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Journal of Virology, March 2000, p. 2142-2150, Vol. 74, No. 5
0022-538X/00/$04.00+0
Copyright © 2000, American Society for Microbiology. All rights reserved.
Sensitivity to a Nonpeptidic Compound (RPR103611)
Blocking Human Immunodeficiency Virus Type 1 Env-Mediated Fusion
Depends on Sequence and Accessibility of the gp41 Loop
Region
Béatrice
Labrosse,
Carole
Treboute, and
Marc
Alizon*
INSERM U.332, Institut Cochin de
Génétique Moléculaire, 75014 Paris, France
Received 16 August 1999/Accepted 2 December 1999
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ABSTRACT |
The triterpene RPR103611 is an efficient inhibitor of membrane
fusion mediated by the envelope proteins (Env, gp120-gp41) of
CXCR4-dependent (X4) human immunodeficiency virus type 1 (HIV-1) strains, such as HIV-1LAI (LAI). Other X4 strains, such as
HIV-1NDK (NDK), and CCR5-dependent (R5) HIV-1 strains, such
as HIV-1ADA (ADA), were totally resistant to RPR103611.
Analysis of chimeric LAI-NDK Env proteins identified a fragment of the
NDK gp41 ectodomain determining drug resistance. A single difference at
position 91, leucine in LAI and histidine in NDK, apparently accounted
for their sensitivity or resistance to RPR103611. We had previously identified a mutation of isoleucine 84 to serine in a drug escape LAI
variant. Both I84 and L91 are located in the "loop region" of gp41
separating the proximal and distal helix domains. Nonpolar residues in
this region therefore appear to be important for the antiviral activity
of RPR103611 and are possibly part of its target. However, another
mechanism had to be envisaged to explain the drug resistance of ADA,
since its gp41 loop region was almost identical to that of LAI. Fusion
mediated by chimeric Env consisting of LAI gp120 and ADA gp41, or the
reciprocal construct, was fully blocked by RPR103611. The gp120-gp41
complex of R5 strains is stable, relative to that of X4 strains, and
this stability could play a role in their drug resistance. Indeed, when
the postbinding steps of ADA infection were performed under mildly
acidic conditions (pH 6.5 or 6.0), a treatment expected to favor
dissociation of gp120, we achieved almost complete neutralization by
RPR103611. The drug resistance of NDK was partially overcome by
preincubating virus with soluble CD4, a gp120 ligand inducing
conformational changes in the Env complex. The antiviral efficacy of
RPR103611 therefore depends on the sequence of the gp41 loop and the
stability of the gp120-gp41 complex, which could limit the
accessibility of this target.
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INTRODUCTION |
The human immunodeficiency virus
type 1 (HIV-1) and HIV-2 envelope glycoproteins (Env) consist of
noncovalent complexes of surface (gp120) and transmembrane (gp41)
subunits, both derived from a gp160 precursor which is oligomerized and
cleaved during its transport to the cell surface (reviewed in
references 9, 26, and 46). The
function of these proteins is to mediate virus entry by allowing
binding of virions to the cell surface and fusion of their lipidic
envelopes with the cell membrane. Our knowledge of the structure of
HIV-1 Env and of the mechanism by which it fulfils its function has
considerably improved over the last years, although a number of aspects
remain to be elucidated. Schematically, the initial steps of virus
entry (binding) are mediated by gp120, while gp41 is responsible for
the membrane fusion process itself. By analogy with the influenza virus
hemagglutinin model, gp41 is thought to become fusion competent after
conformation changes in the gp120-gp41 complex (15, 38),
which are not as yet understood at the molecular level. These events
seem to be usually triggered by the interaction of gp120 with two
classes of cell surface molecules, CD4 and chemokine receptors, in
particular CCR5 or CXCR4, often viewed as HIV coreceptors (reviewed in
references 2, 14, and 20). In
vivo, strains using CXCR4 (termed X4 strains) or both CXCR4 and CCR5
(R5X4) are isolated at later stages of infection, while strains using
CCR5 (R5) are predominant at the earlier stages. The X4 strains, in
particular when adapted to replication in T-cell lines, are
characterized by a relatively labile gp120-gp41 association, evidenced
by the shedding of gp120, spontaneously or upon contact with soluble
CD4 (sCD4) or anti-gp120 antibodies (24, 33, 36), while the
gp120-gp41 complex of R5 strains seems comparatively stable (27,
30).
Like other retroviral transmembrane proteins, gp41 comprises an
N-terminal extracellular domain (ectodomain), a membrane-spanning domain, and a C-terminal cytoplasmic domain, apparently dispensible for
the fusion process (9). The main features of the ectodomain are a hydrophobic N-terminal sequence ("fusion peptide"), thought to insert in the target cell membrane, and two domains with a predicted
-helix conformation separated by a region containing a conserved
dicysteine motif, representing a highly immunogenic determinant
(11). Several residues in the proximal helix and the loop
region of gp41 seem to be involved in interactions with gp120
(13). Peptides corresponding to the proximal (N) and distal (C) helix domains of HIV-1 gp41 spontaneously form highly stable coiled-coil structures with an inner core of three parallel N helices
on which are stacked three C helices placed in an antiparallel orientation (4, 41, 42). Structural analysis of the gp41 ectodomain of the HIV-2-related simian immunodeficiency virus revealed
the same organization (3). Whether the formation of this
structure is the motive force driving the viral and target membranes to
a closer apposition (4, 42) or whether this structure is
already present in the native form of gp41 is not known (3).
