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Delayed fibrin elimination from the lungs of burned rats with endogenous inhibition of the fibrinolytic system
THROMBOSIS RESEARCH Printed in the United
DELAYED RATS
FIBRIN
WITH
vo1.2, pp. Pergamon
States
ELIMINATION
ENDOGENOUS
FROM
INHIBITION
THE OF
LUNGS
THE
365-376,
Press,
OF
1973
Inc.
BURNED
FIBRINOLYTIC
SYSTEM
L. Bagge, Department
C.
Busch,
of Forensic
(Received
L.
Rammer
Medicine,
8.2.1973; Accepted by
and T.
University
in revised Editor P.
Saldeen
of Uppsala,
Sweden
form 28.3.1973. Olsson)
ABSTRACT The elimination of fibrin from the lungs of burned rats with endogenous inhibition of the fibrinolytic system was studied after intravenous injection of thrombin. The fibrin content using labelled fibrinogen and alof the lungs was quantified, bumin. It was found that in burned rats the elimination of fibrin from the lungs was delayed. The lungs of these rats showed micro-atelectases which were more numerous than in rats without fibrinolysis inhibition.
INTRODUCTION Micro-emboli vessels
of patients
(1, 2, 3). damage
containing
fibrin
dying from
The assumption were closely
was supported
A retarding elimination
post-traumatic
that the occurrence
correlated
by the frequent
the blood of these
are frequently
patients
in the pulmonary
pulmonary of fibrin
insufficiency
and the pulmonary
to the state of the fibrinolytic finding of marked
fibrinolysis
system
(l),
inhibition
in
( 3, 4).
effect of an exogenous of intravascular
the development
observed
of pulmonary
inhibition
fibrin from damage
365
of fibrinolysis
upon the rate of
the lungs - and consequently
- has been demonstrated
upon
in animal
366
FIBRIN
experiments lysis
has,
(5,
6, 7).
however,
disappearance fibrinolysis
The
inhibition
ned by a quantitative The study also fibrinogen
effect
from
(48 hours method,
includes
using labelled
Stockholm)
animals. weighing
access
Under
of fibrino-
study the rate of
during the phase of
injury)
fibrinogen
( 8 ) was
ad
of the validities
albumin
exami-
(9).
of human and rat
for this method.
Experimental
Thermal
inhibition
rats
after the thermal
a comparison
Vo1.2,~0.4
In the present
the lungs of burned
MATERIAL
free
of the endogenous
not been investigated.
of fibrin
FROM LUNGS
ELIMINATION
AND
50 female
METHODS
Sprague-Dawley
200 + 5 g were used.
to tap water and food (Ewos
injury.
The method
ether anaesthesia produced
has
been
which
surface
but did not lead to death.
animals
allowed
in detail previously
immersed
a third-degree
were
Farm,
rat pellets). described
the rats were
seconds
The
rats (Anticimex
scald
Control
in water at,90°C
covering
rats were
(8).
for
20
14 % of the body
clipped
and immersed
in water at 38OC. Labelled
fibrinogen.
Blomback 0.
Tangen,
(11)s
Human
and Blomback
(10 ),
AB Pharmacia),
were used.
fibrinogen
and rat fibrinogen prepared
The fibrinogen
using an electrolytic
iodination
until use,
after
labelling,
bility
of 87 %.
(Dowex 1 - X8, iodide.
while
method
The
fibrinogen
50-100
Twenty-four
mesh)
ml and 5 pCi/ml
stable.
The
(about 9 pCi/ml
a tail vein under ether anaesthesia.
for
to
by dr.
human fibrinogen
Both preparations
before
was calculawas
was used immediately had a coagula-
an ion-exchange
injection,
the thrombin
solution,
(kindly supplied
The iodination
was run through
hours before
body weight of the fibrinogen
(12).
fibrinogen.
shortly
according
to Straugn och Wagner 125 I, in our laboratory with
the rat fibrinogen
since it was less
prepared
according
was labelled
ted to be about 0. 5 atoms/molecule freeze-dried
(AB Kabi),
containing
to eliminate
infusion,
0.25
about 0.8
the rat fibrinogen)
column
mg
free
ml/l00
g
protein/
was injected
into
FIBRIN
vo1.2,~0.4
Thrombin
injection.
ved in saline weight tail
vein
siliconized
albumin. serum
Sweden). to injection.
0.5
was
tubes
for
and the lungs cleaned
Radioactivity
spectrometer channels
obtained
counted
exactly
paper
and all the
ether
collected
(about (13 ).
1 ml),
The
free
column
mg
prior
protein/ml
anaesthesia
an 18-
at the bifurcation
in plastic triple
thoracic
dissected.
with
sacrifice.
into the aorta
was
removed,
Ellermann
microhaemato-
cavity from
was
opened
connective
tissue,
and weighed.
