHIMERIC proteins, LIQUID-liquid interfaces, IMMUNOGLOBULINS, ANTIBODY formation, SOLID phase extraction

Abstract

Antibodies play an essential role in modern medicine for diagnostic and therapeutic applications. Even though the production of antibodies is the fastest growing pharmaceutical industry area, the cost of antibodies remains high, which limits access to antibody‐based medicine both in developing and developed countries. The bottleneck and major cost factor in the production is purification of the antibody. Here, a proof‐of‐concept is presented for antibody extraction using ferrofluid microdroplets. An external magnetic field splits oil‐based ferrofluid droplets into an array of daughter microdroplets, which serve as a magnetically tunable, hydrophobic, liquid substrate with a relatively large surface area. A fusion protein (HFBI‐Protein A), added to the solution surrounding the magnetic droplets, adsorbs strongly at the liquid‐liquid interface by the hydrophobin HFBI moiety, creating a bifunctional monolayer that can catch antibody molecules. After adsorption at the liquid‐liquid interface, these antibody molecules can be released by decreasing the pH of the solution. The antibody extraction process is investigated using confocal microscopy and gel electrophoresis. In addition, the effect of HFBI on the field‐induced ferrofluid droplet splitting is examined. This study provides a proof of concept for utilizing liquid‐liquid instead of a solid‐liquid system in antibody handling. [ABSTRACT FROM AUTHOR]

Published

2022

44. Editorial: Understanding and Engineering Antibody-Superantigen Interactions

Author

Samuel Ken-En Gan, Jeremy P. Derrick, and Franca Fraternali

Subjects

superantigens, antibody engineering, protein-protein interactions, antibodies, protein A, protein G, Immunologic diseases. Allergy, RC581-607

Published

2022

45. Anti-leishmaniasis effect of Staphylococcus aureus Protein A on the size of the lesion and parasitic load

Author

Zahra Tavalaei, Mehrdad Zeinalian, Hossein Khanahmad, and Hossein Hejazi

Subjects

protein a, leishmania major, staphylococcus aurous, Medicine, Biology (General), QH301-705.5

Abstract

Background: Many studies in the past have evaluated the role of immune system boosters in the treatment of leishmania major infection. Protein A (PA) is one of the structural components in peptidoglycan cell wall of gram-negative bacteria such as staphylococcus aurous which functions as a stimulator in the cellular immune system. The present study aims to evaluate the anti-inflammatory effect of PA on the recovery of leishmania major infection. Materials and Methods: This study was conducted on 24 female Balb/c-infected mice. The experimental group received PA at a dose of 60 mg/kg for four weeks. There was no intervention for the negative control group; the third group received the solvent of PA and sterile H2O; and the positive control group received Amphotericin B at a dose of 1 mg/kg body weight. At the end of the treatment period, a real-time polymerase chain reaction (PCR) assay was performed to determine parasitic burden, and the size of the lesions was measured by caliper with an accuracy of 0.01 mm. Results: Results showed that PA did slightly decrease the wound spread and growth but not to an extent that can be considered statistically significant. Also, differences in cycle threshold (Ct) values between the treated group and the untreated group was not impressive. Conclusions: Although findings showed that PA isn't such a good candidate for leishmania treatment, it may still be suitable for therapies that use multiple drugs in combination to speed up the healing of leishmaniosis, an issue that merits evaluation in future studies.

Published

2023

46. Expression and Characterization of Intein-Cyclized Trimer of Staphylococcus aureus Protein A Domain Z

Author

Suman Nandy, Vijay M. Maranholkar, Mary Crum, Katherine Wasden, Ujwal Patil, Atul Goyal, Binh Vu, Katerina Kourentzi, William Mo, Amy Henrickson, Borries Demeler, Mehmet Sen, and Richard C. Willson

Subjects

protein A, cyclic Z3, SICLOPPS, tandem mass spectrometry, ITC, DSF, Biology (General), QH301-705.5, Chemistry, QD1-999

