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作 者:司艺玲[1] 韩为东[1] 赵亚力[1] 李琦[1] 宋海静[1] 于力[2] 母义明[3]
机构地区:[1]解放军总医院基础医学研究所分子生物室,北京100853 [2]解放军总医院血液科,北京100853 [3]解放军总医院内分泌科,北京100853
出 处:《中国生物化学与分子生物学报》2006年第8期627-634,共8页Chinese Journal of Biochemistry and Molecular Biology
基 金:北京市自然科学基金项目资助(No.5052024)~~
摘 要:LRP16是一个明确的雌激素(E2)反应性靶基因,已往研究在LRP16基因上游调控区鉴定了一个E2反应性1/2ERE/GC富含的ERα作用位点(-676bp到-214bp;命名为A区).为进一步鉴定雌激素上调LRP16基因表达的最大化反应区域,对LRP16基因上游调控区进行缺失突变,通过相对荧光素酶活性分析观察到LRP16基因的一段5′近端侧翼序列(-213bp到-24bp;命名为B区)具有明显的E2反应性.通过与A区比较,认为B区最大化的呈递了E2对LRP16基因的转激活效应.序列分析表明,B区缺乏经典的ERE元件,而包含多个富含GC序列.针对Sp1的siRNA实验结果提示,Sp1参与了E2对该区域的转激活.针对GC富含区进一步的缺失突变,及荧光素酶活性分析,识别了一段30bp(-213bp到-184bp)的序列在B区呈递E2反应活性中发挥核心作用.超级凝胶电泳实验结果表明,Sp1蛋白与这段30bp的DNA序列在体外存在直接结合作用.染色质免疫共沉淀实验结果证实,ERα、Sp1与B区存在E2依赖性相互作用.本文在LRP16的5′-侧翼区识别了一段最大化呈递E2活性的DNA片段.机制研究表明,在E2存在条件下,ERα通过Sp1与该区域的直接作用上调LRP16基因的表达.LRP16 gene has been characterized as an estrogen-responsive gene. Previous studies have identified an E2-responsive 1/2ERE/GC-rich site at the 5′-flanking promoter of the LRP16 gene (the - 676 bp to -214 bp region, namely region A). To map the responsive fragment that maximally confer the estrogen transactivation within the 5′-regulatory region of LRP16, deletion analyses were further performed. The results of cotransfection and the luciferase assays showed that the fragment from - 213 bp to - 24 bp (namely region B) gave rise to the maximal responsiveness of E2. Sequence analysis showed that the classical ERE (estrogen response element) was lacked within this region, but six GC-rich sites existing. The results of cotransfection assays combining with Spl-siRNA indicated that Spl protein was required for the responsiveness of region B to estrogen. A 30 bp fragment within region B( - 213 bp to - 184 bp) was identified to be essential for the maximal E2-responsiveness by further deletion and mutation analyses. Gel mobility shift assays showed that the Spl protein can directly bind to this region. The results of ChIP confirmed that cooperative c/Spl interactions at region B were necessary for E2-induced transactivation. Taken together, a minimal DNA fragment of LRP16 gene 5′-flanking region was identified, which was essential for the maximal reponsiveness to estrogen. And the interaction of ligand-bound ERα/Spl complex and DNA fragment involved in this regulatory mechanism.
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