首页> 外文期刊>Journal of Neuroscience Methods >Optimization of multiplexed bead-based cytokine immunoassays for rat serum and brain tissue.
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Optimization of multiplexed bead-based cytokine immunoassays for rat serum and brain tissue.

机译:用于大鼠血清和脑组织的基于多重珠子的细胞因子免疫测定的优化。

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The ability to simultaneously quantify multiple signaling molecule protein levels from microscopic neural tissue samples would be of great benefit to deciphering how they affect brain function. This follows from evidence that indicates signaling molecules can be pleiotropic and can have complex interactive behavior that is regionally and cellularly heterogeneous. Multiplexed examination of tissue proteins has been exceedingly difficult because of the absence of available techniques. This void now has been removed by the commercial availability of bead-based immunoassays for targeted proteins that allow analyses of up to 100 (6-150 kDa) proteins from as little as 12 microl. Thus far used only for sera (human and mouse) and culture media, we demonstrate here that sensitive (as low as 2 pg/ml), wide-ranging (up to 2-32 000 pg/ml), accurate (8% intra-assay covariance) and reliable (4-7% inter-assay covariance) measurements can be made of nine exemplary cytokines (e.g., IL-1alpha, IL-1beta, IL-2, IL-4, IL-6, IL-10, GM-CSF, IFN-gamma, TNF-alpha) simultaneously not only from rat serum but, for the first time, also brain tissue. Furthermore, we describe animal handling procedures that minimize stress as determined by serum glucocorticoid levels since they can influence cytokine expression.
机译:从微观神经组织样本中同时量化多种信号分子蛋白质水平的能力,将有助于破译它们如何影响大脑功能。这来自于表明信号分子可以是多效性的并且可以具有区域和细胞异质的复杂相互作用行为的证据。由于缺乏可用的技术,组织蛋白的多重检查非常困难。这种空缺现已通过针对目标蛋白的基于珠子的免疫测定方法的商业可获得性得以消除,该方法可从低至12微升分析多达100种(6-150 kDa)蛋白。到目前为止,仅用于血清(人和小鼠)和培养基,我们在这里证明了灵敏(低至2 pg / ml),范围广(高达2-32 000 pg / ml),准确(8%内-测定协方差)和可靠的测定值(4-7%测定间协方差)可以对九种示例性细胞因子(例如,IL-1alpha,IL-1beta,IL-2,IL-4,IL-6,IL-10)进行测量,GM-CSF,IFN-γ,TNF-α)不仅来自大鼠血清,而且还首次来自脑组织。此外,我们描述了动物处理程序,该程序可最大程度地降低由血清糖皮质激素水平决定的压力,因为它们会影响细胞因子的表达。

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