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, Lauren M.; Lins, Bridget; Janssen, Maria; Bennett, Antonette; Chipman, Paul R.; McKenna, Robert; Chen, Weijun; Muzyczka, Nicholas; Cardone, Giovanni; Baker, Timothy S.; Agbandje‐McKenna, Mavis

doi:10.1128/jvi.00575-16

Cited by 41 publications

(39 citation statements)

References 63 publications

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“…Thus, these positions could constitute potential determinants of tissue tropism in murine ChPVs. Parvoviruses subfamilies Parvovirinae and Densovirinae utilize distinct strategies to stabilize their icosahedral capsids (35). Vertebrate parvoviruses extend the longer side of the jellyroll fold with an additional, N-terminal strand by folding back β-A to interact with the twofold axis of the very same monomer, hence creating an extended ABDIG sheet (36, 37).…”

Section: Discussionmentioning

confidence: 99%

An ancient lineage of highly divergent parvoviruses infects both vertebrate and invertebrate hosts

Pénzes

Souza

Agbandje‐McKenna

et al. 2019

Preprint

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2Chapparvoviruses are a highly divergent group of parvoviruses (family 3 Parvoviridae) first identified in 2013. Interest in these poorly characterized 4 viruses has been raised by recent studies indicating that they are the cause of 5 chronic kidney disease that arises spontaneously in laboratory mice. In this 6 study, we investigate the biological and evolutionary characteristics of 7 chapparvoviruses via comparative analysis of genome sequence data. Our 8 analysis, which incorporates sequences derived from endogenous viral 9 elements (EVEs) as well as exogenous viruses, reveals that 10 chapparvoviruses are an ancient lineage within the family Parvoviridae, 11 clustering separately from members of both currently established parvoviral 12 subfamilies. Consistent with this, they exhibit a number of characteristic 13 genomic and structural features, i.e. a large number of putative auxiliary 14 protein-encoding genes, capsid protein genes non-homologous to any hitherto 15 parvoviral cap, as well as a putative capsid structure lacking the canonical fifth 16 strand of the ABIDG sheet comprising the luminal side of the jelly roll. Our 17 findings demonstrate that the chapparvovirus lineage infects an exceptionally 18 broad range of host species, including both vertebrates and invertebrates.19Furthermore, we observe that chapparvoviruses found in fish are more closely 20 related to those from invertebrates than they are to those that infect amniote 21 vertebrates. This suggests that transmission between distantly related host 22 species may have occurred in the past. Our study provides the first integrated 23 overview of the chapparvovirus group, and revises current views of parvovirus 24 evolution 25 26 AUTHOR SUMMARY 27 Chapparvoviruses are a recently identified group of viruses about 28 which relatively little is known. However, recent studies have shown that these 29 viruses cause disease in laboratory mice and are prevalent in the fecal virome 30 of pigs and poultry, raising interest in their potential impact as pathogens, and 31 utility as experimental tools. We examined the genomes of chapparvoviruses 32 and endogenous viral elements ('fossilized' virus sequences derived from 33 ancestral viruses) using a variety of bioinformatics-based approaches. We 3 1 show that the chapparvoviruses have an ancient origin and are evolutionarily 2 distinct from all other related viruses. Accordingly, their genomes and virions 3 exhibit a range of distinct characteristic features. We examine the distribution 4 of these features in the light of chapparvovirus evolutionary history (which we 5 can also infer from genomic data), revealing new insights into chapparvovirus 6 biology. 7 8

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Section: Discussionmentioning

confidence: 99%

An ancient lineage of highly divergent parvoviruses infects both vertebrate and invertebrate hosts

Pénzes

Souza

Agbandje‐McKenna

et al. 2019

Preprint

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“…The harvested pellet (from lysed cells and polyethylene glycol precipitated supernatant) was freeze/thawed three times with Benzonase (EMD Millipore Cat#712053) treatment. After the third thaw, the resulting clarified supernatant was purified using a step iodixanol gradient followed by anion exchange 46 and then dialyzed into 50 mM HEPES, pH 7.4 with 2 mM MgCl 2 and 150 mM NaCl. The sample concentration was determined by optical density assuming an extinction coefficient of 1.7 mg mL −1 cm −1 ) for AAV2 VLPs.…”

