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核纤层蛋白A/C的“蛋白质组”:从HeLa细胞中纯化不同的含核纤层蛋白A/C复合物,揭示了其在基因调控、mRNA剪接、信号传导、机械传感和核结构等多种作用中的分子基础。

An emerin "proteome": purification of distinct emerin-containing complexes from HeLa cells suggests molecular basis for diverse roles including gene regulation, mRNA splicing, signaling, mechanosensing, and nuclear architecture.

作者信息

Holaska James M, Wilson Katherine L

机构信息

Department of Cell Biology, The Johns Hopkins University School of Medicine, 725 North Wolfe Street, Baltimore, Maryland 21205, USA.

出版信息

Biochemistry. 2007 Jul 31;46(30):8897-908. doi: 10.1021/bi602636m. Epub 2007 Jul 10.

Abstract

Using recombinant bead-conjugated emerin, we affinity-purified seven proteins from HeLa cell nuclear lysates that bind emerin either directly or indirectly. These proteins were identified by mass spectrometry as nuclear alphaII-spectrin, nonmuscle myosin heavy chain alpha, Lmo7 (a predicted transcription regulator; reported separately), nuclear myosin I, beta-actin (reported separately), calponin 3, and SIKE. We now report that emerin binds nuclear myosin I (NMI, a molecular motor) directly in vitro. Furthermore, bead-conjugated emerin bound nuclear alphaII-spectrin and NMI equally well with or without ATP (which stimulates motor activity), whereas ATP decreased actin binding by 65%. Thus alphaII-spectrin and NMI interact stably with emerin. To investigate the physiological relevance of these interactions, we used antibodies against emerin to affinity-purify emerin-associated protein complexes from HeLa cells and then further purified by ion-exchange chromatography to resolve by net charge and by size exclusion chromatography yielding six distinct emerin-containing fractions (0.5-1.6 MDa). Western blotting suggested that each complex had distinct components involved in nuclear architecture (e.g., NMI, alphaII-spectrin, lamins) or gene or chromatin regulation (BAF, transcription regulators, HDACs). Additional constituents were identified by mass spectrometry. One putative gene-regulatory complex (complex 32) included core components of the nuclear corepressor (NCoR) complex, which mediates gene regulation by thyroid hormone and other nuclear receptors. When expressed in HeLa cells, FLAG-tagged NCoR subunits Gps2, HDAC3, TBLR1, and NCoR each co-immunoprecipitated emerin, validating one putative complex. These findings support the hypothesis that emerin scaffolds a variety of functionally distinct multiprotein complexes at the nuclear envelope in vivo. Notably included are nuclear myosin I-containing complexes that might sense and regulate mechanical tension at the nuclear envelope.

摘要

我们使用重组珠偶联emerin,从HeLa细胞核裂解物中亲和纯化出七种直接或间接结合emerin的蛋白质。通过质谱鉴定,这些蛋白质为核αII-血影蛋白、非肌肉肌球蛋白重链α、Lmo7(一种预测的转录调节因子,已单独报道)、核肌球蛋白I、β-肌动蛋白(已单独报道)、钙调蛋白3和SIKE。我们现在报告,emerin在体外直接结合核肌球蛋白I(NMI,一种分子马达)。此外,无论有无ATP(ATP可刺激马达活性),珠偶联emerin与核αII-血影蛋白和NMI的结合效果相同,而ATP使肌动蛋白结合减少65%。因此,αII-血影蛋白和NMI与emerin稳定相互作用。为了研究这些相互作用的生理相关性,我们使用抗emerin抗体从HeLa细胞中亲和纯化emerin相关蛋白复合物,然后通过离子交换色谱进一步纯化,以根据净电荷分离,并通过尺寸排阻色谱得到六个不同的含emerin组分(0.5 - 1.6 MDa)。蛋白质印迹法表明,每个复合物都有参与核结构(如NMI、αII-血影蛋白、核纤层蛋白)或基因或染色质调控(BAF、转录调节因子、组蛋白去乙酰化酶)的不同成分。通过质谱鉴定出了其他成分。一个假定的基因调控复合物(复合物32)包括核共抑制因子(NCoR)复合物的核心成分,该复合物介导甲状腺激素和其他核受体的基因调控。当在HeLa细胞中表达时,FLAG标记的NCoR亚基Gps2、HDAC3、TBLR1和NCoR各自与emerin共免疫沉淀,验证了一个假定的复合物。这些发现支持了emerin在体内核膜上构建多种功能不同的多蛋白复合物的假说。特别值得注意的是包含核肌球蛋白I的复合物,它们可能感知并调节核膜处的机械张力。

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