Sukoyan M A, Belyaev N D, Budker V G, Gradov A A, Pack S D, Serov O L
Mol Gen Genet. 1985;201(3):487-91. doi: 10.1007/BF00331344.
A method for gene transfer by means of interphase nuclei encapsulated within lipid membranes was developed. The method was based on passage of interphase nuclei through a layer of organic solvents containing phospholipids. Evidence was obtained indicating that the nuclei become surrounded by a protective phospholipid membrane: measurements of bound labelled or non-labelled phospholipids; decrease in the permeability of lipid-encapsulated nuclei for high molecular compounds; visualization by direct electron microscopy. Lipid-encapsulated nuclei of mink fibroblasts were used for transformation of mutant mouse LMTK- cells (deficient for thymidine kinase). The frequency of occurrence of HAT-resistant colonies/recipient cell was 1.9 X 10(-5). Biochemical analysis of 14 independent clones demonstrated that they all contained TK1 of mink origin. Analysis of 15 other biochemical markers located on 12 of the mink chromosomes revealed the activities of mink galactokinase (a syntenic marker) in 5 transformed clones, and that of mink aconitase-1 (the marker of mink chromosome 12) in 1 clone. No cytogenetically visible donor chromosomes were identified in the transformed clones. Nine transformed clones were tested for the stability of the TK+ phenotype; of these, the phenotype was expressed stably in 3 and unstably in 6. The method suggested is similar to the gene transfer procedure using total DNA. Its advantage is in ensuring efficient gene transfer and donor DNA integrity.
开发了一种通过脂质膜包裹的间期细胞核进行基因转移的方法。该方法基于间期细胞核穿过一层含有磷脂的有机溶剂。获得的证据表明细胞核被保护性磷脂膜包围:对结合的标记或未标记磷脂的测量;脂质包裹的细胞核对高分子化合物的通透性降低;通过直接电子显微镜观察。水貂成纤维细胞的脂质包裹细胞核用于转化突变小鼠LMTK-细胞(胸苷激酶缺陷)。抗HAT菌落/受体细胞的出现频率为1.9×10(-5)。对14个独立克隆的生化分析表明,它们都含有水貂来源的TK1。对位于12条水貂染色体上的其他15个生化标记的分析显示,5个转化克隆中存在水貂半乳糖激酶(一个同线标记)的活性,1个克隆中存在水貂乌头酸酶-1(水貂12号染色体的标记)的活性。在转化克隆中未鉴定出细胞遗传学上可见的供体染色体。对9个转化克隆进行了TK+表型稳定性测试;其中,3个克隆中表型稳定表达,6个克隆中表型不稳定表达。所提出的方法类似于使用总DNA的基因转移程序。其优点在于确保高效的基因转移和供体DNA完整性。
