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与脆性X智力低下蛋白(FMRP)相关的RNA货物揭示了Fmr1基因敲除小鼠细胞功能的缺陷。

RNA cargoes associating with FMRP reveal deficits in cellular functioning in Fmr1 null mice.

作者信息

Miyashiro Kevin Y, Beckel-Mitchener Andrea, Purk T Patrick, Becker Kevin G, Barret Tanya, Liu Lei, Carbonetto Salvatore, Weiler Ivan Jeanne, Greenough William T, Eberwine James

机构信息

Department of Pharmacology, Department of Psychiatry, University of Pennsylvania School of Medicine, Philadelphia, PA 19104, USA.

出版信息

Neuron. 2003 Feb 6;37(3):417-31. doi: 10.1016/s0896-6273(03)00034-5.

Abstract

The Fragile X mental retardation-1 (Fmr1) gene encodes a multifunctional protein, FMRP, with intrinsic RNA binding activity. We have developed an approach, antibody-positioned RNA amplification (APRA), to identify the RNA cargoes associated with the in vivo configured FMRP messenger ribonucleoprotein (mRNP) complex. Using APRA as a primary screen, putative FMRP RNA cargoes were assayed for their ability to bind directly to FMRP using traditional methods of assessing RNA-protein interactions, including UV-crosslinking and filter binding assays. Approximately 60% of the APRA-defined mRNAs directly associate with FMRP. By examining a subset of these mRNAs and their encoded proteins in brain tissue from Fmr1 knockout mice, we have observed that some of these cargoes as well as the proteins they encode show discrete changes in abundance and/or differential subcellular distribution. These data are consistent with spatially selective regulation of multiple biological pathways by FMRP.

摘要

脆性X智力低下1(Fmr1)基因编码一种具有内在RNA结合活性的多功能蛋白FMRP。我们开发了一种方法,即抗体定位RNA扩增(APRA),以鉴定与体内组装的FMRP信使核糖核蛋白(mRNP)复合物相关的RNA负载。以APRA作为初步筛选,使用评估RNA-蛋白质相互作用的传统方法,包括紫外线交联和滤膜结合试验,检测推定的FMRP RNA负载直接结合FMRP的能力。约60%由APRA定义的mRNA直接与FMRP相关联。通过检查Fmr1基因敲除小鼠脑组织中这些mRNA及其编码蛋白的一个子集,我们观察到其中一些负载以及它们编码的蛋白在丰度和/或亚细胞分布上显示出离散变化。这些数据与FMRP对多种生物学途径的空间选择性调控一致。

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