(Received for publication, January 14, 1997, and in revised form, May 23, 1997)
From the Laboratoire d'Immunologie des Infections
Retrovirales, CNRS ERS155, Institut de Biologie, 34060 Montpellier,
France, the ¶ Centre d'Immunologie de Marseille Luminy, 13288 Marseille, France, the ** Génétique Moléculaire et
Biologie du Développement, CNRS
UPR 420, 94801 Villejuif , France, and the
Department of Pharmacology, School of
Medicine, University of Pennsylvania, Philadelphia,
Pennsylvania 19104-6082
The role of CD4 during the human immunodeficiency
virus type 1 (HIV-1) life cycle in T cells is not restricted to binding functions. HIV-1 binding to CD4 also triggers signals that lead to
nuclear translocation of NF-B and are important to the productive infection process. In addition to its cytoplasmic tail, in the ectodomain, the immunoglobulin (Ig) CDR3-like region of CD4 domain 1 seemed to play a role in this cascade of signals. We demonstrate in
this work that the structural integrity of the CDR3-like loop is
required for signal transduction. Substitutions of negatively charged
residues by positively charged residues within the CDR3-like loop
either inhibited NF-
B translocation after HIV-1 and gp120-anti-gp120 immune complexes binding to E91K,E92K mutants or induced its
constitutive activation for E87K,D88K mutants. Moreover, A2.01-3B
cells expressing the E91K,E92K mutant exhibited a lower
HIV-1Lai replication. These cells, however, expressed
p56lck, demonstrated NF-
B translocation upon PMA
stimulation, bound HIV-1Lai envelope glycoprotein with high
affinity, and contained HIV-1 DNA 24 h after exposure to virus.
E91K, E92K, and E87K,D88K mutant CD4 molecules were unable to bind a
CD4 synthetic aromatically modified exocyclic, CDR3.AME-(82-89), that
mimics the CDR3-like loop structure and binds to native cell surface
CD4. This result together with molecular modeling studies indicates
that the CDR3.AME-(82-89) analog binds to the CDR3-like loop of CD4
and strongly suggests that this region represents a site for CD4
dimerization. The negative charges on the CDR3-like loop thus appear
critical for CD4-mediated signal transduction most likely related to
CD4 dimer formation.
The CD4 molecule is an integral membrane glycoprotein that
contains four extracellular domains (D1-D4) showing structural homology with immunoglobulin V regions (1, 2). This molecule plays a
key regulatory role in the immune system by stabilizing MHC1 class II·T cell
receptor complex interactions (3-5) and also by acting as a
signal-transducing molecule during T cell activation (6, 7), by its
association with the protein-tyrosine kinase p56lck.
Beside its physiological function, CD4 is known to be the primary high
affinity cellular receptor for HIV-1. The virus outer envelope
glycoprotein (HIV-1gp120env) can bind to a protruding ridge
located within the IgV-like D1 domain of CD4 at the CDR2-like region
(8, 9). Increasing evidence indicates that the role played by CD4
during the HIV-1 life cycle in T cells is not limited to its ability to
serve as a receptor for the virus but probably plays other roles that
are important to the productive infection process. Indeed, it has been
found that transfected cells expressing mutated forms of CD4 that lack
the cytoplasmic domain are fusion competent and yet present a defect in
a latter stage of HIV-1 replication cycle which results in delayed
HIV-1 production (10-12). Further studies have demonstrated that
truncation of CD4 cytoplasmic domain blocks NF-
B translocation
induced by HIV-1-mediated oligomerization of native CD4, leading to the
conclusion that under certain circumstances HIV-1 can take advantage of
the signal transduction function of CD4 to prepare the cell for
postfusion events (13, 14). More recently, we have shown that HIV-1
binding to CD4 at the surface of peripheral blood mononuclear cells
activates tyrosine phosphorylation of a number of transducing proteins,
including phosphatidylinositol 4-kinase and mitogen-activated protein
kinase-2 which are possible intermediates in the activation pathway(s)
that regulates the activity of the viral promoter (15) and activates
NF-
B and AP-1 transcription factors (16).
Although the CDR3-like loop in D1 of CD4 plays no role (17) or a minor
role (18) for HIV-1 entry, this region may play an important role
during HIV-1 replication. This was suspected from antiviral properties
of antibodies directed to this region of D1 (17) and synthetic peptides
resembling the CDR3-like loop (19). More recently, we have demonstrated
that anti-CD4 mAb specific for the CDR3-like region inhibited HIV-1
promoter activity and HIV transcription in cells containing an
integrated provirus(es) (20, 21). Moreover, these mAbs inhibit HIV-1
induced mitogen-activated protein kinase-2 activation (22) and
HIV-1-induced nuclear translocation of NF-B (23), indicating that
the CDR3-like loop is involved in signal transduction triggering T cell
activation. Based on the observation that CDR3-like loop-derived
synthetic peptide can bind CD4, it has been proposed (24) that this
region may be involved in CD4 dimerization process which may be
required for CD4-dependent T cell activation. Recently, a
constrained aromatically modified exocyclic (AME) analog that mimics
the CDR3-like loop secondary structure, CDR3.AME-(82-89), was shown to
inhibit CD4-MHC class II binding and T cell activation (25). Since the
CDR3.AME analog binds to cell surface CD4 molecules it has been
proposed that the AME prevents the formation of an essential
homodimeric surface involving the CDR3-like region of CD4 (25).
