Research
interests
Intracellular Ca2+
signalling is one of the most ancient second messenger pathways in cell which is of vital importance in such
diverse physiological functions as muscle contraction, neurotrasmitter release, fertilization, hormone secretion,
gene transcription, metabolic regulation and apoptosis. It is based on ability of cells to maintain low levels of
Ca2+ under resting conditions and to create a rapid and transient
increase of Ca2+ upon the stimulated entry of Ca2+ ions
through the plasma membrane. Key elements for this pathway are Ca2+ pumps and C2+ channels on plasma membrane and
on internal organelles. The goal of our research is to understand molecular mechanisms underlying ion transport into and out
of the cell across the surface membrane, or between different intracellular compartments through structure-function studies of
membrane proteins and the macromolecular assemblies they form.
In our studies we use electron cryomicroscopy and computer reconstruction techniques in conjunction with biochemical, electro physiological and molecular biological techniques. To date, electron cryomicroscopy is proving to be one of the most important structural approaches in cell biological studies. We use "single particle" approach which relies on analysis of large number of electron images of isolated unordered macromolecules preserved in a layer of vitreous ice.
Recent focus has been on structural analysis of integral membrane Ca
2+ release channels that mediate ligand-gated release of Ca2+ from intracelluar stores: the inositol 1,4,5-trisphosphate-sensitive Ca2+ release channel (InsP3R), localized in the endoplasmic reticulum, and the ryanodine-sensitive Ca2+ release channel (ryanodine receptor, RyR), the primary Ca2+ channel in muscle cells. Both channels are large homotetrameric protein complexes with a molecular mass of ~2.3 MDa for RyRs and 1.2 MDa for InsP3Rs. Large size and dynamic properties of these ion channels render their structural determination by standard structural techniques like X-ray crystallography or NMR spectroscopy, while electron cryomicroscopy is able to tackle both, large macromolecular assemblies as well as molecules in different functional states.Another avenue of our research if the L-type voltage-gated Ca
2+ channel (~430 kDa) is a hetero-oligomeric protein complex composed of five subunits. Even though the resolution of our current structures is limited to 20-30 Å, the low-resolution information is often useful for advancing the understanding of the system particularly when the structural studies are carried out along with biochemical labeling or modification. Our ultimate goal is extending these studies to higher resolution (8-10 Å) in order to build an anatomic model of these molecular complexes at well-defined functional states.
Selected
Publications:
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Irina for all your comments/suggestions
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Last update: October 3, 2003
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