In vivo selection of hematopoietic stem cells transduced at a low multiplicity-of-infection with a foamy viral MGMTP140K vector

Cai, Shanbao; Ernstberger, Aaron; Wang, Haiyan; Bailey, Barbara J.; Hartwell, Jennifer R.; Sinn, Anthony L.; Eckermann, Olaf; Linka, Yvonne; Goebel, W. Scott; Pollok, Karen E.

doi:10.1016/j.exphem.2007.11.009

Cited by 21 publications

(22 citation statements)

References 53 publications

(67 reference statements)

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“…44 Here, magselectofection with low MOIs (Յ 3) yielded up to 50% transduced cells ( Figure 4) compared with only 9.5% with an MOI of 5 to 8 using a standard transduction protocol for Lin Ϫ BM cells as reported previously. 45 Importantly, the magselectofected cells were fully competent in colony-forming assays ( Figure 4B-C), and administration in mice also resulted in long-term stable reconstitution and long-term GFP expression ( Figure 4D-F).…”

Section: Discussionmentioning

confidence: 99%

Magselectofection: an integrated method of nanomagnetic separation and genetic modification of target cells

Sanchez-Antequera

Mykhaylyk

Til

et al. 2011

Blood

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Research applications and cell therapies involving genetically modified cells require reliable, standardized, and costeffective methods for cell manipulation. We report a novel nanomagnetic method for integrated cell separation and gene delivery. Gene vectors associated with magnetic nanoparticles are used to transfect/transduce target cells while being passaged and separated through a high gradient magnetic field cell separation column. The integrated method yields excellent target cell purity and recovery. Nonviral and lentiviral magselectofection is efficient and highly specific for the target cell population as demonstrated with a K562/Jurkat T-cell mixture. Both mouse and human enriched hematopoietic stem cell pools were effectively transduced by lentiviral magselectofection, which did not affect the hematopoietic progenitor cell number determined by in vitro colony assays. Highly effective reconstitution of T and B lymphocytes was achieved by magselectofected murine wild-type lineage-negative Sca-1 ؉ cells transplanted into Il2rg ؊/؊ mice, stably expressing GFP in erythroid, myeloid, T-, and B-cell lineages. Furthermore, nonviral, lentiviral, and adenoviral magselectofection yielded high transfection/ transduction efficiency in human umbilical cord mesenchymal stem cells and was fully compatible with their differentiation potential. Upscaling to a clinically approved automated cell separation device was feasible. Hence, once optimized, validated, and approved, the method may greatly facilitate the generation of genetically engineered cells for cell therapies. (Blood. 2011;117(16): e171-e181) IntroductionThe feasibility of using genetically engineered cells for therapy in humans has been demonstrated using various cell types, including tumor cells, 1-3 lymphocytes, dendritic cells, 4,5 fibroblasts, 6,7 hematopoietic stem cells (HSCs), 8,9 and mesenchymal stem cells (MSCs). 10,11 Actual or potential applications are as diverse as immune gene therapy for the treatment of cancer, 1-3 cancer therapy with T cells expressing chimeric T-cell receptors, 12,13 the treatment of hereditary diseases, 8,9,[14][15][16] and a plethora of applications in regenerative medicine. 17 With the emerging field of induced pluripotent stem cells, research in genetically engineered cell therapies has reached yet another level of pace and dimension. Clinical applications will require efficient, reliable, standardized methods for cell manipulation. For optimized reproducibility and wide practicality in a decentralized manner, such methods should compose a minimum number of handling steps and be cost-effective and amenable to automation in a closed system.The goal of this work is to provide a novel methodology for performing genetic modification and cell isolation in a single standardized procedure, which we call "magselectofection" ( Figure 1). It integrates nanomagnetic cell separation, which is an approved clinical application, 18,19 and nanomagnetically guided nucleic acid delivery known as magnetofection. [20][21][22] For magneti...

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Section: Discussionmentioning

confidence: 99%

Magselectofection: an integrated method of nanomagnetic separation and genetic modification of target cells

Sanchez-Antequera

Mykhaylyk

Til

et al. 2011

Blood

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“…After one week, 20 colonies were picked for each mouse and subjected to standard LM-PCR analysis for identifying the location of the provirus in the genome. As described previously, 46 the position of the transgene from each colony was evaluated using the SeqMap website (http://seqmap.compbio.iupui.edu) and confirmed using the http://genome.ucsc.edu and http://www.ensembl.org websites. From each mouse, one proviral integration was detected (Table 2).…”

Section: Evaluation Of Proviral Integrantsmentioning

confidence: 99%

“…45 The DNA from excised bands was cloned into pCR2.1 using the TOPO cloning kit (Invitrogen, Frederick, MD) and then sequenced on an ABI Gene Amp 3770 System (Applied Biosystems, Foster City, CA). As described previously, 46 SeqMap (http://seqmap.compbio.iupui.edu, Indiana University School of Medicine) was used to map the sequences against the mouse genome. This was then confirmed by mapping the positions using the Ensembl website (http://www.ensembl.org) and mus musculus database release 42, December 2006, 47 and the UCSC Genome Browser (http://genome.ucsc.edu).…”

