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由一种红系特异性DNA结合因子介导的非缺失型遗传性胎儿血红蛋白持续存在症中γ-珠蛋白表达增加。

Increased gamma-globin expression in a nondeletion HPFH mediated by an erythroid-specific DNA-binding factor.

作者信息

Martin D I, Tsai S F, Orkin S H

机构信息

Division of Hematology-Oncology, Children's Hospital, Boston, Massachusetts.

出版信息

Nature. 1989 Mar 30;338(6214):435-8. doi: 10.1038/338435a0.

Abstract

In man, a shift from gamma- to beta-globin gene expression in erythroblasts underlies a switch from fetal to adult haemoglobin during development. In hereditary persistence of fetal haemoglobin (HPFH), inappropriately high gamma-globin expression in adult life is associated with deletions in the beta-globin cluster or with single-base changes upstream of the gamma-globin genes. To account for enhanced gamma-gene expression in HPFH of the non-deletion type, we tested the nuclear proteins of human erythroleukaemia cells that bind gamma-promoter sequences in vitro by correlating specific mutations in their binding sites with promoter activity. An erythroid-specific factor (GF-1) binds as a single molecule to the -195 to -170 region and contacts two TATCT(AGATA) motifs, but not the conserved octamer (ATGCAAAT) that separates them. We observe that a single change (at -175, T----C) found in HPFH leads to increased promoter activity only in erythroid cells. This effect is mediated by GF-1, the human counterpart of the chicken erythroid factor Eryf 1. The form of HPFH we studied here is an inherited disorder which can be ascribed to the action of a cell-specific DNA-binding factor on a mutant promoter.

摘要

在人类中,成红细胞中从γ-珠蛋白基因表达向β-珠蛋白基因表达的转变是发育过程中从胎儿血红蛋白向成人血红蛋白转变的基础。在胎儿血红蛋白遗传性持续存在(HPFH)中,成人期γ-珠蛋白表达异常升高与β-珠蛋白基因簇的缺失或γ-珠蛋白基因上游的单碱基变化有关。为了解释非缺失型HPFH中γ基因表达增强的原因,我们通过将其结合位点的特定突变与启动子活性相关联,测试了体外结合γ-启动子序列的人类红白血病细胞核蛋白。一种红系特异性因子(GF-1)以单分子形式结合到 -195至-170区域,并与两个TATCT(AGATA)基序接触,但不与分隔它们的保守八聚体(ATGCAAAT)接触。我们观察到在HPFH中发现的一个单一变化(在-175处,T变为C)仅在红系细胞中导致启动子活性增加。这种效应由GF-1介导,它是鸡红系因子Eryf 1的人类对应物。我们在此研究的HPFH形式是一种遗传性疾病,可归因于细胞特异性DNA结合因子对突变启动子的作用。

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