Single amino acids in the lumenal loop domain influence the stability of the major light-harvesting chlorophyll a/b complex
Autor: | Sonja Geister, Harald Paulsen, Kristina Eggert, Vera Mick, Bo Heinemann |
---|---|
Rok vydání: | 2004 |
Předmět: |
Photosynthetic reaction centre
Protein Folding Photosystem II Pigment binding DNA Mutational Analysis Light-Harvesting Protein Complexes Peas Photosystem II Protein Complex Biology Biochemistry Transmembrane protein Protein Structure Secondary Protein Structure Tertiary B vitamins Amino Acid Substitution Mutant protein Mutagenesis Site-Directed Point Mutation Amino Acids Integral membrane protein Accessory pigment Gene Library Plant Proteins |
Zdroj: | Biochemistry. 43(18) |
ISSN: | 0006-2960 |
Popis: | The major light-harvesting complex of photosystem II (LHCIIb) is one of the most abundant integral membrane proteins. It greatly enhances the efficiency of photosynthesis in green plants by binding a large number of accessory pigments that absorb light energy and conduct it toward the photosynthetic reaction centers. Most of these pigments are associated with the three transmembrane and one amphiphilic alpha helices of the protein. Less is known about the significance of the loop domains connecting the alpha helices for pigment binding. Therefore, we randomly exchanged single amino acids in the lumenal loop domain of the bacterially expressed apoprotein Lhcb1 and then reconstituted the mutant protein with pigments in vitro. The resulting collection of mutated recombinant LHCIIb versions was screened by using a 96-well-format plate-based procedure described previously [Heinemann, B., and Paulsen, H. (1999) Biochemistry 38, 14088-14093], enabling us to test several thousand mutants for their ability to form stable pigment-protein complexes in vitro. At least one-third of the positions in the loop domain turned out to be sensitive targets; i.e., their exchange abolished formation of LHCIIb in vitro. This confirms our earlier notion that the LHCIIb loop domains contribute more specifically to complex formation and/or stabilization than by merely connecting the alpha helices. Among the target sites, glycines and hydrophilic amino acids are more prominently represented than hydrophobic ones. Specifically, the exchange of any of the three acidic amino acids in the lumenal loop abolishes reconstitution of stable pigment-protein complexes, suggesting that ionic interactions with other protein domains are important for correct protein folding or complex stabilization. One hydrophobic amino acid, tryptophan in position 97, has been hit repeatedly in independent mutation experiments. From the LHCIIb structure and previous mutational analyses, we propose a stabilizing interaction between this amino acid and F195 near the C-proximal end of the third transmembrane helix. |
Databáze: | OpenAIRE |
Externí odkaz: |