AUC Insights - Assessing the quality of adeno-associated virus gene therapy vectors by sedimentation velocity analysis
Introduction
Since the first gene therapy study in the late 1980s, there has been an ongoing interest in gene therapy strategies. According to Ginn et al. (1) about 2600 gene therapy clinical trials are being completed, ongoing or approved in 2018. The largest number of trials is concerned with cancer, followed by monogenic and infectious diseases (Table 1). In general, gene therapies can be divided into nonviral or viral delivery systems. Nonviral systems are usually characterized by an undirected and inefficient delivery and only transient expression; on the contrary, they show a larger packaging capacity and a better biosafety profile than viral gene therapies (1). However, the great advantage of viral systems lies in their high delivery efficiency and the exploitation of the viral biology (being able to infect host cells and to exploit their replication machinery). Among the known viral delivery systems, adenoviruses are used most often, followed by retroviruses and adeno-associated viruses (AAV). Interestingly, AAV show an increase in interest in recent years in contrast to other virus types (1). One reason might be the fact that AAV is less immunogenic than other viruses (2).
Gene Therapy Clinical Trials | |
Cancer Diseases | 65% |
Monogenetic Diseases | 11.1% |
Infectious Diseases | 7% |
Cardiovasular Diseases | 6.9% |
Others | 10% |
Tab. 1: Distribution of completed, ongoing or approved clinical trails by disease category 2018, in % (1) |
Adeno-Associated Viruses
AAV is a nonpathogenic, nonenveloped parvovirus with the size of approx. 22 nm that is not able to replicate without the assistance of a helper virus (adeno- or herpes simplex virus) (2). The virus capsid can carry a transgene of about 5kb (including viral ITR sequences) without significant reduction in viral production yields (2). A promoter, the gene of interest and a terminator are cloned between both ITR sequences. After transduction, the transgene is present as an episome in the nucleus from where the expression of the gene of interest takes place. The episomal DNA limits the risk of integration but it might be diluted out after several cell cycles (3). Several AAV serotypes are used as gene therapy vectors. These serotypes show a specific tissue-tropism thus limit their use to certain organs. Efforts are made to optimize the capsid and therefore modulate the viral tropism to certain cell types (4, 5).
Example 1: Quality control of rAAV vectors by AUC
Due to its popularity and increased usage, it is of major interest to assess the quality of clinical-grade rAAV vectors before administration.
3D CG rendered image of Adeno-Associated Virus (AAV) Capsid |
Burnham and colleagues (6) showed that sedimentation velocity analytical ultracentrifugation (AUC) experiments are able to characterize the quality of viral vector productions (ratio between empty and filled capsids). A single AUC experiment provides insights into the composition of the encapsulated DNA, the success of the purification, the presence of aggregates and the ratio between empty, partially filled and filled viral particles. The AAV samples are measured at 260 nm at a speed of 20,000 rpm (6). A peak at 63S corresponds to empty vector capsids whereas a peak at 93S shows the proportion of filled capsids. There are also peaks between 63S and 93S visible, which might be partially filled capsids, and finally larger peaks (larger than 93S) appeared that could be aggregated viral particles. Furthermore, the scientists tried to assess if the AUC is able to discriminate between transgenes of different sizes. Firstly, they used a transgene of 3370 nucleotides in length that yields an s-value of about 92 after sedimentation velocity whereas a transgene of 4200 nucleotides results in a peak with an s-value of 101. Taken together, the AUC is a valuable tool to analyze rAAV vectors notwithstanding the composition and length of the transgene or the viral serotype.
Example 2: Sedimentation Velocity analysis with exceptional resolution proves to be the gold standard for interpreting orthogonal techniques
In the following example, Wang et. al. have investigated the potential of anion exchange chromatography (AEX) for the determination of empty and full AAV capsids and also for other populations in the sample like partially loaded capsids (7). They also mentioned transmission electron microscopy (TEM) and a number of other techniques like ELISA in combination with qPCR as possible methods to verify the quality of AAVs. However, they acknowledge that the AUC is the gold standard in the detection and characterization of AAV particles. TEM is not a quantitative method, giving rather qualitative information on the tested AAV batch. ELISA/qPCR and CDMS are shown to not be accurate enough to provide proper resolution. Finally, they directly compared AEX and AUC: AUC showed a much higher resolution as compared to AEX – as evident in the baseline separation between empty and full capsids in the AUC experiment. The comparable AEX experiment shows the empty capsids as an overlapped shoulder peak of the main filled-capsid peak. The AUC experiment even revealed a small population of what might be fragmented genome capsids. This species was not visible in AEX (Figure 1).
