Activity-Related Conformational Changes in d,d-Carboxypeptidases Revealed by In Vivo Periplasmic Förster Resonance Energy Transfer Assay in Escherichia coli

ABSTRACT One of the mechanisms of β-lactam antibiotic resistance requires the activity of d,d-carboxypeptidases (d,d-CPases) involved in peptidoglycan (PG) synthesis, making them putative targets for new antibiotic development. The activity of PG-synthesizing enzymes is often correlated with their association with other proteins. The PG layer is maintained in the periplasm between the two membranes of the Gram-negative cell envelope. Because no methods existed to detect in vivo interactions in this compartment, we have developed and validated a Förster resonance energy transfer assay. Using the fluorescent-protein donor-acceptor pair mNeonGreen-mCherry, periplasmic protein interactions were detected in fixed and in living bacteria, in single samples or in plate reader 96-well format. We show that the d,d-CPases PBP5, PBP6a, and PBP6b of Escherichia coli change dimer conformation between resting and active states. Complementation studies and changes in localization suggest that these d,d-CPases are not redundant but that their balanced activity is required for robust PG synthesis. IMPORTANCE The periplasmic space between the outer and the inner membrane of Gram-negative bacteria contains many essential regulatory, transport, and cell wall-synthesizing and -hydrolyzing proteins. To date, no assay is available to determine protein interactions in this compartment. We have developed a periplasmic protein interaction assay for living and fixed bacteria in single samples or 96-well-plate format. Using this assay, we were able to demonstrate conformation changes related to the activity of proteins that could not have been detected by any other living-cell method available. The assay uniquely expands our toolbox for antibiotic screening and mode-of-action studies. IMPORTANCE The periplasmic space between the outer and the inner membrane of Gram-negative bacteria contains many essential regulatory, transport, and cell wall-synthesizing and -hydrolyzing proteins. To date, no assay is available to determine protein interactions in this compartment. We have developed a periplasmic protein interaction assay for living and fixed bacteria in single samples or 96-well-plate format. Using this assay, we were able to demonstrate conformation changes related to the activity of proteins that could not have been detected by any other living-cell method available. The assay uniquely expands our toolbox for antibiotic screening and mode-of-action studies.

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Measuring ligand-dependent and ligand-independent interactions between nuclear receptors and associated proteins using Bioluminescence Resonance Energy Transfer (BRET2)

Nuclear Receptor Signaling ◽

10.1621/nrs.04021 ◽

2006 ◽

Vol 4 (1) ◽

pp. nrs.04021 ◽

Cited By ~ 14

Author(s):

Kristen L. Koterba ◽

Brian G. Rowan

Keyword(s):

Energy Transfer ◽

Protein Interactions ◽

Fusion Proteins ◽

Fluorescent Protein ◽

Resonance Energy Transfer ◽

Resonance Energy ◽

Renilla Luciferase ◽

Receptor Protein ◽

Protein Protein Interactions

Bioluminescent resonance energy transfer (BRET2) is a recently developed technology for the measurement of protein-protein interactions in a live, cell-based system. BRET2 is characterized by the efficient transfer of excited energy between a bioluminescent donor molecule (Renilla luciferase) and a fluorescent acceptor molecule (a mutant of Green Fluorescent Protein (GFP2)). The BRET2 assay offers advantages over fluorescence resonance energy transfer (FRET) because it does not require an external light source thereby eliminating problems of photobleaching and autoflourescence. The absence of contamination by light results in low background that permits detection of very small changes in the BRET2 signal. BRET2 is dependent on the orientation and distance between two fusion proteins and therefore requires extensive preliminary standardization experiments to conclude a positive BRET2 signal independent of variations in protein titrations and arrangement in tertiary structures. Estrogen receptor (ER) signaling is modulated by steroid receptor coactivator 1 (SRC-1). To establish BRET2 in a ligand inducible system we used SRC-1 as the donor moiety and ER as the acceptor moiety. Expression and functionality of the fusion proteins were assessed by transient transfection in HEK-293 cells followed by Western blot analysis and measurement of ER-dependent reporter gene activity. These preliminary determinations are required prior to measuring nuclear receptor protein-protein interactions by BRET2. This article describes in detail the BRET2 methodology for measuring interaction between full-length ER and coregulator proteins in real-time, in an in vivo environment.

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Discs large 1 controls daughter-cell polarity after cytokinesis in vertebrate morphogenesis

Proceedings of the National Academy of Sciences ◽

10.1073/pnas.1713959115 ◽

2018 ◽

Vol 115 (46) ◽

pp. E10859-E10868 ◽

Cited By ~ 5

Author(s):

Yuwei Li ◽

Jason A. Junge ◽

Cosimo Arnesano ◽

Garrett G. Gross ◽

Jeffrey H. Miner ◽

...

