4.6 Article

Adenovirus 5 recovery using nanofiber ion-exchange adsorbents

期刊

BIOTECHNOLOGY AND BIOENGINEERING
卷 116, 期 7, 页码 1698-1709

出版社

WILEY
DOI: 10.1002/bit.26972

关键词

anion exchange chromatography; downstream processing; nanofibers; viral vectors

资金

  1. Puridify (GE healthcare) [EP/N013395/1]
  2. Engineering and Physical Sciences Research Council [EP/L01520X/1]
  3. BBSRC [BB/M004848/1] Funding Source: UKRI
  4. EPSRC [EP/R013756/1, EP/M017222/1, EP/N013395/1] Funding Source: UKRI

向作者/读者索取更多资源

Viral vectors such as adenovirus have successful applications in vaccines and gene therapy but the manufacture of the high-quality virus remains a challenge. It is desirable to use the adsorption-based chromatographic separations that so effectively underpin the therapeutic protein manufacture. However fundamental differences in the size and stability of this class of product mean it is necessary to revisit the design of sorbent's morphology and surface chemistry. In this study, the behaviour of a cellulose nanofiber ion-exchange sorbent derivatised with quaternary amine ligands at defined densities is characterised to address this. This material was selected as it has a large accessible surface area for viral particles and rapid process times. Initially, the impact of surface chemistry on infective product recovery using low (440 mu mol/g), medium (750 mu mol/g), and high (1029 mu mol/g) ligand densities is studied. At higher densities product stability is reduced, this effect increased with prolonged adsorption durations of 24 min with just similar to 10% loss at low ligand density versus similar to 50% at high. This could be mitigated by using a high flow rate to reduce the cycle time to similar to 1 min. Next, the impact of ligand density on the separation's resolution was evaluated. Key to understanding virus quality is the virus particle: infectious virus particle ratio. It was found this parameter could be manipulated using ligand density and elution strategy. Together this provides a basis for viral vector separations that allows for their typically low titres and labile nature by using high liquid velocity to minimise both load and on-column times while separating key product and process-related impurities.

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