Cohen-Haguenauer Odile, Péault Bruno, Bauche Cécile, Daniel Marie-Thérèse, Casal Ibrahim, Levy Vincent, Dausset Jean, Boiron Michel, Auclair Christian, Gluckman Eliane, Marty Michel
Laboratory of Biotechnology and Applied Pharmacogenetics, Ecole Normale Supérieure de Cachan, 94235 Cachan Cedex, France.
Proc Natl Acad Sci U S A. 2006 Feb 14;103(7):2340-5. doi: 10.1073/pnas.0510613103. Epub 2006 Feb 6.
Fanconi anemia (FA) is a rare inherited genomic instability syndrome representing one of the best examples of hematopoietic stem cell deficiency. Although FA might be an excellent candidate for bone marrow (BM) genetic correction ex vivo, knockout animal models are not sufficient to guide preclinical steps, and gene therapy attempts have proven disappointing so far. Contributing to these poor results is a characteristic and dramatic early BM-cells die-off when placed in culture. We show here that human primary FA BM cell survival can be ameliorated by using specific culture conditions that limit oxidative stress. When coupled with retrovirus-mediated transfer of the main complementation group FANCA-cDNA, we could achieve long-term reconstitution of the stem cell compartment both in vitro and in vivo. Gene-corrected BM cultures grew for >120 days, and after cultured cell transplantation into NOD/SCID mice, clonogenic human cells carrying the FANCA transgene could be detected 6 months after transduction. By comparison, untransduced cells died in culture by 15 days. Of necessity for ethical reasons, experiments were conducted on a very limited number of primary BM cells. By using low cytokine regimen and conditions matching regulatory requirements, a contingent of gene-corrected cells slowly emerges with an unmet potential for in vivo engraftment. Future therapeutic applications of stem cells might be expanding from these data. In addition, we provide a model of gene-corrected human primary cell growth that carries the potential to better delineate the combined role of both DNA damage and oxidative stress in the pathogenesis of FA.
范可尼贫血(FA)是一种罕见的遗传性基因组不稳定综合征,是造血干细胞缺陷的最佳实例之一。尽管FA可能是体外骨髓(BM)基因校正的理想候选者,但基因敲除动物模型不足以指导临床前步骤,而且到目前为止基因治疗尝试已被证明令人失望。导致这些不佳结果的原因是,置于培养中的BM细胞具有特征性且显著的早期死亡现象。我们在此表明,通过使用限制氧化应激的特定培养条件,可以改善人类原发性FA BM细胞的存活。当与逆转录病毒介导的主要互补组FANCA-cDNA转移相结合时,我们能够在体外和体内实现干细胞区室的长期重建。基因校正的BM培养物生长超过120天,并且在将培养细胞移植到NOD/SCID小鼠中后,转导6个月后可检测到携带FANCA转基因的克隆形成人类细胞。相比之下,未转导的细胞在培养15天时死亡。出于伦理原因,实验仅在非常有限数量的原发性BM细胞上进行。通过使用低细胞因子方案和符合监管要求的条件,一批基因校正细胞缓慢出现,但其体内植入潜力尚未得到满足。干细胞未来的治疗应用可能会从这些数据中得到拓展。此外,我们提供了一种基因校正的人类原代细胞生长模型,它有可能更好地描绘DNA损伤和氧化应激在FA发病机制中的联合作用。