Here we investigated further the structural requirements of the
CDR3-like loop responsible for the cascade of signal transduction events that lead to NF-B translocation after HIV-1 binding to CD4
and probed the role played by the negative charges in this region by
using a series of A2.01 T cell clones expressing different mutants of
CD4. We demonstrate that the negatively charged residues at positions
87, 88, 91, and 92 in the CDR3-like loop play a critical role during
the initiation of the activation signal transduction and in the binding
of the CDR3.AME-(82-89) analog to CD4. Moreover, molecular modeling
data show that the CDR3.AME-(82-89) analog can bind to the CDR3-like
loop and indicate that residues 87, 88, 91, and 92 are essential for
CD4 dimerization.
Monoclonal Antibody, Peptide, and Other Reagents
Anti-CD4 mAbs 13B8-2/IOT4A (IgG1), specific for the CDR3-like loop, and BL4/IOT4 (IgG2a) which binds to the D1-D2 of CD4 were provided by M. Hirn (Immunotech, Marseille, France); ST40/F142.63 (IgG1) which binds to the CDR3-like loop was provided by D. Carrière (Sanofi Corp., Montpellier, France); Leu 3a (IgG1) specific for the CDR2-like loop and FITC-conjugated OKT4 were purchased from Becton Dickinson (Erembodegem-Aalst, Belgium) and Ortho Diagnostics Systems (Raritan, NJ), respectively. Anti-p56lck mAb (3A5) was purchased from TEBU (Le Perray en Yvelines, France); anti-actin (C4) mAb was from ICN Biomedicals Inc. (Costa Mesa, CA). Anti-HLA class I mAb (B9-12-1) was provided by M. Hirn (Immunotech). FITC-labeled goat anti-mouse (GAM) immunoglobulins were purchased from Immunotech. Recombinant soluble CD4 (sCD4) was a gift from D. Klatzmann (Hôpital de la Pitié-Salpétrière, Paris, France). Purified (>90%) HIV-1 recombinant soluble envelope glycoprotein 120 (gp120) produced in baculovirus expression system was purchased from ABT (ABT Europe, London, UK). gp120-anti-gp120 immune complexes were formed by incubating 50 µl of gp120 at 100 µg/ml with 50 µl of human anti-gp120 immunoglobulins and 50 µl of sheep anti-human Ig (Amersham Corp., Buckinghamshire, UK), as described previously (17). The CD4 CDR3.AME-(82-89) analog was synthesized by solid phase methods as described previously (25). Fluoresceinated CDR3.AME-(82-89) analog was prepared using FITC kit (Boehringer Mannheim). Phorbol myristate acetate (PMA) was purchased from Sigma and was used at 10 ng/ml in cell cultures.
Cells and Viruses
The A3.01 (a CD4 positive cell line) (26) was provided by T. Folks (Center for Disease Control, Atlanta, GA). The previously described (12) A2.01/CD4 cells expressing the wild type CD4 and A2.01/CD4.403 cells expressing a truncated form of CD4 were provided by D. Littman (New York, NY). The A2.01 cell clones transfected with the wild type CD4 or CD4 mutants in the Ig CDR3-like loop were previously described (18). Briefly, mutations were introduced in the CD4 cDNA by site-directed mutagenesis, and then the mutated sequence was substituted into the full-length CD4 cDNA present in the retroviral vector pMV7, and A2.01 cells were transfected with the mutant CD4 cDNA using a retrovirus shuttle. A2.01-c26 was transfected with the wild type CD4 gene but fails to express CD4 although it is neomycin-resistant. A2.01-M1 clone expresses CD4 mutant E87G, A2.01-M2 mutant Q89L, A2.01-2B the double mutant E87K,D88K, and A2.01-3B clones (A2.01-3B-1 and A2.01-3B-2, respectively) the double mutant E91K,E92K. Cells were cultured at a density of 5 × 105 per ml in RPMI 1640 medium containing penicillin/streptomycin antibiotic mixture, glutamax, and 10% fetal calf serum (Life Technologies, Inc., Eragny, France), in a 5% CO2 atmosphere. G418 (Life Technologies, Inc.) at 1 mg/ml was added to the culture medium of transfected A2.01 cells. The origin of CEM and MT2 cells was described previously (23).
Viral stocks (HIV-1Lai) were prepared from the chronically
infected CEM cell supernatants, as described previously (27), and kept
frozen at 80 °C until use. After thawing, 100 µl of these stock
viruses at 103 × TCID50 (50% tissue culture
infective dose)/ml was used for infection assays. Heat-inactivated
virus was prepared by incubation for 30 min at 56 °C.
HIV Infection Assay
Cells (5 × 105) were incubated for 30 min at 4 °C in flat-bottom 96-microwell plates (cell culture top performance product (TPP)) with 100 µl of HIV-1 at 103 × TCID50 per ml. Thereafter, cells were washed five times and cultured at 37 °C in 24-microwell plates (TPP). The amount of virus produced by the cells was monitored twice a week by measuring reverse transcriptase activity in 1 ml of cell-free culture supernatant, as described previously (27).
