Definition of Restriction enzyme
Restriction enzyme: An enzyme from bacteria that can
recognize specific base sequences in DNA and cut the DNA at that site
(the restriction site). A restriction enzyme acts as a biochemical
scissors. Also called a restriction endonuclease.
A restriction enzyme is a protein produced by bacteria that
cleaves DNA at specific sites. Bacteria use restriction enzymes to
defend against bacterial viruses called bacteriophages (or phage).
When a phage infects a bacteria, it inserts its DNA into the bacteria
so that it might be replicated. The restriction enzyme prevents
replication of the phage DNA by cutting it into many pieces.
Restriction enzymes were named for their ability to restrict, or
limit, the number of strains of bacteriophage that can
infect bacteria.
Restriction enzymes can be isolated from bacteria and used in the
laboratory to cut DNA. They are indispensable tools in recombinant
DNA technology and genetic engineering. Each restriction enzyme
recognizes a short, specific sequence of nucleotide bases (the four
basic chemical subunits of the linear double-stranded DNA molecule--
adenine, cytosine, thymine, and guanine). These stretches in the DNA
are called recognition sequences and are randomly distributed
throughout the DNA. Different bacterial species make restriction
enzymes that recognize different nucleotide sequences.
After a restriction endonuclease recognizes a sequence, it cuts
through the DNA molecule by catalyzing the hydrolysis (splitting of a
chemical bond by addition of a water molecule) of the bond between
adjacent nucleotides. Bacteria prevent their own DNA from being
degraded in this manner by disguising their recognition sequences.
Enzymes called methylases add methyl groups (--CH3) to adenine or
cytosine bases within the recognition sequence, which is thus
modified and protected from the endonuclease. The restriction enzyme
and its corresponding methylase constitute the restriction-
modification system of a bacterial species.
All restriction enzymes are different. There are three classes of
restriction enzymes, designated types I, II, and III. Types I and III
enzymes are similar in that both restriction and methylase activities
are carried out by one large enzyme complex, in contrast to the type
II system, in which the restriction enzyme is independent of its
methylase. Type II restriction enzymes also differ from the other two
types in that they cleave DNA at specific sites within the
recognition site; the others cleave DNA randomly, sometimes hundreds
of bases from the recognition sequence.
Restriction enzymes were originally discovered and characterized
by the molecular biologists Werner Arber, Hamilton O. Smith, and
Daniel Nathans who shared the 1978 Nobel prize in medicine. The
ability of restriction enzymes to cut DNA at precise locations has
permitted researchers to isolate gene-containing fragments and
recombine them with other molecules of DNA. More than 2,500 type II
restriction enzymes have been identified from a variety of bacterial
species. These enzymes recognize about 200 distinct sequences, which
are four to eight bases in length.
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