1jrq

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(Difference between revisions)

Revision as of 11:26, 21 February 2008

X-ray Structure Analysis of the Role of the Conserved Tyrosine-369 in Active Site of E. coli Amine Oxidase

Overview

Copper amine oxidases are homodimeric enzymes that catalyze two reactions: first, a self-processing reaction to generate the 2,4,5-trihydroxyphenylalanine (TPQ) cofactor from an active site tyrosine by a single turnover mechanism; second, the oxidative deamination of primary amine substrates with the production of aldehyde, hydrogen peroxide, and ammonia catalyzed by the mature enzyme. The importance of active site residues in both of these processes has been investigated by structural studies and site-directed mutagenesis in enzymes from various organisms. One conserved residue is a tyrosine, Tyr369 in the Escherichia coli enzyme, whose hydroxyl is hydrogen bonded to the O4 of TPQ. To explore the importance of this site, we have studied a mutant enzyme in which Tyr369 has been mutated to a phenylalanine. We have determined the X-ray crystal structure of this variant enzyme to 2.1 A resolution, which reveals that TPQ adopts a predominant nonproductive conformation in the resting enzyme. Reaction of the enzyme with the irreversible inhibitor 2-hydrazinopyridine (2-HP) reveals differences in the reactivity of Y369F compared with wild type with more efficient formation of an adduct (lambda(max) = 525 nm) perhaps reflecting increased mobility of the TPQ adduct within the active site of Y369F. Titration with 2-HP also reveals that both wild type and Y369F contain one TPQ per monomer, indicating that Tyr369 is not essential for TPQ formation, although we have not measured the rate of TPQ biogenesis. The UV-vis spectrum of the Y369F protein shows a broader peak and red-shifted lambda(max) at 496 nm compared with wild type (480 nm), consistent with an altered electronic structure of TPQ. Steady-state kinetic measurements reveal that Y369F has decreased catalytic activity particularly below pH 6.5 while the K(M) for substrate beta-phenethylamine increases significantly, apparently due to an elevated pK(a) (5.75-6.5) for the catalytic base, Asp383, that should be deprotonated for efficient binding of protonated substrate. At pH 7.0, the K(M) for wild type and Y369F are similar at 1.2 and 1.5 microM, respectively, while k(cat) is decreased from 15 s(-1) in wild type to 0.38 s(-1), resulting in a 50-fold decrease in k(cat)/K(M) for Y369F. Transient kinetics experiments indicate that while the initial stages of enzyme reduction are slower in the variant, these do not represent the rate-limiting step. Previous structural and solution studies have implicated Tyr369 as a component of a proton shuttle from TPQ to dioxygen. The moderate changes in kinetic parameters observed for the Y369F variant indicate that if this is the case, then the absence of the Tyr369 hydroxyl can be compensated for efficiently within the active site.

About this Structure

1JRQ is a Single protein structure of sequence from Escherichia coli with and as ligands. Active as Amine oxidase (flavin-containing), with EC number 1.4.3.4 Full crystallographic information is available from OCA.

Reference

Conserved tyrosine-369 in the active site of Escherichia coli copper amine oxidase is not essential., Murray JM, Kurtis CR, Tambyrajah W, Saysell CG, Wilmot CM, Parsons MR, Phillips SE, Knowles PF, McPherson MJ, Biochemistry. 2001 Oct 30;40(43):12808-18. PMID:11669617

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Retrieved from "http://52.214.119.220/wiki/index.php/1jrq"

