Coenzyme A

Template:Short description Template:Chembox Coenzyme A (CoA, SHCoA, CoASH) is a coenzyme, notable for its role in the synthesis and oxidation of fatty acids, and the oxidation of pyruvate in the citric acid cycle. All genomes sequenced to date encode enzymes that use coenzyme A as a substrate, and around 4% of cellular enzymes use it (or a thioester) as a substrate. In humans, CoA biosynthesis requires cysteine, pantothenate (vitamin B₅), and adenosine triphosphate (ATP).<ref>Template:Cite journal</ref>

In its acetyl form, coenzyme A is a highly versatile molecule, serving metabolic functions in both the anabolic and catabolic pathways. Acetyl-CoA is utilised in the post-translational regulation and allosteric regulation of pyruvate dehydrogenase and carboxylase to maintain and support the partition of pyruvate synthesis and degradation.<ref>{{#invoke:citation/CS1|citation |CitationClass=web }}</ref>

Discovery of structureEdit

Coenzyme A was identified by Fritz Lipmann in 1946,<ref>Template:Cite journal</ref> who also later gave it its name. Its structure was determined during the early 1950s at the Lister Institute, London, together by Lipmann and other workers at Harvard Medical School and Massachusetts General Hospital.<ref name="Nature">Template:Cite journal</ref> Lipmann initially intended to study acetyl transfer in animals, and from these experiments he noticed a unique factor that was not present in enzyme extracts but was evident in all organs of the animals. He was able to isolate and purify the factor from pig liver and discovered that its function was related to a coenzyme that was active in choline acetylation.<ref name=":0">Template:Cite journal</ref> Work with Beverly Guirard, Nathan Kaplan, and others determined that pantothenic acid was a central component of coenzyme A.<ref>Template:Cite journal</ref><ref>Template:Cite journal</ref> The coenzyme was named coenzyme A to stand for "activation of acetate". In 1953, Fritz Lipmann won the Nobel Prize in Physiology or Medicine "for his discovery of co-enzyme A and its importance for intermediary metabolism".<ref name=":0" /><ref>{{#invoke:citation/CS1|citation |CitationClass=web }}</ref>

BiosynthesisEdit

Coenzyme A is naturally synthesized from pantothenate (vitamin B₅), which is found in food such as meat, vegetables, cereal grains, legumes, eggs, and milk.<ref>{{#invoke:citation/CS1|citation |CitationClass=web }}</ref> In humans and most living organisms, pantothenate is an essential vitamin that has a variety of functions.<ref>{{#invoke:citation/CS1|citation |CitationClass=web }}</ref> In some plants and bacteria, including Escherichia coli, pantothenate can be synthesised de novo and is therefore not considered essential. These bacteria synthesize pantothenate from the amino acid aspartate and a metabolite in valine biosynthesis.<ref name=":3">Template:Cite journal</ref>

In all living organisms, coenzyme A is synthesized in a five-step process that requires four molecules of ATP, pantothenate and cysteine<ref name=":4">Template:Cite journal</ref> (see figure):

1. Pantothenate (vitamin B₅) is phosphorylated to 4′-phosphopantothenate by the enzyme pantothenate kinase (PanK; CoaA; CoaX). This is the committed step in CoA biosynthesis and requires ATP.<ref name=":3" />
2. A cysteine is added to 4′-phosphopantothenate by the enzyme phosphopantothenoylcysteine synthetase (PPCS; CoaB) to form 4'-phospho-N-pantothenoylcysteine (PPC). This step is coupled with ATP hydrolysis.<ref name=":3" />
3. PPC is decarboxylated to 4′-phosphopantetheine by phosphopantothenoylcysteine decarboxylase (PPC-DC; CoaC)
4. 4′-phosphopantetheine is adenylated (or more properly, AMPylated) to form dephospho-CoA by the enzyme phosphopantetheine adenylyl transferase (COASY; PPAT; CoaD)
5. Finally, dephospho-CoA is phosphorylated to coenzyme A by the enzyme dephosphocoenzyme A kinase (COASY, DPCK; CoaE). This final step requires ATP.<ref name=":3" />

