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通过基因工程建立产生白细胞介素-2的细胞。

The establishment of IL-2 producing cells by genetic engineering.

作者信息

Sasada R, Onda H, Igarashi K

出版信息

Cell Struct Funct. 1987 Apr;12(2):205-17. doi: 10.1247/csf.12.205.

Abstract

Expression plasmids containing human interleukin-2(IL-2) cDNA under the control of viral promoters (SV40 early region, MuLV LTR, HTLV-I LTR, and ASV (Y73) LTR) were introduced into TK- mouse L cells and human FL cells to establish IL-2 producing cells. The highest levels of IL-2 producing clones were obtained in TK+ mouse L cells transformed with a recombinant plasmid having MuLV LTR as a promoter, whereas transformed cells of human FL cells (G418r) were revealed to produce IL-2 at the highest level when the cells were transfected with a plasmid containing HTLV LTR as a promoter. These results suggest that these promoter/enhancer regions possess different cell specificities in gene expression. To obtain higher levels of IL-2 production using gene amplification, the hybrid plasmids containing the hamster DHFR and human IL-2 genes were constructed and transfected into DHFR- CHO cells. DHFR+ colonies produced IL-2 at about the same level as that produced by TK+ L cells transformed with the recombinants containing MuLV LTR. Selection of methotrexate-resistant cells resulted in a 5- to 30-fold increase of IL-2 production. These cells produced IL-2 stably for at least 3 months, even in the absence of methotrexate.

摘要

将含有在病毒启动子(SV40早期区域、莫洛尼鼠白血病病毒长末端重复序列(MuLV LTR)、人嗜T细胞病毒I型长末端重复序列(HTLV-I LTR)和阿氏肉瘤病毒(Y73)长末端重复序列)控制下的人白细胞介素-2(IL-2)cDNA的表达质粒导入TK-小鼠L细胞和人FL细胞,以建立产生IL-2的细胞。在用具有MuLV LTR作为启动子的重组质粒转化的TK+小鼠L细胞中获得了产生IL-2水平最高的克隆,而当用人FL细胞(G418抗性)的转化细胞用含有HTLV LTR作为启动子的质粒转染时,发现其产生IL-2的水平最高。这些结果表明,这些启动子/增强子区域在基因表达中具有不同的细胞特异性。为了通过基因扩增获得更高水平的IL-2产生,构建了含有仓鼠二氢叶酸还原酶(DHFR)和人IL-2基因的杂交质粒,并将其转染到DHFR-中国仓鼠卵巢(CHO)细胞中。DHFR+集落产生IL-2的水平与用含有MuLV LTR的重组体转化的TK+ L细胞产生的水平大致相同。选择抗甲氨蝶呤的细胞导致IL-2产生增加5至30倍。这些细胞即使在没有甲氨蝶呤的情况下也能稳定产生IL-2至少3个月。

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