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2. Amplified Type I Interferon Response in Sjögren's Disease via Ectopic Toll‐Like Receptor 7 Expression in Salivary Gland Epithelial Cells Induced by Lysosome‐Associated Membrane Protein 3.

Author

Nakamura, Hiroyuki, Tanaka, Tsutomu, Zheng, Changyu, Afione, Sandra A., Atsumi, Tatsuya, Noguchi, Masayuki, Oliveira, Fabiola Reis, Motta, Ana Carolina F., Chahud, Fernando, Rocha, Eduardo M., Warner, Blake M., and Chiorini, John A.

Subjects
RNA analysis, EPITHELIAL cells, LYSOSOMES, BIOLOGICAL models, IN vitro studies, TOLL-like receptors, CELLULAR signal transduction, IN vivo studies, DESCRIPTIVE statistics, INTERFERONS, GENE expression, MICE, ANIMAL experimentation, GENE expression profiling, SJOGREN'S syndrome, SALIVARY glands, MEMBRANE proteins, SEQUENCE analysis, SYMPTOMS
Abstract

Objective: Lysosome‐associated membrane protein 3 (LAMP3) misexpression in salivary gland epithelial cells plays a causal role in the development of salivary gland dysfunction and autoimmunity associated with Sjögren's disease (SjD). This study aimed to clarify how epithelial LAMP3 misexpression is induced in SjD. Methods: To explore upstream signaling pathways associated with LAMP3 expression, we conducted multiple RNA sequencing analyses of minor salivary glands from patients with SjD, submandibular glands from a mouse model of SjD, and salivary gland epithelial cell lines. A hypothesis generated by the RNA sequencing analyses was further tested by in vitro and in vivo assays with gene manipulation. Results: Transcriptome analysis suggested LAMP3 expression was associated with enhanced type I interferon (IFN) and IFNγ signaling pathways in patients with SjD. In vitro studies showed that type I IFN but not IFNγ stimulation could induce LAMP3 expression in salivary gland epithelial cells. Moreover, we discovered that LAMP3 overexpression could induce ectopic Toll‐like receptor 7 (TLR‐7) expression and type I IFN production in salivary gland epithelial cells both in vitro and in vivo. TLR‐7 knockout mice did not develop any SjD‐related symptoms following LAMP3 induction. Conclusion: Epithelial LAMP3 misexpression can be induced through enhanced type I IFN response in salivary glands. In addition, LAMP3 can promote type I IFN production via ectopic TLR‐7 expression in salivary gland epithelial cells. This positive feedback loop can contribute to maintaining LAMP3 misexpression and amplifying type I IFN production in salivary glands, which plays an essential role in the pathophysiology of SjD. [ABSTRACT FROM AUTHOR]

Published
2024
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3. Adeno-Associated Virus Serotype 1 (AAV1)- and AAV5-Antibody Complex Structures Reveal Evolutionary Commonalities in Parvovirus Antigenic Reactivity

Author

Tseng, Yu-Shan, Gurda, Brittney L, Chipman, Paul, McKenna, Robert, Afione, Sandra, Chiorini, John A, Muzyczka, Nicholas, Olson, Norman H, Baker, Timothy S, Kleinschmidt, Jürgen, and Agbandje-McKenna, Mavis

Subjects
Genetics, Biotechnology, Gene Therapy, Infection, Good Health and Well Being, Antibodies, Monoclonal, Antibodies, Neutralizing, Antibodies, Viral, Cryoelectron Microscopy, Dependovirus, Epitope Mapping, Epitopes, Humans, Image Processing, Computer-Assisted, Macromolecular Substances, Models, Molecular, Protein Binding, Serogroup, Biological Sciences, Agricultural and Veterinary Sciences, Medical and Health Sciences, Virology
Abstract

UnlabelledThe clinical utility of the adeno-associated virus (AAV) gene delivery system has been validated by the regulatory approval of an AAV serotype 1 (AAV1) vector for the treatment of lipoprotein lipase deficiency. However, neutralization from preexisting antibodies is detrimental to AAV transduction efficiency. Hence, mapping of AAV antigenic sites and engineering of neutralization-escaping vectors are important for improving clinical efficacy. We report the structures of four AAV-monoclonal antibody fragment complexes, AAV1-ADK1a, AAV1-ADK1b, AAV5-ADK5a, and AAV5-ADK5b, determined by cryo-electron microscopy and image reconstruction to a resolution of ∼11 to 12 Å. Pseudoatomic modeling mapped the ADK1a epitope to the protrusions surrounding the icosahedral 3-fold axis and the ADK1b and ADK5a epitopes, which overlap, to the wall between depressions at the 2- and 5-fold axes (2/5-fold wall), and the ADK5b epitope spans both the 5-fold axis-facing wall of the 3-fold protrusion and portions of the 2/5-fold wall of the capsid. Combined with the six antigenic sites previously elucidated for different AAV serotypes through structural approaches, including AAV1 and AAV5, this study identified two common AAV epitopes: one on the 3-fold protrusions and one on the 2/5-fold wall. These epitopes coincide with regions with the highest sequence and structure diversity between AAV serotypes and correspond to regions determining receptor recognition and transduction phenotypes. Significantly, these locations overlap the two dominant epitopes reported for autonomous parvoviruses. Thus, rather than the amino acid sequence alone, the antigenic sites of parvoviruses appear to be dictated by structural features evolved to enable specific infectious functions.ImportanceThe adeno-associated viruses (AAVs) are promising vectors for in vivo therapeutic gene delivery, with more than 20 years of intense research now realized in a number of successful human clinical trials that report therapeutic efficacy. However, a large percentage of the population has preexisting AAV capsid antibodies and therefore must be excluded from clinical trials or vector readministration. This report represents our continuing efforts to understand the antigenic structure of the AAVs, specifically, to obtain a picture of "polyclonal" reactivity as is the situation in humans. It describes the structures of four AAV-antibody complexes determined by cryo-electron microscopy and image reconstruction, increasing the number of mapped epitopes to four and three, respectively, for AAV1 and AAV5, two vectors currently in clinical trials. The results presented provide information essential for generating antigenic escape vectors to overcome a critical challenge remaining in the optimization of this highly promising vector delivery system.