Different strategies to block the HIV-1 infectious process at the cell
entry step, either by targeting one of the cellular receptors or the
envelope proteins themselves, are envisioned. To date, the vast
majority of available compounds interfere with the initial steps of
virus entry, i.e., the interaction of gp120 with cell surface
components. The most promising compounds are bicyclams, which are
nonpeptidic antagonists of CXCR4 (1). The extreme genetic
variability of gp120 among isolates (29) and the ability of
HIV-1 to switch from one type of receptor to another (e.g., CXCR4 to
CCR5) by a few mutations in gp120 (39) are obvious
limitations for these strategies. In contrast, gp41 is far more
conserved and does not seem to require further interactions with
cellular proteins to mediate membrane fusion. However, very few
compounds targeting gp41 have been described to date. Peptides derived
from the proximal or the distal -helix regions of gp41 inhibit
cell-cell fusion and HIV-1 entry (44, 45). These compounds could act as dominant-negative inhibitors of the interaction between the proximal and distal helices, thereby preventing gp41 from attaining
its fusion-active conformation (5), but other mechanisms of
action have been proposed (3, 28). Peptides from the distal helix display the most efficient antiviral activity, and one such peptide (T20) was recently found to reduce the virus load in
HIV-1-infected individuals (17). However, cost and
bioavailability issues seem to represent serious limitations to the use
of such peptides on a larger scale.
To our knowledge, the triterpene RPR103611, a betulinic acid derivative
(molecular weight, 712), is the only nonpeptidic antiviral compound
thought to target gp41. It was isolated through random screening and
was found to block cell-cell fusion and HIV-1 infection at a
postbinding step (21). We have characterized a drug escape mutant of the X4 strain HIV-1LAI (LAI) and have found that
its phenotype stemmed from a mutation in the gp41 ectodomain
(19). In addition, the drug-resistant phenotype of an X4
strain of African origin, HIV-1NDK (NDK), was attributed to
differences with LAI in gp41. Here we have further addressed the
mechanism of the resistance of NDK to RPR103611 and have identified a
gp41 residue apparently critical for its antiviral effect.
Unexpectedly, HIV-1ADA (ADA), an R5 strain almost identical
to LAI in its gp41 sequence, was fully resistant to neutralization by
RPR103611. In this case, drug resistance seemed related to the
relatively stable association of the gp120-gp41 complex, probably
limiting access of the drug to its target.
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MATERIALS AND METHODS |
Cell lines and viral strains.
Infections were performed in
target cells derived from the U373MG-CD4 (12) or HeLa-P4
(6) cell line; both of these cell lines are CD4+
and bear the Escherichia coli 
-galactosidase gene
(lacZ) under transcriptional control of the HIV-1 long
terminal repeat (LTR). The U373MG-CD4 cells stably expressing either
CXCR4 or CCR5 (18) and the HeLa-P4 derivatives stably
expressing CCR5 (HeLa-P5) (32) have been described. Cells
were propagated in Dulbecco's modified Eagle's medium (DMEM)
supplemented with 10% fetal calf serum (FCS), antibiotics (penicillin
and streptomycin), and 2 mM glutamine. Virus stocks were supernatants
of HeLa cells transfected with the cloned molecular genomes of the
HIV-1 strains LAI (31), NDK (40),
HIV-189.6 (89.6) (7), and ADA, actually a
recombinant LAI provirus with env from ADA (32,
43). Infectious titers were determined in Hela-P4 cells, except
for ADA, which was titrated in HeLa-P5 cells.
Antibodies, recombinant proteins, and other reagents.
The
sheep anti-gp120 antibody D7324 raised against a peptide from the C
terminus of gp120 (25) was obtained from Aalto BioReagents (Dublin, Ireland). Pooled sera from HIV-1-infected individuals were a
gift from N. Sol (Hôpital St.-Louis, Paris, France).
Peroxidase-conjugated goat anti-human immunoglobulin G was obtained
from Jackson ImmunoResearch Laboratories (West Grove, Pa.). The
betulinic acid derivative RPR103611 was obtained from
Rhône-Poulenc Rorer Laboratories (Vitry-sur-Seine, France) as a
dry powder and diluted in dimethylformamide (10 mM stock solution).
Baculovirus-expressed gp120 from HIV-1IIIB (a LAI variant)
and sCD4 were obtained from Neosystems Laboratories (Strasbourg, France).
Env expression vectors.
The vectors allowing expression of
Env from LAI (NS105) (19) and ADA (32) have been
described. Env LAI mutants were derived from NS105 by site-directed
mutagenesis on a single-stranded template. Mutants were screened for
the creation of restriction enzyme sites and checked by sequencing the
gp41 ectodomain. The 89.6 Env expression vector was obtained by
replacing the KpnI-BamHI fragment of NS105 (nucleotides [nt] 5925 to 8068 in LAI) by a
KpnI-BamHI PCR fragment amplified from the 89.6 env. Sequences of oligonucleotides used for PCR and
site-directed mutagenesis can be provided upon request. The LAI-ADA Env
chimeras, LA-1 and LA-2, were obtained by ligating KpnI
site-to-blunt end (gp120) and blunt end-to-BamHI site (gp41) PCR fragments amplified from ADA env or from LAI
env. Blunt-end ligation created a PvuI site at
the gp120-gp41 junction (see Fig. 5A). The resulting V2I substitution
in gp41 had no apparent effect on its function. The NDK Env expression
vector contained a portion of LAI gp41 corresponding to the membrane
anchor and cytoplasmic domains. It was derived from the previously
described LN-3 vector (19) by replacing a
SalI-MluI fragment (nt 5320 to 6632) by a
SalI-MluI PCR fragment amplified from NDK
env. The LN-7, LN-8, and LN-9 expression vectors have been
described (19). The XbaI site introduced in LAI
env (nt 7669) facilitated construction of LN-10 by
substituting the LAI env XbaI-BamHI fragment for
the corresponding LN-8 fragment. LN-11 was obtained by replacing the ApaLI-BamHI fragment of the NDK Env expression
vector by the corresponding fragment from LN-9. The
HIV-2ROD (ROD) Env expression vector was a cloned ROD
provirus (34) with nucleotides between
HindIII sites (nt 1457 and 5782 located in
gag and vpr, respectively) deleted.
