Virus‐like particle preparation is improved by control over capsomere‐DNA interactions during chromatographic purification

Gerstweiler, Lukas; Bi, Jian; Middelberg, Anton P. J.

doi:10.1002/bit.27687

Cited by 7 publications

(5 citation statements)

References 58 publications

(84 reference statements)

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“…It is important to mention that the feed A260/A280 in Table 1 is calculated based on the peak areas of HMWS, VLPs, and dimers while it was 0.64 for the VLP peak, suggesting that the depleted nucleic acids were mainly associated with (or bound to) the HMWS. This was also observed in a recent study with murine polyomavirus VLPs (Gerstweiler et al, 2021). Both VLPs used in this study lack the C‐terminal protamine‐like region of the wild‐type HBcAg, which reduces packaging of nucleic acids (Crowther et al, 1994; Zlotnick et al, 1997).…”

Section: Resultssupporting

confidence: 81%

Process development for cross‐flow diafiltration‐based VLP disassembly: A novel high‐throughput screening approach

Hillebrandt

Vormittag

Dietrich

et al. 2021

Biotech & Bioengineering

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Virus‐like particles (VLPs) are particulate structures, which are applied as vaccines or delivery vehicles. VLPs assemble from subunits, named capsomeres, composed of recombinantly expressed viral structural proteins. During downstream processing, in vivo‐assembled VLPs are typically dis‐ and reassembled to remove encapsulated impurities and to improve particle morphology. Disassembly is achieved in a high‐pH solution and by the addition of a denaturant or reducing agent. The optimal disassembly conditions depend on the VLP amino acid sequence and structure, thus requiring material‐consuming disassembly experiments. To this end, we developed a low‐volume and high‐resolution disassembly screening that provides time‐resolved insight into the VLP disassembly progress. In this study, two variants of C‐terminally truncated hepatitis B core antigen were investigated showing different disassembly behaviors. For both VLPs, the best capsomere yield was achieved at moderately high urea concentration and pH. Nonetheless, their disassembly behaviors differed particularly with respect to disassembly rate and aggregation. Based on the high‐throughput screening results, a diafiltration‐based disassembly process step was developed. Compared with mixing‐based disassembly, it resulted in higher yields of up to 0.84 and allowed for integrated purification. This process step was embedded in a filtration‐based process sequence of disassembly, capsomere separation, and reassembly, considerably reducing high‐molecular‐weight species.

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Section: Resultssupporting

confidence: 81%

Process development for cross‐flow diafiltration‐based VLP disassembly: A novel high‐throughput screening approach

Hillebrandt

Vormittag

Dietrich

et al. 2021

Biotech & Bioengineering

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“…Ion exchanger has been commonly applied to separate protein and nucleic acids based on the differences of their binding strengths [22]. In this work, an anion exchanger, Q FF, was selected, because of the protein stability on acid condition and the isoelectric point (pI) of HFn and modified HFns.…”

Section: Nucleic Acid Removal By Ion-exchange Chromatography (Iec)mentioning

confidence: 99%

Development of purification process for dual‐function recombinant human heavy‐chain ferritin by the investigation of genetic modification impact on conformation

Yin

Zhang

Jun

et al. 2021

Engineering in Life Sciences

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Ferritin is a promising drug delivery platform and has been functionalized through genetic modifications. This work has designed and expressed a dualfunctional engineered human heavy-chain ferritin (HFn) with the inserted functional peptide PAS and RGDK to extend half-life and improve tumor targeted drug delivery. A facile and cost-effective two-step purification pathway for recombinant HFn was developed. The genetic modification was found to affect HFn conformation, and therefore varied the purification performance. Heat-acid precipitation followed by butyl fast flow hydrophobic interaction chromatography (HIC) has been developed to purify HFn and modified HFns. Nucleic acid removal reached above 99.8% for HFn and modified HFns. However, HFn purity reached above 95% and recovery yield (overall) above 90%, compared with modified HFns purity above 82% and recovery yield (overall) above 58%. It is interesting to find that the inserted functional peptides significantly changed the molecule conformation, where a putative turnover of the E-helix with the inserted functional peptides formed a "flop" conformation, in contrast with the "flip" conformation of HFn. It could be the cause of fragile stability of modified HFns, and therefore less tolerant to heat and acid condition, observed by the lower recovery yield in heat-acid precipitation.

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“…In batch processing, the use of salt‐tolerant mixed‐mode resins with a previous flow‐through step allows processing at elevated salt concentrations, which suppress VP1‐DNA aggregation, and therefore leads to better recovery. The salt‐tolerant mixed‐mode resin furthermore allows an integration of the two‐unit operations without buffer adjustment in between and enables a wide design space (Gerstweiler et al, 2021b, 2021c). The continuous process described in this study, developed by building on these batch studies, produces VLPs of a constant good quality, removes DNA and most contaminants, is scalable and can act as a platform technology for the development for new continuous production pathways of vaccines and biopharmaceuticals other than monoclonal antibodies.…”

Section: Introductionmentioning

confidence: 99%

“…The process couples a flow through Capto™ Q chromatography step followed by a bind-elute multimodal (Capto™ MMC) PCC process with subsequent in-line assembly of VLPs. It has been previously shown that nonpurified VP1 capsomeres form soluble aggregates with microbial DNA at low buffer salt concentrations, hindering purification (Gerstweiler et al, 2021b). In batch processing, the use of salt-tolerant mixed-mode resins with a previous flow-through step allows processing at elevated salt concentrations, which suppress VP1-DNA aggregation, and therefore leads to better recovery.…”

mentioning

confidence: 99%

An integrated and continuous downstream process for microbial virus‐like particle vaccine biomanufacture

Gerstweiler

Billakanti²,

et al. 2022

Biotech & Bioengineering

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In this study, we present the first integrated and continuous downstream process for the production of microbial virus‐like particle vaccines. Modular murine polyomavirus major capsid VP1 with integrated J8 antigen was used as a model virus‐like particle vaccine. The integrated continuous downstream process starts with crude cell lysate and consists of a flow‐through chromatography step followed by periodic counter‐current chromatography (PCC) (bind‐elute) using salt‐tolerant mixed‐mode resin and subsequent in‐line assembly. The automated process showed a robust behavior over different inlet feed concentrations ranging from 1.0 to 3.2 mg ml−1 with only minimal adjustments needed, and produced continuously high‐quality virus‐like particles, free of nucleic acids, with constant purity over extended periods of time. The average size remained constant between 44.8 ± 2.3 and 47.2 ± 2.9 nm comparable to literature. The process had an overall product recovery of 88.6% and a process productivity up to 2.56 mg h−1 mlresin−1 in the PCC step, depending on the inlet concentration. Integrating a flow through step with a subsequent PCC step allowed streamlined processing, showing a possible continuous pathway for a wide range of products of interest.

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Virus‐like particle preparation is improved by control over capsomere‐DNA interactions during chromatographic purification

Cited by 7 publications

References 58 publications

Process development for cross‐flow diafiltration‐based VLP disassembly: A novel high‐throughput screening approach

Process development for cross‐flow diafiltration‐based VLP disassembly: A novel high‐throughput screening approach

Development of purification process for dual‐function recombinant human heavy‐chain ferritin by the investigation of genetic modification impact on conformation

An integrated and continuous downstream process for microbial virus‐like particle vaccine biomanufacture

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