Acetyl-CoA synthetase: Difference between revisions

Acetate-CoA ligase
Identifiers
EC no.	6.2.1.1
CAS no.	9012-31-1
Databases
IntEnz	IntEnz view
BRENDA	BRENDA entry
ExPASy	NiceZyme view
KEGG	KEGG entry
MetaCyc	metabolic pathway
PRIAM	profile
PDB structures	RCSB PDB PDBe PDBsum
Gene Ontology	AmiGO / QuickGO
Search PMC articles PubMed articles NCBI proteins

Acetyl—CoA synthetase (ACS) or Acetate—CoA ligase is an enzyme (EC 6.2.1.1) involved in metabolism of acetate. It is in the ligase class of enzymes, meaning that it catalyzes the formation of a new chemical bond between two large molecules.

Reaction

The two molecules joined together that make up Acetyl CoA synthetase are acetate and coenzyme A (CoA). The complete reaction with all the substrates and products included is:

ATP + Acetate + CoA <=> AMP + Pyrophosphate + Acetyl-CoA ^[1]

Once acetyl-CoA is formed it can be used in the TCA cycle in aerobic respiration to produce energy and electron carriers. This is an alternate method to starting the cycle, as the more common way is producing acetyl-CoA from pyruvate through the pyruvate dehydrogenase complex. The enzyme’s activity takes place in the mitochondrial matrix so that the products are in the proper place to be used in the following metabolic steps.^[2] Acetyl Co-A can also be used in fatty acid synthesis, and a common function of the synthetase is to produce acetyl Co-A for this purpose.^[3]

The reaction catalyzed by acetyl-CoA synthetase takes place in two steps. First, AMP must be bound by the enzyme to cause a conformational change in the active site, which allows the reaction to take place. The active site is referred to as the A-cluster.^[4] A crucial lysine residue must be present in the active site to catalyze the first reaction where Co-A is bound. Co-A then rotates in the active site into the position where acetate can covalently bind to CoA. The covalent bond is formed between the sulfur atom in Co-A and the central carbon atom of acetate.^[5]

The ACS1 form of acetyl-CoA synthetase is encoded by the gene facA, which is activated by acetate and deactivated by glucose.^[6]

Structure

The three dimensional structure of the asymmetric ACS (RCSB PDB ID number: 1PG3) reveals that it is composed of two subunits. Each subunit is then composed primarily of two domains. The larger N-terminal domain is composed of 517 residues, while the smaller C-terminal domain is composed of 130 residues.^[7] Each subunit has an active site where the ligands are held. The crystallized structure of ACS was determined with CoA and Adenosine- 5′-propylphosphate bound to the enzyme. The reason for using Adenosine- 5′-propylphosphate is that it is an ATP competitive inhibitor which prevents any conformational changes to the enzyme. The adenine ring of AMP/ATP is held in a hydrophobic pocket create by residues Ile (512) and Trp (413).^[7]

The source for the crystallized structure is the organism Salmonella typhimurium (strain LT2 / SGSC1412 / ATCC 700720). The gene for ACS was then transfected into Escherichia coli BL21(DE3) for expression. During chromatography in the process to isolate the enzyme, the subunits came out individually and the total structure was determined separately.^[8] The method used to determine the structure was X-ray diffraction with a resolution of 2.3 angstroms. The unit cell values and angles are provided in the following table:

