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Studies of an activity from endothelial cells that inhibits platelet aggregation, serotonin release, and clot retraction
THROYBOSIS RESEARCH Printed in the United
Vol. States
j, pp. 747-7j7, Pergamon Press,
1974 Inc.
STUDIES OF AN ACTIVITY FROH ENDGTHELIAL CELLS THAT INHIBITS PlATELET AGGREGATION, SERCYIONINRELEASE, AND CLOT RETIUCTION
S. R. Saba and R. G. Mason Department of Pathology, University of North Carolina Chapel Hill, North Carolina 27514
(Received
4.11.1974.
Accepted
by Editor
M.I.
Barnhart)
ABSTRACT present in endothelial cells of human umbilical vein An activity origin has been found to inhibit aggregation, serotonin release, and clot retraction. This activity appears to reside in molecules of small size that can be released from in situ or isolated endothelial cells by freeze-thaw treatment or by exposure of cells to ADP, collagen, epinephrine, or thrombin. Relative amounts of inhibitory activity released from endothelial cells vary with the specific plate let aggregating agent used as release inducer and are influenced by use of in situ or isolated cells. Varying the concentration of aggre gating agent varied proportionally the amount of inhibitory activity released from in situ but not from isolated endothelial cells.
INTRODUCTION An activity of endothelial cell origin was described recently (1) that inhibited aggregation of platelets.
This activity could be released from iso-
lated endothelial cells by disruption of the cells or by treatment of cells with certain platelet aggregating agents.
A broad spectrum of action of the
inhibitory activity of endothelial cell origin was shown in that it prevented aggregation of platelets induced by adenosine diphosphate (ADP), collagen, epinephrine, or thrombin.
This inhibitory activity was shown to reside in a
small, heat labile molecule (9OoC, 10 min.). Further characterization of the inhibitory activity of endothelial cell origin has been undertaken.
Semiquantitative studies of the release of the
inhibitory activity both from endothelial cells in situ and from isolated 747
738
INHIBITOR
endothelial
cells
conducted.
The inhibitor
gation
but
to
in
FROM ENDOTHELIAL
response
prevent
to
has
various
been
release
of
found
Vol.j,No.6
CELLS
platelet
aggregating
not
to
serotonin
only
fran
agents
prevent
platelets
have
platelet
and to
been
aggre-
inhibit
clot
retraction.
MATERIALS AND METHODS Endothelial
Cells
and
Human umbilical tals
modified fic
cords
and brought
The umbilical
vein
platelet
lumen of bation
to
(!$g*+-
the in
37’C
were
in
did
obtained
a segment
Ca*+- free)
vein
preparations. from
laboratory.withfn
aggregating
the
at
Inhibitor
this
cord
and
increase
(MTS).
yield.
at
delivery.
and rinsed of
with
the
was placed
22OC for
speci-
in
the
60 minutes.
The incubated
solution
of
endothelial
cells,
was then
supernatant
was used as the inhibitor preparation in studies of platelet aggre-
ment
A control of
the
consisted
same umbilical
of cord
15OOg for
an identical vein
from
activity
Incu-
which
at
inhibitory
of
agent,
centrifuged
the
time
hospi-
aggregating
gation.
now contained
the
A solution
investigation
incubated
inhibitor
of
collaborating
was cannulated
solution
in MTS under
segment
nearby
two hours
each
Tyrode’s agent
not
of
six
15 minutes
preparation which
the
from
aggregating
released at
from
220C;
a different agent
This
control
cal
were
used after intervals greater than 2 hours post delivery or
cords
negligable
inhibitor
activity
unless
seg-
was
omitted.
contained
the
umbili-
unless traumatized cords were used in which cases detectable amounts of inhibitor were present in these controls. Endothelial cells were isolated from human umbilical cord vein by treatment of the in situ cells with 0.22 collagenase (collagenase type IV, Worthington Biochemical Corporation, Freehold, New Jersey) in MTS as previously reported (1).
Isolated endothelial cells were washed two times in FITSand fin-
ally resuspended
in &fTS at
a final
concentration
of
approximately 1000 cells
Vol.j,No.6
per
IXHIBITOR
axa3.
sion
Isolated
test.
This
aggregating ture not
cells cell
agent
in )ITS and
of
agent
platelet
endothelial the
negligable
in
A control
platelet
inhibitor
vein
platelet
before
the
at
centrifuged
mix-
37Oc did
endothelial
preparation
consisted
treated
was omitted.
cells is
from
isolated
serotonin
preparation
of
of
in
isolated
identically
This
control
endothelial
cells
with contained
release
was the
supernatant
in HTS centrifuged referred
to
and
as
at
clot
contraction.
frau
three
15OOg for
freeze-thaw
(,5OO/nm13)
times
frozen
15 minutes
inhibitor
at
preparation.
