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将病毒胸苷激酶基因和人类β-珠蛋白基因导入发育多能性小鼠畸胎瘤细胞。

Introduction of a viral thymidine kinase gene and the human beta-globin gene into developmentally multipotential mouse teratocarcinoma cells.

作者信息

Pellicer A, Wagner E F, el-Kareh A, Dewey M J, Reuser A J, Silverstein S, Axel R, Mintz B

出版信息

Proc Natl Acad Sci U S A. 1980 Apr;77(4):2098-102. doi: 10.1073/pnas.77.4.2098.

Abstract

Teratocarcinoma (TCC) stem cells provide unique prospects for the introduction of specific genes into mice, by virtue of their dual capacity for propagation in vitro and for normal differentiation in embryos. In this study, we have demonstrated that foreign genes amenable to selection in culture can be transferred into the stem cells and expressed. These cells maintain expression of the gene for long periods during differentiation in tumors in vivo in the absence of selective pressure. The cells also integrate an unlinked nonselectable gene at high frequency. Addition of the cloned herpes simplex virus (HSV) thymidine kinase (tk; ATP:thymidine 5'-phosphotransferase, EC 2.7.1.21) gene to cultures of tk(-)TCC cells yielded tk(+) colonies at a frequency of one colony per 4 mug of plasmid DNA. This transformation efficiency, although appreciably lower than for mouse L tk(-) cells, permits the isolation of many transformants. The HSV provenance of the transformed phenotype was verified by the characteristic electrophoretic mobility of the tk protein and by neutralization of the tk activity with specific antiserum. Moreover, blot hybridization tests revealed at least one intact copy of the viral tk gene integrated into the DNA of transformed cells. When injected into syngeneic mice, the cells formed solid tumors with various differentiating tissues. From blot hybridization comparisons with their cell lines of origin, seven of nine tumors examined had maintained the HSV tk gene without significant loss or rearrangement. Viral tk enzyme activity could also be demonstrated in at least some of the tumors. Cotransfer of the cloned human beta-globin gene along with the unlinked HSV tk gene was successful in 2 of 10 tk(+) transformants. Thus, defined genes can be stably introduced into TCC cells in culture and maintained in vivo in a form in which they are transcribed and translated to produce a functional protein.

摘要

畸胎癌(TCC)干细胞为将特定基因导入小鼠提供了独特的前景,这得益于它们在体外增殖以及在胚胎中正常分化的双重能力。在本研究中,我们已经证明,可在培养中进行选择的外源基因能够被转入干细胞并表达。这些细胞在体内肿瘤分化过程中,在没有选择压力的情况下能长时间维持基因表达。这些细胞还能高频整合一个不连锁的非选择基因。将克隆的单纯疱疹病毒(HSV)胸苷激酶(tk;ATP:胸苷5'-磷酸转移酶,EC 2.7.1.21)基因添加到tk(-)TCC细胞培养物中,每4微克质粒DNA可产生频率为一个菌落的tk(+)菌落。这种转化效率虽然明显低于小鼠L tk(-)细胞,但仍能分离出许多转化体。通过tk蛋白特有的电泳迁移率以及用特异性抗血清中和tk活性,证实了转化表型的HSV来源。此外,印迹杂交试验显示至少有一个完整的病毒tk基因拷贝整合到了转化细胞的DNA中。当注入同基因小鼠体内时,这些细胞形成了含有各种分化组织的实体瘤。通过与其起源细胞系的印迹杂交比较,所检测的9个肿瘤中有7个保持了HSV tk基因,没有明显的丢失或重排。在至少一些肿瘤中也能检测到病毒tk酶活性。在10个tk(+)转化体中有2个成功实现了克隆的人β-珠蛋白基因与不连锁的HSV tk基因的共转移。因此,特定基因能够稳定地导入培养的TCC细胞中,并在体内以转录和翻译产生功能性蛋白质的形式得以维持。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/328d/348659/36a4c1227934/pnas00667-0414-a.jpg

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