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利用发光光谱法对镧系(III)离子与钙调蛋白的结合进行表征。

Characterization of lanthanide (III) ion binding to calmodulin using luminescence spectroscopy.

作者信息

Mulqueen P, Tingey J M, Horrocks W D

出版信息

Biochemistry. 1985 Nov 5;24(23):6639-45. doi: 10.1021/bi00344a051.

DOI:10.1021/bi00344a051
PMID:4084548
Abstract

Pulsed dye laser excitation spectroscopy of the 7F0----5D0 transition of Eu(III) reveals only a single peak as this ion is titrated into apocalmodulin. A titration based on the intensity of this transition shows that the first two Eu(III) ions bind quantitatively to two tight sites, followed by weaker binding (Kd = 2 microM) to two additional sites under conditions of high ionic strength (0.5 M KC1). This excitation experiment is also shown to be a general method for measuring contaminating levels of EDTA down to 0.2 microM in proton solutions. Experiments with Tb(III) using both direct laser excitation and indirect sensitization of Tb(III) luminescence through tyrosine residues in calmodulin also give evidence for two tight and two weaker binding sites (Kd = 2-3 microM). The indirect sensitization results primarily upon binding to the two weaker sites, implying that Tb(III) binds first to domains I and II, which are remote from tyrosine-containing domains III and IV. The 7F0----5D0 excitation signal of Eu(III) was used to measure the relative overall affinities of the tripositive lanthanide ions, Ln(III), across the series. Ln(III) ions at the end of the series are found to bind more weakly than those at the beginning and middle of the series. Eu(III) excited-state lifetime measurements in H2O and D2O reveal that two water molecules are coordinated to the Eu(III) at each of the four metal ion binding sites. Measurements of Förster-type nonradiative energy-transfer efficiencies between Eu(III) and Nd(III) in the two tight sites were carried out by monitoring the excited-state lifetimes of Eu(III) in the presence and absence of the energy acceptor ion Nd(III).(ABSTRACT TRUNCATED AT 250 WORDS)

摘要

铕(III)从 7F0 到 5D0 跃迁的脉冲染料激光激发光谱显示,当该离子滴定到脱钙钙调蛋白中时仅出现一个单峰。基于此跃迁强度的滴定表明,前两个铕(III)离子定量结合到两个紧密位点,随后在高离子强度(0.5 M KCl)条件下与另外两个位点的结合较弱(解离常数 Kd = 2 μM)。该激发实验还被证明是一种用于测量质子溶液中低至 0.2 μM 的乙二胺四乙酸(EDTA)污染水平的通用方法。使用直接激光激发以及通过钙调蛋白中酪氨酸残基对铽(III)发光进行间接敏化的铽(III)实验,也证明存在两个紧密结合位点和两个较弱结合位点(Kd = 2 - 3 μM)。间接敏化主要发生在与两个较弱位点结合时,这意味着铽(III)首先结合到结构域 I 和 II,它们远离含酪氨酸的结构域 III 和 IV。铕(III)的 7F0 到 5D0 激发信号用于测量整个系列中三价镧系离子 Ln(III)的相对总体亲和力。发现该系列末尾的 Ln(III)离子结合比系列开头和中间的离子更弱。在 H2O 和 D2O 中对铕(III)激发态寿命的测量表明,在四个金属离子结合位点中的每一个位点上都有两个水分子与铕(III)配位。通过监测在存在和不存在能量受体离子钕(III)的情况下铕(III)的激发态寿命,对两个紧密位点中铕(III)和钕(III)之间的福斯特型非辐射能量转移效率进行了测量。(摘要截断于 250 字)

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