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Multimodal fluorescence microscopy of prion strain specific PrP deposits stained by thiophene-based amyloid ligands

机译:基于噻吩的淀粉样蛋白配体染色的病毒菌株特异PrP沉积物的多峰荧光显微镜

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The disease-associated prion protein (PrP) forms aggregates which vary in structural conformation yet share an identical primary sequence. These variations in PrP conformation are believed to manifest in prion strains exhibiting distinctly different periods of disease incubation as well as regionally specific aggregate deposition within the brain. The anionic luminescent conjugated polythiophene (LCP), polythiophene acetic acid (PTAA) has previously been used to distinguish PrP deposits associated with distinct mouse adapted strains via distinct fluorescence emission profiles from the dye. Here, we employed PTAA and 3 structurally related chemically defined luminescent conjugated oligothiophenes (LCOs) to stain brain tissue sections from mice inoculated with 2 distinct prion strains. Our results showed that in addition to emission spectra, excitation, and fluorescence lifetime imaging microscopy (FLIM) can fruitfully be assessed for optical distinction of PrP deposits associated with distinct prion strains. Our findings support the theory that alterations in LCP/LCO fluorescence are due to distinct conformational restriction of the thiophene backbone upon interaction with PrP aggregates associated with distinct prion strains. We foresee that LCP and LCO staining in combination with multimodal fluorescence microscopy might aid in detecting structural differences among discrete protein aggregates and in linking protein conformational features with disease phenotypes for a variety of neurodegenerative proteinopathies.
机译:疾病相关的pr病毒蛋白(PrP)形成聚集体,其结构构​​象不同,但共有相同的一级序列。据信PrP构象的这些变异在表现出明显不同的疾病潜伏期以及脑内区域特定聚集体沉积的病毒菌株中表现出来。阴离子发光共轭聚噻吩(LCP),聚噻吩乙酸(PTAA)以前已用于通过与染料不同的荧光发射曲线来区分与不同的小鼠适应株相关的PrP沉积物。在这里,我们采用PTAA和3种结构相关的化学定义的发光共轭寡聚噻吩(LCO)对来自接种2种不同病毒菌株的小鼠的脑组织切片进行染色。我们的结果表明,除了发射光谱,激发和荧光寿命成像显微镜(FLIM)可以有效评估与不同distinct病毒菌株相关的PrP沉积物的光学区别。我们的发现支持以下理论:LCP / LCO荧光的改变是由于与与不同distinct病毒菌株相关的PrP聚集体相互作用后,噻吩骨架的构象受到限制。我们预见,LCP和LCO染色与多峰荧光显微镜相结合可能有助于检测离散蛋白聚集体之间的结构差异,并将蛋白构象特征与多种神经退行性蛋白病的疾病表型联系起来。

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