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一种基于细胞的高通量高斯荧光素酶报告基因检测方法,用于鉴定纤连蛋白-3分泌的调节剂。

A high-throughput cell-based Gaussia luciferase reporter assay for identifying modulators of fibulin-3 secretion.

作者信息

Hulleman John D, Brown Steven J, Rosen Hugh, Kelly Jeffery W

机构信息

Department of Chemistry and the Skaggs Institute for Chemical Biology, The Scripps Research Institute, La Jolla, CA, USA.

出版信息

J Biomol Screen. 2013 Jul;18(6):647-58. doi: 10.1177/1087057112469405. Epub 2012 Dec 10.

Abstract

An R345W mutation in fibulin-3 causes its inefficient secretion, increased intracellular steady-state levels, and the macular dystrophy, Malattia Leventinese (ML), a disease similar to age-related macular degeneration. It is unknown whether R345W causes ML through increased intracellular levels, by the secretion of a potentially aggregation-prone protein, or both. To identify small molecules that alter the secretion of fibulin-3, we developed ARPE19 retinal cell lines that inducibly express wild-type (WT) or R345W fibulin-3 fused to an enhanced Gaussia luciferase (eGLuc2). Screening of the Library of Pharmacologically Active Compounds demonstrated that these cell lines and the GLuc assay are suitable for high-throughput chemical screening. Two estrogen-related compounds enhanced fibulin-3 secretion, whereas a diverse series of small molecules reduced fibulin-3 secretion. A counterscreen identified compounds that did not substantially alter the secretion of unfused eGLuc2, demonstrating at least partial selectivity for fibulin-3. A secondary assay using untagged fibulin-3 confirmed that the top three inhibitory compounds reduced R345W fibulin-3 secretion. Interestingly, in untagged fibulin-3 studies, one compound, phorbol 12-myristate 13-acetate, reduced R345W fibulin-3 secretion while minimally enhancing WT fibulin-3 secretion, the desired activity and selectivity we sought for ML. The identified compounds could serve as tools for probing the etiology of fibulin-3-related diseases.

摘要

纤连蛋白-3中的R345W突变导致其分泌效率低下、细胞内稳态水平升高,并引发黄斑营养不良,即莱文廷斯黄斑病变(ML),这是一种与年龄相关性黄斑变性相似的疾病。尚不清楚R345W是通过增加细胞内水平、分泌潜在易聚集蛋白还是两者兼而有之来导致ML。为了鉴定改变纤连蛋白-3分泌的小分子,我们构建了ARPE19视网膜细胞系,该细胞系可诱导表达与增强型高斯荧光素酶(eGLuc2)融合的野生型(WT)或R345W纤连蛋白-3。对药理活性化合物库的筛选表明,这些细胞系和GLuc检测方法适用于高通量化学筛选。两种雌激素相关化合物增强了纤连蛋白-3的分泌,而一系列不同的小分子则降低了纤连蛋白-3的分泌。一项反筛选鉴定出了对未融合的eGLuc2分泌没有实质性影响的化合物,这表明对纤连蛋白-3至少具有部分选择性。使用未标记的纤连蛋白-3进行的二次检测证实,排名前三的抑制性化合物降低了R345W纤连蛋白-3的分泌。有趣的是,在未标记的纤连蛋白-3研究中,一种化合物,佛波醇12-肉豆蔻酸酯13-乙酸酯,降低了R345W纤连蛋白-3的分泌,同时对WT纤连蛋白-3的分泌增强作用最小,这正是我们针对ML所寻求的理想活性和选择性。所鉴定的化合物可作为探究纤连蛋白-3相关疾病病因的工具。

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