Abstract: The localization of the adhesion protein. L-selectin in human neutrophils was determined by sub- cellular fractionation and immunoelectron microscopy.
Changes L-selectin,
in subcellular localization and surface expression alkaline phosphatase, and Mac-i in human
neutrophils
during
stimulation
with inflammatory
Niels Borregaard Lars Kjeldsen Henrik Timothy A. Springer,’ H. Clarke Anderson,’ UI
The
Granulocyte
Denmark;
The
Research
The
Center
University
of
Department
Laboratory,
for
Kansas
Department
Blood
Research,
Medical
Center,
of Immunology,
of
Harvard
Ridgefield,
Abstract: The localization of the adhesion L-selectin in human neutrophils was determined cellular fractionation and immunoelectron and compared with the localization of Mac-i
Medical
School
of Medicine,
and
tDepartment
C7
protein by submicroscopy (amfl2) and
Words:
tory
fMLP
vesicles
.
GM-CSF
.
IL-8
.
LTB4
.
PAF
.
Hospital,
Boston,
Kansas
MA,
City;
and
Mac-l
on
the
tips
and
seemingly
ideal
neutrophils
face lated
cells an
[231.
of intact of secretory
plasma
membrane
in
matory
mediators
[29,
by
their
membrane
on the Because
30].
activation
mobilized
organelle
important
as
of
and which [31],
microvilli
of
secretory
vesiand
appearance of can be accounted membrane into the with
are
inflamidentified
phosphatase
most
sur-
the
alkaline
present ignored
present
in the matrix. in studies of
rapidly
[32],
mobilizable
the nonstimu-
monocytes,
vesicles
albumin is largely
is the
whereas
over
stimulation
ofneutrophils
a rapidly
cells,
that
to
[24] contact
randomly
Secretory
content
neutrophil
rolling
neutrophils vesicle
response
luminal surface this organelle
initial
that
and
prob-
of L-selectin
[25-28],
Mac-I
is
L-selectin
tail
demonstrated
contain
neutrophils
that
endothelial
from
Inc.,
a localization
the
neutrophils
on the surface incorporation
of
23],
mediating
have of
[29],
[2,
on
Oncology,
Francisco
surface
cytoplasmic
excluded
We
San
demonstrated
is distributed
organelle
and
Pharmaceuticals
the
P-selectin
but
eosinophils
Mac-i for by
for
present,
membrane
des,
the
with
when
on
been
ofmicrovilli
through
Mac-i,
of Pathology
of Ca4fornia,
It has
mediated
Copenhagen,
Ingelheim
(a0j32)
ably
of
‘Department
University
understood.
well
F. Bainton11
Rigshospitalet,
SBoehringer
of Pathology,
is present
secre-
.
School,
less
J-
Key
University
selectin
alkaline phosphatase, the marker for secretory vesicles. L-selectin was found to be localized exclusively on the plasma membrane of unstimulated cells and also of stimulated cells, although markedly diminished. This was in contrast to Mac-i, which was also localized in secretory vesicbes and in specific/gelatinase granules as shown previously [Sengelv, H., et al.J. Clin. Invest. (1993) 92, 1467-1476]. Stimulation of neutrophibs with inflammatory mediators such as tumor necrosis factor (TNF), platelet-activating factor (PAF), or f-Met-Leu-Phe (fMLP), induced parallel up-regulation of the surface membrane content of alkaline phosphatase and Mac-i and down-regulation of L-selectin, as evidenced by flow cytometry. Preimbedding immunoelectron microscopy confirmed that L-selectin was present mainly on tips of microvilli in unstimulated cells and showed that alkaline phosphatase and Mac-i were randomly distributed on the surface membrane of fMLP-stimulated cells. These studies indicate that the transition of neutrophils from L-selectin-presenting cells to Mac-i-presenting cells induced by inflammatory mediators is mediated by incorporation of secretory vesicle membrane, rich in Mac-i and devoid of L-selectin, into the plasma membrane. Leukoc Biol. 56: 80-87; 1994.
mediators
Sengel#{243}v Michael S. Diamond,’ Takashi K. Kishimoto,S and Dorothy Hematology,
of
and
most
easily
it is potentially
source
of
very
neutrophil
sur-
face proteins. We therefore decided to address the question whether secretory vesicles contain L-selectin in addition to Mac-i and thus might play a role in continued rolling contact of neutrophils with endothelium by replenishing Lselectin
lost
whether
secretory
case
a highly
tion
of
to
from
the
selective
by
are
devoid
of
secretory
role
neutrophils
adherent,
surface
vesicles from
rolling,
Mac-l-presenting
shedding
[33,
34],
of L-selectin,
or
in which
vesicles
in
the
transi-
L-selectin-presenting cells
must
cells
be
suspected.
