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The human L1 promoter: Variable transcription initiation sites and a major impact of upstream flanking sequence on promoter activity

机译:人类L1启动子:可变的转录起始位点和上游侧翼序列对启动子活性的重大影响

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摘要

Human L1 elements are non-LTR retrotransposons that comprise ∼17% of the human genome. Their 5′-untranslated region (5′-UTR) serves as a promoter for L1 transcription. Now we find that transcription initiation sites are not restricted to nucleotide +1 but vary considerably in both downstream and upstream directions. Transcription initiating upstream explains additional nucleotides often seen between the 5′-target site duplication and the L1 start site. A higher frequency of G nucleotides observed upstream from the L1 can be explained by reverse transcription of the L1 RNA 5′-CAP, which is further supported by extra Gs seen for full-length HERV-W pseudogenes. We assayed 5′-UTR promoter activities for several full-length human L1 elements, and found that upstream flanking cellular sequences strongly influence the L1 5′-UTR promoter. These sequences either repress or enhance the L1 promoter activity. Therefore, the evolutionary success of a human L1 in producing progeny depends not only on the L1 itself, but also on its genomic integration site. The promoter mechanism of L1 is reminiscent of initiator (Inr) elements that are TATA-less promoters expressing several cellular genes. We suggest that the L1 5′-UTR is able to form an Inr element that reaches into upstream flanking sequence.
机译:人类L1元件是非LTR逆转座子,约占人类基因组的17%。它们的5'非翻译区(5'-UTR)充当L1转录的启动子。现在我们发现转录起始位点不限于核苷酸+1,而是在下游和上游方向上有很大的不同。上游转录起始解释了在5'-靶位点重复和L1起始位点之间经常看到的其他核苷酸。在L1上游观察到的G核苷酸频率更高,可以通过L1 RNA 5'-CAP的反转录来解释,这进一步得到了全长HERV-W假基因所见的额外G的支持。我们分析了几种全长人L1元件的5'-UTR启动子活性,并发现上游侧翼细胞序列强烈影响L1 5'-UTR启动子。这些序列抑制或增强L1启动子活性。因此,人类L1在产生后代方面的进化成功不仅取决于L1本身,还取决于其基因组整合位点。 L1的启动子机制让人联想到启动子(Inr)元素,这些元素是表达几种细胞基因的无TATA启动子。我们建议L1 5'-UTR能够形成一个Inr元素,该元素进入上游侧翼序列。

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