Iron-binding proteins are carrier proteins and metalloproteins that are important in iron metabolism[1] and the immune response.[2][3] Iron is required for life.

Iron-dependent enzymes catalyze a variety of biochemical reactions and can be divided into three broad classes depending on the structure of their active site: non-heme mono-iron, non-heme diiron , or heme centers.[4] A well-known family of iron-dependent enzymes include oxygenases that facilitate hydroxyl group addition of one or both atoms from o2. Notable enzymes include tryptophan dioxygenase, ferredoxin, and 2-oxoglutarate dioxygenase.[5]

Heme proteins

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The heme group uses four equatorial ligands in the porphyrin ring, with the two axial ligands being the histidine side chain and molecular oxygen.

Heme proteins are proteins that contain a heme prosthetic group. The heme group consists of a porphyrin ring coordinated with an iron ion. Four nitrogen atoms in the porphyrin ring act as a ligand for the iron in the center. In many cases, the equatorial porphyrin is complemented by one or two axial ligands. An example of this is in hemoglobin, where the porphyrin works together with a histidine side chain and a bound O2 molecule, forming an octahedral complex.

Hemoglobin

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A visual depiction of the conformational change undergone by hemoglobin upon oxygen binding.

Hemoglobin is an oxygen-transport protein found in virtually all vertebrates. Hemoglobin A is the main type found in human adults. It is a tetramer consisting of two alpha and two beta subunits. Each of the four monomeric units contain a heme prosthetic group in which a ferric cation is bound between four nitrogen atoms of a porphyrin ring. Along with a histidine, the apo form has five ligands surrounding the iron atom. Oxygen binds to the empty sixth position to form an octahedral complex in the holo form.[6] Oxygen binding is fully cooperative for each of the subunits because as the first oxygen binds to one of the four heme groups, the protein undergoes a drastic conformational change that sharply increases the oxygen affinity of the other three subunits.[7]

Hemoglobin has various affinities, depending on pH, structure, and CO2 partial pressure. Fetal hemoglobin is a variant containing two gamma subunits instead of two beta subunits. Fetal hemoglobin is the predominant form up until the infant is several months old, and it has a greater oxygen affinity to compensate for the low oxygen tension of supplied maternal blood during pregnancy.[8] Hemoglobin has a lower oxygen affinity at low pH. This allows for rapid dissociation as oxygenated hemoglobin is transported to cells throughout the body. Because of the CO2 production and aqueous formation of carbonic acid in respiring cells, oxygenated hemoglobin dissociates in order to deliver the necessary oxygen to the cells.[9] Hemoglobin has a binding affinity for carbon monoxide that is 250 times greater than for oxygen. This is the basis of carbon monoxide poisoning, as hemoglobin can no longer transport oxygen to cells.

Cytochromes

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Cytochromes are heme-containing enzymes that act as single-electron transporters, most notably as electron shuttles in oxidative phosphorylation and photosynthesis. Types of well-studied cytochromes include cytochromes a-c, cytochrome oxidase, and cytochrome P450.[10] These proteins act as electron shuttles by switching the oxidation state of the heme iron atom between ferrous (Fe2+) and ferric (Fe3+). Various cytochromes in combination with other redox-active molecules form a gradient of standard reduction potentials that increases the efficiency of energy coupling during electron-transfer events.

Iron-sulfur proteins

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Iron-sulfur proteins are those with an iron structure that includes sulfur. There are a variety of forms iron and sulfur can take in proteins, but the most common are [2Fe 2S] and [4Fe 4S]. Clusters are often associated with cysteine residues in the protein chain.[11]

Non-heme proteins

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Transferrin

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Structure visualization of human serum transferrin.

Transferrin is found in human plasma, and it is used to traffic and import non-heme iron.[12] It travels freely in the extracellular space.[13] When its iron is needed by the cell, it is brought into the cytosol by a transferrin receptor. Transferrin can bind two Fe(III) ions, along with an anion (usually carbonate). To release the iron, the carbonate anion is protonated. This changes the carbonate's interaction with the protein, changing the conformation and allowing Fe(III) to be transferred.

Transferrin has a molecular weight of about 80 kDa. It is a glycoprotein, meaning that it has sugars attached to its amino acid chain.