TNF MATERIALS
AND
METHODS
INTRODUCTION Human The key
dynamic event
invading
the
process in
ofneutrophil-endothelial
inflammation
in
microorganisms
in
demonstration
selectins
in
trophils
with
both mediating
from surface
and 21J
80
mediators
intracellular
stores
Journal
the
in
[1-7]
vivo
[22],
of Leukocyte
but
and
of
/32
CSF.
role of
dynamic
[16]
Volume
to
E-selectin
56,
freshly
drawn blood of red cells was Uppsala, Sweden), was centrifuged on Residual erythno-
[35].
1994
fl’s’l LP,
the
TNF,
L-
phosphate; tumor
Reprint tory.
V-lorisiylrnethionyl-leucyl.phenylalanine;
granulocyte-macrophage
Ringer
[20, of
July
were
described
Abbreviations:
synthesis
presentation
neutrophils
previously
and
P-selectin
subsequent
as
neu-
adhesion cells of
of
by
the
integrins
bodies) and
Biology
to
against
irreversible of endothelial
membrane the
of
transbocation
[17-19]
of
a
clarified
contact
(Weibel-Palade plasma
defense been
rolling
subsequent response
cells
insertion into and ICAM-l
in has
and
involves
ofendothelial
and
initial
cells
ICAMs in mediating the [5, 8-15]. The immediate inflammatory
vitro
the
endothelial
general particular,
in
isolated from Sedimentation induced by dextran T-500 (Pharmacia, and the leukocyte-nich supernatant Lymphoprep (Nygaard, Oslo, Norway).
interaction,
Received
Niels of
Copenhagen
January
B4;
ZAS,
zymosan-activated
Borregaard,
Hematology, 0.
factor;
leukotriene
factor;
requests:
Department
DK-2100
CUB4,
necrosis
GM-
colony-stimulating
The
PAF,
platelet-activating
Granulocyte
Rigshospitalet
accepted
March
P.
Krebs-
flictor;
serum. Research L-4042,
Denmark.
7, 1994;
KR
21,
1994.
9
Labora-
Blegdamsvej,
cytes
were
lysed
resuspended
by
in
carried
out
at
of
fractionation, sorter
mM
i0
for
analysis,
was
terminated
ice-cold
buffer
and
pelleted
cells
were
samples
were
dilution at
200g
in
FAGS
2
with for
ice-cold
analysis
mm.
for
gradient This
scribed
fractionation
[35].
In
containing
short,
S
Chemical
Milwaukee,
containing
and
bottom
in
3 mM
15
NaCl,
1
ml
mM
and
200g of
previously
resuspended
kept
for
10
disruption
Na2ATP,
A
on
in
KRP
Marker
mm. were
Azurophil
cells
(100
mM
KC1,
using
as
mM
body
(Dakopatts
for
10
vesicles,
cytosol.
Gradients
the
pump ml
in
band
intermediate and
gelatinase
plasma
clear
were
that
bottom
containing the
described
regions the
granules
and
Percoll as
separate
granules,
a peristaltic 1.4
two-layer
gradient:
(y-band)
MgCl2,
0.5
granules
measured
B
attached
identified
by
(S2) from
to
fraction.
mem-
supernatant
aspirated
each
by
were
enzyme-linked
the
a fraction
col-
catching
antibody A
myeloperoxidase
immunosorbent rabbit
398,
assay
(ELISA)
antimyeloperoxidase
Glostrup,
anti-
Denmark)
after
affinity
D
C
Geiatinase,
Lactofertin, pg/mi
CD11b, U/mi
L-Seiectin, U/mi
28-ml
specific
at super-
proteins
the
ice
mm
mM
the
centrifugation postnuclear
centrifuged
offour in
secretory
deliver
a
and
generation
band
the
at
Nuclei
(Aldrich
buffer 3.5
top
to
of
azurophil
through set
top
of
7.2)
pH
cavitation.
