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Functional dynamics of glycosyltransferases: Solution-state NMR studies of peripheral membrane proteins involved in glycolipid biosynthesis in bacteria
Stockholm University, Faculty of Science, Department of Biochemistry and Biophysics.ORCID iD: 0000-0003-1559-5441
2023 (English)Doctoral thesis, comprehensive summary (Other academic)
Abstract [en]

Antibiotic resistance is an existential threat enabled by bacterial adaptation and fuelled by inappropriate use of medication. The ensuing shortage of effective treatments has led to a rise in deaths linked to resistant bacterial pathogens. Disrupting cell wall biosynthesis can undermine bacterial defences, so new insights into the dynamic function of the enzymes involved could facilitate new therapies.

Glycosyltransferases (GTs), enzymes forming glycosidic bonds, build molecules by transferring a sugar group from a donor to an acceptor. In Gram-negative bacteria, an enzymatic assembly line constructs membrane-anchored virulence factor lipopolysaccharide (LPS), which dominates the outer membrane, forming a protective layer. In mycobacteria, phosphatidyl-myo-inositol mannosides (PIMs) ensure the stability and impermeability of the inner membrane, and are constructed by a similar array of enzymes. In this thesis, bacterial GTs that work at the cytoplasmic leaflet of the inner membrane were investigated.

PimA is an essential mycobacterial enzyme involved in constructing PIMs. It exists in multiple conformations, implying that it undergoes complex conformational changes, including a fold-switch. Associated motions were characterised with NMR dynamics experiments, revealing donor substrate-dependent population shifts and dynamic changes. At least four different states co-exist in solution, regardless of whether or not the enzyme is bound to substrate.

WaaG performs one step in the biosynthesis of LPS in bacteria including E. coli and P.  aeruginosa. As it is not an essential enzyme, EcWaaG-deficient E. coli survive, but are more vulnerable to antibiotics. 19F NMR was employed to detect conformational and dynamic changes in EcWaaG. Upon interaction with bicelle-bound lipids and its donor substrate, UDP-glucose, EcWaaG was shown to experience a dynamic change, while a part of the protein was shown to experience slow conformational change. Hydrolysis of the donor substrate was quantified using 31P NMR. WaaG from P. aeruginosa was also investigated, focusing on the functional mechanism. NMR experiments determined that only UDP-GalNAc was hydrolysed by PaWaaG. When the active site was mutated to resemble that of EcWaaG, it was shown by 31P NMR that the mutated enzyme instead hydrolysed the donor substrate of EcWaaG, UDP-glucose. However, PaWaaG cannot be substituted for EcWaaG in vivo, underlining the importance of the interaction with the lipid-bound acceptor substrate.

Both WaaG and PimA function adjacent to membrane. As larger objects give rise to broader signals, solution-state NMR imposes constraints on the detection of protein-lipid interactions. Small membrane mimetics like lipid bicelles can be used to mimic a membrane, but while they permit detection of effects on protein signals, detecting the effects on lipid signals requires further optimization, as further concentration-dependent challenges arise in multi-component experiments. Thus, lipid dynamics in bicelles designed to exist at low concentrations were characterized using 1H and 13C NMR. Upon binding spin-labelled PimA, paramagnetic relaxation enhancement of the lipids could be observed.

This thesis thus widens the toolkit available to study membrane-associated proteins. It demonstrates that, far from being static structures, biomolecules like lipids and proteins are highly flexible objects whose function can only be understood if dynamics are taken into account.
Place, publisher, year, edition, pages
Stockholm: Department of Biochemistry and Biophysics, Stockholm University , 2023. , p. 68
National Category
Biophysics
Research subject
Biophysics
Identifiers
URN: urn:nbn:se:su:diva-220528ISBN: 978-91-8014-474-2 (print)ISBN: 978-91-8014-475-9 (electronic)OAI: oai:DiVA.org:su-220528DiVA, id: diva2:1792872
Public defence
2023-10-13, Magnélisalen, Kemiska övningslaboratoriet, Svante Arrhenius väg 16B, Stockholm, 14:00 (English)
Opponent
Supervisors
Available from: 2023-09-20 Created: 2023-08-30 Last updated: 2025-02-20Bibliographically approved
List of papers
1. Unveiling the activation dynamics of a fold-switch bacterial glycosyltransferase by 19F NMR
Open this publication in new window or tab >>Unveiling the activation dynamics of a fold-switch bacterial glycosyltransferase by 19F NMR
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2020 (English)In: Journal of Biological Chemistry, ISSN 0021-9258, E-ISSN 1083-351X, Vol. 295, no 29, p. 9868-9878Article in journal (Refereed) Published
Abstract [en]

