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人α1-抗胰蛋白酶基因在体内向肺巨噬细胞的转移。

Transfer of the human Alpha1-antitrypsin gene into pulmonary macrophages in vivo.

作者信息

Ferkol T, Mularo F, Hilliard J, Lodish S, Perales J C, Ziady A, Konstan M

机构信息

Department of Pediatrics, Case Western Reserve University School of Medicine, Cleveland, Ohio, USA.

出版信息

Am J Respir Cell Mol Biol. 1998 May;18(5):591-601. doi: 10.1165/ajrcmb.18.5.2874.

DOI:10.1165/ajrcmb.18.5.2874
PMID:9569229
Abstract

Several viral and nonviral methods have introduced functional genes into the lungs. An alternative strategy, receptor-mediated gene transfer, exploits the ability of receptors on the surface of cells to bind and internalize DNA complexes and could potentially be used to deliver genes to specific cells in the lung. The gene encoding human alpha1-antitrypsin (A1AT) was delivered to macrophages in vitro and in vivo by targeting the mannose receptor with mannose-terminal molecular conjugates. The human A1AT transcript was detected 2 d after transfection of macrophages in culture, but transgene expression was transient. Human A1AT protein was secreted into the culture medium, and Western blot hybridization revealed the mature human antiprotease. In addition, Sprague-Dawley rats underwent intravenous injections of increasing doses of plasmid DNA (0.2 mg, 1.0 mg, and 2.0 mg) complexed to the molecular conjugate. Four days after transfection, human A1AT mRNA was found in lungs from six of the 13 rats (46%) that received the higher doses of plasmid. Transgene expression was limited to cells in perivascular and alveolar regions, which conformed to the distribution of pulmonary macrophages. Human A1AT was measured in the epithelial lining fluid of rats treated with transfection complexes. Animals that received 1.0 mg of plasmid had human A1AT levels of 7.4 +/- 3.4 pM, which was significantly different from nontransfected and mock-transfected controls. Thus the mannose receptor permitted direct delivery of genes to pulmonary macrophages, though transgene expression was detected in the lung only at low levels.

摘要

多种病毒和非病毒方法已将功能基因导入肺部。另一种策略,即受体介导的基因转移,利用细胞表面受体结合并内化DNA复合物的能力,有可能用于将基因递送至肺内特定细胞。通过用甘露糖末端分子缀合物靶向甘露糖受体,将编码人α1-抗胰蛋白酶(A1AT)的基因在体外和体内递送至巨噬细胞。在培养的巨噬细胞转染后2天检测到人类A1AT转录本,但转基因表达是短暂的。人A1AT蛋白分泌到培养基中,蛋白质印迹杂交显示出成熟的人抗蛋白酶。此外,对斯普拉格-道利大鼠静脉注射与分子缀合物复合的递增剂量质粒DNA(0.2mg、1.0mg和2.0mg)。转染后4天,在接受较高剂量质粒的13只大鼠中的6只(46%)的肺中发现了人A1AT mRNA。转基因表达仅限于血管周围和肺泡区域的细胞,这与肺巨噬细胞的分布一致。在用转染复合物处理的大鼠的上皮衬液中检测到人A1AT。接受1.0mg质粒的动物的人A1AT水平为7.4±3.4pM,这与未转染和模拟转染的对照有显著差异。因此,甘露糖受体允许将基因直接递送至肺巨噬细胞,尽管仅在肺中检测到低水平的转基因表达。

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