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Previous Article | Next Article 
Journal of Virology, October 2000, p. 9362-9371, Vol. 74, No. 20
0022-538X/00/$04.00+0
Copyright © 2000, American Society for Microbiology. All rights reserved.
Biochemical Characterization of Rotavirus Receptors
in MA104 Cells
Carlos A.
Guerrero,1,
Selene
Zárate,1
Gabriel
Corkidi,2
Susana
López,1 and
Carlos F.
Arias1,*
Departamento de Genética y
Fisiología Molecular, Instituto de
Biotecnología,1 and Laboratorio
de Procesamiento de Imágenes, Centro de
Instrumentos,2 Universidad Nacional
Autónoma de México, Cuernavaca, Morelos 62250, Mexico
Received 10 March 2000/Accepted 18 July 2000
 |
ABSTRACT |
We have tested the effect of metabolic inhibitors, membrane
cholesterol depletion, and detergent extraction of cell surface molecules on the susceptibility of MA104 cells to infection by rotaviruses. Treatment of cells with tunicamycin, an inhibitor of
protein N glycosylation, blocked the infectivity of the SA-dependent rotavirus RRV and its SA-independent variant nar3 by about 50%, while
the inhibition of O glycosylation had no effect. The inhibitor of
glycolipid biosynthesis
d,l-threo-1-phenyl-2-decanoylamino-3-morpholino-1-propanol (PDMP) blocked the infectivity of RRV, nar3, and the human rotavirus strain Wa by about 70%. Sequestration of cholesterol from the cell
membrane with 
-cyclodextrin reduced the infectivity of the three
viruses by more than 90%. The involvement of N-glycoproteins, glycolipids, and cholesterol in rotavirus infection suggests that the
virus receptor(s) might be forming part of lipid microdomains in the
cell membrane. MA104 cells incubated with the nonionic detergent
octyl--glucoside (OG) showed a ca. 60% reduction in their ability
to bind rotaviruses, the same degree to which they became refractory to
infection, suggesting that OG extracts the potential virus receptor(s)
from the cell surface. Accordingly, when preincubated with the viruses,
the OG extract inhibited the virus infectivity by more than 95%. This
inhibition was abolished when the extract was treated with either
proteases or heat but not when it was treated with neuraminidase,
indicating the protein nature of the inhibitor. Two protein fractions
of around 57 and 75 kDa were isolated from the extract, and these
fractions were shown to have rotavirus-blocking activity. Also,
antibodies to these fractions efficiently inhibited the infectivity of
the viruses in untreated as well as in neuraminidase-treated cells.
Five individual protein bands of 30, 45, 57, 75, and 110 kDa, which
exhibited virus-blocking activity, were finally isolated from the OG
extract. These proteins are good candidates to function as rotavirus receptors.
| |
INTRODUCTION |
Rotaviruses, the leading cause of
severe dehydrating diarrhea in infants and young children worldwide,
are nonenveloped viruses that possess a genome of 11 segments of
double-stranded RNA contained in a triple-layered protein capsid. The
outermost layer is composed of two proteins, VP4 and VP7. VP4 forms
spikes that extend from the surface of the virus and has been
associated with a variety of functions, including the initial
attachment of the virus to the cell membrane and the penetration of the
cell by the virion (14).
Rotaviruses have a very specific cell tropism, infecting only
enterocytes on the tips of intestinal villi (26), which
suggests that specific host receptors must exist. In vitro, they also
display a strict tropism, binding to a variety of cell lines but
infecting efficiently only those of renal or intestinal epithelium
origin (15). Despite the advances in the molecular and
structural biology of the virus, little is known about the rotavirus
cell receptors. Some animal rotavirus strains interact with sialic acid
(SA) on the cell surface, and this interaction is a requirement for the efficient attachment and infection of the virus to susceptible cells
(9, 17, 27, 34, 39, 57). Accordingly, a number of
glycoconjugates bind to and block the infectivity of animal rotaviruses
in vitro and in vivo (3, 4, 6, 17, 32, 46, 52-54, 56, 57).
Some of these glycoconjugates may play a role as possible receptors,
like GM3 gangliosides in newborn piglet intestine (47), GM1
in LLC-MK2 cells (52), and 300- to 330-kDa glycoproteins in
murine enterocytes (3). More recently, it has also been
suggested that 
21, x2, and 41 integrins may be
involved in rotavirus cell entry (11, 24).
The binding of animal rotaviruses RRV and SA11 to an SA-containing cell
receptor is nonessential since variants whose infectivity is no longer
dependent on the binding to these acid sugars have been isolated
(35, 39). The secondary importance of SA as an attachment
site for rotaviruses, at least under laboratory conditions of
infection, is also reflected by the fact that the infectivity of most,
if not all, human rotavirus (HRV) strains is not affected by
neuraminidase treatment of cells (9, 17, 19, 41). Recently,
through competition infection assays using the SA-dependent RRV, its
SA-independent variant nar3, and the naturally neuraminidase-resistant
HRV strain Wa, the existence of at least three cell surface sites
involved in the interaction of rotaviruses with MA104 cells during the
early steps of infection was determined (41).
In this study we used two approaches to characterize the cell surface
structures that could serve as rotavirus receptors. In the first
approach, MA104 cells were treated with metabolic inhibitors of
glycosylation as well as of glycolipid synthesis to determine the
effects on the infectivity of rotaviruses RRV, nar3, and Wa. In the
second approach, the putative receptors for rotaviruses were extracted
with the nonionic detergent octyl--glucoside (OG) under noncytolytic
conditions. The molecules present in the extract, which were shown to
inhibit rotavirus infectivity when incubated with the viruses in
solution, were biochemically characterized and partially purified.
| |
MATERIALS AND METHODS |
Cells and viruses.
The human rotavirus strain Wa and the
rhesus strain RRV were obtained from Harry B. Greenberg, Stanford
University, Stanford, Calif. The SA-independent rotavirus RRV variant
nar3 has been previously described (39, 40). All rotavirus
strains were propagated in MA104 cells as described previously
(13). The rhesus monkey epithelial cell line MA104 was grown
in Eagle's minimal essential medium (MEM) supplemented with 10% fetal
bovine serum (FBS) and was used for all experiments carried out in this work. BHK-21, CHO, and L929 cells were grown in MEM containing 10%
FBS. Reovirus type 1 and poliovirus type 3, Leon strain, were kindly
provided by C. Ramos (CISEI, National Institute of Public Health,
Cuernavaca, Mexico) and R. M. del Angel (CINVESTAV-IPN, Mexico
City, Mexico).
