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Journal of Virology, December 2000, p. 11377-11387, Vol. 74, No. 23
0022-538X/00/$04.00+0
Copyright © 2000, American Society for Microbiology. All rights reserved.
Glycoprotein E of Varicella-Zoster Virus Enhances
Cell-Cell Contact in Polarized Epithelial Cells
Chengjun
Mo,1,*
Eveline E.
Schneeberger,2 and
Ann M.
Arvin1
Department of Pediatrics, Stanford University
School of Medicine, Stanford, California 94305,1
and Department of Pathology, Massachusetts General
Hospital, Boston, Massachusetts 021142
Received 19 June 2000/Accepted 7 September 2000
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ABSTRACT |
Varicella-zoster virus (VZV) infection involves the cell-cell
spread of virions, but how viral proteins interact with the host cell
membranes that comprise intercellular junctions is not known.
Madin-Darby canine kidney (MDCK) cells were constructed to express the
glycoproteins gE, gI, or gE/gI constitutively and were used to examine
the effects of these VZV glycoproteins in polarized epithelial cells.
At low cell density, VZV gE induced partial tight junction (TJ)
formation under low-calcium conditions, whether expressed alone or with
gI. Although most VZV gE was intracellular, gE was also shown to
colocalize with the TJ protein ZO-1 with or without concomitant
expression of gI. Freeze fracture electron microscopy revealed normal
TJ strand morphology in gE-expressing MDCK cells. Functionally, the
expression of gE was associated with a marked acceleration in the
establishment of maximum transepithelial electrical resistance (TER) in
MDCK-gE cells; MDCK-gI and MDCK-gE/gI cells exhibited a similar pattern
of early TER compared to MDCK cells, although peak resistances were
lower than those of gE alone. VZV gE expression altered F-actin
organization and lipid distribution, but coexpression of gI modulated
these effects. Two regions of the gE ectodomain, amino acids (aa) 278 to 355 and aa 467 to 498, although lacking Ca2+ binding
motifs, exhibit similarities with corresponding regions of the cell
adhesion molecules, E-cadherin and desmocollin. These observations
suggest that VZV gE and gE/gI may contribute to viral pathogenesis by
facilitating epithelial cell-cell contacts.
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INTRODUCTION |
Varicella-zoster virus (VZV) is a
human alphaherpesvirus that causes two diseases, varicella (chicken
pox) and herpes zoster (shingles); the latter disease is a recurrent
infection following prolonged latency in sensory ganglia. Despite
genetic similarities, VZV exhibits an extreme host range restriction in
vivo and grows poorly in tissue culture, suggesting that its pathogenic
mechanisms differ from those of related herpesviruses. The herpesvirus
glycoproteins function at several points in the replication cycle,
including viral attachment, entry, envelopment, cell-cell spread, and
egress. The VZV glycoproteins gB, gC, gE, gH, gI, gL, gK, and the
putative gM have some homology with those of herpes simplex virus type 1 (HSV-1), HSV-2, pseudorabies virus (PRV), and the other nonhuman alphaherpesviruses, but VZV lacks gD and gG (12, 24).
Although the spread of VZV is associated with extensive fusion of cell membranes, information about the processes by which VZV and other herpesviruses move to cell junctions, including tight junctions (TJ) as
well as adherens junctions, and invade adjacent, uninfected cells is
limited. These processes are important for VZV replication, since
syncytium formation is a hallmark of VZV infection in vitro and
multinucleated polykaryocytes are common in VZV-infected tissues.
The VZV glycoproteins gE and gI form heterodimers and, like the
corresponding proteins of HSV and PRV, are likely to be involved in
cell-cell spread (3, 4, 15, 19, 30, 56). The functions of
VZV gE and the gE/gI complex are of particular interest because, unlike
the case for other alphaherpesviruses, gE deletion appears to be
incompatible with VZV replication (35). While gI deletion
mutants replicate in melanoma cells, intact gI is necessary to achieve
the polykaryocyte formation characteristic of VZV infection
(35). Full or partial deletion of gI inhibited syncytium
formation, altered the conformation and distribution of gE, and reduced
infectious-virus yields in melanoma cells (35), and gI was
required to generate infectious progeny and to allow normal processing
of gE in Vero cells (11).
