Awardee OrganizationUNIVERSITY OF CALIFORNIA, SAN DIEGO
Description
Abstract Text
DESCRIPTION: Thrombomodulin (TM) is an essential anticoagulant protein that
binds to thrombin and the resulting complex shuts down further production of
thrombin. In the complex, the thrombin active site has new substrate
specificity toward protein C, which when activated by the thrombin- TM
complex shuts down the coagulation cascade. The proposed experiments will
analyze both the structure and function of TM in order to obtain an
atomic-level understanding of how TM alters the activity of thrombin.
Structural information gained from multi-dimensional NMR methods as well as
X-ray crystallography will be integrated with functional information gained
from site-directed mutagenesis of residues in both TM and thrombin.
Particular emphasis will be placed on the nature of the protein-protein
interaction and on the conformational changes that occur during the
interaction. The experimental plan is as follows: 1) Determine the
structure of the smallest active fragment of TM , TMEGF(4-5) using
multi-dimensional NMR methods. 2) Determine the function of essential
residues within the fourth EGF-like domain of TM. Essential residues that
have been shown to coalesce in a clefT on the fourth domain will be
conservatively mutated and analyzed for functional changes using clotting,
protein C activation, and direct binding assays. 3) Determine the function
of essential residues within the fifth EGF-like domain of TM. Essential
residues within the C-terminal loop and tail will be conservatively mutated
and each mutant will be analyzed for functional changes as in Aim 2. 4)
Determine the structural consequences of interesting functionally altered
mutants using methods developed in Aim 1. 5) Express the S195A mutant of
human prothrombin-2 in large quantities in Pichia pastoris. This mutant
thrombin is required for both NMR and X-ray crystallographic studies. 6)
Determine the surface of TMEGF(4-5) that interacts with thrombin using a
combination of X-ray crystallography and isotope-edited NMR as well as
complementary mutagenesis of residues on both TM and thrombin.
Public Health Relevance Statement
Data not available.
NIH Spending Category
No NIH Spending Category available.
Project Terms
X ray crystallographyactive sitesbiophysicsconformationcrystallizationenzyme activityepidermal growth factormutantnuclear magnetic resonance spectroscopyprotein Cprotein purificationprotein sequenceprotein structure functionprothrombinsite directed mutagenesisthrombinthrombomodulinyeasts
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