Osuofa Joshua, Henn Daniel, Zhou Jinxiang, Forsyth Anna, Husson Scott M
Department of Chemical and Biomolecular Engineering, Clemson University, Clemson, South Carolina, USA.
Purilogics, LLC, Greenville, South Carolina, USA.
Biotechnol Prog. 2021 May;37(3):e3129. doi: 10.1002/btpr.3129. Epub 2021 Jan 29.
This contribution reports on a study using Purexa™-MQ multimodal anion-exchange (AEX) membranes for protein polishing at elevated solution conductivities. Dynamic binding capacities (DBC ) of bovine serum albumin (BSA), human immunoglobulins, and salmon sperm DNA (ss-DNA) are reported for various salt types, salt concentrations, flowrates, and pH. Using 1 mg/ml BSA, DBC values for Purexa™-MQ were >90 mg/ml at conductivities up to 15 mS/cm. The membranes maintained a high, salt-tolerant BSA DBC of 89.8 ± 2.7 (SD) over the course of 100 bind-elute cycles. Polishing studies with acidic and basic monoclonal antibodies at >2 kg/L loads showed that Purexa™-MQ had higher clearance of host cell proteins and aggregate species at high conductivity (13 mS/cm) and in the presence of phosphate than other commercial AEX media. Purexa™-MQ also had a high ss-DNA DBC of 50 mg/ml at conductivities up to 15 mS/cm, markedly outperforming other commercial products. In addition to the effectiveness of Purexa™-MQ for protein polishing at elevated solution conductivities, its unusually high binding capacity for ss-DNA indicates potential applications for plasmid DNA purification.
本论文报道了一项关于使用Purexa™-MQ多模式阴离子交换(AEX)膜在提高溶液电导率的情况下进行蛋白质精制的研究。文中报告了牛血清白蛋白(BSA)、人免疫球蛋白和鲑鱼精DNA(ss-DNA)在不同盐类型、盐浓度、流速和pH值下的动态结合容量(DBC)。使用1mg/ml的BSA,在电导率高达15mS/cm时,Purexa™-MQ的DBC值>90mg/ml。在100次结合-洗脱循环过程中,该膜对BSA的DBC保持在89.8±2.7(标准差)的高水平且耐盐。对酸性和碱性单克隆抗体在>2kg/L负载下进行的精制研究表明,在高电导率(13mS/cm)且存在磷酸盐的情况下,Purexa™-MQ比其他市售AEX介质对宿主细胞蛋白和聚集物的清除率更高。在电导率高达15mS/cm时,Purexa™-MQ对ss-DNA的DBC也高达50mg/ml,明显优于其他市售产品。除了Purexa™-MQ在提高溶液电导率时对蛋白质精制的有效性外,其对ss-DNA异常高的结合容量表明其在质粒DNA纯化方面具有潜在应用。
