DB code: T00114

RLCP classification	1.13.30000.42 : Hydrolysis
RLCP classification	3.123.90030.312 : Transfer
CATH domain	3.40.50.880 : Rossmann fold	Catalytic domain
	3.40.50.620 : Rossmann fold	Catalytic domain
	3.30.300.10 : GMP Synthetase; Chain A, domain 3
E.C.	6.3.5.2
CSA	1gpm
M-CSA	1gpm
MACiE	M0234

CATH domain	Related DB codes (homologues)
3.40.50.620 : Rossmann fold	S00314 S00549 S00316 S00317 S00318 S00315 T00085 T00249 D00300 M00177 M00178 T00106
3.40.50.880 : Rossmann fold	D00526 T00021 M00215

Uniprot Enzyme Name
UniprotKB	Protein name	Synonyms	RefSeq	MEROPS	Pfam
P04079	GMP synthase {glutamine-hydrolyzing}	EC 6.3.5.2 Glutamine amidotransferase GMP synthetase GMPS	NP_417002.1 (Protein) NC_000913.2 (DNA/RNA sequence) YP_490735.1 (Protein) NC_007779.1 (DNA/RNA sequence)	C26.957 (Cysteine)	PF00117 (GATase) PF00958 (GMP_synt_C) PF02540 (NAD_synthase) [Graphical View]

KEGG enzyme name
GMP synthase (glutamine-hydrolysing) GMP synthetase (glutamine-hydrolysing) guanylate synthetase (glutamine-hydrolyzing) guanosine monophosphate synthetase (glutamine-hydrolyzing) xanthosine 5'-phosphate amidotransferase guanosine 5'-monophosphate synthetase

UniprotKB: Accession Number	Entry name	Activity	Subunit	Subcellular location	Cofactor
P04079	GUAA_ECOLI	ATP + xanthosine 5''-phosphate + L-glutamine + H(2)O = AMP + diphosphate + GMP + L-glutamate.	Homodimer.

KEGG Pathways
Map code	Pathways	E.C.
MAP00230	Purine metabolism
MAP00251	Glutamate metabolism
MAP00983	Drug metabolism - other enzymes

Compound table
	Cofactors	Substrates				Products				Intermediates
KEGG-id	C00305	C00002	C00655	C00064	C00001	C00020	C00013	C00144	C00025
E.C.
Compound	Magnesium	ATP	Xanthosine 5'-phosphate	L-Glutamine	H2O	AMP	Pyrophosphate	GMP	L-Glutamate
Type	divalent metal (Ca2+, Mg2+)	amine group,nucleotide	amide group,nucleotide	amino acids,amide group	H2O	amine group,nucleotide	phosphate group/phosphate ion	amide group,amine group,nucleotide	amino acids,carboxyl group
ChEBI	18420 18420	15422 15422	15652 15652	18050 58359 18050 58359	15377 15377	16027 16027	29888 29888	17345 17345	16015 16015
PubChem	888 888	5957 5957	73323 73323	5961 6992086 5961 6992086	22247451 962 22247451 962	6083 6083	1023 21961011 1023 21961011	6804 6804	33032 44272391 88747398 33032 44272391 88747398

1gpmA01	Unbound	Unbound	Unbound	Unbound		Unbound	Unbound	Unbound	Unbound
1gpmB01	Unbound	Unbound	Unbound	Unbound		Unbound	Unbound	Unbound	Unbound
1gpmC01	Unbound	Unbound	Unbound	Unbound		Unbound	Unbound	Unbound	Unbound
1gpmD01	Unbound	Unbound	Unbound	Unbound		Unbound	Unbound	Unbound	Unbound
1gpmA02	Unbound	Unbound	Unbound	Unbound		Bound:AMP	Bound:POP	Unbound	Unbound
1gpmB02	Bound:_MG	Unbound	Unbound	Unbound		Bound:AMP	Bound:POP	Unbound	Unbound
1gpmC02	Bound:_MG	Unbound	Unbound	Unbound		Bound:AMP	Bound:POP	Unbound	Unbound
1gpmD02	Bound:_MG	Unbound	Unbound	Unbound		Bound:AMP	Bound:POP	Unbound	Unbound
1gpmA03	Unbound	Unbound	Unbound	Unbound		Unbound	Analogue:PO4	Unbound	Unbound
1gpmB03	Unbound	Unbound	Unbound	Unbound		Unbound	Analogue:PO4	Unbound	Unbound
1gpmC03	Unbound	Unbound	Unbound	Unbound		Unbound	Analogue:PO4	Unbound	Unbound
1gpmD03	Unbound	Unbound	Unbound	Unbound		Unbound	Analogue:PO4	Unbound	Unbound

Reference for Active-site residues
resource	references	E.C.
Swiss-prot;P04079, literature [6]

