Myocarditis following adeno-associated viral gene expression of human soluble TNF receptor (TNFRII-Fc) in baboon hearts

McTiernan, Charles F.; Mathier, Michael A.; Zhu, Xiaodong; Xiao, Xianmin; Klein, Ed; Swan, Christina H.; Mehdi, Haider; Gibson, Gregory A.; Trichel, Anita; Feldman, Arthur M.; McCurry, Kenneth R.; London, Barry

doi:10.1038/sj.gt.3303020

Cited by 36 publications

(24 citation statements)

References 32 publications

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“…2,[8][9][10] However, the systemic perturbation resulting from hydrodynamic injection remains a serious limitation for clinical application, as it can lead to circulatory collapse and even death. To avoid this adverse effect, we have described a retrograde cathetermediated gene delivery procedure 5 with the aim of locally reproducing the intrahepatic conditions mediated by tail vein hydrodynamic injection.…”

Section: Discussionmentioning

confidence: 99%

DNA delivery to ‘ex vivo’ human liver segments

et al. 2011

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Hydrodynamic injection is an efficient procedure for liver gene therapy in rodents but with limited efficacy in large animals, using an 'in vivo' adapted regional hydrodynamic gene delivery system. We study the ability of this procedure to mediate gene delivery in human liver segments obtained by surgical resection. Watertight liver segments were retrogradely injected from hepatic vein with a saline solution containing a plasmid bearing the enhanced green fluorescent protein (eGFP) gene, under different conditions of flow rate (1, 10 and 20 ml s -1 ) and final perfused volume. Samples were cultured for 1 to 2 days and used for microscopy and molecular analysis of gene expression. The fluorescent and immunohistochemistry studies indicated that in segments injected at X10 ml s -1 , good and wide gene expression was present in the liver sections and the molecular analysis reinforced the histological observation in a quantitative manner (index of apparent gene delivery: 10 2 -10 4 eGFP DNA copy per 100 pg of total DNA; transcription index: 10 5 -2Â10 6 eGFP RNA copy per 100 ng of total RNA). In addition, injected gold nanoparticles (15 nm diameter) suggested that DNA delivery to hepatocytes must involve a facilitated permeation process without membrane disruption. In summary, we show that retrograde venous injection of watertight human liver segment is an anadromous procedure that results in wide liver gene delivery and good gene expression. However, additional studies will be necessary to clarify the influence of the prolonged ischemia injury to hepatocytes in our model.

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Section: Discussionmentioning

confidence: 99%

DNA delivery to ‘ex vivo’ human liver segments

et al. 2011

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“…Studies using virus-mediated transfer of shRNA directed against PLB in cardiomyocyte culture have demonstrated that it is an effective method for both knocking down PLB expression and modulating calcium handling (Fechner et al, 2007;Andino et al, 2008), and one study in a rat model of HF demonstrated that AAV-mediated transfer of shRNA is effective in restoring cardiac function and geometry (Suckau et al, 2009). In addition, because the gene product in this case would be a functional RNA and not a mutant protein (dnPLB), this strategy would avoid the potential of evoking a T cell response directed against cells expressing the transgene, as has been reported after AAV-mediated cardiac gene transfer of a modified, soluble TNF receptor in baboons (McTiernan et al, 2007). This is an important consideration when considering large animal and clinical trials.…”

Section: Introductionmentioning

confidence: 99%

Cardiac Gene Transfer of Short Hairpin RNA Directed Against Phospholamban Effectively Knocks Down Gene Expression but Causes Cellular Toxicity in Canines

et al. 2011

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Derangements in calcium cycling have been described in failing hearts, and preclinical studies have suggested that therapies aimed at correcting this defect can lead to improvements in cardiac function and survival. One strategy to improve calcium cycling would be to inhibit phospholamban (PLB), the negative regulator of SERCA2a that is upregulated in failing hearts. The goal of this study was to evaluate the safety and efficacy of using adeno-associated virus (AAV)-mediated cardiac gene transfer of short hairpin RNA (shRNA) to knock down expression of PLB. Six dogs were treated with self-complementary AAV serotype 6 (scAAV6) expressing shRNA against PLB. Three control dogs were treated with empty AAV6 capsid, and two control dogs were treated with scAAV6 expressing dominant negative PLB. Vector was delivered via a percutaneously inserted cardiac injection catheter. PLB mRNA and protein expression were analyzed in three of six shRNA dogs between days 16 and 26. The other three shRNA dogs and five control dogs were monitored long-term to assess cardiac safety. PLB mRNA was reduced 16-fold, and PLB protein was reduced 5-fold, with treatment. Serum troponin elevation and depressed cardiac function were observed in the shRNA group only at 4 weeks. An enzyme-linked immunospot assay failed to detect any T cells reactive to AAV6 capsid in peripheral blood mononuclear cells, heart, or spleen. Microarray analysis revealed alterations in cardiac expression of several microRNAs with shRNA treatment. AAV6-mediated cardiac gene transfer of shRNA effectively knocks down PLB expression but is associated with severe cardiac toxicity. Toxicity may result from dysregulation of endogenous microRNA pathways.

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“…Intramyocardial delivery of human soluble tumor necrosis factor-a receptor II-Fc fusion protein was performed in intact non-human primates; however, it was associated with local myocarditis at the injection sites. 94 A unique approach is the gene delivery of neuronal nitric oxide synthase to cardiac vagus in pigs. 95 Because enhanced vagal function was observed after the gene delivery, additional positive data in a heart failure model may hold more promise.…”

Section: Other Gene Targetsmentioning

confidence: 99%