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Buffer Capacity of Biologies—From Buffer Salts to Buffering by Antibodies

机译:生物的缓冲能力-从缓冲盐到抗体的缓冲

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Controlling pH is essential for a variety of biopharmaceutical process steps. The chemical stability of biologies such as monoclonal antibodies is pH-dependent and slightly acidic conditions are favorable for stability in a number of cases. Since control of pH is widely provided by added buffer salts, the current study summarizes the buffer characteristics of acetate, citrate, histidine, succinate, and phosphate buffers. Experimentally derived values largely coincide with values calculated from a model that had been proposed in 1922 by van Slyke. As high concentrated protein formulations become more and more prevalent for biologies, the self-buffering potential of proteins becomes of relevance. The current study provides information on buffer characteristics for pH ranges down to 4.0 and up to 8.0 and shows that a monoclonal antibody at 50 mglmL exhibits similar buffer capacity as 6 mM citrate or 14 mM histidine (pH 5.0-6.0). Buffer capacity of antibody solutions scales linearly with protein concentration up to more than 200 mglmL. At a protein concentration of 220 mglmL, the buffer capacity resembles the buffer capacity of 30 mM citrate or 50 mM histidine (pH 5.0-6.0). The buffer capacity of monoclonal antibodies is practically identical at the process relevant temperatures 5, 25, and 40°C. Changes in ionic strength of AI=0.15, in contrast, can alter the buffer capacity up to 35%. In conclusion, due to efficient self-buffering by antibodies in the pH range of favored chemical stability, conventional buffer excipients could be dispensable for pH stabilization of high concentrated protein solutions.
机译:控制pH值对于各种生物制药工艺步骤至关重要。诸如单克隆抗体之类的生物制剂的化学稳定性是pH依赖性的,在许多情况下,微酸性条件有利于其稳定性。由于通过添加缓冲盐可以广泛地控制pH,因此当前的研究总结了乙酸盐,柠檬酸盐,组氨酸,琥珀酸盐和磷酸盐缓冲液的缓冲特性。实验得出的值与范·斯莱克(van Slyke)在1922年提出的模型计算得出的值基本一致。随着高浓度蛋白质制剂在生物制剂中越来越流行,蛋白质的自我缓冲潜力变得越来越重要。当前的研究提供了有关pH范围低至4.0至8.0的缓冲液特性的信息,并显示50 mglmL的单克隆抗体具有与6 mM柠檬酸盐或14 mM组氨酸(pH 5.0-6.0)相似的缓冲能力。抗体溶液的缓冲能力与蛋白质浓度高达200 mg / mL呈线性比例关系。在220 mglmL的蛋白质浓度下,缓冲能力类似于30 mM柠檬酸盐或50 mM组氨酸(pH 5.0-6.0)的缓冲能力。在工艺相关温度5、25和40°C下,单克隆抗体的缓冲能力实际上是相同的。相反,AI = 0.15的离子强度的变化最多可改变35%的缓冲容量。总之,由于在有利化学稳定性的pH范围内,抗体可进行有效的自我缓冲,因此对于高浓度蛋白质溶液的pH稳定化,常规缓冲液赋形剂可能是必需的。

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