Keyword(s):

Cell Polarity ◽

Protein Interactions ◽

Protein Function ◽

Resonance Energy Transfer ◽

Resonance Energy ◽

Explant Culture ◽

Scaffolding Protein ◽

Fluorescence Lifetime Imaging ◽

Discs Large

Vertebrate embryogenesis and organogenesis are driven by cell biological processes, ranging from mitosis and migration to changes in cell size and polarity, but their control and causal relationships are not fully defined. Here, we use the developing limb skeleton to better define the relationships between mitosis and cell polarity. We combine protein-tagging and -perturbation reagents with advanced in vivo imaging to assess the role of Discs large 1 (Dlg1), a membrane-associated scaffolding protein, in mediating the spatiotemporal relationship between cytokinesis and cell polarity. Our results reveal that Dlg1 is enriched at the midbody during cytokinesis and that its multimerization is essential for the normal polarity of daughter cells. Defects in this process alter tissue dimensions without impacting other cellular processes. Our results extend the conventional view that division orientation is established at metaphase and anaphase and suggest that multiple mechanisms act at distinct phases of the cell cycle to transmit cell polarity. The approach employed can be used in other systems, as it offers a robust means to follow and to eliminate protein function and extends the Phasor approach for studying in vivo protein interactions by frequency-domain fluorescence lifetime imaging microscopy of Förster resonance energy transfer (FLIM-FRET) to organotypic explant culture.

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Detection of in vivo Protein Interactions in All Bacterial Components by Förster Resonance Energy Transfer with the Superfolder mTurquoise2 ox-mNeongreen FRET Pair

BIO-PROTOCOL ◽

10.21769/bioprotoc.3448 ◽

2019 ◽

Vol 9 (23) ◽

Author(s):

Nils Meiresonne ◽

Elisa Consoli ◽

Laureen Mertens ◽

Tanneke den Blaauwen

Keyword(s):

Energy Transfer ◽

Protein Interactions ◽

Resonance Energy Transfer ◽

Resonance Energy ◽

Fret Pair

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Fluorescence resonance energy transfer in revealing protein–protein interactions in living cells

Emerging Topics in Life Sciences ◽

10.1042/etls20200337 ◽

2021 ◽

Author(s):

Sukesh R. Bhaumik

Keyword(s):

Single Cell ◽

Protein Interactions ◽

Resonance Energy Transfer ◽

Resonance Energy ◽

Living Cells ◽

Biological Processes ◽

Protein Protein Interactions ◽

Functional Mechanisms

Genes are expressed to proteins for a wide variety of fundamental biological processes at the cellular and organismal levels. However, a protein rarely functions alone, but rather acts through interactions with other proteins to maintain normal cellular and organismal functions. Therefore, it is important to analyze the protein–protein interactions to determine functional mechanisms of proteins, which can also guide to develop therapeutic targets for treatment of diseases caused by altered protein–protein interactions leading to cellular/organismal dysfunctions. There is a large number of methodologies to study protein interactions in vitro, in vivo and in silico, which led to the development of many protein interaction databases, and thus, have enriched our knowledge about protein–protein interactions and functions. However, many of these interactions were identified in vitro, but need to be verified/validated in living cells. Furthermore, it is unclear whether these interactions are direct or mediated via other proteins. Moreover, these interactions are representative of cell- and time-average, but not a single cell in real time. Therefore, it is crucial to detect direct protein–protein interactions in a single cell during biological processes in vivo, towards understanding the functional mechanisms of proteins in living cells. Importantly, a fluorescence resonance energy transfer (FRET)-based methodology has emerged as a powerful technique to decipher direct protein–protein interactions at a single cell resolution in living cells, which is briefly described in a limited available space in this mini-review.

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Analysis of Protein Interactions In Vivo with Fluorescence Resonance Energy Transfer (FRET)

Cold Spring Harbor Protocols ◽

10.1101/pdb.prot4581 ◽

2006 ◽

Vol 2006 (28) ◽

pp. pdb.prot4581-pdb.prot4581 ◽

Cited By ~ 2

Author(s):

M. Damelin ◽

P. Silver

Keyword(s):

Energy Transfer ◽

Fluorescence Resonance Energy Transfer ◽

Protein Interactions ◽

Resonance Energy Transfer ◽

Resonance Energy ◽

Fluorescence Resonance

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Thanatin targets the intermembrane protein complex required for lipopolysaccharide transport inEscherichia coli

Science Advances ◽

10.1126/sciadv.aau2634 ◽

2018 ◽

Vol 4 (11) ◽

pp. eaau2634 ◽

Cited By ~ 33

Author(s):

Stefan U. Vetterli ◽

Katja Zerbe ◽

Maik Müller ◽

Matthias Urfer ◽

Milon Mondal ◽

...

