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5-aminolevulinate synthase
5-aminolevulinate synthase
	Aminolevulinic acid synthase dimer, Rhodobacter capsulatus
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EC no.	2.3.1.37
CAS no.	9037-14-3
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Aminolevulinic acid synthase (ALA synthase, ALAS, or delta-aminolevulinic acid synthase) is an enzyme (EC 2.3.1.37) that catalyzes the synthesis of δ-aminolevulinic acid (ALA) the first common precursor in the biosynthesis of all tetrapyrroles such as hemes, cobalamins and chlorophylls.^[1] The reaction is as follows:

succinyl-CoA + glycine

\rightleftharpoons

δ-aminolevulinic acid + CoA + CO₂

This enzyme is expressed in all non-plant eukaryotes and the α-class of proteobacteria and the reaction it catalyses is sometimes referred to as the Shemin pathway for ALA formation.^[2] Other organisms produce ALA through a three enzyme pathway known as the C5 pathway. ALA is synthesized through the condensation of glycine and succinyl-CoA. In humans, transcription of ALA synthase is tightly controlled by the presence of Fe²⁺-binding elements, to prevent accumulation of porphyrin intermediates in the absence of iron. There are two forms of ALA synthase in the body. One form is expressed in red blood cell precursor cells (ALAS2), whereas the other (ALAS1) is ubiquitously expressed throughout the body. The red blood cell form is coded by a gene on chromosome X, whereas the other form is coded by a gene on chromosome 3.

The disease X-linked sideroblastic anemia is caused by mutations in the ALA synthase gene on chromosome X, whereas no diseases are known to be caused by mutations in the other gene. Gain of function mutations in the erythroid specific ALA synthase gene have been shown recently to cause a previously unknown form of porphyria known as X-linked-dominant protoporphyria.

Enzyme structure and properties[edit]

PLP-dependent enzymes are prevalent because they are needed to transform amino acids into other resources.^[1] ALAS is a homodimer with similarly sized sub units and the active sites consisting of amino acid side chains such as arginine, threonine, and lysine exist at a subunity interface.^[1] The protein when extracted from R. spheroids contains 1600-folds and weighs about 80,000 daltons.^[3] Enzymatic activity varies for different sources of the enzyme.^[3]

Reaction mechanism[edit]

The active sites of ALAS utilize three key amino acid side chains: Arg-85 and Thr-430 and Lys-313. Although these three amino acids have been identified to allow this reaction to proceed, they would be inactive without the addition of cofactor pyridoxal 5’-phosphate (PLP) whose role in this synthesis is detailed in the image below. Before the reaction can begin, the PLP cofactor binds to the lysine side chain to form a Schiff base that promotes attack by glycine substrate.^[4]^[5]^[6]^[7] Lysine acts as a general base during this mechanism,.^[1]^[8] In the detailed reaction mechanism, the hydronium atoms that are added in come from a variety of residues that offer hydrogen bonds to facilitate ALA synthesis.^[1] ALA synthase removes the carboxyl group from glycine and the CoA from the succinyl-CoA by means of its prosthetic group pyridoxal phosphate (a vitamin b6 derivative), forming δ-aminolevulinic acid (dALA), so called because the amino group is on the fourth carbon atom in the molecule. This reaction mechanism is particularly unique relative to other enzymes that use the PLP cofactor because Glycine is initially deprotonated by a highly conserved active site lysine, leading to condensation with succinyl-CoA and loss of CoA. Protonation of the carbonyl group of the intermediate by an active site histidine leads to loss of the carboxyl group. The last intermediate is finally reprotonated to produce ALA. Dissociation of ALA from the enzyme is the rate limiting step of the enzymatic reaction and was shown to be depended upon a slow conformational change of the enzyme. The function of pyridoxal phosphate is to facilitate the removal of hydrogen, by utilizing the electrophilic pyridinium ring as an electron sink.

The location of this enzyme in biological systems is indicative of the feedback that it may receive. ALA Synthase has been found in bacteria, yeast, avian and mammalian liver and blood cells and bone marrow. The location of this enzyme in animal cells is within the mitochondria.^[3] Since the enzyme appears to be located near its source of succinyl-CoA and the end of the heme pathway indicates that the starting and end points of heme biosynthesis serves as feedback for ALA synthase.^[3] ALA synthase is also inhibited by hemin and glucose.^[9]

Biological function[edit]

ALAS1 and ALAS2 catalyze the first step in the process of heme synthesis. It is the first irreversible step and is also rate limiting. This means that the beginning of the formation of hemes is very intentional and subject to a variety of areas of feedback. For example, the two substrates, oxaloacetate and glycine, are highly produced by and utilized in other essential biological processes such as glycolysis and the TCA cycle. The image below illustrates the heme synthesis pathway and the role ALAS plays.

