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A universal analysis tool for the detection of asymmetric signal distribution in microscopic images.

机译:用于检测微观图像中不对称信号分布的通用分析工具。

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摘要

Polarization of tissue is achieved by asymmetric distribution of proteins and organelles within individual cells. However, existing quantitative assays to measure this asymmetry in an automated and unbiased manner suffer from significant limitations.Here, we report a new way to assess protein and organelle localization in tissue based on correlative fluorescence analysis. As a proof of principle, we successfully characterized planar cell polarity dependent asymmetry in developing Drosophila melanogaster tissues on the single cell level using fluorescence cross-correlation.Systematic modulation of signal strength and distribution show that fluorescence cross-correlation reliably detects asymmetry over a broad parameter space. The novel method described here produces robust, rapid, and unbiased measurement of biometrical properties of cell components in live tissue that is readily applicable in other model systems.
机译:通过单个细胞内的蛋白质和细胞器的不对称分布来实现组织的偏振。 然而,以自动化和无偏见的方式测量该不偏异性的现有定量测定患有显着的限制。,我们报告了一种新的方法来评估基于相关荧光分析的组织中的蛋白质和细胞器定位。 作为原理的证据,我们使用荧光互相关在单个细胞水平上发展果蝇黑素体组织的平面细胞极性依赖性不对称性。信号强度和分布的系统调制表明,荧光互相关可靠地检测到广泛参数上的不对称性 空间。 这里描述的新方法产生了在其他模型系统中容易地应用的活组织中细胞组分的稳健性,快速和无偏的生物学性质的测量。

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