Published
2015

4. Association of G protein‐coupled receptor 78 with salivary dysfunction in male Sjögren's patients.

Author

Tanaka, Tsutomu, Guimaro, Maria C., Nakamura, Hiroyuki, Perez, Paola, Ji, Youngmi, Michael, Drew G., Afione, Sandra A., Zheng, Changyu, Goldsmith, Corinne, Swaim, William D., Pedersen, Anne Marie Lynge, and Chiorini, John A.

Subjects
IN vitro studies, EPITHELIAL cells, LYSOSOMES, T-test (Statistics), DATA analysis, STATISTICAL significance, RESEARCH funding, APOPTOSIS, IN vivo studies, REVERSE transcriptase polymerase chain reaction, DESCRIPTIVE statistics, ESTRADIOL, GENE expression profiling, CELL death, WESTERN immunoblotting, STATISTICS, SJOGREN'S syndrome, SALIVARY glands, DATA analysis software, CELL receptors
Abstract

Objective: Sjögren's disease (SjD) has a strong sex bias, suggesting an association with sex hormones. Male SjD represents a distinct subset of the disease, but the pathogenic mechanisms of male SjD is poorly characterized. The aim of this study is to identify initiating events related to the development of gland hypofunction and autoimmunity in male SjD patients. Materials and methods: Human minor salivary glands were transcriptomically analyzed with microarrays to detect differentially expressed genes in male SjD patients. Identified genes were tested on their involvement in the disease using conditional transgenic mice and gene‐overexpressing cells. Results: GPR78, an orphan G protein–coupled receptor, was overexpressed in the salivary glands of male SjD patients compared with male healthy controls and female SjD patients. Male GPR78 transgenic mice developed salivary gland hypofunction with increased epithelial apoptosis, which was not seen in control or female transgenic mice. In cell culture, GPR78 overexpression decreased lysosomal integrity, leading to caspase‐dependent apoptotic cell death. GPR78‐induced cell death in vitro was inhibited by treatment with estradiol. Conclusion: GPR78 overexpression can induce apoptosis and salivary gland hypofunction in male mice through lysosomal dysfunction and increased caspase‐dependent apoptosis in salivary gland epithelium, which may drive disease in humans. [ABSTRACT FROM AUTHOR]

Published
2024
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5. Lysosomal exocytosis of HSP70 stimulates monocytic BMP6 expression in Sjogren's syndrome

Author

Mo, Ying-Qian, Nakamura, Hiroyuki, Tanaka, Tsutomu, Odani, Toshio, Perez, Paola, Ji, Youngmi, French, Benjamin N., Pranzatelli, Thomas J.F., Michael, Drew G., Yin, Hongen, Chow, Susan S., Khalaj, Maryam, Afione, Sandra A., Zheng, Changyu, Oliveira, Fabiola Reis, Motta, Ana Carolina F., Ribeiro-Silva, Alfredo, Rocha, Eduardo M., Nguyen, Cuong Q., Noguchi, Masayuki, Atsumi, Tatsuya, Warner, Blake M., and Chiorini, John A.

Subjects
Gene expression -- Research, Immunological research, Autoimmunity -- Genetic aspects -- Health aspects, Heat shock proteins -- Genetic aspects -- Health aspects, Sjogren's syndrome -- Development and progression -- Genetic aspects, Exocytosis -- Research, Lysosomes -- Genetic aspects -- Health aspects, Health care industry
Abstract

BMP6 is a central cytokine in the induction of Sjogren's syndrome-associated (SS-associated) secretory hypofunction. However, the upstream initiation leading to the production of this cytokine in SS is unknown. In this study, RNA ISH on salivary gland sections taken from patients with SS indicated monocytic lineage cells as a cellular source of BMP6. RNA-Seq data on human salivary glands suggested that TLR4 signaling was an upstream regulator of BMP6, which was confirmed by in vitro cell assays and single-cell transcriptomics of human PBMCs. Further investigation showed that HSP70 was an endogenous natural TLR4 ligand that stimulated BMP6 expression in SS. Release of HSP70 from epithelial cells could be triggered by overexpression of lysosome-associated membrane protein 3 (LAMP3), a protein also associated with SS in several transcriptome studies. In vitro studies supported the idea that HSP70 was released as a result of lysosomal exocytosis initiated by LAMP3 expression, and reverse transcription PCR on RNA from minor salivary glands of patients with SS confirmed a positive correlation between BMP6 and LAMP3 expression. BMP6 expression could be experimentally induced in mice by overexpression of LAMP3, which developed an SS-like phenotype. The newly identified LAMP3/HSP70/BMP6 axis provided an etiological model for SS gland dysfunction and autoimmunity., Introduction Sjogren's syndrome (SS) is an autoimmune disease characterized by dry mouth and/or eye symptoms (sicca symptoms) and lymphocytic inflammation in salivary and/or lacrimal glands. The pathogenetic mechanism driving the [...]

Published
2022
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9. Lysosome‐Associated Membrane Protein 3 Induces Lysosome‐Dependent Cell Death by Impairing Autophagic Caspase 8 Degradation in the Salivary Glands of Individuals With Sjögren's Disease.

Author

Nakamura, Hiroyuki, Tanaka, Tsutomu, Zheng, Changyu, Afione, Sandra A., Warner, Blake M., Noguchi, Masayuki, Atsumi, Tatsuya, and Chiorini, John A.

