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Development of Improved Adenosine Deaminase Retroviral Vectors

机译:改进的腺苷脱氨酶逆转录病毒载体的开发

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摘要

A series of adenosine deaminase (ADA) retroviral vectors were designed and constructed with the goal of improved performance over the PA317/LASN vector currently used in clinical trials. First, the bacterial selectable-marker neomycin phosphotransferase (neo) gene was removed to create a “simplified” vector. Second, the Moloney murine leukemia virus long terminal repeat (LTR) promoter used for ADA expression was replaced with either the myeloproliferative sarcoma virus (MPSV) or SL3-3 LTR. Supernatant from each ADA vector was used to transduce ADA-deficient (ADA) B- and T-cell lines as well as primary peripheral blood mononuclear cells (PBMC) from an ADA severe combined immunodeficiency patient. Total ADA enzyme activity and ADA activity per integrant in the transduced cells demonstrated that the MPSV LTR splicing vector design provided the highest level of ADA expression per cell. This ADA(MPSV) vector was then tested in packaging cell lines containing either the gibbon ape leukemia virus envelope (PG13 cells), the murine amphotropic envelope (FLYA13 cells), or the feline endogenous virus RD114 envelope (FLYRD18 cells). The results indicate that FLYRD18/ADA(MPSV), a simplified ADA retroviral vector with the MPSV LTR, provides a 17-fold-higher level of ADA expression in human lymphohematopoietic cells than the PA317/LASN vector currently in use.
机译:设计和构建了一系列腺苷脱氨酶(ADA)逆转录病毒载体,目的是与目前临床试验中使用的PA317 / LASN载体相比,提高性能。首先,去除细菌的选择性标记新霉素磷酸转移酶(neo)基因,以创建“简化”载体。其次,用骨髓增生性肉瘤病毒(MPSV)或SL3-3 LTR替代用于ADA表达的莫洛尼氏鼠白血病病毒长末端重复(LTR)启动子。来自每个ADA载体的上清液被用于转导ADA缺陷(ADA -)B细胞和T细胞系以及ADA -支持>严重的合并免疫缺陷患者。转导细胞中的总ADA酶活性和每个整合子的ADA活性表明,MPSV LTR剪接载体设计提供了每个细胞中最高水平的ADA表达。然后在包含长臂猿白血病病毒包膜(PG13细胞),鼠类两性包膜(FLYA13细胞)或猫内源性病毒RD114包膜(FLYRD18细胞)的包装细胞系中测试此ADA(MPSV)载体。结果表明,FLYRD18 / ADA(MPSV)是一种具有MPSV LTR的简化ADA逆转录病毒载体,与目前使用的PA317 / LASN载体相比,其在人淋巴造血细胞中的ADA表达水平高17倍。

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