Infectivity assay.
MA104 cells in 96-well plates were washed
twice with phosphate-buffered saline (PBS) and then about 1,000 focus-forming units (FFUs) of a trypsin-activated cell lysate
containing rotaviruses RRV, nar3, Wa, or control viruses, reovirus and
poliovirus, was adsorbed to the cells for 45 min at 4°C. After the
adsorption period, the virus inoculum was removed, the cells were
washed once with PBS, MEM was added, and the infection was left to
proceed for 14 h at 37°C. The infected cells were detected by an
immunoperoxidase focus detection assay, using as the detecting antibody
a rabbit polyclonal hyperimmune serum to porcine rotavirus YM, as
described previously (33). The FFUs were counted with the
help of a Visiolab 1000 station (Biocom). This station, which was used
for both image acquisition and analysis, is configured with a Matrox
Meteor RGB frame grabber and a 8295 Cohu RGB CCD color TV camera.
Motorized stages (Marzhauser) were adapted to an inverted Nikon Diaphot 300 microscope. The stage control unit was a Marzhauser Multicontrol MC2000, piloted by Explo (Biocom). Macro command files for Explo were
developed to perform a semiautomated counting of the infected cells. In
this manner, an accurate positioning in the center of each well was
achieved automatically for later predefined scanning and visual
counting of infected cells within a selected well area.
Treatment of MA104 cells with metabolic inhibitors.
Monolayers of MA104 cells in 96-well plates were grown to confluence;
either 2 µg of tunicamycin (Boehringer) per ml or 2 mM benzyl
N-acetyl--D-galactosamide (benzylGalNAc)
(Oxford Glyco Systems) in MEM was added, and the cells were further
incubated for either 24 h (tunicamycin) or 3 days (benzylGalNAc).
To inhibit the synthesis of glycolipids, 60% confluent MA104 cells
were treated with 25 µM
d,l-threo-1-phenyl-2-decanoylamino-3-morpholino-1-propanol (PDMP) (Matreya, Inc.) in MEM-10% FBS for 3 days, replacing the medium with fresh drug daily. After treatment with the respective drug,
the cells were washed twice with PBS and then infected with rotaviruses, reovirus, or poliovirus, as described above. To determine the reconstitution of the susceptibility of the cells to virus infection after drug treatment, the cells were washed twice with PBS at
time zero, MEM was added, and the cell monolayers were kept at 37°C.
At the indicated times, the cells were washed once with PBS and
infected as described above. Cell viability was determined by exclusion
of trypan blue (22).
The effect of tunicamycin and benzylGalNAc on the cellular synthesis of
N- and O-glycans, respectively, was evaluated by detection of sugars on
immunoblots, using a digoxigenin glycan detection kit (Boehringer
Mannheim; no. 1500-783). Under the treatment conditions described
above, glycoconjugates were reduced by about 50% in both tunicamycin-
and benzylGalNAc-treated cells compared to untreated cells (data not shown).
Extraction and immunochemical analyses of lipids from MA104
cells.
PDMP-treated or untreated MA104 cells were harvested by
centrifugation and washed twice with PBS. Total lipids were extracted essentially as described by Guo et al. (19). Thin-layer
chromatography was carried out in a solvent system of
chloroform-methanol-water (5:4:1) containing 12 mM MgCl2.
The plastic plate was dried for 2 h at 37°C and then soaked by
capillarity in n-hexane containing 10% poly(isobutyl
methacrylate) (Aldrich). The glycolipids were then detected
immunochemically on the thin-layer chromatograms, as reported
previously (30), employing the same carbohydrate detection
kit described above. After treatment of MA104 cells with PDMP, as
described above, the content of mono- and disialogangliosides was about
30 to 40% of that found in untreated cells (data not shown).
Cholesterol depletion of MA104 cell monolayers.
Confluent
MA104 cell monolayers in 96-well plates were washed twice with PBS and
then incubated with 10 mM methyl--cyclodextrin (Aldrich) in PBS for
1 h at 37°C with occasional shaking. After this time the cells
were washed twice with PBS and infected as described above.
To replenish the cells with cholesterol after methyl--cyclodextrin
treatment, the drug was removed and the cells in 96-well plates were
washed twice with PBS and then underwent essentially the same treatment
as that described by Falconer et al. (16). Briefly, 200 µl
of MEM-7%FBS with or without 0.1 mM cholesterol (5-cholesten-3-ol-3-hydroxy-5-cholestene) (Sigma), which was freshly made in 100% ethanol, was added per well and left for the
indicated periods. At the end of the incubation time the cells were
washed twice with MEM and infected as described above.
To determine the cholesterol content of untreated or
cyclodextrin-treated MA104 cells, the cells in suspension were
pelleted, the pellet was suspended in 0.8% OG by extensive vortexing,
and the suspension was cleared by centrifugation for 5 min at 2,000 × g in an Eppendorf centrifuge. The cholesterol present in the supernatant or in the cyclodextrin extract of cells was assayed spectrophotometrically using the Boehringer Mannheim diagnostic kit
(no. 139050). All cholesterol determinations were made in the presence
of 0.2% OG.
OG treatment of MA104 cell monolayers.
Confluent MA104 cell
monolayers in 96-well plates were washed twice with PBS. The cells were
then incubated with 0.2% OG (Pierce) in MEM for 90 min at room
temperature with occasional shaking. After this time, the cells were
washed twice with PBS and infected as described above. To determine the
cell viability and the degree of cell membrane permeabilization that
may have been caused by the detergent, we evaluated the ability of the
cells to exclude the vital dye trypan blue and the level of the
cytoplasmic enzyme lactate dehydrogenase in the OG extract
(25). Treatment of cells with 0.2% OG was shown to release
less than 5% of the total lactate dehydrogenase activity. A 100%
lysis was determined by homogenization of the cells in 0.2% OG.
Binding assay.
