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Effects of ligand binding on the conformation and internal dynamics in specific regions of porcine pancreatic phospholipase A{sub}2 with tryptophan as a probe: a study combining time-resolved fluorescence spectroscopy and site-directed mutagenesis

机译:用色氨酸作为探针的猪胰磷脂磷脂酶A {Sub} 2特定区域对特征和内部动力学的影响:一种结合时间分辨荧光光谱和定点诱变的研究

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Exploration of the effect of ligand-protein interactions on conformational substates and internal dynamics in different regions of phospholipase A{sub}2 from porcine pancreas (PLA{sub}2), was performed by combining site-directed mutagenesis and time-resolved fluorescence measurements. The single tryptophan residue (Trp-3) in the wild type protein was replaced by a phenylalanine residue, whereafter Trp was substituted either for leucine-31, located in the calcium binding loop, or for phenylalanine-94, located at the "back side" of the enzyme, in α-helix E (Dijkstra et al., J. Mol. Biol., 147,97-123, 1981). Analyses by the Maximum Entropy Method (MEM) of the total fluorescence intensity decays, provide in each case a distribution of separate lifetime classes, which can be interpreted as reflecting the existence of discrete conformational substates in slow exchange with respect to the time-scale of the decay kinetics. The fluorescence decay of the W94 mutant is. dominated by an extremely short excited state lifetime of ~60 ps, probably arising from the presence of two proximate disulfide bridges. Time-resolved fluorescence anisotropy studies show that the Trp residue near the NH{sub}2 terminus (Trp-3) undergoes a more limited rotational motion than the Trp-31 located in the calcium binding loop. The widest angular rotation is observed at position 94, in α-helix E. Calcium binding displays the strongest influence on the lifetime distribution of Trp-31: a major local conformation corresponding to a lifetime class with a barycenter value of ~5.5 ns and contributing to ~50% of the decay is selected. The conformations giving rise to the short lifetimes (τ{sub}1 and τ{sub}2 lifetime classes) become less important. The contribution of the third lifetime class (c{sub}3) stays at a constant value of 30%. In the presence of calcium, the amplitude of motion is wider than without the ion. There is virtually no effect of calcium binding on the lifetime distribution of the Trp residue at the 3 or the 94 position. Binding of the monomeric substrate analog n-dodecylphosphocholine (C12PN) in the presence of calcium hardly affects neither the Trp-3 excited state population distribution, nor its rotational dynamics. The binding of C12PN monomers to the W31 mutant further increases the contribution of the τ{sub}4 lifetime class at the expense of c{sub}2. A more restricted rotation of the Trp-31 residue is also induced. The binding of the micellar substrate analog n-hexadecylphosphocholine (C16PN) in the presence of calcium is very efficient in modifying the lifetime distribution of Trp-3. Essentially, one major broad lifetime population (centered at ~2.6 ns) is revealed by MEM analysis of the total intensity decay. The internal motion is slowed down and the angle of rotation is much smaller in this conformation. Neither the excited state lifetime distribution of Trp-31 nor its dynamics are affected by micelle binding relative to monomer binding. In conclusion, by placing a single Trp-residue at strategic positions along the peptide chain of PLA{sub}2, relevant to the binding of biological ligands, an excellent model system for the study of selective perturbations of conformational substates and internal dynamics is provided.
机译:通过组合定点诱变和时间分辨荧光测量来进行磷脂酶(PLA {Sub} 2的不同区域对磷脂酶A {Sub} 2不同区域的构象变化物和内部动力学的探索。野生型蛋白质中的单色氨酸残基(TRP-3)被苯丙氨酸残基取代,然后TRP被取代用于位于钙结合环中的亮氨酸-31,或用于位于“后侧的苯丙氨酸-94 “酶,在α-螺旋E中(Dijkstra等,J.Mol.Biol.,147,97-123,1981)。通过总荧光强度衰减的最大熵方法(MEM)分析,在每种情况下提供单独的寿命等级的分布,其可以解释为反映相对于时间尺度的慢速交换中的离散构象变电站的存在衰变动力学。 W94突变体的荧光衰减是。由极短的激发态寿命为主导〜60 ps,可能是两种近似二硫桥的存在。时间分辨的荧光各向异性研究表明,NH {亚} 2末端(TRP-3)附近的TRP残基经历了比位于钙结合环中的TRP-31更有限的旋转运动。在α-螺旋E中观察到最宽的角度旋转。在α-螺旋E中,钙绑定对TRP-31的寿命分布显示最强的影响:对应于具有〜5.5 ns〜5.5 ns和贡献的寿命类别的主要局部构象选择衰减的〜50%。产生短寿命的构象(τ{sub} 1和τ{sub} 2寿命等级)变得不那么重要。第三寿命类(C {Sub} 3)的贡献保持在恒定值30%。在存在钙的情况下,运动的幅度宽于没有离子的情况。在3或94位置的TRP残基的寿命分布几乎没有钙结合的影响。单体底物类似物N-十二烷基磷胆碱(C12PN)在钙的存在下既没有影响TRP-3激发态群体分布,也不会影响其旋转动力学。 C12PN单体与W31突变体的结合进一步增加了τ{sub} 4寿命等级以牺牲C {sub} 2的贡献。还诱导了TRP-31残基的更受限制的旋转。在修饰TRP-3的寿命分布时,胶束基质类似N-十六烷基磷胆碱(C16PN)的结合非常有效。基本上,通过对总强度衰减的MEM分析揭示了一个主要的广泛寿命群体(以〜2.6ns为中心)。内部运动减慢,并且在这种构象中旋转角度小得多。 TRP-31和其动力学的激发态寿命分布都不受胶束结合相对于单体结合的影响。总之,通过沿PLA {sub} 2的肽链将单个TRP残基放置在PLA {Sub} 2的肽链中,提供了与生物配体的结合相关的,提供了研究综合变电站和内部动力学选择性扰动的优秀模型系统。

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