Heme synthesis—note that some reactions occur in the cytoplasm and some in the mitochondrion (yellow)

Disease relevance[edit]

Aminolevulinic Acid Synthase Deficiency results in a lack of ability to create heme since its job is to catalyze the first step in the process. These deficiencies are often a result of genetic mutation that can result in a variety of diseases. One such disease is x-linked sideroblastic anemia which results in the appearance of red blood cells in the bone marrow.^[10] This disease is linked specifically with mutations in the genes that encode for ALAS2.^[10]

References[edit]

^ ^a ^b ^c ^d ^e Hunter, Gregory A.; Ferreira, Gloria C. (November 2011). "Molecular enzymology of 5-Aminolevulinate synthase, the gatekeeper of heme biosynthesis". Biochimica et Biophysica Acta (BBA) - Proteins and Proteomics. 1814 (11): 1467–1473. doi:10.1016/j.bbapap.2010.12.015. PMC 3090494. PMID 21215825.
^ Shemin, David; Rittenberg, D (June 18, 1945). "The utilization of glycine for the synthesis of a porphyrin". Journal of Biological Chemistry. 159: 567–568.
^ ^a ^b ^c ^d Beale, S I (June 1978). "δ-Aminolevulinic Acid in Plants: Its Biosynthesis, Regulation, and Role in Plastid Development". Annual Review of Plant Physiology. 29 (1): 95–120. doi:10.1146/annurev.pp.29.060178.000523.
^ "ALA synthase". flipper e nuvola. Turin University. Retrieved 10 March 2016.
^ Shoolingin-Jordan, Peter M.; Al-Daihan, Sooad; Alexeev, Dmitriy; Baxter, Robert L.; Bottomley, Sylvia S.; Kahari, I.Donald; Roy, Ipsita; Sarwar, Muhammad; Sawyer, Lindsay; Wang, Shu-Fen (Apr 2003). "5-Aminolevulinic acid synthase: mechanism, mutations and medicine". Biochim Biophys Acta. 1647 (1–2): 361–6. doi:10.1016/s1570-9639(03)00095-5. PMID 12686158.
^ CHOI, H (July 2004). "Cloning, expression, and characterization of 5-aminolevulinic acid synthase from Rhodopseudomonas palustris KUGB306". FEMS Microbiology Letters. 236 (2): 175–181. doi:10.1016/j.femsle.2004.05.048. PMID 15251194.
^ Ferreira, Gloria C.; Neame, Peter J.; Dailey, Harry A. (November 1993). "Heme biosynthesis in mammalian systems: Evidence of a schiff base linkage between the pyridoxal 5′-phosphate cofactor and a lysine residue in 5-aminolevulinate synthase". Protein Science. 2 (11): 1959–1965. doi:10.1002/pro.5560021117. PMC 2142290. PMID 8268805.
^ Hunter, Gregory A.; Ferreira, Gloria C. (March 1999). "Lysine-313 of 5-Aminolevulinate Synthase Acts as a General Base during Formation of the Quinonoid Reaction Intermediates". Biochemistry. 38 (12): 3711–3718. doi:10.1021/bi982390w. PMID 10090759.
^ Doss M, Sixel-Dietrich F, Verspohl F (1985). ""Glucose effect" and rate limiting function of uroporphyrinogen synthase on porphyrin metabolism in hepatocyte culture: relationship with human acute hepatic porphyrias" (PDF). J Clin Chem Clin Biochem. 23 (9): 505–13. doi:10.1515/cclm.1985.23.9.505. PMID 4067519.
^ ^a ^b Ajioka, Richard S.; Phillips, John D.; Kushner, James P. (July 2006). "Biosynthesis of heme in mammals". Biochimica et Biophysica Acta (BBA) - Molecular Cell Research. 1763 (7): 723–736. doi:10.1016/j.bbamcr.2006.05.005. PMID 16839620.