I and
Weighed
samples
in the plastic Autowell
131
for
samples
This
II).
contained
blood tubes
was
between
and dissol-
in a gamma-
equipped
and with digital
crossover
radionuclide.
of lungs,
Ellermann
I respectively
corrected
to the lower
with pre-
Studsvik,
0.2
before
Under
Blood
Nuclear,
were
g body
determined
an ion-exchange
5 minutes
introduced
measured
125
dissol-
into a
pump
was
containing
samples.
was
rapidly
(Picker
was
anaesthesia
I (AB Atomenergi,
solution
measurement
were
set for
the higher
saline
measurements.
ved fibrinogen
values
of a
determinations
with filter
ether
II B infusion
run through
abdomen.
were
Roche)
NIH units/100
of the lungs
131
with
was
needle
and fibrinogen
Unita
volume
labelled
radioactivity
under
a Braun
and organ
the opened
Twenty-five
injected
plasma
injected
of blood
siliconized
through
crit
ml
8 ,
367
syringes.
preparation
and 13 pCi/ml
gauge
The
albumin
The
Collection
using
FROM LUNGS
(Topostasin
injection. were
in 5 minutes,
Labelled
thrombin
before
of saline
cision-ground
human
Bovine
shortly
in 1 ml
ELIMINATION
with two
recording.
The
theho
channels
counts
were
More
than 3,000
more
than 10 times
from
always
the background
radioactivity. Calculations. been
described
groups,
The method
of calculating
in a previous
the amount
of fibrin
F=
paper
(9 ).
in the lungs
-
1
Q
(T -
the fibrin For
each
(F,
mg/g)
P -
EVc),
content
in the lungs
has
rat in the experimental was
calculated
as:
FIBRIN
368
ELIMINATION
vo1.2,~0,4
FROM LUNGS
where
Q
is the factor
sisting
of the mean
@asma
fibrinogen
is the total
P
is the plasma
relative
specific
in control
125
T
125
125
for converting
I in the plasma
into mg of fibrin,
radioactivity
(cpm x 103/mg)
conof
rats,
I radioactivity/g
125
I radioactivity
tissue,
I radioactivity/g
tissue,
and the organ plasma
calculated
volume
as the product
of
131 I ratio),
(=organ/plasma
and 125
is the extravascular
EVC
the induction
of intravascular
as the mean difference
I radioactivity/g coagulation
between
tissue,
(saline
calculated
infused
before
into control rats) 125 I radioactivity
the total and the plasma
of the organ.
The
1251 and
13’I radioactivities
in plasma
activity
were calculated 125 I radioactivity
in blood/(l-haematocrit), and the 125 I in plasma and fibrinogen. the difference between the concentrations citrate
were corrected
in serum
as
The fibrinogen
of haematocrit
upon the
dilution of plasma.
For the statistical
evaluation
Morphological
examination.
fixed material
were
PTAH
for
method
Experimental
the thrombin min 5 minutes
Labelled
respectively instead
before
paraffin
fibrinogen
of thrombin.
sections of formalinand by Mallory’s
and thrombin injury.
Groups
5 and 35 minutes
All the animals death.
was used,
of fibrin.
after the thermal
measurements
injection.
p. thick
Student’s t-test
with haematoxylin-eosin
the demonstration
with saline
for radioactivity
of the results, Five
stained
procedure.
24 and 48 hours infused
for the influence
as the radio-
were
were
Control
of rats were
injected
rats
were
sacrificed
after the termination
injected
with labelled
of
albu-
FIBRIN
ELIMINATION
369
FROM LUNGS
RESULTS The
results
are
the termination found the
shown
of the thrombin
in the lungs same
in Tables
I and
II and Fig.
injection,
of normal
and burned
human
rat fibrinogen
whether
or
equal rats
Findings
in the Groups
Five
amounts
a
Fibrinogen,
E p” I
Cpm
5 a
Lung,
cpm
Lung,
mg
of fibrin
(p > 0.1).
The
injected
with labelled
0’
5’
n
3
5
x 103/mg
plasma
fibrinogen
x 103/g
3. 51 t 14.7
0.24
r 3.7
12. 8 2
fibrin/g
were
results
were
Rat Fibrinogen,
Thrombin
T
mg/ml
after
I
Controls
a
minutes
was used.
TABLE Experirtnental Mean - S. D.
1.
1.7
0
1.74
i
35’ 6 0.50
1.50
1.9
15. 6 :
105. 6 :
20.2
24.1
4. 8 ?
