High Efficiency Restriction Enzyme–Free Linear Amplification-Mediated Polymerase Chain Reaction Approach for Tracking Lentiviral Integration Sites Does Not Abrogate Retrieval Bias

Wu, Chuanfeng; Jares, Alexander; Winkler, Thomas; Xie, Jianjun; Métais, Jean‐Yves; Dunbar, Cynthia E.

doi:10.1089/hum.2012.082

Cited by 23 publications

(21 citation statements)

References 29 publications

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“…These clones had normal and stable karyotypes, with G-banding repeated just prior to selected in vivo autologous implantation experiments. The genomic location of the 303 bp non-expressed proviral vector fragment remaining in the genome following the transgene-excision was mapped by a modified restriction enzyme-free linear amplification-mediated polymerase chain reaction (Re-free LAM-PCR) (Wu et al, 2013) in the RhiPSC clones to be used for autologous transplantation (Table S1). The presence of this inert DNA tag allowed unequivocal assessment of the presence or absence of RhiPSCs following in vivo implantation.…”

Section: Resultsmentioning

confidence: 99%

Path to the Clinic: Assessment of iPSC-Based Cell Therapies In Vivo in a Nonhuman Primate Model

Hong

Winkler

et al. 2014

Cell Reports

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Summary Induced pluripotent stem cell (iPSC)-based cell therapies have a great potential for regenerative medicine, but are also potentially associated with tumorigenic risks. Current rodent models are not the optimal predictors of efficiency and safety for clinical application. Therefore, we developed a clinically relevant non-human primate model to assess the tumorigenic potential and in vivo efficacy of both undifferentiated and differentiated iPSCs in the autologous settings without immunosuppression. Undifferentiated autologous iPSCs indeed formed mature teratomas in a dose-dependent manner. However, tumor formation was accompanied by an inflammatory reaction. On the other hand, iPSC-derived mesodermal stromal-like cells formed new bone in vivo without any evidence of teratoma formation. We therefore show for the first time in a large animal model that closely resembles human physiology that undifferentiated autologous iPSCs form teratomas, and that iPSC-derived progenitor cells can give rise to a functional tissue in vivo.

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Section: Resultsmentioning

confidence: 99%

Path to the Clinic: Assessment of iPSC-Based Cell Therapies In Vivo in a Nonhuman Primate Model

Hong

Winkler

et al. 2014

Cell Reports

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“…12 Due to the lower sensitivity of these methods, this analysis was only performed in mice with high numbers of gene modified cells in the BM. Here, 31 insertions in six mice were recovered by the re-free LAM PCR and 55 insertions in three mice by the nrLAM-PCR method ( Supplementary Table S3 ).…”

Section: Resultsmentioning

confidence: 99%

Clonal Dominance With Retroviral Vector Insertions Near the ANGPT1 and ANGPT2 Genes in a Human Xenotransplant Mouse Model

Haemmerle

Phaltane

Rothe

et al. 2014

Molecular Therapy - Nucleic Acids

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Insertional leukemogenesis represents the major risk factor of hematopoietic stem cell (HSC) based gene therapy utilizing integrating viral vectors. To develop a pre-clinical model for the evaluation of vector-related genotoxicity directly in the relevant human target cells, cord blood CD34+ HSCs were transplanted into immunodeficient NOD.SCID.IL2rg−/− (NSG) mice after transduction with an LTR-driven gammaretroviral vector (GV). Furthermore, we specifically investigated the effect of prolonged in vitro culture in the presence of cytokines recently described to promote HSC expansion or maintenance. Clonality of human hematopoiesis in NSG mice was assessed by high throughput insertion site analyses and validated by insertion site-specific PCR depicting a GV typical integration profile with insertion sites resembling to 25% those of clinical studies. No overrepresentation of integrations in the vicinity of cancer-related genes was observed, however, several dominant clones were identified including two clones harboring integrations in the ANGPT1 and near the ANGPT2 genes associated with deregulated ANGPT1- and ANGPT2-mRNA levels. While these data underscore the potential value of the NSG model, our studies also identified short-comings such as overall low numbers of engrafted HSCs, limited in vivo observation time, and the challenges of in-depth insertion site analyses by low contribution of gene modified hematopoiesis.