de-
fluorophosphate WI)
at
as
were
diisopropyl
centrifugation
resuspended
performed
neutrophils
mM
Co.,
After
was
in
PIPES,
by
ml
g/ml)
containing
the
lector,
Subcellular
on
containing
and
10
identified
(/3-band)
branes
fractionation.
loaded
mM
nitrogen
sedimented
and
(1.05/1.12
visually
granules,
subcellular
was
by
were
(P1),
resulted
be
The
buffer
and
(S1)
10
disrupted
cells
mm
natant
(a-band)
of
and
15
density
band
volumes
10
for
could
period
fluoride,
cells/ml
unbroken
F35].
(KRP):
0.95 mM pH 7.4.
by
i0
400g
subcellular
MgSO4, NaH2PO4/Na2HPO4, a 5-mm preincubation
resuspended for
subsequent
x
and cell
fluorescence-activated
centrifugation
taken
cells.
37#{176}C at a
at
3
1.27 mM
mm
15
red
phenylmethanesulfonyl were
Krebs-Ringer-phosphate
after
after
for
subsequent
in
initiated
of
performed
cells/mi
i07/ml
neutrophils
procedures
sedimentation
NaCl, S mM KC1, mM glucose, 10 mM
Stimulation
the
All
was
x
at
(FAGS)
CaCl2, and
3
or
and
indicated.
ofneutrophils
concentration
130
shock
as
4#{176}Cexcept
Stimulation
cell
hypotonic
buffer
pg/mi
2.000
1.500
1,000
I
5
10
15
Fraction
20
25
No
E
10
15
Fraction
No
20
251
25
Fraction
F
10
20
25
Fraction No
No
G Phos, mU/mi
200
E
E 150
:D C
.0
a 0 0 Cl)
0 0
Frtion
No
Fraction
No
15
11
20 Fraction
Fig. other
1.
Subcellular
localization
stimulated
with
is shown.)
(A)
of
membranes);
plasma
branes) and
are Figure
l0
L-selectin;
shown 2 in
left
L-selectin
fMLP
(B) (F)
by the the
of M
Mac-l; latent
following y axis
and
at 37#{176}C(Fig. (C) alkaline
symbols:
lactoferrin
Mac-I. 2).
(a
phosphatase
Mac-l
Isolated
Subcellular marker (a
(*),
marker
L-selectin
neutrophils
were
fractionation of specific
was
divided then
granules);
of secretory
(#{149}), latent
(D)
vesicles); alkaline
in
two
performed gelatinase (G)
is an
phosphatase
equal
parts,
in parallel. (a
marker
insert (U),
one
kept
the
HLA
at
4#{176}C(this
representative
of geiatinase
where and
was
(One
25
No
granules);
results (Y).
for Note
figure)
experiment fractions difference
(E)
HLA 11-20
between
of G.
Borregaard
et al.
Human
neutrophil
adhesion
and
out
receptors
(a (light this
the
of three marker memfigure
purification
on
antibody (Dakopatts as
a
was A
purified sured
by
isolated
azurophil
granules
were
identified
measured
by only
(latent
alkaline
1271.
human
leukocyte
ELISA
(MELISA)
Mac-i
antigen
the
an as
IgGl
by
a
IgG2a
catching
mouse
of
L-selectin
sg/ml)
tions
as
ref.
8 of
against
detecting
antibody.
by
in
with
batch
all
experiments
I domain
using
DREG
biotinylated of
55
buffer
pH
7.2,
1 h. was
diluted
in
After
three
and
200
2-fold
serial
(55
arb.
dilu-
in
B
buffer
(except
for
A.
once
citrate,
1 h, in
pH
mM Color
were
CDiib
A,
[30]).
