Development of Strong Anaerobic Fluorescent Reporters for Clostridium acetobutylicum and Clostridium ljungdahlii Using HaloTag and SNAP-tag Proteins
One of the biggest limitations in the study and engineering of anaerobic organisms is the lack of strong fluorescent reporters capable of strong and real-time fluorescence. Recently, we developed a strong fluorescent reporter system for organisms based on the FAST protein. Here, we report the develo...
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Veröffentlicht in: | Applied and environmental microbiology 2020-10, Vol.86 (20) |
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Zusammenfassung: | One of the biggest limitations in the study and engineering of anaerobic
organisms is the lack of strong fluorescent reporters capable of strong and real-time fluorescence. Recently, we developed a strong fluorescent reporter system for
organisms based on the FAST protein. Here, we report the development of two new strong fluorescent reporter systems for
organisms based on the HaloTag and SNAP-tag proteins, which produce strong fluorescent signals when covalently bound to fluorogenic ligands. These new fluorescent reporters are orthogonal to the FAST ligands and to each other, allowing for simultaneous labeling and visualization. We used HaloTag and SNAP-tag to label the strictly anaerobic organisms
and
We have also identified a new strong promoter for protein expression in
, based on the phosphotransacetylase gene (
) from
Furthermore, the HaloTag and the SNAP-tag, in combination with the previously described FAST system, were successfully used to measure cell populations in bacterial mixed cultures and showed the simultaneous orthogonal labeling of HaloTag and SNAP-tag together with the FAST protein reporter. Finally, we show the expression of recombinant fusion protein of FAST and the ZapA division protein (from
) in
The availability of multiple strong fluorescent reporters is a major addition to the genetic toolkit of
and other anaerobes that will lead to better understanding of these unique organisms.
Up to this point, assays and methods involving fluorescent reporter proteins were unavailable or limited in
organisms and other strict anaerobes. Green fluorescent protein (GFP), mCherry, and flavin-binding proteins (and their derivatives) have been used only in a few clostridia with limited success and yielded low fluorescence compared to aerobic microbial systems. Recently, we reported a new strong fluorescent reporter system based on the FAST protein as a first step in expanding the fluorescence-based reporters for
and other anaerobic microbial platforms. Additional strong orthogonal fluorescent proteins, with distinct emission spectra are needed to allow for (i) multispecies tracking within the growing field of microbial cocultures and microbiomes, (ii) protein localization and tracking in anaerobes, and (iii) identification and development of natural and synthetic promoters, ribosome-binding sites (RBS), and terminators for optimal protein expression in anaerobes. Here, we present two new strong fluorescent reporter systems based on the HaloTag and |
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ISSN: | 0099-2240 1098-5336 |
DOI: | 10.1128/AEM.01271-20 |