VZV gE has multiple functions, including Fc receptor activity for
nonimmune immunoglobulin G (IgG) (31), binding to
mannose-6-phosphate receptors, which may facilitate virus entry, and
interaction with the major tegument protein, IE62, which may be
involved in virion assembly (58). VZV gE has targeting
sequences for the trans-Golgi network (TGN) and is transported from the
endoplasmic reticulum (ER) to the TGN in infected and gE-transfected
cells (1, 20, 59). VZV gI is also a type I membrane protein
that is transported to the TGN and to cellular membranes in
VZV-infected and gI-transfected cells (1, 2). In addition,
VZV gE may serve as a navigator glycoprotein, forming complexes that
direct signal-deficient viral glycoproteins to the TGN (55).
Expression of gE using the vaccinia virus-T7 RNA polymerase
transfection system indicates that gE undergoes endocytosis from the
cell membrane, returning to endosomes and TGN, and recycles back to the
cell membrane in a continual trafficking pattern (43, 44).
Coexpression of gE/gI in vaccinia virus-infected cells also indicates
that gI facilitates gE endocytosis and regulates the trafficking of the
gE/gI Fc receptor complex (41).
The purpose of these experiments was to investigate how VZV gE and gI
and the gE/gI complex may function in epithelial cells. Epithelial cells are important in VZV pathogenesis because the virus
enters the host through respiratory mucosal epithelial cells during
primary infection and is transmitted to susceptible contacts following cell-cell spread and virus release from mucosal and cutaneous
epithelial cells. Madin-Darby canine kidney (MDCK) cell lines
were constructed to express the VZV glycoproteins constitutively. MDCK are polarized epithelial cells in which cellular membrane proteins
are restricted to discrete apical and basolateral domains, whereas the
same proteins are distributed uniformly on the surfaces of fibroblasts
and other nonpolarized cells usually used to investigate VZV
replication in vitro. In epithelial cells, cell-cell adhesion and
formation of TJ are triggered by Ca2+ and are associated
with localization of occludin, ZO-1, ZO-2, E-cadherin, and 
-catenin
to targeted regions of the cell membrane (25, 40). Actin
filaments and other cell structural components are also rearranged when
these cells become confluent (23). We found that VZV gE
expression had multiple effects on MDCK cells. First, it resulted in
partial TJ formation under low-Ca2+ (LC) conditions whether
expressed with or without gI, indicating the capacity to enhance
cell-cell contact. Second, VZV gE expression was associated with rapid
establishment of TJ gate function, measured by transepithelial
electrical resistance (TER) in the presence or absence of gI. As
expected, gE expression on cell membranes was limited relative to the
intracellular signal, but confocal microscopy suggested colocalization
of gE with the cell TJ protein ZO-1. Expression of gE at or near ZO-1
occurred without disruption of normal TJ structures by freeze fracture
electron microscopy. However, VZV gE affected the cytoskeleton protein,
F-actin, and lipid diffusion in MDCK cells, and these effects on
structural components of epithelial cells appeared to be modulated by
the coexpression of gI.
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MATERIALS AND METHODS |
Cells and gE- and gI-expressing cell lines.
