Structures of Selenomonas ruminantium phytase in complex with persulfated phytate: DSP phytase fold and mechanism for sequential substrate hydrolysis

Hsing Mao Chu; Rey Ting Guo; Ting Wan Lin; Chia Cheng Chou; Hui Lin Shr; Hui Lin Lai; Tsung Yin Tang; Kuo Joan Cheng; Brent L. Selinger; Andrew H.J. Wang

doi:10.1016/j.str.2004.08.010

Structures of Selenomonas ruminantium phytase in complex with persulfated phytate: DSP phytase fold and mechanism for sequential substrate hydrolysis

Hsing Mao Chu, Rey Ting Guo, Ting Wan Lin, Chia Cheng Chou, Hui Lin Shr, Hui Lin Lai, Tsung Yin Tang, Kuo Joan Cheng, Brent L. Selinger, Andrew H.J. Wang

Research output: Contribution to journal › Article › peer-review

93 Citations (Scopus)

Abstract

Various inositide phosphatases participate in the regulation of inositol polyphosphate signaling molecules. Plant phytases are phosphatases that hydrolyze phytate to less-phosphorylated myo-inositol derivatives and phosphate. The phytase from Selenomonas ruminantium shares no sequence homology with other microbial phytases. Its crystal structure revealed a phytase fold of the dual-specificity phosphatase type. The active site is located near a conserved cysteine-containing (Cys241) P loop. We also solved two other crystal forms in which an inhibitor, myo-inositol hexasulfate, is cocrystallized with the enzyme. In the "standby" and the "inhibited" crystal forms, the inhibitor is bound, respectively, in a pocket slightly away from Cys241 and at the substrate binding site where the phosphate group to be hydrolyzed is held close to the -SH group of Cys241. Our structural and mutagenesis studies allow us to visualize the way in which the P loop-containing phytase attracts and hydrolyzes the substrate (phytate) sequentially.

Original language	English
Pages (from-to)	2015-2024
Number of pages	10
Journal	Structure
Volume	12
Issue number	11
DOIs	https://doi.org/10.1016/j.str.2004.08.010
Publication status	Published - Nov 2004
Externally published	Yes

ASJC Scopus subject areas

Structural Biology
Molecular Biology

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10.1016/j.str.2004.08.010

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@article{7017c2833f2f4ddf964bcbda8c5e8af4,

title = "Structures of Selenomonas ruminantium phytase in complex with persulfated phytate: DSP phytase fold and mechanism for sequential substrate hydrolysis",

abstract = "Various inositide phosphatases participate in the regulation of inositol polyphosphate signaling molecules. Plant phytases are phosphatases that hydrolyze phytate to less-phosphorylated myo-inositol derivatives and phosphate. The phytase from Selenomonas ruminantium shares no sequence homology with other microbial phytases. Its crystal structure revealed a phytase fold of the dual-specificity phosphatase type. The active site is located near a conserved cysteine-containing (Cys241) P loop. We also solved two other crystal forms in which an inhibitor, myo-inositol hexasulfate, is cocrystallized with the enzyme. In the {"}standby{"} and the {"}inhibited{"} crystal forms, the inhibitor is bound, respectively, in a pocket slightly away from Cys241 and at the substrate binding site where the phosphate group to be hydrolyzed is held close to the -SH group of Cys241. Our structural and mutagenesis studies allow us to visualize the way in which the P loop-containing phytase attracts and hydrolyzes the substrate (phytate) sequentially.",

author = "Chu, {Hsing Mao} and Guo, {Rey Ting} and Lin, {Ting Wan} and Chou, {Chia Cheng} and Shr, {Hui Lin} and Lai, {Hui Lin} and Tang, {Tsung Yin} and Cheng, {Kuo Joan} and Selinger, {Brent L.} and Wang, {Andrew H.J.}",

note = "Funding Information: The synchrotron data collections were conducted with the Biological Crystallography Facilities (Beamline BL17B2 at NSRRC in HsinChu, Taiwan and Taiwan Beamline BL12B2 at SPring-8, Japan) supported by the National Science Council (NSC). This work was supported by the Academia Sinica and the National Science Council (NSC91-3112-P-001-019-Y) to A.H.-J.W. ",

year = "2004",

month = nov,

doi = "10.1016/j.str.2004.08.010",

language = "English",

volume = "12",

pages = "2015--2024",

journal = "Structure",

issn = "0969-2126",

publisher = "Cell Press",

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T1 - Structures of Selenomonas ruminantium phytase in complex with persulfated phytate

T2 - DSP phytase fold and mechanism for sequential substrate hydrolysis

AU - Chu, Hsing Mao

AU - Guo, Rey Ting

AU - Lin, Ting Wan

AU - Chou, Chia Cheng

AU - Shr, Hui Lin

AU - Lai, Hui Lin

AU - Tang, Tsung Yin

AU - Cheng, Kuo Joan

AU - Selinger, Brent L.

AU - Wang, Andrew H.J.

N1 - Funding Information: The synchrotron data collections were conducted with the Biological Crystallography Facilities (Beamline BL17B2 at NSRRC in HsinChu, Taiwan and Taiwan Beamline BL12B2 at SPring-8, Japan) supported by the National Science Council (NSC). This work was supported by the Academia Sinica and the National Science Council (NSC91-3112-P-001-019-Y) to A.H.-J.W.

PY - 2004/11

Y1 - 2004/11

N2 - Various inositide phosphatases participate in the regulation of inositol polyphosphate signaling molecules. Plant phytases are phosphatases that hydrolyze phytate to less-phosphorylated myo-inositol derivatives and phosphate. The phytase from Selenomonas ruminantium shares no sequence homology with other microbial phytases. Its crystal structure revealed a phytase fold of the dual-specificity phosphatase type. The active site is located near a conserved cysteine-containing (Cys241) P loop. We also solved two other crystal forms in which an inhibitor, myo-inositol hexasulfate, is cocrystallized with the enzyme. In the "standby" and the "inhibited" crystal forms, the inhibitor is bound, respectively, in a pocket slightly away from Cys241 and at the substrate binding site where the phosphate group to be hydrolyzed is held close to the -SH group of Cys241. Our structural and mutagenesis studies allow us to visualize the way in which the P loop-containing phytase attracts and hydrolyzes the substrate (phytate) sequentially.

AB - Various inositide phosphatases participate in the regulation of inositol polyphosphate signaling molecules. Plant phytases are phosphatases that hydrolyze phytate to less-phosphorylated myo-inositol derivatives and phosphate. The phytase from Selenomonas ruminantium shares no sequence homology with other microbial phytases. Its crystal structure revealed a phytase fold of the dual-specificity phosphatase type. The active site is located near a conserved cysteine-containing (Cys241) P loop. We also solved two other crystal forms in which an inhibitor, myo-inositol hexasulfate, is cocrystallized with the enzyme. In the "standby" and the "inhibited" crystal forms, the inhibitor is bound, respectively, in a pocket slightly away from Cys241 and at the substrate binding site where the phosphate group to be hydrolyzed is held close to the -SH group of Cys241. Our structural and mutagenesis studies allow us to visualize the way in which the P loop-containing phytase attracts and hydrolyzes the substrate (phytate) sequentially.

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Structures of Selenomonas ruminantium phytase in complex with persulfated phytate: DSP phytase fold and mechanism for sequential substrate hydrolysis

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