External links[edit]

NIH
Abu-Farha M, Niles J, Willmore W (2005). "Erythroid-specific 5-aminolevulinate synthase protein is stabilized by low oxygen and proteasomal inhibition". Biochem Cell Biol. 83 (5): 620–30. doi:10.1139/o05-045. PMID 16234850.
Shemin, D; Rittenberg, D (1945). "The Utilization of Glycine for the Synthesis of a Porphyrin". J. Biol. Chem. 159: 567–8.
SIDEROBLASTIC ANEMIAS -ALAS-2 defect disease

[mol1-1] Hunter, Gregory A.; Ferreira, Gloria C. (November 2011). "Molecular enzymology of 5-Aminolevulinate synthase, the gatekeeper of heme biosynthesis". Biochimica et Biophysica Acta (BBA) - Proteins and Proteomics. 1814 (11): 1467–1473. doi:10.1016/j.bbapap.2010.12.015. PMC 3090494. PMID 21215825.

[2] Shemin, David; Rittenberg, D (June 18, 1945). "The utilization of glycine for the synthesis of a porphyrin". Journal of Biological Chemistry. 159: 567–568.

[plants-3] Beale, S I (June 1978). "δ-Aminolevulinic Acid in Plants: Its Biosynthesis, Regulation, and Role in Plastid Development". Annual Review of Plant Physiology. 29 (1): 95–120. doi:10.1146/annurev.pp.29.060178.000523.

[4] "ALA synthase". flipper e nuvola. Turin University. Retrieved 10 March 2016.

[5] Shoolingin-Jordan, Peter M.; Al-Daihan, Sooad; Alexeev, Dmitriy; Baxter, Robert L.; Bottomley, Sylvia S.; Kahari, I.Donald; Roy, Ipsita; Sarwar, Muhammad; Sawyer, Lindsay; Wang, Shu-Fen (Apr 2003). "5-Aminolevulinic acid synthase: mechanism, mutations and medicine". Biochim Biophys Acta. 1647 (1–2): 361–6. doi:10.1016/s1570-9639(03)00095-5. PMID 12686158.

[6] CHOI, H (July 2004). "Cloning, expression, and characterization of 5-aminolevulinic acid synthase from Rhodopseudomonas palustris KUGB306". FEMS Microbiology Letters. 236 (2): 175–181. doi:10.1016/j.femsle.2004.05.048. PMID 15251194.

[7] Ferreira, Gloria C.; Neame, Peter J.; Dailey, Harry A. (November 1993). "Heme biosynthesis in mammalian systems: Evidence of a schiff base linkage between the pyridoxal 5′-phosphate cofactor and a lysine residue in 5-aminolevulinate synthase". Protein Science. 2 (11): 1959–1965. doi:10.1002/pro.5560021117. PMC 2142290. PMID 8268805.

[8] Hunter, Gregory A.; Ferreira, Gloria C. (March 1999). "Lysine-313 of 5-Aminolevulinate Synthase Acts as a General Base during Formation of the Quinonoid Reaction Intermediates". Biochemistry. 38 (12): 3711–3718. doi:10.1021/bi982390w. PMID 10090759.

[9] Doss M, Sixel-Dietrich F, Verspohl F (1985). ""Glucose effect" and rate limiting function of uroporphyrinogen synthase on porphyrin metabolism in hepatocyte culture: relationship with human acute hepatic porphyrias" (PDF). J Clin Chem Clin Biochem. 23 (9): 505–13. doi:10.1515/cclm.1985.23.9.505. PMID 4067519.

[heme2-10] Ajioka, Richard S.; Phillips, John D.; Kushner, James P. (July 2006). "Biosynthesis of heme in mammals". Biochimica et Biophysica Acta (BBA) - Molecular Cell Research. 1763 (7): 723–736. doi:10.1016/j.bbamcr.2006.05.005. PMID 16839620.

