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* Department of Morphology, Faculty of Medicine, 1211 Geneva 4, Switzerland; and Communicated by C. Ronald Kahn, Harvard Medical School, Boston,
MA, December 20, 2001 (received for review July 30, 2001)
Cell-surface microvilli play a central role in adhesion,
fusion, and signaling processes. Some adhesion and signaling receptors segregate on microvilli but the determinants of this localization remain mostly unknown. In this study, we considered CD4, a receptor involved in immune response and HIV infection, and p56Lck,
a CD4-associated tyrosine kinase. Analysis of CD4 trafficking reveals
that p56Lck binds tightly to CD4 independently of its
activation state and inhibits CD4 internalization. Electron microscopy
analysis established that p56Lck mediates CD4 association
with microvilli whereas biochemical data indicate that
p56Lck expression renders CD4 insoluble by the nonionic
detergent Triton X-100. In addition, cytoskeleton-disrupting agent
increased CD4 solubility, suggesting the involvement of cytoskeletal
elements in CD4 anchoring to microvilli. This concept was supported
further by the observation that the lateral mobility of CD4 within the plasma membrane was decreased in cells expressing p56Lck.
Finally, isolation of detergent-resistant membranes revealed that the
complex CD4-p56Lck is enriched within these domains as
opposed to conditions in which CD4 does not interact with
p56Lck. In conclusion, our results show that
p56Lck targets CD4 to specialized lipid microdomains
preferentially localized on microvilli. This localization, which
prevents CD4 internalization, might facilitate CD4-mediated adhesion
processes and could correspond to the signaling site of the receptor.
CD4 is a 55-kDa glycoprotein
expressed at the surface of various hematopoietic cells (1). In T
helper lymphocytes, CD4 plays a crucial role during antigenic
stimulation by MHC class II-bearing cells. CD4 has a dual function in
this process. First, it acts as an adhesion molecule that binds to
nonpolymorphic regions of MHC class II. Second, CD4 acts as a signal
transduction receptor by triggering the activation of the
CD4-associated tyrosine kinase p56Lck, which
modulates, in turn, signaling through the TCR (2). Whereas the
physiological role of CD4 remains mostly unknown in p56Lck-negative cells (3), a pathological role
for CD4 is well documented in all CD4-positive cells, where CD4 acts as
part of the receptor complex used by HIV to infect its target cell (4).
The p56Lck kinase is a member of the Src family
of nonreceptor tyrosine kinases expressed primarily in thymocytes and T
lymphocytes. This kinase is associated with the cytosolic side of the
plasma membrane and interacts specifically with CD4 through noncovalent bonds coordinated by a Zn2+ ion (5, 6). Although
both CD4 and p56Lck possess the necessary
determinants for their sorting, they associate early in the secretory
pathway and reach the plasma membrane together (7).
A tight regulation of CD4 surface expression is crucial to ensure a
correct immune function or efficient HIV infection (8, 9). Endocytic
processes play a primordial role in the control of CD4 surface
expression, and p56Lck is a key partner in these
events. Indeed, p56Lck inhibits CD4
internalization by preventing CD4 incorporation into clathrin-coated
pits, whereas in p56Lck-negative cells, CD4 is
internalized and recycled to the surface efficiently (10). However, the
exact mechanism by which p56Lck prevents CD4
recruitment in endocytic structures is unknown. One hypothesis is that
the CD4-p56Lck complex behaves like some tyrosine
kinase receptors (i.e., insulin/EGF receptors), which, in their
inactivated state, are anchored to microvilli and therefore are kept
away from the internalization gates. Endocytosis of these receptors
only occurs when they are activated by their ligand, which leads to
receptors' translocation to domains in which endocytosis occurs (11).
Consequently, in the present study, we examined the surface
localization of CD4 in cells expressing or not expressing
p56Lck as well as the role of
p56Lck activation in CD4 trafficking. Our results
indicate that p56Lck targets CD4 within
particular microdomains of the plasma membrane associated with
microvilli and that CD4 internalization is independent of the
p56Lck activation state.
Reagents and Antibodies.
[ Cell Culture, Plasmid Constructs, and Transfection.
The promyelocytic HL60 and CEM T cell lines were cultured in RPMI
medium 1640 supplemented with 10% FCS (GIBCO). 293T cells were grown
in DMEM (GIBCO) supplemented with 10% (vol/vol) FCS. The
p56Lck alleles used in these experiments were
described (12, 13). CD4, p56Lck,
p56LckF505, and
p56LckA273 were expressed
from the cytomegalovirus immediate early promoter, in the pCMX plasmid
vector (14). Transfections of 293T cells were performed by using the
calcium phosphate method (15).