KTS.
or
other
Aggregation
inhibitor
preparation,
preparation,
and 3)
consisted
(1)
of
at
1,000
2)
agent
was used
from
rpm.
to
endothelial
at
least out
with
platelets/mm3) from
in
consisted
MTS substituted
which
agent.
aggregation of
for
was added
aggregating
cells
days
the
of
inhibitor
was prepared
donors
prior
a Chrono-log
MTS substituted
induce
normal
seven
Controls
PRP to
ml of
(500,000
obtained
carried
with
ml of
and 0.1
release
blood
mixtures
mixtures 0.2
(PRP)
for
were
ml KrS,
aggregating
from
medication
studies
PRP stirred
0.1
plasma
previously
37OC with
induce
as the
cord
agent
the
of
incubation
preparation
same umbilical
platelet-rich
aspirin
ture.
ation,
A control
22OC; of
also
volume
exclu-
Aggregation.
as described
Tests
was used
supernataat
Citrated
taken
mixture
B dye
15 minutes
for at
739
erythrosin
an equal
22’~
The supernatant
preparation
of
consisted
Platelet
at
15 minutes
aggregating
endothelial
This
by the
with
yield.
inhibitor
inhibitor
and thawed
incubated
CELLS
activity.
studies
second
95% viable
was mixed
15OOg for
the
the
inhibitory
was used
22Oc.
from
that
A second
80 to
aggregation.
cells
exception
This
at
inhibitor
cell-aggregating studies
were
suspension
was centrifuged increase
FROM ENDOTHELIXL
to
venipunc-
aggregometer
of:
1)
the
for
the
ml of
In each platelets activity
at
control
inhibitor
aggregating
0.1
who had not
agents.
inhibitor case,
the
prepar same
as was used tested
with
to
750
INHIBITOR
these platelets.
FRO!4 ENDOTHELIAL
CELLS
Degree of inhibition of platelet aggregation was determined
by measurement of change in % transmission (ZT) of the aggregometer and by determination of change in the total area which lay under aggregation curves; the areas under curves were cut out and weighed on an analytical balance. Amounts of aggregating agents required to produce a 75% change in %T varied with individual plasmas; ranges of concentrations are given for each aggregation-inducing agent in footnotes to Tables I and II. Release. One tenth ml of serotonin solution (9.1 X 10m6 H, specific activity of 55 m Ci/m mole of Cl4 labeled serotonin creatinine sulfate, Amersham Searle, Chicago, Illinois) was incubated with 0.9 ml PRP for 30 minutes at 37OC.
Two
tenths ml of freeze-thaw inhibitor preparation in MTS was added to 0.2 ml of labeled PRP and incubated for LO minutes before 0.1 ml of aggregating agent was added with stirring for 10 minutes.
The final mixture was centrifuged for
20 minutes at 1500g at 22OC, and the supernatant solution was counted in a Nuclear Chicago Scintillation counter with PBD in toluene as fluor. consisted of:
Controls
1) the control inhibitor preparation, 2) mixtures with MTS sub-
stituted for inhibitor preparation, and 3) mixtures with WTS substituted for aggregating agent. Clot Retraction. To 0.2 ml of PRP was added 0.2 ml of freeze-thaw inhibitor preparation in MTS.
The mixture was incubated at 37OC for one minute before 0.1 ml of
thrombin (2 units/ml) was added.
The final mixture was incubated for 90 min-
utes at 37OC before the degree of clot retraction was quantitated by gravimetric determination of the amount of extruded serum.
The control consisted
of a mixture with MTS substituted for inhibitor preparation. Reagents. ADP and epinephrine were obtained from Sigma Chemical Co., St. Louis,
INHIBITOR
Vol.5,No.6
Missouri and
FROM ENDOTHELIAL
prepared fresh in KTS each day.
Achilles tendons by the method of Hovig (2). this
Collagen was
751
prepared from h-n
One to two and
stock collagen preparation were made vith MTS.
was of bovine origin and was
CELLS
1:4
dilutions
of
Thrombin, 300 units/ml,
highly purified; this was a gift from Dr. R. L.
Lundbled, Dental Research Center, Dnivtrsity of North Carolina, Chapel Hill, North Carolina.
RESULTS Results
of
tests for the presence of inhibitory activity recovered by
incubation of endothtlial cells in situ with aggregating agents are given in Table I.
In studies with endothelial cells in situ, it was found that throm-
TABLE I Effects on Platelet Aggregation of an Agent Released from Endothtlial Cells In Situ in Response to ADP, Collagen, Epinephrint, or Thrombin
X decrease in platelet aggregation* in presence of inhibitory agent (P n * S.D.) y area under curve By%T
Aggregating agent used to induce release of inhibitor from endothtlial cells
Number Concentration of experiments
ADP
10-5 H
36.3 + 12.8
32.3 + 11.4
Collagen
1:2 dilution
11.7 +
9.2
18.2 +
6.0
1:4 dilution
7.4 +
5.1
14.7 +
8.6
Epintphrine
Thrombin
10-5 M
14.0 +, 3.3
12.1 +_ 0.2
10'6 H
11.3 +_ 0.6
8.0 +_ 1.7
1 unit/ml
75.6 + 12.6
54.0 2 19.8
0.5 unit/ml
56.7 +_ 18.5
34.2 +_ 12.1
12.4 f 2.3 13.7 f 1.5 J 0.25 unit/ml _ _ . r . ~. * Ranges of final concentrations f agents used to 1Muce aggrtgatlon or platelets were: ADP, loss to 2X 14 8n ; collagen, 1:4 dilution; tpintphrine, 1 to 2 x 10-s H; and thrombin, 0.1 to 0.2 units/ml.
INHIBITOR
752
bin released released tion
the most inhibitory
progressively
release
phr iae,
or thrombin.
reverse
the action
Results
agent of
while
amounts of
incubated
inhibitory
Addition
CELLS
ADP, epinephrine, Decreasing
inhibitor. with
endothelial
activity
of calcium
Vo1.5,No.6
in tests
the concentra-
cells with
to the reaction
and collagen
in situ
collagen,
mixtures
resulted epine-
did not
of the inhibitor
of tests
endothelial
activity
lesser
of the aggregating
in a decreased
lated
FROM ENDOTHELIAL
with
cells
inhibitory
activity
with aggregating
obtained
agents
by incubation
are shown in Table
of
iso-
II.
