Exploring protein–protein interactions and oligomerization state of pulmonary surfactant protein C (SP-C) through FRET and fluorescence self-quenching

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dc.contributor.authorMorán Lalangui, Juranny Michelle
dc.contributor.authorCoutinho, Ana
dc.contributor.authorPrieto, Manuel
dc.contributor.authorFedorov, Alexander
dc.contributor.authorPérez Gil, Jesús
dc.contributor.authorLoura, Luís M. S.
dc.contributor.authorGarcía Álvarez, María Begoña
dc.date.accessioned2024-07-01T15:30:25Z
dc.date.available2024-07-01T15:30:25Z
dc.date.issued2023-12-20
dc.descriptionAcknowledgments: FPI fellowship from the Spanish Ministry of Science and Innovation. COMPETE2020-Operational Program for Competitiveness and Internationalization, funding by the European Regional Development Fund. This work has been supported by a working visit bursary from EBSA.
dc.description.abstractPulmonary surfactant (PS) is a lipid–protein complex that forms films reducing surface tension at the alveolar air–liquid interface. Surfactant protein C (SP-C) plays a key role in rearranging the lipids at the PS surface layers during breathing. The N-terminal segment of SP-C, a lipopeptide of 35 amino acids, contains two palmitoylated cysteines, which affect the stability and structure of the molecule. The C-terminal region comprises a transmembrane α-helix that contains a ALLMG motif, supposedly analogous to a well-studied dimerization motif in glycophorin A. Previous studies have demonstrated the potential interaction between SP-C molecules using approaches such as Bimolecular Complementation assays or computational simulations. In this work, the oligomerization state of SP-C in membrane systems has been studied using fluorescence spectroscopy techniques. We have performed self-quenching and FRET assays to analyze dimerization of native palmitoylated SP-C and a non-palmitoylated recombinant version of SP-C (rSP-C) using fluorescently labeled versions of either protein reconstituted in different lipid systems mimicking pulmonary surfactant environments. Our results reveal that doubly palmitoylated native SP-C remains primarily monomeric. In contrast, non-palmitoylated recombinant SP-C exhibits dimerization, potentiated at high concentrations, especially in membranes with lipid phase separation. Therefore, palmitoylation could play a crucial role in stabilizing the monomeric α-helical conformation of SP-C. Depalmitoylation, high protein densities as a consequence of membrane compartmentalization, and other factors may all lead to the formation of protein dimers and higher-order oligomers, which could have functional implications under certain pathological conditions and contribute to membrane transformations associated with surfactant metabolism and alveolar homeostasis.
dc.description.departmentDepto. de Bioquímica y Biología Molecular
dc.description.facultyFac. de Ciencias Biológicas
dc.description.facultyFac. de Ciencias Químicas
dc.description.fundingtypeDescuento UCM
dc.description.refereedTRUE
dc.description.sponsorshipMinisterio de Ciencia e Innovación (España)
dc.description.sponsorshipComunidad de Madrid
dc.description.sponsorshipEuropean Commission
dc.description.sponsorshipFundação para a Ciência e a Tecnologia
dc.description.sponsorshipEuropean Biophysical Societies' Association
dc.description.statuspub
dc.identifier.citationMorán-Lalangui M, Coutinho A, Prieto M, Fedorov A, Pérez-Gil J, Loura LMS, et al. Exploring protein–protein interactions and oligomerization state of pulmonary surfactant protein C (SP-C) through FRET and fluorescence self-quenching. Protein Science. 2024; 33(1):e4835.
dc.identifier.doi10.1002/pro.4835
dc.identifier.essn1469-896X
dc.identifier.issn0961-8368
dc.identifier.officialurlhttps://doi.org/10.1002/pro.4835
dc.identifier.relatedurlhttps://onlinelibrary.wiley.com/doi/full/10.1002/pro.4835
dc.identifier.urihttps://hdl.handle.net/20.500.14352/105402
dc.issue.number1
dc.journal.titleProtein Science
dc.language.isoeng
dc.page.final20
dc.page.initial1
dc.publisherWiley
dc.relation.projectIDinfo:eu-repo/grantAgreement/MICINN//PID2021-124932OB-100
dc.relation.projectIDP2018/NMT-4389
dc.relation.projectIDinfo:eu-repo/grantAgreement/FCT//UIDB/00313%2F2020
dc.relation.projectIDinfo:eu-repo/grantAgreement/FCT//UIDB/04565%2F2020
dc.relation.projectIDinfo:eu-repo/grantAgreement/FCT//UIDP/00313%2F2020
dc.relation.projectIDinfo:eu-repo/grantAgreement/FCT//UIDP/04565%2F2020
dc.relation.projectIDinfo:eu-repo/grantAgreement/LA//P/0140%2F2020
dc.rightsAttribution-NonCommercial-NoDerivatives 4.0 Internationalen
dc.rights.accessRightsopen access
dc.rights.urihttp://creativecommons.org/licenses/by-nc-nd/4.0/
dc.subject.cdu577.112
dc.subject.cdu577.2
dc.subject.keywordFRET
dc.subject.keywordOligomerization state
dc.subject.keywordProtein–protein interaction
dc.subject.keywordPulmonary surfactant
dc.subject.keywordSelf-quenching
dc.subject.keywordSurfactant protein C (SP-C)
dc.subject.ucmBioquímica (Química)
dc.subject.ucmBiología molecular (Biología)
dc.subject.unesco2302 Bioquímica
dc.subject.unesco2415 Biología Molecular
dc.titleExploring protein–protein interactions and oligomerization state of pulmonary surfactant protein C (SP-C) through FRET and fluorescence self-quenching
dc.typejournal article
dc.type.hasVersionVoR
dc.volume.number33
dspace.entity.typePublication
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