MDCK clone II/G
cells (36) were grown in Dulbecco minimal essential medium
(DMEM) supplemented with 10% fetal calf serum (FCS), penicillin,
streptomycin, and kanamycin. The gE-expressing cell lines
containing the ORF68 gene were constructed by inserting a PCR
fragment containing the VZV gE-coding region into TA cloning sites of
the pCR3.1 plasmid vector (Invitrogen, Carlsbad, Calif.) to make
the plasmid pVZVgE. Similarly, the gI-expressing cell lines
containing the ORF67 gene were constructed by inserting a PCR fragment
containing the VZV gI-encoding region to make the plasmid pVZVgI. The
expression of the cloned genes was driven by the cytomegalovirus (CMV)
immediate-early promoter from the pCR3.1 vector. Subconfluent MDCK cell
monolayers in six-well cluster plates were transfected with pVZVgE or
pVZVgI or both, using the Lipofectin method. The transfected cells were
incubated for 48 h and then passaged to Falcon 3803 tissue culture
dishes in medium containing 250 mg of G418/ml. After selection for 14 days, surviving colonies were isolated using cloning rings. These
stably transfected cells were designated MDCK-gE, MDCK-gI, and
MDCK-gE/gI. Genomic DNA from MDCK-gE, MDCK-gI, and MDCK-gE/gI cells was
analyzed by PCR using primer pairs gEf and gEb
and gIf and gIb, respectively. G418-resistant
MDCK clones that had the expected 1.8-kb ORF68 DNA fragment from
MDCK-gE or MDCK-gE/gI and 1.1-kb ORF67 DNA fragment from MDCK-gI or
MDCK-gE/gI were expanded in the presence of G418, aliquoted, and stored
in liquid nitrogen. Protein expression of gE or gI was assessed by
Western blotting and immunofluorescence. Three positive clones of
MDCK-gE were obtained from screening 25 cell lines, and 15 clones of
MDCK-gE/gI were recovered from 30 screened cell lines. Three MDCK-gE
clones and three of the MDCK-gE/gI or MDCK cell lines were used at low
passage (<5) for all experiments. The mock transfection control and
gE- or gE/gI-expressing cells were grown at low density, trypsinized,
and plated onto Transwell filters in medium containing LC (5 µM).
Cells were incubated in LC medium for 4 h and then incubated in
DMEM-FCS containing normal (1.8 mM) calcium (NC). The cells from all
gE- or gE/gI-expressing clones could be maintained in NC-containing
medium for up to 5 days with no loss of viability. No differences in
viability compared to that of the parent MDCK clone II/G cells were
observed. For calcium switch experiments, the MDCK cells were grown at
low density and plated onto collagen-coated coverslips or Transwell
filters in LC medium for 4 h. Cells were then grown in NC medium
(calcium switch) or kept in LC medium up to 3 days. Protein kinase C
(PKC) agonist diC8 (1,2-dioctanylglycerol; Sigma, St. Louis, Mo.) at 0.5 mM and PKC inhibitor H7
(1-[5-isoquinolinylsulfonyl]-2-methylpiperazine; Sigma) at 50 µM
were added in some experiments.
Construction of plasmids.
The entire VZV genome of the Oka
strain is contained in four overlapping SuperCos 1 cosmid vectors:
pvFsp4 (1 to 33211), pvSpe5 (21875 to 62008), pvPme19 (53877 to 96188),
and pvSpe21 (94208 to 124884) (34). ORF67 spans VZV
nucleotides 114497 to 115558, while ORF68 extends from nucleotides
115808 to 117676, located within the unique short region in the cosmid
pvSpe21. A 6-kb DNA fragment from nucleotides 111911 to 117989 that
contained ORF67 and ORF68 was subcloned into the plasmid vector pBS to
generate pSac6A (35). The VZV gE open-reading-frame fragment
was amplified from pSac6A using primers gEf and
gEb (5'-ATGGGGACAGTTAA TAAACC-3' and
5'-CGGTGATCACCGGGTCTTATC-3'). The VZV gI open reading frame fragment was amplified from pSac6A using primers gIf and
gIb (5'-CGCGATGTTTTTAATCCAATG-3' and
5'-GTTCTATTTAACAAACGGG-3'). The PCR products were ligated into the pCR3.1 TA cloning vector, yielding the plasmids pVZVgE and pVZVgI.
Antibodies.
The antibodies used in these experiments
included affinity-purified rabbit anti-ZO-1 antibody (Zymed
Laboratories, Inc., South San Francisco, Calif.); rabbit polyclonal
anti-
-catenin, anti--catenin, mouse anti-gP135, and mouse
anti-E-cadherin antibody 3G8 (W. James Nelson, Stanford University,
Stanford, Calif.); mouse anti-VZV gE antibody 3B3 and anti-VZV gI
antibody 6B5 (Charles Grose, University of Iowa, Iowa City, Iowa);
mouse anti-VZV gE antibody 3G8 (Bagher Forghani, California Department
of Health Services, Berkeley, Calif.); Oregon Green 488-conjugated
phalloidin (Molecular Probes, Eugene, Oreg.); donkey anti-rabbit
antibody conjugated with horseradish peroxidase (Amersham, Little
Chalfont, Buckinghamshire, England); and affinity-purified fluorescein-
and Texas Red-labeled secondary antibodies (Jackson ImmunoResearch
Laboratories, Inc., West Grove, Pa.).