Syncytium formation assay.
Subconfluent monolayers of HeLa
cells in six-well trays (~2 × 105 cells per well)
were transfected with Env expression vectors by calcium phosphate
precipitation. An equivalent number of LTR-lacZ target cells
freshly detached by trypsinization were added 20 h after
transfection. After overnight coculture in the absence or presence of
RPR103611 (10 µM), adherent cells were fixed in 0.5% glutaraldehyde
and stained with the -galactosidase substrate X-Gal
(5-bromo-4-chloro-3-indolyl--D-galactopyranoside), as
described previously (8). Blue-stained foci were
scored under ×20 magnification.
Infectivity assays.
Standard infectivity assays were
performed with HeLa-P4 target cells using in situ detection of
-galactosidase activity as the readout. Briefly ~2 × 105 cells were infected with about 103
infectious units (i.u.) in 12-well plates in the absence or presence of
RPR103611 (10 µM), fixed, and stained with X-Gal 20 h later. Infections of HeLa-P4 cells with HIV-1 stocks pretreated with sCD4 were
performed in 96-well flat-bottom microtiter plates. LAI and NDK stocks
were preincubated with concentrations of sCD4 ranging from 1 to 1,000 µg/ml, or were mock-treated, for 1 h at 37°C and then added to
cells (5 × 102 i.u. per well). After overnight
incubation, cells were lysed in 0.5% Nonidet P-40 (50 µl per well)
and -galactosidase activity was quantified using the chromogenic
substrate chlorophenol red--D-galactopyranoside (CPRG)
by measuring absorbance at 575 nm as described previously (8). To study the effect of pH on HIV-1 infectivity, HeLa-P5 cells seeded in 48-well plates were left in contact with ADA or LAI
(~103 i.u. per well) for 2 h at 4°C, in order to
allow virus adsorption but not fusion. Unbound virus was removed by two
washes in phosphate-buffered saline (PBS), and plates were shifted to
37°C. After 30 min, the supernatant was replaced by culture medium
(DMEM-10% FCS) buffered at pH 6, 6.5, 7, or 7.5 with acetic acid and
containing or not containing RPR103611 (10 µM). After 90 min at
37°C, cells were washed and cultured in standard medium (pH 7.4) with
or without RPR103611 (10 µM) for 20 h before being stained with
X-Gal.
Assay for gp120.
Concentrations of gp120 (and gp160) in
cells and supernatants were measured by a previously described sandwich
enzyme-linked immunosorbent assay (ELISA) technique (22).
Briefly, HeLa cells were transfected in 100-mm-diameter petri dishes
with Env expression vectors, and supernatants were replaced 24 h
posttransfection by fresh medium (4 ml). One day later, cell-free
supernatants were harvested and treated with 0.5% Empigen BB
(Calbiochem), while cells were lysed in 0.5 ml of PBS-0.5% Empigen
BB. Quadruplicate samples (100 µl) of supernatants and cell lysates,
diluted in DMEM containing (10% FCS and 0.5% Empigen BB, were added
to microtiter plates (Immulen 2; Dynex Technologies, Guyancourt,
France) coated with affinity-purified sheep anti-HIV-1 gp120 antibody
D7324 (0.5 µg per well). After overnight incubation at 4°C and five
washes in PBS-0.1% Tween 20, 100 µl per well of a 1/500 dilution of
pooled sera from HIV-1-infected individuals in PBS-4% nonfat
milk-0.1% Tween 20 was added. After 1 h at room temperature,
plates were washed five times in PBS-0.1% Tween 20, and 100 µl per
well of a 1/7,500 dilution of peroxidase-conjugated goat anti-human
immunoglobulin G (Calbiochem) in PBS-4% nonfat milk-0.5% Tween 20 was added. After 1 h at room temperature and five washes in
PBS-0.5% Tween 20, 100 µl of a 0.4-mg/ml solution of
2,2'-azinobis(3-ethylbenzthiazoline-6-sulfonic acid (ABTS; Sigma, St.
Louis, Mo.) in 0.6% acetic acid-0.03% H2O2 was added. Absorbance at 405 nm (A405) was read
30 min later. Concentrations of gp120 in samples were deduced by
comparison with the A405 in a series of samples
containing known amounts of recombinant gp120 (ranging from 0.2 to 50 ng/ml) processed in parallel. The threshold of detection of gp120 was 3 ng/ml (0.3 ng per well). The gp120-gp41 association index for a given
Env was calculated, as described by Helseth et al. (13), as
the ratio of the total amount of gp120 (plus gp160) in cell lysate to
the total amount of gp120 in supernatant.
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RESULTS |
Activity of RPR103611 on virus entry via CXCR4 or CCR5.
