Browsing by Subject "Pf3 coat protein"

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    The bacterial membrane insertase YidC : in vivo studies of substrate binding and membrane insertion
    (2015) Klenner, Christian Daniel; Kuhn, Andreas
    YidC of Escherichia coli belongs to the evolutionarily conserved proteins of the Oxa1/YidC/Alb3 insertase family. The transmembrane regions of the core domain, comprising of TM2-6, are the most conserved parts among the homologs and are crucial for the function as a membrane insertase. This is particularly true for the TM2, TM3 and TM5 (KUHN et al., 2003; KIEFER & KUHN, 2007). In bacteria, YidC acts as an independently working membrane insertase and, as well, in cooperation with the Sec translocon for the biogenesis of various membrane proteins. YidC is required for the biogenesis of respiratory complexes, ATP synthase and for example the mechanosensitive channel protein MscL. Also, the coat proteins of filamentous phage Pf3 and M13 require YidC for membrane insertion. The best studied substrate is the Pf3 coat protein of phage Pf3 infecting Pseudomonas aeruginosa – i.e. a small protein of 44 amino acids in length. In the context of this thesis, the YidC-dependent biogenesis of Pf3 coat was analyzed to gain better insight into the entire insertion process. In doing so, a set of more than 100 single cysteine mutants in distinct domains of YidC and Pf3 coat were generated. To study the insertion of Pf3 coat under physiological conditions, an in vivo cross-linking assay was established for capturing YidC-Pf3 interactions within a short period of time after the onset of synthesis (1 minute) using 35S-Met pulse-labelling methods. YidC binds inserting Pf3 coat protein in distinct regions of the highly conserved TM domains involving four of the six TM helices. It was verified that TM3 is indispensable for the function of YidC since four contacting residues were found in this TM helix. A helical wheel projection of substrate binding helices reveals the localization of the contacting residues of each TM segment on one helical face. This implies a helix arrangement of the transmembrane core domain which enables binding of inserting substrate proteins and interactions with transmembrane domains over the entire membrane-spanning part of YidC. The serial mutation of nine from twelve contacting residues, which are strongly hydrophobic in most cases, to serines impaired the function of YidC, whereas the single mutations had no effect. Additionally, the insertion process of translocation deficient Pf3 coat mutants was analyzed for intermediate states of the insertion process. It has been shown that the insertion deficient Pf3 coat mutants are inhibited at a late step of membrane insertion, i.e. forming the YidC contacts in the periplasmic leaflet. Based on this work, further studies confirmed that the identified substrate contacting regions of YidC play a key role in YidC-mediated insertion. The mechanosensitive channel protein MscL, M13 procoat, nascent Foc and the polytopic membrane protein LacY contact YidC at exactly the same positions (NEUGEBAUER et al., 2012; SPANN & KUHN, unpublished results; WICKLES et al., 2014; ZHU et al., 2013b).
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    Untersuchungen zur autonomen und YidC-vermittelten Membraninsertion von Pf3 coat-Protein mit Hilfe Fluoreszenz-spektroskopischer Einzelmolekülmessungen
    (2011) Schönbauer, Anne-Kathrin; Kuhn, Andreas
    Pf3 coat is the capsid protein of the bacteriophage Pf3. The phage leaves the host cell by continuous extrusion without damaging the cell. The protein itself consists of 44 amino acid residues and has a rod-like shape. Because of its simple structure, the protein needs only the help of the insertase YidC to insert into the bacterial inner membrane. 3L-Pf3 coat, a protein mutant with three additional leucine residues in the center of the transmembrane region (TMD), has an increased hydrophobicity. It is independent of YidC and inserts into the membrane autonomously (Serek et al., 2004). In this work, a newly developed physical method was used to find out whether the elongation or the increased hydrophobicity accounts for the autonomous insertion of the protein. For this reason, two new protein mutants were constructed. Each mutant has only one of the changed properties of the 3L-Pf3 coat protein: GAT-Pf3 coat has an elongated TMD with three additional residues (glycine, alanin and threonine). The second mutant, 2M-Pf3 coat, shows an increased hydrophobicity due to the substitution of two alanine residues by two methionine residues at the positions 30 and 31. So it had an increased hydrophobicity like 3L-Pf3 coat. The above mentioned proteins, wt-Pf3 coat and its mutants, were modified with a fluorescent label to follow the proteins with optical methods. The Proteins were first modified with a single cysteine and then labeled by a fluorescent marker, Atto520 maleimid. Proteins with a labeled N-terminal tail were called NC-Pf3 coat, whereas CC-Pf3 coat had a labeled C-terminal tail. In addition, the orientation of the protein in the membrane was identified by quenching the fluorescence of the NC- and CC- labeled proteins. A new method employing single molecules was developed using fluorescence correlation spectroscopy. This method allows real time observations of binding and insertion of the protein into semisynthetical liposomes. By using fluorescent quenching the membrane insertion and binding were distinguished. It became clear that both the elongation of the TMD as well as an increased hydrophobicity play a crucial role in the autonomous insertion of the protein into the membrane. Therefore, the interaction between the hydrophobic region of the protein and the hydrophobic core region of the membrane is important for the binding of the protein and its insertion into the membrane.