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      AAV cis-regulatory sequences are correlated with ocular toxicity

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          Significance

          Adeno-associated viral (AAV) gene therapy is becoming an important therapeutic modality, especially for ocular diseases, due to its efficiency of gene delivery and relative lack of pathogenicity. However, AAV sometimes can cause inflammation and toxicity. We explored such effects using injections into the mouse eye. We found a strong correlation of toxicity and inflammation with the use of promoters that were broadly active, or specifically active in the retinal pigment epithelium. AAVs with photoreceptor-specific promoters were found to be nontoxic at all doses tested. These studies reveal that safer vectors can be designed if assays for relevant and specific cell types are developed and tested with a range of vectors with different genomic elements.

          Abstract

          Adeno-associated viral vectors (AAVs) have become popular for gene therapy, given their many advantages, including their reduced inflammatory profile compared with that of other viruses. However, even in areas of immune privilege such as the eye, AAV vectors are capable of eliciting host-cell responses. To investigate the effects of such responses on several ocular cell types, we tested multiple AAV genome structures and capsid types using subretinal injections in mice. Assays of morphology, inflammation, and physiology were performed. Pathological effects on photoreceptors and the retinal pigment epithelium (RPE) were observed. Müller glia and microglia were activated, and the proinflammatory cytokines TNF-α and IL-1β were up-regulated. There was a strong correlation between cis-regulatory sequences and toxicity. AAVs with any one of three broadly active promoters, or an RPE-specific promoter, were toxic, while AAVs with four different photoreceptor-specific promoters were not toxic at the highest doses tested. There was little correlation between toxicity and transgene, capsid type, preparation method, or cellular contaminants within a preparation. The toxic effect was dose-dependent, with the RPE being more sensitive than photoreceptors. Our results suggest that ocular AAV toxicity is associated with certain AAV cis-regulatory sequences and/or their activity and that retinal damage occurs due to responses by the RPE and/or microglia. By applying multiple, sensitive assays of toxicity, AAV vectors can be designed so that they can be used safely at high dose, potentially providing greater therapeutic efficacy.

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          Electroporation and RNA interference in the rodent retina in vivo and in vitro.

          Takahiko Matsuda, Constance L. Cepko (2004)
          The large number of candidate genes made available by comprehensive genome analysis requires that relatively rapid techniques for the study of function be developed. Here, we report a rapid and convenient electroporation method for both gain- and loss-of-function studies in vivo and in vitro in the rodent retina. Plasmid DNA directly injected into the subretinal space of neonatal rodent pups was taken up by a significant fraction of exposed cells after several pulses of high voltage. With this technique, GFP expression vectors were efficiently transfected into retinal cells with little damage to the operated pups. Transfected GFP allowed clear visualization of cell morphologies, and the expression persisted for at least 50 days. DNA-based RNA interference vectors directed against two transcription factors important in photoreceptor development led to photoreceptor phenotypes similar to those of the corresponding knockout mice. Reporter constructs carrying retinal cell type-specific promoters were readily introduced into the retina in vivo, where they exhibited the appropriate expression patterns. Plasmid DNA was also efficiently transfected into retinal explants in vitro by high-voltage pulses.
          Article 0 comments Cited 349 times – based on 0 reviews     Review now
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            Clades of Adeno-associated viruses are widely disseminated in human tissues.

            Guangping Gao, Luk H Vandenberghe, Mauricio R Alvira (2004)
            The potential for using Adeno-associated virus (AAV) as a vector for human gene therapy has stimulated interest in the Dependovirus genus. Serologic data suggest that AAV infections are prevalent in humans, although analyses of viruses and viral sequences from clinical samples are extremely limited. Molecular techniques were used in this study to successfully detect endogenous AAV sequences in 18% of all human tissues screened, with the liver and bone marrow being the most predominant sites. Sequence characterization of rescued AAV DNAs indicated a diverse array of molecular forms which segregate into clades whose members share functional and serologic similarities. One of the most predominant human clades is a hybrid of two previously described AAV serotypes, while another clade was found in humans and several species of nonhuman primates, suggesting a cross-species transmission of this virus. These data provide important information regarding the biology of parvoviruses in humans and their use as gene therapy vectors.
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              The Rd8 mutation of the Crb1 gene is present in vendor lines of C57BL/6N mice and embryonic stem cells, and confounds ocular induced mutant phenotypes.

              Mary Mattapallil, Eric F Wawrousek, Chi-Chao Chan (2012)
              We noted an unexpected inheritance pattern of lesions in several strains of gene-manipulated mice with ocular phenotypes. The lesions, which appeared at various stages of backcross to C57BL/6, bore resemblance to the rd8 retinal degeneration phenotype. We set out to examine the prevalence of this mutation in induced mutant mouse lines, vendor C57BL/6 mice and in widely used embryonic stem cells. Ocular lesions were evaluated by fundus examination and histopathology. Detection of the rd8 mutation at the genetic level was performed by PCR with appropriate primers. Data were confirmed by DNA sequencing in selected cases. Analysis of several induced mutant mouse lines with ocular disease phenotypes revealed that the disease was associated 100% with the presence of the rd8 mutation in the Crb1 gene rather than with the gene of interest. DNA analysis of C57BL/6 mice from common commercial vendors demonstrated the presence of the rd8 mutation in homozygous form in all C57BL/6N substrains, but not in the C57BL/6J substrain. A series of commercially available embryonic stem cells of C57BL/6N origin and C57BL/6N mouse lines used to generate ES cells also contained the rd8 mutation. Affected mice displayed ocular lesions typical of rd8, which were detectable by funduscopy and histopathology as early as 6 weeks of age. These findings identify the presence of the rd8 mutation in the C57BL/6N mouse substrain used widely to produce transgenic and knockout mice. The results have grave implications for the vision research community who develop mouse lines to study eye disease, as presence of rd8 can produce significant disease phenotypes unrelated to the gene or genes of interest. It is suggested that researchers screen for rd8 if their mouse lines were generated on the C57BL/6N background, bear resemblance to the rd8 phenotype, or are of indeterminate origin.
              Article 0 comments Cited 282 times – based on 0 reviews     Review now
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                Author and article information