Subjects
PROTEIN metabolism, PROTEINS, LYSOSOMES, AUTOPHAGY, ANIMAL experimentation, WESTERN immunoblotting, FLUORESCENT antibody technique, GLYCOPROTEINS, SALIVARY glands, SJOGREN'S syndrome, GLUCAGON-like peptides, CELL death, MICE
Abstract

Objective: Lysosome‐associated membrane protein 3 (LAMP3) overexpression is implicated in the development and progression of Sjögren's disease (SjD) by inducing lysosomal membrane permeabilization (LMP) and apoptotic cell death in salivary gland epithelium. The aim of this study was to clarify the molecular details of LAMP3‐induced lysosome‐dependent cell death and to test lysosomal biogenesis as a therapeutic intervention. Methods: Human labial minor salivary gland biopsies were analyzed using immunofluorescence staining for LAMP3 expression levels and galectin‐3 puncta formation, a marker of LMP. Expression level of caspase 8, an initiator of LMP, was determined by Western blotting in cell culture. Galectin‐3 puncta formation and apoptosis were evaluated in cell cultures and a mouse model treated with glucagon‐like peptide 1 receptor (GLP‐1R) agonists, a known promoter of lysosomal biogenesis. Results: Galectin‐3 puncta formation was more frequent in the salivary glands of SjD patients compared to control glands. The proportion of galectin‐3 puncta–positive cells was positively correlated with LAMP3 expression levels in the glands. LAMP3 overexpression increased caspase 8 expression, and knockdown of caspase 8 decreased galectin‐3 puncta formation and apoptosis in LAMP3‐overexpressing cells. Inhibition of autophagy increased caspase 8 expression, while restoration of lysosomal function using GLP‐1R agonists decreased caspase 8 expression, which reduced galectin‐3 puncta formation and apoptosis in both LAMP3‐overexpressing cells and mice. Conclusion: LAMP3 overexpression induced lysosomal dysfunction, resulting in lysosome‐dependent cell death via impaired autophagic caspase 8 degradation, and restoring lysosomal function using GLP‐1R agonists could prevent this. These findings suggested that LAMP3‐induced lysosomal dysfunction is central to disease development and is a target for therapeutic intervention in SjD. [ABSTRACT FROM AUTHOR]

Published
2023
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10. Salivary gland LAMP3 mRNA expression is a possible predictive marker in the response to hydroxychloroquine in Sjögren's disease.

Author

Nakamura, Hiroyuki, Tanaka, Tsutomu, Ji, Youngmi, Zheng, Changyu, Afione, Sandra A., Warner, Blake M., Oliveira, Fabiola Reis, Motta, Ana Carolina F., Rocha, Eduardo M., Noguchi, Masayuki, Atsumi, Tatsuya, and Chiorini, John A.

Subjects
SALIVARY glands, GENE expression, LYSOSOMES, HYDROXYCHLOROQUINE, CATHEPSIN B, CELL death
Abstract

Hydroxychloroquine (HCQ) is a lysosomotropic agent that is commonly used for treating Sjögren's disease (SjD). However, its efficacy is controversial because of the divergent response to the drug among patients. In a subgroup of SjD patients, lysosome-associated membrane protein 3 (LAMP3) is elevated in expression in the salivary glands and promotes lysosomal dysregulation and lysosome-dependent apoptotic cell death. In this study, chloroquine (CQ) and its derivative HCQ were tested for their ability to prevent LAMP3-induced apoptosis, in vitro and on a mouse model of SjD. In addition, efficacy of HCQ treatment was retrospectively compared between high LAMP3 mRNA expression in minor salivary glands and those with LAMP3 mRNA levels comparable with healthy controls. Study results show that CQ treatment stabilized the lysosomal membrane in LAMP3-overexpressing cells via deactivation of cathepsin B, resulting in decreased apoptotic cell death. In mice with established SjD-like phenotype, HCQ treatment also significantly decreased apoptotic cell death and ameliorated salivary gland hypofunction. Retrospective analysis of SjD patients found that HCQ tended to be more effective in improving disease activity index, symptom severity and hypergammaglobulinemia in patients with high LAMP3 expression compared those with normal LAMP3 expression. Taken together, these findings suggested that by determining salivary gland LAMP3 mRNA level, a patient's response to HCQ treatment could be predicted. This finding may provide a novel strategy for guiding the development of more personalized medicine for SjD. [ABSTRACT FROM AUTHOR]

Published
2023
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17. Defective regulation of outwardly rectifying Cl- channels by protein kinase A corrected by insertion of CFTR

Author

Egan, Marie, Flotte, Terence, Afione, Sandra, Solow, Rikki, Zeitlin, Pamela L., Carter, Barrie J., and Guggino, William B.

Subjects
Chloride channels -- Research, Cystic fibrosis -- Genetic aspects, Protein kinases -- Research, Genetic recombination -- Health aspects, Environmental issues, Science and technology, Zoology and wildlife conservation
Abstract

The expression of recombinant cystic fibrosis (CF) genes by means of adeno-associated virus vectors in CF bronchial epithelial cells stops the defective Cl- secretion, produces conductance Cl- channels and revives protein kinase A stimulation of outwardly rectifying Cl- channels. Hence it may be possible to use gene expression to treat CF, a severe genetic disease that results from a defective gene for the cystic fibrosis transmembrane conductance regulator protein.

Published
1992

18. Lysosome-associated membrane protein 3 misexpression in salivary glands induces a Sjögren's syndrome-like phenotype in mice.

Author

Hiroyuki Nakamura, Tsutomu Tanaka, Pranzatelli, Thomas, Youngmi Ji, Hongen Yin, Perez, Paola, Afione, Sandra A., Shyh-Ing Jang, Goldsmith, Corrine, Chang Yu Zheng, Swaim, William D., Warner, Blake M., Noriyuki Hirata, Masayuki Noguchi, Tatsuya Atsumi, Chiorini, John A., Nakamura, Hiroyuki, Tanaka, Tsutomu, Ji, Youngmi, and Yin, Hongen

Subjects
SIALADENITIS, ANIMAL experimentation, GLYCOPROTEINS, RESEARCH funding, SJOGREN'S syndrome, SALIVARY glands, PHENOTYPES, MICE
Abstract