100
l
of
appropriately
1 h followed l
by of
buffer
washing
developed
10O-jl
standard
washing
peroxidaseB
was
three
added times
Na2HPO4/NaH2PO4,
C Ltoferrin,
U/mi
of
a
standards
buffer
l
albu-
A,
applied,
in
by
serum
of
100
P347) followed
100 5.0.
for Then
(Dakopatts, for
A and
incubated
buffer
Addi200
Na2HPO4/
dilutions
quantitation in
mM
buffer
and
was
X-lOO).
bovine in
The KC1,
with
8
1%
serial
washes
B and in
KC1,
samples
antibody
avidin
sodium
All
Triton
times
with
h.
additional
incubated
buffer
U/ml).
1
of catch-
3 mM
incubating
X-iOO,
along
buffer
by
three
l
NaCl,
7.2, 1%
Triton
100
temperature.
mM
3 mM
washing for
times
and
1%
After applied
conjugated
are
serum
NaCl,
catching
three
(500
blocked
[36}
Immunoplates
Na2HCO3/NaH2CO3,
at room
A
were
mM
incubated
B CD11b,
U/mi
L-S.lectin,
B (500
diluted
as 200
human
sample
A
55
DREG
normal in
diluted
of
buffer
pH
sites
biotinylated
DREG
One
an
overnight in
previous
lactoferrin
used. with
mM
in-
in
and
not
coated
50
Na2HPO4/KH2PO4,
and
of
incubated washed
binding
sample
chain
LM2/l,
the
ELISA and
a 20-fold
a
and
KH2PO4, mm) for
using
against
the
mM
were in
procedure
specified
[39] was
Denmark)
general as
MELISA
diluted
were
tional
a mixed
antibody of
9.6,
wells
by
[301
biotinylated
antibody. 40.
standard
starting
by
described
antibody
g/ml)
detecting
in
used
as
and
as
(2.5
as
characterized
mea-
identified
I assayed
Roskilde,
same
except
interaction
antibody,
pH
the
antibodies
regarding
(Nunc,
be
albumin
region
quantitated
antibody
(0.63 was
Mac-i,
was
catching
could
using
the
avidin-biotin
ing
by
monoclonal
antibody
monoclonal
chain
by vesicles X-lOO
were
ELISA
extracellular
mouse
the
where
Triton
and
class
publications
mea-
identified that
performed of
stan-
(v/v)
membranes (HLA)
quantitated
COOH-terminal
Mac-i
26]
as
[39].
was
CBRM1/23,
0.2%
[25, Plasma
used
[381
of
was
dependent
Secretory
phosphatase
presence
ELISA
used
lactoferrin were
[37].
ELISA
and
was by
granules
alkaline
ELISA
Myeloperoxidase,
granules,
phosphatase)
by ELISA
sured
1 mg/mI
identified
by
the
in
at
Gelatinase
measured
The
antimyeloperoxidase
1:10,000.
were
[36].
[36],
column.
Rabbit
biotinylated diluted
ELISA
gelatinase
was
antibody from
Specific
1:100.
398)
detecting
dard.
myeloperoxidase-Sepharose
diluted
in
100 during
mM
a 30-mm
in-
D gig/mi
Geiatinase,
pg/mi
2.500
2.000
1.500
1,000
500
I
5
10
15
20
25
No
Fraction
Fraction
E
No
Fraction
F
HLA, U/mi
No
Fraction
No
G
Latent Alk. Phos.,
mU/mi
40
20
20
E
E
C
.0
a 45
10
0
1,000
0
Fraction
No
Frtion
-
No
15
11
20
25
Fraction No Fig. lated shown.)
82
2.
Subcellular
with
108 See
localization M
legend
Journal
fMLP of
of L-seiectin at
37#{176}C(this
Figure
of Leukocyte
1 for
and figure).
explanation
Biology
Mac-l.
Isolated
Subcellular of
neutrophils
fractionation
A-G.
Volume
56,
July
were was
1994
then
divided performed
in two
equal in
parallel.
parts,
one (One
kept
at 4#{176}C(Fig.
representative
1) and
experiment
the
other out
of
stimuthree
is
M.F.l.
M.F.l.
cubation
1,800 1,600 1,400 1,200
50
40
by
sodium
10
addition
nm
Fig. 3.
EL-Selectin
Immunofluorescence.