Section: Ligation-mediated Polymerase Chain Reactionmentioning

confidence: 99%

Overnight transduction with foamyviral vectors restores the long-term repopulating activity of Fancc−/− stem cells

Pulliam

Linka

et al. 2008

Blood

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IntroductionFanconi anemia (FA) is a complex recessive inherited disorder that is clinically characterized by variable congenital abnormalities, progressive bone marrow (BM) failure, and a high propensity to develop myeloid and epithelial malignancies. 1-5 On a cellular level, FA is characterized by a profound hypersensitivity upon exposure to DNA cross-linking agents such as mitomycin-C (MMC) or diepoxybutane (DEB). [6][7][8][9] Genetically, germ-line mutations in 13 genes (FANCA/B/C/D1/ D2/E/F/G/I/J/L/M/N) result in the clinical phenotype of FA. 2,8,[10][11][12][13][14] Spontaneous genetic correction of a germ-line mutation leading to repopulation of the entire hematopoietic system with normal progeny has been identified in a few FA patients. [15][16][17][18][19] These observations, in combination with the fact that the hematopoietic system can be functionally corrected in mice with targeted disruptions of FA genes by retroviral vectors expressing human analogues of the targeted mouse genes in stem cells, [20][21][22] have led to 3 clinical stem cell gene therapy phase 1 studies in FA-A and FA-C patients. So far, neither long-term marking/correction of cells nor clinical benefits for the patients were observed. 23,24 Due to the biologic characteristics of the gammaretroviral vectors used for transduction of stem cells, 25,26 optimal gene transfer protocols for delivery of genes to mammalian stem cells require a prestimulation period of 1 to 2 days with cytokines that promote the proliferation and survival of stem/progenitor cells. This is followed by a 2-to 3-day exposure of the target cells to vector containing supernatant on the recombinant fibronectin fragment 28 This gene transfer protocol was successful in transducing hematopoietic stem cells in humans, primates/monkeys, and mice. [29][30][31] However, in murine FA models, prolonged in vitro culture of Fancc Ϫ/Ϫ BM results in a length-of-culture-dependent reduction in myeloid progenitors and repopulating ability, 32,33 and the surviving untransduced Fancc Ϫ/Ϫ repopulating cells have an increased risk of developing cytogenetic abnormalities and myeloid malignancies. 22 Therefore, limiting the in vitro culture would be predicted to enhance both the efficacy and safety for genetic therapies of FA stem cells.Wild-type foamy viruses are the only retroviruses that are not associated with any disease in their natural hosts or in accidentally infected human beings. [34][35][36] It has been shown that vectors based on the prototype (formerly human) foamy virus (FV) can efficiently transduce hematopoietic stem cells from mice, 37 dogs, 38 and nonobese diabetic/ severe combined immunodeficiency (NOD/SCID) repopulating human cells. [39][40][41] Further, FV vectors are at least equally efficient at transduction of CD34 ϩ umbilical cord blood cells engrafting in NOD/SCID mice as lentiviral vectors based on HIV-1. 40 In the present study, we demonstrated for the first time the ability of FV vectors encoding the human FANCC transgene to completely correct Fancc Ϫ/Ϫ myelo...

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“…(Beard et al, 2010;Neff et al, 2005) Numerous transplant studies have convincingly proven that long-term repopulating murine HSCs could be selected in vivo with O 6 -BG/BCNU, O 6 -BG /TMZ, or O 6 -BG /CCNU. (Cai et al, 2008;Davis et al, 2004;Jansen et al, 2002;Kreklau et al, 2003;Milsom et al, 2004;Persons et al, 2003;Persons et al, 2004;Ragg et al, 2000;Sawai et al, 2003;Sawai et al, 2001) In regards to modeling of this approach with human HSPCs, we and others previously demonstrated that MGMT P140K -transduced SCID-repopulating cells and their progeny could be selected in vivo in NOD/SCID mice. Human HSPCs derived from umbilical cord blood (UCB) or granulocyte colony-stimulating factormobilized peripheral blood (MPB) that expressed MGMT P140K could be selected in vivo by www.intechopen.com nonmyeloablative doses of O 6 -BG and BCNU.…”

Section: In Vivo Selection Of Hspcs In Humanized Mouse Modelsmentioning

confidence: 99%

Therapeutic Modulation of DNA Damage and Repair Mechanisms in Blood Cells

Wang¹,

Cai²,

Tonsing-Carter³

et al. 2011

DNA Repair and Human Health

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In vivo selection of hematopoietic stem cells transduced at a low multiplicity-of-infection with a foamy viral MGMTP140K vector

Cited by 21 publications

References 53 publications

Magselectofection: an integrated method of nanomagnetic separation and genetic modification of target cells

Magselectofection: an integrated method of nanomagnetic separation and genetic modification of target cells

Overnight transduction with foamyviral vectors restores the long-term repopulating activity of Fancc−/− stem cells

Therapeutic Modulation of DNA Damage and Repair Mechanisms in Blood Cells

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