Objectives: Sjögren's syndrome (SS) is an autoimmune sialadenitis with unknown aetiology. Although extensive research implicated an abnormal immune response associated with lymphocytes, an initiating event mediated by salivary gland epithelial cell (SGEC) abnormalities causing activation is poorly characterised. Transcriptome studies have suggested alternations in lysosomal function are associated with SS, but a cause and effect linkage has not been established. In this study, we demonstrated that altered lysosome activity in SGECs by expression of lysosome-associated membrane protein 3 (LAMP3) can initiate an autoimmune response with autoantibody production and salivary dysfunction similar to SS.Methods: Retroductal cannulation of the submandibular salivary glands with an adeno-associated virus serotype 2 vector encoding LAMP3 was used to establish a model system. Pilocarpine-stimulated salivary flow and the presence of autoantibodies were assessed at several time points post-cannulation. Salivary glands from the mice were evaluated using RNAseq and histologically.Results: Following LAMP3 expression, saliva flow was significantly decreased and serum anti-Ro/SSA and La/SSB antibodies could be detected in the treated mice. Mechanistically, LAMP3 expression increased apoptosis in SGECs and decreased protein expression related to saliva secretion. Analysis of RNAseq data suggested altered lysosomal function in the transduced SGECs, and that the cellular changes can chemoattract immune cells into the salivary glands. Immune cells were activated via toll-like receptors by damage-associated molecular patterns released from LAMP3-expressing SGECs.Conclusions: These results show a critical role for lysosomal trafficking in the development of SS and establish a causal relationship between LAMP3 misexpression and the development of SS. [ABSTRACT FROM AUTHOR]

Published
2021
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19. Rescue of Adeno-Associated Virus Production by shRNA Cotransfection.

Author

Guimaro, Maria C., Afione, Sandra A., Tanaka, Tsutomu, and Chiorini, John A.

Subjects
*ADENO-associated virus, *GENETIC vectors, *TRANSGENE expression, *GENE therapy, *VECTOR fields, *CELL physiology
Abstract

Adeno-associated virus (AAV) vector technology is rapidly advancing and becoming not only the leading vector platform in the field of gene therapy but also a useful tool for functional genomic studies of novel proteins. As most vectors utilize constitutive promoters, this results in transgene expression during production. Depending on the transgene product, this could induce proapoptotic, cytostatic, or other unknown effects that interfere with producer cell function and, therefore, reduce viral vector yield. This can be a major limitation when trying to characterize poorly described genes. We describe the novel use of shRNA encoding plasmids cotransfected during packaging to limit the expression of the cytotoxic transgene product. This allowed the production of an otherwise unpackageable vector. The approach is simple, versatile, does not require modification of the vector plasmid, and should be easily adaptable to almost any transgene with minimal cost. [ABSTRACT FROM AUTHOR]

Published
2020
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20. Aquaporin gene therapy corrects Sjögren's syndrome phenotype in mice.

Author

Zhennan Lai, Hongen Yin, Cabrera-Pérez, Javier, Guimaro, Maria C., Afione, Sandra, Michael, Drew G., Glenton, Patricia, Patel, Ankur, Swaim, William D., Changyu Zheng, Nguyen, Cuong Q., Nyberg, Fred, and Chiorini, John A.

Subjects
AQUAPORIN genetics, GENE therapy, SJOGREN'S syndrome, PHENOTYPES, LABORATORY mice
Abstract

Primary Sjögren's syndrome (pSS) is a chronic autoimmune disease that is estimated to affect 35 million people worldwide. Currently, no effective treatments exist for Sjögren's syndrome, and there is a limited understanding of the physiological mechanisms associated with xerostomia and hyposalivation. The present work revealed that aquaporin 5 expression, a water channel critical for salivary gland fluid secretion, is regulated by bone morphogenetic protein 6. Increased expression of this cytokine is strongly associated with the most common symptom of primary Sjögren's syndrome, the loss of salivary gland function. This finding led us to develop a therapy in the treatment of Sjögren's syndrome by increasing the water permeability of the gland to restore saliva flow. Our study demonstrates that the targeted increase of gland permeability not only resulted in the restoration of secretory gland function but also resolved the hallmark salivary gland inflammation and systemic inflammation associated with disease. Secretory function also increased in the lacrimal gland, suggesting this local therapy could treat the systemic symptoms associated with primary Sjögren's syndrome. [ABSTRACT FROM AUTHOR]

Published
2016
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21. Identification and Mutagenesis of the Adeno-Associated Virus 5 Sialic Acid Binding Region.

Author

Afione, Sandra, DiMattia, Michael A., Halder, Sujata, Pasquale, Giovanni Di, Agbandje-McKenna, Mavis, and Chiorini, John A.

Subjects
*CARBOHYDRATES, *SIALIC acids, *CARBOXYLIC acids, *GLYCANS, *CRYSTALLOGRAPHY
Abstract

As a genus, the dependoviruses use a diverse group of cell surface carbohydrates for attachment and entry. Despite the fact that a majority of adeno-associated viruses (AAVs) utilize sialic acid (SIA) for binding and transduction, this virus-carbohydrate interaction is poorly understood. Utilizing X-ray crystallography, two SIA binding regions were mapped for AAV5. The first site mapped to the depression in the center of the 3-fold axis of symmetry, while the second site was located under the βHI loop close to the 5-fold axis. Mutagenesis of amino acids 569 and 585 or 587 within the 3-fold depression resulted in elimination or alteration in SIA-dependent transduction, respectively. This change in SIA binding was confirmed using glycan microarrays. Mutagenesis of the second site identified a role in transduction that was SIA independent. Further studies of the mutants at the 3-fold site demonstrated a change in transduction activity and cell tropism in vivo as well as resistance to neutralization by a polyclonal antibody raised against the wild-type virus. Despite the fact that a majority of AAVs utilize sialic acid for binding and transduction, this virus-carbohydrate interaction is poorly understood. Utilizing X-ray crystallography, the sialic acid binding regions of AAV5 were identified and studied using a variety of approaches. Mutagenesis of this region resulted in elimination or alteration in sialic acid-dependent transduction in cell lines. This change in sialic acid glycan binding was confirmed using glycan arrays. Further study also demonstrated a change in transduction and activity and cell tropism in vivo as well as resistance to neutralization by antibodies raised against the wild-type virus. [ABSTRACT FROM AUTHOR]

Published
2015
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22. Long-term transduction of miniature pig parotid glands using serotype 2 adeno-associated viral vectors.

