Ocular Inflammatory Response to Intravitreal Injection of Adeno-Associated Virus Vector: Relative Contribution of Genome and Capsid

Timmers, Adrian M.; Newmark, Judith A.; Turunen, Heikki; Farivar, Tanaz; Liu, Jilin; Song, Chunjuan; Ye, Guo‐Jie; Pennock, Steven; Gaskin, Chantelle; Knop, David R.; Shearman, Mark S.

doi:10.1089/hum.2019.144

Cited by 61 publications

(54 citation statements)

References 27 publications

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“…An alternative hypothesis is that inflammation is associated with specific vector variables, including the immunogenicity of specific viral capsids, high viral dose, and contamination from lipopolysaccharide, proteins, or empty viral capsids owing to different packaging protocols. 6,15,16 To address these possibilities, we used serial OCT imaging as a sensitive method for detecting anterior chamber cell and vitritis in murine eyes. 12,17,18 We also tested four different AAV preparations that varied over a range of viral doses (10 9 -10 11 viral genomes/eye), by packaging capsid (AAV2 or AAV2-7m8), cargo plasmid (see maps in Supplementary Fig.…”

Section: Resultsmentioning

confidence: 99%

“…These findings may be explained by the presence of neutralizing antibodies in the vitreous of Exposed:AAV eyes that could have impacted vector concentration and decreased early innate signaling within the eye. 15,20 Priming also influenced the timing of the adaptive immune response. Both dendritic cells and T cells were significantly more numerous in Exposed:AAV eyes than in Naive:AAV eyes on day 7.…”

Section: Discussionmentioning

confidence: 99%

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Characterization of Gene Therapy Associated Uveitis Following Intravitreal Adeno-Associated Virus Injection in Mice

Tummala

Crain

Rowlan

et al. 2021

Invest. Ophthalmol. Vis. Sci.

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Purpose To characterize the intraocular immune cell infiltrate induced by intravitreal adeno-associated virus (AAV) gene therapy. Methods AAV vectors carrying plasmids expressing green fluorescent protein under the control of PR2.1 were injected intravitreally into AAV naive and AAV primed C57Bl/6 mice. Clinical inflammation was assessed using optical coherence tomography. Intraocular immune cell populations were identified and quantified by flow cytometry on days 1, 7, and 29 after intravitreal injection and compared with sham and fellow eye controls. Results Optical coherence tomography inflammation score and total CD45+ cell number were significantly higher in AAV injected eyes compared to uninjected fellow eye and sham injected controls. Clinically apparent inflammation (vitritis on optical coherence tomography) and cellular inflammation (CD45+ cell number) was significantly increased in AAV injected eyes and peaked around day 7. Vitritis resolved by day 29, but cellular inflammation persisted through day 29. On day 1, neutrophils and activated monocytes were the dominant cell populations in all AAV injected eyes. On day 7, eyes of AAV exposed animals had significantly more dendritic cells and T cells than eyes of AAV naive animals. By day 29, CD8– T cells were the dominant CD45+ cell population in AAV injected eyes. Conclusions Intravitreal AAV injection in mice generates clinically evident inflammation that is mild and seems to resolve spontaneously. However, the total number of intraocular CD45+ cells, particularly T cells, remain elevated. Both innate and adaptive immune cells respond to intravitreal AAV regardless of prior immune status, but the adaptive response is delayed in AAV naive eyes.

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Section: Resultsmentioning

confidence: 99%

Section: Discussionmentioning

confidence: 99%

Characterization of Gene Therapy Associated Uveitis Following Intravitreal Adeno-Associated Virus Injection in Mice

Tummala

Crain

Rowlan

et al. 2021

Invest. Ophthalmol. Vis. Sci.

