Literature DB >> 28072927

Artificial Induction of Native Aquaporin-1 Expression in Human Salivary Cells.

Z Wang1, S Pradhan-Bhatt2,3, M C Farach-Carson4, M J Passineau1.   

Abstract

Gene therapy for dry mouth disorders has transitioned in recent years from theoretical to clinical proof of principle with the publication of a first-in-man phase I/II dose escalation clinical trial in patients with radiation-induced xerostomia. This trial used a prototype adenoviral vector to express aquaporin-1 (AQP1), presumably in the ductal cell layer and/or in surviving acinar cells, to drive transcellular flux of interstitial fluid into the labyrinth of the salivary duct. As the development of this promising gene therapy continues, safety considerations are a high priority, particularly those that remove nonhuman agents (i.e., viral vectors and genetic sequences of bacterial origin). In this study, we applied 2 emerging technologies, artificial transcriptional complexes and epigenetic editing, to explore whether AQP1 expression could be achieved by activating the native gene locus in a human salivary ductal cell line and primary salivary human stem/progenitor cells (hS/PCs), as opposed to the conventional approach of cytomegalovirus promoter-driven expression from an episomal vector. In our first study, we used a cotransfection strategy to express the components of the dCas9-SAM system to create an artificial transcriptional complex at the AQP1 locus in A253 and hS/PCs. We found that AQP1 expression was induced at a magnitude comparable to adenoviral infection, suggesting that AQP1 is primarily silenced through pretranscriptional mechanisms. Because earlier literature suggested that pretranscriptional silencing of AQP1 in salivary glands is mediated by methylation of the promoter, in our second study, we performed global, chemical demethylation of A253 cells and found that demethylation alone induced robust AQP1 expression. These results suggest the potential for success by inducing AQP1 expression in human salivary ductal cells through epigenetic editing of the native promoter.

Entities:  

Keywords:  epigenetic repression; genetic therapy; genetic vectors; progenitor cells; salivary glands; xerostomia

Mesh:

Substances:

Year:  2017        PMID: 28072927      PMCID: PMC5384490          DOI: 10.1177/0022034516685045

Source DB:  PubMed          Journal:  J Dent Res        ISSN: 0022-0345            Impact factor:   6.116


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Review 4.  Development of a gene transfer-based treatment for radiation-induced salivary hypofunction.

Authors:  Bruce J Baum; Changyu Zheng; Ilias Alevizos; Ana P Cotrim; Shuying Liu; Linda McCullagh; Corinne M Goldsmith; Nancy McDermott; John A Chiorini; Nikolay P Nikolov; Gabor G Illei
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Review 6.  Gene therapy returns to centre stage.

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9.  Repurposing the CRISPR-Cas9 system for targeted DNA methylation.

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10.  Induced DNA demethylation by targeting Ten-Eleven Translocation 2 to the human ICAM-1 promoter.

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2.  Inhibitory effect of AQP1 silencing on adhesion and angiogenesis in ectopic endometrial cells of mice with endometriosis through activating the Wnt signaling pathway.

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3.  CRISPR-Cas9 HDR system enhances AQP1 gene expression.

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4.  The expression of water channel proteins during human salivary gland development: a topographic study of aquaporins 1, 3 and 5.

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Review 5.  Radiation-Induced Salivary Gland Dysfunction: Mechanisms, Therapeutics and Future Directions.

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