1. 0
0.70:
16.4 :
+ 0. 55 5. 8
-t 14, 2 0.68
_-_---_--_-_-_---~-~_~~~_~~_~~__~--~-~~~-~_~~_~~_-~__-_-----------_-_-_____--____--~-~~~-~_~~_~~__~--~--~~-~~~~_~~_-~~_-_---------_-n a Q) c ;
Fibrinogen, Cpm
3
mg/ml
x 103/mg
plasma
fibrinogen
10. 61 :
4 1. 69
5.8
+ 0. 8
9.8
t
7.91
4
+ 0.13
6. 53 + 0. 83
5. 5 t 0. 6
5.7
f 0. 5
43. 8 2 23.8
44.9:
13.0
a Lung,
cpm
Lung,
mg
x 103/g fibrin/g
0
2.2
5.5
:
3.3
6.2t
2.9
FIBRIN
370
ELIMINATION
TABLE Experimental nogen. Mean
indings F - S. D.
in the Groups
vo1.2,~0.4
FROM LUNGS
II
injected
with labelled
Controls
a al
Fibrinogen,
0’
5’
n
3
4
plasma
4.03
: 0.37
Fibri-
Thrombin
T
mg/ml
human
35’ 4
1.66:
0.44
7.4:
1.2
7.3:
2.3
49. 5 + 3.4
7.8
t 4.3
0.64:
0. 50
E :
Cpm x 103/mg
fibrinogen
$ z
Lung,
cpm
Lung,
mg fibrin/g
x 103/g
9. 6 2 0.7 5.3
+ 0. 3 0
5. 5 t
1. 2
0.53
+ 0.59
~-~-~___-_-_-_--~-----~-~_-_------------_--___-___-_-_______-_____ -_---_____-_-_----~~~-~-~_-_--~------_--~_-_______-_-_-_-----_____ n a
Fibrinogen,
2 2 p9
Cpm
3
mg/ml
x 103/mg
plasma
fibrinogen
Lung,
cpm
x 103/g
Lung,
mg fibrin/g
-
9.81
2 0.74
2.8
+ 0.6
3. 6 2 0.7 0
5 7.80: 2.2
6 1.40
+ 0.45
2.8
+ 0.2
22.3
2 9.4
7.3
: 3.9
+O.l
19.8 2 8.3 6.6:
6.67
3.3
Non-burned rats ‘- -
Burned rats
8-
F 3
6-
FIG. /
1
The amount of fibrin in the lung after thrombin infusion in rats injected with labelled rat fibrinogen. Mean
+ L S. D.
FIBRIN
vo1.2,~0.4
In the non-burned considerably burned
reduced
rats
(p -
0. 001).
nogen
was
PTAH
killed
of fibrin
had a significantly
higher
Similar
results
sections
injection.
at the 35-minute the lungs numerous
were
Lung
after
the thrombin
was bund. fibrin
obtained
showed
from
vessels
It was, interval. small
in the burned
both normal
At this
content
injection,
time
a
point
the
than the normal
whether
human
and burned
rats
of burned staining.
rat,
2) at the
(Fig.
infrequent
however,
In the rats killed atelectases rats
in both
(Fig.
or
rats
rat fibri-
showing
fibrin
showed
two intervals
groups,
after
in the non-burned
at the 350minute but these
fibrin the rats
interval, were
more
3).
FIG. PTAH
371
FROM LUNGS
used.
in the pulmonary
thrombin
35 minutes
amount
-stained
located
rats
ELIMINATION
2
deposits
in medium-sized
arteriole.
lI'lBl
372
FIG. Lung of burned staining.
Tables
rat,
showing
I and II also
the plasma
in the various
fibrinogen.
The
to a higher
concentration
the thrombin the human
spread
show the relative
fibrinogen
burned rats
but non-significant
wide
micro-atelectasis.
specific groups
radioactivity
specific
fibrinogen.
in the relative
PTAH
(cpm/mg)
of
of rats given human or rat
showed a lower
of nonalabelled
decrease
infusion
3
specific
radioactivity, There
was a slight
radioactivity
both for the rat and - a little more
due
after
pronounced-
for
fibrinogen.
DISCUSSION Fibrin (5).
is eliminated In the present
surprisingly investigation
rapidly
from
a considerably
tion rate in the lungs was found after thermal
the lungs of normal reduced injury.
fibrin
rats
elimina-
FIBRIN
vo1.2,~0.4
The
burned
rats
inhibition
after
ministration
trauma
from
reduction
nolysis The
rat
in the lung
it has
( 5,
LUNGS
previously
been
6 ), it seems
reasonable
rate
in the burned
fibrinolysis
shown
markedly
elimination
373
of endogenous
inhibitors
examic
injection
acid),
that
delays
the ad-
the fibrin
to assume
rats
seems
the lungs
(14).
was
that
due to fibri-
to be mainly
burned
plasminogen
study
we
rise
in plasma
to a similar
results
have
found
responsible
for
the
increase
(tran-
in fibrin
re-
in the
inhibitors
fibrin
the
in plasmino-
to that
activation
impaired
that
inhibitor
equivalent
in plasminogen
(uroki-
activators
in a retardation
at least
of
bur-
thus
elimination
in the
rats.
