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小鼠β-珠蛋白基因附近与潜在Z-DNA区域相关的负调控序列。

A negative regulatory sequence near the mouse beta-maj globin gene associated with a region of potential Z-DNA.

作者信息

Gilmour R S, Spandidos D A, Vass J K, Gow J W, Paul J

出版信息

EMBO J. 1984 Jun;3(6):1263-72. doi: 10.1002/j.1460-2075.1984.tb01961.x.

Abstract

The possible regulatory role of DNA sequences situated 5' to the beta-maj globin gene was investigated by two types of assay. First, a long term transformation assay was used to measure the efficiency of transformation of TK- mouse (LATK-) and hamster (BHKTK-) fibroblast cells with DNA molecules made by covalently linking mouse and human DNA fragments to the herpes simplex virus (HSV-1) thymidine kinase (tk) gene in the plasmid pTK1. When the promoter regions from the mouse beta-maj globin or the human epsilon-globin genes are substituted for the viral promoter in the tk gene transformation occurs with 10-20% of the efficiency of the original plasmid. A fragment (H1), containing sequences between 344 and 1413 bp upstream from the mouse beta-maj globin cap site, almost completely abolishes transformation when inserted next to hybrid tk genes containing the mouse beta-globin or human epsilon-globin promoter but has no effect on the intact tk gene. The effect can be demonstrated with the H1 fragment in either orientation relative to the tk gene. Secondly, in transient expression assays the H1 fragment strongly inhibits transcription when covalently linked to the tk gene under control of either globin promoter, but not when linked to the tk gene with its own promoter. The H1 fragment contains 53 bp of purine-pyrimidine alternation (ACAT)n as part of a larger region potentially capable of adopting a Z-DNA conformation.

摘要

通过两种检测方法研究了位于β-珠蛋白基因5'端的DNA序列可能的调控作用。首先,使用长期转化检测法来测量用通过将小鼠和人类DNA片段共价连接到质粒pTK1中的单纯疱疹病毒(HSV-1)胸苷激酶(tk)基因而制成的DNA分子对TK-小鼠(LATK-)和仓鼠(BHKTK-)成纤维细胞进行转化的效率。当用小鼠β-珠蛋白或人类ε-珠蛋白基因的启动子区域替代tk基因中的病毒启动子时,转化效率为原始质粒的10-20%。一个片段(H1),包含小鼠β-珠蛋白帽位点上游344至1413 bp之间的序列,当插入到含有小鼠β-珠蛋白或人类ε-珠蛋白启动子的杂交tk基因旁边时,几乎完全消除了转化,但对完整的tk基因没有影响。无论H1片段相对于tk基因的方向如何,都可以证明这种效果。其次,在瞬时表达检测中,当H1片段与任何一种珠蛋白启动子控制下的tk基因共价连接时,它会强烈抑制转录,但与带有自身启动子的tk基因连接时则不会。H1片段包含53 bp的嘌呤-嘧啶交替序列(ACAT)n,这是一个更大区域的一部分,该区域可能能够形成Z-DNA构象。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/bcd9/557507/4f4606d839b0/emboj00310-0058-a.jpg

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