Flow Cytometry Analysis
Cells (1 × 105) were incubated for 1 h at 4 °C with PBS containing 0.2% BSA (PBS-BSA) or PBS-BSA supplemented with anti-CD4 mAb at concentrations necessary for saturation of cell surface CD4. After washing three times with PBS-BSA, bound mAb was revealed by addition of 50 µl of a 1:50 dilution of fluoresceinated GAM Ig (Immunotech). After 30 min staining, cells were washed with PBS-BSA, and fluorescence intensity was measured on an EPICS cytofluorometer (Coulter, Margency, France). In some experiments, cells (1 × 106) were incubated for 2 h at 37 °C with 10 µl of gp120 solution (100 µg/ml), washed, and incubated for an additional 1 h at 4 °C with 50 µl of anti-gp120env mAb 110-4 (28) solution (10 µg/ml). Bound gp120-antibody complexes were revealed by FITC-labeled GAM Ig probe as above. In another set of experiments, A2.01, A2.01/CD4, A2.01-2B, and A2.01-3B T cell lines (2 × 105) were incubated with FITC-conjugated CDR3.AME-(82-89) analog diluted at 1:50 in PBS-BSA or with a FITC-conjugated anti-CD4 mAb OKT4 for 1 h at 4 °C and then washed in cold PBS-BSA. Background staining was assessed with a FITC-conjugated mAb specific for chicken Ig (Sigma).
Reverse Transcriptase-Polymerase Chain Reaction (PCR)
PCR detection of reverse-transcribed RNAs was performed
according to the previously published procedure with slight
modifications (17). Briefly, total RNA was extracted in guanidinium
thiocyanate from 4 × 106 cells and resuspended in 40 µl of H2O, 0.1% diethyl pyrocarbonate. To reduce the
amount of DNA originating from lysis, supernatants were treated with
RNase-free DNase (Boehringer Mannheim, 10 units/ml) for 30 min at
20 °C and then for 5 min at 65 °C. To 2 µg of RNA sample (10 µl) was added 200 ng of oligo(dT) primer (1 µl) for 10 min at
65 °C. Each sample was made up with reaction buffer (50 mM Tris-HCl, pH 8.3, 30 mM KCl, 8 mM MgCl2, 9 mM DTT, 320 nM dNTPs) to a final volume of 25 µl and supplemented
with 20 units of RNase inhibitor (Boehringer Mannheim) and 25 units of avian myeloblastosis reverse transcriptase (Boehringer Mannheim), and
then incubated for 90 min at 42 °C. PCR were carried out on 4 µl
of sample supplemented with an amplification mixture containing the
p56-I/p56-II or TK I/TK II oligonucleotide primer pair (23), and 2 units of Taq DNA polymerase. The amplification reaction was
run in a PHC2 thermal cycler (Techne, Cambridge, UK). The amplified
products were electrophoresed in a 2% agarose gel, blotted for 2 h onto Hybond N+ membrane (Amersham Corp.), and hybridized
with -32P-labeled p56lck probe prepared from
pGEX2t-lck vector provided by S. Fisher (ICGM, Paris). A similar method
was used for detection of HIV-1 mRNAs using the M671/VPR3
oligonucleotide primer pair (29) and an
-32P-labeled
HIV-1 probe.
PCR Analysis of HIV-1 DNA
HIV-1 DNA was monitored by PCR analysis (see above) using the
M667/M668 oligonucleotide primer pair (20). The PCR was performed on
total DNA extracts (1 µg) prepared from cells at 24 h following virus exposure. The amplified products were electrophoresed, blotted, hybridized with an -32P-labeled HIV-1 probe, and
visualized by autoradiography.
Western Blot Assay
Cellular lysates were electrophoresed onto 12.5% SDS-polyacrylamide gel electrophoresis and blotted to polyvinylidene difluoride membrane (Millipore). The blot was then incubated for 1 h at room temperature with a blocking solution (PBS containing 10% milk and 0.05% Tween 20) prior to addition of mAb. After 1 h at 20 °C, the blot was washed three times with PBS, 0.05% Tween 20 and incubated for 30 min with 1:5000 dilution of GAM Ig peroxidase conjugate (Immunotech). After 3 washes, bound mAb was detected by incubating the membrane for 1 min with ECL reagent (Amersham Corp.). The membrane was then exposed for 0.5-5 min to hyperfilms-ECL (Amersham Corp.).
NF-B Electrophoretic Mobility Shift Assay (EMSA)
Nuclear extracts were prepared as described previously (13).
Briefly, cells (2 × 106) were centrifuged,
transferred into 1.5-ml Eppendorf tubes and washed 3 times in PBS by
centrifugation at 2,000 rpm for 10 min at 4 °C. The pellet was
resuspended in 400 µl of buffer A (containing 10 mM KCl,
2 mM MgCl2, 0.1 mM EDTA, 1 mM DTT, 0.1 mM phenylmethylsulfonyl fluoride, 4 µg/ml leupeptin, and 10 mM Hepes, pH 7.8). After 15 min
on ice, 50 µl of a solution of 10% Nonidet P-40 was added to the
sample, and cells were homogenized by vortexing and microcentrifuged at
4 °C for 30 s. The pellets were resuspended in 100 µl of
buffer B (containing 50 mM KCl, 300 mM NaCl,
0.1 mM EDTA, 1 mM DTT, 0.1 mM
phenylmethylsulfonyl fluoride, 4 µg/ml leupeptin, 10% glycerol, and
50 mM Hepes pH 7.8) and incubated for 20 min at 4 °C on
a shaker. The nuclear extracts were microcentrifuged at 4 °C for 5 min, and the supernatants were stored at 80 °C until used. The
NF-
B mobility shift assay was performed using 2 µg of protein of
nuclear extract, 1 × 105 cpm of
32P-labeled probe (a double-stranded oligonucleotide
NF-
B with a HIV-1 sequence: sense strand only, 5
-GCTGG GGACT TTCCA
GGGAG GCGT-3
) in buffer C (containing 100 mM KCl, 1 mM DTT, 1 µM ZnSO4, 20%
glycerol, 0.01% Nonidet P-40, and 50 mM Hepes pH 7.9),
supplemented with BSA, tRNA, and poly(dI-dC) in a final volume of 20 µl. After 20 min at room temperature, the mixture was run at 120 V in
a 10% polyacrylamide gel. Sp-1 mobility shift assay was performed using a double-stranded oligonucleotide probe (sense strand only, 5
-GGAGG CGTGG CCTGG GCGGG ACTGG GGAGT GGCGA-3
).
