与主要组织相容性复合体I类基因调控元件结合的核蛋白的发育及组织特异性表达。
Developmental and tissue-specific expression of nuclear proteins that bind the regulatory element of the major histocompatibility complex class I gene.
作者信息
Burke P A, Hirschfeld S, Shirayoshi Y, Kasik J W, Hamada K, Appella E, Ozato K
机构信息
Laboratory of Developmental and Molecular Immunity, National Institute of Child Health and Human Development, Bethesda, Maryland 20892.
出版信息
J Exp Med. 1989 Apr 1;169(4):1309-21. doi: 10.1084/jem.169.4.1309.
Expression of MHC class I genes varies according to developmental stage and type of tissues. To study the basis of class I gene regulation in tissues in vivo, we examined binding of nuclear proteins to the conserved cis sequence of the murine H-2 gene, class I regulatory element (CRE), which contains two independent factor-binding sites, region I and region II. In gel mobility shift analyses we found that extracts from adult tissues that express class I genes, such as spleen and liver, had binding activity to region I. In contrast, extracts from brain, which does not express class I genes, did not show region I binding activity. In addition, fetal tissues that express class I gene at very low levels, also did not reveal region I binding activity. Binding activity to region I became detectable during the neonatal period when class I gene expression sharply increases. Most of these tissues showed binding activity to region II, irrespective of class I gene expression. Although region II contained a sequence similar to the AP-1 recognition site, AP-1 was not responsible for the region II binding activity detected in this work. These results illustrate a correlation between region I binding activity and developmental and tissue-specific expression of MHC class I genes. The CRE exerts an enhancer-like activity in cultured fibroblasts. We evaluated the significance of each factor binding to CRE. Single 2-bp mutations were introduced into the CRE by site-directed mutagenesis and the ability of each mutant to elicit the enhancer activity was tested in transient CAT assays. A mutation that eliminated region I protein binding greatly impaired enhancer activity. A mutation that eliminated region II binding also caused a lesser but measurable effect. We conclude that region I and region II are both capable of enhancing transcription of the class I gene. These results indicate that in vivo regulation of MHC class I gene expression is mediated by binding of trans-acting factors to the CRE.
MHC I类基因的表达根据发育阶段和组织类型而有所不同。为了研究体内组织中I类基因调控的基础,我们检测了核蛋白与小鼠H-2基因保守顺式序列(I类调控元件,CRE)的结合,该序列包含两个独立的因子结合位点,即区域I和区域II。在凝胶迁移率变动分析中,我们发现来自表达I类基因的成年组织(如脾脏和肝脏)的提取物对区域I具有结合活性。相比之下,不表达I类基因的脑提取物未显示区域I结合活性。此外,极低水平表达I类基因的胎儿组织也未显示区域I结合活性。当I类基因表达急剧增加的新生儿期,区域I的结合活性开始可检测到。这些组织中的大多数对区域II显示结合活性,与I类基因表达无关。尽管区域II包含一个与AP-1识别位点相似的序列,但AP-1并非本研究中检测到的区域II结合活性的原因。这些结果说明了区域I结合活性与MHC I类基因的发育和组织特异性表达之间的相关性。CRE在培养的成纤维细胞中发挥类似增强子的活性。我们评估了每个因子与CRE结合的重要性。通过定点诱变将单个2-bp突变引入CRE,并在瞬时CAT分析中测试每个突变体引发增强子活性的能力。消除区域I蛋白结合的突变极大地损害了增强子活性。消除区域II结合的突变也产生了较小但可测量的影响。我们得出结论,区域I和区域II都能够增强I类基因的转录。这些结果表明,MHC I类基因表达的体内调控是由反式作用因子与CRE的结合介导的。
Zotero 插件