Author

Hai, Bo, Yan, Xing, Voutetakis, Antonis, Zheng, Changyu, Cotrim, Ana P., Shan, Zhaochen, Ding, Gang, Zhang, Chunmei, Xu, Junji, Goldsmith, Corinne M., Afione, Sandra, Chiorini, John A., Baum, Bruce J., and Wang, Songlin

Abstract

Background Previously, using an adenoviral vector, we showed that miniature pigs could provide a valuable and affordable large animal model for pre-clinical gene therapy studies to correct parotid gland radiation damage. However, adenoviral vectors lead to short-term transgene expression and, ideally, a more stable correction is required. In the present study, we examined the suitability of using a serotype 2 adeno-associated viral (AAV2) vector to mediate more stable gene transfer in the parotid glands of these animals. Methods Heparan sulfate proteoglycan was detected by immunohistochemistry. β-galactosidase expression was determined histochemically. An AAV2 vector encoding human erythropoietin (hEpo) was administered via Stensen's duct. Salivary and serum hEpo levels were measured using an enzyme-linked immunosorbent assay. Serum chemistry and hematological analyses were performed and serum antibodies to hEpo were measured throughout the study. Vector distribution was determined by a quantitative polymerase chain reaction. Results Transgene expression was vector dose-dependent, with high levels of hEpo being detected for up to 32 weeks (i.e. the longest time studied). hEpo reached maximal levels during weeks 4-8, but declined to approximately 25% of these values by week 32. Haematocrits were elevated from week 2. Transduced animals exhibited low serum anti-hEpo antibodies (1 : 8-1 : 16). Vector biodistribution at animal sacrifice revealed that most copies were in the targeted parotid gland, with few being detected elsewhere. No consistent adverse changes in serum chemistry or hematology parameters were seen. Conclusions AAV2 vectors mediate extended gene transfer to miniature pig parotid glands and should be useful for testing pre-clinical gene therapy strategies aiming to correct salivary gland radiation damage. Copyright © 2009 John Wiley & Sons, Ltd. [ABSTRACT FROM AUTHOR]

Published
2009
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26. Structural and antigenic characterization of the avian adenoassociated virus capsid.

Author

Hsi, Jane, Mietzsch, Mario, Chipman, Paul, Afione, Sandra, Zeher, Allison, Huang, Rick, Chiorini, John, and McKenna, Robert

Subjects
*VIRUS inactivation, *GENE therapy, *ADENO-associated virus, *MONOCLONAL antibodies, *TREATMENT effectiveness, *CAPSIDS, *ADENOVIRUSES
Abstract

All adeno-associated virus (AAV) vectors currently used in clinical trials or approved gene therapy biologics are based on human or non-human primate AAVs. A major challenge for AAV gene therapy is the high prevalence of circulating neutralizing antibodies (NAbs) in the general population targeting the virus capsids leading to vector inactivation and a loss of treatment efficacy. A strategy to escape detection by NAbs is the utilization of AAVs that do not disseminate in the primate population and exhibit low or no antigenicity. One such example is avian AAV (AAAV), which was first identified in preparations of the Olson strain of quail bronchitis, an avian adenovirus. AAAV shows very low sequence identities (~54–58%) to the AAV serotypes including to the sequences of the structurally diverse AAV4 and AAV5. In this study, the structure of empty and genome-filled AAAV capsids was determined by cryo-electron microscopy (cryo-EM) at 2.5 and 3.1 Å resolution. Furthermore, AAAV was found to utilize galactose for cell attachment, similar to AAV9 and AAVrh.10. Characterization of AAAV’s antigenic properties revealed that 30% of human sera from healthy individuals were capable of neutralizing transduction. This high rate of antigenicity is caused by conserved epitopes around the fivefold channel of the capsid allowing cross-reactivity of NAbs. This was further confirmed by mapping a cross-reactive human anti-AAV9 monoclonal antibody using cryo-EM. This structure-function characterization will be beneficial to further expand the current repertoire of AAV vectors in human gene therapy applications. IMPORTANCE AAVs are extensively studied as promising therapeutic gene delivery vectors. In order to circumvent pre-existing antibodies targeting primate-based AAV capsids, the AAAV capsid was evaluated as an alternative to primate-based therapeutic vectors. Despite the high sequence diversity, the AAAV capsid was found to bind to a common glycan receptor, terminal galactose, which is also utilized by other AAVs already being utilized in gene therapy trials. However, contrary to the initial hypothesis, AAAV was recognized by approximately 30% of human sera tested. Structural and sequence comparisons point to conserved epitopes in the fivefold region of the capsid as the reason determinant for the observed cross-reactivity. [ABSTRACT FROM AUTHOR]

Published
2023
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27. Lysosomal exocytosis of HSP70 stimulates monocytic BMP6 expression in Sjögren's syndrome.

Author

Ying-Qian Mo, Hiroyuki Nakamura, Tsutomu Tanaka, Toshio Odani, Perez, Paola, Youngmi Ji, French, Benjamin N., Pranzatelli, Thomas J. F., Michael, Drew G., Hongen Yin, Chow, Susan S., Khalaj, Maryam, Afione, Sandra A., Changyu Zheng, Oliveira, Fabiola Reis, Motta, Ana Carolina F., Ribeiro-Silva, Alfredo, Rocha, Eduardo M., Nguyen, Cuong Q., and Masayuki Noguchi

Subjects
*SJOGREN'S syndrome, *EXOCYTOSIS, *SALIVARY glands, *MEMBRANE proteins, *EPITHELIAL cells, *PROTEINS, *CYTOKINES, *RESEARCH, *LYSOSOMES, *ANIMAL experimentation, *RESEARCH methodology, *CELL physiology, *CELL receptors, *BONE morphogenetic proteins, *RNA, *EVALUATION research, *COMPARATIVE studies, *MICE
Abstract

