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Quantifying Heterogeneity of Individual Organelles in Mixed Populations via Mass Cytometry

机译:通过质量细胞测定法量化混合群体中个体细胞器的异质性

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Macroautophagy is a complex degradative intracellular process by which long-lived proteins and damaged organelles are cleared. Common methods for the analysis of autophagy are bulk measurements which mask organelle heterogeneity and complicate the analysis of interorganelle association and trafficking. Thus, methods for individual organelle quantification are needed to address these deficiencies. Current techniques for quantifying individual autophagy organelles are either low through-put or are dimensionally limited. We make use of the multiparametric capability of mass cytometry to investigate phenotypic heterogeneity in autophagy-related organelle types that have been isolated from murine brain, liver, and skeletal muscle. Detection and phenotypic classification of individual organelles were accomplished through the use of a lanthanide-chelating membrane stain and organelle-specific antibodies. Posthoc sample matrix background correction and nonspecific antibody binding corrections provide measures of interorganelle associations and heterogeneity. This is the first demonstration of multiparametric individual organelle analysis via mass cytometry. The method described here illustrates the potential for further investigation of the inherently complex interorganelle associations, trafficking, and heterogeneity present in most eukaryotic biological systems.
机译:宏观摄影是一种复杂的降解细胞内过程,通过该过程可以清除长寿命和受损的细胞器。用于自噬分析的常用方法是批量测量,其掩盖细胞器异质性,并使室内同期分析复杂化。因此,需要用于解决这些缺陷的个体细胞器量化的方法。用于量化单独的自噬细胞器的当前技术是低通过放置或尺寸限制。我们利用质量细胞测定法的多体形能力来研究从鼠脑,肝脏和骨骼肌中分离的自噬相关细胞石类型中的表型异质性。通过使用镧系元素螯合膜染色和细胞器特异性抗体来完成个体细胞器的检测和表型分类。 POSTHOC样品基质背景校正和非特异性抗体结合校正提供了室内联的缔合和异质性的措施。这是通过质量细胞仪进行多射周个体细胞器分析的第一次证明。这里描述的方法说明了进一步研究在大多数真核生物系统中存在固有的复杂的室内联吻,贩运和异质性的可能性。

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