TABLE II Effects Endothelial
on Platelet Aggregation of an Agent Released from Isolated Cells in Response to ADP, Collagen, Epinephrine, or Thrombin
Aggregating agent used to induce release of inhibitor frcm endothelial cells
Concentration
ADP
5 x 10’5
Number
of !xper iment d
Z decrease in platelet aggregation* in presence of inhibitory agent (I !an + S.D.) By area under curve By7,T 5.6
18.9 +
4.9
10-5 M
30.4 + 15.6
23.5 +
4.5
1:2 dilution
40.7
+ 18.4
39.2 f 20.7
1:8 dilution
48.5
+, 18.6
42.7
Epinephr ine
5 x 10’7
21.0
+
7.3
23.8 +
5.4
Thrombin
0.5
5.8 +_ 3.7
11.0 +
0.9
Collagen
*
M
units/ml
0.25 units/ml 8.1 of agents used Ranges of fina concentration platelets were: ADP, 2 X loto 2 x lo-6 M; epinephrine, 10’5 to 2 X 10-6 M; thrombin, 0.2
Collagen
was found to release
aggregating Lesser
agents
amounts of
thrombin.
In teats
the
were incubated inhibitory with
+
26.0
n
largest with
activity
isolated
3.8 f 4.4 1 5.7 f to induce aggregation of collagen, 1:4 dilution; to 0.44 units/ml.
amounts of
isolated
inhibitory
endothelfal
were released
endothelial
2 13.3
cells,
cells
activity in hTS.
by ADP, epinephrine, decreasing
when
and
the concen-
I?i-HIBITOR FROM
tration
of ADP or collagen
amounts of induced tained
inhibitory
by each of
activity. the agents
from isolated
Effects platelets
is
of
slightly
shovn in Table
of
CELLS
did
not result
Similar
inhibition
tested
endothelial
the presence
ENDOTHELIAL
could
cells
in release
of
of platelet
be demonstrated
smaller aggregation
with
inhibitor
ob-
by freeze-thaw.
inhibitor
III.
753
on the release
ADP, collagen,
of
serotonin
epinephrine,
from
or thrombin
was
TABLE III Effects of the Inhibitory Serotonin from Platelets
Agent used to induce release of serotonin from platelets
Activity of Endothelial Induced by ADP, Collagen,
2 x lo-4
1
of exper intents
X inhibition of release of serote nin by inhibitor obtained from endothelial cells by freeze-thaw
X release of serotonin
Number
Concentratioc
Cell Origin on Release of Epinephrine, or Thrombin
with inhibitor
vithout inhibitor
M
50.6 5
6.6
9.1
+
9.7
82.0
1 x 10’4 M
39.7 +,
9.3
5.7 +
5.6
85.6
Collagen
1:l
66.3 + 10.1
14.6 +_ 9.1
78.0
Ep inephr ine
2 x 10’4 H
64.0 +_
7.9
0.3 +_ 0.3
99.5
1 x 10’4 M
61.8 f.
3.4
0.3 +,
0.3
99.5
1 unit/ml
86.5 +
3.9
38.8 f
13.0
55.1
0.5
77.2 f
9.5
5.1 f
6.7
93.3
ADP
Thraubin
unit/ml
used to induce
release
from endothelial
cells
percent dothellal release
serotonin cell
of
by freeze-thaw
release
origin.
serotonin
treatment.
in the absence
Results
and presence
agents
tested,
also
induced
was obtained expressed
the inhibitor inducer
of
appreciable
as of en-
serotonin release.
the amount of inhibitory activity
was sufficient to prevent 55.0 to 99.5% of the release platelets.
are
of
Thrombin was the most efficient
but ADP, epinephr ine , and collagen
With the release-inducing
Inhibitor
from platelets.
of
eerotonin
from
INHIBITORS
754
The inhibitor
of endothelial
prevention
of clot
endothelial
cells
retraction.
cell
by 58%.
centration,
500/&)
Addition
of
isolated
of clot
CELLS
was also of
the
when added
to recalcified
60X inhibition
origin
Preparations
by freeze-thawing,
retraction
mately
FROM ENDCTHELIAL
intact
titrated
Vo1.5,No.6
an efficient
inhibitor
agent
released
for
from
to titrated
PRP, reduced
clot
endothelial
cells
con-
PRP likewise
(final
resulted
in approxi-
retraction.
DISCUSSION The inhibitory potent This
agent inhibitory
cells
the
for
is
intact
of
labile
plate let
this
cells
is
tory
a broad
is
or of cell
demonstrated
inhibitor
which
activity
fragments. molecule
easily
when
contain
ADP, pre-
and the release
epinephrine,
of platelet
to the presence
of
can be
not only
retraction
by ADP, collagen,
in response
small
mixtures
clot
by exposure
The inhibitor
cells
inhibitory
prevents
spectrum
cells
cells
to be a relatively activity
and retraction.
or thrombin.
function of
and is
commonly used
agents. activity
from isolated cells
indicates
could
the cells
can be recovered
endothelial
of endothelial
activity
cubating
induced
from endothelial
endothelial treatment
endothelial
This
but also
release,
agents.
added to reaction
or thrambin.
from platelets
The inhibitory or
are
aggregation
activity
aggregating
intact
has been shown to be a
from endothelial
aggregating
Inhibitory
(1).
epinephrine,
released
situ
can be released
of
cells
aggregation,
has been shown previously
endothelial
serotonin
Thus,
of platelet
in the absence
heat
collagen, vents
prevention activity
activity
which
from endothelial
to conmonly used platelet
demonstrated This
activity
that
cells
be recovered with
cells. the
with
either
Recovery
from endothelial of
inhibitor
inhibitory
activity
collagenase.
