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在HC11细胞中,用糖皮质激素进行预处理对于牛β-酪蛋白/氯霉素乙酰转移酶(CAT)表达的泌乳诱导至关重要。

Pretreatment with glucocorticoid is essential for lactogenic induction of the bovine beta-casein/CAT expression in HC11 cells.

作者信息

Lee C S, Kim K, Yu D Y, Lee K K

机构信息

Korea Research Institute of Bioscience and Biotechnology, KIST, Taejon, Korea.

出版信息

Endocr Res. 1998 Feb;24(1):65-77. doi: 10.3109/07435809809031869.

Abstract

Hormonal regulation of the bovine beta-casein gene expression was studied in a murine mammary epithelial HC11 cells and compared with that of the rat beta-casein gene expression. CAT expression vectors driven by their promoter sequences were transfected into HC11 cells. Stable transfectents were treated with lactogenic hormones, dexamethasone and prolactin for 2 days in confluent cultures. While the lactogenic hormones synergistically induced a strong activation of the rat beta-casein/CAT expression, neither a single or combined treatment of dexamethasone and prolactin induced the bovine beta-casein/CAT expression. To test a sequential treatment effect of lactogenic hormones on the bovine beta-casein/CAT expression, cells were first treated with either dexamethasone or prolactin for various days and then subjected to the second treatment with both hormones for 2 days. Only dexamethasone-, but not prolactin-pretreated cells showed a strong lactogenic induction. Moreover, the fold induction of dexamethasone-pretreated cells increased gradually as a function of duration of dexamethasone pretreatment. A series of the bovine beta-casein/CAT constructs with different length of the bovine beta-casein 5' flanking region ranged from 0.3 kb to about 15 kb was analyzed in 12-days dexamethasone-pretreated cultures. CAT expression was increased even in 0.3 kb-containing construct, but prominent induction was seen in more than 1.8 kb-containing constructs. Therefore, it could be concluded that a long-term dexamethasone pretreatment is essential for lactogenic induction of the bovine beta-casein expression and the 0.3 kb proximal promoter region is important, but more distal promoter element(s) is necessary for mediating the coordinated action of lactogenic hormones to the bovine beta-casein expression.

摘要

在小鼠乳腺上皮HC11细胞中研究了牛β-酪蛋白基因表达的激素调节,并与大鼠β-酪蛋白基因表达的激素调节进行了比较。将由其启动子序列驱动的CAT表达载体转染到HC11细胞中。在汇合培养物中,对稳定转染子用泌乳激素、地塞米松和催乳素处理2天。虽然泌乳激素协同诱导大鼠β-酪蛋白/CAT表达的强烈激活,但地塞米松和催乳素的单一或联合处理均未诱导牛β-酪蛋白/CAT表达。为了测试泌乳激素对牛β-酪蛋白/CAT表达的序贯处理效果,细胞先用地塞米松或催乳素处理不同天数,然后用两种激素联合处理2天。只有用地塞米松预处理的细胞,而不是用催乳素预处理的细胞,表现出强烈的泌乳诱导。此外,地塞米松预处理细胞的诱导倍数随着地塞米松预处理持续时间的增加而逐渐增加。在经12天地塞米松预处理的培养物中,分析了一系列具有不同长度(从0.3 kb到约15 kb)的牛β-酪蛋白5'侧翼区的牛β-酪蛋白/CAT构建体。即使在含有0.3 kb的构建体中,CAT表达也增加了,但在含有超过1.8 kb的构建体中观察到显著诱导。因此,可以得出结论,长期地塞米松预处理对于牛β-酪蛋白表达调控是必不可少的,0.3 kb的近端启动子区域很重要,但更远端的启动子元件对于介导泌乳激素对牛β-酪蛋白表达的协同作用是必要的。

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