In an
initial study performed before the discovery of the role of chemokine
receptors in HIV entry and cell tropism, two primary HIV-1 isolates of
European origin and three cell line-adapted HIV-1 strains from clade B
(LAI, MN, and RF) were neutralized by RPR103611 with 50% inhibitory
concentrations ranging from 0.05 to 0.75 µM, while cell line-adapted
HIV-1 of African origin (ELI and NDK, both from clade D) and HIV-2
strains (ROD and EHO) were fully resistant to concentrations exceeding
10 µM (21). To directly address the possible importance of
the type of chemokine receptor used by HIV-1 or HIV-2 for their
sensitivity to RPR103611, we have performed syncytium formation assays
with cells expressing different types of Env from HIV-1 (LAI, NDK, ADA,
89.6) or from HIV-2 (ROD) and target cells (U373MG-CD4) expressing
either CXCR4 or CCR5. As expected, LAI and NDK Env only induced fusion
with CXCR4+ cells and ADA Env only induced fusion with
CCR5+ cells. The 89.6 and ROD Env apparently used both
types of receptors with similar efficacies (Fig.
1). Fusion mediated by the LAI Env was fully blocked by 10 µM RPR103611, while fusion mediated by the
NDK Env was only reduced by ~20% (Fig. 1). Fusion mediated by the
89.6 Env with the CXCR4+ or the CCR5+ cells was
completely blocked by RPR103611, while RPR103611 reduced the efficiency
of fusion mediated by the ROD Env by ~25% for both target cells.
Therefore, the drug sensitivity or resistance of the 89.6 and ROD Env
appeared to be independent of the chemokine receptors CXCR4 and CCR5.
The drug resistance of cell fusion mediated by Env from ADA was
unexpected, since this strain belongs to clade B (like LAI and 89.6).
Resistance to RPR103611 was also observed for fusion mediated by Env
from other clade B R5 strains (BaL, Jr-CSF, and YU-2; data not shown).
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FIG. 1.
Effect of RPR103611 on syncytium formation between HIV-1
or HIV-2 Env+ cells and CXCR4+ or
CCR5+ target cells. HeLa cells transfected with Env
expression vectors corresponding to the HIV-1 strains LAI, NDK, 89.6, ADA, and ROD were cocultured overnight with an equivalent number
(~2 × 105 cells per well) of U373MG-CD4 cells
stably expressing CXCR4 or CCR5, in the presence or absence of
RPR103611 (10 µM). Fusion with Env+ cells (also
expressing the HIV-1 or HIV-2 transactivator Tat) activates the
LTR-lacZ transgenes of target cells, allowing detection of
syncytia by their blue staining in the presence of the X-Gal substrate.
Bars, mean numbers of blue foci in three independent transfections with
standard error.
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Role of gp41 in resistance to RPR103611.
By testing the effect
of RPR103611 on cell-cell fusion and HIV-1 infection mediated by a
chimeric LAI-NDK Env, we had previously found that the NDK gp41 was
associated with drug resistance and that the LAI gp41 was associated
with drug sensitivity (19). Here we have refined this
approach by using chimeric LAI-NDK Env in which fragments of the gp41
ectodomain were exchanged (Fig. 2A). All
chimeric Env tested (LN-7 to LN-11) mediated fusion with HeLa-P4 cells
with efficiencies similar to that of the parental Env. As previously
observed, the efficiency of fusion mediated by the LN-7 and LN-8 Env
was only reduced by ~30% in the presence of 10 µM RPR103611 (Fig.
2B), indicating that the first 38 residues of NDK gp41 were dispensible
for the drug-resistant phenotype. Introducing residues 109 to 163 of
the NDK gp41 ectodomain into LAI Env (LN-9) did not modify its
sensitivity to RPR103611. In contrast, residues 39 to 108 of the NDK
gp41 were apparently sufficient to confer drug resistance in the LAI
Env context (LN-10). When this fragment of NDK gp41 was replaced by the
corresponding LAI gp41 fragment (LN-11 chimera), cell fusion was
totally blocked by RPR103611. Exchanging a 70-amino-acid gp41 fragment
was therefore sufficient to revert the phenotype of LAI or NDK Env with
regard to inhibition by RPR103611. This fragment contains the proximal helix domain and most of the loop region of gp41, including the dicysteine motif (Fig. 3).
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FIG. 2.
Inhibition of cell-cell fusion mediated by chimeric
LAI-NDK Env. (A) Schematic representation of wild-type and chimeric
Env. A, B, and X, ApaLI, BamHI, and
XbaI sites, respectively, used to exchange domains of gp41
(see Materials and Methods for details); m.a., membrane anchor domain
of gp41. Hatched bars, NDK sequences; arrow, cleavage site. (B) Extent
of inhibition of fusion between HeLa cells expressing the indicated Env
and HeLa-P4 cells (CD4+, CXCR4+) by RPR103611
(10 µM). The experiment was performed as described for Fig. 1. For
all types of Envs, 5,000 to 10,000 syncytia per well were scored in the
absence of the drug. Numbers represent the means of three independent
wells.
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FIG. 3.
Amino acid sequence of the gp41 extracellular domain of
the HIV-1 strains LAI, NDK, and ADA. The proximal and distal
-helical domains are shaded. Also shown are the dicysteine motif of
the loop region and the positions of the ApaLI and
XbaI sites used to construct LN chimeras.
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In this region of gp41, LAI and NDK Env differ at nine positions (Fig.
3). Each of these nine residues of LAI gp41 was replaced
by its NDK
counterpart, and the resulting mutant LAI Env were
tested for their
ability to mediate fusion with HeLa-P4 target
cells in the presence or
absence of RPR103611 (10 µM). All mutations,
except A96N, were
apparently compatible with the processing and
function of Env, since
the number of syncytia was similar to that
obtained with wild-type LAI
Env (Fig.
4A). As will be seen later,
the
A96N mutation seems to affect the stability of the gp120-gp41
complex.