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+{{short description|Class of enzymes}}
-ALA synthase ({{EC number|2.3.1.37}}), or ALAS, catalyzes the synthesis of [[D-Aminolevulinic acid]] (ALA) the first common precursor in the biosynthesis of all [[tetrapyrroles]] such as hemes, cobalamins and chlorophylls <ref> Hunter, Gregory A. Molecular enzymology of 5-Aminolevulinate synthase, the gatekeeper of heme biosynthesis http://www.sciencedirect.com/science/article/pii/S1570963911000021</ref>. The enzyme is expressed in all non-plant eukaryotes and the α-class of proteobacteria. Other organisms produce ALA through a three enzyme pathway known as the Shemin pathway. ALA is synthesized through the condensation of [[glycine]] and [[succinyl-CoA]]. In humans, transcription of ALA synthase is tightly controlled by the presence of [[iron|Fe<sup>2+</sup>]]-binding elements, to prevent accumulation of porphyrin intermediates in the absence of iron. There are two forms of ALA synthase in the body. One form is expressed in red blood cell precursor cells ([[ALAS2]]), whereas the other ([[ALAS1]]) is ubiquitously expressed throughout the body. The red blood cell form is coded by a gene on chromosome x, whereas the other form is coded by a gene on chromosome 3. The disease X-linked [[sideroblastic anemia]] is caused by mutations in the ALA synthase gene on chromosome X, whereas no diseases are known to be caused by mutations in the other gene. Gain of function mutations in the erythroid specific ALA synthase gene have been shown recently to cause a previously unknown form of porphyria known as X-linked-dominant protoporphyria.
+{{Infobox enzyme
+| Name       = 5-aminolevulinate synthase
-===Enzyme Structure and Properties===
+| EC_number  = 2.3.1.37
-PLP-dependent enzymes are prevalent because they are needed to transform amino acids into other resources <ref>Molecular enzymology of 5-Aminolevulinate synthase, the gatekeeper of heme biosynthesis http://www.sciencedirect.com/science/article/pii/S1570963911000021</ref>. ALAS is a homodimer with similarly sized sub units and the active sites consisting of amino acid side chains such as arginine, threonine, and lysine exist at a subunity interface <ref>Molecular enzymology of 5-Aminolevulinate synthase, the gatekeeper of heme biosynthesis http://www.sciencedirect.com/science/article/pii/S1570963911000021</ref>. The protein when extracted from R. spheroids contains 1600-folds and weighs about 80,000 daltons <ref>d-AminoLevulinic Acid in Plants: Its Biosynthesis, Regulation, and Role in Plastid Development http://www.annualreviews.org/doi/pdf/10.1146/annurev.pp.29.060178.000523</ref>. Enzymatic activity varies for different sources of the enzyme <ref>d-AminoLevulinic Acid in Plants: Its Biosynthesis, Regulation, and Role in Plastid Development http://www.annualreviews.org/doi/pdf/10.1146/annurev.pp.29.060178.000523</ref>.
+| CAS_number = 9037-14-3
+| GO_code    =
+| image      = 2bwo.jpg
+| width      = 270
+| caption    = Aminolevulinic acid synthase dimer, Rhodobacter capsulatus
+}}
+'''Aminolevulinic acid synthase''' ('''ALA synthase''', '''ALAS''', or '''delta-aminolevulinic acid synthase''') is an enzyme ({{EC number|2.3.1.37}}) that catalyzes the synthesis of [[δ-aminolevulinic acid]] (ALA) the first common precursor in the biosynthesis of all [[tetrapyrroles]] such as hemes, cobalamins and chlorophylls.<ref name=mol1>{{cite journal|last1=Hunter|first1=Gregory A.|last2=Ferreira|first2=Gloria C.|title=Molecular enzymology of 5-Aminolevulinate synthase, the gatekeeper of heme biosynthesis|journal=Biochimica et Biophysica Acta (BBA) - Proteins and Proteomics|date=November 2011|volume=1814|issue=11|pages=1467–1473|doi=10.1016/j.bbapap.2010.12.015|pmid=21215825|pmc=3090494}}</ref>
+The reaction is as follows:
+:[[succinyl-CoA]] + [[glycine]] <math>\rightleftharpoons</math> [[Aminolevulinic acid|δ-aminolevulinic acid]] + [[Coenzyme A|CoA]] + CO<sub>2</sub>
+This enzyme is expressed in all non-plant eukaryotes and the α-class of proteobacteria and the reaction it catalyses is sometimes referred to as the Shemin pathway for ALA formation.<ref>{{cite journal |last1=Shemin |first1=David |last2=Rittenberg |first2=D |title=The utilization of glycine for the synthesis of a porphyrin |journal=Journal of Biological Chemistry |date=June 18, 1945 |volume=159 |pages=567–568 }}</ref> Other organisms produce ALA through a three enzyme pathway known as the C5 pathway. ALA is synthesized through the condensation of [[glycine]] and [[succinyl-CoA]]. In humans, transcription of ALA synthase is tightly controlled by the presence of [[iron|Fe<sup>2+</sup>]]-binding elements, to prevent accumulation of porphyrin intermediates in the absence of iron. There are two forms of ALA synthase in the body. One form is expressed in red blood cell precursor cells ([[ALAS2]]), whereas the other ([[ALAS1]]) is ubiquitously expressed throughout the body. The red blood cell form is coded by a gene on chromosome X, whereas the other form is coded by a gene on chromosome 3.
