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Astacin proteases cleave dentin sialophosphoprotein (Dspp) to generate dentin phosphoprotein (Dpp).
[dentin dysplasia]
Dentin
sialophosphoprotein
(
Dspp
)
is
critical
for
proper
dentin
biomineralization
because
genetic
defects
in
DSPP
cause
dentin
dysplasia
type
II
and
dentinogenesis
imperfecta
types
II
and
III
.
Dspp
is
processed
by
proteases
into
smaller
subunits
;
the
initial
cleavage
releases
dentin
phosphoprotein
(
Dpp
)
.
We
incubated
fluorescence
resonance
energy
transfer
(
FRET
)
peptides
containing
the
amino
acid
context
of
the
Dpp
cleavage
site
(
YEFDGKSMQGDDPN
,
designated
Dspp-
FRET
)
or
a
mutant
version
of
that
context
(
YEFDGKSIEGDDPN
,
designated
mutDspp-FRET
)
with
BMP-
1
,
MEP
1
A
,
MEP
1
B
,
MMP-
2
,
MMP-
8
,
MMP-
9
,
MT
1
-
MMP
,
MT
3
-
MMP
,
Klk
4
,
MMP-
20
,
plasmin
,
or
porcine
Dpp
and
characterized
the
peptide
cleavage
products
.
Only
BMP-
1
,
MEP
1
A
,
and
MEP
1
B
cleaved
Dspp-
FRET
at
the
G-D
peptide
bond
that
releases
Dpp
from
Dspp
in
vivo
.
We
isolated
Dspp
proteoglycan
from
dentin
power
and
incubated
it
with
the
three
enzymes
that
cleaved
Dspp-
FRET
at
the
G-D
bond
.
In
each
case
,
the
released
Dpp
domain
was
isolated
,
and
its
N-
terminus
was
characterized
by
Edman
degradation
.
BMP-
1
and
MEP
1
A
both
cleaved
native
Dspp
at
the
correct
site
to
generate
Dpp
,
making
both
these
enzymes
prime
candidates
for
the
protease
that
cleaves
Dspp
in
vivo
.
MEP
1
B
was
able
to
degrade
Dpp
when
the
Dpp
was
at
sufficiently
high
concentration
to
deplete
free
calcium
ion
concentration
.
Immunohistochemistry
of
developing
porcine
molars
demonstrated
that
astacins
are
expressed
by
odontoblasts
,
a
result
that
is
consistent
with
RT-PCR
analyses
.
We
conclude
that
during
odontogenesis
,
astacins
in
the
predentin
matrix
cleave
Dspp
before
the
DDPN
sequence
at
the
N-
terminus
of
Dpp
to
release
Dpp
from
the
parent
Dspp
protein
.
Diseases
Validation
Diseases presenting
"defects in dspp"
symptom
dentin dysplasia
dentinogenesis imperfecta
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