Aggregation-related quenching of LHCII fluorescence in liposomes revealed by single-molecule spectroscopy

Marijonas Tutkus; Jevgenij Chmeliov; Gediminas Trinkunas; Parveen Akhtar; Petar H Lambrev; Leonas Valkunas

doi:10.1016/j.jphotobiol.2021.112174

Aggregation-related quenching of LHCII fluorescence in liposomes revealed by single-molecule spectroscopy

J Photochem Photobiol B. 2021 May:218:112174. doi: 10.1016/j.jphotobiol.2021.112174. Epub 2021 Mar 25.

Authors

Marijonas Tutkus¹, Jevgenij Chmeliov², Gediminas Trinkunas³, Parveen Akhtar⁴, Petar H Lambrev⁴, Leonas Valkunas⁵

Affiliations

¹ Department of Molecular Compound Physics, Center for Physical Sciences and Technology, Saulėtekio Av. 3, LT-10257 Vilnius, Lithuania; Institute of Biotechnology, Life Sciences Center, Vilnius University, Saulėtekio av. 7, LT-10257 Vilnius, Lithuania.
² Department of Molecular Compound Physics, Center for Physical Sciences and Technology, Saulėtekio Av. 3, LT-10257 Vilnius, Lithuania; Institute of Chemical Physics, Faculty of Physics, Vilnius University, Saulėtekio Av. 9-III, LT-10222 Vilnius, Lithuania.
³ Department of Molecular Compound Physics, Center for Physical Sciences and Technology, Saulėtekio Av. 3, LT-10257 Vilnius, Lithuania.
⁴ Biological Research Centre, Szeged, Temesvári körút 62, Szeged 6726, Hungary.
⁵ Department of Molecular Compound Physics, Center for Physical Sciences and Technology, Saulėtekio Av. 3, LT-10257 Vilnius, Lithuania; Institute of Chemical Physics, Faculty of Physics, Vilnius University, Saulėtekio Av. 9-III, LT-10222 Vilnius, Lithuania. Electronic address: leonas.valkunas@ff.vu.lt.

PMID: 33799009
DOI: 10.1016/j.jphotobiol.2021.112174

Abstract

Incorporation of membrane proteins into reconstituted lipid membranes is a common approach for studying their structure and function relationship in a native-like environment. In this work, we investigated fluorescence properties of liposome-reconstituted major light-harvesting complexes of plants (LHCII). By utilizing liposome labelling with the fluorescent dye molecules and single-molecule microscopy techniques, we were able to study truly liposome-reconstituted LHCII and compare them with bulk measurements and liposome-free LHCII aggregates bound to the surface. Our results showed that fluorescence lifetime obtained in bulk and in single liposome measurements were correlated. The fluorescence lifetimes of LHCII were shorter for liposome-free LHCII than for reconstituted LHCII. In the case of liposome-reconstituted LHCII, fluorescence lifetime showed dependence on the protein density reminiscent to concentration quenching. The dependence of fluorescence lifetime of LHCII on the liposome size was not significant. Our results demonstrated that fluorescence quenching can be induced by LHCII - LHCII interactions in reconstituted membranes, most likely occurring via the same mechanism as photoprotective non-photochemical quenching in vivo.

Keywords: Aggregation; Confocal microscopy; Fluorescence; Fluorescence lifetime imaging; Light-harvesting complex II; Liposome-reconstitution; Liposomes; Non-photochemical quenching; Protein density; Single-molecule; Surface immobilization.

MeSH terms

Fluorescent Dyes / chemistry*
Kinetics
Light-Harvesting Protein Complexes / chemistry*
Liposomes / chemistry*
Plant Extracts / chemistry*
Protein Aggregates
Protein Kinases / chemistry*
Single Molecule Imaging
Spectrometry, Fluorescence
Structure-Activity Relationship
Surface Properties

Substances

Fluorescent Dyes
Light-Harvesting Protein Complexes
Liposomes
Plant Extracts
Protein Aggregates
Protein Kinases
light-harvesting complex II kinase