Metalloenzymes all have one feature in common, namely that the metal ion is bound to the protein with one
labile coordination site. As with all
enzymes, the shape of the
active site is crucial. The metal ion is usually located in a pocket whose shape fits the substrate. The metal ion
catalyzes reactions that are difficult to achieve in
organic chemistry.
Carbonic anhydrase . The three coordinating
histidine residues are shown in green,
hydroxide in red and white, and the
zinc in gray. In
aqueous solution,
carbon dioxide forms
carbonic acid :CO2 + H2O H2CO3 This reaction is very slow in the absence of a catalyst, but quite fast in the presence of the
hydroxide ion :CO2 + OH− hydrogencarbonate| A reaction similar to this is almost instantaneous with
carbonic anhydrase. The structure of the active site in carbonic anhydrases is well known from a number of crystal structures. It consists of a
zinc ion coordinated by three
imidazole nitrogen atoms from three
histidine units. The fourth coordination site is occupied by a water molecule. The coordination sphere of the zinc ion is approximately
tetrahedral. The positively-charged zinc ion polarizes the coordinated water molecule, and
nucleophilic attack by the negatively-charged hydroxide portion on carbon dioxide proceeds rapidly. The catalytic cycle produces the bicarbonate ion and the hydrogen ion
Vitamin B12-dependent enzymes The
cobalt-containing
Vitamin B12 (also known as cobalamin) catalyzes the transfer of
methyl (−CH3) groups between two molecules, which involves the breaking of
C−C bonds, a process that is energetically expensive in organic reactions. The metal ion lowers the
activation energy for the process by forming a transient Co−CH3 bond. The structure of the
coenzyme was famously determined by
Dorothy Hodgkin and co-workers, for which she received a
Nobel Prize in Chemistry. It consists of a cobalt(II) ion coordinated to four nitrogen atoms of a
corrin ring and a fifth nitrogen atom from an
imidazole group. In the resting state there is a Co−C
sigma bond with the 5′ carbon atom of
adenosine. This is a naturally occurring
organometallic compound, which explains its function in
trans-methylation reactions, such as the reaction carried out by
methionine synthase.
Nitrogenase (nitrogen fixation) The
fixation of atmospheric nitrogen is an energy-intensive process, as it involves breaking the very stable
triple bond between the nitrogen atoms. The
nitrogenases catalyze the process. One such enzyme occurs in
Rhizobium bacteria. There are three components to its action: a
molybdenum atom at the active site,
iron–sulfur clusters that are involved in transporting the electrons needed to reduce the nitrogen, and an abundant energy source in the form of
magnesium ATP. This last is provided by a
mutualistic symbiosis between the bacteria and a host plant, often a
legume. The reaction may be written symbolically as :N2 + 16 Mg
ATP + 8 e− → 2
NH3 + 16 Mg
ADP +16 Pi + H2 where Pi stands for inorganic
phosphate. The precise structure of the active site has been difficult to determine. It appears to contain a MoFe7S8 cluster that is able to bind the dinitrogen molecule and, presumably, enable the reduction process to begin. Some species of bacteria and archaea have also been shown to have
Vanadium nitrogenases, which contain a VFe3S4 cluster and allows for an alternative pathway of nitrogen fixation in Molybdenum-deficient conditions. The electrons are transported by the associated "P" cluster, which contains two
cubical Fe4S4 clusters joined by sulfur bridges.