Internalization Assays.
Internalization was assayed by using the acid-wash technique as
described (16). Briefly, cells were incubated for 2 h at 4°C
with 125I-anti-CD4 (RPA-T4), washed, and shifted
to 37°C to allow endocytosis. A percentage of
125I-anti-CD4 internalization was expressed as
the ratio of acid-wash-resistant radioactivity to total radioactivity
associated to cells at neutral pH. Alternatively, a FACS-based assay
measuring the internalization of R-phycoerythrin (RPE)-conjugated
anti-CD4 antibodies was used. Briefly, cells were incubated for 1 h at 4°C with RPE-conjugated anti-CD4 antibodies and washed, and
internalization of the immune complex was analyzed by flow cytometry as
described (17).
Immunoprecipitations.
Cells were lysed in buffer A [50 mM Tris·HCl, pH 7.4/50 mM
NaCl/10 mM MgCl2/1 mM EGTA/2 mM
VO4/2.5% glycerol/1% Triton X-100 (TX100)
and mixture of protease inhibitors] for 20 min on ice. Appropriate
antibodies were added to 500-800 µg of precleared lysates, and
immune complexes were pulled down by using protein A-Sepharose.
Immunoprecipitates were washed, resolved by SDS/PAGE, and analyzed by
Western blotting by using the enhanced chemiluminescence kit from
Amersham Pharmacia.
Kinase Assay.
293T cells were lysed 48 h after CD4 and
p56Lck cotransfection in buffer B (50 mM
Tris·HCl, pH 7.5/25 mM KCl/5 mM
MgCl2/1 mM EGTA/1% TX100 and a mixture of
phosphatase/protease inhibitors) for 20 min at 4°C.
p56Lck was immunoprecipitated, and immune
complexes were washed three times with buffer A and once in kinase
buffer (20 mM Mops/5 mM MgCl2/5 mM
MnCl2 and phosphatase inhibitors).
p56Lck coupled to Sepharose beads was resuspended
in 23 µl of kinase buffer containing 4 µCi (1 Ci = 37 GBq) of
[ Electron Microscopy (EM) Analyses.
Surface CD4 localization by autoradiography was performed as described
(16). Briefly, cells were incubated for 2 h at 4°C with
125I-anti-CD4 (RPA-T4), washed twice, and
transferred at 37°C for the indicated times. Cells then were fixed,
dehydrated, and processed for EM autoradiography. Surface CD4
localization by immunogold complexes was performed as described (16).
Briefly, cells were incubated for 90 min at 4°C with Leu-3a anti-CD4,
washed, and incubated a second time with an anti-mouse IgG coupled to
10-nm colloidal gold particles for 90 min at 4°C. Cells then were
washed, fixed, dehydrated, and processed for EM analyses. The ratio of villous vs. nonvillous plasma membrane was determined as described (16).
FACS Analysis.
CD4 solubility in TX100 was assessed as described (18) with minor
modifications. Briefly, cells were labeled with FITC-conjugated anti-CD4 at 4°C in buffer C (10 mM Tris·HCl, pH 8.0/150 mM
NaCl/2 mM MgCl2/2 mM EGTA/1% BSA) for 45 min. Cells then were washed twice, incubated 15 min at 4°C with or
without the addition of 1:10 (vol/vol) of buffer C containing 10%
TX100, and analyzed immediately by flow cytometry. Cytochalasin D
treatment (5 µg/ml, 30 min at 37°C) was performed before CD4
labeling with the FITC-conjugated antibody.
Fluorescence Recovery After Photobleaching (FRAP).
FRAP analysis was performed as described (19) with minor modification.
Cells were labeled with FITC-conjugated anti-CD4 antibodies in cold
KGR+ buffer (Krebs-Ringer phosphate buffer, pH 7.3/10 mM glucose/1
mM CaCl2/1 mM MgCl2), washed, and
processed for fluorescence microscopy analysis. Fluorescently labeled
receptors were photobleached with an argon laser at 488 nm. The ×63
oil-immersion planachromatic objective used gave an estimated bleach
spot radius (w) of 0.89 mm at 1/e2 intensity. The diffusion
coefficient (D, ×10 Isolation of Detergent-Resistant Membranes (DRMs).
