1yfm

From Proteopedia

(Difference between revisions)

Revision as of 14:04, 21 February 2008

RECOMBINANT YEAST FUMARASE

Overview

Crystal structures for both native and recombinant forms of yeast fumarase from Saccharomyces cerevisiae have been completed to moderate resolution by two separate laboratories. The recombinant form was obtained by the construction of an expression plasmid for Escherichia coli. Despite a high level of amino acid sequence similarity, purification of the eukaryotic enzyme from the wild-type prokaryotic enzyme was feasible. The crystal structure of the native form, NY-fumarase, encompasses residues R22 through M484, while the recombinant form, RY-fumarase, consists of residues S27 through L485. Both crystal structures lack the N-terminal translocation segment. Each subunit of the homo-tetrameric protein has three domains. The active site is formed by segments from each of three polypeptide chains. The results of these studies on the eukaryotic proteins are unique, since the recombinant form was done in the absence of dicarboxylic acid and has an unoccupied active site. As a comparison, native fumarase was crystallized in the presence of the competitive inhibitor, meso-tartrate. Meso-tartrate occupies a position close to that of the bound citrate molecule found in the active site of the E. coli enzyme. This inhibitor participates in hydrogen bonding to an active-site water molecule. The independent determination of the two structures provides further evidence that an active-site water molecule may play an active role in the fumarase-catalyzed reaction.

About this Structure

1YFM is a Single protein structure of sequence from Saccharomyces cerevisiae. Active as Fumarate hydratase, with EC number 4.2.1.2 Known structural/functional Site: . Full crystallographic information is available from OCA.

Reference

Crystal structures of native and recombinant yeast fumarase., Weaver T, Lees M, Zaitsev V, Zaitseva I, Duke E, Lindley P, McSweeny S, Svensson A, Keruchenko J, Keruchenko I, Gladilin K, Banaszak L, J Mol Biol. 1998 Jul 17;280(3):431-42. PMID:9665847

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 ==Overview==
-Crystal structures for both native and recombinant forms of yeast fumarase, from Saccharomyces cerevisiae have been completed to moderate resolution, by two separate laboratories. The recombinant form was obtained by the, construction of an expression plasmid for Escherichia coli. Despite a high, level of amino acid sequence similarity, purification of the eukaryotic, enzyme from the wild-type prokaryotic enzyme was feasible. The crystal, structure of the native form, NY-fumarase, encompasses residues R22, through M484, while the recombinant form, RY-fumarase, consists of, residues S27 through L485. Both crystal structures lack the N-terminal, translocation segment. Each subunit of the homo-tetrameric protein has, three domains. The active site is formed by segments from each of three, polypeptide chains. The results of these studies on the eukaryotic, proteins are unique, since the recombinant form was done in the absence of, dicarboxylic acid and has an unoccupied active site. As a comparison, native fumarase was crystallized in the presence of the competitive, inhibitor, meso-tartrate. Meso-tartrate occupies a position close to that, of the bound citrate molecule found in the active site of the E. coli, enzyme. This inhibitor participates in hydrogen bonding to an active-site, water molecule. The independent determination of the two structures, provides further evidence that an active-site water molecule may play an, active role in the fumarase-catalyzed reaction.
+Crystal structures for both native and recombinant forms of yeast fumarase from Saccharomyces cerevisiae have been completed to moderate resolution by two separate laboratories. The recombinant form was obtained by the construction of an expression plasmid for Escherichia coli. Despite a high level of amino acid sequence similarity, purification of the eukaryotic enzyme from the wild-type prokaryotic enzyme was feasible. The crystal structure of the native form, NY-fumarase, encompasses residues R22 through M484, while the recombinant form, RY-fumarase, consists of residues S27 through L485. Both crystal structures lack the N-terminal translocation segment. Each subunit of the homo-tetrameric protein has three domains. The active site is formed by segments from each of three polypeptide chains. The results of these studies on the eukaryotic proteins are unique, since the recombinant form was done in the absence of dicarboxylic acid and has an unoccupied active site. As a comparison, native fumarase was crystallized in the presence of the competitive inhibitor, meso-tartrate. Meso-tartrate occupies a position close to that of the bound citrate molecule found in the active site of the E. coli enzyme. This inhibitor participates in hydrogen bonding to an active-site water molecule. The independent determination of the two structures provides further evidence that an active-site water molecule may play an active role in the fumarase-catalyzed reaction.
 ==About this Structure==
@@ Line 14: / Line 14: @@
 [[Category: Saccharomyces cerevisiae]]
 [[Category: Single protein]]
-[[Category: Banaszak, L.J.]]
+[[Category: Banaszak, L J.]]
-[[Category: Lees, M.R.]]
+[[Category: Lees, M R.]]
-[[Category: Weaver, T.M.]]
+[[Category: Weaver, T M.]]
 [[Category: active site water]]
 [[Category: fumarase]]
@@ Line 24: / Line 24: @@
 [[Category: multi-subunit active site]]
-''Page seeded by [http://oca.weizmann.ac.il/oca OCA ] on Sun Feb  3 10:22:27 2008''
+''Page seeded by [http://oca.weizmann.ac.il/oca OCA ] on Thu Feb 21 16:04:50 2008''

1yfm

From Proteopedia

Revision as of 14:04, 21 February 2008

Overview

About this Structure

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