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首页> 外文期刊>Journal of Applied Phycology >Improved Nile Red staining of Nannochloropsis sp.
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Improved Nile Red staining of Nannochloropsis sp.

机译:Nannochloropsis sp。的改进的尼罗红染色。

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High-throughput screening of microalgae for use as a potential feedstock for biodiesel requires a reliable method for the rapid detection of intracellular neutral lipid content. In this study, we report a modified and improved Nile Red (NR) fluorescence staining procedure for use as a rapid and sensitive screening tool to estimate levels of intracellular neutral lipid in the picopleustonic microalgae, Nannochloropsis sp. Addition of either glycerol or dimethyl sulfoxide (DMSO) into microalgae cultures greatly enhances lipid staining efficiency and increases the fluorescence intensity of stained cells. The optimized procedure requires glycerol and DMSO at the concentration of 0.1 and 0.165 g mL(-1), respectively, for peak fluorescence in a live culture of Nannochloropsis sp. Incubation for 5 min for glycerol-NR staining and 10 min for DMSO-NR staining at room temperature, in darkness, is used for the NR concentration of 0.3 and 0.7 mu g mL(-1) for glycerol and DMSO, respectively. For the selection of lipid-rich cells of Nannochloropsis sp. using flow cytometric cell sorting, the glycerol-NR procedure is recommended as glycerol, unlike DMSO, does not inhibit subsequent growth of sorted cells.
机译:高通量筛选微藻用作生物柴油的潜在原料需要一种可靠的方法来快速检测细胞内中性脂质含量。在这项研究中,我们报告了一种经过改进和改进的尼罗红(NR)荧光染色程序,可用于快速,灵敏地筛选工具,以评估皮膜微囊微藻Nannochloropsis sp。中的细胞内中性脂质水平。将甘油或二甲基亚砜(DMSO)添加到微藻培养物中可大大提高脂质染色效率并增加染色细胞的荧光强度。优化的程序需要分别在浓度为0.1和0.165 g mL(-1)的甘油和DMSO中获得Nannochloropsis sp。的活培养物中的峰值荧光。甘油-NR染色在室温下孵育5分钟,DMSO-NR染色在室温下孵育10分钟,在黑暗中,甘油和DMSO的NR浓度分别为0.3和0.7μg mL(-1)。用于选择Nannochloropsis sp。的富含脂质的细胞。使用流式细胞仪进行细胞分选时,建议使用甘油-NR程序,因为甘油与DMSO不同,它不抑制分选细胞的后续生长。

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