Rotavirus binding was determined by a
nonradioactive assay, essentially as described by Zárate et al.
(59). Briefly, a suspension of 5 × 104
MA104 cells either untreated, previously treated with PDMP or tunicamycin, or extracted with OG or cyclodextrin, as described above,
was incubated for 1 h at 4°C with 300 ng of trypsin-activated purified viruses in MEM-1% bovine serum albumin. The cell-virus complexes were washed three times with ice-cold PBS containing 0.5%
bovine serum albumin. During the last wash, the cells were transferred
to a fresh Eppendorf tube and then lysed in 50 mM Tris (pH 7.5)-150 mM
NaCl-0.1% Triton X-100. The viruses present in the lysates were
quantified by an enzyme-linked immunosorbent assay (59). In
all assays, a binding control with no cells was performed.
To assay the binding-blocking activity of the OG extract, 300 ng of
purified virus particles was incubated with 20 µg of OG-extracted proteins per ml for 90 min at 37°C. The virus-OG extract mixture was
then added to MA104 cells in suspension, and the assay was performed as
described above. The blocking activity of the hyperimmune sera to the
57- and 75-kDa protein fractions (see below) was assayed by
preincubating the MA104 cells with a 1:5 dilution of the corresponding preimmune or hyperimmune sera for 1 h at 4°C. After the cells were washed with PBS, the viruses were added and the assay was carried
out as described above.
Effect of the OG extract on rotavirus infectivity.
Confluent
MA104 cell monolayers in T-flasks were washed twice with PBS-0.5 mM
EDTA and left to detach in this buffer for 30 min at 37°C. The cells
were counted, pelleted at 85 × g for 5 min at 4°C,
resuspended at a concentration of 2.2 × 107 to
2.5 × 107 cells/ml in MEM-0.2% OG, and incubated
with gentle shaking for 90 min at room temperature. After this time the
cells were pelleted, and the concentration of extracted proteins in the
supernatant was determined by the method of Lowry (Bio-Rad); a typical
concentration was approximately 5 µg of protein/106
cells. The inhibitory activity of this extract on the infectivity of
rotaviruses was measured by incubating dilutions of the extract in MEM
with the virus for 90 min at 37°C. As a control, the viruses were
incubated with 0.2% OG in MEM. To test for the specificity of
inhibition, reovirus and poliovirus were assayed in the same manner as
were rotaviruses. The biochemical nature of the inhibitory factor
present in the OG extract from untreated cells was determined by
boiling (95°C) for 15 min or by incubation of the extract (50 µg of
protein/ml) with 2 mg of tosyl phenylalanine chloromethyl ketone
(TPCK)-treated trypsin (Sigma) per ml for 1 h at 37°C or with 36 mU of neuraminidase per ml for 2 h at 37°C.
Preparative gel electrophoresis.
The proteins extracted from
about 5 × 107 cells (in 2 ml of 0.2% OG) were
adjusted with nonreducing Laemmli sample buffer to give the following
final concentrations: 62.5 mM Tris-HCl (pH 6.8), 2% sodium dodecyl
sulfate (SDS), 10% glycerol, and 0.025% bromophenol blue. These
proteins were immediately loaded, without heating, in a single lane of
a 3-mm-thick, 14-cm-wide preparative SDS-11% polyacrylamide gel. The
gel was run at 8 mA until the bromophenol blue ran out of the gel.
After electrophoresis, the gel was stained in 1% Coomassie blue R-250
in water (22) and slices about 3 mm wide were cut and minced
in PBS; the proteins in the gel pieces were eluted into PBS by mild
shaking for 48 h at room temperature. The eluted proteins were
split into several aliquots, precipitated with 5 volumes of acetone,
washed twice with 80% cold acetone, and dried for 1 min in a Savant
evaporator. To analyze the precipitated proteins, one protein aliquot
was resuspended in reducing (5% -mercaptoethanol) Laemmli sample buffer, boiled for 3 min, and run in an SDS-11% polyacrylamide gel.
The ability of the eluted proteins to block rotavirus infectivity was
tested, as described above, using a second protein aliquot resuspended
in MEM with 1 mM -mercaptoethanol. After the first round of gel
purification, the protein fractions with inhibitory activity were run
in a second preparative 7% polyacrylamide gel and all the Coomassie
blue-stained bands were cut out again, eluted, and assayed for
inhibitory activity. After three rounds of preparative gel
electrophoresis, five protein bands, all of which blocked rotavirus
infectivity, were isolated (see Fig. 8). In each case, after the bands
had been cut out, the proteins were eluted, acetone precipitated, and
resuspended in MEM-1 mM -mercaptoethanol, as described above.
Starting from the second preparative gel, the proteins were recovered
by electroelution: the gel slices were immersed in sample buffer (2%
SDS, 19.2 mM glycine, 2.5 mM Tris base) and electroeluted in an ISCO
chamber for 45 min (3 W) using 0.1% SDS-192 mM glycine-25 mM Tris
base as a running buffer.
Preparation of polyclonal antibodies.
The proteins eluted
from fractions 6 (~57 kDa) and 10 (~75 kDa) (see Fig. 5A), which
were shown to have the maximal inhibitory activity for rotavirus
infection, were used to immunize rabbits, as described previously
(22). Briefly, New Zealand White rabbits (3 to 4 kg) were
immunized subcutaneously with 500 µg of protein in Freund's complete
adjuvant. Two booster injections were given subcutaneously at 2-week
intervals with the same amount of protein emulsified in Freund's
incomplete adjuvant. The rabbits were bled after the third
immunization. A sample of serum was obtained from each animal before immunization.
The ability of the sera to block rotavirus infectivity was assayed by
incubating dilutions of the sera with monolayers of MA104 cells in
96-well plates for 90 min at 37°C. The cells were washed twice with
PBS and then infected as described above. The preimmune sera were used
as negative controls. The hyperimmune sera were tested for their
ability to recognize viruses RRV, nar3, and Wa by an enzyme-linked
immunosorbent assay, as described by Menchaca et al. (37);
at the lowest dilution tested (1:100), no reactivity was found (data
not shown). These antisera did not inhibit the hemagglutination of RRV
and nar3 (data not shown).
Western immunoblotting.