1. j; axis),
bar,
l.y
by
FACS mm
(light
alkaline
phosphatase antibodies
were
either
with
each
of
TNF,
doses
regulation dependent
surface dotted
monoclonal
Cells U/mI
These
and
using
CD11b
The
L-selectin
axis),
tensity.
37#{176}C as
formed
by incubating
monoclonal
0.2
were
kept the
pg/mI
found
IL-8, to be
ofMac-l and experiments.
at
membrane bar, (solid
42],
alkaline
as
ZAS,
M
LTB4,
l08
M
maximally
phosphatase.
axis) mean
was
for
fMLP,
at U/mi
and
effective
Results
are
4.
with
the
goid-5 label
is
on
inonocional
00
the
surface
antibody
finally
the
ELISA
reader
for
DREG
1,
37#{176}C or
cells
was
i07/ml
200,
per-
with
lBi2,
osteosarcoma
SO l
an
alkaline
Dakopatts
IgGi
phos-
M736)
or
Mountain twice, SO jl
of
rabbit anti-mouse antibody (Dakothe cells were incubated for 30 mm at washes, the cells were resuspended (PBS)
a FACScan
intensity for fluorescence
preimmune
of
(Becton-Dickinson, 4#{176}C.After washing
saline in
4#{176}C or
at 1 x
class
at
at
containing
1%
formalde-
(Becton-Dickinson).
specific by
Mean
antibodies subtracting
was mean
corrected fluores-
IgG1.
37#{176}C for
Immunoelectron
microscopy
GM-CSF, l0
M
Because
PAF. up-
ofthree
of fixation
monoclonal
in-
sensitivity
antibodies
(alkaline
of the
antigens
CBRM1/29
phosphatase),
detection
[43] ofthese
recognized (Mac-i)
two
by
and
antigens
iBi2 on
the
my
L-Seiectin was
mm
analyzed
kept
human IgGl
30
my
Fig.
was
was
in-
in causing
means
and
cence
determined
fluorescence
stimulated 100
dotted
automatic
ofcells
anti-HLA
preimmune
fluorescence for nonspecific
(open
(heavy
and
Absonbance
Labeling
(LM2/i,
against
[41,
CA)
either
indicated.
antibody
antibody
phosphate-buffered
hyde
of HLA
Mac-l
2.)
37#{176}Cor
l0 5%
bar, given
4#{176}Cor
individually
content
1. y axis),
and
following:
in
#{149}AIk.Phos.
H2SO4.
1 M
Plus
100 l
fluorescein-conjugated patts) was added, and 4#{176}C.After two additional
0HLA
of
containing H202
Finland).
were
at
View,
I
l
in a Multiscan
neutrophils
phatase munine
$()%:bc;tP4
100
buffer
0.03%
analysis
murine 0
of
stimulated of
acid and
Helsinki,
Isolated
.1
phosphate-citric
o-phenylenediamine
at 492
FACS
2”
0
500
stopped
read
30
800 600 400 200
15
(w/v)
(Labsystems,
1,000
bar,
in
0.04%
periormed. tips
of
microvilii
of neutrophils. DREG-200 Transmission (m).
Unstitsiulated against electron
L-seiectin. micrograph
neutrophils A bridge of
were of
a portion
fixed
rabbit
in
2%
anti-mouse of
a neutrophii
formaldehyde. antibody is
0.05% was
given.
As
glutaraldehyde,
applied, can
be
and seen,
washed,
and
immunolabelini. the
majority
with of
the
incubated protein
A
immunogold
x 45,000.
Borregaard
et al.
Human
neutnophil
adhesion
receptors
83
plasma
membrane
was
performed
by
incubating
unfixed
PBS,
cells at 4#{176}Cfor 45 mm with either CBRM1/29 (1 mg/mi) diluted 1:100 or lBi2 (1 mg/ml) diluted 1:20 followed by fixation in 2% paraformaldehyde, 0.05% glutaraldehyde for 30 mm at room temperature. Rabbit anti-mouse antibody (Zymed) diluted 1:200 was then added, followed by protein A-gold-S (1:50 dilution). Immunogold labeling of L-selectin was
performed
before
fixation
as
described
above
or
could
(fMLP)
colony-stimulating
in ethanol.
factor
(GM-CSF;
NJ),
10 U/ml
Granulocyte-macrophage Sandoz
Pharmaceuticals,
ig/ml
ethanol.