Cell extraction, immunoprecipitation, and Western blot
analysis.
MDCK cells were grown on Primaria tissue culture dishes
and extracted in 900 µl of cell lysis buffer (0.1% NP-40, 10 mM Tris [pH 7.5], 1-µg/ml DNase I, 1-µg/ml RNase A, and 1 mM
phenylmethylsulfonyl fluoride) on a rocker platform for 15 min at
4°C. Cells were scraped from the plates and centrifuged at
12,500 × g for 15 min at 4°C. Supernatants were
adjusted with 100 µl of sodium dodecyl sulfate (SDS)
immunoprecipitation buffer (1% SDS, 10 mM Tris [pH 7.5], 2 mM EDTA).
Protein samples were separated on an 8.5% Laemmli gel and
electrotransferred to a nitrocellulose membrane (Immobilon P;
Millipore, Bedford, Mass.). First, mouse monoclonal antibody at a
dilution of 1:2,000 was used as the probe and detected with donkey
anti-rabbit antibody conjugated with horseradish peroxidase (Amersham)
at a dilution of 1:4,000. For protein immunoprecipitation, cell lysates
were incubated with anti-gE (3B3) or anti-gI (6B5) antibody and immune
complexes were separated with protein A-Sepharose CL-4B (Amersham
Pharmacia Biotech, Uppsala, Sweden) on a rocker platform overnight at
4°C. After being washed four times with buffers, the
immunoprecipitates were analyzed on a 10% polyacrylamide gel and
processed for Western blotting as described above.
Immunofluorescence microscopy.
Confluent monolayers of MDCK
cells were grown on coverslips coated with rat tail collagen or
Transwell filters in DMEM-FCS. After 48 h, the cells were washed
with phosphate-buffered saline (PBS), fixed with 1% formaldehyde, and
permeabilized with 0.2% Triton X-100. Then they were blocked with
PBS-0.2% bovine serum albumin (BSA) containing 10% normal goat
serum. After a washing with PBS-0.2% BSA, they were incubated with
antibodies for 1 h at room temperature. After three washes with
PBS-0.2% BSA, the cells were incubated with secondary antibodies
(fluorescein isothiocyanate [FITC] anti-rabbit IgG and Texas Red
anti-mouse IgG). The coverslips were washed with PBS and mounted in
Vectashield (Vector Laboratory, Inc., Burlingame, Calif.). Cells were
examined with a Nikon fluorescence microscope using either a 40× lens
objective or a Molecular Dynamics MultiProbe 2010 laser scanning
confocal microscope. Fluorescence images of stained cells were recorded
using Kodak Ektachrome Elite II (ASA 400) films. Developed positive
images were then digitized with a slide scanner.
Time course of lipid diffusion in MDCK cells in low-density
cultures.
Cells were grown for 10, 23, and 47 h. At each
time, cells were labeled with the lipophilic carbocyanine tracer
CellTracker CM-DiI (Molecular Probes), a phospholipid probe, for 10 min
at 4°C. Cells stained with DiI were fixed and permeabilized. The cells were incubated with primary antibody ZO-1 and subsequently washed
with PBS-BSA before incubation with goat anti-rabbit IgG and
conjugation with FITC. Cells were examined with a confocal microscope.
TER measurement.
TER was determined by applying an
alternating square-wave current across a cell monolayer on a
12-mm-diameter Transwell filter (Costar, Corning, N.Y.) and measuring
the voltage deflection with the Millicell electrical resistance system
(Millipore). This device measures confluence quantitatively and
assesses cell health qualitatively. TER was measured in three or four
filters for all cell lines. TER values were calculated by subtracting
the blank values from the filter and the bathing medium and were
normalized to the area of the monolayer (filter). Monolayer integrity
was monitored after each TER time course study by staining cells with
Hoechst 33342 (Molecular Probes). When the control MDCK II/G clone is
triggered by calcium switch, TER during the first 24 h ranges from
100 to 250 
cm2 (28).
