Mitochondrial hotdog-fold thioesterase

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Revision as of 19:06, 26 May 2024

Overview of thioesterases

Thioesterases are enzymes that catalyze the hydrolysis of thioester bonds, which are the linkage between a carbonyl and a sulfur atom. The ATP-dependent formation of a thioester bond from a carboxylate and a thiol in biomolecules makes them more reactive and is particularly an important commitment step in lipid metabolism. Therefore, thioesterases counteract this activation by releasing upon hydrolysis a molecule with the more stable carboxylate group. For this reason, thioesterases are found at the end of some metabolic pathways but they also may act as regulators of flux.

There are two main families of thioesterases which are distinguished by their folding, named the α/β-hydrolases and the hotdog-fold hydrolases. Notably, these two different families are evolutionarily distant, so the thioesterase activity is a shared feature owing to convergent evolution.

Structure and active site

Thioesterase superfamily members4 (Them4) and 5 (Them5) are proteins found in human mitochondria. These proteins' name come from the single hotdog-fold thioesterase domain in their tertiary structure. The hotdog fold is characterized by a curved antiparallel beta sheet around a long alpha helix. In the case of Them5, this domain encompasses residues 125 to 237. The core beta sheet in Them5 is six-stranded

To analyze these proteins, we shall use the atomic structure of the human Them4 complexed with undecan-2-one-CoA, which is a structural analog of acyl-CoA's and inhibitor of this protein.

It is notable that Them4 and Them5 possess a conserved HGG…D…T motif within the hotdog fold. In Them4, the catalytic residues are Asp161 and Thr177, which interact through a hydrogen bond between the carboxylate in aspartate and the hydroxyl in threonine. For Them5, the catalytic residues are Asp167 and Thr183.

In the proposed catalytic mechanism, the threonine residue induces the polarization of the carbonyl in the thioester bond. Meanwhile, the deprotonated aspartate residue abstracts a proton from a water molecule, making it very reactive and prone to a nucleophilic attack on the thioester bond.

As observed in other single hotdog-fold thioesterases, the biological assembly of Them4 and Them5 is a homodimer with a 2-fold symmetry axis. In this quaternary structure, for Them4 the catalytic residues from one monomer are in proximity to His152, Gly153 and Gly154 from the other monomer, which are proposed to accommodate the thioester substrate within the active site. For Them5, Asp167 and Thr183 from one monomer are close to His158, Gly159 and Gly160 from the other monomer.

As a direct consequence, in each catalytically competent Them4 and Them5 there are two active sites located in the interface between monomers of the obligatory homodimer.

Besides the core hotdog-fold, in both Them4 and Them5 there is another alpha helix in each monomer. This element of secondary structure is tightly attached to the convex side of the curved beta sheet owing to the hydrophobic effect. More specifically, it is an amphiphilic alpha helix whose apolar residues are spatially collapsed over apolar residues in strands 1 and 2 of the core beta sheet. For Them4, this alpha helix is formed by residues 55 to 68, while for Them5 the respective residues are 64 to 79.

Interestingly, at each of the flanking regions of the additional alpha helix, there is a pi-stacking interaction that also contributes to maintaining the local fold. Trp62 and Tyr70 make this interaction at the N-terminal side of the alpha helix while Phe73 and Trp82 are the analogues at the C-terminal side.

Function

From enzymatic activities in vitro, it was shown that Them4 (Zhao et al., 2009) and Them5 (Zhuravleva et al., 2012) have higher kcat/KM for acyl-CoA's with medium and long hydrocarbon chain, such as myristoyl-CoA (14:0), palmitoyl-CoA (16:0), oleoyl-CoA (18:1) and linoleoyl-CoA (18:2). According to Zhuravleva et al. (2012), linoleoyl-CoA (18:2) was a preferred substrate for Them5. From studies with Them5−/− mice, it was identified by mass spectrometry (MS) that loss of Them5 is related to an increase in the levels of monolysocardiolipin (MLCL), which is a metabolite upstream of the cardiolipin remodeling process in mitochondria. Furthermore, the lipidomics analysis by MS for Them5−/− mice also revealed a 2-fold decrease of free fatty acids, notably linoleic (18:2) and linolenic (18:3) acids. This is consistent with the in vitro assay for the recombinant ∆34Them5 which revealed higher kcat/KM for linoleoyl-CoA (18:2). Moreover, it is observed by two-dimensional electron microscopy (2D-EM) and subsequent 3D reconstruction that in hepatocytes from Them5−/− mice, mitochondria were more elongated and interconnected, with a 2-fold increase in volume. With these data, Zhuravleva et al. (2012) propose that Them5 might be a regulator of cardiolipin remodeling through modulation of the unsaturated acyl-CoA pool in mitochondria. This modulation in turn seems to affect mitochondrial morphology.