DRMs were isolated as described (22). Briefly, cells (25 × 106) were solubilized for 30 min on ice with 1 ml
of TNE buffer (10 mM Tris·HCl, pH 7.5/150 mM NaCl/5 mM EDTA
and a mixture of protease inhibitors) containing 1% TX100. Precleared
lysates were adjusted to 40% sucrose and overlaid with 5 ml of 30%
sucrose and 2 ml of 5% sucrose solution prepared in TNE. Samples were
ultracentrifuged in a SW41Ti rotor (Beckman) for 18 h at
200,000 × g. Two-milliliter fractions were collected
from the top and TCA-precipitated. The samples then were processed for
SDS/PAGE and Western blot analysis.
Metabolic Labeling.
Labeling of cells with [3H]palmitic acid was
performed as described (23) with minor modifications. Cells were
labeled with 0.5 mCi/ml of [3H]palmitic acid
for 5 h at 37°C in RPMI medium 1640, washed twice with PBS, and
lysed with 1 ml of buffer D (10 mM Tris·HCl, pH 7.4/1% Nonidet
P-40/0.4% deoxycholate/66 mM EDTA/10 mM
1,10-O-phenanthroline). SDS (0.1%) was added to precleared
lysates, and CD4 was immunoprecipitated by using the OKT4 anti-CD4
antibody. Immunoprecipitates were analyzed by SDS/PAGE and fluorography.
Inhibition of CD4 Endocytosis by p56Lck Is Independent
of p56Lck Kinase Activity.
Studies in cells coexpressing p56Lck and CD4
showed that p56Lck inhibits CD4 internalization
by preventing CD4 interaction with clathrin-coated endocytic structures
(10). In the present study, we assessed whether a similar regulatory
p56Lck function occurs in lymphoid cell lines
naturally expressing p56Lck. CD4 internalization
was measured in p56Lck-positive
CD4+ CEM T lymphocytes and
CD4
Cell Biology
p56Lck anchors CD4 to distinct microdomains
on microvilli
,,
,, and Department of Health and Environment,
Faculty of Health Sciences, S-581 85 Linköping, Sweden
Abstract
Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
Introduction
Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
Materials and Methods
Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
-32P]ATP was purchased from Amersham
Pharmacia, and [3H]palmitic acid was purchased
from NEN. Other chemicals were of analytical grade and obtained from
Fluka or Sigma. Polyclonal anti-CD4 antibody used for Western analysis
was provided by the National Institutes of Health AIDS Research and
Reference Reagent Program (Rockville, MD). R-phycoerythrin- and
FITC-conjugated mAbs to CD4 were purchased from Dako; RPA-T4 was
purchased from PharMingen; Leu-3a, from Roche Molecular Biochemicals;
OKT4, from Ortho Diagnostics; mAbs to p56Lck were
purchased from Santa Cruz Biotechnology; mAbs to CD71, from Zymed, and
polyclonal antibodies to AlkP, from Rockland (Gilbertsville, PA).
-32P]ATP (5,000 Ci/mmol) and 5 µg of
acid-denatured enolase as exogenous substrate and incubated for 20 min
at 30°C. Products of the kinase reaction were resolved by SDS/PAGE
and analyzed by autoradiography.
10
cm2/s), denoting the rate of receptor diffusion
at 37°C, was calculated according to ref. 20, and the mobile fraction
(R, %), reflecting the proportion of mobile receptors, was determined
according to ref. 21.
Results
Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
Namalwa B lymphocytes stably transfected
with CD4 and in p56Lck-negative
CD4+ cell lines (HL60 promyelocytes and U937
monocytes). Our results support a
p56Lck-dependent inhibition of CD4
internalization in hematopoietic cell lines naturally expressing the
kinase (Fig. 1A).
View larger version (41K):
[in a new window]
Fig. 1.
p56Lck prevents CD4 endocytosis independently of the kinase
activation state. (A) Rates of CD4 internalization were
calculated based on the percentage of the total cell-associated
radioactivity incorporated after 5 min at 37°C by using iodinated
anti-CD4 antibodies as described in Materials and
Methods. (B) Kinase activity of
p56Lck mutants was assessed in a kinase assay monitoring
phosphorylation of enolase as a substrate. As a control of the
reaction, 2 µM PP2 was used to inhibit the reaction. Data are
representative of three independent experiments. (C)
Internalization of CD4 in 293T cells expressing p56Lck
mutants by using a FACS-based assay as described in Materials
and Methods. Data are means ± SE of four independent
experiments. (D) p56Lck association with CD4
in 293T cells cotransfected with CD4 and p56Lck mutants.
