Structure of neurotropic adeno-associated virus AAVrh.8

Halder, Sujata; Vliet, Kim Van; Smith, J. W. G.; Duong, Thao; McKenna, Robert; Wilson, James M.; Agbandje‐McKenna, Mavis

doi:10.1016/j.jsb.2015.08.017

Cited by 50 publications

(37 citation statements)

References 124 publications

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“…6A). This additional density is proximal to but does not overlap with the position of the nucleotide density observed in the capsid interior of the majority of other wt-AAV serotype capsid structures determined to date (58). While a nucleotide model was not built into this 3-fold density, its absence in the AAV2-R432A is consistent with its DNA packaging defect.…”

Section: Resultsmentioning

confidence: 79%

Cryo-electron Microscopy Reconstruction and Stability Studies of the Wild Type and the R432A Variant of Adeno-associated Virus Type 2 Reveal that Capsid Structural Stability Is a Major Factor in Genome Packaging

Drouin

Lins

Janssen

et al. 2016

J Virol

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The adeno-associated viruses (AAV) are promising therapeutic gene delivery vectors and better understanding of their capsid assembly and genome packaging mechanism is needed for improved vector production. Empty AAV capsids assemble in the nucleus prior to genome packaging by virally encoded Rep proteins. To elucidate the capsid determinants of this process, structural differences between wild-type (wt) AAV2 and a packaging deficient variant, AAV2-R432A, were examined using cryo-electron microscopy and three-dimensional image reconstruction both at an ϳ5.0-Å resolution (medium) and also at 3.8-and 3.7-Å resolutions (high), respectively. The high resolution structures showed that removal of the arginine side chain in AAV2-R432A eliminated hydrogen bonding interactions, resulting in altered intramolecular and intermolecular interactions propagated from under the 3-fold axis toward the 5-fold channel. Consistent with these observations, differential scanning calorimetry showed an ϳ10°C decrease in thermal stability for AAV2-R432A compared to wt-AAV2. In addition, the medium resolution structures revealed differences in the juxtaposition of the less ordered, N-terminal region of their capsid proteins, VP1/2/3. A structural rearrangement in AAV2-R432A repositioned the ␤A strand region under the icosahedral 2-fold axis rather than antiparallel to the ␤B strand, eliminating many intramolecular interactions. Thus, a single amino acid substitution can significantly alter the AAV capsid integrity to the extent of reducing its stability and possibly rendering it unable to tolerate the stress of genome packaging. Furthermore, the data show that the 2-, 3-, and 5-fold regions of the capsid contributed to producing the packaging defect and highlight a tight connection between the entire capsid in maintaining packaging efficiency. IMPORTANCEThe mechanism of AAV genome packaging is still poorly understood, particularly with respect to the capsid determinants of the required capsid-Rep interaction. Understanding this mechanism may aid in the improvement of AAV packaging efficiency, which is currently ϳ1:10 (10%) genome packaged to empty capsid in vector preparations. This report identifies regions of the AAV capsid that play roles in genome packaging and that may be important for Rep recognition. It also demonstrates the need to maintain capsid stability for the success of this process. This information is important for efforts to improve AAV genome packaging and will also inform the engineering of AAV capsid variants for improved tropism, specific tissue targeting, and host antibody escape by defining amino acids that cannot be altered without detriment to infectious vector production.T he adeno-associated viruses (AAVs) have emerged as attractive gene therapy vectors because they can package foreign genes and achieve stable, long-term gene expression in a broad range of tissues, with no known pathogenicity (1-3). AAVs are small, nonenveloped, icosahedral viruses (ϳ260 Å in diameter) that package ϳ4.7 kb of single-stran...

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Section: Resultsmentioning

confidence: 79%

Cryo-electron Microscopy Reconstruction and Stability Studies of the Wild Type and the R432A Variant of Adeno-associated Virus Type 2 Reveal that Capsid Structural Stability Is a Major Factor in Genome Packaging

Drouin

Lins

Janssen

et al. 2016

J Virol

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“…Notably, an AAV8-selective affinity resin was useful for the purification of a related serotype, AAVrh8R, while the performance of this serotype on an AAV9 selective resin was unsatisfactory. This result suggests that despite considerable sequence homology between AAV9 and AAVrh8R, 20 the epitope responsible for binding to the AAV9 resin is not shared; however, a common, as yet unidentified epitope facilitates binding of AAVrh8R to an AAV8-specific resin. These data are important, because they suggest that existing off-the-shelf serotype-specific affinity resins may be useful for the purification of disparate AAV capsids with conserved epitopes.…”

Section: Discussionmentioning

confidence: 94%

Universal Method for the Purification of Recombinant AAV Vectors of Differing Serotypes

Nass

Mattingly

Woodcock

et al. 2018

Molecular Therapy - Methods & Clinical Development

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103

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The generation of clinical good manufacturing practices (GMP)-grade adeno-associated virus (AAV) vectors requires purification strategies that support the generation of vectors of high purity, and that exhibit a good safety and efficacy profile. To date, most reported purification schemas are serotype dependent, requiring method development for each AAV gene therapy product. Here, we describe a platform purification process that is compatible with the purification of multiple AAV serotypes. The method generates vector preparations of high purity that are enriched for capsids with full vector genomes, and that minimizes the fractional content of empty capsids. The two-column purification method, a combination of affinity and ion exchange chromatographies, is compatible with a range of AAV serotypes generated by either the transient triple transfection method or the more scalable producer cell line platform. In summary, the adaptable purification method described can be used for the production of a variety of high-quality AAV vectors suitable for preclinical testing in animal models of diseases.

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“…AAV has evolved to enter cells through initial interactions with carbohydrates present on the surface of target cells, typically sialic acid, galactose and heparin sulfate [ 29 , 30 ]. Subtle differences in sugar-binding preferences, encoded in capsid sequence differences, can influence cell-type transduction preferences of the various AAV variants [ 31 – 33 ]. For example, AAV9 has a preference for primary cell binding through galactose as a result of unique amino acid differences in its capsid sequence [ 34 ].…”

Section: Aav Capsid Selection and Optimizationmentioning

confidence: 99%

Adeno-Associated Virus (AAV) as a Vector for Gene Therapy

et al. 2017

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There has been a resurgence in gene therapy efforts that is partly fueled by the identification and understanding of new gene delivery vectors. Adeno-associated virus (AAV) is a non-enveloped virus that can be engineered to deliver DNA to target cells, and has attracted a significant amount of attention in the field, especially in clinical-stage experimental therapeutic strategies. The ability to generate recombinant AAV particles lacking any viral genes and containing DNA sequences of interest for various therapeutic applications has thus far proven to be one of the safest strategies for gene therapies. This review will provide an overview of some important factors to consider in the use of AAV as a vector for gene therapy.

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Structure of neurotropic adeno-associated virus AAVrh.8

Cited by 50 publications

References 124 publications

Cryo-electron Microscopy Reconstruction and Stability Studies of the Wild Type and the R432A Variant of Adeno-associated Virus Type 2 Reveal that Capsid Structural Stability Is a Major Factor in Genome Packaging

Cryo-electron Microscopy Reconstruction and Stability Studies of the Wild Type and the R432A Variant of Adeno-associated Virus Type 2 Reveal that Capsid Structural Stability Is a Major Factor in Genome Packaging

Universal Method for the Purification of Recombinant AAV Vectors of Differing Serotypes

Adeno-Associated Virus (AAV) as a Vector for Gene Therapy

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