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Prostaglandin F synthase

January 01, 1970

In enzymology, a prostaglandin-F synthase (PGFS; EC 1.1.1.188) is an enzyme that catalyzes the chemical reaction:

prostaglandin-F synthase
Identifiers
EC no.1.1.1.188
CAS no.55976-95-9
Databases
IntEnzIntEnz view
BRENDABRENDA entry
ExPASyNiceZyme view
KEGGKEGG entry
MetaCycmetabolic pathway
PRIAMprofile
PDB structuresRCSB PDB PDBe PDBsum
Gene OntologyAmiGO / QuickGO
Search
PMCarticles
PubMedarticles
NCBIproteins
(5Z,13E)-(15S)-9alpha,11alpha,15-trihydroxyprosta-5,13-dienoate + NADP+ (5Z,13E)-(15S)-9alpha,15-dihydroxy-11-oxoprosta-5,13-dienoate + NADPH + H+

Thus, the two products of this enzyme are 9α,11β–PGF2 and NADP+, whereas its three substrates are Prostaglandin D2, NADPH, and H+.

PGFS is a monomeric wild-type protein that was first purified from bovine lung (PDB ID: 2F38).[1] This enzyme belongs to the family of aldo-keto reductase (AKR) based on its high substrate specificity, its high molecular weight (38055.48 Da) and amino acid sequence.[2] In addition, it is categorized as C3 (AKR1C3) because it is an isoform of 3α-hydroxysteroid dehydrogenase.[3]

The function of PGFS is to catalyze the reduction of aldehydes and ketones to their corresponding alcohols. In humans, these reactions take place mostly in the lungs and in the liver.[4] More specifically, PGFS catalyzes the reduction of PGD2 to 9α,11β–PGF2 and PGH2 to PGF2α by using NADPH as cofactor.[2]

Nomenclature edit

This enzyme belongs to the family of oxidoreductases, specifically those acting on the CH-OH group of donor with NAD+ or NADP+ as acceptor. The systematic name of this enzyme class is (5Z,13E)-(15S)-9alpha,11alpha,15-trihydroxyprosta-5,13-dienoate:NADP+ 11-oxidoreductase.

Other names in common use include prostaglandin-D2 11-reductase, reductase, 15-hydroxy-11-oxoprostaglandin, PGD2 11-ketoreductase, PGF synthetase, prostaglandin 11-ketoreductase, prostaglandin D2-ketoreductase, prostaglandin F synthase, prostaglandin F synthetase, synthetase, prostaglandin F, prostaglandin-D2 11-reductase, PGF synthetase, NADPH-dependent prostaglandin D2 11-keto reductase, and prostaglandin 11-keto reductase. This enzyme participates in arachidonic acid metabolism.

Structure edit

As of late 2007, 7 structures have been solved for this class of enzymes, with PDB accession codes 1RY0, 1RY8, 1VBJ, 1XF0, 1ZQ5, 2F38, and 2FGB.

The primary structure of prostaglandin F synthase consists of 323 amino acid residues.[5] The secondary structure consists of 17 α-helices which contain 130 residues and 18 β-strands which contain 55 residues as well as many random coils. The tertiary structure is a single subunit.[2]

The active site of the enzyme is referred to as an (α/β)8 barrel because it consists of 8 α-helices and 8 β-strands. More specifically, the eight α-helices surround the eight β-strands which form the cylindrical core of the active site.[2] In addition, the active site of the enzyme contains also three random coils which help to connect the helices and strands together.[6] The size of the active site of the enzyme is large enough not only to bind NADPH cofactor but also to bind the substrates PGD2 or PGH2.[3]

Reaction edit

 
Reduction of PGD2 and PGH2.

In order for the PGFS enzyme to catalyze the reduction of the substrates PGH2 or PGD2, the cofactor NADPH must be present in the active site. This cofactor is present deep within the cavity of the enzyme and forms a hydrogen bond with it, whereas the substrate is located closer to the mouth of the cavity which limits its interaction with PGFS. The rate determining step of the catalysis is the binding of NADPH cofactor in the active site of the enzyme. This is because the binding of NADPH occurs before the binding of the substrate. NADPH is an important cofactor because it is involved in the hydride transfer which is necessary for the reduction to take place.[3]

More specifically, in order for the hydride transfer to occur, the substrate (PGD2) has to bind to the active site of the enzyme PGFS. The substrate binds to the active site through hydrogen bonding between the carbonyl group of PGD2 and the hydroxyl group of tyrosine (Y55) as well as one of the imidazole nitrogen of histidine (H117). The hydride shift from NADPH reduces the carbonyl group of PGD2 and forms a new sp3 hydroxyl group (9α,11β–PGF2).[3]