Data are representative of three independent experiments.
p56Lck Anchors CD4 to Microvilli.
Previous studies suggested that p56Lck does not
simply mask an endocytosis signal but has additional effects (10). One
hypothesis is that p56Lck anchors CD4 to
microvilli, where endocytosis does not occur. We thus investigated the
native distribution of CD4 at the ultrastructural level in CEM
(p56Lck+) and HL60
(p56Lck) cells, which represent the most
extreme phenotypes in terms of constitutive CD4 internalization (Fig.
1A). CD4 was tagged with
125I-labeled anti-CD4 antibodies and localized by
quantitative EM autoradiography (Fig.
2A). At 4°C, approximately
45% and 20% of the labeling was found associated with microvilli in
CEM and HL60 cells, respectively (Fig. 2B). At
37°C, CD4 remains associated with microvilli on CEM cells whereas it
redistributes almost exclusively to the nonvillous surface in HL60
cells (Fig. 2B). Because the ratio of villous
membranes vs. planar membranes is similar in CEM and HL60 cells
(34.2 ± 1.6% and 29.6 ± 2.1% of villous membranes, respectively), CD4 concentrates (up to 1.5-fold) on microvilli in
p56Lck-positive cells whereas it preferentially
associates with planar domains in p56Lck-negative
cells.
|
The CD4-p56Lck Complex Interacts with Cytoskeletal
Elements.
Microvilli are characterized by a dense cytoskeleton core made of a
bundle of actin and its associated proteins (26). This suggests that
molecules associating with microvilli might interact with cytoskeletal
elements and, thus, be insoluble by nonionic detergent such as TX100 at
4°C. We thus investigated CD4 and p56Lck TX100
solubility and observed that CD4 and p56Lck are
mostly insoluble by TX100 in CEM cells whereas, in
p56Lck-negative HL60 cells, CD4 displays an
opposite pattern of solubility (Fig.
3A). Similar results were
obtained by using a FACS-based assay to quantitate the extent of CD4
solubility (Fig. 3B). In CEM cells, 45% of the initial CD4
labeling remained associated with cells after solubilization but this
value dropped to 15% in HL60 cells (Fig. 3C). Of note, the
percentage of CD4 insolubility correlates closely to the percentage of
CD4 association with microvilli (see Fig. 2B). In
addition, cytochalasin D, which prevents actin polymerization but does
not disrupt the p56Lck-CD4 complex, increases to
80-85% of the TX100-soluble CD4 fraction in both cell types,
indicating that disruption of the cytoskeleton renders CD4 soluble to a
similar extent in p56Lck-positive and
p56Lck-negative cells (Fig. 3C).
|
Lateral Mobility of CD4 Is Restricted in p56Lck-Expressing Cells. To further support a role of p56Lck in anchoring CD4 to particular domains/structures of the plasma membrane, the lateral mobility of CD4 in the plane of the plasma membrane was measured by FRAP analysis. As shown in Fig. 4, in CEM cells, the lateral diffusion coefficient of CD4 at 37°C is 3- to 4-fold lower than in HL60 cells, suggesting that p56Lck restricts CD4 mobility in the plasma membrane. The mobile fraction, in contrast, was lower in HL60 cells than in CEM cells, which could be related to the segregation of a large fraction of CD4 in clathrin-coated pits under these conditions.
|
p56Lck Mediates CD4 Association with DRMs. CD4 insolubility by TX100 at low temperature also might reflect its association with specialized lipid microdomains termed DRMs (27). CD4 and p56Lck previously have been reported to be concentrated in DRMs in T lymphocytes (28), but no information is available as to whether CD4 association with DRMs is p56Lck-dependent. To answer this question, we isolated biochemically DRMs in CEM and HL60 cells and analyzed the distribution of CD4 and p56Lck within these microdomains. Alkaline phosphatase (AlkP), a glycosylphosphatidylinositol-anchored protein specifically associated with DRMs, and the transferrin receptor (CD71), a transmembrane molecule excluded from DRMs, were used as markers of the fractionation procedure. As shown in Fig. 5A, CD4 and p56Lck are present in DRMs in CEM cells. However, in HL60 cells, CD4 was undetectable in DRMs, suggesting that the localization of this receptor in DRMs depended on p56Lck. In support of these data, disruption of the CD4-p56Lck complex in CEM cells by 1,10-O-phenanthroline substantially shifted CD4 out of DRMs whereas p56Lck remains associated with these microdomains (Fig. 5B).