Freeze fracture electron microscopy.
Monolayers of cells
grown in 75-cm2 plastic tissue culture flasks were washed
briefly twice with 0.1 M PBS (pH 7.4) and fixed in 2% glutaraldehyde
(Ernest F. Fullam, Inc., Schenectady, N.Y.) in PBS for 30 min at room
temperature. After rinsing in PBS, cells were removed from the
substratum by using a plastic cell scraper (Nunc Inc., Naperville,
Ill.). The detached cells were infiltrated with 25% glycerol in 0.1 M
cacodylate buffer (pH 7.3), frozen in a liquid nitrogen slush, and
freeze fractured in a Balzers 400 freeze fracture unit (Balzers,
Liechtenstein). Replicas were cleaned in sodium hypochlorite, washed in
distilled water, placed on Formvar-coated grids, and examined with
a 301 electron microscope (Philips, Eindhoven, The Netherlands). In a
given replica, all TJ images were photographed. The number of TJ
parallel strands was counted on electron micrographs by overlaying the
area of the TJ with a transparency marked at 1-cm intervals. Since the magnification for all micrographs examined was 62,500×, counts were
effectively made at 160-nm intervals. Total TJ length examined by
morphometry in each group ranged from 6.4 to 9.4 µm. When the histograms were constructed for the strand frequency, the strand counts were normalized to the greatest total length measured. All
freeze fracture experiments were performed and analyzed as a
double-blind study.
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RESULTS |
Expression of VZV gE in MDCK-gE and VZV gEgI in MDCK-gE/gI
cells.
Three positive clones of MDCK-gE and MDCK-gE/gI along with
two MDCK control cell lines were tested for gE and gI expression. GP135, an actin-associated apical membrane protein in MDCK cells (41), was used as a housekeeping protein to assess the
loading of each sample (Fig. 1A). Western
blotting with anti-gE antibody yielded a 92-kDa protein from MDCK-gE or
MDCK-gE/gI cell lysates that was not present in MDCK cell lysates (Fig.
1B). Anti-gI antibody recognized a 55-kDa band in all three MDCK-gE/gI
clones tested (Fig. 1C). Clones were chosen for further analysis based
upon the consistency of gE/gI protein expression.
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FIG. 1.
Western blot analysis of constitutively gE- or
gE/gI-expressing cell lines. Two clones of MDCK control cells, three
clones of MDCK-gE-expressing cells, and three clones of
MDCK-gE/gI-expressing cells were grown on six-well cluster plates for
20 h and then extracted in lysis buffer. Proteins were separated
by SDS-8.5% polyacrylamide gel electrophoresis, transferred to
nitrocellulose membrane, and probed with anti-gP135 monoclonal antibody
(A) or anti-gI monoclonal antibody (C). The same cell lysates were
immunoprecipitated with anti-gE monoclonal antibody, separated by
SDS-10% polyacrylamide gel electrophoresis, transferred to
nitrocellulose membrane, and probed with anti-gE monoclonal antibody
(B).
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To determine the distribution of gE in MDCK-gE clones with or without
coexpression of gI, the cells were grown on filters
and probed with
anti-gE antibody 3G8. In addition to gE, the cellular
TJ plaque
protein, which is required for TJ integrity, was detected
with
anti-ZO-1 antibody (
27) and cells were stained for
E-cadherin,
which localizes primarily to the basolateral membrane in
confluent
MDCK cells (
8). Laser scanning confocal microscopy
of the clones
of MDCK-gE and MDCK-gE/gI cells revealed that most gE was
in intracellular
sites, as was expected from transient expression of gE
in other
systems. However, colocalization of gE with ZO-1 along cell
membranes
was observed (Fig.
2). Confocal
XZ sections also indicated colocalization
of some gE and ZO-1 in
MDCK-gE and MDCK-gE/gI cells (Fig.
2).
VZV gE did not appear to
colocalize with E-cadherin, which was
detected at the same lateral
membrane sites in confluent MDCK
cells with or without expression of gE
or gE/gI (data not shown).
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FIG. 2.