The low level of fusion mediated by the A96N mutant was
apparently
resistant to RPR103611. Among the fully functional
Env LAI mutants,
only the leucine 91-to-histidine (L91H) substitution
was associated
with drug resistance. Fusion mediated by other
mutants was completely
blocked in the presence of the drug. This
experiment included the
previously characterized drug escape LAI
mutant carrying the isoleucine
84-to-serine (I84S) mutation.
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FIG. 4.
Inhibition of cell-cell fusion and infection mediated by
wild-type and mutant HIV-1 Env. Assays of syncytium formation (A)
between HeLa cells transfected with Env expression vectors and HeLa-P4
cells were performed as described for Fig. 1. Infections of HeLa-P4
cells (B) in the presence or absence of RPR103611 (10 µM) were
performed in six-well trays using wild-type or mutant LAI or NDK. Cells
were stained with X-Gal 20 h after infection. Viral stocks were
supernatants of transiently transfected HeLa cells. The inocula were
adjusted to yield ~1,000 blue foci per well in the absence of the
drug, except for the A96N LAI mutant, for which undiluted stock was
used. Bars, means of three independent wells with standard error.
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The effects of the I84S, L91H, and A96N mutations on HIV-1 infection
were tested by subcloning the corresponding mutant
env genes
into a LAI provirus. The A96N mutation abolished HIV-1 infectivity,
and
the effect of RPR103611 could not therefore be tested. Infection
mediated by virus carrying the I84S and L91H mutations was only
slightly reduced in the presence of 10 µM RPR103611 (Fig.
4B).
Parallel results were therefore obtained in infection and cell
fusion
assays.
Since the L91H mutation was sufficient to revert the phenotype of LAI
Env, we have tested the effect of the reciprocal mutation
(H91L) in the
context of NDK gp41. Cell fusion and HIV-1 infection
mediated by the
LN-7 chimeric Env (NDK gp41 ectodomain) bearing
this H91L mutation were
totally blocked by 10 µM RPR103611 (Fig.
4). These experiments showed
that the drug resistance of NDK could
be explained by a single amino
acid difference with respect to
LAI in gp41. The L91H mutation and the
previously characterized
drug escape mutation I84S both replace a
hydrophobic residue of
the loop region of gp41 by a polar residue. The
L91 and I84 residues
are conserved among clade B HIV-1 strains
(
29) but not among
clade D HIV-1 strains or among HIV-2
strains, which may explain
their drug
resistance.
Drug resistance of R5 strains.
In the region of gp41 that we
found important for sensitivity or resistance to RPR103611 (residues 38 to 109), the HIV-1 strain ADA differs from LAI by five conservative
substitutions (Fig. 3). Three of these ADA residues (V69, R77, and
D109) are also found in the NDK sequence, with no apparent role in the
drug resistance phenotype. We have addressed the possible role of the
two other ADA residues (L72 and T107) by site-directed mutagenesis in
the LAI gp41 context. The V72L and S107T mutations did not affect the
efficiency and drug sensitivity of fusion with HeLa-P4 cells (data not shown).
To define whether the gp120 or gp41 of ADA was responsible for the
drug-resistant phenotype, each one was replaced by the
corresponding
Env subunit of LAI, thus yielding the LA-1 and LA-2
chimeric Env (Fig.
5A). As expected, fusion mediated by LA-1
(ADA
gp120) was CCR5 dependent, while fusion mediated by LA-2 (LAI
gp120) was CXCR4 dependent (Fig.
5B). Fusion mediated by LA-1
was less
efficient than fusion mediated by the parental Env (about
50%),
although the number of syncytia remained high, indicating
relatively
efficient processing and expression of this chimeric
Env. Fusion
mediated by LA-1 and LA-2 was fully blocked in the
presence of
RPR103611, which confirmed that the minor sequence
differences in gp41
did not determine the phenotypic differences
between LAI and ADA. This
ruled out a direct role for gp120 in
the drug resistance of ADA. Since
the gp120 and gp41 of ADA only
expressed a drug-resistant phenotype
when they were associated,
we were led to envisage a potential role for
the stability of
the gp120-gp41 complex of R5 strains in their
resistance to RPR103611.
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FIG. 5.
Inhibition of cell-cell fusion mediated by HIV-1 LAI-ADA
Env chimeras. (A) Schematic representation of wild-type and chimeric
Env. K, P, and B, KpnI, PvuI, and
BamHI sites, respectively, used for construction of chimeric
env (see Materials and Methods); m.a., membrane anchor
domain. (B) Fusion of HeLa cells expressing indicated Env and
U373MG-CD4 cells expressing either CXCR4 or CCR5, in the presence or
absence of RPR103611. The experiment was performed and presented as
described for Fig. 1.
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Role of gp120-gp41 stability.
The stability of the gp120-gp41
association can be indirectly assessed by measuring the amount of gp120
shed in the supernatant of Env+ cells (13). When
HeLa cells were transfected with different Env expression vectors,
similar amounts of cell-associated gp120 (and gp160) were measured by
quantitative ELISA (Fig. 6). As expected, measurements made in parallel in cell-free supernatants revealed a
markedly higher level of gp120 in cells transfected with LAI Env than
in cells transfected with ADA Env (Fig. 6). Assuming an association
index (cell-associated/cell-free gp120) of 1 for LAI Env, we obtained a
value of 6.7 for ADA Env (Table 1). The LA-1 and LA-2 chimeras formed apparently weaker gp120-gp41 complexes, with relative association indexes of 2.8 and 3.5, respectively (Table 1
and Fig. 6).
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FIG. 6.