(b
from endothelial
MTS in the absence
is
rare
cells
of aggregating
cells
from in situ
not generated
occasions,
in situ agents.
in
by
inhibi-
simply
by in-
In each
INHIBITOR
Vol.j,N0.6
case in which release sence
of
FROM ENDOTBELIAL
inhibitor
of added aggregating
signs
of
thrombin
of
cells.
lated
endothelial
release.
the process
might
render
thrwbin.
relatively
in situ
high since along
in these
the cord
work is
the differential
with
of
isolating
normally
frees
surface.
in situ of
The ability release
antithrombotic induced
of
the
likely
cord
showed obvious
this
are
cells
inducer
of
endothelial
is cells with
but
a possible
inhibitor in tests are
vein. less
such sensi-
not known.
The
to collagen
is
preparation
attachment.
endothelial
from the Achilles of
iso-
of
some form of collagen
from their
the efficiency
was
with
cells cord
iso-
amounts
inducer
the collagenase
which anchor
thranbin
enhanced
cells tendon
used
However, may differ collagen
as a release in-
effect
of
thrombiu
in
collagen.
inhibitor
to prevent
serotonin from platelets properties.
in contact
At any rate,
may reflect
in tests
to collagen
endothelial
large
thrombin
hand,
alteration
and reactivity
Finally,
cells,
of
and with
released
as a release that
effect
in situ
them from umbilical
isolated
structures
subendothelial of
is
the endothelial
cells
endothelial
effective
of
these
used here.
the presence
nature of
one cell
thrombin
more sensitive
sensitivity cells
cells
was the most active
It
in composition
preparation
tion
in the ab-
the umbilical
or that
On the other
situ.
The exact
studies
considerably
also
occurred
be shown that
in situ,
moderately
the cells
the collagenase-sensitive
ducer
cells
endothelial
isolated
collagen
in
with
inducer.
was only cells
during
alteration
but’with
cells,
endothelial
interest,
the present
cells
as a release
Collagen
to
of
when tested
activity,
inactive
altered
could
postdelivery
With endothelial
nearly
tive
aspect
and collagen
inhibitory
with
it
755
trauma.
An interesting
lated
from eudothelial
agents,
used was more than two hours
CELLS
The inhibitor
by ADP, epinephrine,
not only
indicates prevents
or thrombin.
platelet
that the
this first
In addition,
aggregation agent
but
has potent
wave of aggregathe
inhibitor
756
IXHIBITOR
prevents
FROM ENDOTHELIAL
the second wave of platelet
the release
reaction
Diminution evidence
of
of clot
retraction spectrum
is not essential
inhibition
traction.
hence the
inhibition
of
Prevention inhibitor lation
of clot
of calcium
cells
inhibitor
is
take
up the
inhibitory
trum inhibitor
amounts (4). is
of
studied
is
platelet
Further
on platelets.
functions
agent
inhibitor for
of
not known.
Alternatively,
characterization
clot
re-
retraction
suggests
by
that
intracellular
the
reguIt
release
is
from
thrombostheain.
activity
within
synthesize
stimuli
the endothelial it.
in plasma
these
endothe-
and store
to appropriate
and concentrate
both of
release
to prevent
of
may be present of
retraction
of thrasbostheain.
cells
in response
aggregation
clot
such as the
inhibitory
from plasma
clot
and aggregation
be released
Platelet
inhibited
may influence
contraction
further
the platelet
reaction
may function
of the
is
Recently,
and contraction
Whether endothelial
activity
platelet
this
here
release,
the
activity
release
retraction,
location
not known.
agents
by prevent ion of
inhibitory
upon the occurrence
of Ca2+ needed
which can then
as aggregating
apparently
retraction.
reaotion.
that
The ultrastructural Lial
clot
ion concentration
sites
of
release
basic
to speculate
intracellular
effects
the platelet
inhibitor
influences
tempting
of
the platelet
by the
for
has been shown to be dependent
reaction (3);
aggregation,
Vo1.5,No.6
of platelets.
the broad
aggregation
CELLS
inhibitory
cell A broad
this such may spec-
in small activities
in progrese.
ACKNWLEWEMENTS
Supported in part by grants !%04-HL 46351, HL 13296, and M 14228 from the National Heart and Lung Institute, cootract P&43-68-977 with the Artificial Kidney-Chronic Uremia Program of the National Institute for Arthritis, Metabolism, and Digestive Diseases, and grant 938 from the Council for Tobacco Research--U.S.A., Inc.
Vo1.5,No.6
INHIBITOR
FROM ENDOTHELIAL
757
CELLS
RlwERENCES
S.R., ZUCKPX, W.H., and WbSCN, RX. Some properties isolated from hman umbilical cord vein. 3. m.
1.
S&A, cells
2.
HOVIG, T. Release of a platelet-aggregating phate) frop rabbit blood platelets induced Thromb. Diath. Hsemorrh. 2: 264, 1963.
3.
DE GARTANO,G., BUT'TECCHIA, D., and VKRMYIKN,J. Retraction of reptilaseclots in the presence of agents inducing or inhibiting the platelet adhesion-aggregation reaction. Thromb. m. 2: 71, 1973.
4.
MASON, R.C., SABA, S.R., of platelet aggregation.
and CHUANG,.H.Y.K. &I. J. m. 74:
of endothelial 6: 456, 1973.
substance (adenosine diphosby saline “extract” of tendons.
