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鸡βA-珠蛋白基因在转基因小鼠中的位点独立表达。

Site-independent expression of the chicken beta A-globin gene in transgenic mice.

作者信息

Reitman M, Lee E, Westphal H, Felsenfeld G

机构信息

Laboratory of Molecular Biology, National Institute of Diabetes and Digestive and Kidney Diseases, National Institutes of Health, Bethesda, Maryland 20892.

出版信息

Nature. 1990;348(6303):749-52. doi: 10.1038/348749a0.

Abstract

The level of expression of exogenous genes carried by transgenic mice typically varies from mouse to mouse and can be quite low. This behaviour is attributed to the influence of the mouse chromatin near the site of transgene integration. This 'position effect' has been seen in transgenic mice carrying the human beta-globin gene. It was however, abolished when DNase I hypersensitive sites (normally found 65 to 44 kilobases (kb) upstream) were linked to the human beta-globin transgene. Thus, the upstream DNA (previously named a dominant control or locus activation region, now denoted a locus control region) conferred the ability to express human beta-globin at high levels dependent on copy number on every mouse carrying the construct. We report here an investigation of chicken beta A-globin gene expression in transgenic mice. A 4.5-kb fragment carrying the beta A-globin gene and its downstream enhancer, without any far upstream elements, is sufficient to ensure that every transgenic mouse expresses chicken globin messenger RNA at levels proportional to the transgene copy number. Thus the chicken DNA elements that allow position-independent expression can function in mice. In marked contrast to the human beta cluster, these elements are no farther than 2 kb from the gene. The location of the elements within the cluster demonstrates that position independence can be mediated by DNA that does not define a gene cluster boundary.

摘要

转基因小鼠携带的外源基因的表达水平通常因小鼠个体而异,且可能相当低。这种行为归因于转基因整合位点附近小鼠染色质的影响。这种“位置效应”在携带人类β-珠蛋白基因的转基因小鼠中已被观察到。然而,当DNase I超敏位点(通常位于上游65至44千碱基(kb)处)与人类β-珠蛋白转基因相连时,这种效应就被消除了。因此,上游DNA(以前称为显性控制或基因座激活区域,现在称为基因座控制区域)赋予了携带该构建体的每只小鼠根据拷贝数高水平表达人类β-珠蛋白的能力。我们在此报告对转基因小鼠中鸡βA-珠蛋白基因表达的研究。一个携带βA-珠蛋白基因及其下游增强子的4.5-kb片段,没有任何远上游元件,就足以确保每只转基因小鼠以与转基因拷贝数成比例的水平表达鸡珠蛋白信使RNA。因此,允许位置独立表达的鸡DNA元件在小鼠中也能发挥作用。与人类β基因簇形成鲜明对比的是,这些元件距离基因不超过2 kb。基因簇内元件的位置表明,位置独立性可以由不界定基因簇边界的DNA介导。

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