Bucchini D, Lasserre C, Kunst F, Lovell-Badge R, Pictet R, Jami J
Institut Jacques Monod du Centre National de la Recherche Scientifique et de l'Université Paris 7, France.
EMBO J. 1983;2(2):229-32. doi: 10.1002/j.1460-2075.1983.tb01410.x.
Transformation of PCC4 mouse teratocarcinoma stem cells was obtained using a dominant selective marker, the enzyme xanthine-guanine phosphoribosyltransferase (XGPRT), coded by the bacterial Eco.gpt gene placed under the control of the early SV40 genes in the vector pSV2gpt. An average of 20 colonies of transformed cells was obtained, using the calcium phosphate technique, 10 microg DNA vector, no carrier DNA and 1 x 10(6) recipient cells. Five independent Eco.gpt-transformed PCC4 cell lines were propagated in selective medium and assayed for XGPRT activity. All of them had the ability to convert [14C]xanthine to xanthine monophosphate. pSV2gpt sequences were present and associated with high mol. wt. cellular DNA. pSV2gpt sequences and XGPRT activity were both conserved in the three clones that were propagated in non-selective medium for 30 generations. The transformed PCC4 cells retained their ability to produce, in host mice, teratocarcinoma tumors composed of embryonal carcinoma and various differentiated tissues. Thus, pSV2gpt can be used as a dominant marker to select teratocarcinoma stem cells co-transformed with genes that are not selectable by themselves.
利用显性选择标记——由细菌Eco.gpt基因编码的黄嘌呤-鸟嘌呤磷酸核糖转移酶(XGPRT),实现了PCC4小鼠畸胎瘤干细胞的转化。该基因置于载体pSV2gpt中早期SV40基因的控制之下。采用磷酸钙技术,使用10微克DNA载体、无载体DNA以及1×10⁶个受体细胞,平均获得了20个转化细胞集落。五个独立的经Eco.gpt转化的PCC4细胞系在选择培养基中传代培养,并检测其XGPRT活性。所有细胞系均有能力将[¹⁴C]黄嘌呤转化为黄嘌呤单磷酸。pSV2gpt序列存在且与高分子量细胞DNA相关。在非选择培养基中传代培养30代的三个克隆中,pSV2gpt序列和XGPRT活性均得以保留。转化后的PCC4细胞在宿主小鼠体内仍保留产生由胚胎癌和各种分化组织组成的畸胎瘤肿瘤的能力。因此,pSV2gpt可作为显性标记,用于筛选与自身不可选择的基因共转化的畸胎瘤干细胞。
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