Molecular Modeling
Construction of MutantsMolecular modeling was carried out using QUANTA (Molecular Simulations, Inc., Cambridge, MA). The coordinates of CD4 were obtained from Brookhaven Protein data base (30), and the solvent molecules were removed. The mutant models were minimized while holding the remainder of the structure fixed except CDR3-like region, preserving the overall structure. The entire structure was subjected to conjugate gradient energy minimization for 2000 cycles to convergence, followed by an equilibration and production run of molecular dynamics at 300,000 for 60 ps. Molecular dynamics was performed to allow a change in the conformation in the loop, if more favorable. All energy calculations were performed at a dielectric constant of 1. Final energy values were calculated using CHARMm which is part of QUANTA. Electrostatic calculations were performed with GRASP (31). Charged amino acid groups were assigned full charges as provided in GRASP. The electrostatic calculations were performed with distance-dependent dielectric constants from 1, at the interior, to 80, at the outer surface.
Positioning of AME Cyclic PeptideThe CDR3-AME cyclic peptide adopts very similar conformation of the native CDR3 loop of CD4 (25). A dimeric model of CD4 was built with D1 as dimeric interface using an antibody VH-VL domain as template. The CDR3-AME peptide was positioned by superimposing the CDR3-AME to the CDR3 of one of the dimeric molecule. Since this region is solvated, no attempt was made to dock this peptide to the CD4 molecule. The positioning was done only for reference purpose.
To analyze whether the CDR3-like region in the
first extracellular domain of the CD4 molecule may be involved in
HIV-1-induced NF-B translocation, we used a series of CD4 mutants
that have been recently constructed (18) and were stably expressed in the A2.01 T cell line, a CD4 negative line derived from the CD4 positive parent A3.01 (5). Fig. 1
summarizes the amino acid changes introduced in the CD4 molecule.
Mutant CD4 molecules with a substitution of Gly for Glu at position 87 (E87G) were expressed in A2.01-M1 cell line; the Q89L substitution was
expressed in A2.01-M2 and the double substitutions E87K,D88K in
A2.01-2B and E91K,E92K in A2.01-3B. A3.01 cells that express the
native CD4 molecule, A2.01-c26 which did not express CD4 although
transfected with the CD4 wild type gene, and A2.01/CD4.403 cells
expressing a truncated form of CD4 lacking the whole cytoplasmic domain
were used as controls. The CD4 phenotype of the A3.01 and A2.01 cell lines and of the different clones was studied by indirect
immunofluorescent staining and flow cytometry. Representative
cytofluorometric profiles are shown in Fig.
2. A2.01-c26 was the only clone that was
not stained with anti-CD4 mAb. All other clones expressed CD4, although there were slight variations in the level of expression; binding of
anti-CD4 mAb BL4 was found with all these cells. Binding of anti-CD4
mAb ST40 was disrupted only for clones A2.01-2B and A2.01-3B expressing CD4 molecules with the double substitutions E87K,D88K and
E91K,E92K, respectively. As shown in Fig.
3, the different clones used in this
study expressed the lck mRNA (Fig. 3A), and the p56lck protein was detected (Fig. 3B),
indicating that conditions for CD4-dependent signal
transduction through p56lck were conserved.
These results, together with previous work (18), indicate that the mutations introduced into CD4 had a local influence affecting only the CDR3-like loop structure. These mutations had no obvious effect on the conformation of domain 1.
NF-We previously
demonstrated that heat-inactivated HIV-1 (iHIV) binding to CD4 induced
NF-B activation in cells expressing wild type CD4 but failed to
induce NF-
B activation in cells expressing a truncated CD4 molecule.
To study whether such an activation signal may follow binding of
HIV-1Lai to cells expressing CD4 mutants, electrophoretic
mobility shift assays (EMSA) were performed. As shown in Fig.
4A, a shift of labeled NF-
B
oligonucleotide was observed when mixed with nuclear extracts from
A3.01 (lane 2), A2.01-M2 (lane 10), and A2.01-M1
(lane 12), exposed to iHIV. In contrast, no
protein·NF-
B oligonucleotide complex was found when the
oligonucleotide was mixed with nuclear extracts from A2.01/CD4.403
cells (lane 4) or A2.01-3B exposed to iHIV (lane 6). Similar results were obtained using two different clones
(A2.01-3B-1 and A2.01-3B-2) of A2.01-3B cells (Fig.
