Mito Stress Assay of PBMCs With Seahorse XFe96 Flux Analyzer and Comparison of Poly-D-Lysine and Poly-L-Lysine for Cell Affinity.

IF 1 Q3 BIOLOGY
Kumudu Subasinghe, Raymond Berry, Megan Rowe, Ali Winters, Shaohua Yang, Nicole Phillips
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引用次数: 0

Abstract

The Seahorse 96 XF Analyzer (Agilent Technologies, Santa Clara, CA, USA) has been an effective tool in non-invasively measuring mitochondrial function for the past decade. It is a high-throughput respirometer that is considered the "gold standard" for quantifying mitochondrial function and bioenergetics in cells. Peripheral blood mononuclear cells (PBMCs) play a selective role in immune system responses and are key components of human immunity. Recent studies have suggested that these cell populations provide an overview of systemic changes within the body and therefore provide a source of sensitive biomarkers. Assessing mitochondrial function in PBMCs has been shown to provide an indication of metabolic stress associated with diseases such as diabetes and neurodegenerative conditions such as Alzheimer's disease. In this protocol, we use two adhesive compounds, Poly-D-Lysine (PDL) and Poly-L-Lysine (PLL), at 50 μg/mL each per well, to immobilize PBMCs to a specialized Seahorse microplate to perform mitochondrial stress assay using the Seahorse Analyzer. We compared six cell densities of PBMCs to identify the optimal cell density for use in Seahorse Mito Stress analysis. This protocol includes the immobilization of freshly isolated PBM cells into a Seahorse microplate, hydration and calibration of the sensor cartridge, cell seeding, running the Seahorse Analyzer for the Mito Stress test, and simple data analysis to compare the effectiveness of PLL and PDL as the coating agent for PBMCs. The data analysis indicates that there is no statistical difference between PLL and PDL. Key features • Designed for Seahorse 96-XF Analyzer, allowing it to work with lower cell densities and accommodate a greater number of replicates with high-throughput capabilities. • Two widely used cell adhesive compounds, Poly-D-Lysine and Poly-L-Lysine, are compared for their effectiveness in immobilizing PBMCs onto specialized Seahorse microplates. • The protocol takes two days to complete.

用海马XFe96通量分析仪测定PBMCs的Mito胁迫及聚d -赖氨酸和聚l -赖氨酸对细胞亲和力的比较
Seahorse 96 XF分析仪(Agilent Technologies, Santa Clara, CA, USA)在过去十年中一直是一种有效的非侵入性测量线粒体功能的工具。它是一种高通量呼吸计,被认为是量化细胞中线粒体功能和生物能量学的“金标准”。外周血单核细胞(Peripheral blood mononuclear cells, PBMCs)在免疫系统反应中起选择性作用,是人体免疫系统的关键组成部分。最近的研究表明,这些细胞群提供了体内系统变化的概述,因此提供了敏感生物标志物的来源。评估pbmc的线粒体功能已被证明可以提供与糖尿病和阿尔茨海默病等神经退行性疾病相关的代谢应激的指示。在本方案中,我们使用两种粘合剂,聚d -赖氨酸(PDL)和聚l -赖氨酸(PLL),每孔50 μg/mL,将pbmc固定在专用海马微孔板上,使用海马分析仪进行线粒体应激分析。我们比较了六种pbmc的细胞密度,以确定用于海马水户应激分析的最佳细胞密度。该方案包括将新分离的PBM细胞固定在Seahorse微孔板上,水化和校准传感器盒,细胞播种,运行Seahorse分析仪进行Mito压力测试,以及简单的数据分析,以比较PLL和PDL作为pbmc包膜剂的有效性。数据分析表明,PLL与PDL之间无统计学差异。•专为Seahorse 96-XF分析仪设计,使其能够在较低的细胞密度下工作,并具有高通量能力,可容纳更多数量的重复。•两种广泛使用的细胞粘合剂化合物,聚d -赖氨酸和聚l -赖氨酸,比较了它们在固定pbmc到专用海马微孔板上的有效性。•该协议需要两天才能完成。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
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CiteScore
1.50
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