BMP6 is a central cytokine in the induction of Sjögren's syndrome-associated (SS-associated) secretory hypofunction. However, the upstream initiation leading to the production of this cytokine in SS is unknown. In this study, RNA ISH on salivary gland sections taken from patients with SS indicated monocytic lineage cells as a cellular source of BMP6. RNA-Seq data on human salivary glands suggested that TLR4 signaling was an upstream regulator of BMP6, which was confirmed by in vitro cell assays and single-cell transcriptomics of human PBMCs. Further investigation showed that HSP70 was an endogenous natural TLR4 ligand that stimulated BMP6 expression in SS. Release of HSP70 from epithelial cells could be triggered by overexpression of lysosome-associated membrane protein 3 (LAMP3), a protein also associated with SS in several transcriptome studies. In vitro studies supported the idea that HSP70 was released as a result of lysosomal exocytosis initiated by LAMP3 expression, and reverse transcription PCR on RNA from minor salivary glands of patients with SS confirmed a positive correlation between BMP6 and LAMP3 expression. BMP6 expression could be experimentally induced in mice by overexpression of LAMP3, which developed an SS-like phenotype. The newly identified LAMP3/HSP70/BMP6 axis provided an etiological model for SS gland dysfunction and autoimmunity. [ABSTRACT FROM AUTHOR]

Published
2022
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29. Adeno-Associated Virus Serotype 1 (AAV1)- and AAV5-Antibody Complex Structures Reveal Evolutionary Commonalities in Parvovirus Antigenic Reactivity.

Author

Yu-Shan Tseng, Gurda, Brittney L., Chipman, Paul, McKenna, Robert, Afione, Sandra, Chiorini, John A., Muzyczka, Nicholas, Olson, Norman H., Baker, Timothy S., Kleinschmidt, Jürgen, and Agbandje-McKenna, Mavis

Subjects
*ADENO-associated virus, *LIPOPROTEIN lipase, *EPITOPES, *SEROTYPES, *PHENOTYPES
Abstract

The clinical utility of the adeno-associated virus (AAV) gene delivery system has been validated by the regulatory approval of an AAV serotype 1 (AAV1) vector for the treatment of lipoprotein lipase deficiency. However, neutralization from preexisting antibodies is detrimental to AAV transduction efficiency. Hence, mapping of AAV antigenic sites and engineering of neutralization-escaping vectors are important for improving clinical efficacy. Wereport the structures of four AAV-monoclonal antibody fragment complexes, AAV1-ADK1a, AAV1-ADK1b, AAV5-ADK5a, and AAV5-ADK5b, determined by cryo-electron microscopy and image reconstruction to a resolution of ~11 to 12 Å. Pseudoatomic modeling mapped the ADK1a epitope to the protrusions surrounding the icosahedral 3-fold axis and the ADK1b and ADK5a epitopes, which overlap, to the wall between depressions at the 2- and 5-fold axes (2/5-fold wall), and the ADK5b epitope spans both the 5-fold axis-facing wall of the 3-fold protrusion and portions of the 2/5-fold wall of the capsid. Combined with the six antigenic sites previously elucidated for different AAV serotypes through structural approaches, including AAV1 and AAV5, this study identified two common AAV epitopes: one on the 3-fold protrusions and one on the 2/5-fold wall. These epitopes coincide with regions with the highest sequence and structure diversity between AAV serotypes and correspond to regions determining receptor recognition and transduction phenotypes. Significantly, these locations overlap the two dominant epitopes reported for autonomous parvoviruses. Thus, rather than the amino acid sequence alone, the antigenic sites of parvoviruses appear to be dictated by structural features evolved to enable specific infectious functions. The adeno-associated viruses (AAVs) are promising vectors for in vivo therapeutic gene delivery, with more than 20 years of intense research now realized in a number of successful human clinical trials that report therapeutic efficacy. However, a large percentage of the population has preexisting AAV capsid antibodies and therefore must be excluded from clinical trials or vector readministration. This report represents our continuing efforts to understand the antigenic structure of the AAVs, specifically, to obtain a picture of "polyclonal" reactivity as is the situation in humans. It describes the structures of four AAV-antibody complexes determined by cryo-electron microscopy and image reconstruction, increasing the number of mapped epitopes to four and three, respectively, for AAV1 and AAV5, two vectors currently in clinical trials. The results presented provide information essential for generating antigenic escape vectors to overcome a critical challenge remaining in the optimization of this highly promising vector delivery system. [ABSTRACT FROM AUTHOR]

Published
2015
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30. Molecular Characterization of the Heparin-Dependent Transduction Domain on the Capsid of a Novel Adeno-Associated Virus Isolate, AAV(VR-942).

Author

Schmidt, Michael, Govindasamy, Lakshmanan, Afione, Sandra, Kaludov, Nick, Agbandje-McKenna, Mavis, and Chiorini, John A.

Subjects
*ADENOVIRUS diseases, *ADENOVIRUSES, *SIMIAN viruses, *HEPARIN, *VIRUSES
Abstract

A new adeno-associated virus (AAV), referred to as AAV(VR-942), has been isolated as a contaminant of adenovirus strain simian virus 17. The sequence of the rep gene places it in the AAV serotype 2 (AAV2) complementation group, while the capsid is only 88% identical to that of AAV2. High-level AAV(VR-942) transduction activity requires cell surface heparan sulfate proteoglycans, although AAV(VR-942) lacks residues equivalent to the AAV2 R585 and R588 amino acid residues essential for mediating the interaction of AAV2 with the heparan sulfate proteoglycan receptor. Instead, AAV(VR-942) uses a distinct transduction region. This finding shows that distinct domains on different AAV isolates can be responsible for the same activities. [ABSTRACT FROM AUTHOR]

Published
2008
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31. Adeno-Associated Virus Type 12 (AAV12): a Novel AAV Serotype with Sialic Acid- and Heparan Sulfate Proteoglycan-Independent Transduction Activity.

Author

Schmidt, Michael, Voutetakis, Antonis, Afione, Sandra, Changyu Zheng, Mandikian, Danielle, and Chiorini, John A.