5 lanes 3-6), indicating that
the lack of activation by iHIV was likely related to the mutation in
the CDR3-like loop. Unexpectedly, the A2.01-2B cells constitutively
expressed a large amount of nuclear NF-
B (Fig. 4A, lane
7), and no detectable increase of nuclear NF-
B was observed after iHIV binding to this CD4 mutant (Fig. 4A, lane 8).
Such observation was reproducible using two different clones
(A2.01-2B-1 and A2.01-2B-2) of A2.01-2B cells (Fig. 5, lanes
7-10).
As shown above (see Fig. 3), A2.01-3B cells express p56lck and
therefore should be able to transduce CD4-dependent signals
stimulating NF-B translocation. To confirm that the lack of NF-
B
translocation in A2.01-3B can be ascribed neither to a defect in the
ability of the A2.01-3B clones to translocate NF-
B nor to a lack of
gp120 binding to the E91K,E92K mutant CD4 molecule, two sets of
experiments were performed. First, the ability of A2.01-3B cells to
translocate NF-
B after stimulation with PMA was tested using EMSA.
As shown in Fig. 6, PMA induced a shift
of labeled oligonucleotide migration when mixed with nuclear extracts
from A3.01 and A2.01-3B cells (lanes 4 and 8,
respectively). In addition, NF-
B translocation was found with
extracts from A3.01 cells exposed to iHIV (lane 2) but was
not found with extracts from A3.01 cells exposed to iHIV previously
incubated with 10 µg/ml sCD4 for 2 h at 37 °C (lane
3), indicating that induction of NF-
B translocation following A3.01 cell exposure to iHIV required interaction between HIV-1 and cell
surface CD4. Next, we compared the ability of the A3.01, A2.01, and
A2.01-3B clones to bind recombinant gp120 envelope glycoprotein
(gp120) from HIV-1Lai. As shown in Fig.
7, gp120 binds to A2.01-3B clone to the
same extent as to the A3.01 clone. The weak binding of gp120 to A2.01
cells that lack CD4 expression suggests that a fraction of recombinant
gp120 binds to target cells independently of CD4 recognition and should
be therefore considered as background.
We have previously reported that gp120-anti-gp120 immune complex
binding to wild type CD4 expressed at the surface of peripheral blood
mononuclear cells induced NF-B translocation similar to that induced
by iHIV-1 (16). Since gp120 was found to bind A2.01-3B (see Fig. 7),
we assessed whether gp120-anti-gp120 immune complexes were able to
stimulate NF-
B translocation in these cells. As shown in Fig.
8, we observed a shift of labeled
oligonucleotide migration when mixed with nuclear extracts from A3.01
and A2.01-3B cells exposed to PMA (lanes 5 and
10, respectively). NF-
B translocation was also observed
with extracts from A3.01 cells exposed to iHIV (lane 2) and
gp120-anti-gp120 immune complexes (lane 4) but was not found
with extracts from A2.01-3B cells exposed either to iHIV (lane
7) or gp120-anti-gp120 immune complexes (lane 9).
These results indicate that the integrity of the CDR3-like loop Glu-91,
Glu-92 residues is required to elicit NF-B activation after HIV-1-,
and gp120-anti-gp120 immune complexes binding to the CDR2-like loop in
D1 of cell surface CD4.
To assess
whether the defect of A2.01-3B cells to translocate NF-B after
HIV-1 binding may delay HIV-1 production, as demonstrated in cells
expressing mutant CD4 lacking the cytoplasmic region (13), HIV-1
replication was measured. When cells were infected at low virus input
(102 × TCID50), a low and delayed viral
replication was consistently observed in A2.01-3B and A2.01/CD4.403
cells compared with A3.01 cells and with the other CD4 mutant
expressing cells (A2.01-M1, A2.01-M2, and A2.01-2B) (Fig.
9A). To ensure that the
impaired HIV-1 production found in A2.01-3B cells could not be
ascribed to a defect in virus entry and retrotranscription in these
cells, a PCR assay was performed on the different cells 24 h after
virus exposure. As shown in Fig. 9B, HIV-1 DNA was found in
A2.01-3B cells in similar amount as in the other cell lines. Moreover, a semi-quantitative reverse transcriptase-PCR performed on A2.01/CD4 and A2.01-3B cells 72 h after virus exposure indicates that HIV-1 mRNAs were less abundant in A2.01-3B cells than in cells
expressing the wild type CD4 molecule (Fig. 9C).
Effect of substitutions in the CDR3-like loop
on HIV-1 productive infection. A, A2.01/CD4 (), A2.01-M1
(
), A2.01-M2 (
), A2.01-2B (
), A2.01-3B (
), A2.01/CD4.403
(
), A2.01 (
) cells were exposed to 100 µl of
HIV-1Lai (103 × TCID50/ml), and
virus production was followed by measuring reverse transcriptase
(RT) activity. Reverse transcriptase activity less than
1.5 × 103 cpm/ml was considered as negative
(straight line). The data have been calculated from
quadriplicate experiments. To facilitate reading of Fig. 5A,
the results of infection experiments are depicted in the form of two
separated panels and virus production in A2.01/CD4 cells and A2.01
cells is shown in both panels; for identical reasons, virus
production in A3.01 cells, which is very similar to that observed in
A2.01/CD4 cells, is not shown. B, viral DNA in HIV-1 exposed
A2.01 (lane 1), A3.01 (lane 2), A2.01/CD4
(lane 3), A2.01-M1 (lane 4), A2.01-M2 (lane
5), A2.01-2B (lane 6), A2.01-3B (lane 7),
and A2.01/CD4.403 (lane 8) cells was monitored at 24 h
following virus exposure by PCR analysis using the M667/M668
oligonucleotide primer pair. The controls PCR were performed on pBRU
plasmid (lane 9) and H20 (lane 10).