The protonation of the carbonyl oxygen is facilitated at low pH when histidine is used and at high pH when tyrosine is used for hydrogen bonding with the substrate. On the one hand, histidine is an ideal proton donor at low pH because of its pKa value (6.00), which means that it is protonated at a pH below 6.00. On the other hand, tyrosine is an ideal proton donor at higher pH because of its pKa value (10.1). The type of amino acid that is used for protonation depends on the substrate. For example, reduction of PGD2 in the human body occurs at a pH range of 6-9, which makes histidine an ideal proton donor.[3]

The hydride that is transferred to the carbonyl oxygen of PGD2 causes weakening of the hydrogen bond between the substrate and the enzyme. This has as a result the cleavage of the product (9α,11β–PGF2) from the active site of the enzyme.[3]

Use edit

In general, prostaglandins are molecules that are used for inflammation, muscle contraction and blood clotting.[3] Prostaglandin F synthase (PGFS) is very important enzyme because it catalyzes the formation of 9α,11β–PGF2 and PGF2α which are critical for the contraction of bronchial, vascular and arterial smooth muscle.[2]

Also, this enzyme can be used in cancer research. Recent studies have shown that there is a correlation between high levels of PGFS in gastrointestinal tumors and the effectiveness of non-steroidal anti-inflammatory drugs (NSAID). The inhibition of PGFS by NSAID could turn out to be a very important medicinal field in the development of anti-cancer medication.[6]    

Inhibition  edit

 
Chemical structure of bimatoprost

Prostaglandin F synthase can be inhibited not only by NSAIDs such as indometacin and suprofen but also by a molecule known as bimatoprost (BMP). BMP, an analogue of PGD2 is an ocular hypotensive agent that binds to the active site of the PGFS enzyme. This means that it inhibits the action of PGFS to catalyze the conversion of PGD2 to 9α,11β–PGF2 and PGH2 to PGF2α because it inhibits the substrate to bind to the active site of the enzyme.[6]

References edit

  1. ^ Watanabe K, Yoshida R, Shimizu T, Hayaishi O (June 1985). "Enzymatic formation of prostaglandin F2 alpha from prostaglandin H2 and D2. Purification and properties of prostaglandin F synthetase from bovine lung". The Journal of Biological Chemistry. 260 (11): 7035–41. doi:10.1016/S0021-9258(18)88884-6. PMID 3858278.
  2. ^ a b c d e Watanabe K (August 2002). "Prostaglandin F synthase". Prostaglandins & Other Lipid Mediators. 68–69: 401–7. doi:10.1016/s0090-6980(02)00044-8. PMID 12432932.
  3. ^ a b c d e f g Komoto J, Yamada T, Watanabe K, Takusagawa F (March 2004). "Crystal structure of human prostaglandin F synthase (AKR1C3)". Biochemistry. 43 (8): 2188–98. doi:10.1021/bi036046x. PMID 14979715.
  4. ^ Yoshikawa K, Takei S, Hasegawa-Ishii S, Chiba Y, Furukawa A, Kawamura N, et al. (January 2011). "Preferential localization of prostamide/prostaglandin F synthase in myelin sheaths of the central nervous system". Brain Research. 1367: 22–32. doi:10.1016/j.brainres.2010.10.019. PMID 20950588. S2CID 43094318.
  5. ^ "RCSB PDB - 2F38: Crystal structure of prostaglandin F synathase containing bimatoprost". RCSB Protein Data Bank Bank. Retrieved 2020-12-08.
  6. ^ a b c Komoto J, Yamada T, Watanabe K, Woodward DF, Takusagawa F (February 2006). "Prostaglandin F2alpha formation from prostaglandin H2 by prostaglandin F synthase (PGFS): crystal structure of PGFS containing bimatoprost". Biochemistry. 45 (7): 1987–96. doi:10.1021/bi051861t. PMID 16475787.

Further reading edit

  • Reingold DF, Kawasaki A, Needleman P (May 1981). "A novel prostaglandin 11-keto reductase found in rabbit liver". Biochimica et Biophysica Acta (BBA) - Enzymology. 659 (1): 179–88. doi:10.1016/0005-2744(81)90282-5. PMID 7248318.
  • Watanabe K, Shimizu T, Hayaishi O (1981). "Enzymatic conversion of prostaglandin-D2 to prostaglandin-F in the rat lung". Biochem. Int. 2: 603–610.
  • Wong PY (May 1981). "Purification and partial characterization of prostaglandin D2 11-keto reductase in rabbit liver". Biochimica et Biophysica Acta (BBA) - Enzymology. 659 (1): 169–78. doi:10.1016/0005-2744(81)90281-3. PMID 7248317.
  • Wong PY (1982). "Purification of PGD2 11-ketoreductase from rabbit liver". Prostaglandins and Arachidonate Metabolites. Methods in Enzymology. Vol. 86. pp. 117–25. doi:10.1016/0076-6879(82)86179-X. ISBN 978-0-12-181986-6. PMID 7132748.

