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用于分析不同蛋白质表达程度的细胞群体中亚核蛋白组织的定量方法。

Quantitative methods to analyze subnuclear protein organization in cell populations with varying degrees of protein expression.

作者信息

Voss Ty C, Demarco Ignacio A, Booker Cynthia F, Day Richard N

机构信息

University of Virginia Health Sciences Center, Departments of Medicine and Cell Biology, Charlottesville, Virginia 22908, USA.

出版信息

J Biomed Opt. 2005 Mar-Apr;10(2):024011. doi: 10.1117/1.1891085.

DOI:10.1117/1.1891085
PMID:15910085
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC1201427/
Abstract

The control of gene transcription is dependent on DNA-binding and coregulatory proteins that assemble in distinct regions of the cell nucleus. We use multispectral wide-field microscopy of cells expressing transcriptional coregulators labeled with fluorescent proteins (FP) to study the subnuclear localization and function of these factors in living cells. In coexpression studies, the glucocorticoid receptor interacting protein (GRIP) coactivator protein and the silencing mediator of retinoid and thyroid (SMRT) corepressor protein form spherical subnuclear focal bodies that are spatially distinct, suggesting that specific protein interactions concentrate these divergent proteins in separate subnuclear regions. However, the variability of these subnuclear bodies between cells within the population makes analysis based on "representative images" difficult, if not impossible. To address this issue, we develop a protocol for unbiased selection of cells from the population, followed by the automated quantification of the subnuclear organization of the labeled proteins. Statistical methods identify a significant linear correlation between the FP-coregulator expression level and subnuclear focal body formation for both FP-GRIP and FP-SMRT. Importantly, we confirm that these changes in subnuclear organization could be statistically normalized for differences in coregulator expression level. This integrated quantitative image analysis method will allow the rigorous comparison of different experimental cell populations that express variable levels of FP fusion proteins.

摘要

基因转录的控制取决于在细胞核不同区域组装的DNA结合蛋白和共调节蛋白。我们利用多光谱宽场显微镜对表达用荧光蛋白(FP)标记的转录共调节因子的细胞进行研究,以探讨这些因子在活细胞中的亚核定位和功能。在共表达研究中,糖皮质激素受体相互作用蛋白(GRIP)共激活蛋白和视黄酸及甲状腺沉默介质(SMRT)共抑制蛋白形成了在空间上不同的球形亚核焦点体,这表明特定的蛋白质相互作用将这些不同的蛋白质集中在不同的亚核区域。然而,群体中细胞之间这些亚核体的变异性使得基于“代表性图像”的分析即便不是不可能,也是困难的。为了解决这个问题,我们开发了一种从群体中无偏选择细胞的方案,随后对标记蛋白的亚核组织进行自动定量分析。统计方法确定了FP-GRIP和FP-SMRT的FP-共调节因子表达水平与亚核焦点体形成之间存在显著的线性相关性。重要的是,我们证实这些亚核组织的变化可以针对共调节因子表达水平的差异进行统计学归一化。这种综合定量图像分析方法将允许对表达不同水平FP融合蛋白的不同实验细胞群体进行严格比较。

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2
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3
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