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小鼠铁调节蛋白(IRP)-1和-2基因条件性等位基因的产生。

Generation of conditional alleles of the murine Iron Regulatory Protein (IRP)-1 and -2 genes.

作者信息

Galy Bruno, Ferring Dunja, Hentze Matthias W

机构信息

European Molecular Biology Laboratory, Heidelberg, Germany.

出版信息

Genesis. 2005 Dec;43(4):181-8. doi: 10.1002/gene.20169.

Abstract

Central aspects of cellular iron metabolism are controlled by IRP1 and IRP2, which are ubiquitously expressed in mouse organs and cells. Total and constitutive deficiency of both IRPs causes embryonic lethality in the mouse. To bypass the early lethality and to study organ-specific and/or temporal functions of IRP1 and/or IRP2 we generated Irp1 and Irp2 conditional alleles. We used mouse lines where a betaGeo gene trap construct was inserted into the second intron of the Irp1 and the Irp2 gene, generating hypomorphic alleles by interrupting the corresponding open reading frame near the amino-termini. The gene trap cassettes are flanked by Frt sites and were co-inserted with LoxP sites flanking exon 3. Flp-mediated removal of the gene trap construct generates floxed alleles with wildtype functions. For both Irp genes, Cre-assisted deletion of exon 3 generates complete null alleles that, in the case of IRP2, are associated with altered body iron distribution and compromised hematopoiesis. If not removed, the gene trap construct causes partially penetrant embryonic lethality unrelated to IRP deficiency when inserted within the Irp1 but not the Irp2 locus. We discuss the implications for functional genomics in the mouse.

摘要

细胞铁代谢的核心方面由铁调节蛋白1(IRP1)和铁调节蛋白2(IRP2)控制,它们在小鼠器官和细胞中普遍表达。两种铁调节蛋白的完全和组成型缺陷会导致小鼠胚胎致死。为了绕过早期致死性并研究IRP1和/或IRP2的器官特异性和/或时间性功能,我们构建了Irp1和Irp2条件等位基因。我们使用了将βGeo基因捕获构建体插入Irp1和Irp2基因的第二个内含子中的小鼠品系,通过在氨基末端附近中断相应的开放阅读框产生低表达等位基因。基因捕获盒两侧是Frt位点,并与外显子3两侧的LoxP位点共同插入。Flp介导的基因捕获构建体的去除产生具有野生型功能的floxed等位基因。对于这两个Irp基因,Cre辅助删除外显子3会产生完全无效等位基因,就IRP2而言,这与体内铁分布改变和造血功能受损有关。如果不被去除,当基因捕获构建体插入Irp1位点而非Irp2位点时,会导致与IRP缺陷无关的部分显性胚胎致死。我们讨论了对小鼠功能基因组学的影响。

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