The proteins present in the 0.2% OG
extract were separated in an 11% polyacrylamide gel and transferred to
nitrocellulose. The transferred proteins were incubated with the sera
to the 57- and 75-kDa fractions, diluted 1:1,000 in PBS. The bound
antibodies were developed by incubation with protein A-peroxidase, and
3-amino-9-ethyl-carbazole (Sigma) was added as a substrate, as
previously described by Arias et al. (1).
Immunofluorescence.
MA104 cells grown on glass coverslips to
approximately 80% confluence were fixed with 4% paraformaldehyde in
PBS for 20 min at 37°C. After this time the cells were washed twice
with PBS, either permeabilized or not by incubation with PBS-0.5%
Triton X-100 for 5 min at room temperature, and then washed twice with PBS with gentle swirling. The fixed cells were blocked with 1 M glycine
for 1 h at 37°C, washed twice with PBS, and then incubated with
a 1:1,000 (anti-57-kDa fraction) or 1:1,500 (anti-75 kDa fraction)
dilution of the sera for 90 min at 37°C. The cells were washed four
times with PBS and then incubated in the dark for 1 h at 4°C
with a goat anti-rabbit immunoglobulin G coupled to fluorescein
isothiocyanate (Dako Co.), diluted 1:100 in PBS. The cells were washed
four times with PBS and mounted on glass slides on 10% glycerol in
PBS. The slides were analyzed using a Bio-Rad MRC-600 microscope. The
preimmune sera were used as negative controls.
| |
RESULTS |
Inhibitors of N glycosylation and glycolipid synthesis block
rotavirus infection.
To assess the biochemical nature of the
cellular receptor for rotaviruses, MA104 cells were treated with
specific inhibitors of glycosylation prior to infection. Two inhibitors
were used: tunicamycin, which blocks an early step in the
N-glycosylation pathway involving transfer between UDP-GlcNAc and
dolichol-1-phosphate (12), and benzylGalNAc, which is a
competitive inhibitor of the transferase
(N-acetyl--D-galactosaminyltransferase)
involved in the first step of the biosynthesis of most types of
O-linked carbohydrates (5). In addition, we used the
synthetic analog of ceramide, PDMP, to inhibit the biosynthesis of the
glycosphingolipid precursor glucosylceramide (45). The cells
pretreated with the inhibitors were then infected with either wild-type
RRV, the neuraminidase-resistant RRV variant nar3, or the HRV strain Wa.
Treatment of cells with 2 µg of tunicamycin per ml for 24 h
before infection inhibited the infectivity of rotaviruses RRV and nar3
by about 50%, while preincubation of the cells for 3 days with PDMP,
the inhibitor of glycolipids synthesis, blocked the infectivity of the
viruses by about 80% (RRV and Wa) or 60% (nar3) (Table
1). On the other hand, inhibition of O
glycosylation by benzylGalNAc had no effect on the infectivity of RRV
but increased the infectivity of nar3 and Wa by about 50%, indicating
that under conditions where the levels of cell surface O-linked
carbohydrates are decreased, these viruses infect the cell more
efficiently. The total cell content of N- and O-glycoproteins was
reduced by at least 50% by the corresponding inhibitory drug (data not
shown). The infectivity of reovirus and poliovirus, which were used as controls, was not inhibited by any of these three drugs, with poliovirus actually showing a twofold increase in infectivity in the
cells treated with tunicamycin (Table 1), as has been reported for
other viruses like human immunodeficiency virus type 2 and
B-lymphotropic papovavirus (28, 43).
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TABLE 1.
Effect of metabolic inhibitors, cell membrane cholesterol
depletion, and OG on the infectivity of rotaviruses in MA104 cells
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Under the conditions employed, the inhibitors did not have a
significant effect on cell protein synthesis, as judged by
electrophoresis of 35S-labeled proteins, or on the
viability of cells, as judged by trypan blue exclusion (data not
shown). To control for a possible nonspecific, toxic effect of the
drugs on the replication of rotaviruses, in a separate experiment we
added the inhibitors immediately after the virus had been adsorbed for
45 min at 4°C. Under these conditions the drugs did not affect
rotavirus infectivity, with the exception of rotavirus Wa, whose
infectivity was decreased about 50% by tunicamycin; for this reason,
this inhibition was considered to be nonspecific. The effect of the
inhibitors was reversible since the cells became fully susceptible to
rotavirus infection by about 20 and 24 h after removing
tunicamycin and PDMP, respectively (data not shown). Taken together
these results suggest that glycolipids and N-glycosylated but not
O-glycosylated proteins are important for rotavirus infection. To
determine if the treatment of cells with tunicamycin and PDMP inhibited
the attachment of the virus to the cell surface or if the inhibition of
infectivity occurred at a postattachment step, we performed binding
assays using cells treated with the different drugs. We found that
treatment of cells with tunicamycin did not affect the binding of
either of the three viruses tested while treatment of cells with PDMP
did not affect the attachment of RRV and Wa but decreased the binding
of nar3 by 54% (Table 2). This level of
inhibition in the attachment of the virus to cells is very similar to
the 60% inhibition in the infectivity of nar3 caused by PDMP (Table
1), which suggests that most if not all of the blockage in the
infectivity of nar3 in PDMP-treated cells is due to an inhibition of
the binding of this variant to the cell surface.
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TABLE 2.
Effect of metabolic inhibitors, cell membrane cholesterol
depletion, and OG on the binding of rotaviruses to MA104 cells
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Infection of octyl--glucoside-extracted cells.
As a
different approach to characterize the rotavirus receptor, we used the
nonionic detergent OG to extract the receptor from the cell membrane
under noncytolytic conditions, as has been described for other virus
receptors (2, 10, 23, 36, 49, 55). MA104 cells were
incubated with 0.2% OG for 90 min at room temperature; under these
conditions the cells maintained their viability and integrity, as
judged by trypan blue exclusion and the low levels of lactate
dehydrogenase activity, a cytosolic marker detected in the OG extract
(less than 5% of total enzyme activity). The cells extracted with the
detergent were found to be about 60% refractory to infection by the
three viruses tested (Table 1). As described above for the metabolic
inhibitors, this effect was also found to be reversible; if the
detergent was washed away after the treatment period, the cells fully
regained their susceptibility for infection at about 8 h
posttreatment (Fig. 1A), which most
probably accounts for the time of synthesis, transport, and
accumulation of the receptor in the cell membrane at the levels needed
for the virus to efficiently infect the cell. Of interest, the
attachment of all three viruses to OG-extracted cells was inhibited by
60 to 70% (Table 2), indicating that the reduced infectivity of the
viruses in OG-treated cells might be due to a decreased ability of the
virus particles to bind to the cell surface.
