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作 者:韦启泽[1] 刘德培[1] 陶吉中[1] 刘庆辉[1] 贾佩臣[1] 雷学锋[1] 陈松森[1] 梁植权[1]
机构地区:[1]中国医学科学院基础医学研究所,武汉同济医科大学
出 处:《中华医学杂志》1995年第11期694-696,共3页National Medical Journal of China
基 金:国家863高科技发展计划资助
摘 要:为寻找合适长度的红系增强子,在不影响病毒滴度和前病毒整合稳定性前提下,提高外源β-珠蛋白基因的表达水平,作者将完整β基因(β)或部分缺失IVSII(第二内含子)的β-基因(Δβ)和不同长度的红系增强子(36、292、与341bp)分别克隆于反转录病毒载体N2A上,重组体分别转染ψ-2单向性包装细胞系,由ψ-2出芽的病毒颗粒感染PA317双向性包装细胞系,筛选病毒滴度较高,前病毒整合完整的PA317细胞克隆的病毒上清感染鼠红白血病(MEL)细胞,用RNase保护实验检测β-珠蛋白基因的表达。结果表明,不仅获得了稳定的前病毒整合和较高的病毒滴度,而且含292bp和341bp红系增强子的β-基因表达水平接近或达到内源性α基因。Our previous works have verified that the β-globin gene carrying larg fragments of erythroid enhancer transferred by retrovirus vector caused the unstable provirus integration and low virus titer in infected cells,but the 36bp enhancer had not this negative effect.In order to circumvent this problem,we inserted the intact β-globin gene (β)or partially IVSII deleted β-globin gene (Δβ)and truncated erythroid enhancer(36bp,292bp and 341bp)into the N2A retrovirus vector.Recombinants were transfected into Ψ-2 ecotropic pachaging cells first, then the produced virus were used to infect PA317 amphotropic packaging cells.Virus supernatent from PA317 clonies with high virus titer and intact provirus integration was used to infect MEL cells. RNase protection assay was used to detect the expression of β-globin gene. Results showed that not only the stable provirus integration and high virus titer of the transferred genes,but also the high levels expression of β-globin gene carrying 292bp or 341bp erythroid enhancer were got.
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