conceivable
contributory
burned
rats
ments,
however, was
upon
RES
prolonged
coagulation
cause
of the
burned
and
non-burned the fact
5 to 35 minutes against
this
A third
possible
fibrin
rats
that
was
in the
experi-
administered
from
plays
elimination
In previous
of intravenously
probably
the
lung
a negligible
role
trypan
in the in this
rat
( 6)
res-
model. burned
in the
between
rats
fibrin
at the later
no difference
seen
fibrin
(15 ).
elimination
in the
difference
activity
effect
experimental
butory
lungs
the
inhibition
present
of the delayed
of the RES
no significant
observed
in the
However,
cause
is a reduction
and therefore
More
the
consists
activation
plasminogen-activation
giving
increase
post-burn
of plasminogen
In a recent
of a magnitude
The
2 days
whereas
of a synthetic
inhibition
rats
inhibitors
(8).
in an amount
from rats
in the
not changed
gen-activation moval
in the burned
and in antiplasmin,
are
intravenous
the
lung
increases
inhibitors)
pect
As
in the phase
fibrinolysis
inhibition
twofold
blue
( 8).
in fibrin
fibrinolysis
nase
One
the
were
FROM
inhibition.
about
ned
study
of synthetic
elimination the
in this
ELIMINATION
content
interval
in the the
is another of the
after
consumption
burned
possible lungs
contribetween
the thrombininfusion. of fibrinogen
and non-burned
rats
from argues
possibility.
in the
contributory burned
rats.
cause No
may
reduction
be a reduced in blood
flow
blood
flow
through
through the
liver
FIBRIN
374
in mice
(15)
or through
period,
but pulmonary
the kidneys blood
The increase
in the number
ned rats may
be explained
vascular
fibrin
deposits
administration
duced
Recently
impaired
to occur
in rats
inhibition for
In this
study the
quantification
slight
2 days
ted for
effect
of the lungs
to the intra-
been shown that the
in rats
changes
(17)
and dogs
in the lungs
after
may
be a factor
deposition
in organs
in-
that the radioactivity
radioactivity
from
(cpm/mg)
decrease
of fibrin
point of view,
human fibrinogen
may
also
It
quite
similarly.
showed
that both fibrinogens
tolerates
The
concentrations
by the method
both
after are
used.
is preferable,
a
sui-
From
a
but,
freeze-drying,
as
is not
as was shown in the present
be used,
the
of the two fibrinogens
of rat fibrinogen which
for
was compared.
of the two fibrinogens
in organs
rat fibrinogen,
of importance
method
the lungs
appears
the use
that the
and rat fibrinogen
at low fibrinogen
It therefore
been shown
in the kidneys.
by the present
eliminated
has also
and it is thus possible
in the use of human
I and II)
infusion.
in the kidneys
system
reliability
as a satisfactory
available,
of the bur-
inhibitors
a burn (18),
of fibrin
the quantification
theoretical long
after
but non-significant
the thrombin
as far as we know.
in the lungs
It has earlier
fibrinolysis
elimination
in and were
specific
studied
exposure
the morphological
fibrin
was found (Tables
relative
(16) is seen in this post-burn
not been
rats.
vo1.2,No.k
LUNGS
coagulation.
of fibrin
accumulated
has
in these
of the fibrinolytic
the injurious
in rats
by the longer
increases
intravascular
flow
FROM
of micro-atelectases
of synthetic
(7 ) markedly
ELIMINATION
in-
vestigation.
Aknowledgements Supported
by grants
40X-2035-08B), macia.
from
the Swedish
the Torsten
Medical
and Ragnar
Research
Sbderberg
Council
foundation
(No B73-
and AB
Phar-
FIBRIN
ELIMINATION
375
FROM LUNGS
References
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2.
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1967.
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insuffi-
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Experimental
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Saldeen,
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545-549,
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360-371,
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).
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FIBRIN
376
ELIMINATION
FROM LUNGS
Vo1.2,~0.4
14.
Bagge, L., Rammer, L. and Saldeen, T. Experimental investiga tion concerning the importance of inhibition of plasminogen activation for the delayed post-traumatic elimination of intravascular fibrin. In press. Forens. Sci.
15.
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elimination
in the
DELAYED RATS
FIBRIN
WITH
vo1.2, pp. Pergamon
States
ELIMINATION
ENDOGENOUS
FROM
INHIBITION
THE OF
LUNGS
THE
365-376,
Press,
OF
1973
Inc.
BURNED
FIBRINOLYTIC
SYSTEM
L. Bagge, Department
C.
Busch,
of Forensic
(Received
L.
Rammer
Medicine,
8.2.1973; Accepted by
and T.
University
in revised Editor P.
