BLBS102-c09 BLBS102-Simpson March 21, 2012 11:15 Trim: 276mm X 219mm Printer Name: Yet to Come
9 Enzymes in Food Processing 189modification of gluten. The enzymes are able to do this by in-
creasing the viscoelastic, gas-retaining, and thermosetting prop-
erties of the dough. The action of these enzymes results in bene-
fits such as shorter time of mixing, better flow, improved shaping,
and increased gas retention of the flour or dough (Mathewson
1998).MetalloproteasesThe term metalloproteases is used to encompass those proteases
that have metal ions in their active sites. These enzymes typically
require an essential metal ion (e.g., Ni^2 +,Mg^2 +,Mn^2 +,Ca^2 +,
Zn^2 +, and Co^2 +) for functional activity. Urease is an example
of the nickel (Ni^2 +)-containing metalloenzymes. It catalyzes the
breakdown of urea into carbon dioxide (CO 2 ) and ammonia
(NH 3 ). The urease-catalyzed reaction occurs as follows:
(NH 2 ) 2 CO+H 2 O→CO 2 +2NH 3The NH 3 thus produced functions to neutralize gastric acid
in the stomach. Urease is found in bacteria, yeast, and several
higher plants. The major sources of urease include the Jack bean
(Canavalia ensiformis) plant and the bacteriaB. pasteurii.The
enzyme is also found in large quantities in soybeans and other
plant seeds, in certain animal tissues (e.g., liver, blood, and mus-
cle), in intestinal bacteria (e.g.,Eubacterium aerofaciens,E.
lentum,andPeptostreptococcus productus), and in yeasts (e.g.,
Candida curvata, C. humicola, C. bogoriensis,C. diffluens,and
RhodotorulaandCryptococcusspecies), as well as the blue-
green algae (Anabaena doliolumandAnacystis nidulans). Ex-
amples of the metalloproteases that are Mg^2 +dependent include
inorganic diphosphatase that catalyzes the cleavage of diphos-
phate into inorganic phosphates, that is,
Diphosphate+H 2 O⇔2 Phosphateand phosphatidylinositol triphosphate 3-phosphatase that
catalyzes the hydrolysis of phosphatidylinositol 3,4,5-
trisphosphate, that is,
Phosphatidylinositol 3, 4 ,5-trisphosphate+H 2 O
⇔Phosphatidylinositol 4,5-bisphosphate+PhosphateAn example of metalloproteases containing manganese
(Mn^2 +) metal ions is phosphoadenylylsulfatase, which partici-
pates in sulfur metabolism and catalyzes the hydrolytic cleavage
of 3′-phosphoadenylyl sulfate into adenosine 3′,5′-bisphosphate
and sulfate:
3 ′-Phosphoadenylyl sulfate+H 2 O
⇔Adenosine 3′, 5 ′-Bisphosphate+SulfateA well-known calcium (Ca^2 +)-containing metalloprotease is
lactonase, which hydrolyzes lactones into their corresponding
hydroacids, that is,
Lactone(s)+H 2 O⇔4-Hydroxyacid(s)The enzyme lactonase also participates in the metabolism of
galactose and ascorbic acid.
Other metalloproteases contain zinc (Zn^2 +) metal ions,
e.g., glutamate carboxypeptidase and glutamyl aminopepti-
dase. Glutamate carboxypeptidase catalyzes the hydrolysisofN-acetylaspartylglutamic acid into glutamic acid andN-
acetylaspartate as shown in the following reaction:N-Acetylaspartylglutamate+H 2 O
⇔Glutamic acid+N-Acetylaspartatewhile glutamyl aminopeptidase (also known as aminopeptidase
A) catalyzes the hydrolysis of glutamic and aspartic acid residues
from the N-termini of polypeptides, e.g.,Aspartic acid-polypeptide+H 2 O
⇔Aspartic acid+PolypeptideGlutamyl aminopeptidase is important because of its capacity
to degrade angiotensin II into angiotensin III, which promote
vasoconstriction and high blood pressure. Both glutamate car-
boxypeptidase and glutamyl aminopeptidase are present in mem-
branes. Another important Zn^2 +-containing metalloprotease is
theinsulin-degrading enzymethat is found in humans and de-
grades short chain polypeptides such as theβ-chain of insulin,
glucagon, transforming growth factor, and endorphins. Collage-
nases are also Zn^2 +dependent and they act to break down the
peptide bonds in collagen. Cobalt (Co^2 +)-containing metallo-
proteases include methylmalonyl coenzyme A mutase that con-
verts methyl malonyl-CoA to succinyl-CoA, which is involved
in the extraction of energy from proteins and fats; other Co^2 +-
containing metalloenzymes are methionine aminopeptidase and
nitrile hydratase (Kobayashi and Shimizu 1999).
Sources of metalloproteases include those derived from an-
imals, like carboxypeptidases A and B, collagenases, gelati-
nases, and procollagen proteinase; microbial ones such as
thermolysin, lysostaphin (fromStaphylococcussp), acidolysin
(fromClostridium acetobutylicum), and neutral metallopro-
teases (fromBacillussp); as well as plant types like the zinc-
dependent endoproteases in the seeds of grass pea (Lathyrus
sativusL.). Agents or substances that are capable of bind-
ing or interacting with the catalytic metal ions tend be po-
tent inhibitors of this group of enzymes. Examples of these
inhibitors include phosphoramidon, ethylenediaminetetraacetic
acid (EDTA), methylamine, vitamin B-12, dimercaprol, por-
phine, phosphonates, and 1,10-phenanthroline.
Common commercially available metalloenzymes are Neu-
trase (Novo Nordisk 1993) and Thermoase (Amano Enzymes)
and some of the industrial applications of metalloenzymes in-
clude the synthesis of peptides for use as low calorie sweetener
and drugs for the food and pharmaceutical industries, respec-
tively. Thermolysin and vimelysin (fromVibriosp) are both
used for the synthesis of aspartame (Murakami et al. 1998); in
this regard, vimelysin is superior to thermolysin for synthesis
of the dipeptide at low temperatures. The metalloprotease ther-
molysin is also used in combination with other proteases (pro-
tease cocktails) for the production of food protein hydrolysates
and flavor-enhancing peptides and for accelerating the ripening
of dry sausages (Fernandez et al. 2000). They are also used for
the hydrolysis of slaughterhouse waste, and in the brewing in-
dustry to facilitate filtration of beer and production of low calorie
beers.