@@ Line 1: / Line 1: @@
-[[Image:1jrq.jpg|left|200px]]<br /><applet load="1jrq" size="450" color="white" frame="true" align="right" spinBox="true"
+[[Image:1jrq.jpg|left|200px]]<br /><applet load="1jrq" size="350" color="white" frame="true" align="right" spinBox="true"
 caption="1jrq, resolution 2.15&Aring;" />
 '''X-ray Structure Analysis of the Role of the Conserved Tyrosine-369 in Active Site of E. coli Amine Oxidase'''<br />
 ==Overview==
-Copper amine oxidases are homodimeric enzymes that catalyze two reactions:, first, a self-processing reaction to generate the, 2,4,5-trihydroxyphenylalanine (TPQ) cofactor from an active site tyrosine, by a single turnover mechanism; second, the oxidative deamination of, primary amine substrates with the production of aldehyde, hydrogen, peroxide, and ammonia catalyzed by the mature enzyme. The importance of, active site residues in both of these processes has been investigated by, structural studies and site-directed mutagenesis in enzymes from various, organisms. One conserved residue is a tyrosine, Tyr369 in the Escherichia, coli enzyme, whose hydroxyl is hydrogen bonded to the O4 of TPQ. To, explore the importance of this site, we have studied a mutant enzyme in, which Tyr369 has been mutated to a phenylalanine. We have determined the, X-ray crystal structure of this variant enzyme to 2.1 A resolution, which, reveals that TPQ adopts a predominant nonproductive conformation in the, resting enzyme. Reaction of the enzyme with the irreversible inhibitor, 2-hydrazinopyridine (2-HP) reveals differences in the reactivity of Y369F, compared with wild type with more efficient formation of an adduct, (lambda(max) = 525 nm) perhaps reflecting increased mobility of the TPQ, adduct within the active site of Y369F. Titration with 2-HP also reveals, that both wild type and Y369F contain one TPQ per monomer, indicating that, Tyr369 is not essential for TPQ formation, although we have not measured, the rate of TPQ biogenesis. The UV-vis spectrum of the Y369F protein shows, a broader peak and red-shifted lambda(max) at 496 nm compared with wild, type (480 nm), consistent with an altered electronic structure of TPQ., Steady-state kinetic measurements reveal that Y369F has decreased, catalytic activity particularly below pH 6.5 while the K(M) for substrate, beta-phenethylamine increases significantly, apparently due to an elevated, pK(a) (5.75-6.5) for the catalytic base, Asp383, that should be, deprotonated for efficient binding of protonated substrate. At pH 7.0, the, K(M) for wild type and Y369F are similar at 1.2 and 1.5 microM, respectively, while k(cat) is decreased from 15 s(-1) in wild type to 0.38, s(-1), resulting in a 50-fold decrease in k(cat)/K(M) for Y369F. Transient, kinetics experiments indicate that while the initial stages of enzyme, reduction are slower in the variant, these do not represent the, rate-limiting step. Previous structural and solution studies have, implicated Tyr369 as a component of a proton shuttle from TPQ to dioxygen., The moderate changes in kinetic parameters observed for the Y369F variant, indicate that if this is the case, then the absence of the Tyr369 hydroxyl, can be compensated for efficiently within the active site.
+Copper amine oxidases are homodimeric enzymes that catalyze two reactions: first, a self-processing reaction to generate the 2,4,5-trihydroxyphenylalanine (TPQ) cofactor from an active site tyrosine by a single turnover mechanism; second, the oxidative deamination of primary amine substrates with the production of aldehyde, hydrogen peroxide, and ammonia catalyzed by the mature enzyme. The importance of active site residues in both of these processes has been investigated by structural studies and site-directed mutagenesis in enzymes from various organisms. One conserved residue is a tyrosine, Tyr369 in the Escherichia coli enzyme, whose hydroxyl is hydrogen bonded to the O4 of TPQ. To explore the importance of this site, we have studied a mutant enzyme in which Tyr369 has been mutated to a phenylalanine. We have determined