Enzyme nomenclature abbreviations in parentheses represent mammalian, other eukaryotic, and prokaryotic enzymes respectively. In mammals steps 4 and 5 are catalyzed by a bifunctional enzyme called COASY.<ref name="Evers">Template:Cite journal</ref> This pathway is regulated by product inhibition. CoA is a competitive inhibitor for Pantothenate Kinase, which normally binds ATP.<ref name=":3" /> Coenzyme A, three ADP, one monophosphate, and one diphosphate are harvested from biosynthesis.<ref name=":4" />

Coenzyme A can be synthesized through alternate routes when intracellular coenzyme A level are reduced and the de novo pathway is impaired.<ref>Template:Cite journal</ref> In these pathways, coenzyme A needs to be provided from an external source, such as food, in order to produce 4′-phosphopantetheine. Ectonucleotide pyrophosphates (ENPP) degrade coenzyme A to 4′-phosphopantetheine, a stable molecule in organisms. Acyl carrier proteins (ACP) (such as ACP synthase and ACP degradation) are also used to produce 4′-phosphopantetheine. This pathway allows for 4′-phosphopantetheine to be replenished in the cell and allows for the conversion to coenzyme A through enzymes, PPAT and PPCK.<ref>Template:Cite journal</ref>

A 2024 article<ref>Template:Cite journal</ref> detailed a plausible chemical synthesis mechanism for the pantetheine component (the main functional part) of coenzyme A in a primordial prebiotic world.

Commercial productionEdit

Coenzyme A is produced commercially via extraction from yeast, however this is an inefficient process (yields approximately 25 mg/kg) resulting in an expensive product. Various ways of producing CoA synthetically, or semi-synthetically have been investigated, although none are currently operating at an industrial scale.<ref>Template:Cite journal</ref>

FunctionEdit

Fatty acid synthesisEdit

Since coenzyme A is, in chemical terms, a thiol, it can react with carboxylic acids to form thioesters, thus functioning as an acyl group carrier. It assists in transferring fatty acids from the cytoplasm to mitochondria. A molecule of coenzyme A carrying an acyl group is also referred to as acyl-CoA. When it is not attached to an acyl group, it is usually referred to as 'CoASH' or 'HSCoA'. This process facilitates the production of fatty acids in cells, which are essential in cell membrane structure.

Coenzyme A is also the source of the phosphopantetheine group that is added as a prosthetic group to proteins such as acyl carrier protein and formyltetrahydrofolate dehydrogenase.<ref>Template:Cite journal</ref><ref>Template:Cite journal</ref>

Energy productionEdit

Coenzyme A is one of five crucial coenzymes that are necessary in the reaction mechanism of the citric acid cycle. Its acetyl-coenzyme A form is the primary input in the citric acid cycle and is obtained from glycolysis, amino acid metabolism, and fatty acid beta oxidation. This process is the body's primary catabolic pathway and is essential in breaking down the building blocks of the cell such as carbohydrates, amino acids, and lipids.<ref>Template:Cite book</ref>

RegulationEdit

When there is excess glucose, coenzyme A is used in the cytosol for synthesis of fatty acids.<ref name=":2">Template:Cite journal</ref> This process is implemented by regulation of acetyl-CoA carboxylase, which catalyzes the committed step in fatty acid synthesis. Insulin stimulates acetyl-CoA carboxylase, while epinephrine and glucagon inhibit its activity.<ref>Template:Cite book</ref>

During cell starvation, coenzyme A is synthesized and transports fatty acids in the cytosol to the mitochondria. Here, acetyl-CoA is generated for oxidation and energy production.<ref name=":2" /> In the citric acid cycle, coenzyme A works as an allosteric regulator in the stimulation of the enzyme pyruvate dehydrogenase.

