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嵌合慢病毒载体增强造血细胞的转导。

Enhanced Transduction of Hematopoietic Cells with Chimeric Lentiviral Vectors.

机构信息

Division of Innovative Therapies, UMR E007, Institute of Biology François Jacob, CEA, Paris-Sud University, Paris-Saclay University, Fontenay aux Roses, France.

Université Paris Diderot, Sorbonne Paris Cité, Paris, France.

出版信息

Hum Gene Ther. 2019 Oct;30(10):1306-1323. doi: 10.1089/hum.2018.179. Epub 2019 May 15.

Abstract

Recent marketing approval for genetically engineered hematopoietic stem and T cells bears witness to the substantial improvements in lentiviral vectors over the last two decades, but evaluations of the long-term efficacy and toxicity of gene and cell therapy products will, nevertheless, require further studies in nonhuman primate models. monkeys from Mauritius have a low genetic diversity and are particularly useful for reproducible drug testing. In particular, they have a genetically homogeneous class I major histocompatibility complex system that probably mitigates the variability of the response to simian immunodeficiency virus infection. However, the transduction of simian cells with human immunodeficiency virus type 1 (HIV-1)-derived vectors is inefficient due to capsid-specific restriction factors, such as the tripartite motif-containing protein tripartite motif 5α, which prevent infection with non-host-adapted retroviruses. This study introduced the modified capsid of the macaque-trophic HIV-1 clone MN4/LSQD into the packaging system and compared transduction efficiencies between hematopoietic cells transduced with this construct and cells transduced with HIV-1 NL4-3-derived packaging constructs. Capsid modification increased transduction efficiency in all hematopoietic cells tested (by factors of up to 10), including hematopoietic progenitor cells, repopulating cells, and T cells from Mauritian , regardless of vector structure or purification method. The study also established culture conditions similar to those used in clinical practice for the efficient transduction of hematopoietic stem and progenitor CD34 cells. These results suggest that the procedure is suitable for use in Mauritian , which can therefore be used as a model in preclinical studies for hematopoietic gene and cell therapy.

摘要

最近,基因工程造血干细胞和 T 细胞的上市批准见证了过去 20 年来慢病毒载体的重大改进,但基因和细胞治疗产品的长期疗效和毒性评估仍需要进一步在非人类灵长类动物模型中进行研究。毛里求斯的猴子遗传多样性较低,特别适合用于可重复的药物测试。特别是,它们具有遗传上同质的 I 类主要组织相容性复合物系统,这可能减轻了对猿猴免疫缺陷病毒感染的反应的可变性。然而,由于衣壳特异性限制因子,例如包含三部分基序的蛋白三部分基序 5α,用源自人类免疫缺陷病毒 1(HIV-1)的载体转导灵长类细胞的效率较低,该因子阻止非宿主适应的逆转录病毒感染。本研究将猕猴嗜性 HIV-1 克隆 MN4/LSQD 的修饰衣壳引入包装系统,并比较了用这种构建体转导的造血细胞与用 HIV-1 NL4-3 衍生的包装构建体转导的细胞之间的转导效率。衣壳修饰提高了所有测试的造血细胞(高达 10 倍)的转导效率,包括造血祖细胞、重编程细胞和来自毛里求斯的 T 细胞,无论载体结构或纯化方法如何。该研究还建立了与临床实践中用于高效转导造血干细胞和祖细胞 CD34 细胞相似的培养条件。这些结果表明,该程序适用于毛里求斯,可以作为造血基因和细胞治疗的临床前研究模型。

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