Abstract

Staphylococcus aureus protein A (SpA) is an IgG Fc-binding virulence factor that is widely used in antibody purification and as a scaffold to develop affinity molecules. A cyclized SpA Z domain could offer exopeptidase resistance, reduced chromatographic ligand leaching after single-site endopeptidase cleavage, and enhanced IgG binding properties by preorganization, potentially reducing conformational entropy loss upon binding. In this work, a Z domain trimer (Z3) was cyclized using protein intein splicing. Interactions of cyclic and linear Z3 with human IgG1 were characterized by differential scanning fluorimetry (DSF), surface plasmon resonance (SPR), and isothermal titration calorimetry (ITC). DSF showed a 5 ℃ increase in IgG1 melting temperature when bound by each Z3 variant. SPR showed the dissociation constants of linear and cyclized Z3 with IgG1 to be 2.9 nM and 3.3 nM, respectively. ITC gave association enthalpies for linear and cyclic Z3 with IgG1 of −33.0 kcal/mol and −32.7 kcal/mol, and −T∆S of association 21.2 kcal/mol and 21.6 kcal/mol, respectively. The compact cyclic Z3 protein contains 2 functional binding sites and exhibits carboxypeptidase Y-resistance. The results suggest cyclization as a potential approach toward more stable SpA-based affinity ligands, and this analysis may advance our understanding of protein engineering for ligand and drug development.

Published

2023

47. Different VH3-Binding Protein A Resins Show Comparable VH3-Binding Mediated By product Separation Capabilities Despite Having Varied Dynamic Binding Capacities Towards A VH3 Fab.

Author

Hu L, Wang R, Wu Q, Wan Y, and Li Y

Abstract

Background: Protein A resins have been widely used for product capture during mAb, bispecific antibody (bsAb), and Fc-fusion protein purification. While Protein A ligands mainly bind the Fc region, many of them can also bind the VH3 domain. During mAb/bsAb purification, certain truncated byproducts may contain the same Fc region as the product but fewer numbers of the VH3 domain. In such a scenario, VH3-binding Protein A resins provide a potential means for byproduct separation based on the difference in VH3-binding valency. As the ligands of different VH3-binding Protein A resins are derived from distinct domains of the native Protein A, it would be interesting to know whether they possess comparable capabilities for separating species with the same Fc region but different numbers of VH3 domain., Objective: This study aims to explore the potential of different VH3-binding Protein A resins for separating antibody species with the same Fc region but different numbers of VH3 domain., Methods: The VH3 Fab was released from a VH3-containing mAb by papain digestion. Post digestion, the released VH3 Fab was purified sequentially using CaptureSelect CH1-XL and MabSelect SuRe affinity chromatography. The purified VH3 Fab was used as the load material to assess the dynamic binding capacity (DBC) of five VH3-binding Protein A resins (i.e., Amshpere A3, Jetted A50, MabCapture C, MabSelect and MabSelect PrismA). The potential of VH3-binding Protein A resins for separating species having the same Fc region but different numbers of VH3 domain was evaluated using an artificial mixture composed of the product and a truncated byproduct, which contained one and zero VH3 domain, respectively (both species contained the same Fc region). Sodium dodecyl sulfate-polyacrylamide gel electrophoresis (SDS-PAGE) was used to monitor Fab purification and separation of species containing the same Fc region but different numbers of VH3 domain., Results: When loaded with an isolated VH3 Fab, different VH3-binding Protein A resins showed varied DBCs. Nevertheless, when these Protein A resins were used to separate a truncated byproduct, which contained the Fc region only without any VH3 domain, from the product, which included one VH3 domain in addition to the Fc region, they showed comparable capabilities for separating these two species., Conclusion: Although different VH3-binding Protein A resins showed varied DBCs towards a VH3 Fab, they exhibited comparable capabilities for separating species with the same Fc region but different numbers of VH3 domain., (Copyright© Bentham Science Publishers; For any queries, please email at epub@benthamscience.net.)

Published

2024

48. Calcium chloride and arginine show diametrically opposite effects on antibody elution in Protein A and Protein L chromatography.