                Journal
                Journal ID (nlm-ta): Proc Natl Acad Sci U S A
                Journal ID (iso-abbrev): Proc. Natl. Acad. Sci. U.S.A
                Journal ID (hwp): pnas
                Journal ID (pmc): pnas
                Journal ID (publisher-id): PNAS
                Title: Proceedings of the National Academy of Sciences of the United States of America
                Publisher: National Academy of Sciences
                ISSN (Print): 0027-8424
                ISSN (Electronic): 1091-6490
                Publication date (Print): 19 March 2019
                Publication date (Electronic): 4 March 2019
                Publication date PMC-release: 4 March 2019
                Volume: 116
                Issue: 12
                Pages: 5785-5794
                Affiliations
                [1] aDepartment of Biomedical Sciences, City University of Hong Kong , Kowloon, Hong Kong SAR, China;
                [2] bShenzhen Research Institute, City University of Hong Kong , Shenzhen 518057, China;
                [3] cDepartment of Genetics, Harvard Medical School , Boston, MA 02115;
                [4] dRetina Service, Massachusetts Eye and Ear Infirmary, Harvard Medical School , Boston, MA 02114;
                [5] eHoward Hughes Medical Institute , Chevy Chase, MD 20815
                Author notes
                2To whom correspondence may be addressed. Email: wenjun.xiong@ 123456cityu.edu.hk or cepko@ 123456genetics.med.harvard.edu .

                Contributed by Constance L. Cepko, January 27, 2019 (sent for review December 19, 2018; reviewed by Deniz Dalkara and Mark A. Kay)

                Author contributions: W.X., D.M.W., Y.X., and C.L.C. designed research; W.X., D.M.W., Y.X., S.K.W., M.J.C., X.J., P.R., S.R.Z., and S.M. performed research; W.X., D.M.W., Y.X., S.K.W., M.J.C., X.J., P.R., S.R.Z., S.M., and C.L.C. analyzed data; and W.X., D.M.W., Y.X., and C.L.C. wrote the paper.

                Reviewers: D.D., Université Pierre et Marie Curie; and M.A.K., Stanford University.

                1W.X., D.M.W., and Y.X. contributed equally to this work.

                Article
                Publisher ID: 201821000
                DOI: 10.1073/pnas.1821000116
                PMC ID: 6431174
                PubMed ID: 30833387
                SO-VID: 1c32bea8-f307-498e-b1c5-89fc58de13c1
                Copyright © Copyright © 2019 the Author(s). Published by PNAS.
                License:

                This open access article is distributed under Creative Commons Attribution-NonCommercial-NoDerivatives License 4.0 (CC BY-NC-ND).

                History
                Page count
                Pages: 10
                Funding
                Funded by: Howard Hughes Medical Institute (HHMI) 100000011
                Award ID: NA
                Award Recipient : Constance L Cepko
                Funded by: Astellas Pharma (Astellas) 501100004948
                Award ID: NA
                Award Recipient : Constance L Cepko
                Funded by: City University of Hong Kong (CityU) 100007567
                Award ID: 9610345
                Award Recipient : Wenjun Xiong
                Funded by: Research Grants Council, University Grants Committee (RGC, UGC) 501100002920
                Award ID: 21105916
                Award Recipient : Wenjun Xiong
                Funded by: National Natural Science Foundation of China (NSFC) 501100001809
                Award ID: 81770937
                Award Recipient : Wenjun Xiong
                Funded by: HHS | NIH | National Eye Institute (NEI) 100000053
                Award ID: K08-EY023993-05
                Award Recipient : David Mingdar Wu Award Recipient : Yunlu Xue
                Funded by: Massachusetts Lions Eye Research Fund, Iraty Award
                Award ID: NA
                Award Recipient : David Mingdar Wu Award Recipient : Michelle Chung
                Funded by: HHS | NIH | National Eye Institute (NEI) 100000053
                Award ID: U01 EY025497
                Award Recipient : David Mingdar Wu Award Recipient : Yunlu Xue
                Funded by: Howard Hughes medical Institute Medical Student Fellowship
                Award ID: NA
                Award Recipient : David Mingdar Wu Award Recipient : Michelle Chung
                Categories
                Subject: PNAS Plus
                Subject: Biological Sciences
                Subject: Neuroscience
                Series title: PNAS Plus

                Keywords: aav,gene therapy,toxicity,retina,retinal pigment epithelium
                Data availability:
                Keywords: aav, gene therapy, toxicity, retina, retinal pigment epithelium

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