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Rapid and simplified purification of recombinant adeno-associated virus.


ABSTRACT: Preclinical gene therapy studies both in vitro and in vivo require high purity preparations of adeno-associated virus (AAV). Current methods for purification of AAV entail the use of centrifugation over either a CsCl or iodixanol gradient, or the use of chromatography. These methods can be cumbersome and expensive, necessitating ultrahigh speed gradient centrifugation or, for chromatography the use of other expensive equipment. In addition, these methods are time consuming, and the viral yield is not high. Currently no commercial purification kits are available for other than AAV serotype 2. A simplified method was used for the purification of AAV, with a viral yield that is able to be used effectively in adult and embryo mice. The method does not require ultrahigh speed gradient centrifugation nor chromatography. Instead, polyethylene glycol (PEG)/aqueous two-phase partitioning is used to remove soluble proteins from the PEG8000 precipitated virus-protein mixture. The procedure obtained rapidly up to 95% recovery of high quality purified AAV. The entire purification process, including HEK293 cell transfection, can be completed readily within one week, with purity seemingly higher than that obtained after one round of CsCl gradient purification.

SUBMITTER: Guo P 

PROVIDER: S-EPMC3374034 | biostudies-literature | 2012 Aug

REPOSITORIES: biostudies-literature

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Rapid and simplified purification of recombinant adeno-associated virus.

Guo Ping P   El-Gohary Yousef Y   Prasadan Krishna K   Shiota Chiyo C   Xiao Xiangwei X   Wiersch John J   Paredes Jose J   Tulachan Sidhartha S   Gittes George K GK  

Journal of virological methods 20120426 2


Preclinical gene therapy studies both in vitro and in vivo require high purity preparations of adeno-associated virus (AAV). Current methods for purification of AAV entail the use of centrifugation over either a CsCl or iodixanol gradient, or the use of chromatography. These methods can be cumbersome and expensive, necessitating ultrahigh speed gradient centrifugation or, for chromatography the use of other expensive equipment. In addition, these methods are time consuming, and the viral yield i  ...[more]

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