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FIG. 1.
(A) Recovery of the susceptibility of MA104 cells to
rotavirus infection after extraction with OG. Cell monolayers in
96-well plates were extracted with 0.2% OG and allowed to recover in
MEM at 37°C. At the indicated times, the monolayers were washed with
PBS and infected with rotaviruses. (B) Inhibition of rotavirus
infectivity by the OG extract from MA104 cells. The indicated
concentrations of OG-extracted protein were incubated with the viruses
for 90 min at 37°C. The virus-protein mixtures were used to infect
MA104 cell monolayers in 96-well plates. In both panels, the percent
infectivity is relative to the infectivity of the viruses incubated in
0.2% OG. Error bars represent 1 standard error of the mean of three or
more experiments carried out in duplicate.
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The OG extract inhibits rotavirus infection.
Since treatment
of MA104 cells with OG diminished the ability of the viruses to attach
to and thus to infect cells, it is likely that the detergent was
extracting cell surface molecules involved in the initial interaction
of rotaviruses with the cell, possibly the rotavirus receptor(s). If
this were the case, the molecule(s) present in the OG extract could
interact with the virus in solution, preventing the binding of the
virus to the cell membrane and thus blocking its infectivity. We found
that incubation of the OG extract with either of the three rotavirus strains did block their infectivity in a concentration-dependent manner
(Fig. 1B). At the maximum concentration tested, 400 µg of protein per
ml, the infectivity of the viruses was inhibited by about 95%; 50%
inhibition was achieved at about 40 µg of protein per ml. In
contrast, the infectivity of poliovirus and reovirus was not affected
by the extract (Fig. 1B). These results strongly suggest a specific
interaction of the viruses with the OG-solubilized cell surface
molecules. Preincubation of the viruses with a solution of 0.2% OG did
not affect their infectivity. The infectivity in the presence of OG was
taken as the 100% value for each virus.
The inhibition of rotavirus infectivity caused by the OG extract seems
to be due to a blockage in cell attachment since preincubation of the
viruses with 20 µg of the OG-extracted protein per ml decreased RRV
binding to the cell by 40%, nar3 binding by 41%, and Wa binding by
43% (Table 3). These percentages are in
close agreement with the degree of inhibition of infectivity achieved
with this concentration of extract (Fig. 1B).
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TABLE 3.
Effect of the OG extract, and antibodies to 75 kDa OG
protein fraction, on the binding of rotaviruses to
MA104 cellsa
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The inhibitory capacity of OG extracts obtained from BHK, CHO, and L
cells, which are about 1,000-fold less susceptible to rotavirus
infection than MA104 cells, was determined. As can be seen in Fig.
2, the OG extracts from the three poorly
permissive cells showed some inhibitory activity, although in all cases
this activity was less pronounced than that observed with the extract from MA104 cells.
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FIG. 2.
Inhibition of rotavirus infectivity by OG extracts from
cells poorly permissive to rotavirus infection. OG-extracted proteins
(20 µg/ml) from CHO, BHK, L, or MA104 cells (as indicated) were
incubated with the viruses for 90 min at 37°C. The virus-protein
mixtures were used to infect MA104 cell monolayers in 96-well plates.
The percent infectivity is relative to the infectivity of the viruses
incubated in 0.2% OG. Error bars represent 1 standard error of the
mean of three experiments carried out in duplicate.
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Biochemical nature of the inhibitory component present in the MA104
OG cell extract.
To determine the biochemical nature of the
inhibitory component present in the OG cell extract, we tested the
effect of heat inactivation, neuraminidase, and proteolytic treatment
on the inhibitory activity of the extract. We found that either boiling for 15 min or treatment with trypsin completely abolished the inhibitory activity while treatment with neuraminidase had no effect on
the blocking capacity of the extract (Fig.
3). These results indicate that the
inhibitory component of the extract is a protein.
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FIG. 3.
Biochemical nature of the inhibitory factor present in
the OG extract. A 0.2% OG extract was obtained from cells in
suspension. Just prior to the incubation with the virus, the extract
was either boiled (95°C) for 15 min (heat), incubated with 2 mg of
trypsin per ml of extract for 1 h at 37°C (trypsin), or
incubated with 36 mU of neuraminidase per ml (NA). The untreated
extract (no treatment) was used as a positive control. Viruses and
extract (100 µg of protein extract per ml of virus) were mixed and
incubated for 90 min at 37°C, and then MA104 cells in 96-well plates
were infected with the virus-protein mixtures. The percent infectivity
is relative to the infectivity of viruses incubated with a solution of
0.2% OG in MEM (virus control). Error bars represent 1 standard error
of the mean of three or more experiments carried out in duplicate.
|
|
The profile of proteins extracted with OG is shown in Fig.
4A, lane 5. Treatment with tunicamycin,
PDMP, or neuraminidase modifies this profile (lanes 2 to 4), reflecting
the modification in the carbohydrate content of glycoproteins caused by
tunicamycin and neuraminidase. In the case of PDMP, this result
suggests that the impaired synthesis of glycolipids alters either the
transport of proteins to the plasma membrane or their extractability
from the cell surface by OG. In this regard, it is of interest that the
OG extract from PDMP-treated cells failed to block rotavirus infectivity (data not shown), suggesting that the inhibitory proteins could not be extracted from these cells.
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FIG. 4.
Analysis of the proteins extracted from MA104 cells.
Cell monolayers were treated with either neuraminidase, tunicamycin, or
PDMP, as described in Materials and Methods, and the cells were then
extracted with 0.2% OG for 90 min at room temperature. (A) The
extracted proteins were separated by electrophoresis under reducing
conditions in an SDS-11% polyacrylamide gel and silver stained.