Antioxidant function and regulationEdit

Discovery of the novel antioxidant function of coenzyme A highlights its protective role during cellular stress. Mammalian and bacterial cells subjected to oxidative and metabolic stress show significant increase in the covalent modification of protein cysteine residues by coenzyme A.<ref>Template:Cite journal</ref><ref name="Tsuchiya 1909–1937">Template:Cite journal</ref> This reversible modification is termed protein CoAlation (Protein-S-SCoA), which plays a similar role to protein S-glutathionylation by preventing the irreversible oxidation of the thiol group of cysteine residues.

Using anti-coenzyme A antibody<ref>Template:Cite journal</ref> and liquid chromatography tandem mass spectrometry (LC-MS/MS) methodologies, more than 2,000 CoAlated proteins were identified from stressed mammalian and bacterial cells.<ref name=":1">Template:Cite journal</ref> The majority of these proteins are involved in cellular metabolism and stress response.<ref name=":1" /> Different research studies have focused on deciphering the coenzyme A-mediated regulation of proteins. Upon protein CoAlation, inhibition of the catalytic activity of different proteins (e.g., metastasis suppressor NME1, peroxiredoxin 5, GAPDH, among others) is reported.<ref>Template:Cite journal</ref><ref>Template:Cite journal</ref><ref name="Tsuchiya 1909–1937"/><ref>Template:Cite journal</ref> To restore the protein's activity, antioxidant enzymes that reduce the disulfide bond between coenzyme A and the protein cysteine residue play an important role. This process is termed protein deCoAlation. Thioredoxin A and Thioredoxin-like protein (YtpP), two bacterial proteins, are shown to deCoAlate proteins.<ref>Template:Cite journal</ref>

Use in biological researchEdit

Coenzyme A is available from various chemical suppliers as the free acid and lithium or sodium salts. The free acid of coenzyme A is detectably unstable, with around 5% degradation observed after 6 months when stored at −20 °C,<ref name="Dawson_2002" /> and near complete degradation after 1 month at 37 °C.<ref>{{#invoke:citation/CS1|citation |CitationClass=web }}</ref> The lithium and sodium salts of CoA are more stable, with negligible degradation noted over several months at various temperatures.<ref>{{#invoke:citation/CS1|citation |CitationClass=web }}</ref> Aqueous solutions of coenzyme A are unstable above pH 8, with 31% of activity lost after 24 hours at 25 °C and pH 8. CoA stock solutions are relatively stable when frozen at pH 2–6. The major route of CoA activity loss is likely the air oxidation of CoA to CoA disulfides. CoA mixed disulfides, such as CoA-S–S-glutathione, are commonly noted contaminants in commercial preparations of CoA.<ref name="Dawson_2002" /> Free CoA can be regenerated from CoA disulfide and mixed CoA disulfides with reducing agents such as dithiothreitol or 2-mercaptoethanol.

Non-exhaustive list of coenzyme A-activated acyl groupsEdit

Template:Category see also

• Acetyl-CoA
• fatty acyl-CoA (activated form of all fatty acids; only the CoA esters are substrates for important reactions such as mono-, di-, and triacylglycerol synthesis, carnitine palmitoyl transferase, and cholesterol esterification)
  • Propionyl-CoA
  • Butyryl-CoA
  • Myristoyl-CoA
  • Crotonyl-CoA
• Acetoacetyl-CoA
• Coumaroyl-CoA (used in flavonoid and stilbenoid biosynthesis)
• Benzoyl-CoA
• Phenylacetyl-CoA
• Acyl derived from dicarboxylic acids
  • Malonyl-CoA (important in chain elongation in fatty acid biosynthesis and polyketide biosynthesis)
  • Succinyl-CoA (used in heme biosynthesis)
  • Hydroxymethylglutaryl-CoA (used in isoprenoid biosynthesis)
  • Pimelyl-CoA (used in biotin biosynthesis)

ReferencesEdit

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BibliographyEdit

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