Shedding of gp120 in supernatants of cells expressing
HIV-1 Env. About 106 HeLa cells were transfected in a
100-mm-diameter plate with the indicated Env expression vector. The
supernatant was replaced 24 h later by 4 ml of culture medium
containing or not containing RPR103611 (10 µM). After another 24 h, supernatant and adherent cells were independently harvested, and the
concentrations of gp120 were determined by ELISA (see Materials and
Methods) by comparison with samples containing known amounts of
recombinant gp120 processed in parallel. Bars, total amounts of gp120
in the supernatant and in the cells for a given transfected plate
(means of at least four independent transfections).
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The spontaneous gp120 shedding was lower in cells expressing Env from
NDK than in cells expressing LAI Env (association index
of 3.5; Table
1), in agreement with a previous report (
35).
This indicated
a stabler gp120-gp41 association for NDK Env. The
amounts of shed gp120
for wild-type NDK Env and the LN-7 chimeric
Env (LAI gp120-NDK gp41)
were similar, suggesting that gp41 rather
than gp120 determined the
relative stabilities of the LAI and
NDK Env complexes. In the LN-7 Env
context, the H91L mutation
markedly reduced the stability of the
gp120-gp41 complex while
point mutations I84S and L91H did not seem to
modify the stability
of the LAI gp120-gp41 complex (Fig.
6, Table
1).
The A96N mutation
was associated with a very large amount of gp120
shedding (Fig.
6). Instability of the Env complex probably explained
the lack
of activity of this mutant. Finally, incubating cells with 10
µM RPR103611 did not detectably increase shedding of the NDK or
LAI
gp120 (Fig.
6), which represented another argument against
the activity
of this compound on
gp120.
Drug sensitivity of ADA at low pH.
For R5 strains, it is not
usually possible to induce dissociation of the gp120-gp41 complex and
gp120 shedding upon incubation of virions and gp120 ligands such as
sCD4 (27, 30) incubation in acidic pH conditions was
previously shown to enhance the effect of sCD4 on X4 HIV-1 strains
(10). We have therefore sought to use low-pH conditions as a
means to reduce the stability of the gp120-gp41 association and to
possibly facilitate the effect of RPR103611. Since this treatment was
likely to be detrimental to the initial steps of HIV-1 infection
(binding), and possibly to early postbinding steps if they require a
tight gp120-gp41 association, it was omitted during the binding step
performed at 4°C and during the first 30 min following the shift of
temperature to 37°C. At this time, the culture medium was replaced by
medium at pH 6, 6.5, 7, or 7.5, containing or not containing RPR103611
(10 µM) and incubation was pursued for 90 min at 37°C. Cells were
then grown in standard culture medium, with or without the drug, and then fixed and stained to reveal HIV-1 infection. Usage of HeLa-P5 cells, which express both CCR5 and CXCR4, allowed a comparison of the
effects of RPR103611 on LAI and ADA in the same target cells.
For LAI, incubation at pH 6 resulted in a twofold reduction of the
infectious titer relative to incubations at pH 6.5 or higher.
At all pH
conditions tested, infection was totally blocked by
RPR103611 (Fig.
7A), showing that the drug was fully
active in
this pH range and could block infection when added after
adsorption,
as we previously observed (
19). A different
situation for infections
with ADA was observed. There was a very
limited inhibitor effect
at neutral pH, like that in the previous cell
fusion experiments,
while infection was reduced by approximately 90 and
70% at pHs
6.5 and 6, respectively (Fig.
7B). In acidic conditions, we
could
therefore achieve partial neutralization of an otherwise fully
resistant HIV-1 strain.
View larger version (21K):
[in this window]
[in a new window]
|
FIG. 7.
Effect of pH on neutralization of LAI (A) and ADA (B) by
RPR103611. HeLa-P5 cells (CXCR4+, CCR5+) in
48-well plates were left in contact with virus for 2 h at 4°C to
allow binding but not the subsequent steps of virus entry. After
unbound virus was washed off, plates were shifted to 37°C to initiate
fusion (30 min), and then supernatant was replaced by culture medium
buffered at the indicated pH (7.5 to 6.0) and containing or not
containing RPR103611 (10 µM). After another 90 min, supernatant was
replaced by standard cell culture medium containing or not containing
RPR103611, and cells were stained with X-Gal 20 h later. Bars,
means of three independent wells.
|
|
Relative drug sensitivity of NDK in the presence of sCD4.
The acidic treatment could also confer sensitivity to RPR103611
on NDK (data not shown). To address the possible influence of the
stability of the gp120-gp41 complex, we took advantage of the ability
of sCD4 to induce conformational changes in the gp120-gp41 complex of
X4 HIV-1 strains. Incubation of LAI with 1-µg/ml or higher sCD4
concentrations abolished infectivity (Fig. 8A), while NDK was more resistant to the
antiviral effect of sCD4 (Fig. 8B), in agreement with a previous report
(35). When infections were performed in the presence of 10 µM RPR103611, we observed a reduced infectivity when NDK had been in
contact with sCD4 concentrations higher than 1 µg/ml (Fig. 8B). As
expected, RPR103611 had no significant effect on untreated virus.
Therefore, contact with sCD4 concentrations apparently too low to
reduce NDK infectivity (1 and 5 µg/ml) or only reducing it by
10% (10 µg/ml) could result in a partial sensitivity to RPR103611
(Fig. 8B and C). As previously observed with acidic treatment of ADA,
we were able to achieve partial neutralization of a drug-resistant
strain by applying a treatment expected to dissociate the gp120-gp41
complex. However, in both cases, we did not observe complete
neutralization, as is achieved for drug-sensitive HIV-1 strains.