Author

Qu J, Wan Y, and Li Y

Abstract

Protein A and Protein L affinity chromatographies are extensively used in mAb and bispecific antibody (bsAb) purification. In addition to product capture, they are both capable of separating certain product-related by-products and aggregates under appropriate conditions. For both types of chromatography, previous studies suggested that adding a salt additive to the mobile phase can significantly improve the resolution between product and by-products/aggregates. Nevertheless, the effects of different salt additives on antibody elution in Protein A and Protein L chromatography have not been compared. In the current study, we compared the effects of three salt additives, sodium chloride (NaCl), calcium chloride (CaCl 2 ), and arginine hydrochloride (Arg·HCl), on antibody elution in Protein A and Protein L chromatography. Interestingly, while NaCl suppressed antibody elution in both types of chromatography, CaCl 2 , and Arg·HCl promoted antibody elution in Protein A chromatography but suppressed antibody elution in Protein L chromatography. In addition, we evaluated the effect of each salt gradient on aggregate removal by Protein L chromatography. The information provided by the current study should be useful to the selection of conditions/additives for improving by-product removal by Protein A and Protein L chromatography., Competing Interests: The authors declare no conflicts of interest., (© 2024 The Journal of Biological Methods, All rights reserved.)

Published

2024

49. The first report on the sortase-mediated display of bioactive protein A from Staphylococcus aureus (SpA) on the surface of the vegetative form of Bacillus subtilis.

Author

Ghaedmohammadi, Samira and Ahmadian, Gholamreza

Subjects

*BACILLUS subtilis, *STAPHYLOCOCCUS aureus, *IMMUNE complexes, *IMMUNOGLOBULIN G, *PROTEINS

Abstract

Protein A (SpA) is one of the most important Staphylococcus aureus cell wall proteins. It includes five immunoglobulin (Ig)-binding domains which can bind to immune complexes through the Fc region of immunoglobulins. The binding of SpA to the polymeric supports can be used to prepare affinity chromatography resins, which are useful for immunoprecipitation (IP) of antibodies. Protein A is also used to purify many anti-cancer antibodies. In this study, SpA was displayed on the surface of Bacillus subtilis cells using a sortase-mediated system to display the target protein to the B. subtilis cell wall. A series of plasmids consisting of cassettes for cell wall-directed protein A as well as negative controls were constructed and transformed into B. subtilis WASD (wprA sigD) cells. SDS-PAGE, western blot, flow cytometry, functional IgG purification assay, and a modified ELISA assay were used to confirm the surface display of SpA and evaluate its function. Semi-quantitative ELISA results showed that the binding capacity of lyophilized Bs-SpA is 100 μg IgG from rabbit serum per 1 mg of cells under optimal experimental conditions. Low production costs, optimal performance, and the use of a harmless strain compared to a similar commercial product predict the possible use of SpA immobilization technology in the future. [ABSTRACT FROM AUTHOR]

Published

2021

50. Enhancing protein A productivity and resin utilization within integrated or intensified processes.

Author

Brinkmann, Alex and Elouafiq, Sanaa

Abstract

Recent interest in continuous manufacturing of biologics has driven the development and evaluation of multicolumn chromatography systems to drive down resin costs by increasing productivity and maximizing resin utilization, especially for the expensive protein A capture step. Single‐pass tangential flow filtration can be used to reduce the volume of perfusion harvest, enabling a further increase in the productivity of the capture step by up to fivefold. However, there are expected to be practical limits for the productivity of the capture step, which must be determined based on the manufacturing batch size, duration, and frequency, especially as it relates to efficient utilization of the column lifetime. For short fed‐batch manufacturing campaigns, intensified capture processes may result in up to 82% lower resin consumption, while avoiding the long‐term storage of used resin. For perfusion processes and longer fed‐batch campaigns, it may be more efficient to operate at a lower productivity that enables the column lifetime to be routinely achieved and achieves the desired resin and buffer savings without introducing unnecessary process risk or complexity. An intensified batch capture process, "super‐batch," will be compared as an alternative to multicolumn chromatography processes to achieve high productivity and resin utilization with a potentially simpler process. [ABSTRACT FROM AUTHOR]

Published

2021