Analytical separation of plasmid DNA isoforms using anion exchanging chromatographic monoliths with 6 µm channels

Pavlin, Nejc; Černigoj, Urh; Bavčar, Mojca; Plesničar, Tjaša; Mavri, Jan; Zidar, Martin; Bone, Matevž; Kralj Savič, Urška; Sever, Tadej; Štrancar, Aleš

doi:10.1002/elps.202300031

Cited by 5 publications

(5 citation statements)

References 25 publications

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“…A part of the published manuscripts was also presented at the last Monolith Summer Symposium that was held last year in Portorož, Slovenia. As a logical consequence of the spirit of this time, the topics of most papers that are summarized here are dealing with purification of nanoparticles like viruses [1][2][3], plasmid DNA isoforms [4,5] and RNA drug substances [6]. As is well known, monolithic stationary phases (including membranes) were firstly developed for fast separation of proteins [7], but only the last manuscript in this issue reports the development of a new monolithic stationary phase for protein separation [8].…”

Section: Introductionmentioning

confidence: 99%

“…The next three papers are dedicated to fractionation of materials containing different DNA and RNA forms [4][5][6]. Kralj et al reported the optimization of production of large plasmid DNA isoforms with sizes over 10 kbp using anion exchange monoliths.…”

Section: Introductionmentioning

confidence: 99%

“…Pavlin et al [5] demonstrated again that channel diameter plays a crucial role in production of plasmid DNA (pDNA) purification processes. They demonstrated that pDNA open circular forms can be physically entrapped inside narrow channels of monolith, and demonstrated that this type of monolithic problem can be solved by the use of a column with larger (6 µm) channels with a fine-tuned surface chemistry.…”

Section: Introductionmentioning

confidence: 99%

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Editorial

Josic

2023

Electrophoresis

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Section: Introductionmentioning

confidence: 99%

Section: Introductionmentioning

confidence: 99%

Section: Introductionmentioning

confidence: 99%

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Editorial

Josic

2023

Electrophoresis

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“…Plasmids pHELP (11.6 kbp, 19% OC, 81% SC), pmFIX6 (6.7 kbp, 1% OC, 7% lin, 82% SC, 10% multimers [MM]; 1.8% gDNA), pGMAAV8_Rep-Cap (7.3 kbp, 7% OC, 1% lin, 92% SC; 0.25% gDNA) and pIVTeGFP (3.3 kbp, 4% OC, 67% SC, 28% MM) were stored in 50 mM TRIS, 10 mM EDTA, 0.75 M NaCl, pH 7.2. Isoform purity for each of the plasmids was determined by CIMac pDNA AEX HPLC analysis as described previously (Pavlin et al, 2023) and the gDNA content was determined with qPCR.…”

mentioning

confidence: 99%

“…Column (6 µm chan-nels) were performed as previously described (Pavlin et al, 2023). Samples were diluted with binding MP used for analysis to reduce AS concentration below 0.5 M (e.g., samples in 1.55 M AS were diluted three times) and to reduce pDNA concentration, ideally to 10 ng/µL (e.g., sample with 90 ng of pDNA/µL was diluted nine times).…”

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confidence: 99%

Selective hydrophobic interaction chromatography for high purity of supercoiled DNA plasmids

Božič,

Sedlar,

Kralj

et al. 2024

Biotech & Bioengineering

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High purity of plasmid DNA (pDNA), particularly in supercoiled isoform (SC), is used for various biopharmaceutical applications, such as a transfecting agent for production of gene therapy viral vectors, for pDNA vaccines, or as a precursor for linearized form that serves as a template for mRNA synthesis. In clinical manufacturing, pDNA is commonly extracted from Escherichia coli cells with alkaline lysis followed by anion exchange chromatography or tangential flow filtration as a capture step for pDNA. Both methods remove a high degree of host cell contaminants but are unable to generically discriminate between SC and open‐circular (OC) pDNA isoforms, as well as other DNA impurities, such as genomic DNA (gDNA). Hydrophobic interaction chromatography (HIC) is commonly used as polishing purification for pDNA. We developed HIC‐based polishing purification methodology that is highly selective for enrichment of SC pDNA. It is generic with respect to plasmid size, scalable, and GMP compatible. The technique uses ammonium sulfate, a kosmotropic salt, at a concentration selective for SC pDNA binding to a butyl monolith column, while OC pDNA and gDNA are removed in flow‐through. The approach is validated on multiple adeno‐associated virus‐ and mRNA‐encoding plasmids ranging from 3 to 12 kbp. We show good scalability to at least 300 mg of >95% SC pDNA, thus paving the way to increase the quality of genomic medicines that utilize pDNA as a key raw material.

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Effect of plasmid DNA isoforms on preparative anion exchange chromatography

Kralj,

Kodermac,

Bergoč

et al. 2023

Electrophoresis

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Increased need for plasmid DNA (pDNA) with sizes above 10 kbp (large pDNA) in gene therapy and vaccination brings the need for its large‐scale production with high purity. Chromatographic purification of large pDNA is often challenging due to low process yields and column clogging, especially using anion‐exchanging columns. The goal of our investigation was to evaluate the mass balance and pDNA isoform composition at column outlet for plasmids of different sizes in combination with weak anion exchange (AEX) monolith columns of varying channel size (2, 3 and 6 µm channel size). We have proven that open circular pDNA (OC pDNA) isoform is an important driver of reduced chromatographic performance in AEX chromatography. The main reason for the behaviour is the entrapment of OC pDNA in chromatographic supports with smaller channel sizes. Entrapment of individual isoforms was characterised for porous beads and convective monolithic columns. Convective entrapment of OC pDNA isoform was confirmed on both types of stationary phases. Porous beads in addition showed a reduced recovery of supercoiled pDNA (on an 11.6 kbp plasmid) caused by diffusional entrapment within the porous structure. Use of convective AEX monoliths or membranes with channel diameter >3.5 µm has been shown to increase yields and prevent irreversible pressure build‐up and column clogging during purification of plasmids at least up to 16 kbp in size.

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Analytical separation of plasmid DNA isoforms using anion exchanging chromatographic monoliths with 6 µm channels

Cited by 5 publications

References 25 publications

Editorial

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Selective hydrophobic interaction chromatography for high purity of supercoiled DNA plasmids

Effect of plasmid DNA isoforms on preparative anion exchange chromatography

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