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荧光激活和吸收移位标签(FAST)在产甲烷古菌流式细胞术中的应用。

Application of the Fluorescence-Activating and Absorption-Shifting Tag (FAST) for Flow Cytometry in Methanogenic Archaea.

机构信息

School of Chemical Engineering, Department of Bioproducts and Biosystems, Aalto University, Espoo, Finland.

出版信息

Appl Environ Microbiol. 2023 Apr 26;89(4):e0178622. doi: 10.1128/aem.01786-22. Epub 2023 Mar 15.

Abstract

Methane-producing archaea play a crucial role in the global carbon cycle and are used for biotechnological fuel production. Methanogenic model organisms such as Methanococcus maripaludis and Methanosarcina acetivorans have been biochemically characterized and can be genetically engineered by using a variety of existing molecular tools. The anaerobic lifestyle and autofluorescence of methanogens, however, restrict the use of common fluorescent reporter proteins (e.g., GFP and derivatives), which require oxygen for chromophore maturation. Recently, the use of a novel oxygen-independent fluorescent activation and absorption-shifting tag (FAST) was demonstrated with . Similarly, we now describe the use of the tandem activation and absorption-shifting tag protein 2 (tdFAST2), which fluoresces when the cell-permeable fluorescent ligand (fluorogen) 4-hydroxy-3,5-dimethoxybenzylidene rhodanine (HBR-3,5DOM) is present. Expression of tdFAST2 in and is noncytotoxic and tdFAST2:HBR-3,5DOM fluorescence is clearly distinguishable from the autofluorescence. In flow cytometry experiments, mixed methanogen cultures can be distinguished, thereby allowing for the possibility of high-throughput investigations of the characteristic dynamics within single and mixed cultures. Methane-producing archaea play an essential role in the global carbon cycle and demonstrate great potential for various biotechnological applications, e.g., biofuel production, carbon dioxide capture, and electrochemical systems. Oxygen sensitivity and high autofluorescence hinder the use of common fluorescent proteins for studying methanogens. By using tdFAST2:HBR-3,5DOM fluorescence, which functions under anaerobic conditions and is distinguishable from the autofluorescence, real-time reporter studies and high-throughput investigation of the mixed culture dynamics of methanogens via flow cytometry were made possible. This will further help accelerate the sustainable exploitation of methanogens.

摘要

产甲烷古菌在全球碳循环中起着至关重要的作用,并且被用于生物技术燃料生产。产甲烷模式生物,如 Methanococcus maripaludis 和 Methanosarcina acetivorans,已经在生物化学方面得到了表征,并且可以通过使用各种现有的分子工具进行基因工程改造。然而,产甲烷菌的厌氧生活方式和自发荧光限制了常用荧光报告蛋白(例如 GFP 和衍生物)的使用,因为这些蛋白需要氧来成熟发色团。最近,一种新型的不依赖于氧的荧光激活和吸收转移标签(FAST)在 中得到了应用。同样,我们现在描述了串联激活和吸收转移标签蛋白 2(tdFAST2)的使用,当细胞通透性荧光配体(荧光团)4-羟基-3,5-二甲氧基苯亚甲基罗丹宁(HBR-3,5DOM)存在时,tdFAST2 会发出荧光。tdFAST2 在 和 中的表达是非细胞毒性的,并且 tdFAST2:HBR-3,5DOM 荧光与自发荧光明显区分开来。在流式细胞术实验中,可以区分混合产甲烷菌培养物,从而有可能对单个和混合培养物中的特征动力学进行高通量研究。产甲烷古菌在全球碳循环中起着至关重要的作用,并在各种生物技术应用中展示出巨大的潜力,例如生物燃料生产、二氧化碳捕获和电化学系统。氧敏感性和高自发荧光阻碍了常用荧光蛋白在研究产甲烷菌中的应用。通过使用 tdFAST2:HBR-3,5DOM 荧光,它可以在厌氧条件下发挥作用并且与自发荧光区分开来,从而可以进行实时报告研究和通过流式细胞术对产甲烷菌混合培养物动力学进行高通量研究。这将进一步有助于加速产甲烷菌的可持续开发。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/77f5/10132111/ddcb7102f002/aem.01786-22-f001.jpg

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