Tumor
necrosis UK),
Amersham,
with
the
main
peak
of
the
phosphatase localizing close to marker HLA and L-selectin, while vesicles are found in a broad region
factor (TNF; iO4U/ml in
region
to
the
region
marker
the the from
latent
alkaline
plasma membrane rest of the secretory the peak in the light
containing
specific
granules.
The separation of HLA and L-selectin from latent alkaline phosphatase and from Mac-i is evident when focus is made on the light membrane region of the gradient as seen in Figure 1G. The localization of Mac-i in secretory vesicles and L-selectin in the plasma membrane is further illustrated by the translocation in response to stimulation with fMLP (Fig. 2). Stimulation of intact cells with fMLP results in nearly selective and complete exocytosis of secretory vesicles. This is evidenced by the disappearance of latent alkaline
(Sigma),
East
in H20. Recombinant interleukin-8 from Dr. K. Thestrup-Pedersen, Department Marselisborg Hospital, Aarhus, in PBS. Leukotriene B4 (LTB4; Sigma), Platelet-activating factor (PAF; Sigma),
ous gift matology, 10
gradient,
membrane
1 mM
(Sigma).
The distribution of L-selectin in subcellular fractions of unstimulated neutrophils (Fig. 1) indicates that L-selectin is present exclusively in the plasma membrane, whereas Mac-i is localized with a main peak in specific/gelatinase granules and a second peak colocalizing with secretory vesicles. The distribution of secretory vesicles is bimodal in this two-layer
be
of stimuli
N-Formylmethionyl-leucyl-phenylalanine
BSA
International,
RESULTS AND DISCUSSION
paper.
Source
(w/v)
H20.
performed after fixation by adding mAb DREG 200 diluted 1:200 (stock 2 mg/ml). The cells were subsequently refixed in 1.5% glutaraldehyde for 45 mm at 22#{176}C,washed in sodium cacodylate buffer, postfixed in 1% 0s04 in veronal-acetate buffer, stained with aqueous 1% uranyl acetate, dehydrated in ethyl alcohol, and embedded in Epon. Detailed morphometric analyses of these localizations are the subject of a separate
0.5%
Amersham
Hanover,
(a generof DerDenmark), 1 mM in 1 mM in
F, I,
Fig. 5.
Alkaline monoclonal
with rabbit OIl
the
84
anti-mouse
the
resting
l)re5efl(e
Journal
phosphatase antibody
on lBl2
antibody neutrophil of alkaline
the surface of neutrophils. against alkaline phosphatase.
followed (Fig.
4),
phosphatase
of Leukocyte
by the
protein
plasma on
Biology
A gold-5. membrane
the
plasma
Volume
Neutrophils The cells and has
processed become
membrane
56,
July
for very
in
were were
transmission irregular
a random
1994
stimulated then fixed
with l0 M fMLP in 2% formaldehyde, electron
with distribution.
large
microscopy. extensions
x30,000.
for
10 mm at 37#{176}C, chilled 0.05% glutaraldehyde,
Note or
ruffles.
that The
instead immunogold
ofthe
to 4#{176}C,and immunolabeled small label
microvilli (arrows)
labeled with found indicates
phosphatase
(alkaline
secretory
vesicles
phosphatase [26]).
Now,
present
on
complete
the
inside
colocalization
of of
Mac-i and L-selectin in the plasma membrane is observed as a result of translocation of Mac-i from secretory vesicles to the plasma membrane, whereas the main pant of Mac-i present in specific/gelatinase granules is unchanged. The level of L-selectin is reduced as a result of stimulationinduced shedding, the mechanism of which is still unclear [33]. This demonstrates that secretory vesicles, although endocytic in origin [27], are not simply inside-out plasma membrane vesicles but are organelles organized with a selective membrane composition, highly enriched in Mac-i and cytochrome b558 relative to the plasma membrane [29, 30] and devoid of HLA and L-selectin as demonstrated here, but sharing alkaline phosphatase with the plasma membrane. Thus, the incorporation of secretory vesicle membrane into the plasma membrane can be expected to affect profoundly the profile of proteins present in the plasma membrane rather than just adding more membrane with the same protein composition. Such changes in the protein profile of the plasma membrane can be observed and quantified by immunofluorescence on single cells.