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“…Intravitreal injections target a larger retinal area. Intravitreal injections of empty rAAV capsids can induce a temporary immune inflammation of the aqueous and the vitreous [ 303 ]. Enzymatic digestion (proteasome inhibitors) of the ILM or ILM/outer limiting membrane (OLM) or disruptions of the ILM/OLM by the disease can alter rAAV infection and allow rAAV infection deeper into the retina [ 99 , 294 , 304 , 305 ].…”

Section: Transgene and Bioactivity Assays In Ocular Tissuementioning

confidence: 99%

“…However, the innate, humoral, and cell-mediated immune response might contribute to vector toxicity. For example, intravitreally injected empty rAAV capsids can induce a transient inflammation of the aqueous and the vitreous body [ 303 ]. Most importantly, cis-regulatory-sequence, rAAV-capsid, and transgene-related toxicity need to be investigated in the retinal degeneration model.…”

Section: Transgene and Bioactivity Assays In Ocular Tissuementioning

confidence: 99%

“…Most importantly, cis-regulatory-sequence, rAAV-capsid, and transgene-related toxicity need to be investigated in the retinal degeneration model. Further, the more efficient gene expression cassettes might allow a rescue strategy at lower rAAV titers, thereby causing less toxicity and lower transient inflammation [ 303 ].…”

Section: Transgene and Bioactivity Assays In Ocular Tissuementioning

confidence: 99%

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Recombinant Adeno-Associated Viral Vectors (rAAV)-Vector Elements in Ocular Gene Therapy Clinical Trials and Transgene Expression and Bioactivity Assays

Buck

Wijnholds

2020

IJMS

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Inherited retinal dystrophies and optic neuropathies cause chronic disabling loss of visual function. The development of recombinant adeno-associated viral vectors (rAAV) gene therapies in all disease fields have been promising, but the translation to the clinic has been slow. The safety and efficacy profiles of rAAV are linked to the dose of applied vectors. DNA changes in the rAAV gene cassette affect potency, the expression pattern (cell-specificity), and the production yield. Here, we present a library of rAAV vectors and elements that provide a workflow to design novel vectors. We first performed a meta-analysis on recombinant rAAV elements in clinical trials (2007–2020) for ocular gene therapies. We analyzed 33 unique rAAV gene cassettes used in 57 ocular clinical trials. The rAAV gene therapy vectors used six unique capsid variants, 16 different promoters, and six unique polyadenylation sequences. Further, we compiled a list of promoters, enhancers, and other sequences used in current rAAV gene cassettes in preclinical studies. Then, we give an update on pro-viral plasmid backbones used to produce the gene therapy vectors, inverted terminal repeats, production yield, and rAAV safety considerations. Finally, we assess rAAV transgene and bioactivity assays applied to cells or organoids in vitro, explants ex vivo, and clinical studies.

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Formulation and Evaluation of Polymer‐Based Nanoparticles for Intravitreal Gene‐Delivery Applications

et al. 2022

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The advent of the first-ever retinal gene therapy product, involving subretinal administration of a virus-based gene delivery platform, has garnered hope that this state-of-the-art therapeutic modality may benefit a broad spectrum of patients with diverse retinal disorders. On the other hand, clinical studies have revealed limitations of the applied delivery strategy that may restrict its universal use. To this end, intravitreal administration of synthetic gene-delivery platforms, such as polymer-based nanoparticles (PNPs), has emerged as an attractive alternative to the current mainstay. To achieve success, however, it is imperative that synthetic platforms overcome key biological barriers in human eyes encountered following intravitreal administration, including the vitreous gel and inner limiting membrane (ILM). Here, we introduce a series of experiments, from the fabrication of PNPs to a comprehensive evaluation in relevant experimental models, to determine whether PNPs overcome these barriers and efficiently deliver therapeutic gene payloads to retinal cells. We conclude the article by discussing a few important considerations for successful implementation of the strategy.

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Ocular Inflammatory Response to Intravitreal Injection of Adeno-Associated Virus Vector: Relative Contribution of Genome and Capsid

Cited by 61 publications

References 27 publications

Characterization of Gene Therapy Associated Uveitis Following Intravitreal Adeno-Associated Virus Injection in Mice

Characterization of Gene Therapy Associated Uveitis Following Intravitreal Adeno-Associated Virus Injection in Mice

Recombinant Adeno-Associated Viral Vectors (rAAV)-Vector Elements in Ocular Gene Therapy Clinical Trials and Transgene Expression and Bioactivity Assays

Formulation and Evaluation of Polymer‐Based Nanoparticles for Intravitreal Gene‐Delivery Applications

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