-===Reaction Mechanism===
-[[File:ALAS Reaction Mechanism Image.jpg|thumb|center|framed|Aminolevulinic Acid Reaction Mechanism]]
+The disease X-linked [[sideroblastic anemia]] is caused by mutations in the ALA synthase gene on chromosome X, whereas no diseases are known to be caused by mutations in the other gene. Gain of function mutations in the erythroid specific ALA synthase gene have been shown recently to cause a previously unknown form of porphyria known as X-linked-dominant protoporphyria.
-The active sites of ALAS utilize three key amino acid side chains: Arg-85 and Thr-430 and Lys-313. Although these three amino acids have been identified to allow this reaction to proceed, they would be inactive without the addition of cofactor pyridoxal 5’-phosphate (PLP) whose role in this synthesis is detailed in the image above. Before the reaction can begin, the PLP cofactor binds to the lysine side chain to form a Schiff base that promotes attack by glycine substrate <ref>5-Aminolevulinic acid synthase: mechanism, mutations and medicine. http://www.ncbi.nlm.nih.gov/pubmed/12686158
-</ref> , <ref>ALA synthase http://flipper.diff.org/app/pathways/info/6362</ref> , <ref>Cloning, expression, and characterization of 5-aminolevulinic acid synthase from Rhodopseudomonas palustris KUGB306 http://www.sciencedirect.com/science/article/pii/S037810970400401X</ref> , <ref>Heme biosynthesis in mammalian systems: Evidence of a Schiff base linkage between the pyridoxal 5’-phosphate cofactor and a lysine residue in 5-aminolevulinate synthase
-http://onlinelibrary.wiley.com/doi/10.1002/pro.5560021117/abstract</ref>.  Lysine acts as a general base during this mechanism <ref>Molecular enzymology of 5-Aminolevulinate synthase, the gatekeeper of heme biosynthesis http://www.sciencedirect.com/science/article/pii/S1570963911000021
-</ref>, <ref>Lysine-313 of 5-Aminolevulinate Synthase Acts as a General Base during Formation of the Quinonoid Reaction Intermediates http://pubs.acs.org/doi/abs/10.1021/bi982390w</ref>.In the detailed reaction mechanism, the hydronium atoms that are added in come from a variety of residues in that offer hydrogen bonds to facilitate ALA synthesis <ref>Molecular enzymology of 5-Aminolevulinate synthase, the gatekeeper of heme biosynthesis http://www.sciencedirect.com/science/article/pii/S1570963911000021
-</ref>.ALA synthase removes the [[carboxyl]] group from glycine and the [[coenzyme A|CoA]] from the succinyl-CoA by means of its prosthetic group [[pyridoxal phosphate]] (a vitamin b6 derivative), forming δ-aminolevulinic acid (dALA), so called because the [[amino]] group is on the fourth carbon atom in the molecule. This reaction mechanism is particularly unique relative to other enzymes that use the PLP cofactor because  Glycine is initially deprotonated by a highly conserved active site lysine, leading to condensation with succinyl-CoA and loss of CoA. Protonation of the carbonyl group of the intermediate by an active site histidine leads to loss of the carboxyl group. The last intermediate is finally reprotonated to produce ALA. Dissociation of ALA from the enzyme is the rate limiting step of the enzymatic reaction and was shown to be depended upon a slow conformational change of the enzyme. The function of [[pyridoxal phosphate]] is to facilitate the removal of hydrogen, by utilizing the electrophilic [[pyridinium]] ring as an electron sink.
+==Enzyme structure and properties==
-The location of this enzyme in biological systems is indicative of the feedback that it may receive. ALA Synthase has been found in bacteria, yeast, avian and mammalian liver and blood cells and bone marrow. The location of this enzyme in animal cells is within the mitochondria<ref>d-AminoLevulinic Acid in Plants: Its Biosynthesis, Regulation, and Role in Plastid Development http://www.annualreviews.org/doi/pdf/10.1146/annurev.pp.29.060178.000523
-</ref>. Since the enzyme appears to be located near its source of succinyl-CoA and the end of the heme pathway indicates that the starting and end points of heme biosynthesis serves as feedback for ALA Synthase <ref>d-AminoLevulinic Acid in Plants: Its Biosynthesis, Regulation, and Role in Plastid Development http://www.annualreviews.org/doi/pdf/10.1146/annurev.pp.29.060178.000523
+PLP-dependent enzymes are prevalent because they are needed to transform amino acids into other resources.<ref name=mol1 /> ALAS is a homodimer with similarly sized sub units and the active sites consisting of amino acid side chains such as arginine, threonine, and lysine exist at a subunity interface.<ref name=mol1 /> The protein when extracted from R. spheroids contains 1600-folds and weighs about 80,000 daltons.<ref  name=plants>{{cite journal|last1=Beale|first1=S I|title=δ-Aminolevulinic Acid in Plants: Its Biosynthesis, Regulation, and Role in Plastid Development|journal=Annual Review of Plant Physiology|date=June 1978|volume=29|issue=1|pages=95–120|doi=10.1146/annurev.pp.29.060178.000523}}</ref> Enzymatic activity varies for different sources of the enzyme.<ref name=plants />
