Stable oncogenic transformation induced by microcell-mediated gene transfer.

Y Lü, D G Blair
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Abstract

Oncogenes have been identified using DNA-mediated transfection, but the size of the transferable and unrearranged DNA, gene rearrangement and amplification which occur during the transfection process limit the use of the techniques. We have evaluated microcell-mediated gene transfer techniques for the transfer and analysis of dominant oncogenes. MNNG-HOS, a transformed human cell line which contained the met oncogene mapping to human chromosome 7 was infected with retroviruses carrying drug resistance markers and used to optimize microcell preparation and transfer. Stable and drug-resistant hybrids containing single human chromosomes as well as the foci of the transformed cells containing the activated met oncogene and intact human chromosomes were obtained. Hybridization analysis with probes (i.e. col1A2, pJ3.11) mapping up to 1 Mb away from met shows that the cells from the individual foci contain different amounts of apparently unrearranged human DNA associated with the oncogene, and the microcell-generated transformants retain more distal markers than those observed in either DNA- or chromosome-mediated transfers. In conjunction with other techniques, microcell fusion should be useful for gene mapping as well as the study of gene function and expression in cell transformation and malignancy.

微细胞介导的基因转移诱导的稳定的致癌转化。
已经用DNA介导的转染技术鉴定了致癌基因,但是转染过程中可转移和未重排DNA的大小、基因重排和扩增限制了该技术的使用。我们已经评估了微细胞介导的基因转移技术用于显性癌基因的转移和分析。用携带耐药标记的逆转录病毒感染转染人细胞系MNNG-HOS,将其定位于人7号染色体,优化微细胞制备和转移。获得了含有单个人类染色体的稳定和耐药杂交体,以及含有活化的致癌基因和完整的人类染色体的转化细胞的焦点。用探针(如col1A2, pJ3.11)对距离met 1 Mb的区域进行杂交分析表明,来自单个病灶的细胞含有不同数量的与癌基因相关的明显未重排的人类DNA,并且微细胞产生的转化子保留了比DNA或染色体介导转移中观察到的更多的远端标记。与其他技术相结合,微细胞融合应该有助于基因定位以及研究基因功能和细胞转化和恶性肿瘤的表达。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
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