Sandbox Wabash 28 Fumarase

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<scene name='72/726358/H188n_site_a/1'>Modifying site A</scene> (H188N) produced an enzyme with approximately 200-fold less specific activity than the wild type. Crystalographic data showed little to no changes in site B whereas the presence of N188 encouraged increased H-bonding with a water molecule instead of the ligand (represented by the inhibitor citrate in the crystal).
<scene name='72/726358/H188n_site_a/1'>Modifying site A</scene> (H188N) produced an enzyme with approximately 200-fold less specific activity than the wild type. Crystalographic data showed little to no changes in site B whereas the presence of N188 encouraged increased H-bonding with a water molecule instead of the ligand (represented by the inhibitor citrate in the crystal).
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Although modifications at <scene name='72/726358/H129n_site_b/1'>site B</scene> (H129N) also changed H-bonding patterns in the site. The net result was little to no conformation change at either site A or B. The catalytic studies demonstrated a small, but significantly larger specific activity in the mutant. Citrate (the inhibitor representative of the substrate) remained bound to site A.
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Although modifications at <scene name='72/726358/H129n_site_b/1'>site B</scene> (H129N) also changed H-bonding patterns in the site. The net result was little to no conformation change at either site A or B. The catalytic studies demonstrated a small, but significantly larger specific activity in the mutant. Citrate (the inhibitor representative of the substrate) remained bound to <scene name='72/726358/H129n_site_b/3'>site A</scene> as with the wild type.
Cohesively, these results are indicative that site A (especially H188) is the catalytic active site.
Cohesively, these results are indicative that site A (especially H188) is the catalytic active site.

Revision as of 01:56, 28 February 2016

Fumarase

PDB ID 1yfe

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