共查询到20条相似文献,搜索用时 15 毫秒
1.
A Zarain-Herzberg D H MacLennan M Periasamy 《The Journal of biological chemistry》1990,265(8):4670-4677
2.
Expression and regulation of immunoglobulin heavy chain gene transfected into lymphoid cells 总被引:119,自引:44,他引:75
下载免费PDF全文
![点击此处可从《The EMBO journal》网站下载免费的PDF全文](/ch/ext_images/free.gif)
Neuberger MS 《The EMBO journal》1983,2(8):1373-1378
3.
4.
5.
6.
7.
8.
9.
10.
11.
12.
13.
Expression of the sulfonamide resistance gene from plasmid R46 总被引:5,自引:0,他引:5
14.
Inducible DNA-protein interactions of the murine kappa immunoglobulin enhancer in intact cells: comparison with in vitro interactions. 总被引:6,自引:4,他引:2
下载免费PDF全文
![点击此处可从《Nucleic acids research》网站下载免费的PDF全文](/ch/ext_images/free.gif)
R Hromas U Pauli A Marcuzzi D Lafrenz H Nick J Stein G Stein B Van Ness 《Nucleic acids research》1988,16(3):953-967
The large intron of the kappa immunoglobulin gene contains a cis-acting enhancer element, which is important in the tissue-specific expression of the gene. We have confirmed the binding activity of a sequence-specific factor present in lymphoid extracts derived from cell lines expressing, or induced to express, the kappa gene. We have extended these studies to show the binding activity is present in normal activated splenic B cells as well as lambda producing cells, and have demonstrated by DNAse footprint analysis full protection of a sequence containing the 11 bp homology to the SV-40 core enhancer. We have compared these in vitro binding studies with an analysis of protein-DNA interactions in intact murine cell lines using genomic sequencing techniques. We demonstrate significant alterations in DMS reactivity of DNA in the murine 70Z/3 cell line after it is induced to kappa expression. These alterations occur at guanine residues which are part of the the 11 bp core sequence, and are identical to those observed in cells constitutively expressing kappa. This provides direct evidence for the induced binding of the tissue specific factor to intact chromatin. In intact chromatin we also observed significant alteration in the reactivity of a guanine, 3' of the core sequence, which is part of a potential secondary DNA structure, and protection of four residues that are part of a region homologous to the heavy chain enhancer. 相似文献
15.
16.
17.
18.
19.
目的:克隆端粒、端粒酶结合因子hPinx1基因的启动子,分析并鉴定其活性调控元件。方法:采用PCR技术从人肝癌细胞系HepG2基因组中扩增出hPinx1启动子,构建到萤光素酶报告基因载体pGL3-basic中,确定所扩增的DNA序列,在HepG2细胞中检测其活性。结果:克隆了hPinx1基因转录起始位点上游4661bp且序列正确;活性分析表明hPinx1启动子含有多个调控元件,其中核心序列位于530bp内,在1329-2174bp间存在正调控序列,在2174-4661 bp间存在负调控序列。结论:构建的hPinx1启动子具有活性,为hPinx1的功能研究提供了重要基础。 相似文献