-</ref>. ALA synthase is also inhibited by [[hemin]] and [[glucose]].<ref>{{cite journal | author = Doss M, Sixel-Dietrich F, Verspohl F | title = "Glucose effect" and rate limiting function of uroporphyrinogen synthase on porphyrin metabolism in hepatocyte culture: relationship with human acute hepatic porphyrias. | journal = J Clin Chem Clin Biochem | volume = 23 | issue = 9 | pages = 505–13 | year = 1985 | pmid = 4067519 | doi=10.1515/cclm.1985.23.9.505}}</ref>
+==Reaction mechanism==
-[[Image:Heme synth step1.png|thumb|center|300px|Heme synthesis]]
+The active sites of ALAS utilize three key amino acid side chains: Arg-85 and Thr-430 and Lys-313. Although these three amino acids have been identified to allow this reaction to proceed, they would be inactive without the addition of cofactor pyridoxal 5’-phosphate (PLP) whose role in this synthesis is detailed in the image below. Before the reaction can begin, the PLP cofactor binds to the lysine side chain to form a Schiff base that promotes attack by glycine substrate.<ref>{{cite web|title=ALA synthase|url=http://flipper.diff.org/app/pathways/info/6362|website=flipper e nuvola|publisher=Turin University|access-date=10 March 2016}}</ref><ref>{{cite journal|last1=Shoolingin-Jordan|first1=Peter M.|last2=Al-Daihan|first2=Sooad|last3=Alexeev|first3=Dmitriy|last4=Baxter|first4=Robert L.|last5=Bottomley|first5=Sylvia S.|last6=Kahari|first6=I.Donald|last7=Roy|first7=Ipsita|author-link7=Ipsita Roy|last8=Sarwar|first8=Muhammad|last9=Sawyer|first9=Lindsay|last10=Wang|first10=Shu-Fen|date=Apr 2003|title=5-Aminolevulinic acid synthase: mechanism, mutations and medicine.|journal=Biochim Biophys Acta|volume=1647|issue=1–2|pages=361–6|doi=10.1016/s1570-9639(03)00095-5|pmid=12686158}}</ref><ref>{{cite journal|last1=CHOI|first1=H|title=Cloning, expression, and characterization of 5-aminolevulinic acid synthase from Rhodopseudomonas palustris KUGB306|journal=FEMS Microbiology Letters|date=July 2004|volume=236|issue=2|pages=175–181|doi=10.1016/j.femsle.2004.05.048|pmid=15251194|doi-access=free}}</ref><ref>{{cite journal|last1=Ferreira|first1=Gloria C.|last2=Neame|first2=Peter J.|last3=Dailey|first3=Harry A.|title=Heme biosynthesis in mammalian systems: Evidence of a schiff base linkage between the pyridoxal 5′-phosphate cofactor and a lysine residue in 5-aminolevulinate synthase|journal=Protein Science|date=November 1993|volume=2|issue=11|pages=1959–1965|doi=10.1002/pro.5560021117|pmid=8268805|pmc=2142290}}</ref> Lysine acts as a general base during this mechanism,.<ref name=mol1 /><ref>{{cite journal|last1=Hunter|first1=Gregory A.|last2=Ferreira|first2=Gloria C.|title=Lysine-313 of 5-Aminolevulinate Synthase Acts as a General Base during Formation of the Quinonoid Reaction Intermediates|journal=Biochemistry|date=March 1999|volume=38|issue=12|pages=3711–3718|doi=10.1021/bi982390w|pmid=10090759}}</ref> In the detailed reaction mechanism, the hydronium atoms that are added in come from a variety of residues that offer hydrogen bonds to facilitate ALA synthesis.<ref name=mol1 />
+ALA synthase removes the [[carboxyl]] group from glycine and the [[coenzyme A|CoA]] from the succinyl-CoA by means of its prosthetic group [[pyridoxal phosphate]] (a vitamin b6 derivative), forming δ-aminolevulinic acid (dALA), so called because the [[amino]] group is on the fourth carbon atom in the molecule. This reaction mechanism is particularly unique relative to other enzymes that use the PLP cofactor because Glycine is initially deprotonated by a highly conserved active site lysine, leading to condensation with succinyl-CoA and loss of CoA. Protonation of the carbonyl group of the intermediate by an active site histidine leads to loss of the carboxyl group. The last intermediate is finally reprotonated to produce ALA. Dissociation of ALA from the enzyme is the rate limiting step of the enzymatic reaction and was shown to be depended upon a slow conformational change of the enzyme. The function of [[pyridoxal phosphate]] is to facilitate the removal of hydrogen, by utilizing the electrophilic [[pyridinium]] ring as an electron sink.
+:[[File:ALAS Reaction Mechanism Image.jpg|675px]]
+The location of this enzyme in biological systems is indicative of the feedback that it may receive. ALA Synthase has been found in bacteria, yeast, avian and mammalian liver and blood cells and bone marrow. The location of this enzyme in animal cells is within the mitochondria.<ref name =plants /> Since the enzyme appears to be located near its source of succinyl-CoA and the end of the heme pathway indicates that the starting and end points of heme biosynthesis serves as feedback for ALA synthase.<ref name =plants /> ALA synthase is also inhibited by [[hemin]] and [[glucose]].<ref>{{cite journal |vauthors=Doss M, Sixel-Dietrich F, Verspohl F | title = "Glucose effect" and rate limiting function of uroporphyrinogen synthase on porphyrin metabolism in hepatocyte culture: relationship with human acute hepatic porphyrias. | journal = J Clin Chem Clin Biochem | volume = 23 | issue = 9 | pages = 505–13 | year = 1985 | pmid = 4067519 | doi=10.1515/cclm.1985.23.9.505| url = https://edoc.hu-berlin.de/bitstream/18452/13180/1/cclm.1985.23.9.505.pdf }}</ref>