Unit Cell

Length (Å)	Angle (°)
a= 59.981	α= 90.00
b= 143.160	β= 91.57
c= 71.934	γ= 90.00

Biological Significance

The role of the ACS enzyme is to combine acetate and CoA to form acetyl CoA, however its significance is much larger. The most well known function of the product from this enzymatic reaction is the use of Acetyl-CoA in the role of the TCA cycle as well as in the production of fatty acid. Recent research has also shown that this enzyme is vital to the action of histone acetylation as well as gene regulation.^[9] The effect this acetylation has is far reaching in mammals. It has been shown that downregulation of the acs gene in the hippocampal region of mice results in lower levels of histone acetylation, but also impairs the long-term spatial memory of the animal. This result points to a link between cellular metabolism, gene regulation and cognitive function.^[9] This enzyme has shown to be an interesting biomarker for the presence of tumors in colorectal carcinomas. When the gene is present, the cells are able to take in acetate as a food source to convert it to Acetyl-CoA during stressed conditions. In the cases of advanced carcinoma tumors, the genes for this enzyme were down regulated and indicated a poor 5-year survival rate.^[10] Expression of the enzyme has also been linked to the development of metastatic tumor nodes, leading to a poor survival rate in patients with renal cell carcinomas.^[11]

Regulation

The activity of the enzyme is controlled in several ways. The essential lysine residue in the active site plays an important role in regulation of activity. The lysine molecule can be deacetylated by another class of enzyme called sirtuins. In mammals, the cytoplasmic-nuclear synthetase (AceCS1) is activated by SIRT1 while the mitochondrial synthetase (AceCS2) is activated by SIRT3. This action increases activity of this enzyme.^[12] The exact location of the lysine residue varies between species, occurring at Lys-642 in humans, but is always present in the active site of the enzyme.^[13] Since there is an essential allosteric change that occurs with the binding of an AMP molecule, the presence of AMP can contribute to regulation of the enzyme. Concentration of AMP must be high enough so that it can bind in the allosteric binding site and allow the other substrates to enter the active site. Also, copper ions deactivate acetyl Co-A synthetase by occupying the proximal site of the A-cluster active site, which prevents the enzyme from accepting a methyl group to participate in the Wood-Ljungdahl Pathway.^[4] The presence of all the reactants in the proper concentration is also needed for proper functioning as in all enzymes. Acetyl—CoA synthetase is also produced when it is needed for fatty acid synthesis, but, under normal conditions, the gene is inactive and has certain transcriptional factors that activate transcription when necessary.^[3] In addition to sirtuins, protein deacetylase (AcuC) also can modify acetyl—CoA synthetase at a lysine residue. However, unlike sirtuins, AcuC does not require NAD+ as a cosubstrate.^[14]

Role in gene expression

While acetyl-CoA synthetase’s activity is usually associated with metabolic pathways, the enzyme also participates in gene expression. In yeast, acetyl-CoA synthetase delivers acetyl-CoA to histone acetyltransferases for histone acetylation. Without correct acetylation, DNA cannot condense into chromatin properly, which inevitably results in transcriptional errors.^[15]

