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Caspase cleavage of GFAP produces an assembly-compromised proteolytic fragment that promotes filament aggregation.
[alexander disease]
IF
(
intermediate
filament
)
proteins
can
be
cleaved
by
caspases
to
generate
proapoptotic
fragments
as
shown
for
desmin
.
These
fragments
can
also
cause
filament
aggregation
.
The
hypothesis
is
that
disease-causing
mutations
in
IF
proteins
and
their
subsequent
characteristic
histopathological
aggregates
could
involve
caspases
.
GFAP
(
glial
fibrillary
acidic
protein
)
,
a
closely
related
IF
protein
expressed
mainly
in
astrocytes
,
is
also
a
putative
caspase
substrate
.
Mutations
in
GFAP
cause
AxD
(
Alexander
disease
)
.
The
overexpression
of
wild-
type
or
mutant
GFAP
promotes
cytoplasmic
aggregate
formation
,
with
caspase
activation
and
GFAP
proteolysis
.
In
this
study
,
we
report
that
GFAP
is
cleaved
specifically
by
caspase
6
at
VELD
²²âµ
in
its
L
12
linker
domain
in
vitro
.
Caspase
cleavage
of
GFAP
at
Asp
²²âµ
produces
two
major
cleavage
products
.
While
the
C-
GFAP
(
C-
terminal
GFAP
)
is
unable
to
assemble
into
filaments
,
the
N-
GFAP
(
N-
terminal
GFAP
)
forms
filamentous
structures
that
are
variable
in
width
and
prone
to
aggregation
.
The
effect
of
N-
GFAP
is
dominant
,
thus
affecting
normal
filament
assembly
in
a
way
that
promotes
filament
aggregation
.
Transient
transfection
of
N-
GFAP
into
a
human
astrocytoma
cell
line
induces
the
formation
of
cytoplasmic
aggregates
,
which
also
disrupt
the
endogenous
GFAP
networks
.
In
addition
,
we
generated
a
neo-epitope
antibody
that
recognizes
caspase-cleaved
but
not
the
intact
GFAP
.
Using
this
antibody
,
we
demonstrate
the
presence
of
the
caspase-generated
GFAP
fragment
in
transfected
cells
expressing
a
disease-causing
mutant
GFAP
and
in
two
mouse
models
of
AxD
.
These
findings
suggest
that
caspase-mediated
GFAP
proteolysis
may
be
a
common
event
in
the
context
of
both
the
GFAP
mutation
and
excess
.
Diseases
Validation
Diseases presenting
"cytoplasmic aggregate formation"
symptom
alexander disease
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