Naturally 91a, 1974.
occurring
inhibitors
Vol. States
j, pp. 747-7j7, Pergamon Press,
1974 Inc.
STUDIES OF AN ACTIVITY FROH ENDGTHELIAL CELLS THAT INHIBITS PlATELET AGGREGATION, SERCYIONINRELEASE, AND CLOT RETIUCTION
S. R. Saba and R. G. Mason Department of Pathology, University of North Carolina Chapel Hill, North Carolina 27514
(Received
4.11.1974.
Accepted
by Editor
M.I.
Barnhart)
ABSTRACT present in endothelial cells of human umbilical vein An activity origin has been found to inhibit aggregation, serotonin release, and clot retraction. This activity appears to reside in molecules of small size that can be released from in situ or isolated endothelial cells by freeze-thaw treatment or by exposure of cells to ADP, collagen, epinephrine, or thrombin. Relative amounts of inhibitory activity released from endothelial cells vary with the specific plate let aggregating agent used as release inducer and are influenced by use of in situ or isolated cells. Varying the concentration of aggre gating agent varied proportionally the amount of inhibitory activity released from in situ but not from isolated endothelial cells.
INTRODUCTION An activity of endothelial cell origin was described recently (1) that inhibited aggregation of platelets.
This activity could be released from iso-
lated endothelial cells by disruption of the cells or by treatment of cells with certain platelet aggregating agents.
A broad spectrum of action of the
inhibitory activity of endothelial cell origin was shown in that it prevented aggregation of platelets induced by adenosine diphosphate (ADP), collagen, epinephrine, or thrombin.
This inhibitory activity was shown to reside in a
small, heat labile molecule (9OoC, 10 min.). Further characterization of the inhibitory activity of endothelial cell origin has been undertaken.
Semiquantitative studies of the release of the
inhibitory activity both from endothelial cells in situ and from isolated 747
738
INHIBITOR
endothelial
cells
conducted.
The inhibitor
gation
but
to
in
FROM ENDOTHELIAL
response
prevent
to
has
various
been
release
of
found
Vol.j,No.6
CELLS
platelet
aggregating
not
to
serotonin
only
fran
agents
prevent
platelets
have
platelet
and to
been
aggre-
inhibit
clot
retraction.
MATERIALS AND METHODS Endothelial
Cells
and
Human umbilical tals
modified fic
cords
and brought
The umbilical
vein
platelet
lumen of bation
to
(!$g*+-
the in
37’C
were
in
did
obtained
a segment
Ca*+- free)
vein
preparations. from
laboratory.withfn
aggregating
the
at
Inhibitor
this
cord
and
increase
(MTS).
yield.
at
delivery.
and rinsed of
with
the
was placed
22OC for
speci-
in
the
60 minutes.
The incubated
solution
of
endothelial
cells,
was then
supernatant
was used as the inhibitor preparation in studies of platelet aggre-
ment
A control of
the
consisted
same umbilical
of cord
15OOg for
an identical vein
from
activity
Incu-
which
at
inhibitory
of
agent,
centrifuged
the
time
hospi-
aggregating
gation.
now contained
the
A solution
investigation
incubated
inhibitor
of
collaborating
was cannulated
solution
in MTS under
segment
nearby
two hours
each
Tyrode’s agent
not
of
six
15 minutes
preparation which
the
from
aggregating
released at
from
220C;
a different agent
This
control
cal
were
used after intervals greater than 2 hours post delivery or
cords
negligable
inhibitor
activity
unless
seg-
was
omitted.
contained
the
umbili-
unless traumatized cords were used in which cases detectable amounts of inhibitor were present in these controls. Endothelial cells were isolated from human umbilical cord vein by treatment of the in situ cells with 0.22 collagenase (collagenase type IV, Worthington Biochemical Corporation, Freehold, New Jersey) in MTS as previously reported (1).
Isolated endothelial cells were washed two times in FITSand fin-
ally resuspended
in &fTS at
a final
concentration
of
approximately 1000 cells
Vol.j,No.6
per
IXHIBITOR
axa3.
sion
Isolated
test.
This
aggregating ture not
cells cell
agent
in )ITS and
of
agent
platelet
endothelial the
negligable
in
A control
platelet
inhibitor
vein
platelet
before
the
at
centrifuged
mix-
37Oc did
endothelial
preparation
consisted
treated
was omitted.
cells is
from
isolated
serotonin
preparation
of
of
in
isolated
identically
This
control
endothelial
cells
with contained
release
was the
supernatant
in HTS centrifuged referred
to
and
as
at
clot
contraction.
frau
three
15OOg for
freeze-thaw
(,5OO/nm13)
times
frozen
15 minutes
inhibitor
at
preparation.
KTS.
or
other
Aggregation
inhibitor
preparation,
preparation,
and 3)
consisted
(1)
of
at
1,000
2)
agent
was used
from
rpm.
to
endothelial
at
least out
with
platelets/mm3) from
in
consisted
MTS substituted
which
agent.
aggregation of
for
was added
aggregating
cells
days
the
of
inhibitor
was prepared
donors
prior
a Chrono-log
MTS substituted
induce
normal
seven
Controls
PRP to
ml of
(500,000
obtained
carried
with
ml of
and 0.1
release
blood
mixtures
mixtures 0.2
(PRP)
for
were
ml KrS,
aggregating
from
medication
studies
PRP stirred
0.1
plasma
previously
37OC with
induce
as the
cord
agent
the
of
incubation
preparation
same umbilical
platelet-rich
aspirin
ture.