View larger version (31K):
[in this window]
[in a new window]
|
FIG. 8.
Effect of pretreatment of LAI and NDK with sCD4 on
neutralization by RPR103611. HeLa-P4 cells were infected in 96-well
trays (~1.25 × 104 per well) with LAI (A) or NDK (B
and C) stocks preincubated for 60 min at 37°C with the indicated
concentrations of sCD4. RPR103611 (10 µM) was present during
virus-cell contact and subsequent steps when indicated but not during
the pretreatment. Cells were washed and lysed in situ 20 h
postinfection, and -galactosidase activity was measured with the
chromogenic CRPG substrate by determining the
A575 (A). Bars, percentages of infectivity of
sCD4-treated viral stocks relative to untreated stocks. In panel C, the
effect of RPR103611 on untreated viral stocks is also shown. Results
are the means of three independent experiments.
|
|
| |
DISCUSSION |
The betulinic acid derivative RPR103611 is a potent inhibitor of
HIV-1 entry and fusion, but its activity is clearly strain dependent.
Antiviral activity of RPR103611 against LAI and other cell line-adapted
HIV-1 strains belonging to clade B was initially reported, while HIV-2
strains (ROD, EHO) and two clade D HIV-1 strains (ELI and NDK) were
fully resistant (19, 21). By exchanging env gene
domains between LAI and NDK, we found that the ectodomain of gp41 was
apparently determining their sensitivity or resistance to RPR103611
(19). Here we have refined this approach and found that a
discrete domain of 70 residues from the NDK gp41 ectodomain was
sufficient to confer drug resistance in the LAI Env context. Reciprocally, the same fragment from LAI gp41 conferred sensitivity in
an NDK Env context. This fragment contains part of the proximal helix
and the loop region located between the proximal and distal helices of
gp41. We had previously mapped a drug escape mutation in LAI in the
same region of gp41 at isoleucine 84 (19). Here we found
that a single amino acid difference at position 91, a leucine for LAI
and a histidine for NDK, was sufficient to account for their distinct
phenotypes. Indeed, fusion mediated by the LAI Env mutant carrying the
L91H mutation was resistant to RPR103611, while the H91L mutation
caused reversion of the phenotype of a chimeric construct bearing the
ectodomain of NDK gp41. Other amino acid differences between LAI and
NDK had no apparent role, with the possible exception of the
replacement of alanine 96 of LAI by asparagine in NDK. The effect of
the A96N mutation was difficult to appreciate since it markedly reduced
fusion efficiency and abolished HIV-1 infectivity. Since the H91L
mutation was sufficient to revert the NDK phenotype, it seems that the
N96 residue does not have a major role.
The L91 residue is part of the dicysteine motif, which is a hallmark of
the transmembrane proteins of retroviruses (11). Its
sequence is highly conserved among HIV-1 strains, with a leucine at
position 91 except in clade D strains, which have a histidine (29). This may explain the drug resistance of the clade D
strains ELI (21) and MAL (data not shown). The sequence of
the gp41 dicysteine motif is different in HIV-2; in particular, there
is a conserved glutamine in place of the LAI L91 residue
(29). Also, in the gp41 of ROD and most HIV-2 strains, the
residue corresponding to the I84 of LAI is a serine. Both features
could contribute to the drug resistance of the HIV-2 strains tested
(19, 21).
The I84S and L91H mutations conferring drug resistance to HIV-1
represent replacements of nonpolar by polar amino acids. These residues
are not part of the available HIV-1 gp41 crystal structure (4, 41,
42) but are expected to be in close proximity, according to the
simian immunodeficiency virus gp41 structure (3). It is
therefore possible that both I84 and L91 contribute to the
formation of a pocket binding RPR103611 through hydrophobic interactions. Analysis of the effect of other mutations at these positions would be necessary to validate this model.
We sought to obtain evidence for the interaction of the loop region of
gp41 with RPR103611 by testing its ability to compete with the binding
of the anti-gp41 monoclonal antibodies (MAbs) 50-69 and 3D6
(47). Their epitopes correspond to a region of gp41 masked
in the gp120-gp41 complex and become exposed upon treatment with sCD4
(36). Flow cytometry experiments were performed with
LAI-infected cells expressing relatively high levels of Env, judging by
staining with anti-gp120 antibodies. Preincubating cells with a fully
active antiviral RPR103611 concentration (10 µM) did not
significantly decrease reactivity with the 50-69 and 3D6 MAbs when
either fractions of stained cells or mean fluorescence intensities were
considered (data not shown). However, these results did not rule out
the possibility of a direct interaction of RPR103611 with the loop
region of gp41 if, for example, the binding sites of the drug and
antibodies tested are distinct or the affinity of gp41 for RPR103611 is
lower. It is even conceivable that RPR103611 only interacts with a
transient conformational state of gp41.