January 01, 1970
prostaglandin, synthase, enzymology, prostaglandin, synthase, pgfs, enzyme, that, catalyzes, chemical, reaction, prostaglandin, synthaseidentifiersec, 188cas, 55976, 9databasesintenzintenz, viewbrendabrenda, entryexpasynicezyme, viewkeggkegg, entrymetacycmetab. In enzymology a prostaglandin F synthase PGFS EC 1 1 1 188 is an enzyme that catalyzes the chemical reaction prostaglandin F synthaseIdentifiersEC no 1 1 1 188CAS no 55976 95 9DatabasesIntEnzIntEnz viewBRENDABRENDA entryExPASyNiceZyme viewKEGGKEGG entryMetaCycmetabolic pathwayPRIAMprofilePDB structuresRCSB PDB PDBe PDBsumGene OntologyAmiGO QuickGOSearchPMCarticlesPubMedarticlesNCBIproteins 5Z 13E 15S 9alpha 11alpha 15 trihydroxyprosta 5 13 dienoate NADP displaystyle rightleftharpoons 5Z 13E 15S 9alpha 15 dihydroxy 11 oxoprosta 5 13 dienoate NADPH H Thus the two products of this enzyme are 9a 11b PGF2 and NADP whereas its three substrates are Prostaglandin D2 NADPH and H PGFS is a monomeric wild type protein that was first purified from bovine lung PDB ID 2F38 1 This enzyme belongs to the family of aldo keto reductase AKR based on its high substrate specificity its high molecular weight 38055 48 Da and amino acid sequence 2 In addition it is categorized as C3 AKR1C3 because it is an isoform of 3a hydroxysteroid dehydrogenase 3 The function of PGFS is to catalyze the reduction of aldehydes and ketones to their corresponding alcohols In humans these reactions take place mostly in the lungs and in the liver 4 More specifically PGFS catalyzes the reduction of PGD2 to 9a 11b PGF2 and PGH2 to PGF2a by using NADPH as cofactor 2 Contents 1 Nomenclature 2 Structure 3 Reaction 4 Use 5 Inhibition 6 References 7 Further readingNomenclature editThis enzyme belongs to the family of oxidoreductases specifically those acting on the CH OH group of donor with NAD or NADP as acceptor The systematic name of this enzyme class is 5Z 13E 15S 9alpha 11alpha 15 trihydroxyprosta 5 13 dienoate NADP 11 oxidoreductase Other names in common use include prostaglandin D2 11 reductase reductase 15 hydroxy 11 oxoprostaglandin PGD2 11 ketoreductase PGF2a synthetase prostaglandin 11 ketoreductase prostaglandin D2 ketoreductase prostaglandin F synthase prostaglandin F synthetase synthetase prostaglandin F2a prostaglandin D2 11 reductase PGF synthetase NADPH dependent prostaglandin D2 11 keto reductase and prostaglandin 11 keto reductase This enzyme participates in arachidonic acid metabolism Structure editAs of late 2007 update 7 structures have been solved for this class of enzymes with PDB accession codes 1RY0 1RY8 1VBJ 1XF0 1ZQ5 2F38 and 2FGB The primary structure of prostaglandin F synthase consists of 323 amino acid residues 5 The secondary structure consists of 17 a helices which contain 130 residues and 18 b strands which contain 55 residues as well as many random coils The tertiary structure is a single subunit 2 The active site of the enzyme is referred to as an a b 8 barrel because it consists of 8 a helices and 8 b strands More specifically the eight a helices surround the eight b strands which form the cylindrical core of the active site 2 In addition the active site of the enzyme contains also three random coils which help to connect the helices and strands together 6 The size of the active site of the enzyme is large enough not only to bind NADPH cofactor but also to bind the substrates PGD2 or PGH2 3 Reaction edit nbsp Reduction of PGD2 and PGH2 In order for the PGFS enzyme to catalyze the reduction of the substrates PGH2 or PGD2 the cofactor NADPH must be present in the active site This cofactor is present deep within the cavity of the enzyme and forms a hydrogen bond with it whereas the substrate is located closer to the mouth of the cavity which limits its interaction with PGFS The rate determining step of the catalysis is the binding of NADPH cofactor in the active site of the enzyme This is because the binding of NADPH occurs before the binding of the substrate NADPH is an important cofactor because it is involved in the hydride transfer which is necessary for the reduction to take place 3 More specifically in order for the hydride transfer to occur the substrate PGD2 has to bind to the active site of the enzyme PGFS The substrate binds to the active site through hydrogen bonding between the carbonyl group of PGD2 and the hydroxyl group of tyrosine Y55 as well as one of the imidazole nitrogen of histidine H117 The hydride shift from NADPH