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尼罗红孵育时间对读取荧光前的酵母中性脂质定量有很大影响。

Nile Red Incubation Time Before Reading Fluorescence Greatly Influences the Yeast Neutral Lipids Quantification.

作者信息

Ramírez-Castrillón Mauricio, Jaramillo-Garcia Victoria P, Lopes Barros Helio, Pegas Henriques João A, Stefani Valter, Valente Patricia

机构信息

Graduate Program in Cell and Molecular Biology, Biotechnology Center, Universidade Federal do Rio Grande do Sul, Porto Alegre, Brazil.

Research Group in Mycology (GIM), Universidad Santiago de Cali, Santiago de Cali, Colombia.

出版信息

Front Microbiol. 2021 Mar 4;12:619313. doi: 10.3389/fmicb.2021.619313. eCollection 2021.

Abstract

High-throughput screening methodologies to estimate lipid content in oleaginous yeasts use Nile red fluorescence in a given solvent and optimized excitation/emission wavelengths. However, Nile red fluorescence stabilization has been poorly analyzed, and high variability occurs when relative fluorescence is measured immediately or a few minutes after dye addition. The aim of this work was to analyze the fluorescence of Nile red at different incubation times using a variety of solvents and oleaginous/non-oleaginous yeast strains. We showed that fluorescence stabilization occurs between 20 and 30 min, depending on the strain and solvent. Therefore, we suggest that fluorescence measurements should be followed until stabilization, where Relative Fluorescence Units should be considered after stabilization for lipid content estimation.

摘要

用于评估产油酵母中脂质含量的高通量筛选方法,是在特定溶剂及优化的激发/发射波长条件下利用尼罗红荧光。然而,尼罗红荧光的稳定性分析不足,在添加染料后立即或几分钟后测量相对荧光时会出现高度变异性。本研究的目的是使用多种溶剂和产油/非产油酵母菌株,分析不同孵育时间下尼罗红的荧光。我们发现,荧光稳定性在20至30分钟之间出现,这取决于菌株和溶剂。因此,我们建议应持续监测荧光直至稳定,在稳定后应使用相对荧光单位来估计脂质含量。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/56d2/7969498/c6624d77462e/fmicb-12-619313-g001.jpg

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本文引用的文献

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