Establishing Live-Cell Single-Molecule Localization Microscopy Imaging and Single-Particle Tracking in the Archaeon Haloferax volcanii

Turkowyd, Bartosz; Schreiber, Sandra; Wörtz, Julia; Segal, Ella Shtifman; Mevarech, Moshe; Duggin, Iain G.; Marchfelder, Anita; Endesfelder, Ulrike

doi:10.3389/fmicb.2020.583010

Cited by 26 publications

(23 citation statements)

References 46 publications

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“…Alternative fluorescent proteins could be expressed from our pMT-85 backbone, and multiple options are available in the literature, including the well-characterized mMaple3 (79), PAmCherry (80) or Dendra2 (81). These alternatives should nonetheless be properly benchmarked, as it was shown the performances of different fluorescent proteins can vary greatly in a given microbial species (82).…”

Section: Discussionmentioning

confidence: 99%

Imaging minimal bacteria at the nanoscale: a reliable and versatile process to perform Single Molecule Localization Microscopy in mycoplasmas

Rideau

Villa

Belzanne

et al. 2022

Preprint

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Mycoplasmas are the smallest free-living organisms. These bacteria are important models for both fundamental and Synthetic Biology, owing to their highly reduced genomes. They are also relevant in the medical and veterinary fields, as they are pathogenic of both humans and most livestock species. Mycoplasma cells have minute sizes, often in the 300-800 nanometers range. As these dimensions are close to the diffraction limit of visible light, fluorescence imaging in mycoplasmas is often poorly informative. Recently developed Super-Resolution Imaging techniques can break this diffraction limit, improving the imaging resolution by an order of magnitude and offering a new nanoscale vision of the organization of these bacteria. These techniques have however not been applied to mycoplasmas before. Here, we describe an efficient and reliable protocol to perform Single-Molecule Localization Microscopy (SMLM) imaging in mycoplasmas. We provide a polyvalent transposon-based system to express the photo-convertible fluorescent protein mEos3.2, enabling Photo-Activated Localization Microscopy (PALM) in most Mycoplasma species. We also describe the application of direct STochastic Optical Reconstruction Microscopy (dSTORM). We showcase the potential of these techniques by studying the subcellular localization of two proteins of interest. Our work highlights the benefits of state-of-the-art microscopy techniques for mycoplasmology and provides an incentive to further the development SMLM strategies to study these organisms in the future.

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Section: Discussionmentioning

confidence: 99%

Imaging minimal bacteria at the nanoscale: a reliable and versatile process to perform Single Molecule Localization Microscopy in mycoplasmas

Rideau

Villa

Belzanne

et al. 2022

Preprint

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“…H133 also contains deletions in the leuB and pyrE2 genes that were not used in this work. Furthermore, deletion of the crtI (HVO_2528) gene, which is involved in biosynthesis of the carotenoid pigment bacterioruberin, and is not essential nor has an effect on fitness (T urkowyd et al . 2020) resulted in a white phenotype.…”

Section: Methodsmentioning

confidence: 99%

“…The unique construction of the current mated pair however prevents such recombination events from happening as the cassettes were inserted into the same genomic location, hence the mated cells are forced to contain two different types of genomes and are essentially held under selection in a heteropolyploid state. In addition to the metabolic selectable marker, a second marker was introduced to one of the pair strains -a deletion in the crtI (HVO_2528) gene, which is involved in biosynthesis of the carotenoid pigment bacterioruberin and is not essential nor has an effect on fitness (TURKOWYD et al 2020). This deletion resulted in a white phenotype (WR807) in contrast with the other strain that remained naturally pigmented (red), (WR780).…”

Section: The Heteropolyploid State Is Stable Under Selectionmentioning

confidence: 99%

Differences in homologous recombination and maintenance of heteropolyploidy between Haloferax volcanii and Haloferax mediterranei

Altman-Price

Dattani

Sharon

et al. 2022

Preprint

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Polyploidy, the phenomenon of having more than one copy of the genome in an organism, is common among haloarchaea. While providing short-term benefits for DNA repair, polyploidy is generally regarded as an evolutionary trap that by the notion of the Mullers ratchet will inevitably conclude in the species decline or even extinction due to a gradual reduction in fitness. In most reported cases of polyploidy in archaea, the genetic state of the organism is considered as homoploidy i.e. all copies of the genome are identical. Here we demonstrate that while this is indeed the prevalent genetic status in the halophilic archaeon H. volcanii, its close relative H. mediterranei maintains a prolonged heteroploidy state in a non-selective environment once a second allele is introduced. Moreover, a strong genetic linkage was observed between two distant loci in H. mediterranei indicating a low rate of homologous recombination while almost no such linkage was shown in H. volcanii indicating a high rate of recombination in the latter species. We suggest that H. volcanii escapes Mullers ratchet by means of an effective chromosome- equalizing gene-conversion mechanism facilitated by highly active homologous recombination, whereas H. mediterranei must elude the ratchet via a different, yet to be elucidated mechanism.

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“…Raw single-molecule microscopy movie data often contains nonstructured background noise with different photophysical characteristics as the fluorophores of interest, caused by for example residual out-of-focus fluorophores e.g. in the immersion oil or sample buffer, or by autofluorescence within the biological sample itself (Turkowyd et al, 2019(Turkowyd et al, , 2020. Additionally, out-of-focus fluorophores under HiLo or TIRF illumination will display different blinking characteristics compared to in-focus fluorophores, and can therefore also be filtered out.…”

Section: Module 1: Temporal Median Image Filteringmentioning

confidence: 99%

Raw Data to Results: A Hands-On Introduction and Overview of Computational Analysis for Single-Molecule Localization Microscopy

2022

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Single-molecule localization microscopy (SMLM) is an advanced microscopy method that uses the blinking of fluorescent molecules to determine the position of these molecules with a resolution below the diffraction limit (∼5–40 nm). While SMLM imaging itself is becoming more popular, the computational analysis surrounding the technique is still a specialized area and often remains a “black box” for experimental researchers. Here, we provide an introduction to the required computational analysis of SMLM imaging, post-processing and typical data analysis. Importantly, user-friendly, ready-to-use and well-documented code in Python and MATLAB with exemplary data is provided as an interactive experience for the reader, as well as a starting point for further analysis. Our code is supplemented by descriptions of the computational problems and their implementation. We discuss the state of the art in computational methods and software suites used in SMLM imaging and data analysis. Finally, we give an outlook into further computational challenges in the field.

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Establishing Live-Cell Single-Molecule Localization Microscopy Imaging and Single-Particle Tracking in the Archaeon Haloferax volcanii

Cited by 26 publications

References 46 publications

Imaging minimal bacteria at the nanoscale: a reliable and versatile process to perform Single Molecule Localization Microscopy in mycoplasmas

Imaging minimal bacteria at the nanoscale: a reliable and versatile process to perform Single Molecule Localization Microscopy in mycoplasmas

Differences in homologous recombination and maintenance of heteropolyploidy between Haloferax volcanii and Haloferax mediterranei

Raw Data to Results: A Hands-On Introduction and Overview of Computational Analysis for Single-Molecule Localization Microscopy

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