ation,
A control
22OC; of
also
volume
exclu-
Aggregation.
as described
Tests
was used
supernataat
Citrated
taken
mixture
B dye
15 minutes
for at
739
erythrosin
an equal
22’~
The supernatant
preparation
of
consisted
Platelet
at
15 minutes
aggregating
endothelial
This
by the
with
yield.
inhibitor
inhibitor
and thawed
incubated
CELLS
activity.
studies
second
95% viable
was mixed
15OOg for
the
the
inhibitory
was used
22Oc.
from
that
A second
80 to
aggregation.
cells
exception
This
at
inhibitor
cell-aggregating studies
were
suspension
was centrifuged increase
FROM ENDOTHELIXL
to
venipunc-
aggregometer
of:
1)
the
for
the
ml of
In each platelets activity
at
control
inhibitor
aggregating
0.1
who had not
agents.
inhibitor case,
the
prepar same
as was used tested
with
to
750
INHIBITOR
these platelets.
FRO!4 ENDOTHELIAL
CELLS
Degree of inhibition of platelet aggregation was determined
by measurement of change in % transmission (ZT) of the aggregometer and by determination of change in the total area which lay under aggregation curves; the areas under curves were cut out and weighed on an analytical balance. Amounts of aggregating agents required to produce a 75% change in %T varied with individual plasmas; ranges of concentrations are given for each aggregation-inducing agent in footnotes to Tables I and II. Release. One tenth ml of serotonin solution (9.1 X 10m6 H, specific activity of 55 m Ci/m mole of Cl4 labeled serotonin creatinine sulfate, Amersham Searle, Chicago, Illinois) was incubated with 0.9 ml PRP for 30 minutes at 37OC.
Two
tenths ml of freeze-thaw inhibitor preparation in MTS was added to 0.2 ml of labeled PRP and incubated for LO minutes before 0.1 ml of aggregating agent was added with stirring for 10 minutes.
The final mixture was centrifuged for
20 minutes at 1500g at 22OC, and the supernatant solution was counted in a Nuclear Chicago Scintillation counter with PBD in toluene as fluor. consisted of:
Controls
1) the control inhibitor preparation, 2) mixtures with MTS sub-
stituted for inhibitor preparation, and 3) mixtures with WTS substituted for aggregating agent. Clot Retraction. To 0.2 ml of PRP was added 0.2 ml of freeze-thaw inhibitor preparation in MTS.
The mixture was incubated at 37OC for one minute before 0.1 ml of
thrombin (2 units/ml) was added.
The final mixture was incubated for 90 min-
utes at 37OC before the degree of clot retraction was quantitated by gravimetric determination of the amount of extruded serum.
The control consisted
of a mixture with MTS substituted for inhibitor preparation. Reagents. ADP and epinephrine were obtained from Sigma Chemical Co., St. Louis,
INHIBITOR
Vol.5,No.6
Missouri and
FROM ENDOTHELIAL
prepared fresh in KTS each day.
Achilles tendons by the method of Hovig (2). this
Collagen was
751
prepared from h-n
One to two and
stock collagen preparation were made vith MTS.
was of bovine origin and was
CELLS
1:4
dilutions
of
Thrombin, 300 units/ml,
highly purified; this was a gift from Dr. R. L.
Lundbled, Dental Research Center, Dnivtrsity of North Carolina, Chapel Hill, North Carolina.
RESULTS Results
of
tests for the presence of inhibitory activity recovered by
incubation of endothtlial cells in situ with aggregating agents are given in Table I.
In studies with endothelial cells in situ, it was found that throm-
TABLE I Effects on Platelet Aggregation of an Agent Released from Endothtlial Cells In Situ in Response to ADP, Collagen, Epinephrint, or Thrombin
X decrease in platelet aggregation* in presence of inhibitory agent (P n * S.D.) y area under curve By%T
Aggregating agent used to induce release of inhibitor from endothtlial cells
Number Concentration of experiments
ADP
10-5 H
36.3 + 12.8
32.3 + 11.4
Collagen
1:2 dilution
11.7 +
9.2
18.2 +
6.0
1:4 dilution
7.4 +
5.1
14.7 +
8.6
Epintphrine
Thrombin
10-5 M
14.0 +, 3.3
12.1 +_ 0.2
10'6 H
11.3 +_ 0.6
8.0 +_ 1.7
1 unit/ml
75.6 + 12.6
54.0 2 19.8
0.5 unit/ml
56.7 +_ 18.5
34.2 +_ 12.1
12.4 f 2.3 13.7 f 1.5 J 0.25 unit/ml _ _ . r . ~. * Ranges of final concentrations f agents used to 1Muce aggrtgatlon or platelets were: ADP, loss to 2X 14 8n ; collagen, 1:4 dilution; tpintphrine, 1 to 2 x 10-s H; and thrombin, 0.1 to 0.2 units/ml.
INHIBITOR
752
bin released released tion
the most inhibitory
progressively
release
phr iae,
or thrombin.
reverse
the action
Results
agent of
while
amounts of
incubated
inhibitory
Addition
CELLS
ADP, epinephrine, Decreasing
inhibitor. with
endothelial
activity
of calcium
Vo1.5,No.6
in tests
the concentra-
cells with
to the reaction
and collagen
in situ
collagen,
mixtures
resulted epine-
did not
of the inhibitor
of tests
endothelial
activity
lesser
of the aggregating
in a decreased
lated
FROM ENDOTHELIAL
with
cells
inhibitory
activity
with aggregating
obtained
agents
by incubation
are shown in Table
of
iso-
II.
