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Analysis of Proteasome-Dependent Proteolysis in Haloferax volcanii Cells, Using Short-Lived Green Fluorescent Proteins†

机译:使用短寿命的绿色荧光蛋白分析火山嗜盐杆菌细胞中蛋白酶体依赖性蛋白水解†

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摘要

Proteasomes are energy-dependent proteases that are central to the quality control and regulated turnover of proteins in eukaryotic cells. Dissection of this proteolytic pathway in archaea, however, has been hampered by the lack of substrates that are easily detected in whole cells. In the present study, we developed a convenient reporter system by functional expression of a green fluorescent protein variant with C-terminal fusions in the haloarchaeon Haloferax volcanii. The levels of this reporter protein correlated with whole-cell fluorescence that was readily detected in culture. Accumulation of the reporter protein was dependent on the sequence of the C-terminal amino acid fusion, as well as the presence of an irreversible, proteasome-specific inhibitor (clasto-lactacystin β-lactone). This inhibitor was highly specific for H. volcanii 20S proteasomes, with a Ki of ∼40 nM. In contrast, phenylmethanesulfonyl fluoride did not influence the levels of fluorescent reporter protein or inhibit 20S proteasomes. Together, these findings provide a powerful tool for the elucidation of protein substrate recognition motifs and the identification of new genes which may be involved in the proteasome pathway of archaea.
机译:蛋白酶体是能量依赖型蛋白酶,对于真核细胞中蛋白质的质量控制和调节周转至关重要。但是,由于缺乏在整个细胞中容易检测到的底物,因此在古细菌中解剖该蛋白水解途径受到了阻碍。在本研究中,我们通过在卤代古细菌Haloferax volcanii中具有C端融合的绿色荧光蛋白变体功能性表达,开发了一种便捷的报告系统。该报道蛋白的水平与在培养中容易检测到的全细胞荧光相关。报告蛋白的积累取决于C端氨基酸融合序列,以及不可逆的蛋白酶体特异性抑制剂(clasto-lactacystinβ-lactone)的存在。该抑制剂对火山嗜血杆菌20S蛋白酶体具有高度特异性,Ki约为40 nM。相反,苯基甲磺酰氟不影响荧光报告蛋白的水平或抑制20S蛋白酶体。总之,这些发现为阐明蛋白质底物识别基序和鉴定可能与古细菌蛋白酶体途径有关的新基因提供了有力工具。

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