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Discussion |
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Abstract
Introduction
Materials and Methods
Results
Discussion
References
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In this study, we demonstrate that the tyrosine kinase p56Lck plays a crucial role in CD4 localization and trafficking at the plasma membrane. Specifically, we reached the following conclusions: (i) p56Lck prevents CD4 internalization by maintaining this receptor on microvilli; (ii) CD4 binding to p56Lck as well as the inhibition of CD4 internalization by p56Lck are independent of p56Lck activity; (iii) p56Lck mediates CD4 association with cytoskeletal elements, CD4 localization on microvilli, and CD4 segregation within DRMs, strongly suggesting that CD4 is associated with DRMs located on microvilli; and (iv) CD4 association with DRMs/microvilli in p56Lck-expressing cells correlates with a restricted lateral mobility of CD4 in the plasma membrane.
Compartmentalization of specific signaling or adhesion molecules on microvilli is now well established. Receptor segregation on microvilli might play a role in cell-cell and cell-substratum adhesion (31, 32) as well as in membrane fusion processes (33). Why localization of adhesion/fusion molecules on microvilli is functionally relevant is not clearly understood, but the morphology and dynamic of microvilli may provide a scaffold for the presentation of these molecules and potentially could be instrumental in targeting adhesion/fusion molecules where functionally appropriate. In addition, the cylindrical shape and narrow diameter of microvilli may provide the low radius of curvature required to overcome the inherent repulsive interactions between cell surfaces during cell adhesion processes. The functional relevance of signaling receptors' association with microvilli is also unclear. We have described previously that the insulin and epidermal growth factor receptors preferentially segregate on microvillar domains in various cell types (11). In addition, G-coupled seven-transmembrane proteins such as CCR5 and CXCR4 also associate predominantly with microvilli on macrophages and lymphocytes (34). On the basis of these observations, it is tempting to speculate that such localization might favor the binding of soluble, circulating ligands and, therefore, might represent a particular surface domain involved in receptor signaling.
The localization of receptors on microvilli might reflect their tight
coupling to the cytoskeleton. Indeed, microvilli are actin-filled cell
extensions enriched in a panel of actin-associated cytoskeletal
proteins (26). In this regard, cytoskeletal proteins such as talin and
-actinin have been proposed to mediate localization of adhesion
molecules on microvilli (31, 32). Other candidates are the members of
the ERM family (35). Unfortunately, except for the epidermal growth
factor receptor, which has been shown to bind actin (36), little
information is available on potential cytoskeletal partners anchoring
signaling receptors to microvilli. Present observations showing that
the CD4 TX100 solubility is cytochalasin D-sensitive support the
concept of such an association of signaling receptors with cytoskeletal
elements on microvilli, but further studies are required to identified
the exact molecules involved.
CD4 is not only sequestered on microvilli but also concentrated in DRMs when p56Lck is expressed. Based on the observations that (i) CD4 associates with microvilli and DRMs in the same experimental conditions (time and temperature) and (ii) CD4 segregation on microvilli and in DRMs is p56Lck-dependent, we propose that CD4 associates with DRMs located on microvilli. In support of these conclusions are the recent observations that cholesterol-enriched microdomains may be linked to cytoskeletal elements through protein of the annexin family (37) and that prominin, a pentaspan membrane protein, is retained on microvilli concomitantly with a segregation in cholesterol-based microdomains (38). Thus, microvilli, possibly through their high concentration in cytoskeletal elements, could play a key role in the sorting of proteins specifically segregated in DRMs.
CD4 association with DRMs and cytoskeletal elements in p56Lck-expressing cells is corroborated further by our FRAP analysis. Indeed, interactions with the cytoskeleton and the membrane cholesterol/phospholipid ratio play a crucial role in the mobility of cell membrane glycoprotein (39, 40). Thus, the net decrease in CD4 mobility measured for cells expressing p56Lck could reflect dynamic interactions of the CD4-p56Lck complex with the cytoskeleton and/or lipids.
The concomitant localization of CD4 and p56Lck in DRMs and microvilli is consistent with previously described mechanisms leading to T cell activation. Indeed, DRMs concentrate the bulk of the signaling machinery necessary to activate T cells in response to antigen stimulation, including CD4 and p56Lck (41). Upon TCR activation, a coalescence of lipid rafts containing relevant molecules for the immune response as well as a capping of CD4 are observed (42, 43). The role of the cytoskeleton in the aggregation of other components of the TCR-signaling machinery is still unclear; however, in the case of CD4, this coreceptor is within lipid rafts and capping of this molecule depends on the cytoskeleton reorganization (18), thus establishing a link between lipid rafts as signaling platforms and the cytoskeleton. These observations raise the interesting hypothesis that plasma membrane domains highly concentrating cytoskeletal elements such as microvilli could represent potential cellular sites mediating these signaling processes.