OG-extracted proteins from MA104 cells treated with neuraminidase (lane
2), tunicamycin (lane 3), or PDMP (lane 4) or left untreated (lane 5)
are shown. Lane 1 contains molecular mass markers. (B) Cells in
suspension were extracted with 10 mM -cyclodextrin for 1 h at
37°C, as described in Materials and Methods. Proteins in untreated
cells (lane 1), extracted cells (lane 2), and the cyclodextrin extract
(lane 3) were analyzed by gel electrophoresis.
|
|
Cholesterol depletion of MA104 cells inhibits rotavirus
infectivity.
It has been proposed that glycosphingolipids,
cholesterol, and proteins can interact specifically in cell membranes
to form microdomains termed rafts (46). Given the
involvement of glycolipids and N-glycosylated proteins on rotavirus
infectivity, we tested if depletion of the cell cholesterol would have
any effect on virus infectivity. To do this, we incubated the cells
with 10 mM -cyclodextrin for 1 h at 37°C; this treatment has
been shown to selectively extract cholesterol from the plasma membrane
in preference to other membrane lipids (28). Under these
conditions, about two-thirds (65%) of the cell cholesterol was removed
(see Materials and Methods). The treatment of cells with
-cyclodextrin inhibited the infectivity of RRV, nar3, and Wa
rotavirus strains by more than 90% but had no effect on the
infectivity of reovirus and poliovirus (Table 1). It is noteworthy that
the binding of the three rotavirus strains was not affected (Table 2),
indicating that the decrease in the cholesterol content of the cell
affects virus infectivity at a postattachment step.
The protein profile of cells treated with -cyclodextrin was not very
different from that of untreated cells (Fig. 4B, lanes 1 and 2), even
though this antibiotic extracted a small amount of protein from the
cells (lane 3).
To demonstrate that the depletion of cholesterol was the cause of the
reduction of virus infectivity after the -cyclodextrin treatment,
cells in 96-well plates were washed twice with MEM, and then either MEM
alone, MEM-7% FBS, or MEM-7% FBS containing 0.1 mM cholesterol was
added for different times. At the end of the incubation period, the
cells were washed twice and infected with rotaviruses. At 8 h
posttreatment, the cells incubated in the presence of cholesterol had
fully recovered their susceptibility to rotaviruses while the cells
incubated with MEM alone or MEM-7% FBS were still about 80 and 50%
refractory to rotavirus infection, respectively (data not shown).
Fractionation of the inhibitory components present in the OG
extract from MA104 cells.
To characterize the proteins that block
rotavirus infection, we fractionated the OG extract obtained from MA104
cells by preparative SDS-polyacrylamide gel electrophoresis. After the
gel electrophoresis, slices of a single-lane gel were cutout, and the
proteins were eluted in PBS, concentrated by precipitation with
acetone, and resuspended in PBS with 1 mM -mercaptoethanol. This
method has been successful for recovering proteins with enzymatic
activity (20, 48). The proteins obtained from the different
fractions (Fig. 5B) were tested for their
ability to block rotavirus infection. Proteins eluted from two
well-defined regions of the gel, around 57- and 75 kDa, had the ability
to efficiently inhibit the infectivity of all three rotaviruses tested
(Fig. 5A). The pattern of inhibition observed in Fig. 5A was found to
be consistent in independent gel fractionation experiments.
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FIG. 5.
Inhibition of rotavirus infectivity by OG-extracted
proteins fractionated by gel electrophoresis. About 250 µg of
proteins extracted with 0.2% OG from MA104 cells was separated by
preparative SDS-polyacrylamide gel electrophoresis under nonreducing
conditions. After electrophoresis, the gel was stained with Coomassie
blue in water, gel slices were cut out, and the proteins were eluted.
(A) Inhibitory activity of the eluted proteins present in the fractions
shown in panel B. (B) Gel electrophoresis of the eluted protein
fractions. Only the portion of the gel where inhibitory activity was
found is shown; the remaining higher- and lower-molecular-mass protein
fractions had no inhibitory activity.
|
|
Antibodies to the OG extract protein fractions inhibit rotavirus
infection.
Protein fractions 6 and 10 in Fig. 5A, which represent
the peak of inhibitory activity, were used to immunize rabbits. The hyperimmune sera obtained against these two fractions were found to
block the infectivity of all three strains of rotavirus when preincubated with the cells for 90 min at 37°C prior to addition of
the virus, while the preimmune sera had no effect (shown for the serum
to the 75-kDa protein fraction in Fig.
6A). The inhibitory effect of the two
antisera was not additive since a mixture of the two inhibited
rotavirus infectivity by about 70% at a dilution of 1/100 (data not
shown). Of interest, both sera blocked the infectivity of HRV Wa and
that of the SA-independent variant nar3 in cells treated with
neuraminidase (shown for the serum to the 75-kDa fraction in Fig. 6B),
suggesting that they contain antibodies to an SA-independent rotavirus
receptor. In a binding inhibition assay, the serum to the 75-kDa
fraction did not inhibit the attachment of rotavirus RRV to MA104 cells
but inhibited 32% of the binding of nar3 and 72% of that of Wa (Table
3). The blocking specificity of these antisera was confirmed by the
following assays: they did not recognize any of the three viruses by
enzyme-linked immunosorbent assay, and they did not inhibit the
hemagglutination activity of RRV and nar3. Furthermore, the sera were
shown not to inhibit the infectivity of poliovirus or that of reovirus
in an FFU reduction assay as described in Materials and Methods for
rotavirus (data not shown).
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FIG. 6.