the X-ray crystal structure of this variant enzyme to 2.1 A resolution, which reveals that TPQ adopts a predominant nonproductive conformation in the resting enzyme. Reaction of the enzyme with the irreversible inhibitor 2-hydrazinopyridine (2-HP) reveals differences in the reactivity of Y369F compared with wild type with more efficient formation of an adduct (lambda(max) = 525 nm) perhaps reflecting increased mobility of the TPQ adduct within the active site of Y369F. Titration with 2-HP also reveals that both wild type and Y369F contain one TPQ per monomer, indicating that Tyr369 is not essential for TPQ formation, although we have not measured the rate of TPQ biogenesis. The UV-vis spectrum of the Y369F protein shows a broader peak and red-shifted lambda(max) at 496 nm compared with wild type (480 nm), consistent with an altered electronic structure of TPQ. Steady-state kinetic measurements reveal that Y369F has decreased catalytic activity particularly below pH 6.5 while the K(M) for substrate beta-phenethylamine increases significantly, apparently due to an elevated pK(a) (5.75-6.5) for the catalytic base, Asp383, that should be deprotonated for efficient binding of protonated substrate. At pH 7.0, the K(M) for wild type and Y369F are similar at 1.2 and 1.5 microM, respectively, while k(cat) is decreased from 15 s(-1) in wild type to 0.38 s(-1), resulting in a 50-fold decrease in k(cat)/K(M) for Y369F. Transient kinetics experiments indicate that while the initial stages of enzyme reduction are slower in the variant, these do not represent the rate-limiting step. Previous structural and solution studies have implicated Tyr369 as a component of a proton shuttle from TPQ to dioxygen. The moderate changes in kinetic parameters observed for the Y369F variant indicate that if this is the case, then the absence of the Tyr369 hydroxyl can be compensated for efficiently within the active site.
 ==About this Structure==
-JRQ is a [http://en.wikipedia.org/wiki/Single_protein Single protein] structure of sequence from [http://en.wikipedia.org/wiki/Escherichia_coli Escherichia coli] with CU and CA as [http://en.wikipedia.org/wiki/ligands ligands]. Active as [http://en.wikipedia.org/wiki/Amine_oxidase_(flavin-containing) Amine oxidase (flavin-containing)], with EC number [http://www.brenda-enzymes.info/php/result_flat.php4?ecno=1.4.3.4 1.4.3.4] Full crystallographic information is available from [http://ispc.weizmann.ac.il/oca-bin/ocashort?id=1JRQ OCA].
+JRQ is a [http://en.wikipedia.org/wiki/Single_protein Single protein] structure of sequence from [http://en.wikipedia.org/wiki/Escherichia_coli Escherichia coli] with <scene name='pdbligand=CU:'>CU</scene> and <scene name='pdbligand=CA:'>CA</scene> as [http://en.wikipedia.org/wiki/ligands ligands]. Active as [http://en.wikipedia.org/wiki/Amine_oxidase_(flavin-containing) Amine oxidase (flavin-containing)], with EC number [http://www.brenda-enzymes.info/php/result_flat.php4?ecno=1.4.3.4 1.4.3.4] Full crystallographic information is available from [http://oca.weizmann.ac.il/oca-bin/ocashort?id=1JRQ OCA].
 ==Reference==
@@ Line 14: / Line 14: @@
 [[Category: Escherichia coli]]
 [[Category: Single protein]]
-[[Category: Knowles, P.F.]]
+[[Category: Knowles, P F.]]
-[[Category: Kurtis, C.R.]]
+[[Category: Kurtis, C R.]]
-[[Category: McPherson, M.J.]]
+[[Category: McPherson, M J.]]
-[[Category: Murray, J.M.]]
+[[Category: Murray, J M.]]
-[[Category: Parsons, M.R.]]
+[[Category: Parsons, M R.]]
-[[Category: Phillips, S.E.V.]]
+[[Category: Phillips, S E.V.]]
-[[Category: Saysell, C.G.]]
+[[Category: Saysell, C G.]]
 [[Category: Tambarajah, W.]]
-[[Category: Wilmot, C.M.]]
+[[Category: Wilmot, C M.]]
 [[Category: CA]]
 [[Category: CU]]
@@ Line 29: / Line 29: @@
 [[Category: tpq]]
-''Page seeded by [http://ispc.weizmann.ac.il/oca OCA ] on Tue Nov 20 18:31:33 2007''
+''Page seeded by [http://oca.weizmann.ac.il/oca OCA ] on Thu Feb 21 13:26:00 2008''

1jrq

From Proteopedia

Revision as of 11:26, 21 February 2008

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