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首页> 外文期刊>The Journal of Nuclear Medicine >Labeling of cerebral amyloid beta deposits in vivo using intranasal basic fibroblast growth factor and serum amyloid P component in mice.
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Labeling of cerebral amyloid beta deposits in vivo using intranasal basic fibroblast growth factor and serum amyloid P component in mice.

机译:在小鼠中使用鼻内碱性成纤维细胞生长因子和血清淀粉样蛋白P组分在体内标记脑淀粉样蛋白β沉积物。

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There is currently no method for noninvasive imaging of amyloid beta (Abeta) deposition in Alzheimer's disease (AD). Because Abeta plaques are characteristic of AD and Abeta deposits contain abundant heparan sulfate proteoglycans that can bind basic fibroblast growth factor (bFGF) and serum amyloid P component (SAP), we investigated a novel route of ligand delivery to the brain to assess Abeta deposition in a transgenic (Tg) mouse model overexpressing Abeta-protein precursor. METHODS: The biodistribution of bFGF injected intranasally was studied using (125)I-bFGF in Tg and wild-type control mice and by unlabeled bFGF and SAP immunocytochemistry with light and electron microscopy. RESULTS: Three- to 5-fold higher amounts of (125)I-bFGF were found in the brain of Tg mice than that of wild-type mice (P < 0.05). bFGF or SAP given intranasally labeled cerebral Abeta plaques in the cortex and microvessels of Tg mice but not in wild-type mice. Weak bFGF staining and no SAP staining were detected in Tg mice without intranasal injection of the ligands. bFGF and SAP stained neurons around the rim of Abeta deposits and throughout the cortex in Tg mice. There was only weak staining of neurons in Tg mice without intranasal injection of bFGF and no staining of SAP in Tg mice without intranasal injection of SAP. No bFGF or SAP staining was evident in wild-type control mice. CONCLUSION: We report a novel noninvasive method for labeling Abeta plaques. This method may be modified for human studies using intranasal injection of radiolabeled ligands and imaging with SPECT or PET.
机译:当前尚无用于对阿尔茨海默氏病(AD)中的淀粉样β(Abeta)沉积物进行无创成像的方法。由于Abeta斑块是AD的特征,并且Abeta沉积物含有丰富的硫酸乙酰肝素蛋白聚糖,可以结合碱性成纤维细胞生长因子(bFGF)和血清淀粉样蛋白P组分(SAP),因此我们研究了配体向大脑输送的新途径,以评估Abeta沉积过表达Abeta蛋白前体的转基因(Tg)小鼠模型。方法:使用(125)I-bFGF在Tg和野生型对照小鼠中并通过未标记的bFGF和SAP免疫细胞化学以及光学和电子显微镜研究鼻内注射bFGF的生物分布。结果:与野生型小鼠相比,Tg小鼠的大脑中发现的(125)I-bFGF含量高3至5倍(P <0.05)。在Tg小鼠的皮层和微血管中给鼻内标记的脑Abeta斑块给予bFGF或SAP,而在野生型小鼠中则不然。在没有鼻内注射配体的情况下,在Tg小鼠中未检测到弱的bFGF染色并且没有SAP染色。在Tg小鼠的Abeta沉积物边缘和整个皮质中,bFGF和SAP染色的神经元。没有鼻内注射bFGF的Tg小鼠只有神经元的弱染色,而没有鼻内注射的SAP的Tg小鼠没有SAP的染色。在野生型对照小鼠中没有bFGF或SAP染色是明显的。结论:我们报告了一种新颖的无创方法来标记Abeta斑块。可以通过鼻内注射放射性标记的配体并用SPECT或PET成像对这种方法进行人类研究。

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