Them4 is also called Akt C-Terminal Modulator Protein (CTMP), owing to previous data suggesting that it interacts with the serine-threonine protein kinase Akt1 in an inferred mechanism of regulating apoptosis. However, this putative activity is not well defined yet.

References

Zhao, H., Martin, B. M., Bisoffi, M., & Dunaway-Mariano, D. (2009). The Akt C-terminal modulator protein is an acyl-CoA thioesterase of the Hotdog-Fold family. Biochemistry, 48(24), 5507-5509. https://doi.org/10.1021/bi900710w

Zhao, H., Lim, K., Choudry, A., Latham, J. A., Pathak, M. C., Dominguez, D., ... & Dunaway-Mariano, D. (2012). Correlation of structure and function in the human hotdog-fold enzyme hTHEM4. Biochemistry, 51(33), 6490-6492. https://doi.org/10.1021/bi300968n

Zhuravleva, E., Gut, H., Hynx, D., Marcellin, D., Bleck, C. K., Genoud, C., ... & Hemmings, B. A. (2012). Acyl coenzyme A thioesterase Them5/Acot15 is involved in cardiolipin remodeling and fatty liver development. Molecular and cellular biology, 32(14), 2685-2697. https://doi.org/10.1128/MCB.00312-12

Proteopedia Page Contributors and Editors (what is this?)

Marcelo Mesa, Thabata Fernanda Oliveira, Eduardo Ferraro, Michal Harel

Retrieved from "http://52.214.119.220/wiki/index.php/Mitochondrial_hotdog-fold_thioesterase"

