Targeting transgene to the heart and liver with AAV9 by different promoters

Summary Adeno‐associated virus (AAV) has become one of the most promising gene transfer tools for gene therapy. This work aims to evaluate tropism, gene transfer efficiency and safety of AAV9 vectors produced with recombinant baculovirus (rBac)‐based system. AAV9‐CMV‐GFP and AAV9‐CBA‐GFP were produc...

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Bibliographic Details
Published in:Clinical and experimental pharmacology & physiology 2015-10, Vol.42 (10), p.1108-1117
Main Authors: Chen, Bang-Dang, He, Chun-Hui, Chen, Xiao-Cui, Pan, Shuo, Liu, Fen, Ma, Xiang, Li, Xiao-Mei, Gai, Min-Tao, Tao, Jing, Ma, Yi-Tong, Yang, Yi-Ning, Gao, Xiao-Ming
Format: Article
Language:English
Subjects:
AAV9
Actins - genetics
Adeno-associated virus
Animals
Apoptosis - genetics
Baculovirus
CBA promoter
Chickens - genetics
CMV promoter
Cytomegalovirus
Cytomegalovirus - genetics
Dependovirus - genetics
Dependovirus - physiology
Genetic Vectors - genetics
heart
Hepatocytes - cytology
Hepatocytes - metabolism
Hepatocytes - virology
liver
Male
Mice
Mice, Inbred C57BL
Myocytes, Cardiac - cytology
Myocytes, Cardiac - metabolism
Myocytes, Cardiac - virology
Promoter Regions, Genetic - genetics
rBac-based system
Safety
Transduction, Genetic - methods
Transgenes - genetics
Viral Tropism
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Summary:Summary Adeno‐associated virus (AAV) has become one of the most promising gene transfer tools for gene therapy. This work aims to evaluate tropism, gene transfer efficiency and safety of AAV9 vectors produced with recombinant baculovirus (rBac)‐based system. AAV9‐CMV‐GFP and AAV9‐CBA‐GFP were produced using a rBac system, 1 × 1011 particles of each vectors were administered intravenously (i.v.) into mice and animals were killed at 1, 2, 3, 4, 5 and 8 weeks after administration. The GFP expression in different organs was analyzed by fluorescence imaging and Western blot. Viral genomic quantities were measured using qPCR. In vitro transduction efficiency of AAV9 vectors in primary cardiomyocytes and hepatocytes was determined by flow cytometry. Toxicity of AAV9 vectors was evaluated by determining certain cardiac and liver injury biomarkers and renal function test in vivo and TUNEL analysis in vitro. The data showed that AAV9 viral particles packaged by the rBac system were fully functional in vivo and in vitro. The CMV promoter predominantly induced higher cardiac GFP transgene expression and DNA copy numbers while the CBA promoter resulted in robust GFP expression and high vector DNA copy numbers in mouse liver, both in a time‐dependent increased manner. Such distinct preferential effects were also observed in the heart and liver as early as 3 and 5 days after co‐infection. Both the AAV9‐CMV and AAV9‐CBA viral packages did not induce heart, liver and renal damage and cell apoptosis. These results indicated that AAV9‐CMV can efficiently and safely direct cardiac gene transfer, whereas AAV9‐CBA is preferential for liver gene delivery.
ISSN:0305-1870
1440-1681
DOI:10.1111/1440-1681.12453