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AlphaScreen技术在高通量筛选中的应用:现状

The use of AlphaScreen technology in HTS: current status.

作者信息

Eglen Richard M, Reisine Terry, Roby Philippe, Rouleau Nathalie, Illy Chantal, Bossé Roger, Bielefeld Martina

机构信息

President, Molecular Medicine, PerkinElmer Life and Analytical Sciences, 940 Winter St., Waltham, MA 02451-1457, USA.

出版信息

Curr Chem Genomics. 2008 Feb 25;1:2-10. doi: 10.2174/1875397300801010002.

Abstract

AlphaScreen (Amplified Luminescent Proximity Homogeneous Assay Screen) is versatile assay technology developed to measuring analytes using a homogenous protocol. This technology is an example of a bead-based proximity assay and was developed from a diagnostic assay technology known as LOCI (Luminescent Oxygen Channeling Assay). Here, singlet oxygen molecules, generated by high energy irradiation of Donor beads, travel over a constrained distance (approx. 200 nm) to Acceptor beads. This results in excitation of a cascading series of chemical reactions, ultimately causing generation of a chemiluminescent signal.In the past decade, a wide variety of applications has been reported, ranging from detection of analytes involved in cell signaling, including protein:protein, protein:peptide, protein:small molecule or peptide:peptide interactions. Numerous homogeneous HTS-optimized assays have been reported using the approach, including generation of second messengers (such as accumulation of cyclic AMP, cyclic GMP, inositol [1, 4, 5] trisphosphate or phosphorylated ERK) from liganded GPCRs or tyrosine kinase receptors, post-translational modification of proteins (such as proteolytic cleavage, phosphorylation, ubiquination and sumoylation) as well as protein-protein and protein-nucleic acid interactions.Recently, the basic AlphaScreen technology was extended in that the chemistry of the Acceptor bead was modified such that emitted light is more intense and spectrally defined, thereby markedly reducing interference from biological fluid matrices (such as trace hemolysis in serum and plasma). In this format, referred to as AlphaLISA, it provides an alternative technology to classical ELISA assays and is suitable for high throughput automated fluid dispensing and detection systems.Collectively, AlphaScreen and AlphaLISA technologies provide a facile assay platform with which one can quantitate complex cellular processes using simple no-wash microtiter plate based assays. They provide the means by which large compound libraries can be screened in a high throughput fashion at a diverse range of therapeutically important targets, often not readily undertaken using other homogeneous assay technologies. This review assesses the current status of the technology in drug discovery, in general, and high throughput screening (HTS), in particular.

摘要

阿尔法筛选技术(放大发光邻近均相分析筛选技术)是一种通用的分析技术,旨在通过均相检测方法来测量分析物。该技术是基于微珠的邻近分析技术的一个实例,它由一种名为LOCI(发光氧通道分析)的诊断分析技术发展而来。在此技术中,供体微珠经高能辐射产生的单线态氧分子会在有限的距离(约200纳米)内传输至受体微珠。这会引发一系列级联化学反应的激发,最终导致化学发光信号的产生。在过去十年中,已报道了各种各样的应用,范围涵盖参与细胞信号传导的分析物检测,包括蛋白质:蛋白质、蛋白质:肽、蛋白质:小分子或肽:肽相互作用。使用该方法已报道了许多均相高通量筛选(HTS)优化分析,包括从配体结合的GPCR或酪氨酸激酶受体生成第二信使(如环磷酸腺苷、环磷酸鸟苷、肌醇[1,4,5]三磷酸或磷酸化细胞外信号调节激酶的积累)、蛋白质的翻译后修饰(如蛋白水解切割、磷酸化、泛素化和类泛素化)以及蛋白质 - 蛋白质和蛋白质 - 核酸相互作用。最近,基本的阿尔法筛选技术得到了扩展,受体微珠的化学性质经过修饰,使得发射光更强且光谱更明确,从而显著减少生物流体基质(如血清和血浆中的微量溶血)的干扰。以这种形式,即阿尔法丽莎技术,它为传统酶联免疫吸附测定(ELISA)分析提供了一种替代技术,适用于高通量自动化液体分配和检测系统。总体而言,阿尔法筛选技术和阿尔法丽莎技术提供了一个便捷的分析平台,利用基于简单无需洗涤的微孔板分析,人们可以对复杂的细胞过程进行定量分析。它们提供了一种手段,通过这种手段可以以高通量方式在各种具有重要治疗意义的靶点上筛选大型化合物库,而这些靶点通常难以使用其他均相分析技术进行研究。本综述评估了该技术在药物发现,特别是高通量筛选(HTS)方面的当前状况。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/ff4e/2775125/8b3be4d7e6fb/TOCHGENJ-1-2_F1.jpg

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