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“…(Kustikova et al, 2009b;Maetzig et al, 2011), we have established a method to analyze multiple samples in a single 454 pyrosequencing run, which allowed us to retrieve up to 2700 sequences per sample. The clonal repertoire reflected at this sequencing depth, however, is not exhaustive, partly because of the limitations imposed by the use of a given specific restriction enzyme (Harkey et al, 2007;Gabriel et al, 2009;Wu et al, 2013) and partly because of sampling issues. Moreover, the LM-PCR method can be skewed, as can any method that employs PCR amplification of intermediate products, toward amplification of smaller PCR products, among other limitations (Berry et al, 2012;Bystrykh et al, 2012), although we could not show that small amplicons had an effect on the extent to which the pyrosequencing reads correlate with the qPCR data ( Supplementary Fig.…”

Section: Typical Pcr Parameters Do Not Explain the Inconsistency Of Tmentioning

confidence: 99%

“…Newly developed techniques, such as nonrestrictive LAM-PCR (Gabriel et al, 2009), a phage Mu transposition-based method (Brady et al, 2011), shear-splink (Koudijs et al, 2011), and Re-free LAM-PCR (Wu et al, 2013), eliminate the restriction enzyme bias and may thus also temper PCRassociated bias related to GC content, secondary structure, and amplicon length. As an alternative to the vector mark, vectors might be supplied with DNA barcodes (Gerrits et al, 2010;Lu et al, 2011).…”

Section: Typical Pcr Parameters Do Not Explain the Inconsistency Of Tmentioning

confidence: 99%

Evaluating a Ligation-Mediated PCR and Pyrosequencing Method for the Detection of Clonal Contribution in Polyclonal Retrovirally Transduced Samples

Brugman

Suerth

Rothe

et al. 2013

Human Gene Therapy Methods

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Retroviral gene transfer has proven therapeutic potential in clinical gene therapy trials but may also cause abnormal cell growth via perturbation of gene expression in the locus surrounding the insertion site. By establishing clonal marks, retroviral insertions are also used to describe the regenerative potential of individual cells. Deep sequencing approaches have become the method of choice to study insertion profiles in preclinical models and clinical trials. We used a protocol combining ligation-mediated polymerase chain reaction (LM-PCR) and pyrosequencing for insertion profiling and quantification in cells of various tissues transduced with various retroviral vectors. The presented method allows simultaneous analysis of a multitude of DNA-barcoded samples per pyrosequencing run, thereby allowing cost-effective insertion screening in studies with multiple samples. In addition, we investigated whether the number of pyrosequencing reads can be used to quantify clonal abundance. By comparing pyrosequencing reads against site-specific quantitative PCR and by performing spike-in experiments, we show that considerable variation exists in the quantification of insertion sites even when present in the same clone. Our results suggest that the protocol used here and similar approaches might misinterpret abundance clones defined by insertion sites, unless careful calibration measures are taken. The crucial variables causing this variation need to be defined and methodological improvements are required to establish pyrosequencing reads as a quantification measure in polyclonal situations.

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High Efficiency Restriction Enzyme–Free Linear Amplification-Mediated Polymerase Chain Reaction Approach for Tracking Lentiviral Integration Sites Does Not Abrogate Retrieval Bias

Cited by 23 publications

References 29 publications

Path to the Clinic: Assessment of iPSC-Based Cell Therapies In Vivo in a Nonhuman Primate Model

Path to the Clinic: Assessment of iPSC-Based Cell Therapies In Vivo in a Nonhuman Primate Model

Clonal Dominance With Retroviral Vector Insertions Near the ANGPT1 and ANGPT2 Genes in a Human Xenotransplant Mouse Model

Evaluating a Ligation-Mediated PCR and Pyrosequencing Method for the Detection of Clonal Contribution in Polyclonal Retrovirally Transduced Samples

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