Immunofluorescence analysis of gE distribution in
MDCK-gE and MDCK-gE/gI cells. Clones of MDCK-gE- or
MDCK-gE/gI-expressing cells and the MDCK control cells were grown on
Transwell filters for 20 h and were fixed and permeabilized. The
cells were incubated with the primary antibodies, rabbit anti-ZO-1 or
murine anti-gE monoclonal antibody, before incubation with secondary
antibodies, goat anti-mouse IgG conjugated with Texas Red or goat
anti-rabbit IgG conjugated with FITC. Cells were examined by confocal
microscopy. ZO-1 expression; gE staining; and the overlay of ZO-1 and
gE staining, visualized by xy analysis of cell monolayers,
are shown. ZO-1 and gE expression were subjected to xz
analysis. Bar, 10 µm.
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Effects of VZV gE and gI on cell-cell contact and TJ
formation.
Calcium switch was used to investigate the effect of gE
and gI on MDCK cell-cell contact and TJ formation as detected by
confocal microscopy (21). E-cadherin belongs to a family of
Ca2+-dependent adhesion molecules. As the
E-cadherin-catenin complex mediates Ca2+-dependent
cell-cell adhesion, E-cadherin becomes localized to the basolateral
membranes of MDCK cells (10); removal of calcium makes
cadherins accessible to proteases and disrupts cell adhesion (52). As expected, MDCK cells in LC medium showed only
occasional staining with anti-ZO-1 antibody at sites of intercellular
contact, indicating that no triggering of cell adhesion and TJ
formation had occurred. In contrast, ZO-1 was detected in a continuous
pattern along the plasma membrane at several sites of intercellular
contact after 20 h of incubation of the clones of MDCK-gE or
MDCK-gE/gI cells in LC medium (Fig.
3A and B, middle panels; and Fig. 3A, right panel). NC conditions were not required to trigger partial TJ
formation by MDCK-gE or MDCK-gE/gI cells. With the "switch" of MDCK cells to NC medium, confluent monolayers were established. And
as expected, ZO-1 was detected in a reticular pattern, indicating the
translocation of TJ proteins to regions of cell-cell contact in all
cell lines. These data suggested that VZV gE has functions that promote
cell-cell contact and TJ formation in the absence of Ca2+
triggering of E-cadherins (Fig. 3A).
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FIG. 3.
The effects of VZV gE on cell-cell adhesion and TJ
formation. Clones of MDCK-gE and MDCK-gE/gI cells and MDCK controls
were grown on glass coverslips in LC or NC medium for 20 h. Cells
were fixed and permeabilized before incubation with rabbit anti-ZO-1
and FITC-conjugated anti-rabbit IgG and were examined by confocal
microscopy. (A) Membrane staining with ZO-1 is observed at cell
contacts between MDCK-gE and MDCK-gE/gI cells but not between MDCK
cells under LC conditions; MDCK cells under LC conditions have the
characteristic morphology of single cells prior to triggering of
monolayer formation by Ca2+. With the switch to NC medium,
all cell lines have the expected localization of ZO-1 to cell-cell
junctions. (B) diC8, a PKC agonist, permitted some localization of ZO-1
to cell membranes in MDCK cells under LC conditions, and ZO-1
localization in MDCK-gE-expressing cells became extensive; the PKC
inhibitor H7 partially blocked TJ formation between MDCK-gE cells,
resulting in a punctate pattern of ZO-1 under LC conditions. Arrows,
ZO-1 protein.
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Under NC conditions, E-cadherin binding of extracellular
Ca
2+ triggers the assembly of cell junctions and TJ sealing
in monolayers
of MDCK cells. Several pathways may be involved in these
processes,
including the PKC cascade, the calmodulin pathway, and the G
protein
signaling pathway (
5). To determine whether the
functional
effect of gE on induction of TJ formation was downstream of
the
PKC cascade, the PKC agonist diC8 or the PKC inhibitor H7 was
added
to cells in LC medium (
6). As expected, diC8 induced
partial
TJ formation between MDCK cells grown in LC in the control
experiments
(Fig.
3B, left panel). The PKC inhibitor H7 partially
blocked TJ
formation between MDCK-gE cells, resulting in a punctate
pattern of
ZO-1 under LC conditions (Fig.
