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Novel Fluorescently-labeled Enzyme Substrates for the Sensitive Detection of HIV-protease

机译:用于敏感检测的艾滋病毒蛋白酶的新型荧光标记的酶底物

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In this paper we applied the efficient fluorescence quenching of the red-absorbing oxazine derivative MR121 by the amino acid tryptophan to develop a new fluorescence based enzyme assay that can be used for detection of exopeptidases and endopeptidases. Therefore, we developed peptide substrates labeled with only one chromophore, which is quenched by a neighbored tryptophan residue via photoinduced electron transfer. The specific cleavage site for the target enzyme is located between the chromophore and the tryptophan residue. After digestion of the substrate the contact formation between tryptophan and fluorescent dye is precluded and a significant increase in fluorescence intensity occurs. To demonstrate the new assay technique for exopeptidases, a substrate for the Carboxypeptidase A was designed and a detection limit below the picomolar range (~10-13 M) was achieved with standard fluorescence spectrometry. The primary objective was the detection of the HIV-protease, which is an endopeptidase digesting substrates containing seven specific amino acids in the cleavage site. We designed a substrate, which enables the detection of 10-9 M HIVprotease, whereas the continuous monitoring of the fluorescence signal also allows kinetic studies.
机译:在本文中,我们通过氨基酸色氨酸施加了红色吸收的恶唑衍生物MR121的有效荧光猝灭,以开发一种新的荧光基酶测定,其可用于检测外肽酶和内肽酶。因此,我们开发了仅用一种发色团标记的肽底物,其通过光致电子转移通过相邻的色氨酸残基淬灭。靶酶的特异性切割位点位于发色团和色氨酸残余物之间。在消化基质后,含有色氨酸和荧光染料之间的接触形成,发生荧光强度的显着增加。为了证明用于外部肽酶的新测定技术,设计了用于羧肽酶A的基材,并通过标准荧光光谱法实现了低于PICOMOLAR范围(〜10-13M)的检测极限。主要目的是检测艾滋病毒蛋白酶,其是含有七种特异性氨基酸的内肽酶消化底物。我们设计了一种基板,其能够检测10-9米的毛明酶,而对荧光信号的连续监测也可以允许动力学研究。

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