Abstract
We have studied Hansenula polymorpha Pex5p and Pex8p using fluorescence correlation spectroscopy (FCS). Pex5p is the Peroxisomal Targeting Signal 1 (PTS1) receptor and Pex8p is an intraperoxisomal protein. Both proteins are essential for PTS1 protein import and have been shown to physically interact. We used FCS to analyze the molecular role of this interaction. FCS is a very sensitive technique that allows analysis of dynamic processes of fluorescently marked molecules at equilibrium in a very tiny volume. We used this technique to determine the oligomeric state of both peroxins and to analyze binding of Pex5p to PTS1 peptides and Pex8p. HpPex5p and HpPex8p were overproduced in Escherichia coli, purified by affinity chromatography, and, when required, labeled with the fluorescent dye Alexa Fluor 488. FCS measurements revealed that the oligomeric state of HpPex5p varied, ranging from monomers at slightly acidic pH to tetramers at neutral pH. HpPex8p formed monomers at all pH values tested. Using fluorescein-labeled PTS1 peptide and unlabeled HpPex5p, we established that PTS1 peptide only bound to tetrameric HpPex5p. Upon addition of HpPex8p, a heterodimeric complex was formed consisting of one HpPex8p and one HpPex5p molecule. This process was paralleled by dissociation of PTS1 peptide from HpPex5p, indicating that Pex8p may play an important role in cargo release from the PTS1 receptor. Our data show that FCS is a powerful technique to explore dynamic physical interactions that occur between peroxins during peroxisomal matrix protein import.
Highlights
Peroxisomes are single membrane-bound organelles that are present in most aerobic eukaryotic cells
To understand the molecular role of the physical interaction between Pex5p and Pex8p in matrix protein import, we studied these peroxins using a novel approach in peroxisome research, namely fluorescence correlation spectroscopy (FCS)
Our studies indicate that FCS is a powerful technique to explore the dynamics of physical interactions that occur during peroxisomal matrix protein import
Summary
Peptides and Proteins—Peptides PTS1 (ASKL-COOH) and Fl-PTS1 (ASSASKL-COOH covalently bound to fluorescein (Fl) at the N terminus) were purchased from Eurosequence (Groningen, the Netherlands). Analysis of the Functionality of HpPex5p-His and HpPex8p-His6— The functionality of carboxyl-terminal His6-tagged HpPex5p was tested by introducing the HpPEX5-HIS6 gene under control of the endogenous promoter (PPEX5) in a H. polymorpha PEX5 deletion strain (⌬pex5) (9) To this purpose the PEX5-HIS6 cassette was isolated as a 1.8-kb NcoI (blunted)-HindIII fragment from the pQE60-PEX5-HIS6 plasmid and ligated into the shuttle vector pHS5 together with a 0.5-kb BamHI (blunted) SacI PEX5 promoter fragment (BamHI site introduced by PCR). The dimensions of the confocal detection volume and the structural parameter are obtained from global analysis of the autocorrelation curves of the standard Rhodamine 110 in water having a diffusion constant of 280 m2sϪ1 (13). Assuming a more or less globular shape of the molecules, Equation 4 allows us to derive the molecular mass of a protein by comparing it with the known molecular mass of a reference compound
Sign-in/Register to view highlights & summary Sign-in/Register to access full text options 
Free) 
Talk to us
Join us for a 30 min session where you can share your feedback and ask us any queries you have
Schedule a call