The amplified products were electrophoresed, blotted, hybridized with a
radiolabeled HIV-1 probe, and visualized by autoradiography.
C, PCR analysis of HIV-1 spliced mRNAs in A2.01/CD4 and
A2.01-3B infected cells. Total RNAs were extracted from cells 72 h after infection and retrotranscribed into DNA. PCR was then performed
using the M671/VPR3 primer pair and various dilutions of
retrotranscribed products (lanes 4-8 and lanes
11-15 corresponding to 1:1, 1:2, 1:5, 1:10, and 1:50 dilutions of
sample, respectively). The amplified fragments were hybridized with a radiolabeled HIV-1 probe and visualized by autoradiography. A control
is shown (lane 1) in which an RNA-free sample was prepared for PCR. Other controls consisted of RNA samples not submitted to
reverse transcrip-tion (lanes 3 and 10) and of
RNA extracted from uninfected cells (lanes 2 and 9). Products of PCR amplification of
retrotranscribed thymidine kinase (TK) RNA, are shown as
control.
These results indicate that substitution of positive for negatively charged residues at positions 91 and 92 within the CDR3-like loop impairs HIV-1 replication at the stage of early transcription.
Mutations in the CDR3-like Loop Affect the Binding of the CDR3.AME-(82-89) Analog to CD4 and Disrupt the Putative CD4 Dimerization RegionIn an attempt to get further insights into
the mode of action of the CDR3-like loop in signal transduction
regulation, we used a CD4 exocyclic analog, named CDR3.AME-(82-89).
This analog mimics the CDR3 loop structure and was previously shown to
inhibit CD4-MHC class II binding and antagonize CD4 function through
its binding to CD4 (25). The ability of FITC-labeled CDR3.AME-(82-89) analog to bind the wild type CD4 molecule and mutant forms of CD4 was
investigated. As shown in Fig. 10, the
FITC-conjugated CDR3.AME-(82-89) analog bound to A2.01/CD4 cells, and
its binding level was comparable to that of mAb OKT4. Conversely, no
binding to A2.01-2B and A2.01-3B cells could be detected, although
mutant CD4 molecules were strongly expressed at the surface of these cells, as evidenced by OKT4 mAb binding. Interestingly, the binding pattern of the CDR3.AME-(82-89) analog was identical to that observed with the ST40 mAb, specific for the CDR3-like region of CD4 domain 1 (see Fig. 2), suggesting that the CDR3.AME-(82-89) analog binds to
this region. No binding to CD4-negative A2.01 cells was detected.
The possibility that the CDR3.AME-(82-89) analog binds to the CDR3
loop of CD4 was further examined by computer-assisted molecular modeling studies of the interaction between this analog and the first 2 domains of CD4. As shown in Fig. 11,
A and B, the CDR3.AME-(82-89) analog
(red) was predicted to bind to the CDR3-like loop
(yellow) of CD4 (white), suggesting that the CDR3
loop represents a main dimerization site for CD4 molecules. In the
crystal structure of CD4 (11, 12), the CDR3 loop is stabilized by a
disulfide bond, salt links, and solvent molecules. Whereas the
Glu-87/Asp-88 residues from CDR3-like loop occur at the periphery of
the putative interface between the analog and CD4, residues
Glu-91/Glu-92 occur at the core of the interface. Although the
interactions cannot be docked accurately since these regions in the
crystal structure contain water molecules, hydrophobic residues at the
bottom of the peptide loop such as isoleucine at position 4 (Ile-4) and N-terminal residues would presumably interact with Ile-83 of CD4, if we
assume that the role of the peptide is to displace water. Similarly,
Tyr-12 at the top of the analog would interact with Asp-88 of CD4.
To highlight the role of Glu-87/Asp-88 and Glu-91/Glu-92 residues in CDR3.AME-(82-89) analog binding to CD4 and CD4 dimerization, mutant models of CD4 were constructed. Structural analysis reveals that in the wild type CD4 molecule (Fig. 11C, a), the conformation of the CDR3 loop is rigid and reinforced by a disulfide bond at the bottom of the loop and by several salt links. Fig. 11C shows the surface charge distribution in D1-D2 domains of CD4. Negatively charged residues (red) Glu-87/Asp-88 are located at the periphery of the putative dimeric interface (shown by circle) and are neutralized by neighboring positively charged lysine residues (Lys-90 at the interface, Lys-29, and Lys-35, below the CDR3 loop). Residues Glu-91/Glu-92 are located at the core of the putative dimeric interface and are neutralized by lysine residues from CD4 N terminus and a water molecule in the crystal structure. Mutation E87K/D88K changes the charge spectrum at the dimeric interface (Fig. 11C, b). However, the core of the interface, where Glu-91 and Glu-92 provide some stability by interacting with N-terminal lysine residues, does not show significant changes. Conversely, mutation E91K/E92K changes the charge spectrum of the interface completely (Fig. 11C, c). The interface totally becomes positively charged (blue). The mutation not only alters the electrostatic property of the dimeric interface, it potentially alters the conformation of the CDR3 loop. This change occurs through repulsion between Lys-91, Lys-92, and the neighboring N-terminal lysine residues.