Active-site residues
PDB	Catalytic residues	Cofactor-binding residues	Modified residues	Main-chain involved in catalysis	Comment

1gpmA01	CYS 86;HIS 181;GLU 183			GLY 59;TYR 87;GLY 88
1gpmB01	CYS 86;HIS 181;GLU 183			GLY 59;TYR 87;GLY 88
1gpmC01	CYS 86;HIS 181;GLU 183			GLY 59;TYR 87;GLY 88
1gpmD01	CYS 86;HIS 181;GLU 183			GLY 59;TYR 87;GLY 88
1gpmA02	SER 235;SER 240;LYS 381	ASP 239(Magnesium binding)		GLY 236;GLY 237
1gpmB02	SER 235;SER 240;LYS 381	ASP 239(Magnesium binding)		GLY 236;GLY 237
1gpmC02	SER 235;SER 240;LYS 381	ASP 239(Magnesium binding)		GLY 236;GLY 237
1gpmD02	SER 235;SER 240;LYS 381	ASP 239(Magnesium binding)		GLY 236;GLY 237
1gpmA03
1gpmB03
1gpmC03
1gpmD03

References for Catalytic Mechanism
References	Sections	No. of steps in catalysis
[1]	Fig.11, p.2646	2
[6]	Fig.1, p.75	2
[8]	Scheme 3

References
[1]
Resource
Comments
Medline ID
PubMed ID	6378670
Journal	Fed Proc
Year	1984
Volume	43
Pages	2640-7
Authors	Villafranca JJ
Title	Use of 31P and 13C NMR to study enzyme mechanisms.
Related PDB
Related UniProtKB
[2]
Resource
Comments	GATASE DOMAIN.
Medline ID	85131126
PubMed ID	2982857
Journal	J Biol Chem
Year	1985
Volume	260
Pages	3350-4
Authors	Zalkin H, Argos P, Narayana SV, Tiedeman AA, Smith JM
Title	Identification of a trpG-related glutamine amide transfer domain in Escherichia coli GMP synthetase.
Related PDB
Related UniProtKB	P04079
[3]
Resource
Comments
Medline ID
PubMed ID	3911001
Journal	Methods Enzymol
Year	1985
Volume	113
Pages	273-8
Authors	Zalkin H
Title	GMP synthetase.
Related PDB
Related UniProtKB
[4]
Resource
Comments
Medline ID
PubMed ID	8208731
Journal	Proteins
Year	1994
Volume	18
Pages	394-403
Authors	Tesmer JJ, Stemmler TL, Penner-Hahn JE, Davisson VJ, Smith JL
Title	Preliminary X-ray analysis of Escherichia coli GMP synthetase: determination of anomalous scattering factors for a cysteinyl mercury derivative.
Related PDB
Related UniProtKB
[5]
Resource
Comments
Medline ID
PubMed ID	8895556
Journal	EMBO J
Year	1996
Volume	15
Pages	5125-34
Authors	Rizzi M, Nessi C, Mattevi A, Coda A, Bolognesi M, Galizzi A
Title	Crystal structure of NH3-dependent NAD+ synthetase from Bacillus subtilis.
Related PDB
Related UniProtKB
[6]
Resource
Comments	X-RAY CRYSTALLOGRAPHY (2.2 ANGSTROMS).
Medline ID	96133732
PubMed ID	8548458
Journal	Nat Struct Biol
Year	1996
Volume	3
Pages	74-86
Authors	Tesmer JJ, Klem TJ, Deras ML, Davisson VJ, Smith JL
Title	The crystal structure of GMP synthetase reveals a novel catalytic triad and is a structural paradigm for two enzyme families.
Related PDB	1gpm
Related UniProtKB	P04079
[7]
Resource
Comments
Medline ID
PubMed ID	11395405
Journal	Annu Rev Biochem
Year	2001
Volume	70
Pages	149-80
Authors	Huang X, Holden HM, Raushel FM
Title	Channeling of substrates and intermediates in enzyme-catalyzed reactions.
Related PDB
Related UniProtKB
[8]
Resource
Comments
Medline ID
PubMed ID	11170408
Journal	Biochemistry
Year	2001
Volume	40
Pages	876-87
Authors	Chittur SV, Klem TJ, Shafer CM, Davisson VJ
Title	Mechanism for acivicin inactivation of triad glutamine amidotransferases.
Related PDB
Related UniProtKB

