Adeno-associated virus 2-mediated gene transfer: role of a cellular serine/threonine protein phosphatase in augmenting transduction efficiency

Zhao, Weihong; Wu, Jie; Zhong, Li; Srivastava, Arun

doi:10.1038/sj.gt.3302886

Cited by 16 publications

(27 citation statements)

References 49 publications

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“…FKBP52 (F), phosphorylated at tyrosine residues (red symbol) and serine/threonine (yellow symbol), which strongly inhibits the second-strand DNA synthesis of a conventional ssAAV vector, is dephosphorylated at tyrosine residues by T-cell protein tyrosine phosphatase (TC-PTP; blue semi-oval), and at serine/threonine residues by protein phosphatase 5 (PP5; green semi-oval) expressed from scAAV-TC-PTP and scAAV-PP5 vectors, which allows more efficient viral second-strand DNA synthesis of conventional ssAAV vector, and consequently, leads to more efficient transgene expression. 12 Consistent with our hypothesis, we observed an additive effect in the increase in EGFP expression in HeLa, KB and 293 cells when both TC-PTP and PP5 expression plasmids were cotransfected (Figure 2b). In anticipation of extending these studies to an in vivo animal model, we next wished to deliver TC-PTP and PP5 genes via scAAV vectors.…”

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confidence: 90%

“…3,4 Thus, failure to undergo viral second-strand synthesis remains a predominant rate-limiting step in the observed low efficiency of singlestranded AAV (ssAAV) vector-mediated transgene expression both in vitro and in vivo. [5][6][7][8][9][10][11][12][13][14] The use of selfcomplementary AAV (scAAV) vectors that bypass the requirement for viral second-strand DNA synthesis can circumvent this problem. 13 However, their widespread use is limited by their limited packaging capacity (B3.3 kb), 15 which is significantly less than that of conventional ssAAV vectors (B6 kb).…”

mentioning

confidence: 99%

“…8,9,11,[17][18][19] We have also documented that FKBP52 is dephosphorylated at Tyr residues by the cellular T-cell protein tyrosine phosphatase (TC-PTP), and at Ser/Thr residues by protein phosphatase 5 (PP5). 9,12 Dephosphorylated FKBP52 can no longer bind to the Dsequence, which in turn, facilitates the viral secondstrand DNA synthesis, and augments the transgene expression from ssAAV2 vectors. We have demonstrated augmentation in ssAAV vector-mediated transgene expression in transgenic mice overexpressing TC-PTP, 9 and in mice deficient in FKBP52.…”

mentioning

confidence: 99%

“…However, the observed increases were only modest, approximately 5-to 6-fold. 11,12 In an attempt to further augment the transduction efficiency of ssAAV vectors, we reasoned that coinfection with AAV-TC-PTP and AAV-PP5 vectors together may exert, at the very least, an additive effect. As both TC-PTP and PP5 cDNA sizes (B2.5 kb) are within the packaging capacity of scAAV vectors 15 and AAV2 remains the best characterized serotype for gene transfer protocols, 20,21 we examined whether coinfection with scAAV2-TC-PTP+scAAV2-PP5 vectors might augment the transduction efficiency of conventional ssAAV2 vectors.…”

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confidence: 99%

“…The scAAV2 plasmids containing the RSV promoter-driven murine TC-PTP (scAAV2-TC-PTP) and the RSV promoter-driven human PP5 (scAAV2-PP5) were constructed by standard cloning methods as described previously. 11,12 Highly purified stocks of recombinant scAAV2-TC-PTP and scAAV2-PP5 vectors were generated by the triple-plasmid transfection protocol as described previously. 22 The physical particle titers of recombinant vector stocks were determined by quantitative DNA slot-blot analyses.…”

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confidence: 99%

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Strategies for improving the transduction efficiency of single-stranded adeno-associated virus vectors in vitro and in vivo

Jayandharan

Zhong

et al. 2008

Gene Ther

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Recombinant vectors based on adeno-associated virus type 2 (AAV) target the liver efficiently, but the transgene expression is limited to B5% of murine hepatocytes. Viral second-strand DNA synthesis continues to be a rate-limiting step for efficient transduction by the single-stranded AAV (ssAAV) vectors. This is due, in part, to the presence of a cellular chaperone (FK506-binding) protein, FKBP52, phosphorylated forms of which interact with the D-sequence in the inverted terminal repeats of AAV2 genome and inhibit the viral second-strand DNA synthesis. Our previous studies have documented that dephosphorylation of FKBP52 at tyrosine residues by the cellular T-cell protein tyrosine phosphatase (TC-PTP), and at serine/threonine residues by protein phosphatase 5 (PP5) enhances viral secondstrand DNA synthesis and consequently, the transgene expression. We have also reported that coinfection with a self-complementary AAV (scAAV)-TC-PTP vector results in up to sixfold increase in the transduction efficiency of conventional ssAAV2 vectors in primary murine hepatocytes in vivo. We reasoned that coinfection with scAAV-TC-PTP and scAAV-PP5 vectors may lead to a further increase in the transduction efficiency of ssAAV2 vectors. We demonstrate here that this strategy does indeed lead to B16-fold increase in the transduction efficiency of conventional ssAAV vectors in primary murine hepatocytes in vivo following tail-vein injections. Neither scAAV2-TC-PTP nor scAAV2-PP5 vectors alone or together had any adverse effect on the hepatocytes. Thus, this coinfection strategy may be useful for achieving expression from recombinant ssAAV2 vectors containing larger genes, such as coagulation factor VIII, which exceed the packaging capacity of scAAV vectors, for the potential gene therapy of hemophilia A.

