Purification, cloning, and primary structure of an enantiomer-selective amidase from Brevibacterium sp. strain R312: structural evidence for genetic coupling with nitrile hydratase

Mayaux, Jean‐François; Cerebelaud, E; Soubrier, F; Faucher, Didier; Petre, Dominique

doi:10.1128/jb.172.12.6764-6773.1990

Cited by 151 publications

(122 citation statements)

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“…The AS family of hydrolases is found in a wide range of organisms, including archaea (3), eubacteria (1,(4)(5)(6), fungi (7), nematodes, plants, insects, birds (8), and mammals (9,10). Unlike most AS enzymes, FAAH is an integral membrane protein (9,10), which presumably facilitates its role in degrading a large number of amidated lipids in vivo.…”

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confidence: 99%

Structure-Based Design of a FAAH Variant That Discriminates between the N-Acyl Ethanolamine and Taurine Families of Signaling Lipids

McKinney

Cravatt

2006

Biochemistry

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Fatty acid amide hydrolase (FAAH) inactivates a large and diverse class of endogenous signaling lipids termed fatty acid amides. Representative fatty acid amides include the N-acyl ethanolamines (NAEs) anandamide, which serves as an endogenous ligand for cannabinoid receptors, and N-oleoyl and N-palmitoyl ethanolamine, which produce satiety and anti-inflammatory effects, respectively. Global metabolite profiling studies of FAAH (-/-) mice have recently identified a second class of endogenous FAAH substrates: the N-acyl taurines (NATs). To determine the metabolic and signaling functions performed by NAEs and NATs in vivo, a FAAH variant that discriminates between these two substrate classes would be of value. Here, we report the structure-guided design of a point mutant in the active site of FAAH that selectively disrupts interactions with NATs. This glycine-to-aspartate (G268D) mutant was found to exhibit wildtype kinetic parameters with NAEs, but more than a 100-fold reduction in activity with NATs attributable to combined effects on K m and k cat values. These in vitro properties were also observed in living cells, where WT-FAAH and the G268D mutant displayed equivalent hydrolytic activity with NAEs, but the latter enzyme was severely impaired in its ability to catabolize NATs. The G268D FAAH mutant may thus serve as a valuable research tool to illuminate the unique roles played by the NAE and NAT classes of signaling lipids in vivo.Fatty acid amide hydrolase (FAAH) 1 is a member of the amidase signature (AS) family, a diverse group of metabolic enzymes characterized by a conserved serine-and glycinerich stretch of approximately 130 amino acids (1, 2). The AS family of hydrolases is found in a wide range of organisms, including archaea (3), eubacteria (1, 4-6), fungi (7), nematodes, plants, insects, birds (8), and mammals (9, 10). Unlike most AS enzymes, FAAH is an integral membrane protein (9, 10), which presumably facilitates its role in degrading a large number of amidated lipids in vivo.The endogenous fatty acid amide substrates hydrolyzed by FAAH fall into multiple structural classes that display distinct biological activities. A principal class of endogenous FAAH substrates is the N-acyl ethanolamines (NAEs, Figure 1A), which includes several signaling lipids, such as the endogenous cannabinoid N-arachidonoyl ethanolamine or anandamide (C20:4 NAE) (11), the satiating factor N-oleoyl ethanolamine (C18:1 NAE) (12), and the anti-inflammatory substance N-palmitoyl ethanolamine (C16:0 NAE) (13,14).FAAH also hydrolyzes fatty acid primary amides, including oleamide, which has been isolated from the cerebrospinal fluid of sleep-deprived cats (15) and, upon injection into rats, found to induce physiological sleep (16). More recently, global metabolite profiling has been applied to tissues from FAAH(-/-) mice, revealing a third class of substrates, the N-acyl taurines (NATs, Figure 1B) (17). FAAH regulates complementary sets of NATs in the nervous system and peripheral tissues bearing long chain saturat...

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confidence: 99%

Structure-Based Design of a FAAH Variant That Discriminates between the N-Acyl Ethanolamine and Taurine Families of Signaling Lipids

McKinney

Cravatt

2006

Biochemistry

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“…Fatty acid amide hydrolase (FAAH) 1 (1)(2)(3)(4)(5) is the only identified mammalian member of a family of amidase enzymes known as the "amidase signature" family (6). Despite the presence of these enzymes in prokaryotic (6)(7)(8)(9)(10) and eukaryotic (1,(11)(12)(13) organisms, little is yet known about their catalytic mechanism and structural features.…”

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confidence: 99%

“…Despite the presence of these enzymes in prokaryotic (6)(7)(8)(9)(10) and eukaryotic (1,(11)(12)(13) organisms, little is yet known about their catalytic mechanism and structural features.…”