In contrast to AUC, every chromatographic technique uses a matrix, which particles have to pass through. Thus, not only can particles interact with the matrix, but also dilution effects might dissolve aggregated AAV particles and finally might falsify the true picture of a virus batch. AUC as a matrix-free in-method allows the characterization in a near-native environment.
Optima AUC
- First-principle technique that does not depend on a matrix and does not require standards
- Samples are analyzed in their native state with almost no buffer restrictions
- One experiment reveals information about shape, diameter, mass, stoichiometry, purity, formulation heterogeneity, aggregation, association and conformation of a protein or protein complex
- Optical systems
- Rayleigh Interface
- UV absorbance
- Sample volume:
Max. Volume for 2-sector centerpieces: 450μl
Max. volume for 6-channel equilibrium center-pieces: 120μl - Wavelength range: 190-800 nm
- Molecular weight range:
102 Da (i.e. Peptides/Oligosaccharides) -108 Da (i.e. Viruses/Organelles) - Concentration range:
UV absorption: 0.005 – 1-2 mg/ml Lutenizing
Hormone Interference: 0.025 – 4-5 mg/ml BSA
References
- Gene therapy clinical trials worldwide to 2017: An update. Ginn SL, Amaya AK, Alexander IE, Edelstein M & Abedi MR; (2018) Journal of Gene Medicine 20:e3015
- Adeno-Associated Virus (AAV) as a Vector for Gene Therapy. Naso MF, Tomkowicz B, Perry III WL & Strohl WR; (2017) BioDrugs 31:317-334/li>
- Gene therapy comes of age. Dunbar CE, High KA, Joung JK, Kohn DB, Ozawa K & Sadelain M; (2018) Science 359, Issue 6372, eaan4672/li>
- A brain microvascular endothelial cell-specific viral vector with the potential to treat neurovascular and neurological diseases. Körbelin J, Dogbevia G, Michelfelder S, Ridder DA, Hunger A, Wenzel J, Seismann H, Lampe M, Bannach J, Pasparakis M, Kleinschmidt JA, Schwaninger M & Trepel M; (2016) EMBO Molecular Medicine, (8)6/li>
- Pulmonary Targeting of Adeno-associated Viral Vectors by Next-generation Sequencing-guided Screening of Random Capsid Displayed Peptide Libraries. Körbelin J, Sieber T, Michelfelder S, Lunding L, Spies E, Hunger A, Alawi M, Rapti K, Indenbirken D, Müller OJ, Pasqualini R, Arap W, Kleinschmidt JA & Trepel M; (2016) Molecular Therapy, (24)6, 1050-1061/li>
- Analytical Ultracentrifugation as an Approach to Characterize Recombinant AAV Vectors. Burnham B, Nass S, Kong E, Mattingly M, Woodcock D, Song A, Wadsworth S, Cheng SH, Scaria A & O`Riodran CR; (2015) Human Gene Therapy Methods, 26(6), 228-42/li>
- Developing an Anion Exchange Chromatography Assay for Determining Empty and Full Capsid Contents in AAV6.2. Wang C, Mulagapati SHR, Chen Z, Du J, Zhao X, Chen L, Linke T, Gao C, Schmelzer AE & Liu D; (2019) Molecular Therapy Methods & Clinical Development, 15:257-63
(*) This image is used under a Creative Commons Attribution 4.0 International license (https://creativecommons.org/licenses/by/4.0/), and the image has not been edited.
