Fluorescent proteins as in-vivo and in-situ reporters to study the development of a Saccharomyces cerevisiae yeast biofilm and its invasion by the bacteria Escherichia coli

Förster resonance energy transfer (FRET) microscopy is a powerful fluorescence microscopy method to study the nanoscale organization of multiprotein assemblies in vivo. Moreover, many biochemical and biophysical processes can be followed by employing sophisticated FRET biosensors directly in living cells. Here, we summarize existing FRET experiments and biosensors applied in yeasts Saccharomyces cerevisiae and Schizosaccharomyces pombe, two important models of fundamental biomedical research and efficient platforms for analyses of bioactive molecules. We aim to provide a practical guide on suitable FRET techniques, fluorescent proteins, and experimental setups available for successful FRET experiments in yeasts.

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C-terminal eYFP fusion impairs Escherichia coli MinE function

Open Biology ◽

10.1098/rsob.200010 ◽

2020 ◽

Vol 10 (5) ◽

pp. 200010

Author(s):

Navaneethan Palanisamy ◽

Mehmet Ali Öztürk ◽

Emir Bora Akmeriç ◽

Barbara Di Ventura

Keyword(s):

Escherichia Coli ◽

In Silico ◽

Fluorescent Protein ◽

Fluorescent Proteins ◽

Yellow Fluorescent Protein ◽

Time Lapse ◽

Enhanced Yellow Fluorescent Protein ◽

Min Proteins

The Escherichia coli Min system plays an important role in the proper placement of the septum ring at mid-cell during cell division. MinE forms a pole-to-pole spatial oscillator with the membrane-bound ATPase MinD, resulting in MinD concentration being the lowest at mid-cell. MinC, the direct inhibitor of the septum initiator protein FtsZ, forms a complex with MinD at the membrane, mirroring its polar gradients. Therefore, MinC-mediated FtsZ inhibition occurs away from mid-cell. Min oscillations are often studied in living cells by time-lapse microscopy using fluorescently labelled Min proteins. Here, we show that, despite permitting oscillations to occur in a range of protein concentrations, the enhanced yellow fluorescent protein (eYFP) C-terminally fused to MinE impairs its function. Combining in vivo , in vitro and in silico approaches, we demonstrate that eYFP compromises the ability of MinE to displace MinC from MinD, to stimulate MinD ATPase activity and to directly bind to the membrane. Moreover, we reveal that MinE-eYFP is prone to aggregation. In silico analyses predict that other fluorescent proteins are also likely to compromise several functionalities of MinE, suggesting that the results presented here are not specific to eYFP.

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Composition of the λ plasmid heritable replicationcomplex

Biochemical Journal ◽

10.1042/bj20011488 ◽

2002 ◽

Vol 364 (3) ◽

pp. 857-862 ◽

Cited By ~ 10

Author(s):

Katarzyna POTRYKUS ◽

Sylwia BARAŃSKA ◽

Alicja WĘGRZYN ◽

Grzegorz WĘGRZYN

Keyword(s):

Escherichia Coli ◽

Saccharomyces Cerevisiae ◽

Protein Synthesis ◽

Plasmid Dna ◽

Pcr Analysis ◽

Cross Linking ◽

Bacteriophage Λ ◽

Yeast Saccharomyces Cerevisiae ◽

Replication Complex

Previous studies indicated during replication of plasmids derived from bacteriophage λ (the so-called λ plasmids), that, once assembled, replication complex can be inherited by one of the two daughter plasmid copies after each replication round, and may function in subsequent replication rounds. It seems that similar processes occur during replication of other DNA molecules, including chromosomes of the yeast Saccharomyces cerevisiae. However, apart from some suggestions based on genetic experiments, composition of the λ heritable replication complex remains unknown. In amino acid-starved Escherichia coli relA mutants, replication of λ plasmid DNA is carried out exclusively by the heritable replication complex as assembly of new complexes is impaired due to inhibition of protein synthesis. Here, using a procedure based on in vivo cross-linking, cell lysis, immunoprecipitation with specific sera, de-cross-linking and PCR analysis, we demonstrate that the λ heritable replication complex consists of O, P, DnaB and, perhaps surprisingly, DnaK proteins.

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Expression of the Escherichia coli dam methylase in Saccharomyces cerevisiae: effect of in vivo adenine methylation on genetic recombination and mutation.

