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12 research outputs found

Helicase Motif III in SecA is essential for coupling preprotein binding to translocation ATPase

Author: Baud Catherine
Economou Anastassios
Frank Miriam
Karamanou Spyridoula
Papanikou Efrosyni
Sianidis Giorgos
Publication venue
Publication date: 23/07/2004
Field of study

The SecA ATPase is a protein translocase motor and a superfamily 2 (SF2) RNA helicase. The ATPase catalytic core (‘DEAD motor') contains the seven conserved SF2 motifs. Here, we demonstrate that Motif III is essential for SecA-mediated protein translocation and viability. SecA Motif III mutants can bind ligands (nucleotide, the SecYEG translocase ‘channel', signal and mature preprotein domains), can catalyse basal and SecYEG-stimulated ATP hydrolysis and can be activated for catalysis. However, Motif III mutation specifically blocks the preprotein-stimulated ‘translocation ATPase' at a step of the reaction pathway that lies downstream of ligand binding. A functional Motif III is required for optimal ligand-driven conformational changes and kinetic parameters that underlie optimal preprotein-modulated nucleotide cycling at the SecA DEAD motor. We propose that helicase Motif III couples preprotein binding to the SecA translocation ATPase and that catalytic activation of SF2 enzymes through Motif-III-mediated action is essential for both polypeptide and nucleic-acid substrates

Crossref

PubMed Central

Global Co-ordination of Protein Translocation by the SecA IRA1 Switch

Author: Anastassios Economou
Baud
Breukink
Breyton
Brundage
Caruthers
Catherine Baud
Dapic
Delagoutte
den Blaauwen
den Blaauwen
Ding
Douville
Driessen
Duong
Duong
Economou
Economou
Economou
Economou
Eleftheria Vrontou
Fekkes
Giorgos Sianidis
Hartl
Hirano
Hunt
Jarosik
Karamanou
Kimura
Koonin
Kourtz
Lill
Manting
Miller
Mitchell
Schiebel
Sharma
Sianidis
Singleton
Song
Spyridoula Karamanou
Triplett
Yap
Yoshida
Publication venue: 'American Society for Biochemistry & Molecular Biology (ASBMB)'
Publication date
Field of study

Crossref

Type III protein translocase : HrcN is a peripheral ATPase that is activated by oligomerization

Author: Brown Ian
Chalkiadaki Aggeliki
Economou Anastassios
Engel Andreas
Gomez-Serrano Amalia
Karamanou Spyridoula
Lustig Ariel
Mansfield John
Panopoulos Nickolas J.
Politou Anastasia S.
Pozidis Charalambos
Pugsley Anthony P.
Sianidis Giorgos
Stahlberg Henning
Tampakaki Anastasia P.
Publication venue: American Society of Biological Chemists
Publication date: 01/01/2003
Field of study

Type III protein secretion (TTS) is catalyzed by translocases that span both membranes of Gram-negative bacteria. A hydrophilic TTS component homologous to F1/V1-ATPases is ubiquitous and essential for secretion. We show that hrcN encodes the putative TTS ATPase of Pseudomonas syringae pathovar phaseolicola and that HrcN is a peripheral protein that assembles in clusters at the membrane. A decahistidinyl HrcN derivative was overexpressed in Escherichia coli and purified to homogeneity in a folded state. Hydrodynamic analysis, cross-linking, and electron microscopy revealed four distinct HrcN forms: I, 48 kDa (monomer); II, approximately 300 kDa (putative hexamer); III, 575 kDa (dodecamer); and IV, approximately 3.5 MDa. Form III is the predominant form of HrcN at the membrane, and its ATPase activity is dramatically stimulated (<700-fold) over the basal activity of Form I. We propose that TTS ATPases catalyze protein translocation as activated homo-oligomers at the plasma membrane

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