Fold-switch pathways remodel the secondary structure topology of proteins in response to the cellular environment. It is a major challenge to understand the dynamics of these folding processes. Here, we conducted an in-depth analysis of the α-helix–to–β-strand and β-strand–to–α-helix transitions and domain motions displayed by the essential mannosyltransferase PimA from mycobacteria. Using 19F NMR, we identified four functionally relevant states of PimA that coexist in dynamic equilibria on millisecond-to-second timescales in solution. We discovered that fold-switching is a slow process, on the order of seconds, whereas domain motions occur simultaneously but are substantially faster, on the order of milliseconds. Strikingly, the addition of substrate accelerated the fold-switching dynamics of PimA. We propose a model in which the fold-switching dynamics constitute a mechanism for PimA activation.
Keywords
protein structure, protein fold-switching, protein dynamics, conformational dynamics, protein function, enzyme catalysis, F-19 NMR, relaxation dispersion, carbohydrate active enzymes, glycosyltransferases
National Category
Biological Sciences
Identifiers
urn:nbn:se:su:diva-184456 (URN)10.1074/jbc.RA120.014162 (DOI)000553333300008 ()32434931 (PubMedID)
Available from: 2020-10-23 Created: 2020-10-23 Last updated: 2023-09-01Bibliographically approved
2. Lipid- and substrate-induced conformational and dynamic changes in a glycosyltransferase involved in E. coli LPS synthesis revealed by 19F and 31P NMR
Open this publication in new window or tab >>Lipid- and substrate-induced conformational and dynamic changes in a glycosyltransferase involved in E. coli LPS synthesis revealed by 19F and 31P NMR
2023 (English)In: Biochimica et Biophysica Acta - Biomembranes, ISSN 0005-2736, E-ISSN 1879-2642, Vol. 1865, no 8, article id 184209Article in journal (Refereed) Published
Abstract [en]

WaaG is a glycosyltransferase (GT) involved in the synthesis of the bacterial cell wall, and in Escherichia coli it catalyzes the transfer of a glucose moiety from the donor substrate UDP-glucose onto the nascent lipopolysaccharide (LPS) molecule which when completed constitutes the major component of the bacterium's outermost defenses. Similar to other GTs of the GT-B fold, having two Rossman-like domains connected by a short linker, WaaG is believed to undergo complex inter-domain motions as part of its function to accommodate the nascent LPS and UDP-glucose in the catalytic site located in the cleft between the two domains. As the nascent LPS is bulky and membrane-bound, WaaG is a peripheral membrane protein, adding to the complexity of studying the enzyme in a biologically relevant environment. Using specific 5-fluoro-Trp labelling of native and inserted tryptophans and 19F NMR we herein studied the dynamic interactions of WaaG with lipids using bicelles, and with the donor substrate. Line-shape changes when bicelles are added to WaaG show that the dynamic behavior is altered when binding to the model membrane, while a chemical shift change indicates an altered environment around a tryptophan located in the C-terminal domain of WaaG upon interaction with UDP-glucose or UDP. A lipid-bound paramagnetic probe was used to confirm that the membrane interaction is mediated by a loop region located in the N-terminal domain. Furthermore, the hydrolysis of the donor substrate by WaaG was quantified by 31P NMR.
Keywords
glycosyltransferase, membrane interaction, substrate interaction, solution NMR, bicelle, lipids
National Category
Biophysics
Research subject
Biophysics
Identifiers
urn:nbn:se:su:diva-220488 (URN)10.1016/j.bbamem.2023.184209 (DOI)001070814300001 ()37558175 (PubMedID)2-s2.0-85169551058 (Scopus ID)
Funder
Swedish Research Council, 621-2018-03395
Available from: 2023-08-29 Created: 2023-08-29 Last updated: 2025-02-20Bibliographically approved
3. Structural and functional insights into the Pseudomonas aeruginosa glycosyltransferase WaaG and the implications for lipopolysaccharide biosynthesis
Open this publication in new window or tab >>Structural and functional insights into the Pseudomonas aeruginosa glycosyltransferase WaaG and the implications for lipopolysaccharide biosynthesis
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2023 (English)In: Journal of Biological Chemistry, ISSN 0021-9258, E-ISSN 1083-351X, Vol. 299, no 10, article id 105256Article in journal (Refereed) Published
Abstract [en]