Saldeen
of Uppsala,
Sweden
form 28.3.1973. Olsson)
ABSTRACT The elimination of fibrin from the lungs of burned rats with endogenous inhibition of the fibrinolytic system was studied after intravenous injection of thrombin. The fibrin content using labelled fibrinogen and alof the lungs was quantified, bumin. It was found that in burned rats the elimination of fibrin from the lungs was delayed. The lungs of these rats showed micro-atelectases which were more numerous than in rats without fibrinolysis inhibition.
INTRODUCTION Micro-emboli vessels
of patients
(1, 2, 3). damage
containing
fibrin
dying from
The assumption were closely
was supported
A retarding elimination
post-traumatic
that the occurrence
correlated
by the frequent
the blood of these
are frequently
patients
in the pulmonary
pulmonary of fibrin
insufficiency
and the pulmonary
to the state of the fibrinolytic finding of marked
fibrinolysis
system
(l),
inhibition
in
( 3, 4).
effect of an exogenous of intravascular
the development
observed
of pulmonary
inhibition
fibrin from damage
365
of fibrinolysis
upon the rate of
the lungs - and consequently
- has been demonstrated
upon
in animal
366
FIBRIN
experiments lysis
has,
(5,
6, 7).
however,
disappearance fibrinolysis
The
inhibition
ned by a quantitative The study also fibrinogen
effect
from
(48 hours method,
includes
using labelled
Stockholm)
animals. weighing
access
Under
of fibrino-
study the rate of
during the phase of
injury)
fibrinogen
( 8 ) was
ad
of the validities
albumin
exami-
(9).
of human and rat
for this method.
Experimental
Thermal
inhibition
rats
after the thermal
a comparison
Vo1.2,~0.4
In the present
the lungs of burned
MATERIAL
free
of the endogenous
not been investigated.
of fibrin
FROM LUNGS
ELIMINATION
AND
50 female
METHODS
Sprague-Dawley
200 + 5 g were used.
to tap water and food (Ewos
injury.
The method
ether anaesthesia produced
has
been
which
surface
but did not lead to death.
animals
allowed
in detail previously
immersed
a third-degree
were
Farm,
rat pellets). described
the rats were
seconds
The
rats (Anticimex
scald
Control
in water at,90°C
covering
rats were
(8).
for
20
14 % of the body
clipped
and immersed
in water at 38OC. Labelled
fibrinogen.
Blomback 0.
Tangen,
(11)s
Human
and Blomback
(10 ),
AB Pharmacia),
were used.
fibrinogen
and rat fibrinogen prepared
The fibrinogen
using an electrolytic
iodination
until use,
after
labelling,
bility
of 87 %.
(Dowex 1 - X8, iodide.
while
method
The
fibrinogen
50-100
Twenty-four
mesh)
ml and 5 pCi/ml
stable.
The
(about 9 pCi/ml
a tail vein under ether anaesthesia.
for
to
by dr.
human fibrinogen
Both preparations
before
was calculawas
was used immediately had a coagula-
an ion-exchange
injection,
the thrombin
solution,
(kindly supplied
The iodination
was run through
hours before
body weight of the fibrinogen
(12).
fibrinogen.
shortly
according
to Straugn och Wagner 125 I, in our laboratory with
the rat fibrinogen
since it was less
prepared
according
was labelled
ted to be about 0. 5 atoms/molecule freeze-dried
(AB Kabi),
containing
to eliminate
infusion,
0.25
about 0.8
the rat fibrinogen)
column
mg
free
ml/l00
g
protein/
was injected
into
FIBRIN
vo1.2,~0.4
Thrombin
injection.
ved in saline weight tail
vein
siliconized
albumin. serum
Sweden). to injection.
0.5
was
tubes
for
and the lungs cleaned
Radioactivity
spectrometer channels
obtained
counted
exactly
paper
and all the
ether
collected
(about (13 ).
1 ml),
The
free
column
mg
prior
protein/ml
anaesthesia
an 18-
at the bifurcation
in plastic triple
thoracic
dissected.
with
sacrifice.
into the aorta
was
removed,
Ellermann
microhaemato-
cavity from
was
opened
connective
tissue,
and weighed.
I and
Weighed
samples
in the plastic Autowell
131
for
samples
This
II).
contained
blood tubes
was
between
and dissol-
in a gamma-
equipped
and with digital
crossover
radionuclide.
of lungs,
Ellermann
I respectively
corrected
to the lower
with pre-
Studsvik,
0.2
before
Under
Blood
Nuclear,
were
g body
determined
an ion-exchange
5 minutes
introduced
measured
125
dissol-
into a
pump
was
containing
samples.
was
rapidly
(Picker
was
anaesthesia
I (AB Atomenergi,
solution
measurement
were
set for
the higher
saline
measurements.
ved fibrinogen
values
of a
determinations
with filter
ether
II B infusion
run through
abdomen.
were
Roche)
NIH units/100
of the lungs
131
with
was
needle
and fibrinogen
Unita
volume
labelled
radioactivity
under
a Braun
and organ
the opened
Twenty-five
injected
plasma
injected
of blood
siliconized
through
crit
ml
8 ,
367
syringes.
preparation
and 13 pCi/ml
gauge
The
albumin
The
Collection
using
FROM LUNGS
(Topostasin
injection. were
in 5 minutes,
Labelled
thrombin
before
of saline
cision-ground
human
Bovine
shortly
in 1 ml
ELIMINATION
with two
recording.
