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评价炔基修饰的异戊二烯作为蛋白质类异戊二烯化的化学报告物。

Evaluation of alkyne-modified isoprenoids as chemical reporters of protein prenylation.

机构信息

Department of Chemistry, University of Minnesota, Minneapolis, MN 55455, USA.

出版信息

Chem Biol Drug Des. 2010 Dec;76(6):460-71. doi: 10.1111/j.1747-0285.2010.01037.x. Epub 2010 Oct 11.

Abstract

Protein prenyltransferases catalyze the attachment of C15 (farnesyl) and C20 (geranylgeranyl) groups to proteins at specific sequences localized at or near the C-termini of specific proteins. Determination of the specific protein prenyltransferase substrates affected by the inhibition of these enzymes is critical for enhancing knowledge of the mechanism of such potential drugs. Here, we investigate the utility of alkyne-containing isoprenoid analogs for chemical proteomics experiments by showing that these compounds readily penetrate mammalian cells in culture and become incorporated into proteins that are normally prenylated. Derivatization via Cu(I) catalyzed click reaction with a fluorescent azide reagent allows the proteins to be visualized and their relative levels to be analyzed. Simultaneous treatment of cells with these probes and inhibitors of prenylation reveals decreases in the levels of some but not all of the labeled proteins. Two-dimensional electrophoretic separation of these labeled proteins followed by mass spectrometric analysis allowed several labeled proteins to be unambiguously identified. Docking experiments and density functional theory calculations suggest that the substrate specificity of protein farnesyl transferase may vary depending on whether azide- or alkyne-based isoprenoid analogs is employed. These results demonstrate the utility of alkyne-containing analogs for chemical proteomic applications.

摘要

蛋白质 prenyltransferases 催化 C15(法呢基)和 C20(香叶基)基团在特定蛋白质的 C 末端或附近的特定序列处附着到蛋白质上。确定受这些酶抑制影响的特定蛋白质 prenyltransferase 底物对于增强对这些潜在药物机制的了解至关重要。在这里,我们通过表明这些化合物容易穿透培养中的哺乳动物细胞并整合到正常 prenylated 的蛋白质中,研究了炔烃包含的类异戊二烯类似物在化学蛋白质组学实验中的用途。通过 Cu(I) 催化的点击反应与荧光叠氮试剂进行衍生化,允许可视化蛋白质并分析其相对水平。同时用这些探针和 prenylation 抑制剂处理细胞会导致一些但不是所有标记蛋白质的水平降低。对这些标记的蛋白质进行二维电泳分离,然后进行质谱分析,可以明确鉴定出几种标记的蛋白质。对接实验和密度泛函理论计算表明,蛋白质法尼基转移酶的底物特异性可能取决于是否使用叠氮化物或炔烃类异戊二烯类似物。这些结果表明炔烃类包含的类似物在化学蛋白质组学应用中的有用性。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/78b4/3058306/b37be6e30b42/nihms238263f1.jpg

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