胸苷激酶缺失、悬浮培养的Walker癌256细胞系的建立与鉴定。

In Vitro Pub Date : 1984-07-01 DOI:10.1007/BF02639771
F Arvelo, A Yabrudi, M E Delgado, N González-Cadavid
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引用次数: 1

摘要

在含5%牛血清的培养基中悬浮培养大鼠Walker癌肉瘤256细胞系,培养350代以上,平均群体翻倍时间为17 h,培养效率为56%,菌落形成效率为32%,在软琼脂中具有良好的菌落形成能力。通过透射电镜和扫描电镜检查,这些细胞在形态上与实体瘤和腹水中的细胞难以区分。核型的特征是65条染色体的模态数和一个标记的异心染色体的存在。细胞表达胸苷激酶、γ -谷氨酰转肽酶和碱性磷酸酶;被豆豆蛋白A粘合;并且可以被三重胸腺嘧啶阻滞同步。它们诱导大鼠皮下(实体)和腹腔内(腹水)的原发性肿瘤;经尾静脉注射后能够转移;侵入鸡胚的绒毛膜尿囊膜。悬浮中的细胞可以转移到单层中,在不影响其他研究参数的情况下大大降低其致瘤性,并且可以切换回悬浮培养。DNA介导转染表明,来自这些细胞的DNA可以转化NIH-3T3细胞系。单层细胞在含有brdurd的培养基中生长后,建立了一个亚系,该亚系克隆到一个胸腺嘧啶激酶缺陷系中,该系不能在HAT培养基中生长,其特性与亲本野生型细胞相似。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
Establishment and characterization of cell lines from the Walker carcinoma 256 able to grow in suspension culture and deficient in thymidine kinase.

A cell line from the Walker carcinosarcoma 256 of the rat has been established in suspension culture in medium with 5% bovine calf serum for over 350 generations, with an average population doubling time of 17 h, a plating efficiency of 56%, a colony forming efficiency of 32%, and a good capacity to form colonies in soft agar. The cells are morphologically indistinguishable from those in the solid tumor and ascites as checked by transmission and scanning electron microscopy. The karyotype is characterized by a modal number of 65 chromosomes and by the presence of a marker metacentric chromosome. The cells express thymidine kinase, gamma-glutamyl transpeptidase, and alkaline phosphatase; are agglutinable by concanavalin A; and can be synchronized by the triple thymidine block. They induce primary tumors, both subcutaneously (solid) and intraperitoneally (ascitic), in the rat; are able to metastasize upon injection by the tail vein; and invade the chorioallantoic membrane of the chick embryo. Cells in suspension can be transferred to monolayers, considerably decreasing their tumorigenicity without affecting the other parameters studied, and can be switched back to suspension culture. DNA-mediated transfection showed that DNA from these cells can transform the NIH-3T3 line. Upon growth of the monolayers in a BrdUr-containing medium, a sub-line was established that was cloned into a thymidine kinase-deficient line unable to grow in HAT medium and with properties otherwise similar to those of the parental wild type cells.

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