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Literature DB >> 18023013

Self-buffering antibody formulations.

Yatin R Gokarn¹, Eva Kras, Carrie Nodgaard, Vasumathi Dharmavaram, R Matthew Fesinmeyer, Heather Hultgen, Stephen Brych, Richard L Remmele, David N Brems, Susan Hershenson.

Abstract

Monoclonal antibodies (mAbs) often require the development of high-concentration formulations. In such cases, and when it is desirable to formulate a mAb around pH 5.0, we explored a novel approach of controlling the formulation pH by harnessing the ability of mAbs to "self-buffer." Buffer capacities of four representative IgG(2) molecules (designated mAb1 through mAb4) were measured in the pH 4-6 range. The buffer capacity results indicated that the mAbs possessed a significant amount of buffer capacity, which increased linearly with concentration. By 60-80 mg/mL, the mAb buffer capacities surpassed that of 10 mM acetate, which is commonly employed in formulations for buffering in the pH 4-6 range. Accelerated high temperature stability studies (50 degrees C over 3 weeks) conducted with a representative antibody in a self-buffered formulation (50 mg/mL mAb1 in 5.25% sorbitol, pH 5.0) and with solutions formulated using conventional buffers (50 mg/mL mAb1 in 5.25% sorbitol, 25 or 50 mM acetate, glutamate or succinate, also at pH 5.0) indicated that mAb1 was most resistant to the formation of soluble aggregates in the self-buffered formulation. Increased soluble aggregate levels were observed in all the conventionally buffered (acetate, glutamate, and succinate) formulations, which further increased with increasing buffer strength. The long-term stability of the self-buffered liquid mAb1 formulation (60 mg/mL in 5% sorbitol, 0.01% polysorbate 20, pH 5.2) was comparable to the conventionally buffered (60 mg/mL in 10 mM acetate or glutamate, 5.25% sorbitol, 0.01% polysorbate 20, pH 5.2) formulations. No significant change in pH was observed after 12 months of storage at 37 and 4 degrees C for the self-buffered formulation. The 60 mg/mL self-buffered formulation of mAb1 was also observed to be stable to freeze-thaw cycling (five cycles, -20 degrees C --> room temperature). Self-buffered formulations may be a better alternative for the development of high-concentration antibody and protein dosage forms.

Entities: Chemical Gene

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Year: 2008 PMID： 18023013 DOI： 10.1002/jps.21232

Source DB: PubMed Journal: J Pharm Sci ISSN： 0022-3549 Impact factor: 3.534

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Cited

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3. Challenges in Determining Intrinsic Viscosity Under Low Ionic Strength Solution Conditions.

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4. Light-Induced Covalent Buffer Adducts to Histidine in a Model Protein.

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Review 5. Best Practices for Aggregate Quantitation of Antibody Therapeutics by Sedimentation Velocity Analytical Ultracentrifugation.

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6. Evaluation of the physical stability of the EC5 domain of E-cadherin: effects of pH, temperature, ionic strength, and disulfide bonds.

Authors: Kai Zheng; C Russell Middaugh; Teruna J Siahaan
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Self-buffering antibody formulations.

Review 1. Stability of protein pharmaceuticals: an update.

2. Critical examination of the colloidal particle model of globular proteins.

3. Challenges in Determining Intrinsic Viscosity Under Low Ionic Strength Solution Conditions.

4. Light-Induced Covalent Buffer Adducts to Histidine in a Model Protein.

Review 5. Best Practices for Aggregate Quantitation of Antibody Therapeutics by Sedimentation Velocity Analytical Ultracentrifugation.

6. Evaluation of the physical stability of the EC5 domain of E-cadherin: effects of pH, temperature, ionic strength, and disulfide bonds.

7. Effect of ions on agitation- and temperature-induced aggregation reactions of antibodies.

8. Study on the effect of solution conditions on heat induced-aggregation of human alpha interferon.

9. Protein-protein interactions in dilute to concentrated solutions: α-chymotrypsinogen in acidic conditions.

10. The effect of arginine glutamate on the stability of monoclonal antibodies in solution.