Superoxide dismutase The
superoxide ion, is generated in biological systems by reduction of molecular
oxygen. It has an unpaired
electron, so it behaves as a
free radical. It is a powerful
oxidizing agent. These properties render the superoxide ion very
toxic and are deployed to advantage by
phagocytes to kill invading
microorganisms. Otherwise, the superoxide ion must be destroyed before it does unwanted damage in a cell. The
superoxide dismutase enzymes perform this function very efficiently. The formal
oxidation state of the oxygen atoms is −. In solutions at neutral
pH, the superoxide ion
disproportionates to molecular oxygen and
hydrogen peroxide. :2 + 2 H+ → O2 + H2O2 In biology this type of reaction is called a
dismutation reaction. It involves both oxidation and reduction of superoxide ions. The
superoxide dismutase (SOD) group of enzymes increase the
rate of reaction to near the diffusion-limited rate. The key to the action of these enzymes is a metal ion with variable oxidation state that can act either as an oxidizing agent or as a reducing agent. :Oxidation: M(
n+1)+ + → M
n+ + O2 :Reduction: M
n+ + + 2 H+ → M(
n+1)+ + H2O2. In human SOD, the active metal is
copper, as Cu(II) or Cu(I), coordinated
tetrahedrally by four
histidine residues. This enzyme also contains
zinc ions for stabilization and is activated by copper chaperone for superoxide dismutase (
CCS). Other
isozymes may contain
iron, manganese or
nickel. The activity of Ni-SOD involves nickel(III), an unusual oxidation state for this element. The active site nickel geometry cycles from
square planar Ni(II), with thiolate (Cys2 and Cys6) and backbone nitrogen (His1 and Cys2) ligands, to
square pyramidal Ni(III) with an added axial His1 side chain ligand.
Chlorophyll-containing proteins (left) and
chlorophyll (right), two extremely different molecules when it comes to function, are quite similar when it comes to its atomic shape. There are only three major structural differences; a
magnesium atom (Mg) in chlorophyll, as opposed to
iron (Fe) in hemoglobin. Additionally, chlorophyll has an extended
isoprenoid tail and an additional
aliphatic cyclic structure off the macrocycle. |391x391px Chlorophyll plays a crucial role in
photosynthesis. It contains a
magnesium enclosed in a
chlorin ring. However, the magnesium ion is not directly involved in the photosynthetic function and can be replaced by other divalent ions with little loss of activity. Rather, the
photon is absorbed by the chlorin ring, whose electronic structure is well-adapted for this purpose. Initially, the absorption of a photon causes an
electron to be excited into a
singlet state of the Q band. The
excited state undergoes an
intersystem crossing from the singlet state to a
triplet state in which there are two electrons with parallel
spin. This species is, in effect, a
free radical, and is very reactive and allows an electron to be transferred to acceptors that are adjacent to the chlorophyll in the
chloroplast. In the process chlorophyll is oxidized. Later in the photosynthetic cycle, chlorophyll is reduced back again. This reduction ultimately draws electrons from water, yielding molecular oxygen as a final oxidation product.
Hydrogenase Hydrogenases are subclassified into three different types based on the active site metal content: iron–iron hydrogenase, nickel–iron hydrogenase, and iron hydrogenase. All hydrogenases catalyze reversible
H2 uptake, but while the [FeFe] and [NiFe] hydrogenases are true
redox catalysts, driving H2 oxidation and H+ reduction :H2 2 H+ + 2 e− the [Fe] hydrogenases catalyze the reversible
heterolytic cleavage of H2. :H2 H+ + H−
Ribozyme and deoxyribozyme Since discovery of
ribozymes by
Thomas Cech and
Sidney Altman in the early 1980s, ribozymes have been shown to be a distinct class of metalloenzymes. Many ribozymes require metal ions in their active sites for chemical catalysis; hence they are called metalloenzymes. Additionally, metal ions are essential for structural stabilization of ribozymes.
Group I intron is the most studied ribozyme which has three metals participating in catalysis. Other known ribozymes include
group II intron,
RNase P, and several small viral ribozymes (such as
hammerhead,
hairpin,
HDV, and
VS) and the large subunit of ribosomes. Several classes of ribozymes have been described.
Deoxyribozymes, also called DNAzymes or catalytic DNA, are artificial DNA-based catalysts that were first produced in 1994. Almost all DNAzymes require metal ions. Although ribozymes mostly catalyze cleavage of RNA substrates, a variety of reactions can be catalyzed by DNAzymes including RNA/DNA cleavage, RNA/DNA ligation, amino acid phosphorylation and dephosphorylation, and carbon–carbon bond formation. Yet, DNAzymes that catalyze RNA cleavage reaction are the most extensively explored ones. 10-23 DNAzyme, discovered in 1997, is one of the most studied catalytic DNAs with clinical applications as a therapeutic agent. Several metal-specific DNAzymes have been reported including the GR-5 DNAzyme (
lead-specific), the CA1-3 DNAzymes (
copper-specific), the 39E DNAzyme (
uranyl-specific) and the NaA43 DNAzyme (
sodium-specific). == Signal-transduction metalloproteins ==