TABLE II Effects Endothelial
on Platelet Aggregation of an Agent Released from Isolated Cells in Response to ADP, Collagen, Epinephrine, or Thrombin
Aggregating agent used to induce release of inhibitor frcm endothelial cells
Concentration
ADP
5 x 10’5
Number
of !xper iment d
Z decrease in platelet aggregation* in presence of inhibitory agent (I !an + S.D.) By area under curve By7,T 5.6
18.9 +
4.9
10-5 M
30.4 + 15.6
23.5 +
4.5
1:2 dilution
40.7
+ 18.4
39.2 f 20.7
1:8 dilution
48.5
+, 18.6
42.7
Epinephr ine
5 x 10’7
21.0
+
7.3
23.8 +
5.4
Thrombin
0.5
5.8 +_ 3.7
11.0 +
0.9
Collagen
*
M
units/ml
0.25 units/ml 8.1 of agents used Ranges of fina concentration platelets were: ADP, 2 X loto 2 x lo-6 M; epinephrine, 10’5 to 2 X 10-6 M; thrombin, 0.2
Collagen
was found to release
aggregating Lesser
agents
amounts of
thrombin.
In teats
the
were incubated inhibitory with
+
26.0
n
largest with
activity
isolated
3.8 f 4.4 1 5.7 f to induce aggregation of collagen, 1:4 dilution; to 0.44 units/ml.
amounts of
isolated
inhibitory
endothelfal
were released
endothelial
2 13.3
cells,
cells
activity in hTS.
by ADP, epinephrine, decreasing
when
and
the concen-
I?i-HIBITOR FROM
tration
of ADP or collagen
amounts of induced tained
inhibitory
by each of
activity. the agents
from isolated
Effects platelets
is
of
slightly
shovn in Table
of
CELLS
did
not result
Similar
inhibition
tested
endothelial
the presence
ENDOTHELIAL
could
cells
in release
of
of platelet
be demonstrated
smaller aggregation
with
inhibitor
ob-
by freeze-thaw.
inhibitor
III.
753
on the release
ADP, collagen,
of
serotonin
epinephrine,
from
or thrombin
was
TABLE III Effects of the Inhibitory Serotonin from Platelets
Agent used to induce release of serotonin from platelets
Activity of Endothelial Induced by ADP, Collagen,
2 x lo-4
1
of exper intents
X inhibition of release of serote nin by inhibitor obtained from endothelial cells by freeze-thaw
X release of serotonin
Number
Concentratioc
Cell Origin on Release of Epinephrine, or Thrombin
with inhibitor
vithout inhibitor
M
50.6 5
6.6
9.1
+
9.7
82.0
1 x 10’4 M
39.7 +,
9.3
5.7 +
5.6
85.6
Collagen
1:l
66.3 + 10.1
14.6 +_ 9.1
78.0
Ep inephr ine
2 x 10’4 H
64.0 +_
7.9
0.3 +_ 0.3
99.5
1 x 10’4 M
61.8 f.
3.4
0.3 +,
0.3
99.5
1 unit/ml
86.5 +
3.9
38.8 f
13.0
55.1
0.5
77.2 f
9.5
5.1 f
6.7
93.3
ADP
Thraubin
unit/ml
used to induce
release
from endothelial
cells
percent dothellal release
serotonin cell
of
by freeze-thaw
release
origin.
serotonin
treatment.
in the absence
Results
and presence
agents
tested,
also
induced
was obtained expressed
the inhibitor inducer
of
appreciable
as of en-
serotonin release.
the amount of inhibitory activity
was sufficient to prevent 55.0 to 99.5% of the release platelets.
are
of
Thrombin was the most efficient
but ADP, epinephr ine , and collagen
With the release-inducing
Inhibitor
from platelets.
of
eerotonin
from
INHIBITORS
754
The inhibitor
of endothelial
prevention
of clot
endothelial
cells
retraction.
cell
by 58%.
centration,
500/&)
Addition
of
isolated
of clot
CELLS
was also of
the
when added
to recalcified
60X inhibition
origin
Preparations
by freeze-thawing,
retraction
mately
FROM ENDCTHELIAL
intact
titrated
Vo1.5,No.6
an efficient
inhibitor
agent
released
for
from
to titrated
PRP, reduced
clot
endothelial
cells
con-
PRP likewise
(final
resulted
in approxi-
retraction.
DISCUSSION The inhibitory potent This
agent inhibitory
cells
the
for
is
intact
of
labile
plate let
this
cells
is
tory
a broad
is
or of cell
demonstrated
inhibitor
which
activity
fragments. molecule
easily
when
contain
ADP, pre-
and the release
epinephrine,
of platelet
to the presence
of
can be
not only
retraction
by ADP, collagen,
in response
small
mixtures
clot
by exposure
The inhibitor
cells
inhibitory
prevents
spectrum
cells
cells
to be a relatively activity
and retraction.
or thrombin.
function of
and is
commonly used
agents. activity
from isolated cells
indicates
could
the cells
can be recovered
endothelial
of endothelial
activity
cubating
induced
from endothelial
endothelial treatment
endothelial
This
but also
release,
agents.
added to reaction
or thrambin.
from platelets
The inhibitory or
are
aggregation
activity
aggregating
intact
has been shown to be a
from endothelial
aggregating
Inhibitory
(1).
epinephrine,
released
situ
can be released
of
cells
aggregation,
has been shown previously
endothelial
serotonin
Thus,
of platelet
in the absence
heat
collagen, vents
prevention activity
activity
which
from endothelial
to conmonly used platelet
demonstrated This
activity
that
cells
be recovered with
cells. the
with
either
Recovery
from endothelial of
inhibitor
inhibitory
activity
collagenase.