Subjects
*RECOMBINANT viruses, *GENE therapy, *IMMUNE response, *PROTEOGLYCANS, *SERUM, *SALIVARY glands, *GENETIC transformation
Abstract

Recombinant adeno-associated virus (rAAV) is a promising vector for gene therapy. Recent isolations of novel AAV serotypes have led to significant advances by broadening the tropism and increasing the efficiency of gene transfer to the desired target cell. However, a major concern that remains is the strong preexisting immune responses to several vectors. In this paper, we describe the isolation and characterization of AAV12, an AAV serotype with unique biological and immunological properties. In contrast to those of all other reported AAVs, AAV12 cell attachment and transduction do not require cell surface sialic acids or heparan sulfate proteoglycans. Furthermore, rAAV12 is resistant to neutralization by circulating antibodies from human serum. The feasibility of rAAV12 as a vector was demonstrated in a mouse model in which muscle and salivary glands were transduced. These characteristics make rAAV12 an interesting candidate for gene transfer applications. [ABSTRACT FROM AUTHOR]

Published
2008
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32. 745. AAV12, Isolated from Vervet Monkey, Has Unique Tropism and Biological as Well as Neutralization Properties.

Author

Schmidt, Michael, Voutetakis, Antonis, Afione, Sandra, Changyu Zheng, and Chiorini, John A.

Subjects
*GENETIC transduction, *MICROBIAL genetics, *CERCOPITHECUS aethiops, *CANCER genetics, *CANCER treatment, *GENETIC engineering
Abstract

As part of an ongoing study to identify and characterize novel AAV isolates, we have screened virus isolates stored at the American Type Culture Collection. In a sample of adenovirus isolated from Vervet monkey (Cercopithecus aethiops) we have identified a new AAV with limited sequence homology to known AAVs and termed it AAV12. The capsid protein of AAV12 demonstrated highest homology with AAV11 and AAV4, 84% and 78% respectively, whereas AAV5 VP1 displayed lowest similarity with 53%. The Rep78 amino acid sequence of AAV12 is 89% identical to AAV4 and AAV11.To initially characterize AAV12, we analyzed the cellular elements that mediate transduction of recombinant virus. All AAVs characterized so far utilize either the glycosaminoglycan (GAG) heparan sulfate or sialic acid as receptor or attachment factor. Competition experiments with GAGs as well as the enzymatic removal of cell surface sialic acid demonstrated that AAV12 does not utilized GAGs or sialic acid as receptor. Involvement of glycolipids in the transduction process was excluded by studies utilizing inhibitors of glycolipid synthesis, whereas inhibition of transduction was observed after proteolytic digest of the cell prior to infection, suggesting that the AAV12 receptor is a protein. To analyze, if the AAV12 receptor complex includes a carbohydrate component, we screened a panel of mono- and oligosaccharides for their potential to compete with AAV12 transduction. Mannose and mannosamine inhibited AAV12 transduction, suggesting that these carbohydrates are part of the AAV12 receptor.The unique virus-cell interaction suggests a unique tropism of AAV12. This was confirmed by transduction experiments with recombinant virus in a broad panel of human cancer cell lines. The utility of AAV12 to mediate gene transfer was analyzed in mouse studies, where rAAV12 mediated gene transfer to salivary glands comparable with rAAV2.A potential limitation of utilizing AAV vectors in clinical studies is a strong pre-existing immunity to AAV in many patients. We therefore assayed A AV12 for neutralization by human immunoglobulin G (IgG) with a pool of intravenous immune globulin from 5000 human subjects (IVIG). rAAV12 was 100 times more resistant in an in vitro assay to neutralization by IVIG than either rAAV2 or rAVV6.The unique biological properties of AAV12, including its low neutralization by human IgGs, suggest that rAAV12 might be utilized as vector for gene therapy applications.Molecular Therapy (2006) 13, S288–S288; doi: 10.1016/j.ymthe.2006.08.827 [ABSTRACT FROM AUTHOR]

Published
2006
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33. 1122. Transgenic Vasoactive Intestinal Peptide Shows Local Disease Modifying Effects in a Murine Model of Sjögren's Syndrome

Author

Lodde, Beatrijs M., Mineshiba, Fumi, Wang, Jianghua, Cotrim, Ana P., Afione, Sandra, Tak, Paul P., and Baum, Bruce J.

Subjects
*PEPTIDES, *SJOGREN'S syndrome
Abstract

An abstract of the article "Transgenic Vasoactive Intestinal Peptide Shows Local Disease Modifying Effects in a Murine Model of Sjögren's Syndrome," by Beatrijs M. Lodde and colleagues is presented.

Published
2005
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34. Lysosome-associated membrane protein 3 misexpression in salivary glands induces a Sjögren's syndrome-like phenotype in mice.

Author

Nakamura H, Tanaka T, Pranzatelli T, Ji Y, Yin H, Perez P, Afione SA, Jang SI, Goldsmith C, Zheng CY, Swaim WD, Warner BM, Hirata N, Noguchi M, Atsumi T, and Chiorini JA

Subjects
Animals, Humans, Lysosomal Membrane Proteins genetics, Lysosomal Membrane Proteins metabolism, Mice, Phenotype, Salivary Glands, Sialadenitis pathology, Sjogren's Syndrome
Abstract

Objectives: Sjögren's syndrome (SS) is an autoimmune sialadenitis with unknown aetiology. Although extensive research implicated an abnormal immune response associated with lymphocytes, an initiating event mediated by salivary gland epithelial cell (SGEC) abnormalities causing activation is poorly characterised. Transcriptome studies have suggested alternations in lysosomal function are associated with SS, but a cause and effect linkage has not been established. In this study, we demonstrated that altered lysosome activity in SGECs by expression of lysosome-associated membrane protein 3 (LAMP3) can initiate an autoimmune response with autoantibody production and salivary dysfunction similar to SS., Methods: Retroductal cannulation of the submandibular salivary glands with an adeno-associated virus serotype 2 vector encoding LAMP3 was used to establish a model system. Pilocarpine-stimulated salivary flow and the presence of autoantibodies were assessed at several time points post-cannulation. Salivary glands from the mice were evaluated using RNAseq and histologically., Results: Following LAMP3 expression, saliva flow was significantly decreased and serum anti-Ro/SSA and La/SSB antibodies could be detected in the treated mice. Mechanistically, LAMP3 expression increased apoptosis in SGECs and decreased protein expression related to saliva secretion. Analysis of RNAseq data suggested altered lysosomal function in the transduced SGECs, and that the cellular changes can chemoattract immune cells into the salivary glands. Immune cells were activated via toll-like receptors by damage-associated molecular patterns released from LAMP3-expressing SGECs., Conclusions: These results show a critical role for lysosomal trafficking in the development of SS and establish a causal relationship between LAMP3 misexpression and the development of SS., Competing Interests: Competing interests: None declared., (© Author(s) (or their employer(s)) 2021. Re-use permitted under CC BY. Published by BMJ.)