These results indicate that the CDR3.AME-(82-89) analog most likely binds to cell surface CD4 CDR3-like loop and that this region is involved in CD4 dimer formation. Mutations changing both charge distribution at the interface and CDR3-like loop conformation would prevent CD4 dimerization.
We demonstrate in this study that the CDR3-like loop of CD4 domain
1 plays an essential role in the signal transduction pathway that
triggers activation of NF-B after HIV-1 binding to CD4. We show that
E91K,E92K substitutions within the CDR3-like loop result in the
inability of this mutant molecule to transduce signals triggering
NF-
B activation and also lead to impaired replication of HIV-1.
Moreover these mutations suppress the binding of the CD4
CDR3.AME-(82-89) analog, a peptide derivative that mimics the
CDR3-like loop structure and binds to native CD4, suggesting possible
role played by this region in dimer formation.
In the past few years, several studies have reported evidence
indicating that T cell activation signals are delivered to target cells
by HIV-1 antigens (32-36). Most recently, we reported that binding of
HIV-1 to the CDR2-like loop of CD4 domain 1 stimulates NF-B
translocation (13, 16) and that this event requires the integrity of
the cytoplasmic domain of CD4 (13). It is worth noting that the
interaction of Leu 3a mAb with the CDR2-like loop also triggers AP-1
translocation (36). Several reports have suggested that the "early"
HIV-1 transcription events are regulated by NF-
B protein, and the
"late" transcription events are regulated by Tat and Sp-1 (37-40).
Based on these observations, we have proposed that HIV-1 binding to
cell surface CD4 stimulates a signaling pathway(s) that results in
nuclear translocation of NF-
B and thereby regulates the early
transcription of HIV-1 (13). In agreement with this hypothesis, we have
found that viral production was delayed in cells expressing mutant
forms of CD4 that lack the cytoplasmic tail, although the rate of viral
entry and retrotranscription was apparently not different from that
found in cells expressing the wild type CD4 (10-13).
We have recently observed that binding of 13B8-2 mAb to the CDR3-like
loop of CD4 domain 1 inhibits mitogen-activated protein kinase-2
activation (22) and NF-B translocation induced by HIV-1 binding to
CD4 (23), indicating that the CDR3-like loop may play an important role
in T cell activation. To investigate this possibility, we studied the
effects of mutations affecting four negatively charged residues within
the CDR3-like region on signal transduction pathway that triggers
activation of NF-
B after HIV-1 binding to CD4 and on viral
production. The structural integrity of the CDR3-like loop mutant
molecules was established by binding experiments using a panel of CD4
mAbs (see Fig. 2). Consistent with previous results reported by one of
us who tested 9 anti-D1, 1 anti-D2, and 1 anti-D4 anti-CD4 mAbs for
binding to the mutants CD4 (18), we found no evidence of global
distortion of the CD4 conformation and no obvious effect on the
structure of D1. Moreover, these mutations do not affect the binding of gp120 to the CDR2-like loop in D1 (see Fig. 7). Only a local effect in
the CDR3-like loop was found for double substitution mutants E87K,D88K
and E91K,E92K, as detected by the loss of ST40 mAb binding to A2.01-2B
and A2.01-3B cells.
We observed that cells expressing the CD4 mutants exhibit different
ability to translocate NF-B after iHIV binding to CD4. Cells
(A2.01-3B) expressing the E91K,E92K mutant CD4 molecule were
refractory to iHIV-induced activation and exhibited a significant reduction in virus production after exposure to low concentrations of
HIV-1Lai. According to the mAb binding results, these
effects cannot be attributable to the density of CD4 molecules on the surface of the A2.01-3B cells nor to alterations of CD4 overall conformation although local conformational changes in the CDR3-like loop might play a role (see Fig. 2). They cannot be due either to an
impaired accessibility of HIV-1 to CD4 as demonstrated by efficient
binding of recombinant HIV-1Lai gp120 to A2.01-3B cells (see Fig. 6) or to a defect in p56lck expression (see Fig. 3),
or to a defect of NF-
B translocation, since NF-
B translocation
was observed under PMA stimulation (see Fig. 5). The reduction in virus
production thus apparently correlates with a defect in the capacity of
the CD4 molecule to transduce an activation signal resulting in NF-
B
translocation. The reduced reverse transcriptase activity in those
cells was more pronounced when cells were exposed to low virus input
(data not shown). Altogether these results indicate that negatively
charged residues Glu-91 and Glu-92 in the CDR3-like loop play a role in
activation signal transduction.
In contrast to A2.01-3B cells, A2.01-2B cells expressing CD4 mutant
E87K,D88K seemed to be constitutively activated and were shown to
express high amounts of nuclear NF-B in the absence of exogenous
stimuli (Fig. 4). Although this result was unexpected, it was
reproducible with two different clones of A2.01-2B cells. The fact
that two clones demonstrated similar activation status suggests that
the constitutive NF-
B translocation is probably not related to a
putative integration of the CD4 construct in the vicinity of a cellular
gene controlling cell activation. Chronic activation of these clones
was further established by flow cytometry experiments indicating that
they express elevated surface CD25 antigen.2 Interestingly, both
mutants E91K,E92K and E87K,D88K exhibited a similar loss of ST40 mAb
binding, indicating that these four negatively charged residues are
involved in the ST40 epitope but play distinct functional roles in
transduction of signals mediated by CD4.