The
theho
channels
counts
were
More
than 3,000
more
than 10 times
from
always
the background
radioactivity. Calculations. been
described
groups,
The method
of calculating
in a previous
the amount
of fibrin
F=
paper
(9 ).
in the lungs
-
1
Q
(T -
the fibrin For
each
(F,
mg/g)
P -
EVc),
content
in the lungs
has
rat in the experimental was
calculated
as:
FIBRIN
368
ELIMINATION
vo1.2,~0,4
FROM LUNGS
where
Q
is the factor
sisting
of the mean
@asma
fibrinogen
is the total
P
is the plasma
relative
specific
in control
125
T
125
125
for converting
I in the plasma
into mg of fibrin,
radioactivity
(cpm x 103/mg)
conof
rats,
I radioactivity/g
125
I radioactivity
tissue,
I radioactivity/g
tissue,
and the organ plasma
calculated
volume
as the product
of
131 I ratio),
(=organ/plasma
and 125
is the extravascular
EVC
the induction
of intravascular
as the mean difference
I radioactivity/g coagulation
between
tissue,
(saline
calculated
infused
before
into control rats) 125 I radioactivity
the total and the plasma
of the organ.
The
1251 and
13’I radioactivities
in plasma
activity
were calculated 125 I radioactivity
in blood/(l-haematocrit), and the 125 I in plasma and fibrinogen. the difference between the concentrations citrate
were corrected
in serum
as
The fibrinogen
of haematocrit
upon the
dilution of plasma.
For the statistical
evaluation
Morphological
examination.
fixed material
were
PTAH
for
method
Experimental
the thrombin min 5 minutes
Labelled
respectively instead
before
paraffin
fibrinogen
of thrombin.
sections of formalinand by Mallory’s
and thrombin injury.
Groups
5 and 35 minutes
All the animals death.
was used,
of fibrin.
after the thermal
measurements
injection.
p. thick
Student’s t-test
with haematoxylin-eosin
the demonstration
with saline
for radioactivity
of the results, Five
stained
procedure.
24 and 48 hours infused
for the influence
as the radio-
were
were
Control
of rats were
injected
rats
were
sacrificed
after the termination
injected
with labelled
of
albu-
FIBRIN
ELIMINATION
369
FROM LUNGS
RESULTS The
results
are
the termination found the
shown
of the thrombin
in the lungs same
in Tables
I and
II and Fig.
injection,
of normal
and burned
human
rat fibrinogen
whether
or
equal rats
Findings
in the Groups
Five
amounts
a
Fibrinogen,
E p” I
Cpm
5 a
Lung,
cpm
Lung,
mg
of fibrin
(p > 0.1).
The
injected
with labelled
0’
5’
n
3
5
x 103/mg
plasma
fibrinogen
x 103/g
3. 51 t 14.7
0.24
r 3.7
12. 8 2
fibrin/g
were
results
were
Rat Fibrinogen,
Thrombin
T
mg/ml
after
I
Controls
a
minutes
was used.
TABLE Experirtnental Mean - S. D.
1.
1.7
0
1.74
i
35’ 6 0.50
1.50
1.9
15. 6 :
105. 6 :
20.2
24.1
4. 8 ?
1. 0
0.70:
16.4 :
+ 0. 55 5. 8
-t 14, 2 0.68
_-_---_--_-_-_---~-~_~~~_~~_~~__~--~-~~~-~_~~_~~_-~__-_-----------_-_-_____--____--~-~~~-~_~~_~~__~--~--~~-~~~~_~~_-~~_-_---------_-n a Q) c ;
Fibrinogen, Cpm
3
mg/ml
x 103/mg
plasma
fibrinogen
10. 61 :
4 1. 69
5.8
+ 0. 8
9.8
t
7.91
4
+ 0.13
6. 53 + 0. 83
5. 5 t 0. 6
5.7
f 0. 5
43. 8 2 23.8
44.9:
13.0
a Lung,
cpm
Lung,
mg
x 103/g fibrin/g
0
2.2
5.5
:
3.3
6.2t
2.9
FIBRIN
370
ELIMINATION
TABLE Experimental nogen. Mean
indings F - S. D.
