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体内过表达胞质和线粒体谷胱甘肽还原酶的逆转录病毒的生成。

Generation of retroviruses for the overexpression of cytosolic and mitochondrial glutathione reductase in macrophages in vivo.

机构信息

Department of Laboratory Medicine, Kenezy Gyula Hospital, Debrecen, Hungary.

出版信息

Cytotechnology. 2007 May;54(1):5-14. doi: 10.1007/s10616-007-9046-7. Epub 2007 Feb 23.

Abstract

Retroviral gene transfer and bone marrow transplantation has been used by many investigators to study the role of macrophage proteins in different mouse models of human disease. While this approach is faster and less expensive than generating transgenic mice with macrophage-specific promoters and applicable to a wider array of mouse models, it has been hampered by two major drawbacks: labor-intensive cloning procedures involved in generating retroviral vectors for each gene of interest and low viral titers. Here we describe the construction of a MSCV-based retroviral vector that can serve as an acceptor vector for commercially available Cre-lox-compatible donor vectors. Using this new retroviral vector in combination with a FACS approach to enhance viral titers, we generated high-titer retroviruses carrying either EGFP-tagged cytosolic or EGFP-tagged mitochondria-targeted glutathione reductase. We show that the introduction of these constructs via retroviral gene transfer and bone marrow transplantation into atherosclerosis-prone LDL receptor-null mice results in the long-term increase in macrophage glutathione reductase activity.

摘要

逆转录病毒基因转移和骨髓移植已被许多研究人员用于研究巨噬细胞蛋白在不同人类疾病小鼠模型中的作用。虽然这种方法比使用具有巨噬细胞特异性启动子的转基因小鼠更快、更经济,并且适用于更广泛的小鼠模型,但它受到两个主要缺点的阻碍:生成感兴趣的每个基因的逆转录病毒载体涉及劳动密集型克隆程序,以及病毒滴度低。在这里,我们描述了一种基于 MSCV 的逆转录病毒载体的构建,该载体可用作商业上可获得的 Cre-lox 兼容供体载体的接受载体。使用这种新的逆转录病毒载体结合 FACS 方法来提高病毒滴度,我们生成了携带 EGFP 标记的胞质或 EGFP 标记的线粒体靶向谷胱甘肽还原酶的高滴度逆转录病毒。我们表明,通过逆转录病毒基因转移和骨髓移植将这些构建体引入易患动脉粥样硬化的 LDL 受体缺失小鼠中,可导致巨噬细胞谷胱甘肽还原酶活性的长期增加。

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