Requirement for CD4 dimerization in transducing signals was suspected from the observation that cross-linking of CD4 can trigger autophosphorylation of p56lck (27). We found here that mutants E91K,E92K and E87K,D88K were unable to bind the CD4 CDR3.AME-(82-89) analog that mimics the CDR3-like loop and specifically binds to native CD4 (25). These results, together with molecular modeling studies, indicate that the CDR3.AME-(82-89) analog binds to the CDR3-like loop (see Fig. 11) and that residues 87/88 and 91/92 can potentially be involved in this binding. Moreover our results strongly suggest that the CDR3-like loop constitutes a primary site for CD4 dimerization. Our model shows that residues 89-93 form the core of the dimeric interface and residues 87/88 are at the periphery. The involvement of the CDR3-like region in CD4 dimerization has been previously proposed (24) based on the demonstration that CDR3-like loop-derived synthetic peptides can bind recombinant CD4 molecules. Further evidence in favor of this dimerization site has recently been obtained by some of us (25); it was found that CDR3.AME-(82-89) analog binding to CD4 inhibits CD4-HLA class II interaction and antigen-induced T cell activation, an effect consistent with prevention of CD4 homodimer formation and signal transduction.
In this regard, the defect of NF-B translocation after iHIV binding
to CD4 and the reduction in virus production generated by the E91K,E92K
mutant might result from prevention of CD4 dimerization. Indeed,
calculation for the E91K,E92K mutant drastically changes the
conformation of the CDR3-like loop. So it seems that these mutations
not only disrupt the dimerization, it can also disrupt the CDR3-like
loop. These data clearly indicate that both CD4 dimerization and
CDR3-like loop structure are essential for efficient signaling and
suggest that binding of multivalent molecules to the CDR2-like loop
would induce CD4 dimerization at the CDR3-like loop. In light of this
model, molecules that react with the CDR3-like region (20, 41-43)
might exert their anti-HIV properties by uncoupling CD4 from the signal
transduction machinery, thereby preventing cell activation. It is very
likely that the CDR3.AME-(82-89) analog would act like a "spacer"
between the CD4 dimers accounting for its inhibitory effects on T cell
activation in MHC class II restricted immune response (25) and for its
anti-HIV-1 properties (44). Other antiviral agents might exert their
anti-HIV properties by inducing conformational changes in CD4 that
block CD4 dimerization. For example, the triphenylmethane polymer ATA
that binds to part of the gp120 binding site induces conformational
changes of the OKT4E epitope that is thought to arise from the tertiary
structure of D1 through the juxtaposition of residues Gln-20, Lys-21,
and Glu-91, via the S-S bond fixing the stem of the CDR3-like loop of
D1 (45).
The opposite effects induced by the E87K,D88K mutation that seemed to
generate a constitutive activation of A2.01-2B cells, which express
high amounts of nuclear NF-B in absence of exogenous stimuli, are
intriguing. Although residues Glu-87 and Asp-88 are at the periphery of
the CD4 dimeric interface and exposed to solvents, their replacement by
lysine does not show any significant changes in the CDR3-like loop. So
it is possible that any instability caused by mutations can be
compensated either by conformation changes or by solvents. Such subtle
changes might account for the creation of new interaction sites
facilitating mutant CD4 homodimer formation and consequently,
constitutive cell activation, as detected in A2.01-2B cells. According
to this hypothesis, the presence of CD4 dimers at the cell surface
might prevent the CDR3.AME-(82-89) analog from binding to the
E87K,D88K CD4 mutant. Alternatively, subtle changes in the charge
balance might be responsible for its impaired binding. Further studies
will be needed to determine whether E87K,D88K mutations favor NF-
B
translocation or whether the two clones demonstrate high nuclear
amounts of NF-
B for another reason which remains to be
determined.
Although CD4 can likely forms dimers (46), it is not known whether a dimeric CD4 state exists at the surface of helper T cell only under certain conditions or whether there is a monomer/dimer equilibrium. Native CD4 may be normally monomeric and oligomerize by interacting with HLA class II or HIV-1. Sweet and co-workers (47) have reported crystallographic studies of sCD4 suggesting that it oligomerizes by interaction between its D3-D4 regions. Most recently, Sakihama and co-workers (48) have reached the same conclusions, based on the observation that replacement of D3-D4 domains by D1-D2 of CD4 or the extracellular domain of CD2 prevented HLA class II binding to these chimeric membrane CD4 molecules. It is, however, not known how the D1-D2 domains are associated with D3-D4 on the cell surface. It is possible that D1 domain makes a primary contact followed by D3-D4 domain in a dimer formation. Moreover, it has been demonstrated that the membrane-proximal CD4 domain appears to be important for the overall conformation of CD4 (5), and replacement of this domain might have an indirect rather than a direct role in CD4 dimer formation. Our data and these results do not rule out that several domains of CD4, including the D1, D3, and D4, participate in CD4 oligomerization.
In conclusion, our results provide the first functional evidence indicating that negatively charged residues within the CDR3-like loop can play a role in CD4-mediated activation signals transduced in T cells after virus envelope binding to the CDR2-like loop. Moreover, they strongly suggest that the CDR3-like loop represents a main site for CD4 dimerization.
We are indebted to D. Carrière, S. Fisher, M. Hirn, D. Klatzmann, and D. Littman for kind gifts of reagents or cells. We thank Sandrine El Marhomy for excellent technical assistance. We thank Q. Sattentau for stimulating discussions.