Longevity of rAAV vector and plasmid DNA in blood after intramuscular injection in nonhuman primates: implications for gene doping

Ni, Weiyi; Guiner, Caroline Le; Gernoux, Gwladys; Penaud-Budloo, Magalie; Moullier, Philippe; Snyder, Richard O.

doi:10.1038/gt.2011.19

Cited by 44 publications

(86 citation statements)

References 44 publications

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“…This relates to a very recent report demonstrating that intramuscularly injected conventional plasmid is rapidly eliminated (Ni et al 2011). Equally we noted that the signal for exogenous FAK was importantly reduced in transfected soleus muscle 7 days after transfection.…”

Section: Discussionmentioning

confidence: 99%

“…While the detection of genetic modiWcation has been shown for virus-mediated transfection of skeletal muscle with expression construct for the secreted hematopoietic factor erythropoietin (Beiter et al 2011;Ni et al 2011) it is unlikely that this transfection technology would be a method of choice. This is explained by various drawbacks including the induction of immune responses that reduce the success of repeated applications, the costs of production of GMO quality vectors and possibly fatal consequences due to the virulence of the approach (Raper et al 2003).…”

Section: Electronic Supplementary Materialsmentioning

confidence: 99%

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A polymerase chain reaction-based methodology to detect gene doping

Carter

Flueck

2011

Eur J Appl Physiol

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The non-therapeutic use of genes to enhance athletic performance (gene doping) is a novel threat to the World of Sports. Skeletal muscle is a prime target of gene therapy and we asked whether we can develop a test system to produce and detect gene doping. Towards this end, we introduced a plasmid (pCMV-FAK, 3.8 kb, 50 g) for constitutive expression of the chicken homologue for the regulator of muscle growth, focal adhesion kinase (FAK), via gene electro transfer in the anti-gravitational muscle, m. soleus, or gastrocnemius medialis of rats. Activation of hypertrophy signalling was monitored by assessing the ribosomal kinase p70S6K and muscle Wbre cross section. Detectability of the introduced plasmid was monitored with polymerase chain reaction in deoxyribonucleic acids (DNA) from transfected muscle and serum. Muscle transfection with pCMV-FAK elevated FAK expression 7-and 73-fold, respectively, and increased mean cross section by 52 and 16% in targeted muscle Wbres of soleus and gastrocnemius muscle 7 days after gene electro transfer. Concomitantly p70S6K content was increased in transfected soleus muscle (+110%). Detection of the exogenous plasmid sequence was possible in DNA and cDNA of muscle until 7 days after transfection, but not in serum except close to the site of plasmid deposition, 1 h after injection and surgery. The Wndings suggest that the reliable detection of gene doping in the immoral athlete is not possible unless a change in the current practice of tissue sampling is applied involving the collection of muscle biopsy close to the site of gene injection.

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Section: Discussionmentioning

confidence: 99%

Section: Electronic Supplementary Materialsmentioning

confidence: 99%

A polymerase chain reaction-based methodology to detect gene doping

Carter

Flueck

2011

Eur J Appl Physiol

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“…[29] Using the same approach, it was demonstrated that detecting doping transgene in blood of nonhuman primates was possible. [25] Indeed, intramuscular injection of a conventional plasmid and rAAV vectors resulted in the presence of DNA that could be detected at high levels in blood and that rAAV genomes can persist for several months in WBCs.…”

Section: Detection Of Gene Dopingmentioning

confidence: 99%

“…[25] However, due to its high invasiveness, muscle biopsy would be impossible for sample harvesting. Direct injection into a target tissue has been considered as an approach which leads to entry of minutes amounts of transgenic DNA into the blood stream.…”

Section: Detection Of Gene Dopingmentioning

confidence: 99%

“…[1] Various direct detection methods based on nested and real-time polymerase chain reaction (PCR) have been proposed for the detection of gene doping practices. [24][25][26][28][29][30] Those approaches are based on subtle differences between the sequences of a doping transgene and its endogenous counterpart in genomic DNA (gDNA). Indeed, the gene sequences of transgenic DNA (tDNA) do not contain intron sequence parts of the gDNA which allows the detection of trace amounts of a transgene in a large background of gDNA.…”

Section: Detection Of Gene Dopingmentioning

confidence: 99%

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Loop‐mediated isothermal amplification (LAMP) as an alternative to PCR: A rapid on‐site detection of gene doping

Salamin

Kuuranne

Saugy

et al. 2017

Drug Testing and Analysis

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Innovation in medical research has been diverted at multiple occasions to enhance human performance. The predicted great progress in gene therapy has raised some concerns regarding its misuse in the world of sports (gene doping) for several years now. Even though there is no evidence that gene doping has ever been used in sports, the continuous improvement of gene therapy techniques increases the likelihood of abuse. Therefore, since 2004, efforts have been invested by the anti-doping community and WADA for the development of detection methods. Several nested PCR and qPCR-based strategies exploiting the absence of introns in the transgenic DNA have been proposed for the long-term detection of transgene in blood. Despite their great sensitivity, those protocols are hampered by limitations of the techniques that can be cumbersome and costly. The purpose of this perspective is to describe a new approach based on loop-mediated isothermal amplification (LAMP) for the detection of gene doping. This protocol enables a rapid and simple method to amplify nucleic acids with a high sensitivity and specificity and with a simple visual detection of the results. LAMP is already being used in clinical application for the detection of viruses or mutations. Therefore, this technique has the potential to be further developed for the detection of foreign genetic material in elite athletes.

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Detection of EPO gene doping in blood

Neuberger

Jurkiewicz

Moser

et al. 2012

Drug Testing and Analysis

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Gene doping--or the abuse of gene therapy--will continue to threaten the sports world. History has shown that progress in medical research is likely to be abused in order to enhance human performance. In this review, we critically discuss the progress and the risks associated with the field of erythropoietin (EPO) gene therapy and its applicability to EPO gene doping. We present typical vector systems that are employed in ex vivo and in vivo gene therapy trials. Due to associated risks, gene doping is not a feasible alternative to conventional EPO or blood doping at this time. Nevertheless, it is well described that about half of the elite athlete population is in principle willing to risk its health to gain a competitive advantage. This includes the use of technologies that lack safety approval. Sophisticated detection approaches are a prerequisite for prevention of unapproved and uncontrolled use of gene therapy technology. In this review, we present current detection approaches for EPO gene doping, with a focus on blood-based direct and indirect approaches. Gene doping is detectable in principle, and recent DNA-based detection strategies enable long-term detection of transgenic DNA (tDNA) following in vivo gene transfer.

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Longevity of rAAV vector and plasmid DNA in blood after intramuscular injection in nonhuman primates: implications for gene doping

Cited by 44 publications

References 44 publications

A polymerase chain reaction-based methodology to detect gene doping

A polymerase chain reaction-based methodology to detect gene doping

Loop‐mediated isothermal amplification (LAMP) as an alternative to PCR: A rapid on‐site detection of gene doping

Detection of EPO gene doping in blood

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