The
incorporation
plasma
membrane
against
alkaline
stimulation
may
be
of secretory
with
phosphatase.
of
with
in
results
inflammatory
controlling
in
membrane
into
a monoclonal
the
incorporation
the
antibody
(Fig.
3) that
mediators
that
It is demonstrated
neutrophils
operative
interaction
vesicle
is monitored
neutrophil-endothelial
of
secretory
vesicle
mem-
brane into the plasma membrane, as evidenced by the parallel increase in the amounts of alkaline phosphatase and Mac-i in the plasma membrane. It is observed that the amount of L-selectin is reduced following stimulation. This has previously been shown to be due to stimulation-induced shedding with
of L-selectin
exocytosis
[33].
Although
of secretory
this occurs in parallel these two phenomena do
vesicles,
not seem to be causally related because stimuli that mobilize secretory vesicles efficiently may differ in their capacity to induce shedding of L-selectin (TNF versus PAF) (Fig. 3). It has previously been shown by enzyme cytochemistry that alkaline phosphatase, the membrane marker of secretory vesicles [25-27], is localized in intracellular vesicles in unstimulated neutrophils [44] and that stimulation causes these to fuse to form intracellular tubular structures that are in communication with the cell surface [45]. Our results demonstrate
that
after
mobilization
of secretory
vesicles,
the
i...
0-
,
.
1.,
.
:
: :
.
,
‘
0. :
.
45 ,
.
,.
:
,
:: ,1
. .-i-.+
;
-
. -. .
‘t
‘
,
.
S
.
,.-.
:
e
., -. :.
“
.
.
- . Cl
._‘;
--
on the surface
antibody CBR Ml/29 with rabbit anti-mouse is found
randomly
ofneutrophils.
against the a chain antibody, followed distributed
on
both
Neutrophils of Mac-I by protein ruffles
and
were stimulated with l0 M fMLP for 10 mm at 37#{176}C,chilled (CD11b). The cells were then fixed in 2% formaldehyde, 0.05% A gold’5, and processed for transmission electron microscopy.
other
parts
of
the
plasma
membrane.
Borregaard
-
‘
4’ ‘
. _t.
Fig. 6. Mac-l
,
;,4%
\,*1.
--- I .
‘
.-.
.
.
-
-
,‘...:_,,,,_.
to 4#{176}C, and labeled with monoclonal glutaraldehyde and immunolabeled The immunogold label (arrowheads)
x 60,000.
et a!.
Human
neutrophil
adhesion
receptors
85
associated
alkaline
phosphatase
and
Mac-i
become
-independent
accessi-
ble to macromolecules such as antibodies and hence are incorporated into the plasma membrane, where they may interact with the surroundings of the cell. To further visualize this, intact cells were labeled with monoclonal antibody against L-selectin, alkaline phosphatase, or Mac-i, and the membrane topology of these proteins was determined by immunoelectron microscopy. Figure 4 confirms the localization of L-selectin on the tips of microvilli by preimbedding immunoelectron microscopy of unstimulated cells as previously demonstrated both in frozen thin sections [2] and by scanning electron microscopy [23]. Figures 5 and 6 show that both alkaline phosphatase and Mac-i are randomly distributed on the surface of fMLP-stimulated cells. We found no lar
indication structures
that alkaline as reported
phosphatase previously
5. von
J.D.,
The expert technical assistance of Charlotte Horn, Pia L. Olsen, and Yvonne Jacques is gratefully appreciated. This work was supported by the Danish Cancer Society, the Danish Medical Research Council, NIH-CA 31799 (T.A.S.), NIH-DK10486 (D.F.B.), the Novo Fund, the Lundbeck Fund, Anders Hasselbalch’s Fund, Amalie Jcrgensen’s Fund, and Ane Kathrine Plesner’s Fund. NB. is the recipient of a Neye research professorship.
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