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Strategies for improving the transduction efficiency of single-stranded adeno-associated virus vectors in vitro and in vivo

Jayandharan

Zhong

et al. 2008

Gene Ther

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Adeno‐associated Viral Vectors in Gene Therapy

Zhong

Srivastava

2007

Encyclopedia of Life Sciences

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Recombinant vectors based on a nonpathogenic human parvovirus, the Adeno‐associated virus 2 (AAV), have gained attention as a potentially safe and useful alternative to the more commonly used retroviral and adenoviral vectors. AAV vectors are currently in use in phase I/II clinical trials for gene therapy of a number of diseases such as cystic fibrosis, α‐1 antitrypsin deficiency, muscular dystrophy, Batten disease and Parkinson disease. Several salient features of AAV vectors and the availability of promising results with animal models of human diseases provide the impetus to suggest that they will be used in potential gene therapy of a number of human diseases, both genetic and acquired, in not too distant a future.

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Adeno‐associated virus‐mediated gene transfer

Srivastava

2008

J of Cellular Biochemistry

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Although the remarkable versatility and efficacy of recombinant adeno-associated virus 2 (AAV2) vectors in transducing a wide variety of cells and tissues in vitro, and in numerous pre-clinical animal models of human diseases in vivo, have been well established, the published literature is replete with controversies with regard to the efficacy of AAV2 vectors in hematopoietic stem cell (HSC) transduction. A number of factors have contributed to these controversies, the molecular bases of which have begun to come to light in recent years. With the availability of several novel serotypes (AAV1 through AAV12), rational design of AAV capsid mutants, and strategies (selfcomplementary vector genomes, hematopoietic cell-specific promoters), it is indeed becoming feasible to achieve efficient transduction of HSC by AAV vectors in a murine serial bone marrow transplantation model in vivo, where stable integration of the proviral AAV genome does not lead to any overt hematological abnormalities. Thus, a better understanding of the AAV-HSC interactions, and the availability of a vast repertoire of novel serotype vectors, are likely to have significant implications in the use of AAV vectors in high-efficiency transduction of HSCs as well as in gene therapy applications involving the hematopoietic system. KeywordsAdeno-associated virus; Viral vectors; Gene transfer; Gene expression; Hematopoietic stem cells Gene therapy with vectors based on retroviruses and adenoviruses has been attempted in a number of clinical trials [Edelstein et al., 2007]. Initially, retroviral vectors yielded encouraging results, but the development of T cell lymphoma in non-human primates, and more recently, the development of T-cell leukemia in three children in a clinical trial for gene therapy of X-linked severe-combined immunodeficiency with these vectors has raised serious safety concerns [Deichmann et al., 2007;Hacein-Bey-Abina et al., 2003;Kohn et al., 2003]. Similarly, questions were raised with reference to efficacy of adenoviral vectors in gene therapy of cystic fibrosis, and subsequently, the death of a patient in a clinical trial for gene therapy of was attributed to the use of first-generation adenoviral vectors [Raper et al., 2003].A third group of viruses, termed parvoviruses, have to date not been associated with any malignant disease. In fact, parvoviruses have been shown to possess anti-tumor properties [Asokan and Samulski, 2005;Li et al., 2005]. Parvoviruses are among the smallest of known viruses, which contain a single-stranded DNA genome, and infect all vertebrates. One parvovirus of human origin, the adeno-associated virus 2 (AAV2), has been studied [Berns and Bohenzky, 1987;Muzyczka et al., 1984]. Although ∼90% of the human population is sero-positive for AAV2, no known disease has thus far been associated with AAV2 infection. AAV2 requires co-infection with a helper-virus, such as adenovirus, for its optimal replication, but in the absence of a helper-virus, the AAV2 genome integrates site-specifically into the huma...

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Adeno-associated virus 2-mediated gene transfer: role of a cellular serine/threonine protein phosphatase in augmenting transduction efficiency

Cited by 16 publications

References 49 publications

Strategies for improving the transduction efficiency of single-stranded adeno-associated virus vectors in vitro and in vivo

Strategies for improving the transduction efficiency of single-stranded adeno-associated virus vectors in vitro and in vivo

Adeno‐associated Viral Vectors in Gene Therapy

Adeno‐associated virus‐mediated gene transfer

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