Published
2021
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35. Gene-edited pseudogene resurrection corrects p47 phox -deficient chronic granulomatous disease.

Author

Merling RK, Kuhns DB, Sweeney CL, Wu X, Burkett S, Chu J, Lee J, Koontz S, Di Pasquale G, Afione SA, Chiorini JA, Kang EM, Choi U, De Ravin SS, and Malech HL

Abstract

Pseudogenes are duplicated genes with mutations rendering them nonfunctional. For single-gene disorders with homologous pseudogenes, the pseudogene might be a target for genetic correction. Autosomal-recessive p47 phox -deficient chronic granulomatous disease (p47-CGD) is a life-threatening immune deficiency caused by mutations in NCF1 , a gene with 2 pseudogenes, NCF1B and NCF1C . The most common NCF1 mutation, a GT deletion (ΔGT) at the start of exon 2 (>90% of alleles), is constitutive to NCF1B and NCF1C . NCF1 ΔGT results in premature termination, undetectable protein expression, and defective production of antimicrobial superoxide in neutrophils. We examined strategies for p47-CGD gene correction using engineered zinc-finger nucleases targeting the exon 2 ΔGT in induced pluripotent stem cells or CD34 + hematopoietic stem cells derived from p47-CGD patients. Correction of ΔGT in NCF1 pseudogenes restores oxidase function in p47-CGD, providing the first demonstration that targeted restoration of pseudogene function can correct a monogenic disorder., Competing Interests: Conflict-of-interest disclosure: The authors declare no competing financial interests.

Published
2016
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36. Hepatitis Delta Virus Detected in Salivary Glands of Sjögren's Syndrome Patients and Recapitulates a Sjögren's Syndrome-Like Phenotype in Vivo .

Author

Weller ML, Gardener MR, Bogus ZC, Smith MA, Astorri E, Michael DG, Michael DA, Zheng C, Burbelo PD, Lai Z, Wilson PA, Swaim W, Handelman B, Afione SA, Bombardieri M, and Chiorini JA

Abstract

Background: Low-level, chronic viral infections have been suspect in the development of select autoimmune diseases, including primary Sjögren's syndrome (pSS). Multiple studies have shown stimulation of antiviral response pathways in pSS tissues suggestive of a viral infection. Yet, with this data in hand, a causal link between a viral infection and development of pSS had not been identified. Therefore, a study was designed to further define the viral landscape within pSS-affected salivary gland tissue to identify potential viral-mediated triggers in the pathogenesis of this autoimmune disease., Methods: A viral microarray was utilized to measure viral transcripts present in salivary gland tissue from patients diagnosed with pSS compared to healthy controls. Murine models of salivary gland localized HDV antigen expression were developed to evaluate the capacity of a chronic HDV signature to trigger the development of a pSS-like phenotype., Results: Through this analysis, two distinct viral profiles were identified, including the increased presence of hepatitis delta virus (HDV) in 50% of pSS patients evaluated. Presence of HDV antigen and sequence were confirmed in minor salivary gland tissue. Patients with elevated HDV levels in salivary gland tissue were negative for detectible hepatitis B virus (HBV) surface antigen and antibodies to HBV or HDV. Expression of HDV antigens in vivo resulted in reduced stimulated saliva flow, increase in focal lymphocytic infiltrates, and development of autoantibodies., Conclusion: Identification of HDV in pSS patients and induction of a complete pSS-like phenotype in vivo provides further support of a viral-mediated etiopathology in the development of pSS.

Published
2016
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37. Transposase-mediated construction of an integrated adeno-associated virus type 5 helper plasmid.

Author

Smith RH, Afione SA, and Kotin RM

Subjects
Animals, Cells, Cultured, Cloning, Molecular, Haplorhini, Humans, Kidney embryology, Kidney immunology, Models, Genetic, Dependovirus genetics, Gene Transfer Techniques, Plasmids genetics, Recombination, Genetic, Transposases genetics, Virus Replication genetics
Abstract

Adeno-associated viruses (AAVs) are replication-defective parvoviruses that require helper virusfunctionsfor efficient productive replication. The AAVs are currently premier candidates as vectors for human gene therapy applications. In particular; much recent interest has been expressed concerning recombinant AAV serotype 5 (rAAV-5) vectors, as they appear to utilize cellular receptors distinctfrom those of the prototypical AAV serotype (AAV-2) and have been reported to have transduction properties in vivo that differ significantly from those of the prototype. One of the most popular current methodsfor the production of rAAVs involves co-transfection of human 293 cells with three plasmids: (i) an adenovirus (Ad)-derived helper plasmid containing Ad genes required for AAV replication, (ii) an AAV-derived plasmid encoding complementing AAV genes (ie., the viral rep and cap genes), and (iii) a target plasmid containing a transgene of interestflanked by AAV inverted terminal repeats (ITRs) that confer packaging and replication capabilities upon the ITR-flanked heterologous DNA. Here we describe novel plasmid reagents designed for convenient and efficient production of rAAV-S. An integrated helper plasmid containing all Ad genes requiredfor the efficient production of recombinant AAV as well as the complementing AAV genes on the same plasmid backbone, was constructed via transposase-mediated insertion into an Ad helper plasmid of a transposable element containing the AAV-5 rep and cap genes linked to a selectable marker This simple strategy can be used in the rapid and efficient construction of integrated helper plasmids derived from any reported AAV serotype for which a molecular clone exists.

Published
2002
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