@@ Line 14: / Line 14: @@
 Thioesterase superfamily members4 (Them4) and 5 (Them5) are proteins found in human [https://en.wikipedia.org/wiki/Mitochondrion mitochondria]. These proteins' name come from the '''single hotdog-fold thioesterase''' domain in their tertiary structure.
 The hotdog fold is characterized by a curved antiparallel [[beta sheet]] around a long [[alpha helix]]. In the case of Them5, this domain encompasses residues 125 to 237. The core beta sheet in Them5 is six-stranded
+To analyze these proteins, we shall use the atomic structure of the human Them4 complexed with undecan-2-one-CoA, which is a structural analog of acyl-CoA's and inhibitor of this protein.
 It is notable that Them4 and Them5 possess a conserved HGG…D…T motif within the hotdog fold. In Them4, the catalytic residues are Asp161 and Thr177, which interact through a [[hydrogen bond]] between the carboxylate in aspartate and the [https://en.wikipedia.org/wiki/Hydroxy_group hydroxyl] in threonine. For Them5, the catalytic residues are Asp167 and Thr183.
 In the proposed [https://en.wikipedia.org/wiki/Enzyme_catalysis catalytic mechanism], the threonine residue induces the [https://en.wikipedia.org/wiki/Dielectric#Dielectric_polarisation polarization] of the carbonyl in the thioester bond. Meanwhile, the deprotonated aspartate residue abstracts a proton from a water molecule, making it very '''reactive''' and prone to a [https://en.wikipedia.org/wiki/Nucleophile nucleophilic attack] on the thioester bond.
 As observed in other single hotdog-fold thioesterases, the [[biological assembly]] of Them4 and Them5 is a [https://en.wikipedia.org/wiki/Protein_dimer homodimer] with a 2-fold symmetry axis. In this quaternary structure, for Them4 the catalytic residues from one monomer are in proximity to His152, Gly153 and Gly154 from the other monomer, which are proposed to accommodate the thioester substrate within the active site. For Them5, Asp167 and Thr183 from one monomer are close to His158, Gly159 and Gly160 from the other monomer.
@@ Line 27: / Line 28: @@
 == Function ==
-From enzymatic activities ''in vitro'', it was shown that a recombinant ∆34Them5 with preserved catalytic residues is capable of hydrolyzing the thioester bond of acyl-CoA's. Interestingly, it shows higher ''k''cat/KM for acyl-CoA's with medium and long hydrocarbon chain, such as myristoyl-CoA (14:0), palmitoyl-CoA (16:0), oleoyl-CoA (18:1) and linoleoyl-CoA (18:2). From the long chain acyl-CoA's tested, '''linoleoyl-CoA''' (18:2) was a preferred substrate.
+From enzymatic activities ''in vitro'', it was shown that Them4 (Zhao ''et al.'', 2009) and Them5  (Zhuravleva ''et al.'', 2012) have higher ''k''cat/KM for acyl-CoA's with medium and long hydrocarbon chain, such as myristoyl-CoA (14:0), palmitoyl-CoA (16:0), oleoyl-CoA (18:1) and linoleoyl-CoA (18:2). According to Zhuravleva ''et al.'' (2012), '''linoleoyl-CoA''' (18:2) was a preferred substrate for Them5.
 From studies with Them5−/− mice, it was identified by [https://en.wikipedia.org/wiki/Mass_spectrometry mass spectrometry] (MS) that loss of Them5 is related to an increase in the levels of monolysocardiolipin (MLCL), which is a metabolite upstream of the [https://en.wikipedia.org/wiki/Cardiolipin cardiolipin] remodeling process in mitochondria.
 Furthermore, the [https://en.wikipedia.org/wiki/Lipidomics lipidomics] analysis by MS for Them5−/− mice also revealed a 2-fold decrease of free fatty acids, notably linoleic (18:2) and linolenic (18:3) acids. This is consistent with the ''in vitro'' assay for the recombinant ∆34Them5 which revealed higher ''k''cat/KM for linoleoyl-CoA (18:2).
 Moreover, it is observed by [https://en.wikipedia.org/wiki/Transmission_electron_microscopy two-dimensional electron microscopy] (2D-EM) and subsequent 3D reconstruction that in [https://en.wikipedia.org/wiki/Hepatocyte hepatocytes] from Them5−/− mice, mitochondria were more elongated and interconnected, with a 2-fold increase in volume.
-With these data, Zhuravleva ''et al.'' propose that '''Them5 might be a regulator of cardiolipin remodeling''' through modulation of the unsaturated acyl-CoA pool in mitochondria. This modulation in turn seems to affect mitochondrial morphology.
+With these data, Zhuravleva ''et al.'' (2012) propose that '''Them5 might be a regulator of cardiolipin remodeling''' through modulation of the unsaturated acyl-CoA pool in mitochondria. This modulation in turn seems to affect mitochondrial morphology.
-== Disease ==
+Them4 is also called Akt C-Terminal Modulator Protein (CTMP), owing to previous data suggesting that it interacts with the serine-threonine protein kinase Akt1 in an inferred mechanism of regulating apoptosis. However, this putative activity is not well defined yet.
 </StructureSection>
 == References ==
+Zhao, H., Martin, B. M., Bisoffi, M., & Dunaway-Mariano, D. (2009). The Akt C-terminal modulator protein is an acyl-CoA thioesterase of the Hotdog-Fold family. Biochemistry, 48(24), 5507-5509.
+https://doi.org/10.1021/bi900710w
+Zhao, H., Lim, K., Choudry, A., Latham, J. A., Pathak, M. C., Dominguez, D., ... & Dunaway-Mariano, D. (2012). Correlation of structure and function in the human hotdog-fold enzyme hTHEM4. Biochemistry, 51(33), 6490-6492.
+https://doi.org/10.1021/bi300968n
 Zhuravleva, E., Gut, H., Hynx, D., Marcellin, D., Bleck, C. K., Genoud, C., ... & Hemmings, B. A. (2012). Acyl coenzyme A thioesterase Them5/Acot15 is involved in cardiolipin remodeling and fatty liver development. Molecular and cellular biology, 32(14), 2685-2697.
 https://doi.org/10.1128/MCB.00312-12

Mitochondrial hotdog-fold thioesterase

From Proteopedia

Revision as of 19:06, 26 May 2024

Overview of thioesterases

Structure and active site

Function

References

Proteopedia Page Contributors and Editors (what is this?)

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