Separation and Sizing of a Virus Mixture Using Asymmetrical Flow Field- Flow Fractionation Coupled to Multi-Angle Light Scattering

ID: 0018

Application: Viruses, Biopharmaceuticals

Technology: AF4-MALS-RI

Info: Postnova AF2000, PN3621 MALS, PN3150 RI

Keywords: Asymmetrical Flow Field-Flow Fractionation, Virus, Biopharmaceuticals, Multi-Angle Light Scattering

George Bou-Assaf^(a), Andy Blum^(a), Omar Matalka^(a), Ruth Frenkel^(a), Robert Reed^(b), Soheyl Tadjiki^(b)
^(a) Analytical Development, Biogen, Cambridge, MA; ^(b) Postnova Analytics Inc, Salt Lake City, UT

Introduction

Viruses are increasingly used as gene therapy delivery vehicles due to their versatility and safety. They can be loaded with DNA or RNA and delivered to a specific location in the body to treat or cure a disease [1]. One of the biggest challenges for manufacturing a homogeneous virus sample is the presence of viral aggregates, which negatively affect transduction efficiency, biodistribution, and immunogenicity [2]. Due to their relatively large size, often over 50 nm in diameter, virus aggregates are challenging to separate and characterize by column-based chromatography techniques such as size exclusion chromatography (SEC). In this Application Note, we present data on separation of a virus mixture using Asymmetric Flow Field-Flow fractionation (AF4) and measurement of their radius of gyration (R_g).

A schematic for the AF4 channel is shown in Figure 1. The combination of cross flow and channel flow enable size separation over the course of the analysis: small particles elute and reach the connected detectors before larger particles, including aggregates.

Experimental Details and Results

A virus mixture sample was created by combining smaller adeno-associated viruses (AAV) with larger adenovirus type 5 (Ad5) in solution to simulate a sample with virus monomer and aggregates. To separate the viruses by size, an AF4 (Postnova AF2000) was used, coupled to a Postnova 21-angle multi-angle light scattering (MALS, PN3621) detector for measuring the R_g. Both the AAV-only and virus mixture samples were analyzed by AF4-MALS to highlight the differences between the samples. The carrier solution was phosphate buffered saline (PBS). The AF4 membrane used was 10 kDa regenerated cellulose.

$Figure 2. Analysis of AAV-only sample. The curves are replicate AF4-MALS fractograms, overlaid with Rg values (black and red dots).$

$Figure 3. Analysis of AAV and Ad5 virus mixture sample. The curves are replicate AF4-MALS fractograms, overlaid with Rg values (black and red dots).$

In Figure 3, the virus mixture is separated into multiple peaks, with the R_g plotted as black and red dots. The monomers have measured R_g values consistent with AAVs, at about 12.5 nm, with the slight shoulder (aggregates) still observed as in the AAV-only sample. A second peak between 33 and 40 min corresponds to the Ad5 virus, whereas a third peak which elutes between 40 and 50 minutes are aggregates of the Ad5 virus. The Ad5 virus and its aggregates have radii in the range of 30-55 nm, most likely too large to be successfully separated by SEC.

Conclusion

The data presented here demonstrates that AF4-MALS is a powerful tool in the separation of virus particles. It can separate viruses and aggregates from a few nm up to >100 nm. This means that AF4-MALS can easily separate and size multi-modal virus samples, including the larger Ad5 virus and its aggregates with high resolution and precision.

References

[1] M.F. Naso, B. Tomkowicz, W.L. Perry III & W.R. Strohl, BioDrugs, 2017, 31(4), 317–334.
[2] J.F. Wright, T. Le, J. Prado, J. Bahr-Davidson, P.H. Smith, Z. Zhen, J.M. Sommer, G.F. Pierce, G. Qu, Molecular Therapy, 2005, 12(1), 171-178.

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AppNotes