Hanazono Yutaka, Terao Keiji, Shibata Hiroaki, Nagashima Takeyuki, Ageyama Naohide, Asano Takayuki, Ueda Yasuji, Kato Ikunoshin, Kume Akihiro, Hasegawa Mamoru, Ozawa Keiya
Division of Genetic Therapeutics, Center for Molecular Medicine, Jichi Medical School, Tochigi, Japan.
J Gene Med. 2002 Sep-Oct;4(5):470-7. doi: 10.1002/jgm.307.
The green fluorescent protein (GFP) has proven a useful marker in retroviral gene transfer studies targeting hematopoietic stem cells (HSCs) in mice. However, several investigators have reported very low in vivo peripheral blood marking levels in nonhuman primates after transplantation of HSCs transduced with the GFP gene. We retrovirally marked cynomolgus monkey HSCs with the GFP gene, and tracked in vivo marking levels within both bone marrow progenitor cells and mature peripheral blood cells following autologous transplantation after myeloablative conditioning.
Bone marrow cells were harvested from three cynomolgus macaques and enriched for the primitive fraction by CD34 selection. CD34(+) cells were transduced with one of three retroviral vectors all expressing the GFP gene and were infused after myeloablative total body irradiation (500 cGy x 2). Following transplantation, proviral levels and fluorescence were monitored among clonogenic bone marrow progenitors and mature peripheral blood cells.
Although 13-37% of transduced cells contained the GFP provirus and 11-13% fluoresced ex vivo, both provirus and fluorescence became almost undetectable in the peripheral blood within several months after transplantation regardless of the vectors used. However, on sampling of bone marrow at multiple time points, significant fractions (5-10%) of clonogenic progenitors contained the provirus and fluoresced ex vivo reflecting a significant discrepancy between GFP gene marking levels within bone marrow cells and their mature peripheral blood progeny. The discrepancy (at least one log) persisted for more than 1 year after transplantation. Since no cytotoxic T lymphocytes against GFP were detected in the animals, an immune response against GFP is an unlikely explanation for the low levels of transduced peripheral blood cells. Administration of granulocyte colony stimulating factor and stem cell factor resulted in mobilization of transduced bone marrow cells detectable as mature granulocyte progeny which expressed the GFP gene, suggesting that transduced progenitor cells in bone marrow could be mobilized into the peripheral blood and differentiated into granulocytes.
Low levels of GFP-transduced mature cells in the peripheral blood of nonhuman primates may reflect a block to differentiation associated with GFP; this block can be overcome in part by nonphysiological cytokine treatment ex vivo and in vivo.
绿色荧光蛋白(GFP)已被证明是小鼠造血干细胞(HSC)逆转录病毒基因转移研究中的一种有用标记物。然而,一些研究人员报告称,在用GFP基因转导的HSC移植后,非人类灵长类动物体内外周血标记水平非常低。我们用GFP基因对食蟹猴HSC进行逆转录病毒标记,并在清髓性预处理后的自体移植后,追踪骨髓祖细胞和成熟外周血细胞内的体内标记水平。
从三只食蟹猴采集骨髓细胞,通过CD34选择富集原始部分。用三种均表达GFP基因的逆转录病毒载体之一转导CD34(+)细胞,并在清髓性全身照射(500 cGy×2)后注入。移植后,在克隆形成性骨髓祖细胞和成熟外周血细胞中监测前病毒水平和荧光。
尽管13 - 37%的转导细胞含有GFP前病毒,且11 - 13%在体外发出荧光,但无论使用何种载体,移植后数月外周血中前病毒和荧光几乎都无法检测到。然而,在多个时间点采集骨髓样本时,相当一部分(5 - 10%)克隆形成祖细胞含有前病毒并在体外发出荧光,这反映出骨髓细胞及其成熟外周血后代中GFP基因标记水平存在显著差异。这种差异(至少一个对数级)在移植后持续超过1年。由于在动物体内未检测到针对GFP的细胞毒性T淋巴细胞,因此针对GFP的免疫反应不太可能是转导外周血细胞水平低的原因。给予粒细胞集落刺激因子和干细胞因子导致可检测到的转导骨髓细胞动员,其作为表达GFP基因的成熟粒细胞后代,这表明骨髓中的转导祖细胞可被动员到外周血并分化为粒细胞。
非人类灵长类动物外周血中GFP转导的成熟细胞水平低可能反映了与GFP相关的分化阻滞;这种阻滞可通过体外和体内的非生理性细胞因子治疗部分克服。
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