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一种用于快速筛选解旋酶调节剂的计算机模拟和体外实验流程。

An in silico and in vitro pipeline for the rapid screening of helicase modulators.

作者信息

Papakonstantinou Eleni, Bacopoulou Flora, Megalooikonomou Vasileios, Efthimiadou Aspasia, Vlachakis Dimitrios

机构信息

Laboratory of Genetics, Department of Biotechnology, School of Food, Biotechnology and Development, Agricultural University of Athens, Athens, Greece.

Lab of Molecular Endocrinology, Center of Clinical, Experimental Surgery and Translational Research, Biomedical Research Foundation of the Academy of Athens, Athens, Greece.

出版信息

EMBnet J. 2020;25. doi: 10.14806/ej.25.0.927. Epub 2020 Feb 13.

Abstract

To evaluate the potency of potential helicase modulators, we developed an assay of helicase enzyme activity. Using a DNA or RNA biotin labelled oligonucleotide and after the addition of a recombinant helicase, the nucleic acid unwinds, causing the emission of luminescence, which is quantified with a particular antibody. In our assay, one of the DNA oligos was biotinylated, while the other was labelled with digoxygenin (DIG), both in their 5' termini. The biotin molecule immobilises the DNA duplex on a neutravidin-coated plate and the helicase activity is measured through the unwinding of DNA, due to ATP activation. The subsequent release of DIG-labelled oligos results in a luminescence signal measured with a chemiluminescence antibody. Our goal was to provide a high throughput screening method for potential helicase inhibitors. The method described in this paper has been demonstrated to be fast, easy and reproducible and doesn't use radiochemicals.

摘要

为了评估潜在解旋酶调节剂的效力,我们开发了一种解旋酶酶活性测定方法。使用DNA或RNA生物素标记的寡核苷酸,加入重组解旋酶后,核酸解旋,导致发光,用特定抗体进行定量。在我们的测定中,其中一条DNA寡核苷酸在其5'末端进行了生物素化,而另一条则用洋地黄毒苷(DIG)标记。生物素分子将DNA双链固定在中性抗生物素蛋白包被的板上,通过ATP激活导致的DNA解旋来测量解旋酶活性。随后释放的DIG标记寡核苷酸会产生用化学发光抗体测量的发光信号。我们的目标是为潜在的解旋酶抑制剂提供一种高通量筛选方法。本文所述方法已被证明快速、简便且可重复,并且不使用放射性化学物质。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/0426/7079759/de75c52f3f05/nihms-1562337-f0001.jpg

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