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confidence: 99%

Comparative Characterization of a Wild Type and Transmembrane Domain-Deleted Fatty Acid Amide Hydrolase: Identification of the Transmembrane Domain as a Site for Oligomerization

et al. 1998

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Fatty acid amide hydrolase (FAAH) is an integral membrane protein responsible for the hydrolysis of a number of primary and secondary fatty acid amides, including the neuromodulatory compounds anandamide and oleamide. Analysis of FAAH's primary sequence reveals the presence of a single predicted transmembrane domain at the extreme N-terminus of the enzyme. A mutant form of the rat FAAH protein lacking this N-terminal transmembrane domain (∆TM-FAAH) was generated and, like wild type FAAH (WT-FAAH), was found to be tightly associated with membranes when expressed in COS-7 cells. Recombinant forms of WT-and ∆TM-FAAH expressed and purified from Escherichia coli exhibited essentially identical enzymatic properties which were also similar to those of the native enzyme from rat liver. Analysis of the oligomerization states of WT-and ∆TM-FAAH by chemical cross-linking, sedimentation velocity analytical ultracentrifugation, and size exclusion chromatography indicated that both enzymes were oligomeric when membrane-bound and after solubilization. However, WT-FAAH consistently behaved as a larger oligomer than ∆TM-FAAH. Additionally, SDS-PAGE analysis of the recombinant proteins identified the presence of SDS-resistant oligomers for WT-FAAH, but not for ∆TM-FAAH. Self-association through FAAH's transmembrane domain was further demonstrated by a FAAH transmembrane domain-GST fusion protein which formed SDS-resistant dimers and large oligomeric assemblies in solution.

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“…Highly enantioselective amidases have also been observed by other investigators with various a-substituted amides (Kieny L'Homme et al, 1981;Asano et al, 1989;Mayaux et al, 1990Mayaux et al, , 1991Kakeya et al, 1991;Cohen et al, 1992). In general, these activities were found after screening of strains from culture collections or in bacteria which were initially enriched with different often aliphatic nitriles or amides.…”

Section: Discussionmentioning

confidence: 52%

“…The enzymatic hydrolysis of nitriles represents a very convenient synthetic method for amides and/or carboxylic acids due to the mild reaction conditions. Furthermore, these enzymatic reactions also allow the enantioselective synthesis of optical active amides and carboxylic acids from racemic precursors (Mayaux et al, 1990(Mayaux et al, , 1991Yamamoto et al, 1990;Kakeya et al, 1991;Bianchi et al, 1991;Bhalla et al, 1992;Cohen et al, 1992;Layh et al, 1992).…”

Section: Discussionmentioning

confidence: 99%

Enantioselective hydrolysis of racemic naproxen nitrile and naproxen amide to S-naproxen by new bacterial isolates

Layh

Stolz

Böhme

et al. 1994

Journal of Biotechnology

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Bacteria were enriched from soil samples with succinate as a carbon source and racemic naproxen nitrile [2-(6-methoxy-2-naphthyl)propionitrile] as sole source of nitrogen. Since naproxen nitrile was only poorly soluble in water media amended with different water-immiscible organic phases were used for the enrichments. With pristane (2,6,10,14-tetramethylpentadecane) as the organic phase two bacterial strains were isolated (strain C3II and strain MP50) which were identified as rhodococci. Cells of both strains converted naproxen nitrile via naproxen amide to naproxen. From racemic naproxen nitrile Rhodococcus sp. C3II formed S-naproxen amide and subsequently S-naproxen. Racemic naproxen amide was hydrolysed to S-naproxen. Rhodococcus sp. MP50 converted racemic naproxen nitrile predominantly to R-naproxen amide and racemic naproxen amide to S-naproxen. With both strains racemic naproxen amide was converted to S-naproxen with an enantiomeric excess > 99% at a conversion rate up to 80% of the theoretical value. In strain C3II the enzymes which hydrolysed naproxen nitrile and naproxen amide were present only at a low constitutive level. In contrast, in Rhodococcus sp. MP50 these activities were induced when grown in the presence of various nitriles.

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Purification, cloning, and primary structure of an enantiomer-selective amidase from Brevibacterium sp. strain R312: structural evidence for genetic coupling with nitrile hydratase

Cited by 151 publications

References 27 publications

Structure-Based Design of a FAAH Variant That Discriminates between the N-Acyl Ethanolamine and Taurine Families of Signaling Lipids

Structure-Based Design of a FAAH Variant That Discriminates between the N-Acyl Ethanolamine and Taurine Families of Signaling Lipids

Comparative Characterization of a Wild Type and Transmembrane Domain-Deleted Fatty Acid Amide Hydrolase: Identification of the Transmembrane Domain as a Site for Oligomerization

Enantioselective hydrolysis of racemic naproxen nitrile and naproxen amide to S-naproxen by new bacterial isolates

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