Molecular and Cellular Biology ◽

10.1128/mcb.5.4.610 ◽

1985 ◽

Vol 5 (4) ◽

pp. 610-618 ◽

Cited By ~ 22

Author(s):

M F Hoekstra ◽

R E Malone

Keyword(s):

Escherichia Coli ◽

Saccharomyces Cerevisiae ◽

Genetic Recombination ◽

Shuttle Vector ◽

Yeast Cells ◽

Adenine Methylation ◽

Dna Adenine Methylase ◽

Allele Specific ◽

Dam Methylase

The Escherichia coli DNA adenine methylase (dam) gene has been introduced into Saccharomyces cerevisiae on a yeast-E. coli shuttle vector. Sau3AI, MboI, and DpnI restriction enzyme digests and Southern hybridization analysis indicated that the dam gene is expressed in yeast cells and methylates GATC sequences. Analysis of digests of total genomic DNA indicated that some GATC sites are not sensitive to methylation. The failure to methylate may reflect an inaccessibility to the methylase due to chromosome structure. The effects of this in vivo methylation on the processes of recombination and mutation in mitotic cells were determined. A small but definite general increase was found in the frequency of mitotic recombination. A similar increase was observed for reversion of some auxotrophic markers; other markers demonstrated a small decrease in mutation frequency. The effects on mutation appear to be locus (or allele) specific. Recombination in meiotic cells was measured and was not detectably altered by the presence of 6-methyladenine in GATC sequences.

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Visualization of Periplasmic and Cytoplasmic Proteins with a Self-Labeling Protein Tag

Journal of Bacteriology ◽

10.1128/jb.00864-15 ◽

2016 ◽

Vol 198 (7) ◽

pp. 1035-1043 ◽

Cited By ~ 35

Author(s):

Na Ke ◽

Dirk Landgraf ◽

Johan Paulsson ◽

Mehmet Berkmen

Keyword(s):

Escherichia Coli ◽

Fluorescent Protein ◽

Fluorescent Proteins ◽

Living Cells ◽

Functional Protein ◽

Content Type ◽

Additional Tool

ABSTRACTThe use of fluorescent and luminescent proteins in visualizing proteins has become a powerful tool in understanding molecular and cellular processes within living organisms. This success has resulted in an ever-increasing demand for new and more versatile protein-labeling tools that permit light-based detection of proteins within living cells. In this report, we present data supporting the use of the self-labeling HaloTag protein as a light-emitting reporter for protein fusions within the model prokaryoteEscherichia coli. We show that functional protein fusions of the HaloTag can be detected bothin vivoandin vitrowhen expressed within the cytoplasmic or periplasmic compartments ofE. coli. The capacity to visually detect proteins localized in various prokaryotic compartments expands today's molecular biologist toolbox and paves the path to new applications.IMPORTANCEVisualizing proteins microscopically within living cells is important for understanding both the biology of cells and the role of proteins within living cells. Currently, the most common tool is green fluorescent protein (GFP). However, fluorescent proteins such as GFP have many limitations; therefore, the field of molecular biology is always in need of new tools to visualize proteins. In this paper, we demonstrate, for the first time, the use of HaloTag to visualize proteins in two different compartments within the model prokaryoteEscherichia coli. The use of HaloTag as an additional tool to visualize proteins within prokaryotes increases our capacity to ask about and understand the role of proteins within living cells.

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Recombinant RquA catalyzes the in vivo conversion of ubiquinone to rhodoquinone in Escherichia coli and Saccharomyces cerevisiae

Biochimica et Biophysica Acta (BBA) - Molecular and Cell Biology of Lipids ◽

10.1016/j.bbalip.2019.05.007 ◽

2019 ◽

Vol 1864 (9) ◽

pp. 1226-1234 ◽

Cited By ~ 9

Author(s):

Ann C. Bernert ◽

Evan J. Jacobs ◽

Samantha R. Reinl ◽

Christina C.Y. Choi ◽

Paloma M. Roberts Buceta ◽

...

Keyword(s):

Escherichia Coli ◽

Saccharomyces Cerevisiae

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Anatomy of a twin DNA replication factory

Biochemical Society Transactions ◽

10.1042/bst20200640 ◽

2020 ◽

Vol 48 (6) ◽

pp. 2769-2778

Author(s):

Huilin Li ◽

Nina Y. Yao ◽

Michael E. O'Donnell

Keyword(s):

Escherichia Coli ◽

Saccharomyces Cerevisiae ◽

Bacillus Subtilis ◽

Dna Replication ◽

In Vivo Studies ◽

Replication Forks ◽

Structural Studies ◽

Replication Factory ◽

Higher Eukaryotes

The replication of DNA in chromosomes is initiated at sequences called origins at which two replisome machines are assembled at replication forks that move in opposite directions. Interestingly, in vivo studies observe that the two replication forks remain fastened together, often referred to as a replication factory. Replication factories containing two replisomes are well documented in cellular studies of bacteria (Escherichia coli and Bacillus subtilis) and the eukaryote, Saccharomyces cerevisiae. This basic twin replisome factory architecture may also be preserved in higher eukaryotes. Despite many years of documenting the existence of replication factories, the molecular details of how the two replisome machines are tethered together has been completely unknown in any organism. Recent structural studies shed new light on the architecture of a eukaryote replisome factory, which brings with it a new twist on how a replication factory may function.