Inhibitory activity of hyperimmune sera to OG-extracted
proteins. (A and B) OG protein fractions 6 and 10 shown in Fig. 5B,
containing polypeptides of around 57 and 75 kDa, respectively, were
used to raise antibodies in rabbits. Serial dilutions of the preimmune
(dashed lines) and hyperimmune (continuous lines) sera to the 75-kDa
protein fraction were incubated with untreated (A) or neuraminidase
(NA)-treated (B) MA104 cells for 90 min at 37°C before addition of
the virus. Similar inhibition results were obtained with the serum to
the 57-kDa protein fraction (data not shown). Error bars represent 1 standard error of the mean of three or more experiments carried out in
duplicate. (C) Immunoblot analysis of the OG-extracted proteins. The
proteins extracted from MA104 cells with 0.2% OG were separated in an
SDS-11% polyacrylamide gel under reducing conditions and transferred
to nitrocellulose. The transferred proteins were incubated with a
1,000-fold dilution of the preimmune (lanes 1 and 2) or hyperimmune
(lanes 3 and 4) sera to the 57-kDa (lanes 2 and 4) or 75-kDa (lanes 1 and 3) protein fractions. The bound antibodies were developed by
incubation with protein A-peroxidase and a chromogenic substrate.
|
|
By Western blotting, the sera to the 75-kDa fraction recognized a
protein of about 73 kDa and, to a lesser extent, a protein of about 57 kDa in the 0.2% OG cell extract (Fig. 6C, lane 3). Of interest, the
serum to the 57-kDa protein fraction also recognized proteins of 73 and
57 kDa, although the latter protein was recognized more efficiently by
this serum (lane 4). The preimmune sera did not recognize any of these
proteins (lanes 1 and 2).
The hyperimmune sera were shown to recognize proteins on the surface of
the MA104 cells, as judged by their reactivity with nonpermeabilized
cells by flow cytometry (data not shown) and by indirect
immunofluorescence (shown for the anti-75-kDa serum in Fig.
7). The pattern of immunofluorescence
(for both anti-57- and anti-75-kDa sera) was patchy over the surface of
the cell, but there was a higher concentration of the fluorescent
signal on the intercellular junctions (Fig. 7A). In permeabilized
cells, a weak signal associated mainly with the nuclei was found (Fig. 7B). No fluorescent signal was detected when the preimmune sera were
used to stain either permeabilized or nonpermeabilized cells (Fig. 7C
and D).
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FIG. 7.
Immunofluorescence of cells incubated with the serum to
the 75-kDa OG protein fraction. MA104 cells were fixed with
paraformaldehyde and permeabilized with Triton X-100 (B and D) or not
permeabilized (A and C). The cells were incubated with a 1:1,500
dilution of the preimmune (C and D) or hyperimmune (A and B) sera to
the 75-kDa protein fraction for 90 min at 37°C and stained with a
goat anti-rabbit immunoglobulin G coupled to fluorescein
isothiocyanate.
|
|
Purification of the cellular proteins which block rotavirus
infectivity.
The proteins with rotavirus blocking activity were
purified by SDS-polyacrylamide gel electrophoresis from an OG extract
obtained from MA104 cells. After three rounds of purification by gel
electrophoresis, using the inhibitory activity of the proteins as
marker, we were able to isolate five bands with molecular masses of
approximately 110, 75, 57, 45, and 30 kDa (Fig.
8) which were able to inhibit the
infectivity of all three rotavirus strains tested. Although these
proteins consistently inhibited rotavirus infectivity through the
rounds of purification carried out, the final amount of protein recovered was small, which prevented us from determining the precise specific inhibitory activity for each protein and testing if they were
recognized by the hyperimmune sera. Table
4 shows the results of a blocking
infectivity assay with the purified proteins; in this blocking assay,
the same amount of protein shown in the gel in Fig. 8 was used. The
relative inhibitory activity of each protein for all three viruses was
found to be 75 kDa > 110 kDa > 45 kDa = 30 kDa > 57 kDa. Given the fractionation method employed, it is quite possible
that each of these bands may represent more than one protein species.
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FIG. 8.
Isolated proteins with inhibitory activity for rotavirus
infectivity. The protein bands that were shown to block rotavirus
infectivity after three rounds of purification by preparative gel
electrophoresis (see Table 4) were analyzed in an 11% polyacrylamide
gel under reducing conditions. The protein bands were detected by
silver staining.
|
|
| |
DISCUSSION |
The entry of rotaviruses into MA104 cells seems to be a multistep
process involving interactions of the virus surface protein VP4 and
maybe of VP7 with more than one cell surface site present in either the
same or a different cellular structure(s) (11, 41).
In the present study we employed two approaches to characterize the
biochemical nature of the rotavirus receptor(s). In the first approach
we used metabolic inhibitors of glycosylation and synthesis of
glycolipids to study their effect on the infectivity of three different
rotavirus strains. We found that tunicamycin, an inhibitor of protein N
glycosylation, diminished the infectivity of rotaviruses RRV and nar3
despite their differential dependence on SA for infectivity, implying
that these viruses interact with N-linked glycoproteins at some point
during cell entry. The fact that the treatment of cells with this drug
did not affect the binding of the viruses suggests that the blockage
occurs after the initial attachment of the virion to the cell surface.
Tunicamycin has been successfully used to specifically analyze the role
of N-glycans as receptors for several viruses (7, 28, 43, 44).
Treatment of MA104 cells with PDMP, an inhibitor of glycolipid
biosynthesis, resulted in the more pronounced inhibition of infectivity
observed for all three rotavirus strains (Table 1). Interaction of
rotaviruses with gangliosides GM1 and GM3 has been reported (47,
52), and this interaction has been shown to be SA dependent. In
this case, however, the inhibition caused by PDMP seems not to be the
result of a deficient attachment of the SA-dependent rotavirus RRV to
the cell surface since it was not significantly affected (Table 2).
This observation suggests that RRV does not interact, or at least does
not interact exclusively, with the SA present on PDMP-sensitive
gangliosides. On the other hand, the binding of the SA-independent
variant nar3 was decreased in PDMP-treated cells, suggesting that
either glycosphingolipids or, more probably, a protein whose correct
transport or conformation depends on their presence might be used by
nar3 to attach to the cell. Of interest, the binding of the HRV strain
Wa was not affected by PDMP, in agreement with the suggestion that nar3
and Wa, despite having an infectivity resistant to neuraminidase
treatment of cells, bind to different cell surface sites
(41). Finally, the fact that PDMP, but not tunicamycin,
affected the attachment of nar3 suggests that the inhibition caused by
the N-glycosylation inhibitor is not due to its reported ability to
inhibit ganglioside biosynthesis (50, 58).
In addition to the involvement of N-glycosylated proteins and
glycolipids in rotavirus entry, we found that cholesterol depletion inhibited the infectivity of rotaviruses by more than 90% (Table 1).
