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Ligand binding studies by high speed centrifugal precipitation and linear spectral summation using ultraviolet–visible absorption spectroscopy

机译：配体结合研究通过高速离心沉淀和紫外可见吸收光谱法进行的线性光谱求和

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class="kwd-title">Method name: Linear spectral summation and high speed centrifugal separation for UV–Vis absorption spectroscopy class="kwd-title">Keywords: LCN1, Lipocalin1, Lipocalins, Insoluble ligands, Lipid interactions, Protein-lipid binding complexes, Spectral analysis class="head no_bottom_margin" id="abs0010title">AbstractIn ligand-protein binding experiments the major challenge is to separate bound from free ligand. Equilibrium and gel filtration separation techniques are often hampered by competition for the ligand and non-specific binding. Biophysical assays have attempted to circumvent this problem using titration calorimetry and spectroscopic methods. However, insoluble ligands require solvents that can overwhelm the discernible enthalpic changes of the protein and ligands. Spectroscopic methods are effective but may suffer from insensitivity (NMR) or the need for a lipid analog e.g., fluorescence and electron paramagnetic resonance. Our purpose is to compare the standard fluorescence assay to a technique we call high speed centrifugal precipitation. High speed centrifugal precipitation is suited to ligands that are insoluble in aqueous. The method permits separation of insoluble free ligand from that bound to the protein. The concentration of the each fraction can be precisely measured by absorbance spectrophotometry.A second technique, linear spectral summation has been published for protein-ligand associations using fluorescence of labeled ligands []. Here, the method is altered for use with ultraviolet-visible (UV–Vis) absorption spectroscopy. If the ligand complex shows a shift in the peak absorption of >8 nm, the bound and free concentrations can be measured simultaneously. The composite spectra of the samples are fit by linearly scaling UV–Vis absorption spectra of pure bound and free components at each point. class="first-line-outdent" id="lis0005">

• Ligand- protein binding kinetics is accessible with an ordinary spectrophotometer.

• Concentrations are accurately measured from molar extinction coefficients.

• The methods are ideal for lipid ligands that show absorption spectral peaks shifts in the bound and free states and/or are insoluble.

机译：<！-fig ft0-> <！-fig @ position =“ anchor” mode =文章f4-> <！-fig mode =“ anchred” f5-> <！-fig / graphic | fig / alternatives / graphic mode =“ anchored” m1-> class =“ kwd-title”>方法名称：用于UV-Vis吸收光谱的线性光谱求和和高速离心分离 class =“ kwd -title“>关键字： LCN1，Lipocalin1，Lipocalins，不溶性配体，脂质相互作用，蛋白质-脂质结合复合物，光谱分析 class =” head no_bottom_margin“ id =” abs0010title“>摘要在配体-蛋白质结合实验的主要挑战是将结合与游离配体分开。平衡和凝胶过滤分离技术通常会因竞争配体和非特异性结合而受阻。生物物理测定法已经尝试使用滴定量热法和光谱法来解决该问题。但是，不溶性配体需要能够压倒蛋白质和配体的明显焓变的溶剂。光谱方法是有效的，但是可能会受到不敏感性（NMR）或对脂质类似物例如荧光和电子顺磁共振的需求。我们的目的是将标准荧光测定与我们称为高速离心沉淀的技术进行比较。高速离心沉淀适用于不溶于水的配体。该方法允许将不溶性游离配体从与蛋白质结合的游离配体中分离出来。各个部分的浓度可以通过吸收分光光度法精确测量。第二种技术是使用标记的配体的荧光技术对蛋白质-配体缔合进行线性光谱求和。在这里，该方法已更改为可用于紫外可见（UV-Vis）吸收光谱法。如果配体络合物的峰值吸收峰位移大于8nm，则可以同时测量结合浓度和游离浓度。通过线性缩放每个点上纯结合和自由组分的UV-Vis吸收光谱，可以拟合样品的复合光谱。 class =“ first-line-outdent” id =“ lis0005”> <！-列表行为= simple prefix-word = mark-type = none max-label-size = 9->

•普通蛋白质的分光光度计可检测配体-蛋白的结合动力学。

•浓度是根据摩尔消光系数精确测量的。

•该方法对于脂质配体而言是理想的，这些脂质配体在结合态和自由态中显示吸收光谱峰位移和/或不溶的。

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期刊名称 MethodsX
作者
Ben J. Glasgow; Adil R. Abduragimov;
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作者单位

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年(卷),期 2018(5),-1
年度 2018
页码 345–351
总页数 7
原文格式 PDF
正文语种
中图分类
关键词
LCN1 Lipocalin1 Lipocalins Insoluble ligands Lipid interactions Protein-lipid binding complexes Spectral analysis;

机译：LCN1;Lipocalin1;Lipocalins;不溶性配体;脂质相互作用;蛋白质-脂质结合复合物;光谱分析;

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专利

1. Ligand binding studies by high speed centrifugal precipitation and linear spectral summation using ultraviolet–visible absorption spectroscopy [J] . Ben J. Glasgow, Adil R. Abduragimov MethodsX . 2018,第1期

机译：使用紫外线可见吸收光谱通过高速离心沉淀和线性光谱求和的配体结合研究
2. A Simple Model-Free Method for Direct Assessment of Fluorescent Ligand Binding by Linear Spectral Summation [J] . Oktay K. Gasymov, Adil R. Abduragimov, Ben J. Glasgow Journal of Fluorescence . 2014,第1期

机译：通过线性光谱求和直接评估荧光配体结合的简单无模型方法
3. Study on the Interaction between CdSe Quantum Dots and Bovine Serum Albumin with Ultraviolet Visible Absorption Spectroscopy [J] . He You HAN, De Hong HU, Jian Gong LIANG, 中国化学快报（英文版） . 2006,第007期

机译：紫外可见吸收光谱法研究CdSe量子点与牛血清白蛋白的相互作用
4. Absorption spectroscopy in the ultraviolet and visible spectral range of hexavalent chromium aqueous solutions [C] . Anna G. Mignani, IROE-CNR, Firenze, Environmental Sensing and Applications . 1999

机译：六价铬水溶液在紫外和可见光谱范围内的吸收光谱
5. Towards the understanding of binding environments of metals bound to hematite nanoparticles and redox active ligands using X-ray absorption spectroscopy [D] . Werellapatha, Kalpani. 2016

机译：使用X射线吸收光谱法了解与赤铁矿纳米颗粒和氧化还原活性配体结合的金属的结合环境
6. A Simple Model-Free Method for Direct Assessment of Fluorescent Ligand Binding by Linear Spectral Summation [O] . Oktay K. Gasymov, Adil R. Abduragimov, Ben J. Glasgow -1

机译：通过线性光谱求和直接评估荧光配体结合的简单无模型方法
7. A Simple Model-Free Method for Direct Assessment of Fluorescent Ligand Binding by Linear Spectral Summation [O] . Oktay K. Gasymov, Adil R. Abduragimov, Ben J. Glasgow 2013

机译：一种简单的无模型方法，用于通过线谱求和直接评估荧光配体结合

Ligand binding studies by high speed centrifugal precipitation and linear spectral summation using ultraviolet–visible absorption spectroscopy

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