Thomas Dolly, Mostoslavsky Gustavo
Section of Gastroenterology, Department of Medicine, Center for Regenerative Medicine (CReM), Boston University School of Medicine, Boston, MA, USA.
Methods Mol Biol. 2014;1114:441-50. doi: 10.1007/978-1-62703-761-7_29.
The ability to efficiently transduce hematopoietic stem cells (HSC) represents a powerful methodology by which to study the role of specific genes on HSC function, as well as to broaden the potential of gene therapy for hematopoietic related diseases. While retroviruses have been used extensively to transduce a variety of cell types, HIV-derived lentiviruses prove superior for transduction of quiescent HSC due to their ability to infect non-dividing cells. Quality of lentiviral supernatants and starting cells are vital to obtain reproducible consistent results, and therefore, here we describe the production of concentrated lentiviral preparations, the purification of HSC from total mouse bone marrow, and their transduction to obtain long-term HSC engraftment with persistent gene transfer and expression of the desired transgene.
高效转导造血干细胞(HSC)的能力代表了一种强大的方法,通过该方法可以研究特定基因对HSC功能的作用,以及拓宽基因治疗造血相关疾病的潜力。虽然逆转录病毒已被广泛用于转导多种细胞类型,但源自HIV的慢病毒因其能够感染非分裂细胞而被证明在转导静止HSC方面更具优势。慢病毒上清液和起始细胞的质量对于获得可重复的一致结果至关重要,因此,在这里我们描述了浓缩慢病毒制剂的生产、从小鼠全骨髓中纯化HSC以及它们的转导,以实现长期HSC植入并持续进行基因转移和所需转基因的表达。