-===Biological Function===
-ALAS1 and ALAS2 catalyze the first step in the process of heme synthesis. It is the first irreversible step and is also rate limiting. This means that the beginning of the formation of hemes is very intentional and subject to a variety of areas of feedback. For example, the two substrates, oxaloacetate and glycine, are highly produced by and utilized in other essential biological processes such as glycolysis and the TCA cycle. The image below illustrates the heme synthesis pathway and the role ALAS plays.
+[[Image:Heme synth step1.png|thumb|center|300px|Heme synthesis]]
-{{-}}
-[[Image:Heme_synthesis.png|center|framed|Heme synthesis&mdash;note that some reactions occur in the [[cytoplasm]] and some in the [[mitochondrion]] (yellow)]]
+==Biological function==
+ALAS1 and ALAS2 catalyze the first step in the process of heme synthesis. It is the first irreversible step and is also rate limiting. This means that the beginning of the formation of hemes is very intentional and subject to a variety of areas of feedback. For example, the two substrates, oxaloacetate and glycine, are highly produced by and utilized in other essential biological processes such as glycolysis and the TCA cycle. The image below illustrates the heme synthesis pathway and the role ALAS plays.
+{{Clear}}
+[[Image:Heme synthesis.png|center|framed|Heme synthesis&mdash;note that some reactions occur in the [[cytoplasm]] and some in the [[mitochondrion]] (yellow)]]
+==Disease relevance==
+Aminolevulinic Acid Synthase Deficiency results in a lack of ability to create heme since its job is to catalyze the first step in the process. These deficiencies are often a result of genetic mutation that can result in a variety of diseases. One such disease is x-linked sideroblastic anemia which results in the appearance of red blood cells in the bone marrow.<ref name=heme2>{{cite journal|last1=Ajioka|first1=Richard S.|last2=Phillips|first2=John D.|last3=Kushner|first3=James P.|author-link3=James P. Kushner|title=Biosynthesis of heme in mammals|journal=Biochimica et Biophysica Acta (BBA) - Molecular Cell Research|date=July 2006|volume=1763|issue=7|pages=723–736|doi=10.1016/j.bbamcr.2006.05.005|pmid=16839620|doi-access=free}}</ref> This disease is linked specifically with mutations in the genes that encode for ALAS2.<ref name=heme2 />
-===Disease Relevance===
-Aminolevulinic Acid Synthase Deficiency results in a lack of ability to create heme since its job is to catalyze the first step in the process. These deficiencies are often a result of genetic mutation that can result in a variety of diseases. One such disease is s-linked sideroblastic anemia which results in the appearance red cells in the marrow <ref>Biosynthesis of heme in mammals http://www.sciencedirect.com/science/article/pii/S0167488906001121
-</ref>. This disease is linked specifically with mutations in the genes that encode for ALAS2 <ref>Biosynthesis of heme in mammals http://www.sciencedirect.com/science/article/pii/S0167488906001121
-</ref>.
 ==References==
@@ Line 38: / Line 43: @@
 ==External links==
-* [http://ghr.nlm.nih.gov/gene=alas1 NIH]
+* [https://web.archive.org/web/20051028105722/http://ghr.nlm.nih.gov/gene%3Dalas1 NIH]
-* {{cite journal | author = Abu-Farha M, Niles J, Willmore W | title = Erythroid-specific 5-aminolevulinate synthase protein is stabilized by low oxygen and proteasomal inhibition | journal = Biochem Cell Biol | volume = 83 | issue = 5 | pages = 620–30 | year = 2005 | pmid = 16234850 | doi = 10.1139/o05-045}}
+* {{cite journal |vauthors=Abu-Farha M, Niles J, Willmore W | title = Erythroid-specific 5-aminolevulinate synthase protein is stabilized by low oxygen and proteasomal inhibition | journal = Biochem Cell Biol | volume = 83 | issue = 5 | pages = 620–30 | year = 2005 | pmid = 16234850 | doi = 10.1139/o05-045}}
-*{{cite journal | author = Shemin, D and Rittenberg, D | title = The Utilization of Glycine for the Synthesis of a Porphyrin | journal = J. Biol. Chem. | issue = 159 | pages = 567–8 | year = 1945}}
+*{{cite journal |author1=Shemin, D  |author2=Rittenberg, D | title = The Utilization of Glycine for the Synthesis of a Porphyrin | journal = J. Biol. Chem. | volume= 159 | pages = 567–8 | year = 1945}}
 * [http://sickle.bwh.harvard.edu/sideroblastic.html SIDEROBLASTIC ANEMIAS -ALAS-2 defect disease]
-{{Acyltransferases}}
 {{Porphyrin biosynthesis enzymes}}
+{{Acyltransferases}}
+{{Enzymes}}
+{{Portal bar|Biology|border=no}}
 [[Category:EC 2.3.1]]