Comments
According to the literature [6], [7], separate reactions occur at the N-terminal glutaminase domain (CATH 3.40.50.880) and at the ATP pyrophosphatase domain (CATH 3.40.50.620). At the N-terminal glutaminase domain, which contains a catalytic triad (Cys86/His181/Glu183) and an oxyanion hole (composed of mainchain amide of Gly59/Tyr88/Gly88), hydrolysis of the sidechain amide of glutamine occurs by the trypsin-like reaction mechanism (see [6] & [8]). (1) Cys86 acts as a nucleophile to make an attack on the carbonyl carbon. His181 and Glu183 assist this reaction. (2) The transient negative charge on the intermediate will be stabilized by the oxyanion hole. (3) A water molecule, activated by His181, may hydrolyze the intermediate. At the ATP pyrophosphatase domain, two successive transfer reactions, transfer of AMP to carbonyl oxygen (O2 atom) of the XMP base, and transfer of the purine nucleotide to amine of ammonia molecule, released by the N-terminal domain. According to the active-site structure and the data of the homologous enzyme (S00315 in EzCatDB), the transfer reaction of AMP to the carbonyl oxygen of XMP proceeds, probably as follows: (A1) Mg2+ ion, Ser235, Gly236, Gly237 and Ser240 from P-loop and Lys381 stabilizes the leaving pyrophosphate, by neutralizing the negative charges, and also activate the transferred group, alpha-phosphate of ATP, by enhancing the electrophilicity of the phosphate group through polarization. (A2) The acceptor group, the carbonyl oxygen (O2) atom of the XMP base, makes a nucleophilic attack on the transferred group, the alpha-phosphate of ATP. (A3) The Mg2+ ion stabilize the pentacovalent transition-state. (A4) O2-Adenyl-XMP intermediate is formed, releasing the pyrophosphate. The detailed mechanism of the transfer of the nucleotide to amine of the ammonia molecule has not been elucidated. However, it will probably proceeds as follows: (B1) Some group must act as a general base, to deprotonate the ammonium ion. However, it is not clear which group will activate the ammonium ion. (Probably, the remaining pyrophosphate or Asp340, considering the structure) (B2) The activated ammonium makes a nucleophilic attack on the C2 atom of the O2-adenyl-XMP intermediate, forming a tetrahedral transition-state adduct. (B3) Some group must stabilize the tetrahedral transition-state. However, it is not clear which group is involved in the stabilization. Mg2+ ion will stabilize the leaving phosphate of AMP. (B4) Finally, GMP and AMP are formed. More biochemical data will be required, to elucidate the mechanism.

Comments

According to the literature [6], [7], separate reactions occur at the N-terminal glutaminase domain (CATH 3.40.50.880) and at the ATP pyrophosphatase domain (CATH 3.40.50.620).
At the N-terminal glutaminase domain, which contains a catalytic triad (Cys86/His181/Glu183) and an oxyanion hole (composed of mainchain amide of Gly59/Tyr88/Gly88), hydrolysis of the sidechain amide of glutamine occurs by the trypsin-like reaction mechanism (see [6] & [8]).
(1) Cys86 acts as a nucleophile to make an attack on the carbonyl carbon. His181 and Glu183 assist this reaction.
(2) The transient negative charge on the intermediate will be stabilized by the oxyanion hole.
(3) A water molecule, activated by His181, may hydrolyze the intermediate.
At the ATP pyrophosphatase domain, two successive transfer reactions, transfer of AMP to carbonyl oxygen (O2 atom) of the XMP base, and transfer of the purine nucleotide to amine of ammonia molecule, released by the N-terminal domain.
According to the active-site structure and the data of the homologous enzyme (S00315 in EzCatDB), the transfer reaction of AMP to the carbonyl oxygen of XMP proceeds, probably as follows:
(A1) Mg2+ ion, Ser235, Gly236, Gly237 and Ser240 from P-loop and Lys381 stabilizes the leaving pyrophosphate, by neutralizing the negative charges, and also activate the transferred group, alpha-phosphate of ATP, by enhancing the electrophilicity of the phosphate group through polarization.
(A2) The acceptor group, the carbonyl oxygen (O2) atom of the XMP base, makes a nucleophilic attack on the transferred group, the alpha-phosphate of ATP.
(A3) The Mg2+ ion stabilize the pentacovalent transition-state.
(A4) O2-Adenyl-XMP intermediate is formed, releasing the pyrophosphate.
The detailed mechanism of the transfer of the nucleotide to amine of the ammonia molecule has not been elucidated. However, it will probably proceeds as follows:
(B1) Some group must act as a general base, to deprotonate the ammonium ion. However, it is not clear which group will activate the ammonium ion. (Probably, the remaining pyrophosphate or Asp340, considering the structure)
(B2) The activated ammonium makes a nucleophilic attack on the C2 atom of the O2-adenyl-XMP intermediate, forming a tetrahedral transition-state adduct.
(B3) Some group must stabilize the tetrahedral transition-state. However, it is not clear which group is involved in the stabilization. Mg2+ ion will stabilize the leaving phosphate of AMP.
(B4) Finally, GMP and AMP are formed.
More biochemical data will be required, to elucidate the mechanism.

Created	Updated
2004-09-27	2009-02-26