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设计并生物物理特性分析拟南芥感应肽模拟衣藻质体醌结合位。

Design and biophysical characterization of atrazine-sensing peptides mimicking the Chlamydomonas reinhardtii plastoquinone binding niche.

机构信息

Institute of Crystallography, CNR, Rome, Italy.

出版信息

Phys Chem Chem Phys. 2013 Aug 21;15(31):13108-15. doi: 10.1039/c3cp51955d.

DOI:10.1039/c3cp51955d
PMID:23824019
Abstract

The plastoquinone (Q(B)) binding niche of the Photosystem II (PSII) D1 protein is the subject of intense research due to its capability to bind also anthropogenic pollutants. In this work, the Chlamydomonas reinhardtii D1 primary structure was used as a template to computationally design novel peptides enabling the binding of the herbicide atrazine. Three biomimetic molecules, containing the Q(B)-binding site in a loop shaped by two α-helices, were reconstituted by automated protein synthesis, and their structural and functional features deeply analysed by biophysical techniques. Standing out among the others, the biomimetic mutant peptide, D1pepMut, showed high ability to mimic the D1 protein in binding both Q(B) and atrazine. Circular dichroism spectra suggested a typical properly-folded α-helical structure, while isothermal titration calorimetry (ITC) provided a complete thermodynamic characterization of the molecular interaction. Atrazine binds to the D1pepMut with a high affinity (Kd = 2.84 μM), and a favourable enthalpic contribution (ΔH = -11.9 kcal mol(-1)) driving the interaction. Fluorescence spectroscopy assays, in parallel to ITC data, provided hyperbolic titration curves indicating the occurrence of a single atrazine binding site. The binding resulted in structural stabilisation of the D1pepMut molecule, as suggested by atrazine-induced cooperative profiles for the fold-unfold transition. The interaction dynamics and the structural stability of the peptides in response to the ligand were particularly considered as mandatory parameters for biosensor/biochip development. These studies paved the way to the set-up of an array of synthetic mutant peptides with a wide range of affinity towards different classes of target analytes, for the development of optical nanosensing platforms for herbicide detection.

摘要

类囊体醌 (Q(B)) 结合位是光系统 II (PSII) D1 蛋白的研究热点,因为它还能够结合人为污染物。在这项工作中,使用莱茵衣藻 D1 一级结构作为模板,通过计算设计新型肽,使莠去津能够结合。通过自动蛋白质合成重建了三个含有 Q(B)-结合位点的拟肽,该结合位点由两个α-螺旋形成的环组成,并通过生物物理技术对其结构和功能特征进行了深入分析。在其他肽中,拟肽突变体 D1pepMut 表现出高结合 Q(B)和莠去津的能力,引人注目。圆二色性谱表明具有典型的适当折叠的α-螺旋结构,而等温滴定量热法 (ITC) 提供了分子相互作用的完整热力学特征。莠去津与 D1pepMut 具有高亲和力 (Kd = 2.84 μM) 和有利的焓贡献 (ΔH = -11.9 kcal mol(-1)) 驱动相互作用。荧光光谱测定法与 ITC 数据平行,提供了双曲线滴定曲线,表明存在单个莠去津结合位点。结合导致 D1pepMut 分子结构稳定,正如 ITC 数据表明的折叠-展开转变的协同性。肽对配体的相互作用动力学和结构稳定性被认为是生物传感器/生物芯片发展的必要参数。这些研究为开发针对不同类目标分析物的具有广泛亲和力的合成突变肽阵列铺平了道路,用于开发莠去津光学纳米传感平台。

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