Author: Kneller, Daniel W.; Phillips, Gwyndalyn; Kovalevsky, Andrey; Coates, Leighton
                    Title: Roomâ€temperature neutron and Xâ€ray data collection of 3CL M(pro) from SARSâ€CoVâ€2  Cord-id: zp3zj82f  Document date: 2020_10_2
                    ID: zp3zj82f
                    
                    Snippet: The replication of SARSâ€CoVâ€2 produces two large polyproteins, pp1a and pp1ab, that are inactive until cleavage by the viral chymotrypsinâ€like cysteine protease enzyme (3CL M(pro)) into a series of smaller functional proteins. At the heart of 3CL M(pro) is an unusual catalytic dyad formed by the side chains of His41 and Cys145 and a coordinated water molecule. The catalytic mechanism by which the enzyme operates is still unknown, as crucial information on the protonation states within the 
                    
                    
                    
                     
                    
                    
                    
                    
                        
                            
                                Document: The replication of SARSâ€CoVâ€2 produces two large polyproteins, pp1a and pp1ab, that are inactive until cleavage by the viral chymotrypsinâ€like cysteine protease enzyme (3CL M(pro)) into a series of smaller functional proteins. At the heart of 3CL M(pro) is an unusual catalytic dyad formed by the side chains of His41 and Cys145 and a coordinated water molecule. The catalytic mechanism by which the enzyme operates is still unknown, as crucial information on the protonation states within the active site is unclear. To experimentally determine the protonation states of the catalytic site and of the other residues in the substrateâ€binding cavity, and to visualize the hydrogenâ€bonding networks throughout the enzyme, roomâ€temperature neutron and Xâ€ray data were collected from a large H/Dâ€exchanged crystal of ligandâ€free (apo) 3CL M(pro).
 
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