Section: Methodsmentioning

confidence: 99%

Sub-2 Å Ewald curvature corrected structure of an AAV2 capsid variant

et al. 2018

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Single-particle cryogenic electron microscopy (cryo-EM) provides a powerful methodology for structural biologists, but the resolutions typically attained with experimentally determined structures have lagged behind microscope capabilities. Here, we exploit several technical advances to improve resolution, including per-particle contrast transfer function (CTF) refinement and correction for Ewald sphere curvature. The latter is demonstrated with several experimental samples and should become more standard as resolutions increase or at lower microscope accelerating voltages. The combined application of the described methods to micrographs recorded on a Titan Krios enables structure determination at ~1.86-Å resolution of an adeno-associated virus serotype 2 variant (AAV2), an important gene-delivery vehicle. The resulting structural details provide an improved model for understanding the biology of AAV that will guide future vector development for gene therapy.

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“…Trimeric subunits are colored green and pentameric subunits are colored cyan. Mutations with respect to the original I53-50 protein assembly 7 are colored blue (increases positive charge and/or decreases negative charge [e.g., E→N, N→K, E→K]), orange (no change in charge [e.g., E→D, N→T, K→R]), or red (decreases positive charge and/or increases negative charge [e.g., N→E, K→N, K→E]). b .…”

Section: Figurementioning

confidence: 99%

“…Several generations of evolution resulted in drastically improved genome packaging (>133-fold), stability in whole murine blood (from less than 3.7% to 71% of packaged RNA protected after 6 hours of treatment), and in vivo circulation time (from less than 5 minutes to 4.5 hours). The resulting synthetic nucleocapsids package one full-length RNA genome for every 11 icosahedral assemblies, similar to the best recombinant adeno-associated virus (AAV) vectors 7, 8 . Our results show that there are simple evolutionary paths through which protein assemblies can acquire virus-like genome packaging and protection.…”

mentioning

confidence: 99%

Evolution of a designed protein assembly encapsulating its own RNA genome

Butterfield

Lajoie

Gustafson

et al. 2017

Nature

184

237

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The challenges of evolution in a complex biochemical environment—coupling genotype to phenotype and protecting the genetic material—are solved elegantly in biological systems by nucleic acid encapsulation. In the simplest examples, viruses use capsids to surround their genomes. While these naturally occurring systems have been modified to change their tropism1 and to display proteins or peptides2–4, billions of years of evolution have favored efficiency at the expense of modularity, making viral capsids difficult to engineer. Synthetic systems composed of non-viral proteins could provide a “blank slate” to evolve desired properties for drug delivery and other biomedical applications, while avoiding the safety risks and engineering challenges associated with viruses. Here we create synthetic nucleocapsids—computationally designed icosahedral protein assemblies5, 6 with positively charged inner surfaces capable of packaging their own full-length mRNA genomes—and explore their ability to evolve virus-like properties by generating diversified populations using Escherichia coli as an expression host. Several generations of evolution resulted in drastically improved genome packaging (>133-fold), stability in whole murine blood (from less than 3.7% to 71% of packaged RNA protected after 6 hours of treatment), and in vivo circulation time (from less than 5 minutes to 4.5 hours). The resulting synthetic nucleocapsids package one full-length RNA genome for every 11 icosahedral assemblies, similar to the best recombinant adeno-associated virus (AAV) vectors7, 8. Our results show that there are simple evolutionary paths through which protein assemblies can acquire virus-like genome packaging and protection. Considerable effort has been directed at “top-down” modification of viruses to be safe and effective for drug delivery and vaccine applications1, 9, 10; the ability to computationally design synthetic nanomaterials and to optimize them through evolution now enables a complementary “bottom-up” approach with considerable advantages in programmability and control.

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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

Cited by 41 publications

References 63 publications

An ancient lineage of highly divergent parvoviruses infects both vertebrate and invertebrate hosts

An ancient lineage of highly divergent parvoviruses infects both vertebrate and invertebrate hosts

Sub-2 Å Ewald curvature corrected structure of an AAV2 capsid variant

Evolution of a designed protein assembly encapsulating its own RNA genome

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