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首页> 外文期刊>Molecular and Cellular Biology >A transcriptional enhancer and an interferon-responsive sequence in major histocompatibility complex class I genes.
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A transcriptional enhancer and an interferon-responsive sequence in major histocompatibility complex class I genes.

机译:主要组织相容性复合体I类基因中的转录增强子和干扰素应答序列。

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The major histocompatibility complex class I antigens play an indispensable role in cell-cell interactions. Perturbation of their expression has been shown to have deleterious physiological consequences, including the escape of transformed cells from immune detection. In an attempt to understand how class I genes are regulated, we dissected the Ld gene to identify potential control regions. By using a test vector containing the simian virus 40 early promoter placed upstream of the bacterial chloramphenicol acetyltransferase (cat) gene, we demonstrated the presence of a transcriptional enhancer within the 5'-flanking region. The sequence is functional in both orientations and has been mapped within 350 base pairs upstream of the Ld transcriptional start site. Although human adenovirus 12 can suppress endogenous class I genes, it cannot down-regulate the activity of the transiently transfected cat gene which has been placed under the control of the Ld enhancer and promoter. Our results suggested that if the human adenovirus 12-induced function regulates the expression of class I genes by a trans mechanism, then its target site must not be within 1.9 kilobases of the 5'-flanking region. Treatment of cells with interferon increases the accumulation of class I transcripts. Expression of the cat gene under the control of the Ld enhancer and promoter also can be up-regulated by interferon. Our study shows that the target sequence required for this enhancement resides, at least in part, within the same 350-base pair segment which contains the transcriptional enhancer.
机译:主要的组织相容性复合物I类抗原在细胞间相互作用中起着不可或缺的作用。已经证明其表达的扰动具有有害的生理学后果,包括从免疫检测中逃脱转化细胞。为了了解I类基因是如何调控的,我们解剖了Ld基因以鉴定潜在的控制区域。通过使用包含猿猴病毒40早期启动子的测试载体,该载体位于细菌氯霉素乙酰转移酶(cat)基因的上游,我们证明了在5'侧翼区域内存在转录增强子。该序列在两个方向上均具有功能,并已被定位在Ld转录起始位点上游的350个碱基对内。尽管人腺病毒12可以抑制内源性I类基因,但它不能下调已经置于Ld增强子和启动子控制下的瞬时转染的cat基因的活性。我们的研究结果表明,如果人类腺病毒12诱导的功能通过反式机制调节I类基因的表达,则其靶位点不得位于5'侧翼区域的1.9公里范围内。用干扰素处理细胞会增加I类转录本的积累。 cat基因在Ld增强子和启动子控制下的表达也可以被干扰素上调。我们的研究表明,这种增强所需的靶序列至少部分位于包含转录增强子的同一350个碱基对的片段内。

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