Lactoferrin

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Lactoferrin is a member of the transferrin family and is the predominant protein found in mammal exocrine secretions, such as tears, milk, and saliva. It is composed of approximately 700 residues and exists mainly as a tetramer, with the monomer:tetramer ratio being 1:4 at 10 μM protein concentrations.[14] The tertiary structure is composed of two lobes, termed N and C lobes, each containing one iron-binding pocket. Each pocket contributes four amino acids (two tyrosines, one histidine, and one aspartate) and, along with two carbonate or bicarbonate anions, forms a six-membered coordinate around the iron cation. It is this specific combination that makes lactoferrin's iron affinity 300 times greater than transferrin.[15]

 
Depiction of lactoferrin (left) competitively binding iron over an E. coli siderophore (right).

Lactoferrin has significant antimicrobial properties. It is found in the highest concentration of 150 ng/mL in human colostrum (the type of milk produced at the end stages of pregnancy), providing much needed immune support to newly born infants.[16] It was widely believed that lactoferrin was only a bacteriostatic agent due to its high iron affinity and its ability to sequester free iron atoms from pathogenic microbes. It is now known, however, that the major antimicrobial driving force lies in the bactericidal properties of its iron-bound pocket and a specific peptide lactoferricin located at the N-lobe. Lactoferrin is able to bind to the LPS (lipopolysaccharide) layer of bacteria, and in its holo form the iron atom oxidizes the lipopolysaccharides to lyse the outer membrane and simultaneously produce toxic hydrogen peroxide.[17] Additionally, upon cleavage of lactoferrin by trypsin, the peptide lactoferricin is produced which binds to H+-ATPase, disrupting proton translocation and ultimately killing the cell.[18]

Ferritin

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Protein structure of fully assembled ferritin. A single subunit is colored in purple.

Ferritin is an iron reservoir for an individual cell. It is found in all cells types and localized in the cytosol. Ferritin is a large protein composed of 24 subunits surrounding a core full of iron atoms. It is capable of holding 0-4500 iron atoms,[19] which can be used as a reservoir for cellular needs. Iron is stored when there is excess, and retrieved when iron is needed again.[12] The subunits are a mixture of H (heavy or heart) and L (light or liver). The subunits form a cluster 70-80 Angstroms wide, which is then filled with iron ferrihydrite.[20]

Ferritin is a highly conserved protein through all domains of life. It is so conserved that subunits from horses and humans can assemble together into a functional protein.[12] Each subunit is composed of five alpha helices.

Ferritin is used to diagnose low iron levels in humans.[19] It can be used to indicate the level of bioavailable iron, which is helpful for diagnosing anemia. The usual range for men is 18-270 ng/mL and the range for women is 18-160 ng/mL.[21]

