Chromosomal Integration Pattern of a Helper-Dependent Minimal Adenovirus Vector with a Selectable Marker Inserted into a 27.4-Kilobase Genomic Stuffer

Author:

Hillgenberg Moritz12,Tönnies Holger3,Strauss Michael2

Affiliation:

1. DeveloGen AG, D-13125 Berlin-Buch,1

2. Humboldt-Universität zu Berlin, AG Molekulare Zellbiologie, D-13122 Berlin-Buch,2 and

3. Humboldt-Universität zu Berlin, Medizinische Fakultät, Institut für Humangenetik, Molekulare Zytogenetik, Campus Virchow-Klinikum, D-13353 Berlin,3 Germany

Abstract

ABSTRACT Helper-dependent minimal adenovirus vectors are promising tools for gene transfer and therapy because of their high capacity and the absence of immunostimulatory or cytotoxic viral genes. In order to characterize this new vector system with respect to its integrative properties, the integration pattern of a minimal adenovirus vector with a neo r gene inserted centrally into a noncoding 27.4-kb genomic stuffer element derived from the human X chromosome after infection of a sex chromosome aneuploid (X0) human glioblastoma cell line was studied. Our results indicate that even extensive homologies and abundant chromosomal repeat elements present in the vector did not lead to integration of the vector via homologous or homology-mediated mechanisms. Instead, integration occurred primarily by insertion of a monomer with no or little loss of sequences at the vector ends, apparently at random sites, which is very similar to E1 deletion adenovirus vectors. It is therefore unlikely that the incorporation of stuffer elements derived from human genomic DNA, which were shown to allow long-term transgene expression in vivo in a number of studies, leads to an enhanced risk of insertional mutagenesis. Furthermore, our findings indicate that the potential of minimal adenovirus vectors as tools for targeted insertion and gene targeting is limited despite the possibility of incorporating long stretches of homologous sequences. However, we found an enhanced efficiency of stable neo r transduction of the minimal adenovirus vector compared to an E1 deletion adenovirus vector, possibly caused by the absence of potential growth-inhibitory viral genes. Complete integration of the vector and tolerance of the integrated vector sequences by the cell might indicate a potential use of these vectors as tools for stable transfer of (large) genes.

Publisher

American Society for Microbiology

Subject

Virology,Insect Science,Immunology,Microbiology

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2. A review of 65 years of human adenovirus seroprevalence;Expert Review of Vaccines;2019-05-27

3. Introduction to Gene and Stem-Cell Therapy;Molecular and Cellular Therapies for Motor Neuron Diseases;2017

4. Helper-Dependent Adenoviral Vectors for Gene Therapy of Inherited Diseases;Safety and Efficacy of Gene-Based Therapeutics for Inherited Disorders;2017

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