The fact that the clade B HIV-1 strain ADA was fully resistant to
RPR103611, despite being almost identical to LAI in the gp41 loop
region and in particular at the I84 and L91 residues, led us to
envisage another possible mechanism for HIV-1 drug resistance. Like
other macrophage-tropic HIV-1 strains, ADA is strictly dependent on the
CCR5 receptor pathway. Usage of this receptor did not seem to be the
direct cause of drug resistance, since infection by the R5X4 HIV-1
strain 89.6 was blocked by RPR103611 in target cells expressing CCR5
but not CXCR4. Fusion mediated by chimeric Env consisting of gp120 from
ADA and gp41 from LAI or the reciprocal construction was also fully
blocked by RPR103611. The drug resistance phenotype of ADA therefore
seemed to result from the combination of determinants in the two
envelope subunits. A feature of R5 strains that could account for these
observations is the higher stability of the gp120-gp41 complex relative
to that of X4 strains (27, 30). This might limit the access
of compounds to regions of gp41 that are masked by gp120 in the native
complex (37). For R5 strains, these regions of gp41 may not
become accessible, or may become so too late for compounds to exert
their antiviral activity. This issue was addressed by performing part
of the cell entry process in mildly acidic conditions (pH 6 or 6.5), a
treatment expected to favor dissociation of gp120 and gp41. By this
method, we observed a marked reduction (up to 90%) in the infectious
titer of ADA in the presence of RPR103611, while LAI infection was
totally blocked. It is noteworthy that RPR103611 was added to cells 30 min after cells were shifted from 4 to 37°C in order to initiate virus-cell fusion. This confirmed that the antiviral activity of
RPR103611 is exerted at a postbinding step of the HIV-1 entry process.
The drug resistance of ADA and other R5 strains was not therefore due
to the lack of a target sequence but rather was probably due to
constraints on its accessibility. Besides differences in the stability
of the gp120-gp41 complex, there could be differences between R5 and X4
strains in the nature or the kinetics of the conformational changes
eventually allowing gp41 to mediate fusion (16).
Contrary to LAI, the gp120-gp41 complex of NDK is also relatively
stable (35), which could have contributed to its resistance to RPR103611. Indeed, when NDK was preincubated with sCD4
concentrations too low to reduce infectivity, we observed partial
neutralization by RPR103611. Like the low-pH conditions for ADA, a
treatment expected to favor dissociation of the gp120-gp41 complex
conferred RPR103611 sensitivity on an otherwise fully resistant HIV-1 strain.
The stability of the gp120-gp41 complex can be indirectly quantified by
measuring gp120 shed in the supernatant of Env+ cells. This
amount is markedly higher for LAI than for ADA, resulting in relative
gp120-gp41 association indexes of 1 and 6.7, respectively. The index
was markedly reduced for the two LAI-ADA gp120-gp41 chimeras (2.8 and
3.3), consistent with their drug sensitivity. It was on the same order
of magnitude (3.5) for NDK, suggesting that parameters other than Env
stability contributed to the phenotype. While the H91L mutation in NDK
gp41 reduced the stability of Env, the I84S and L91H mutations
conferring drug resistance to LAI did not modify the association index.
The observation that the drug resistance of ADA and NDK could be
counteracted by treatments expected to improve gp41 access does not
necessarily exclude a direct role for the gp41 sequence (in particular
the presence of hydrophobic residues I84 and L91) in neutralization by
RPR103611. Furthermore, low pH (for ADA) and sCD4 (for NDK) treatments
only permitted partial neutralization by 10 µM RPR103611, while the 50% inhibitory concentration was 2 orders of magnitude lower for the
fully sensitive HIV-1 strains (21).
The lack of activity of RPR103611 on R5 HIV-1 strains certainly limits
its therapeutic value, although this class of compounds could be of
interest at late stages of infection. They may nevertheless represent
valuable tools to address the mechanism by which the transmembrane
protein mediates fusion of the virus envelope with the cell membrane
and possibly contributes to subsequent steps. Although these postfusion
steps are not as well known, it appears that virus entry requires the
formation of a fusion pore and its dilatation to a diameter allowing
passage of the viral capsid (23). It will be of interest to
compare the activity of RPR103611 with that of antiviral peptides
derived from the gp41 helix domains. Our preliminary studies suggested
similar kinetics for the antiviral activity of these compounds (data
not shown). Their antiviral effects were additive, suggesting that the
targets were not identical. This is consistent with our finding that
the target of gp41 was the loop region, while peptides are expected to
act on the helical regions. For peptides of the gp41 helices, high
concentrations were required to block lipid exchange between fusion
effector and target cells, while markedly lower concentrations blocked both the formation of fusion pores and HIV-1 entry (28).
This led to the proposal that the antiviral activity of these peptides at low concentrations was not due to the disruption of the gp41 coiled-coil structure or to competition with its formation but rather
to the blocking of a step following lipid mixing. This step should
therefore be posterior to the interaction of the fusion peptide with
the target membrane and the close apposition with the virus envelope.
Peptides could, for example, prevent the clustering of gp41 trimers to
form a proteinaceous pore or, conversely, could prevent their
dissociation to allow dilatation of the pore. Testing the effect of
RPR103611 on the exchange of lipids between cells should provide
further information and should contribute to the understanding of the
mechanism by which gp41 mediates HIV-1 entry.
| |
ACKNOWLEDGMENTS |
We thank J. Richardson and N. Heveker (ICGM) for comments on the
manuscript, Y. Hénin (Rhône-Poulenc Rorer) for the gift of
RPR103611, N. Sol (Hôpital Saint-Louis) for the gift of anti-HIV sera, and T. Teste-Lasserre and F. Letourneur (ICGM) for help with
gp120 ELISA and DNA sequencing.
This work was supported by the Agence Nationale de Recherches sur le SIDA.
| |
FOOTNOTES |
*
Corresponding author. Mailing address: INSERM U.332,
Institut Cochin de Génétique Moléculaire, 22 rue
Méchain, 75014 Paris, France. Phone: 33-1-40 51 64 86. Fax:
33-1-40 51 77 49. E-mail: alizon{at}cochin.inserm.fr.
| |
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Journal of Virology, March 2000, p. 2142-2150, Vol. 74, No. 5
0022-538X/00/$04.00+0
Copyright © 2000, American Society for Microbiology. All rights reserved.
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Abstract
Introduction