The glycosyltransferase WaaG in Pseudomonas aeruginosa (PaWaaG) is involved in the synthesis of the core region of lipopolysaccharides. It is a promising target for developing adjuvants that could help in the uptake of antibiotics. Herein, we have determined structures of PaWaaG in complex with the nucleotide-sugars UDP-glucose, UDP-galactose, and UDP-GalNAc. Structural comparison with the homolog from Escherichia coli (EcWaaG) revealed five key differences in the sugar-binding pocket. Solution-state NMR analysis showed that WT PaWaaG specifically hydrolyzes UDP-GalNAc and unlike EcWaaG, does not hydrolyze UDP-glucose. Furthermore, we found that a PaWaaG mutant (Y97F/T208R/N282A/T283A/T285I) designed to resemble the EcWaaG sugar binding site, only hydrolyzed UDP-glucose, underscoring the importance of the identified amino acids in substrate specificity. However, neither WT PaWaaG nor the PaWaaG mutant capable of hydrolyzing UDP-glucose was able to complement an E. coli ΔwaaG strain, indicating that more remains to be uncovered about the function of PaWaaG in vivo. This structural and biochemical information will guide future structure-based drug design efforts targeting PaWaaG.
Keywords
Pseudomonas aeruginosa, WaaG, glycosyltransferase, lipopolysaccharide, X-ray crystallography, NMR
National Category
Structural Biology
Research subject
Biochemistry
Identifiers
urn:nbn:se:su:diva-220525 (URN)10.1016/j.jbc.2023.105256 (DOI)001166256400001 ()37716703 (PubMedID)2-s2.0-85173583816 (Scopus ID)
Funder
Swedish Research Council, 2022-03681Swedish Cancer Society, 20 1287 PjFNovo Nordisk Foundation, 0071844Carl Tryggers foundation , CTS 21:1637Swedish Research Council, 2022-03014Knut and Alice Wallenberg FoundationSwedish Research Council, 2018-03395
Available from: 2023-08-30 Created: 2023-08-30 Last updated: 2024-10-02Bibliographically approved
4. Dilute Bicelles for Glycosyltransferase Studies, Novel Bicelles with Phosphatidylinositol
Open this publication in new window or tab >>Dilute Bicelles for Glycosyltransferase Studies, Novel Bicelles with Phosphatidylinositol
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2022 (English)In: Journal of Physical Chemistry B, ISSN 1520-6106, E-ISSN 1520-5207, Vol. 126, no 30, p. 5655-5666Article in journal (Refereed) Published
Abstract [en]

Solution-state NMR can be used to study protein–lipid interactions, in particular, the effect that proteins have on lipids. One drawback is that only small assemblies can be studied, and therefore, fast-tumbling bicelles are commonly used. Bicelles contain a lipid bilayer that is solubilized by detergents. A complication is that they are only stable at high concentrations, exceeding the CMC of the detergent. This issue has previously been addressed by introducing a detergent (Cyclosfos-6) with a substantially lower CMC. Here, we developed a set of bicelles using this detergent for studies of membrane-associated mycobacterial proteins, for example, PimA, a key enzyme for bacterial growth. To mimic the lipid composition of mycobacterial membranes, PI, PG, and PC lipids were used. Diffusion NMR was used to characterize the bicelles, and spin relaxation was used to measure the dynamic properties of the lipids. The results suggest that bicelles are formed, although they are smaller than “conventional” bicelles. Moreover, we studied the effect of MTSL-labeled PimA on bicelles containing PI and PC. The paramagnetic label was shown to have a shallow location in the bicelle, affecting the glycerol backbone of the lipids. We foresee that these bicelles will be useful for detailed studies of protein–lipid interactions. 
National Category
Chemical Sciences
Identifiers
urn:nbn:se:su:diva-207911 (URN)10.1021/acs.jpcb.2c02327 (DOI)000834242900001 ()35880265 (PubMedID)2-s2.0-85135596847 (Scopus ID)
Available from: 2022-08-23 Created: 2022-08-23 Last updated: 2024-11-06Bibliographically approved

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