in the Groups
vo1.2,~0.4
FROM LUNGS
II
injected
with labelled
Controls
a al
Fibrinogen,
0’
5’
n
3
4
plasma
4.03
: 0.37
Fibri-
Thrombin
T
mg/ml
human
35’ 4
1.66:
0.44
7.4:
1.2
7.3:
2.3
49. 5 + 3.4
7.8
t 4.3
0.64:
0. 50
E :
Cpm x 103/mg
fibrinogen
$ z
Lung,
cpm
Lung,
mg fibrin/g
x 103/g
9. 6 2 0.7 5.3
+ 0. 3 0
5. 5 t
1. 2
0.53
+ 0.59
~-~-~___-_-_-_--~-----~-~_-_------------_--___-___-_-_______-_____ -_---_____-_-_----~~~-~-~_-_--~------_--~_-_______-_-_-_-----_____ n a
Fibrinogen,
2 2 p9
Cpm
3
mg/ml
x 103/mg
plasma
fibrinogen
Lung,
cpm
x 103/g
Lung,
mg fibrin/g
-
9.81
2 0.74
2.8
+ 0.6
3. 6 2 0.7 0
5 7.80: 2.2
6 1.40
+ 0.45
2.8
+ 0.2
22.3
2 9.4
7.3
: 3.9
+O.l
19.8 2 8.3 6.6:
6.67
3.3
Non-burned rats ‘- -
Burned rats
8-
F 3
6-
FIG. /
1
The amount of fibrin in the lung after thrombin infusion in rats injected with labelled rat fibrinogen. Mean
+ L S. D.
FIBRIN
vo1.2,~0.4
In the non-burned considerably burned
reduced
rats
(p -
0. 001).
nogen
was
PTAH
killed
of fibrin
had a significantly
higher
Similar
results
sections
injection.
at the 35-minute the lungs numerous
were
Lung
after
the thrombin
was bund. fibrin
obtained
showed
from
vessels
It was, interval. small
in the burned
both normal
At this
content
injection,
time
a
point
the
than the normal
whether
human
and burned
rats
of burned staining.
rat,
2) at the
(Fig.
infrequent
however,
In the rats killed atelectases rats
in both
(Fig.
or
rats
rat fibri-
showing
fibrin
showed
two intervals
groups,
after
in the non-burned
at the 350minute but these
fibrin the rats
interval, were
more
3).
FIG. PTAH
371
FROM LUNGS
used.
in the pulmonary
thrombin
35 minutes
amount
-stained
located
rats
ELIMINATION
2
deposits
in medium-sized
arteriole.
lI'lBl
372
FIG. Lung of burned staining.
Tables
rat,
showing
I and II also
the plasma
in the various
fibrinogen.
The
to a higher
concentration
the thrombin the human
spread
show the relative
fibrinogen
burned rats
but non-significant
wide
micro-atelectasis.
specific groups
radioactivity
specific
fibrinogen.
in the relative
PTAH
(cpm/mg)
of
of rats given human or rat
showed a lower
of nonalabelled
decrease
infusion
3
specific
radioactivity, There
was a slight
radioactivity
both for the rat and - a little more
due
after
pronounced-
for
fibrinogen.
DISCUSSION Fibrin (5).
is eliminated In the present
surprisingly investigation
rapidly
from
a considerably
tion rate in the lungs was found after thermal
the lungs of normal reduced injury.
fibrin
rats
elimina-
FIBRIN
vo1.2,~0.4
The
burned
rats
inhibition
after
ministration
trauma
from
reduction
nolysis The
rat
in the lung
it has
( 5,
LUNGS
previously
been
6 ), it seems
reasonable
rate
in the burned
fibrinolysis
shown
markedly
elimination
373
of endogenous
inhibitors
examic
injection
acid),
that
delays
the ad-
the fibrin
to assume
rats
seems
the lungs
(14).
was
that
due to fibri-
to be mainly
burned
plasminogen
study
we
rise
in plasma
to a similar
results
have
found
responsible
for
the
increase
(tran-
in fibrin
re-
in the
inhibitors
fibrin
the
in plasmino-
to that
activation
impaired
that
inhibitor
equivalent
in plasminogen
(uroki-
activators
in a retardation
at least
of
bur-
thus
elimination
in the
rats.
conceivable
contributory
burned
rats
ments,
however, was
upon
RES
prolonged
coagulation
cause
of the
burned
and
non-burned the fact
5 to 35 minutes against
this
A third
possible
fibrin
rats
that
was
in the
experi-
administered
from
plays
elimination
In previous
of intravenously
probably
the
lung
a negligible
role
trypan
in the in this
rat
( 6)
res-
model. burned
in the
between
rats
fibrin
at the later
no difference
seen
fibrin
(15 ).
elimination
in the
difference
activity
effect
experimental
butory
lungs
the
inhibition
present
of the delayed
of the RES
no significant
observed
in the
However,
cause
is a reduction
and therefore
More
the
consists
activation
plasminogen-activation
giving
increase
post-burn
of plasminogen
In a recent
of a magnitude
The
2 days
whereas
of a synthetic
inhibition
rats
inhibitors
(8).