Keyword(s):

Protein Interactions ◽

Macromolecular Complex ◽

Gram Negative Bacteria ◽

Periplasmic Protein ◽

Protein Protein Interactions ◽

Inner Membrane ◽

Gram Negative ◽

Research Priority ◽

Naturally Occurring ◽

Bacterial Outer Membrane

With the increasing resistance of many Gram-negative bacteria to existing classes of antibiotics, identifying new paradigms in antimicrobial discovery is an important research priority. Of special interest are the proteins required for the biogenesis of the asymmetric Gram-negative bacterial outer membrane (OM). Seven Lpt proteins (LptA to LptG) associate in most Gram-negative bacteria to form a macromolecular complex spanning the entire envelope, which transports lipopolysaccharide (LPS) molecules from their site of assembly at the inner membrane to the cell surface, powered by adenosine 5′-triphosphate hydrolysis in the cytoplasm. The periplasmic protein LptA comprises the protein bridge across the periplasm, which connects LptB2FGC at the inner membrane to LptD/E anchored in the OM. We show here that the naturally occurring, insect-derived antimicrobial peptide thanatin targets LptA and LptD in the network of periplasmic protein-protein interactions required to assemble the Lpt complex, leading to the inhibition of LPS transport and OM biogenesis inEscherichia coli.

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In vivo detection of RNA-binding protein interactions with cognate RNA sequences by fluorescence resonance energy transfer

RNA ◽

10.1261/rna.1678209 ◽

2009 ◽

Vol 15 (11) ◽

pp. 2063-2071 ◽

Cited By ~ 15

Author(s):

M. Huranova ◽

J. A. Jablonski ◽

A. Benda ◽

M. Hof ◽

D. Stanek ◽

...

Keyword(s):

Energy Transfer ◽

Fluorescence Resonance Energy Transfer ◽

Protein Interactions ◽

Rna Binding ◽

Rna Binding Protein ◽

Resonance Energy Transfer ◽

Resonance Energy ◽

Rna Sequences ◽

In Vivo Detection

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Oligomerization of the UDP-glucuronosyltransferase 1A Proteins

Journal of Biological Chemistry ◽

10.1074/jbc.m609417200 ◽

2006 ◽

Vol 282 (7) ◽

pp. 4821-4829 ◽

Cited By ~ 53

Author(s):

Theresa N. Operaña ◽

Robert H. Tukey

Keyword(s):

Protein Interactions ◽

Fluorescent Protein ◽

Resonance Energy Transfer ◽

Resonance Energy ◽

Conclusive Evidence ◽

Live Cells ◽

Protein Protein Interactions ◽

Dietary Nutrients ◽

Membrane Bound

UDP-glucuronosyltransferases (UGTs) are membrane-bound proteins localized to the endoplasmic reticulum and catalyze the formation of β-d-glucopyranosiduronic acids (glucuronides) using UDP-glucuronic acid and acceptor substrates such as drugs, steroids, bile acids, xenobiotics, and dietary nutrients. Recent biochemical evidence indicates that the UGT proteins may oligomerize in the membrane, but conclusive evidence is still lacking. In the present study, we have used fluorescence resonance energy transfer (FRET) to study UGT1A oligomerization in live cells. This technique demonstrated that UGT1A1, UGT1A3, UGT1A4, UGT1A6, UGT1A7, UGT1A8, UGT1A9, and UGT1A10 self-oligomerize (homodimerize). Heterodimer interactions were also explored, and it was determined that UGT1A1 was capable of binding with UGT1A3, UGT1A4, UGT1A6, UGT1A7, UGT1A8, UGT1A9, and UGT1A10. In addition to the in vivo FRET analysis, UGT1A protein-protein interactions were demonstrated through co-immunoprecipitation experiments. Co-expression of hemagglutinin-tagged and cyan fluorescent protein-tagged UGT1A proteins, followed by immunoprecipitation with anti-hemagglutinin beads, illustrated the potential of each UGT1A protein to homodimerize. Co-immunoprecipitation results also confirmed that UGT1A1 was capable of forming heterodimer complexes with all of the UGT1A proteins, corroborating the FRET results in live cells. These preliminary studies suggest that the UGT1A family of proteins form oligomerized complexes in the membrane, a property that may influence function and substrate selectivity.

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