See also

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References

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  1. ^ Brock JH (1989). "Iron-binding proteins". Acta Paediatrica Scandinavica. Supplement. 361: 31–43. doi:10.1111/apa.1989.78.s361.31. PMID 2485582. S2CID 44752615.
  2. ^ De Sousa M, Breedvelt F, Dynesius-Trentham R, Trentham D, Lum J (1988). "Iron, iron-binding proteins and immune system cells". Annals of the New York Academy of Sciences. 526 (1): 310–22. Bibcode:1988NYASA.526..310S. doi:10.1111/j.1749-6632.1988.tb55515.x. PMID 3291685. S2CID 12756539.
  3. ^ Kaplan J, Ward DM (August 2013). "The essential nature of iron usage and regulation". Current Biology. 23 (15): R642-6. doi:10.1016/j.cub.2013.05.033. PMC 3928970. PMID 23928078.
  4. ^ Solomon EI, Brunold TC, Davis MI, Kemsley JN, Lee SK, Lehnert N, Neese F, Skulan AJ, Yang YS, Zhou J (January 2000). "Geometric and electronic structure/function correlations in non-heme iron enzymes". Chemical Reviews. 100 (1): 235–350. doi:10.1021/cr9900275. PMID 11749238.
  5. ^ Cheng AX, Han XJ, Wu YF, Lou HX (January 2014). "The function and catalysis of 2-oxoglutarate-dependent oxygenases involved in plant flavonoid biosynthesis". International Journal of Molecular Sciences. 15 (1): 1080–95. doi:10.3390/ijms15011080. PMC 3907857. PMID 24434621.
  6. ^ Menis, Oscar (1968). "Technical Note 454". Analytical Coordination Chemistry Section: Summary of Activities July 1967 to June 1968. Gaithersburg, MD: Analytical Coordination Chemistry Section Analytical Chemistry Division Institute for Materials Research. doi:10.6028/nbs.tn.454.
  7. ^ Mihailescu MR, Russu IM (March 2001). "A signature of the T → R transition in human hemoglobin". Proceedings of the National Academy of Sciences of the United States of America. 98 (7): 3773–7. Bibcode:2001PNAS...98.3773M. doi:10.1073/pnas.071493598. PMC 31128. PMID 11259676.
  8. ^ Berg JM, Tymoczko JL, Stryer L (2002). Biochemistry (5th ed.). New York: W.H. Freeman. ISBN 0716730510. OCLC 48055706.
  9. ^ Hasselbalch KA (December 1964). "Calculation Of The Hydrogen Ion Concentration Of Blood From Free And Bound Carbon Dioxide Oxygen Binding As A Function Of Ph". Survey of Anesthesiology. 8 (6): 607–32. doi:10.1097/00132586-196412000-00059.
  10. ^ L., Lehninger, Albert (2000). Lehninger principles of biochemistry. Nelson, David L. (David Lee), 1942-, Cox, Michael M. (3rd. ed.). New York: Worth Publishers. ISBN 1572591536. OCLC 42619569.{{cite book}}: CS1 maint: multiple names: authors list (link)
  11. ^ Johnson, Deborah C.; Dean, Dennis R.; Smith, Archer D.; Johnson, Michael K. (Feb 18, 2005). "Structure, Function, and Formation of Biological Iron-Sulfur Clusters". Annual Review of Biochemistry. 74 (1): 247–281. doi:10.1146/annurev.biochem.74.082803.133518. ISSN 0066-4154. PMID 15952888.
  12. ^ a b c Aisen P, Enns C, Wessling-Resnick M (October 2001). "Chemistry and biology of eukaryotic iron metabolism". The International Journal of Biochemistry & Cell Biology. 33 (10): 940–59. doi:10.1016/s1357-2725(01)00063-2. PMID 11470229.
  13. ^ "TF - Serotransferrin precursor - Homo sapiens (Human) - TF gene & protein". www.uniprot.org. Retrieved 2018-11-11.
  14. ^ Baker EN, Baker HM (November 2005). "Molecular structure, binding properties and dynamics of lactoferrin". Cellular and Molecular Life Sciences. 62 (22): 2531–9. doi:10.1007/s00018-005-5368-9. PMC 11139133. PMID 16261257. S2CID 218464085.
  15. ^ Mazurier J, Spik G (May 1980). "Comparative study of the iron-binding properties of human transferrins. I. Complete and sequential iron saturation and desaturation of the lactotransferrin". Biochimica et Biophysica Acta. 629 (2): 399–408. doi:10.1016/0304-4165(80)90112-9. PMID 6770907.
  16. ^ Sánchez L, Calvo M, Brock JH (May 1992). "Biological role of lactoferrin". Archives of Disease in Childhood. 67 (5): 657–61. doi:10.1136/adc.67.5.657. PMC 1793702. PMID 1599309.
  17. ^ Farnaud S, Evans RW (November 2003). "Lactoferrin--a multifunctional protein with antimicrobial properties". Molecular Immunology. 40 (7): 395–405. doi:10.1016/S0161-5890(03)00152-4. PMID 14568385.
  18. ^ Kuwata H, Yip TT, Yip CL, Tomita M, Hutchens TW (April 1998). "Bactericidal domain of lactoferrin: detection, quantitation, and characterization of lactoferricin in serum by SELDI affinity mass spectrometry". Biochemical and Biophysical Research Communications. 245 (3): 764–73. doi:10.1006/bbrc.1998.8466. PMID 9588189.
  19. ^ a b Andrews NC (July 2008). "Forging a field: the golden age of iron biology". Blood. 112 (2): 219–30. doi:10.1182/blood-2007-12-077388. PMC 2442739. PMID 18606887.
  20. ^ Crichton RR, Charloteaux-Wauters M (May 1987). "Iron transport and storage". European Journal of Biochemistry. 164 (3): 485–506. doi:10.1111/j.1432-1033.1987.tb11155.x. PMID 3032619.
  21. ^ "What Is a Ferritin Blood Test? What Do the Results Mean?". WebMD. Retrieved 2018-11-11.