How does p56Lck direct CD4 to DRMs/microvilli? p56Lck interacts with CD4 early in the secretory pathway, and both reach the plasma membrane together (44). Consistent with our data suggesting that p56Lck mediates CD4 segregation on microvilli/DRMs, p56Lck targeting to the plasma membrane and association with DRMs occur independently of CD4 expression, indicating that p56Lck contains the determinants necessary to localize in DRMs (7, 44). One of these determinants is likely to be posttranscriptional modifications such as myristoylation or palmitoylation (45, 46). Indeed, p56Lck palmitoylation has been shown to be crucial to allow p56Lck association with CD4 and membranes (44, 47). However, in the case of CD4, palmitoylation of the molecule does not correlate with segregation within DRMs in p56Lck-negative cells, and, thus, palmitoylation does not appear to be sufficient to trigger association with DRMs. These observations could appear in contradiction with those of Arcaro et al. (29), who suggested that CD8 palmitoylation is necessary to target CD8 to DRMs and to mediate the interaction with p56Lck. However, in light of our results, it is possible that unpalmitoylated CD8 could not associate with DRMs because it cannot interact with p56Lck. Thus, taken together, the present and previous studies support a model in which palmitoylation of CD4 might be crucial to allow interaction with p56Lck along the secretory pathway and traveling of the complex to the plasma membrane. However, targeting of these complexes to DRMs likely is due only to p56Lck potentially through the presence of other determinants in p56Lck such as myristoylated moieties.
In p56Lck-positive cells, CD4 has to translocate
out of DRMs and slide out of microvilli to be internalized by
clathrin-coated pits (48). Physiologically, CD4 internalization in T
lymphocytes occurs in response to antigenic stimulation, a process
initiated by p56Lck activation subsequently to
CD4 and TCR binding to MHC II (24). By analogy with tyrosine kinase
receptors (49), we hypothesized that activation of
p56Lck could trigger the dissociation of the
CD4-p56Lck complex, leading to CD4 translocation
and internalization. However, we observed that
p56Lck activation does not result in the
p56Lck-CD4 complex dissociation and CD4
internalization is not induced. In addition, the stability of the
p56Lck-CD4 complex is not dependent on the lipid
raft or cytoskeleton integrity because neither cytochalasin D nor
cyclodextrin affects the complex stability (data not shown). Thus, it
is likely that p56Lck-independent signaling is
responsible for inducing CD4-p56Lck dissociation
and CD4 internalization. An interesting candidate is protein kinase
C-, which, in response to phorbol 12-myristate 13-acetate, induces
CD4 internalization by dissociating the
CD4-p56Lck complex in DRMs and promoting CD4 (but
not p56Lck) translocation out of these domains
(50).
The physiologic role of CD4 in p56Lck-negative cells remains an open question. Signaling through CD4 independently of p56Lck has been described, but information is still fragmentary and no consensus function for CD4 has been reached (3). However, our data and others (51), indicating a different CD4 localization and trafficking in p56Lck-negative cells as compared with T lymphocytes, presume a distinct function for CD4 and raise exciting questions for specialists working on hematopoiesis and macrophage function.
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Acknowledgements |
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We thank G. Porcheron-Berthet and C. Giroud for technical assistance as well as Dr. K.-E. Magnusson for valuable discussions. This work was supported by Fonds National Suisse pour la Recherche Scientifique Grants 31-55170.98, 31-53686.98, and 31-65392.01; the Swedish Medical Research Council (Project 6251); and by the Swedish Research Council for Engineering Sciences (Project 230-99-392).
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Abbreviations |
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DRMs, detergent-resistant membranes; TX100, Triton X-100; EM, electron microscopy; FRAP, fluorescence recovery after photobleaching.
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Footnotes |
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M.F. and M.-A.P. contributed equally to this work.
§ To whom reprint requests should be addressed at: Department of Morphology, Centre Médical Universitaire, 1 Rue Michel-Ser-vet, 1211 Geneva 4, Switzerland. E-mail: jean-louis.carpentier{at}medecine.unige.ch.
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References |
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Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
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