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- Fundamentals of Ultracentrifugal Virus Purification
- 产品目录
- 单页
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专家访谈
- Background and Current Status of the Introduction of Flow Cytometers
- Benefits-of-the-coulter-principle-in-the-manufacturing-for-ips-cell-derived-natural-killer-cells
- Central Diagnosis in the Treatment of Childhood Leukemia 1
- Central Diagnosis in the Treatment of Childhood Leukemia 2
- Challenges-in-viability-cell-counting
- Contribution of Cytobank to 1-cell analysis of the cancer microenvironment
- Development of technology for social implementation of synthetic biology
- Flow Cytometry Testing in Hospital Laboratories
- Fundamentals of Ultracentrifugal Virus Purification
- The MET ONE 3400+ Automates Routine Environmental Monitoring for GMP Cleanroom Compliance
- Tumor Suppressor Gene p53 research and DNA Cleanup Process
- Fundamentals of Ultracentrifugal Virus Purification
- Dr Yabui UCF Lecture
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主题报告
- Applications of Ultracentrifugation in Purification and Characterization of Biomolecules
- Automating Genomic DNA Extraction from Whole Blood and Serum with GenFind V3 on the Biomek i7 Hybrid Genomic Workstation
- ABRF 2019: Automated Genomic DNA Extraction from Large Volume Whole Blood
- Automated library preparation for the MCI Advantage Cancer Panel at Miami Cancer Institute utilizing the Beckman Coulter Biomek i5 Span-8 NGS Workstation
- Automating Cell Line Development for Biologics
- Cell-Line Engeneering
- Characterizing the Light-Scatter Sensitivity of the CytoFLEX Flow Cytometer
- AACR 2019: Isolation and Separation of DNA and RNA from a Single Tissue or Cell Culture Sample
- Mastering Cell Counting
- Preparing a CytoFLEX for Nanoscale Flow Cytometry
- A Prototype CytoFLEX for High-Sensitivity, Multiparametric Nanoparticle Analysis
- ABRF 2019: Simultaneous DNA and RNA Extraction from Formalin-Fixed Paraffin Embedded (FFPE) Tissue
- Quantification of AAV Capsid Loading Fractions: A Comparative Study
- Using Standardized Dry Antibody Panels for Flow Cytometry in Response to SARS-CoV2 Infection
- 产品说明书
- 实验步骤
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白皮书
- Centrifugation is a complete workflow solution for protein purification and protein aggregation quantification
- AUC Insights - Analysis of Protein-Protein-Interactions by Analytical Ultracentrifugation
- A General Guide to Lipid Nanoparticles
- Addressing issues in purification and QC of Viral Vectors
- GMP Cleanrooms Classification and Routine Environmental Monitoring
- Purification of Biomolecules by DGUC
- AUC Insights - Assessing the quality of adeno-associated virus gene therapy vectors by sedimentation velocity analysis
- AUC Insights - Sample concentration in the Analytical Ultracentrifuge AUC and the relevance of AUC data for the mass of complexes, aggregation content and association constants
- Analyzing Biological Systems with Flow Cytometry
- 亚可见颗粒物检测新进展:USP <1788>的最新修订
- Changes to USP <643> Total Organic Carbon
- Characterization of RNAdvance Viral XP RNA Extraction Kit using AccuPlex™ SARS–CoV–2 Reference Material Kit
- CytoFLEX Platform Flow Cytometers with IR Laser Configurations: Considerations for Red Emitting Dyes
- Evaluation of the Analytical Performance of the AQUIOS CL Flow Cytometer in a Multi-Center Study
- Simultaneous Isolation and Parallel Analysis of gDNA and total RNA for Gene Therapy
- Hydraulic Particle Counter Sample Preparation
- Inactivation of COVID–19 Disease Virus SARS–CoV–2 with Beckman Coulter Viral RNA Extraction Lysis Buffers
- Tips for Cell Sorting
- IVD-R Annex I Global Safety and Performances Requirements
- Liquid Biopsy Cancer Biomarkers – Current Status, Future Directions
- MET ONE 3400+ IT Implementation Guide
- Reproducibility in Flow Cytometry
- SuperNova v428: New Bright Polymer Dye for Flow Cytometry
- SuperNova v428: New Bright Polymer Dye for Flow Cytometry
- Japan Document
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应用手册