in an amount
from rats
in the
not changed
gen-activation moval
in the burned
and in antiplasmin,
are
intravenous
the
lung
increases
inhibitors)
pect
As
in the phase
fibrinolysis
inhibition
twofold
blue
( 8).
in fibrin
fibrinolysis
nase
One
the
were
FROM
inhibition.
about
ned
study
of synthetic
elimination the
in this
ELIMINATION
content
interval
in the the
is another of the
after
consumption
burned
possible lungs
contribetween
the thrombininfusion. of fibrinogen
and non-burned
rats
from argues
possibility.
in the
contributory burned
rats.
cause No
may
reduction
be a reduced in blood
flow
blood
flow
through
through the
liver
FIBRIN
374
in mice
(15)
or through
period,
but pulmonary
the kidneys blood
The increase
in the number
ned rats may
be explained
vascular
fibrin
deposits
administration
duced
Recently
impaired
to occur
in rats
inhibition for
In this
study the
quantification
slight
2 days
ted for
effect
of the lungs
to the intra-
been shown that the
in rats
changes
(17)
and dogs
in the lungs
after
may
be a factor
deposition
in organs
in-
that the radioactivity
radioactivity
from
(cpm/mg)
decrease
of fibrin
point of view,
human fibrinogen
may
also
It
quite
similarly.
showed
that both fibrinogens
tolerates
The
concentrations
by the method
both
after are
used.
is preferable,
a
sui-
From
a
but,
freeze-drying,
as
is not
as was shown in the present
be used,
the
of the two fibrinogens
of rat fibrinogen which
for
was compared.
of the two fibrinogens
in organs
rat fibrinogen,
of importance
method
the lungs
appears
the use
that the
and rat fibrinogen
at low fibrinogen
It therefore
been shown
in the kidneys.
by the present
eliminated
has also
and it is thus possible
in the use of human
I and II)
infusion.
in the kidneys
system
reliability
as a satisfactory
available,
of the bur-
inhibitors
a burn (18),
of fibrin
the quantification
theoretical long
after
but non-significant
the thrombin
as far as we know.
in the lungs
It has earlier
fibrinolysis
elimination
in and were
specific
studied
exposure
the morphological
fibrin
was found (Tables
relative
(16) is seen in this post-burn
not been
rats.
vo1.2,No.k
LUNGS
coagulation.
of fibrin
accumulated
has
in these
of the fibrinolytic
the injurious
in rats
by the longer
increases
intravascular
flow
FROM
of micro-atelectases
of synthetic
(7 ) markedly
ELIMINATION
in-
vestigation.
Aknowledgements Supported
by grants
40X-2035-08B), macia.
from
the Swedish
the Torsten
Medical
and Ragnar
Research
Sbderberg
Council
foundation
(No B73-
and AB
Phar-
FIBRIN
ELIMINATION
375
FROM LUNGS
References
1.
Saldeen, sinsk 217,
2.
Om
T.
forenings
Saldeen,
Virchows.
Lindquist,
O.,
Rammer,
L.
death.
and
Saldeen,
Acta
chir.
T.
20-25,
in an autopsy
1967.
T.
Pulmonary
inhibition
Inhibition
insuffi-
in a post-trau-
138,
stand.
Diathes.
Experimental
T.
Saldeen,
T.
545-549,
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haemorrh.
) 22,
Arfors,
360-371,
1972. in post-
(Stuttg.)
24,
Busch,
C., L.
intravenous
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Stand.
J.
Busch,
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vess$s
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K. E., P.,
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berg,
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(Stuttg. 7.
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445-452,
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Rammer,
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T.
Quantitation
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).
In press. 10.
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B.
fibrinogen. 11.
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Arkiv W.
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lo,
M.
Purification
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R, M.
A simple
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198-206,
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Rosa,
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Scassle3111ati, G. A. and with I by electrolytic 86,
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519-526,
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Determination of fibrinogen and fibriDiathes. haemorrh. (Stuttg. ) 8,
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376
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FROM LUNGS
Vo1.2,~0.4
14.
Bagge, L., Rammer, L. and Saldeen, T. Experimental investiga tion concerning the importance of inhibition of plasminogen activation for the delayed post-traumatic elimination of intravascular fibrin. In press. Forens. Sci.
15.
Schildt, trauma
16.
Renal Rammer, L. effect of intravascular press.
17.
Saldeen, T. The importance of intravascular coagulation and inhibition of the fibrinolytic system in experimental fat embolism. J. Trauma, lo, 287-298, 1970.
18.
Impaired fibrin Rammer, L. and Busch, C. kidneys of burned rats. To be published.
thermal and mechanical B. Function of the RES after in mice. Acta chir. stand. 136, 359-364, 1970. function in burned rats with reference to the coagulation. Stand. J. urol. nephrol. In
elimination
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