Deoxyribonuclease IV (phage-T4-induced) (, ''endodeoxyribonuclease IV (phage T4-induced)'', ''E. coli endonuclease IV'', ''endodeoxyribonuclease'', ''redoxyendonuclease'', ''deoxriboendonuclease'', ''Escherichia coli endonuclease II'', ''endonuclease II'', ''DNA-adenine-transferase'') is catalyzes the degradation nucleotides
in
DsDNA by attacking the 5'-terminal end.
Deoxyribonuclease IV is a type of deoxyribonuclease that has both an exonucleolytic and an endonucleolytic activity.
It functions at abasic or apurinic-apyrimidininc sites when the cell is undergoing
nucleotide excision repair
Nucleotide excision repair is a DNA repair mechanism. DNA damage occurs constantly because of chemicals (e.g. intercalating agents), radiation and other mutagens. Three excision repair pathways exist to repair single stranded DNA damage: Nucle ...
pathway. In addition, the endonuclease IV consists of several activities such as AP endonuclease, 3'-diesterase, 3'->5' exonuclease, and 3'phosphatase.
The endonuclease IV is encoded by denB of bacteriophage T4 and its binding sequence is 5′-dT, , dCdAdCdTdTdC-3′. It has been discovered that
serine
Serine (symbol Ser or S) is an α-amino acid that is used in the biosynthesis of proteins. It contains an α-amino group (which is in the protonated − form under biological conditions), a carboxyl group (which is in the deprotonated − form un ...
176 residue plays a crucial role in increasing the hydrolysis rate of the endonuclease of a consensus sequence containing cytidine. The endonuclease IV falls under a structurally resembling members with apyrimidininc endonuclease I (APE1).
Discovery
Deoxyribonuclease IV was first isolated from rabbit tissues in 1968. Specifically, it was found in rabbit bone marrow by Lindahl. And its molecular weight was determined to be 42,000
dalton. It was discovered that this enzyme resembles several microbial
endonuclease
Endonucleases are enzymes that cleave the phosphodiester bond within a polynucleotide chain. Some, such as deoxyribonuclease I, cut DNA relatively nonspecifically (without regard to sequence), while many, typically called restriction endonucleases ...
activities of
DNA polymerase I
DNA polymerase I (or Pol I) is an enzyme that participates in the process of prokaryotic DNA replication. Discovered by Arthur Kornberg in 1956, it was the first known DNA polymerase (and the first known of any kind of polymerase). It was initiall ...
found in
Escherichia coli, which appear to be necessary for DNA repair and recombination. It also resembles gamma exonuclease, which performs an important function in recombination of bacteriophage.
Structure
DNase IV is composed of 185 amino acid residues with
magnesium ions acting as a cofactor. Divalent metal ions such as
Mg²⁺
Magnesium is a chemical element with the symbol Mg and atomic number 12. It is a shiny gray metal having a low density, low melting point and high chemical reactivity. Like the other alkaline earth metals (group 2 of the periodic t ...
act as cofactor during the cleavage of 5'-mononucleotides. DNase IV prefers to attack native DNA acting as an endonuclease with metal ions either Mg++ or Mn++.
Its TIM beta barrel core surrounded by helices with three metal ions —either three Zn2+ or two Zn2+ and one Mn2+ which plays crucial role in AP excision repair.
Function
DNase IV attacks dsDNA at 5' ends by liberating 5' mononucleotides but it does not attack any monomers in polydeoxyribonucleotides in a random fashion. It cleaves polydeoxyribonucleotides in an exonucleolytic fashion from 5' end, meaning it removes a nucleotide chain that is adjacent to the 5' terminal end rather than cleaving a nucleotide located in the middle of the chain. DNase IV works by attacking multiple polynucleotide chains at the same time.
Since it does not cleave dsDNA in a processive way, the rate of hydrolysis of this enzyme is faster than native DNA in terms of kinetics.
DNase IV does not recognize specific sequences on DNA for non-staggered cleavage. However, it requires two base pairs at one cleavage site, and the other cleavage site of double-stranded DNA should have more than 10 base pairs.
Enzyme Activities in cell environment and DNA
70% of the total DNase IV activitiy was found in the cytoplasm while 30% was found in cell nuclei.
In human body, DNase IV was required for cleavage of a reaction intermediate generated by template strand displacement during gap-filling.
During the endonuclease activity, conformational change in DNA occurs in a way that exposes the abasic site by benting the DNA by 90 degrees, which invovles flipping out the sugar moiety into a small pocket that would not form watson-crick base pair.
DNase IV acts on double stranded DNA in repair by breaking phosphodiester bonds, but the number of cleavages by this enzyme is smaller than the extent of polymerization of DNA.
Difference between DNase III vs. DNase IV
In crude cell extracts from lymphoid organs, DNase III and DNase IV show major activities because DNase I activity is inhibited. The activities of DNase III and DNase IV depend on two Mg++ as cofactors and these enzymes are localized in cell nuclei. Even though they require same divalent metal to function, there are major difference in liberating polynucleotides. DNase III cleaves a single strand of DNA from 3' terminal end but DNase IV cleaves a double strand of DNA from 5' terminal end.
Because DNase III degrades single stranded DNA, the rate of hydrolysis of DNase III is more rapid than that of DNase IV.
See also
*
Phage T4
Escherichia virus T4 is a species of bacteriophages that infect ''Escherichia coli'' bacteria. It is a double-stranded DNA virus in the subfamily ''Tevenvirinae'' from the family Myoviridae. T4 is capable of undergoing only a lytic lifecycle ...
References
External links
*
{{Portal bar, Biology, border=no
EC 3.1.21