2pui

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==Overview==
==Overview==
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The methionine salvage pathway is ubiquitous in all organisms, but, metabolic variations exist between bacteria and mammals., 5-Methylthioribose (MTR) kinase is a key enzyme in methionine salvage in, bacteria and the absence of a mammalian homolog suggests that it is a good, target for the design of novel antibiotics. The structures of the apo-form, of Bacillus subtilis MTR kinase, as well as its ADP, ADP-PO(4), AMPPCP, and AMPPCP-MTR complexes have been determined. MTR kinase has a bilobal, eukaryotic protein kinase fold but exhibits a number of unique features., The protein lacks the DFG motif typically found at the beginning of the, activation loop and instead coordinates magnesium via a DXE motif, (Asp(250)-Glu(252)). In addition, the glycine-rich loop of the protein, analogous to the "Gly triad" in protein kinases, does not interact, extensively with the nucleotide. The MTR substrate-binding site consists, of Asp(233) of the catalytic HGD motif, a novel twin arginine motif, (Arg(340)/Arg(341)), and a semi-conserved W-loop, which appears to, regulate MTR binding specificity. No lobe closure is observed for MTR, kinase upon substrate binding. This is probably because the enzyme lacks, the lobe closure/inducing interactions between the C-lobe of the protein, and the ribosyl moiety of the nucleotide that are typically responsible, for lobe closure in protein kinases. The current structures suggest that, MTR kinase has a dissociative mechanism.
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The methionine salvage pathway is ubiquitous in all organisms, but metabolic variations exist between bacteria and mammals. 5-Methylthioribose (MTR) kinase is a key enzyme in methionine salvage in bacteria and the absence of a mammalian homolog suggests that it is a good target for the design of novel antibiotics. The structures of the apo-form of Bacillus subtilis MTR kinase, as well as its ADP, ADP-PO(4), AMPPCP, and AMPPCP-MTR complexes have been determined. MTR kinase has a bilobal eukaryotic protein kinase fold but exhibits a number of unique features. The protein lacks the DFG motif typically found at the beginning of the activation loop and instead coordinates magnesium via a DXE motif (Asp(250)-Glu(252)). In addition, the glycine-rich loop of the protein, analogous to the "Gly triad" in protein kinases, does not interact extensively with the nucleotide. The MTR substrate-binding site consists of Asp(233) of the catalytic HGD motif, a novel twin arginine motif (Arg(340)/Arg(341)), and a semi-conserved W-loop, which appears to regulate MTR binding specificity. No lobe closure is observed for MTR kinase upon substrate binding. This is probably because the enzyme lacks the lobe closure/inducing interactions between the C-lobe of the protein and the ribosyl moiety of the nucleotide that are typically responsible for lobe closure in protein kinases. The current structures suggest that MTR kinase has a dissociative mechanism.
==About this Structure==
==About this Structure==
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[[Category: S-methyl-5-thioribose kinase]]
[[Category: S-methyl-5-thioribose kinase]]
[[Category: Single protein]]
[[Category: Single protein]]
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[[Category: Ku, S.Y.]]
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[[Category: Ku, S Y.]]
[[Category: ADP]]
[[Category: ADP]]
[[Category: CPS]]
[[Category: CPS]]
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[[Category: methionine recycling pathway]]
[[Category: methionine recycling pathway]]
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''Page seeded by [http://oca.weizmann.ac.il/oca OCA ] on Wed Jan 23 14:14:41 2008''
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''Page seeded by [http://oca.weizmann.ac.il/oca OCA ] on Thu Feb 21 18:33:06 2008''

Revision as of 16:33, 21 February 2008

Image:2pui.gif

2pui, resolution 2.20Å

Drag the structure with the mouse to rotate

Structures of 5-methylthioribose kinase reveal substrate specificity and unusual mode of nucleotide binding

Overview

The methionine salvage pathway is ubiquitous in all organisms, but metabolic variations exist between bacteria and mammals. 5-Methylthioribose (MTR) kinase is a key enzyme in methionine salvage in bacteria and the absence of a mammalian homolog suggests that it is a good target for the design of novel antibiotics. The structures of the apo-form of Bacillus subtilis MTR kinase, as well as its ADP, ADP-PO(4), AMPPCP, and AMPPCP-MTR complexes have been determined. MTR kinase has a bilobal eukaryotic protein kinase fold but exhibits a number of unique features. The protein lacks the DFG motif typically found at the beginning of the activation loop and instead coordinates magnesium via a DXE motif (Asp(250)-Glu(252)). In addition, the glycine-rich loop of the protein, analogous to the "Gly triad" in protein kinases, does not interact extensively with the nucleotide. The MTR substrate-binding site consists of Asp(233) of the catalytic HGD motif, a novel twin arginine motif (Arg(340)/Arg(341)), and a semi-conserved W-loop, which appears to regulate MTR binding specificity. No lobe closure is observed for MTR kinase upon substrate binding. This is probably because the enzyme lacks the lobe closure/inducing interactions between the C-lobe of the protein and the ribosyl moiety of the nucleotide that are typically responsible for lobe closure in protein kinases. The current structures suggest that MTR kinase has a dissociative mechanism.

About this Structure

2PUI is a Single protein structure of sequence from Bacillus subtilis with , and as ligands. Active as S-methyl-5-thioribose kinase, with EC number 2.7.1.100 Full crystallographic information is available from OCA.

Reference

Structures of 5-methylthioribose kinase reveal substrate specificity and unusual mode of nucleotide binding., Ku SY, Yip P, Cornell KA, Riscoe MK, Behr JB, Guillerm G, Howell PL, J Biol Chem. 2007 Jul 27;282(30):22195-206. Epub 2007 May 23. PMID:17522047

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