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(Nanowerk NewsCells rely on protein complexes known as ATP synthases or ATPases for their energy needs – adenosine triphosphate (ATP) Structural biologist Professor Leonid Sazanov and his research group from the Institute of Science and Technology Austria (IST Austria) in Klosterneuburg, Austria evolutionary tree of these essential molecular machines.
These results are obtained using the latest cryo-electron microscopy methods revealed in the newspaper Science ("Structure and Conformational Plasticity of the Intact Thermus thermophilus V / A-type ATPase ").
Rotary power
ATP synthases / ATPases are broad membrane-protein complexes which share overall gross building plans and rotary catalysis mechanisms. This protein family includes F-type enzyme found in mitochondria (power factories of the cell), chloroplasts (organelles that conduct photosynthesis in plants) and bacteria; V (vacuolar) -type found in intracellular compartments in eukaryotes (higher organisms with nucleus) and A (archaeal) -type found in prokaryotes – archaea (ancient microorganisms) and some bacteria.
The proteins consist of a globular F1 / V1 / A1 domain synthesizing / hydrolyzing ATP and a membrane-embedded Fo / Vo / Ao domain translocating protons. F-type enzymes are well studied and their atomic structures are known. F1 and F domains are connected by the central stalk or shaft / rotor, which rotates inside F1 driving ATP synthesis. The rotor is attached to the so-called c-ring which is driven by the proton flow between the ring and the membrane-embedded stator.
The rotation of F1 is prevented by the single peripheral stalk, which keeps F1 anchored to the stator. The overall architecture of this unique molecular machine thus resembles that of a turbine or a water mill, driven by the flow of protons rather than water.
Different flavors of ATPases
F-and-type enzymes usually function to produce ATP, driven by proton flow across the membrane. V-type enzymes usually work in reverse, using ATP to pump protons. V- and A-ATPases are structurally similar but they differ from each other in the presence of V1 and Vo. V-type enzymes probably evolved from the A-type and because of these similarities A-type is also termed V / A-ATPase.
Some bacteria, including Thermus thermophilus, acquired an A-type enzyme. Long Zhou, postdoc in the Sazanov research group of IST Austria, has purified and studied this enzyme (ThV1Vo) by cryo-EM. In contrast to F-type, for V-type ATPases only the structures of the isolated V1 and V domains were determined previously. How V1 is Coupled to the Knowledge of the Full Catalytic Cycle Was Lacking.
Plasticity and competition
The scientists determined not only that, but in all five structures of the entire ThV1Vo enzyme, using cryo-electron microscopy methods developed recently in the so-called "resolution revolution" of this technique. The structures represent several conformational states of the enzyme differing by the position of the rotor inside the stator.
Global conformational plasticity of ThV1Vo is revealed as substantial V1 wobbling in space in transition from one state to another. It is a result of mechanical competition between rotation of the central bent rotor and stiffness of the stator. V1-Vo coupling is achieved via close structural and electrostatic match between the shaft and V-type specific subunit linking it to the c-ring.
The visualization of the proton path revealed significant differences in the distribution of proteins in F-ATPases, with a strict "check-point" preventing "slipping" of the enzyme.
Why additional complexity?
Instead of a single peripheral stalk of F-type enzymes, A-types such as ThV1Vo have two peripheral stalks, while eukaryotic V-types have three. But what is the advantage of V1 and Vo? The F1 / V1 domain has a three-fold symmetry and so one ATP molecule is produced (or consumed) for each 120 ° rotation of the stator inside F1 / V1.
Professor Leonid Sazanov says: "In V / A-ATPases this step is a one-off 120 ° rotation, in contrast to F-ATP synthase where it is divided into several sub-steps. Thus, greater plasticity may be required in these steps in order to link these steps in the V1 to smaller sub-steps in the field. This additional flexibility can be provided by additional peripheral stalks and connecting subunits. Our new structures show how this is achieved, providing a framework for the whole V-ATPase family ".
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