reduces the carbonyl group of PGD2 and forms a new sp3 hydroxyl group 9a 11b PGF2 3 The protonation of the carbonyl oxygen is facilitated at low pH when histidine is used and at high pH when tyrosine is used for hydrogen bonding with the substrate On the one hand histidine is an ideal proton donor at low pH because of its pKa value 6 00 which means that it is protonated at a pH below 6 00 On the other hand tyrosine is an ideal proton donor at higher pH because of its pKa value 10 1 The type of amino acid that is used for protonation depends on the substrate For example reduction of PGD2 in the human body occurs at a pH range of 6 9 which makes histidine an ideal proton donor 3 The hydride that is transferred to the carbonyl oxygen of PGD2 causes weakening of the hydrogen bond between the substrate and the enzyme This has as a result the cleavage of the product 9a 11b PGF2 from the active site of the enzyme 3 Use editIn general prostaglandins are molecules that are used for inflammation muscle contraction and blood clotting 3 Prostaglandin F synthase PGFS is very important enzyme because it catalyzes the formation of 9a 11b PGF2 and PGF2a which are critical for the contraction of bronchial vascular and arterial smooth muscle 2 Also this enzyme can be used in cancer research Recent studies have shown that there is a correlation between high levels of PGFS in gastrointestinal tumors and the effectiveness of non steroidal anti inflammatory drugs NSAID The inhibition of PGFS by NSAID could turn out to be a very important medicinal field in the development of anti cancer medication 6 Inhibition edit nbsp Chemical structure of bimatoprost Prostaglandin F synthase can be inhibited not only by NSAIDs such as indometacin and suprofen but also by a molecule known as bimatoprost BMP BMP an analogue of PGD2 is an ocular hypotensive agent that binds to the active site of the PGFS enzyme This means that it inhibits the action of PGFS to catalyze the conversion of PGD2 to 9a 11b PGF2 and PGH2 to PGF2a because it inhibits the substrate to bind to the active site of the enzyme 6 References edit Watanabe K Yoshida R Shimizu T Hayaishi O June 1985 Enzymatic formation of prostaglandin F2 alpha from prostaglandin H2 and D2 Purification and properties of prostaglandin F synthetase from bovine lung The Journal of Biological Chemistry 260 11 7035 41 doi 10 1016 S0021 9258 18 88884 6 PMID 3858278 a b c d e Watanabe K August 2002 Prostaglandin F synthase Prostaglandins amp Other Lipid Mediators 68 69 401 7 doi 10 1016 s0090 6980 02 00044 8 PMID 12432932 a b c d e f g Komoto J Yamada T Watanabe K Takusagawa F March 2004 Crystal structure of human prostaglandin F synthase AKR1C3 Biochemistry 43 8 2188 98 doi 10 1021 bi036046x PMID 14979715 Yoshikawa K Takei S Hasegawa Ishii S Chiba Y Furukawa A Kawamura N et al January 2011 Preferential localization of prostamide prostaglandin F synthase in myelin sheaths of the central nervous system Brain Research 1367 22 32 doi 10 1016 j brainres 2010 10 019 PMID 20950588 S2CID 43094318 RCSB PDB 2F38 Crystal structure of prostaglandin F synathase containing bimatoprost RCSB Protein Data Bank Bank Retrieved 2020 12 08 a b c Komoto J Yamada T Watanabe K Woodward DF Takusagawa F February 2006 Prostaglandin F2alpha formation from prostaglandin H2 by prostaglandin F synthase PGFS crystal structure of PGFS containing bimatoprost Biochemistry 45 7 1987 96 doi 10 1021 bi051861t PMID 16475787 Further reading editReingold DF Kawasaki A Needleman P May 1981 A novel prostaglandin 11 keto reductase found in rabbit liver Biochimica et Biophysica Acta BBA Enzymology 659 1 179 88 doi 10 1016 0005 2744 81 90282 5 PMID 7248318 Watanabe K Shimizu T Hayaishi O 1981 Enzymatic conversion of prostaglandin D2 to prostaglandin F2a in the rat lung Biochem Int 2 603 610 Wong PY May 1981 Purification and partial characterization of prostaglandin D2 11 keto reductase in rabbit liver Biochimica et Biophysica Acta BBA Enzymology 659 1 169 78 doi 10 1016 0005 2744 81 90281 3 PMID 7248317 Wong PY 1982 Purification of PGD2 11 ketoreductase from rabbit liver Prostaglandins and Arachidonate Metabolites Methods in Enzymology Vol 86 pp 117 25 doi 10 1016 0076 6879 82 86179 X ISBN 978 0 12 181986 6 PMID 7132748 Portal nbsp Biology Retrieved from https en wikipedia org w index php title Prostaglandin F synthase amp oldid 1220586855, wikipedia, wiki, book, books, library,

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