v t e Transferases: acyltransferases (EC 2.3)
2.3.1: other than amino-acyl groups	acetyltransferases: Acetyl-Coenzyme A acetyltransferase N-Acetylglutamate synthase Choline acetyltransferase Dihydrolipoyl transacetylase Acetyl-CoA C-acyltransferase Beta-galactoside transacetylase Chloramphenicol acetyltransferase N-acetyltransferase Serotonin N-acetyl transferase HGSNAT ARD1A Histone acetyltransferase P300/CBP NAT2 palmitoyltransferases: Carnitine O-palmitoyltransferase CPT1 CPT2 Serine C-palmitoyltransferase SPTLC1 SPTLC2 other: Acyltransferase like 2 Aminolevulinic acid synthase Beta-ketoacyl-ACP synthase Glyceronephosphate O-acyltransferase Lecithin—cholesterol acyltransferase Glycerol-3-phosphate O-acyltransferase 1-acylglycerol-3-phosphate O-acyltransferase 2-acylglycerol-3-phosphate O-acyltransferase ABHD5
2.3.2: Aminoacyltransferases	Gamma-glutamyl transpeptidase Peptidyl transferase Transglutaminase Tissue transglutaminase Keratinocyte transglutaminase Factor XIII
2.3.3: converted into alkyl on transfer	Citrate synthase Decylcitrate synthase Citrate (Re)-synthase Decylhomocitrate synthase 2-methylcitrate synthase 2-ethylmalate synthase 3-ethylmalate synthase ATP citrate lyase Malate synthase HMG-CoA synthase HMGCS2 2-hydroxyglutarate synthase 3-propylmalate synthase 2-isopropylmalate synthase Homocitrate synthase Sulfoacetaldehyde acetyltransferase

v t e Enzymes
Activity	Active site Binding site Catalytic triad Oxyanion hole Enzyme promiscuity Diffusion-limited enzyme Cofactor Enzyme catalysis
Regulation	Allosteric regulation Cooperativity Enzyme inhibitor Enzyme activator
Classification	EC number Enzyme superfamily Enzyme family List of enzymes
Kinetics	Enzyme kinetics Eadie–Hofstee diagram Hanes–Woolf plot Lineweaver–Burk plot Michaelis–Menten kinetics
Types	EC1 Oxidoreductases (list) EC2 Transferases (list) EC3 Hydrolases (list) EC4 Lyases (list) EC5 Isomerases (list) EC6 Ligases (list) EC7 Translocases (list)