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鉴定出人类嗜T淋巴细胞病毒I型(HTLV-I)长末端重复序列中负责最大基因表达的两个不同元件。

Identification of two distinct elements in the long terminal repeat of HTLV-I responsible for maximum gene expression.

作者信息

Ohtani K, Nakamura M, Saito S, Noda T, Ito Y, Sugamura K, Hinuma Y

出版信息

EMBO J. 1987 Feb;6(2):389-95. doi: 10.1002/j.1460-2075.1987.tb04767.x.

Abstract

Human T-cell leukemia virus type I has a unique sequence, pX, between env and the 3' long terminal repeat (LTR). One of its products, p40, activates gene expression directed by the LTR in a trans-acting manner. We have analysed the mechanism of this trans-activation mediated by p40 in human T cells co-transfected with a plasmid expressing p40 using the transient CAT gene expression. We identified two distinct elements in the LTR which are involved in maximum gene expression. The first was present in a 230-bp fragment upstream from TATA box in the U3 region and behaved as a classical enhancer. This region was also shown to be responsible for trans-activation by p40. This element alone together with functional p40 could direct the gene expression at only approximately 10% of the level achieved by the complete LTR and p40. The second element was present within a 300-bp fragment downstream from the RNA start site and profoundly enhanced the gene expression in a way independent from trans-activation mechanism. This enhancement was observed only when the element was located immediately downstream from the RNA start site without orientation preference. These two elements participate independently in the enhancement of gene expression.

摘要

人类I型T细胞白血病病毒在env基因和3'长末端重复序列(LTR)之间有一个独特的序列pX。其产物之一p40以反式作用方式激活由LTR指导的基因表达。我们利用瞬时CAT基因表达分析了在与表达p40的质粒共转染的人T细胞中,由p40介导的这种反式激活的机制。我们在LTR中鉴定出两个不同的元件,它们参与最大程度的基因表达。第一个元件存在于U3区域中TATA框上游的一个230 bp片段中,表现为一个典型的增强子。该区域也被证明是p40反式激活所必需的。单独这个元件与功能性p40一起只能指导基因表达达到完整LTR和p40所实现水平的约10%。第二个元件存在于RNA起始位点下游的一个300 bp片段内,以一种独立于反式激活机制的方式显著增强基因表达。只有当该元件位于RNA起始位点紧邻下游且无方向偏好时,才观察到这种增强作用。这两个元件独立参与基因表达的增强。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/1eda/553408/f67ce412ba5e/emboj00242-0106-a.jpg

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