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Improving 3-methylphenol (m-cresol) production in yeast via in vivo glycosylation or methylation

FEMS Yeast Research ◽

10.1093/femsyr/foaa063 ◽

2020 ◽

Vol 20 (8) ◽

Author(s):

Julia Hitschler ◽

Eckhard Boles

Keyword(s):

Saccharomyces Cerevisiae ◽

De Novo ◽

Wild Type ◽

Biotechnological Production ◽

Yeast Saccharomyces Cerevisiae ◽

In Situ Extraction ◽

Methylsalicylic Acid Synthase ◽

In The Wild

ABSTRACT Heterologous expression of 6-methylsalicylic acid synthase (MSAS) together with 6-MSA decarboxylase enables de novo production of the platform chemical and antiseptic additive 3-methylphenol (3-MP) in the yeast Saccharomyces cerevisiae. However, toxicity of 3-MP prevents higher production levels. In this study, we evaluated in vivo detoxification strategies to overcome limitations of 3-MP production. An orcinol-O-methyltransferase from Chinese rose hybrids (OOMT2) was expressed in the 3-MP producing yeast strain to convert 3-MP to 3-methylanisole (3-MA). Together with in situ extraction by dodecane of the highly volatile 3-MA this resulted in up to 211 mg/L 3-MA (1.7 mM) accumulation. Expression of a UDP-glycosyltransferase (UGT72B27) from Vitis vinifera led to the synthesis of up to 533 mg/L 3-MP as glucoside (4.9 mM). Conversion of 3-MP to 3-MA and 3-MP glucoside was not complete. Finally, deletion of phosphoglucose isomerase PGI1 together with methylation or glycosylation and feeding a fructose/glucose mixture to redirect carbon fluxes resulted in strongly increased product titers, with up to 897 mg/L 3-MA/3-MP (9 mM) and 873 mg/L 3-MP/3-MP as glucoside (8.1 mM) compared to less than 313 mg/L (2.9 mM) product titers in the wild type controls. The results show that methylation or glycosylation are promising tools to overcome limitations in further enhancing the biotechnological production of 3-MP.

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Structure of hibernating ribosomes studied by cryoelectron tomography in vitro and in situ

The Journal of Cell Biology ◽

10.1083/jcb.201005007 ◽

2010 ◽

Vol 190 (4) ◽

pp. 613-621 ◽

Cited By ~ 67

Author(s):

Julio O. Ortiz ◽

Florian Brandt ◽

Valério R.F. Matias ◽

Lau Sennels ◽

Juri Rappsilber ◽

...

Keyword(s):

Escherichia Coli ◽

Stress Response ◽

Spatial Organization ◽

Three Dimensional ◽

E Coli ◽

Escherichia Coli Cells ◽

Three Dimensional Configuration

Ribosomes arranged in pairs (100S) have been related with nutritional stress response and are believed to represent a “hibernation state.” Several proteins have been identified that are associated with 100S ribosomes but their spatial organization has hitherto not been characterized. We have used cryoelectron tomography to reveal the three-dimensional configuration of 100S ribosomes isolated from starved Escherichia coli cells and we have described their mode of interaction. In situ studies with intact E. coli cells allowed us to demonstrate that 100S ribosomes do exist in vivo and represent an easily reversible state of quiescence; they readily vanish when the growth medium is replenished.

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Single-molecule imaging of electroporated dye-labelled CheY in live Escherichia coli

Philosophical Transactions of the Royal Society B Biological Sciences ◽

10.1098/rstb.2015.0492 ◽

2016 ◽

Vol 371 (1707) ◽

pp. 20150492 ◽

Cited By ~ 7

Author(s):

Diana Di Paolo ◽

Oshri Afanzar ◽

Judith P. Armitage ◽

Richard M. Berry

Keyword(s):

Escherichia Coli ◽

Single Molecule ◽

Organic Dyes ◽

Fluorescent Proteins ◽

Response Regulator ◽

Single Molecule Level ◽

Flagellar Motors ◽

Regulator Protein ◽

Response Regulator Protein

For the past two decades, the use of genetically fused fluorescent proteins (FPs) has greatly contributed to the study of chemotactic signalling in Escherichia coli including the activation of the response regulator protein CheY and its interaction with the flagellar motor. However, this approach suffers from a number of limitations, both biological and biophysical: for example, not all fusions are fully functional when fused to a bulky FP, which can have a similar molecular weight to its fused counterpart; they may interfere with the native interactions of the protein and the chromophores of FPs have low brightness and photostability and fast photobleaching rates. A recently developed technique for the electroporation of fluorescently labelled proteins in live bacteria has enabled us to bypass these limitations and study the in vivo behaviour of CheY at the single-molecule level. Here we show that purified CheY proteins labelled with organic dyes can be internalized into E. coli cells in controllable concentrations and imaged with video fluorescence microscopy. The use of this approach is illustrated by showing single CheY molecules diffusing within cells and interacting with the sensory clusters and the flagellar motors in real time. This article is part of the themed issue ‘The new bacteriology’.

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