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Arginine and di-arginine ligands for plasmid DNA purification using negative chromatography

separation and purification Technology. 2018; 
Sara Cardoso, Pedro de Alcantara Pessoa Filho, Fani Sousa, Adriano RodriguesAzzoni
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Proteins, Expression, Isolation and Analysis … ng/μL). 2.2.11. Endotoxin quantification. Endotoxin contamination was evaluated using the GenScript (USA, Inc.) ToxinSensor? Chromogenic Limulus ameobocyte lysate kit according to the supplier's instructions. The samples … Get A Quote

摘要

The increasing number of applications requiring highly purified plasmid DNA (pDNA) generates a corresponding need for simple, scalable, and cost-effective purification processes. Due to the pDNA large size and complex shape, the use of commercial chromatographic beads often results in poor yields and low binding capacities when operated in a positive mode. An alternative to overcome this limitation is the design of chromatographic ligand-resin systems able to efficiently operate in negative mode, where host impurities (especially low molecular weight RNA) are efficiently captured and separated from the target pDNA. In this work, arginine amino acid and di-arginine peptide (arginine-arginine) were immobil... More

關鍵詞

Plasmid DNA purification; Negative chromatography; Arginine; Di-arginine;Agarose resin.
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