These findings are of interest with regard to the recent description of
functional lipid microdomains, or rafts, in the cell membrane
(51). These rafts have been proposed to be composed of
cholesterol, glycosphingolipids (gangliosides among others), and a
specific set of associated proteins. They are thought to function as
specialized platforms for apical cell sorting of proteins and signal
transduction. For some proteins which form part of these lipid
microdomains (oxytocin receptor, placental alkaline phosphatase, gD1
decay-accelerating factor), the disassembly of the rafts by cholesterol
depletion disrupts or modifies the receptor activity, even though the
receptor might be present in the same abundance on the cell membrane
(21, 29). In this regard, the finding that the attachment of
RRV, nar3, and Wa to cholesterol-depleted cells is not affected while
their infectivity is severely impaired is consistent with the
possibility that the rotavirus receptor(s) might be forming part of
some of these lipid microdomains. It is tempting to hypothesize that in
cholesterol-depleted cells, the receptor(s) retains its ability to bind
rotavirus particles but in order to fully promote virus entry it must
be organized in a lipid microdomain. In addition, the fact that the OG
extract from PDMP-treated cells failed to show inhibitory activity
suggests that PDMP treatment may have disrupted the lipid raft
organization such than one or more of the active proteins in Fig. 8
never became associated with or localized within these membrane
microdomains and as result are not extracted with OG. Experiments are
under way to test this hypothesis.
The infectivity of the two nonenveloped viruses that were used as
controls, poliovirus and reovirus, was not inhibited by the described
drugs, showing that the effect observed on the infectivity of
rotaviruses was specific. The human poliovirus receptor is an integral
membrane protein with the conserved amino acids and domain structure
characteristic of members of the immunoglobulin superfamily (31,
38). The nature of the reovirus receptor is less well defined;
most of the available evidence suggest that reovirus binds to multiple
sialoglycoproteins rather to a single homogeneous species on the cell
surface (8, 18, 42).
In a second approach to characterize the rotavirus receptor, MA104
cells were incubated with a solution of 0.2% OG. It has been shown
that at low concentrations, like the one used in this work, OG is able
to extract proteins from the cell surface without impairing the
viability of the cells (see Results) (23, 36). This nonionic
detergent has been useful in experiments to obtain the receptors for
Semliki Forest virus, parvovirus, vesicular stomatitis virus,
polyomavirus, simian virus 40, and rabies virus from intact cell
monolayers (2, 10, 23, 36, 49, 55). MA104 cells extracted
with OG lost their ability to bind rotaviruses by about the same extent
(60%) to which they became refractory to infection, suggesting that OG
extracts from the cell surface the receptor molecules needed by all
three strains of rotavirus to attach to and thus infect the cell. In
agreement with this finding is the fact that the OG extract, when
preincubated with these viruses, inhibited both their binding to and
infection of MA104 cells. This suggests that the putative
OG-solubilized cell receptors are able to interact with the viruses in
solution. The inhibitory activity of the OG extract was lost by
treatment with proteases and heat but not by treatment with
neuraminidase, indicating that the active component is a protein.
To test for a correlation between the susceptibility of the cell line
and the ability of the OG extract to inhibit rotavirus infection, we
obtained OG extracts from BHK, CHO, and L cells, which are about
1,000-fold less susceptible to rotavirus infection than are MA104
cells. The extracts from these three cell lines inhibited the
infectivity of rotaviruses to different degrees but in general to a
lesser extent than that achieved with the MA104 cell extract (Fig. 2).
As suggested in this work and by others (11, 41), these
results might be explained if more than one cell surface molecule were
implicated in rotavirus infection, which would make possible the
absence of one of the receptor molecules in the less susceptible cell
lines while other surface components, which could be extracted with OG
and block rotavirus infectivity, would still be present.
Two protein fractions with blocking activity for rotavirus infectivity
were obtained by gel fractionation of the OG extract of the MA104
cells. The hyperimmune sera prepared against these two fractions were
shown to react primarily with two polypeptides of 73 and 57 kDa.
Although it is not possible to be certain if the more immunogenic
proteins are the active inhibitory components of the extract, it seems
at least that the inhibitory antibodies present in both hyperimmune
sera recognize the same cell surface molecule or different molecules in
a protein complex since the blocking efficiency of the individual sera
was not additive and since the cell surface recognition patterns
obtained with the two antisera were strikingly similar.
Five individual protein bands with inhibitory activity for rotavirus
infectivity were isolated from the OG extract. These proteins need to
be assayed to test the specificity of their inhibitory activity and to
investigate if they are somehow related to each other. However, the
fact that all of these proteins block the infectivity of RRV, nar3, and
Wa rotaviruses suggest that at least one of them, or a complex formed
by more than one, could be a common cellular receptor for rotaviruses.
The determination of the identity of these proteins should help to
define the cell surface molecules involved in the interactions that
seem to occur between rotaviruses and the cell surface during infection.
As a working hypothesis, we propose that the rotavirus receptor is
likely to be a complex of several cell components including gangliosides, N-linked glycoproteins, and probably other proteins which
might all associate in lipid rafts and need the lipid microdomain organization to function efficiently in the binding and internalization of rotavirus particles. The protein components of this proposed complex
could include the integrin molecules that have been reported recently
(11, 24).
| |
ACKNOWLEDGMENTS |
We thank Rafaela Espinosa for the immunofluorescence experiments,
Pavel Isa for the flow cytometric analysis, and Leticia Vega Alvarado
for her contribution to the development of the command files to
semiautomatically count infected cells.
This work was partially supported by grants 75197-527106 from the
Howard Hughes Medical Institute, G0012-N9607 from the National Council for Science and Technology
Mexico, and
IN207496/IN201399 from DGAPA-UNAM.
| |
FOOTNOTES |
*
Corresponding author. Mailing address: Instituto de
Biotecnología/UNAM, A.P. 510-3, Colonia Miraval, Cuernavaca,
Morelos 62250, México. Phone: (52-73) 29-1661. Fax (52-73)
17-2388. E-mail: arias{at}ibt.unam.mx.
Permanent address: Departamento de Bioquímica, Facultad de
Medicina, Universidad Nacional de Colombia, Bogotá, Colombia.
| |
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Abstract
Introduction