(b
from endothelial
MTS in the absence
is
rare
cells
of aggregating
cells
from in situ
not generated
occasions,
in situ agents.
in
by
inhibi-
simply
by in-
In each
INHIBITOR
Vol.j,N0.6
case in which release sence
of
FROM ENDOTBELIAL
inhibitor
of added aggregating
signs
of
thrombin
of
cells.
lated
endothelial
release.
the process
might
render
thrwbin.
relatively
in situ
high since along
in these
the cord
work is
the differential
with
of
isolating
normally
frees
surface.
in situ of
The ability release
antithrombotic induced
of
the
likely
cord
showed obvious
this
are
cells
inducer
of
endothelial
is cells with
but
a possible
inhibitor in tests are
vein. less
such sensi-
not known.
The
to collagen
is
preparation
attachment.
endothelial
from the Achilles of
iso-
of
some form of collagen
from their
the efficiency
was
with
cells cord
iso-
amounts
inducer
the collagenase
which anchor
thranbin
enhanced
cells tendon
used
However, may differ collagen
as a release in-
effect
of
thrombiu
in
collagen.
inhibitor
to prevent
serotonin from platelets properties.
in contact
At any rate,
may reflect
in tests
to collagen
endothelial
large
thrombin
hand,
alteration
and reactivity
Finally,
cells,
of
and with
released
as a release that
effect
in situ
them from umbilical
isolated
structures
subendothelial of
is
the endothelial
cells
endothelial
effective
of
these
used here.
the presence
nature of
one cell
thrombin
more sensitive
sensitivity cells
cells
was the most active
It
in composition
preparation
tion
in the ab-
the umbilical
or that
On the other
situ.
The exact
studies
considerably
also
occurred
be shown that
in situ,
moderately
the cells
the collagenase-sensitive
ducer
cells
endothelial
isolated
collagen
in
with
inducer.
was only cells
during
alteration
but’with
cells,
endothelial
interest,
the present
cells
as a release
Collagen
to
of
when tested
activity,
inactive
altered
could
postdelivery
With endothelial
nearly
tive
aspect
and collagen
inhibitory
with
it
755
trauma.
An interesting
lated
from eudothelial
agents,
used was more than two hours
CELLS
The inhibitor
by ADP, epinephrine,
not only
indicates prevents
or thrombin.
platelet
that the
this first
In addition,
aggregation agent
but
has potent
wave of aggregathe
inhibitor
756
IXHIBITOR
prevents
FROM ENDOTHELIAL
the second wave of platelet
the release
reaction
Diminution evidence
of
of clot
retraction spectrum
is not essential
inhibition
traction.
hence the
inhibition
of
Prevention inhibitor lation
of clot
of calcium
cells
inhibitor
is
take
up the
inhibitory
trum inhibitor
amounts (4). is
of
studied
is
platelet
Further
on platelets.
functions
agent
inhibitor for
of
not known.
Alternatively,
characterization
clot
re-
retraction
suggests
by
that
intracellular
the
reguIt
release
is
from
thrombostheain.
activity
within
synthesize
stimuli
the endothelial it.
in plasma
these
endothe-
and store
to appropriate
and concentrate
both of
release
to prevent
of
may be present of
retraction
of thrasbostheain.
cells
in response
aggregation
clot
such as the
inhibitory
from plasma
clot
and aggregation
be released
Platelet
inhibited
may influence
contraction
further
the platelet
reaction
may function
of the
is
Recently,
and contraction
Whether endothelial
activity
platelet
this
here
release,
the
activity
release
retraction,
location
not known.
agents
by prevent ion of
inhibitory
upon the occurrence
of Ca2+ needed
which can then
as aggregating
apparently
retraction.
reaotion.
that
The ultrastructural Lial
clot
ion concentration
sites
of
release
basic
to speculate
intracellular
effects
the platelet
inhibitor
influences
tempting
of
the platelet
by the
for
has been shown to be dependent
reaction (3);
aggregation,
Vo1.5,No.6
of platelets.
the broad
aggregation
CELLS
inhibitory
cell A broad
this such may spec-
in small activities
in progrese.
ACKNWLEWEMENTS
Supported in part by grants !%04-HL 46351, HL 13296, and M 14228 from the National Heart and Lung Institute, cootract P&43-68-977 with the Artificial Kidney-Chronic Uremia Program of the National Institute for Arthritis, Metabolism, and Digestive Diseases, and grant 938 from the Council for Tobacco Research--U.S.A., Inc.
Vo1.5,No.6
INHIBITOR
FROM ENDOTHELIAL
757
CELLS
RlwERENCES
S.R., ZUCKPX, W.H., and WbSCN, RX. Some properties isolated from hman umbilical cord vein. 3. m.
1.
S&A, cells
2.
HOVIG, T. Release of a platelet-aggregating phate) frop rabbit blood platelets induced Thromb. Diath. Hsemorrh. 2: 264, 1963.
3.
DE GARTANO,G., BUT'TECCHIA, D., and VKRMYIKN,J. Retraction of reptilaseclots in the presence of agents inducing or inhibiting the platelet adhesion-aggregation reaction. Thromb. m. 2: 71, 1973.
4.
MASON, R.C., SABA, S.R., of platelet aggregation.
and CHUANG,.H.Y.K. &I. J. m. 74:
of endothelial 6: 456, 1973.
substance (adenosine diphosby saline “extract” of tendons.
Naturally 91a, 1974.
occurring
inhibitors