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该运动神经元存活蛋白相互作用组包括 Myb 结合蛋白 1a。

The SMN interactome includes Myb-binding protein 1a.

机构信息

Wolfson Centre for Inherited Neuromuscular Disease, RJAH Orthopaedic Hospital, Oswestry SY10 7AG, United Kingdom.

出版信息

J Proteome Res. 2010 Jan;9(1):556-63. doi: 10.1021/pr900884g.

Abstract

Understanding networks of interacting proteins is a major goal in cell biology. The survival of motor neurons protein (SMN) interacts, directly or indirectly, with a large number of other proteins and reduced levels of SMN cause the inherited disorder spinal muscular atrophy (SMA). Some SMN interactions are stable and stoichiometric, such as those with gemins, while others are expected to be transient and substoichiometric, such as the functional interaction of SMN with coilin in Cajal bodies. This study set out to determine whether novel components of the extensive SMN interactome can be identified by a proteomic approach. SMN complexes were immuno-precipitated from HeLa nuclear extracts, using anti-SMN monoclonal antibody attached to magnetic beads, digested with trypsin, separated by capillary-liquid chromatography and analyzed by MALDI TOF/TOF mass spectrometry. One-hundred and one proteins were detected with a p value of <0.05, SMN, gemins and U snRNPs being the dominant "hits". Sixty-nine of these were rejected after MALDI analysis of two control pull-downs using antibodies against unrelated nuclear proteins. The proteins found only in anti-SMN pulldowns were either known SMN partners, and/or contained dimethylated RG domains involved in direct interaction with the SMN tudor domain, or they were known binding partners of such direct SMN interactors. Myb-binding protein 1a, identified as a novel candidate, is a mainly nucleolar protein of unknown function but it partially colocalized with SMN in Cajal bodies in HeLa cell nucleoplasm and, like SMN, was reduced in cells from an SMA patient.

摘要

理解相互作用的蛋白质网络是细胞生物学的主要目标。运动神经元存活蛋白(SMN)直接或间接地与大量其他蛋白质相互作用,SMN 水平降低会导致遗传性疾病脊髓性肌萎缩症(SMA)。一些 SMN 相互作用是稳定和化学计量的,例如与 gemins 的相互作用,而其他相互作用预计是瞬时和亚化学计量的,例如 SMN 与 Cajal 体中 coilin 的功能相互作用。本研究旨在确定是否可以通过蛋白质组学方法鉴定广泛的 SMN 相互作用组的新成分。使用与磁性珠结合的抗 SMN 单克隆抗体从 HeLa 核提取物中免疫沉淀 SMN 复合物,用胰蛋白酶消化,通过毛细管液相色谱分离,并用 MALDI TOF/TOF 质谱分析。用 p 值 <0.05 检测到 101 种蛋白质,SMN、gemins 和 U snRNPs 是主要的“命中”。在用针对非相关核蛋白的抗体进行的两次对照下拉分析的 MALDI 分析后,有 69 种被拒绝。仅在抗 SMN 下拉中发现的蛋白质要么是已知的 SMN 伴侣,要么含有参与与 SMN 结构域直接相互作用的二甲基化 RG 结构域,要么是这些直接 SMN 相互作用体的已知结合伴侣。Myb 结合蛋白 1a 被鉴定为一种新的候选蛋白,它是一种主要位于核仁的未知功能蛋白,但它在 HeLa 细胞核质的 Cajal 体中与 SMN 部分共定位,并且与 SMN 一样,在来自 SMA 患者的细胞中减少。

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