Industrial Usage

References

1. KEGG
2. Schwer B, Bunkenborg J, Verdin RO, Andersen JS, Verdin E (July 2006). "Reversible lysine acetylation controls the activity of the mitochondrial enzyme acetyl-CoA synthetase 2". Proceedings of the National Academy of Sciences of the United States of America. 103 (27): 10224–9. doi:10.1073/pnas.0603968103. PMC 1502439. PMID 16788062.
3. Ikeda Y, Yamamoto J, Okamura M, Fujino T, Takahashi S, Takeuchi K, Osborne TF, Yamamoto TT, Ito S, Sakai J (September 2001). "Transcriptional regulation of the murine acetyl-CoA synthetase 1 gene through multiple clustered binding sites for sterol regulatory element-binding proteins and a single neighboring site for Sp1". The Journal of Biological Chemistry. 276 (36): 34259–69. doi:10.1074/jbc.M103848200. PMID 11435428.
4. Bramlett MR, Tan X, Lindahl PA (August 2003). "Inactivation of acetyl-CoA synthase/carbon monoxide dehydrogenase by copper". Journal of the American Chemical Society. 125 (31): 9316–7. doi:10.1021/ja0352855. PMID 12889960.
5. Jogl G, Tong L (February 2004). "Crystal structure of yeast acetyl-coenzyme A synthetase in complex with AMP". Biochemistry. 43 (6): 1425–31. doi:10.1021/bi035911a. PMID 14769018.
6. De Cima S, Rúa J, Perdiguero E, del Valle P, Busto F, Baroja-Mazo A, de Arriaga D (Apr 7, 2005). "An acetyl-CoA synthetase not encoded by the facA gene is expressed under carbon starvation in Phycomyces blakesleeanus". Research in Microbiology. 156 (5–6): 663–9. doi:10.1016/j.resmic.2005.03.003. PMID 15921892.
7. Gulick, Andrew M.; Starai, Vincent J.; Horswill, Alexander R.; Homick, Kristen M.; Escalante-Semerena, Jorge C. "The 1.75 Å Crystal Structure of Acetyl-CoA Synthetase Bound to Adenosine-5'-propylphosphate and Coenzyme A†". Biochemistry. 42 (10): 2866–2873. doi:10.1021/bi0271603.
8. Gulick, A.M.; Starai, V.J.; Horswill, A.R.; Homick, K.M.; Escalante-Semerena, J.C. (2003). "Acetyl CoA Synthetase, Acetylated on Lys609". Biochemistry. 42. doi:10.2210/pdb1pg3/pdb.
9. Mews, Philipp; Donahue, Greg; Drake, Adam M.; Luczak, Vincent; Abel, Ted; Berger, Shelley L. (2017/06). "Acetyl-CoA synthetase regulates histone acetylation and hippocampal memory". Nature. 546 (7658): 381–386. doi:10.1038/nature22405. ISSN 1476-4687. {{cite journal}}: Check date values in: |date= (help)
10. Bae, Jeong Mo; Kim, Jung Ho; Oh, Hyeon Jeong; Park, Hye Eun; Lee, Tae Hun; Cho, Nam-Yun; Kang, Gyeong Hoon (2017/02). "Downregulation of acetyl-CoA synthetase 2 is a metabolic hallmark of tumor progression and aggressiveness in colorectal carcinoma". Modern Pathology. 30 (2): 267–277. doi:10.1038/modpathol.2016.172. ISSN 1530-0285. {{cite journal}}: Check date values in: |date= (help)
11. Zhang, Shaojin; He, Juanjuan; Jia, Zhankui; Yan, Zechen; Yang, Jinjian. "Acetyl-CoA synthetase 2 enhances tumorigenesis and is indicative of a poor prognosis for patients with renal cell carcinoma". Urologic Oncology: Seminars and Original Investigations. doi:10.1016/j.urolonc.2018.01.013.
12. Schwer B, Bunkenborg J, Verdin RO, Andersen JS, Verdin E (July 2006). "Reversible lysine acetylation controls the activity of the mitochondrial enzyme acetyl-CoA synthetase 2". Proceedings of the National Academy of Sciences of the United States of America. 103 (27): 10224–9. doi:10.1073/pnas.0603968103. PMC 1502439. PMID 16788062.
13. Hallows WC, Lee S, Denu JM (July 2006). "Sirtuins deacetylate and activate mammalian acetyl-CoA synthetases". Proceedings of the National Academy of Sciences of the United States of America. 103 (27): 10230–5. doi:10.1073/pnas.0604392103. PMC 1480596. PMID 16790548.
14. Gardner JG, Grundy FJ, Henkin TM, Escalante-Semerena JC (August 2006). "Control of acetyl-coenzyme A synthetase (AcsA) activity by acetylation/deacetylation without NAD(+) involvement in Bacillus subtilis". Journal of Bacteriology. 188 (15): 5460–8. doi:10.1128/JB.00215-06. PMC 1540023. PMID 16855235.
15. Takahashi H, McCaffery JM, Irizarry RA, Boeke JD (July 2006). "Nucleocytosolic acetyl-coenzyme a synthetase is required for histone acetylation and global transcription". Molecular Cell. 23 (2): 207–17. doi:10.1016/j.molcel.2006.05.040. PMID 16857587.