3B, right panel, arrows).
The fact that
some TJ formation was maintained indicates that
gE functions as more
than just a PKC agonist and suggests that
there is an alternative
pathway for the enhancement of ZO-1 translocation
and TJ formation by
gE.
When control MDCK cells were triggered to form cell-cell contact by
Ca
2+-dependent, E-cadherin effects, ZO-1 was localized
almost exclusively
to sites of intercellular contact. ZO-1 showed its
usual very
limited expression on membranes that constituted the outer
margins
of MDCK cells at the edge of the monolayer (Fig.
4). Although
the difference could not be
quantitated, the consistent observation
for all clones of MDCK-gE or
MDCK-gE/gI cells was that ZO-1 could
be detected more commonly in cell
membranes along boundaries where
there were no adjacent cells than in
control MDCK cells. This
observation suggests that VZV gE and gE/gI may
have novel effects
on the distribution of the TJ protein ZO-1.
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FIG. 4.
Effect of expression of gE on ZO-1 and lipid diffusion
in low-density cells. MDCK, MDCK-gE, and MDCK-gE/gI cells were grown on
coverslips for 23 h. Cells were stained with DiI to identify
intracellular lipids, fixed, and permeabilized. The cells were
incubated with rabbit anti-ZO-1 before incubation with FITC-conjugated
goat anti-rabbit IgG. Cells were examined by confocal microscopy. Bar,
5 µm. Arrows: left panel, cell membranes; middle and right panels,
ZO-1 in cell membranes.
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VZV gE and gE/gI enhance the establishment of TER.
The gate
function of TJ, as distinguished from their barrier function, regulates
ion and solute diffusion through paracellular spaces (49).
The effects of gE and gI on TJ gate function were measured by TER, a
test of ion diffusion. The establishment of TER by MDCK-gE, MDCK-gI,
MDCK-gE/gI, and MDCK cells was compared at intervals over a 54-h period
under LC or NC conditions (Fig. 5). Under
LC conditions, TER remained very low in the clones of MDCK-gE as well
as in MDCK cells; failure to establish TJ gate function was consistent
with the discontinuous ZO-1 staining observed in MDCK-gE and gE/gI
cells grown in LC medium (Fig. 3). After a switch to NC medium, the TER
of MDCK-gE cell monolayers reached a very high resistance of 420 cm2 by 20 h (Fig. 5); MDCK cells expressing gE/gI or
gI alone also developed high TER in a short time. For MDCK-gE,
MDCK-gE/gI, and MDCK-gI cells, resistance was sustained at much higher
levels than in MDCK cells for up to 30 h; for MDCK-gE clones, it
remained above TER for MDCK cells at the last time point of 54 h.
MDCK cells expressing gE/gI reached a high maximum TER after
approximately 10 h, although the maximum resistance was somewhat
lower than that observed in MDCK-gE cell monolayers. To exclude the
possibility that the process for generating G418 selected MDCK clones
altered the characteristic TER of the parent MDCK II/G clone, cells
selected for retention of pTRE, a plasmid that does not express VZV
proteins (MDCK-TRE), were tested; both control MDCK cells and the
clones of MDCK-TRE showed the expected TER during the first 48 h
after calcium switch, ranging from 100 to 250 cm2 (data
not shown). These data suggested that TJ gate function was enhanced in
the presence of gE, gE/gI, or gI at early times after cellular
confluence was established. Although TER remained significantly higher
than in control MDCK cells, interactions between gE and gI appear to
modulate the effect of gE alone on TJ gate function in MDCK-gE/gI
cells. Based on the acceleration of endocytosis when both gE and gI are
present (1, 43), this difference may reflect an increased
return of gE from TJ sites to endosomes or to the TGN in
gE/gI-expressing cells.
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FIG. 5.
Development of TER in MDCK cells constitutively
expressing VZV gE, gI, or gE/gI. The kinetics of TER was measured
sequentially over 54 h in clones of VZV gE-, gI-, or
gE/gI-expressing MDCK cells, tested from the time of calcium switch, at
time zero to NC conditions. The y axis indicates TER, and
the x axis indicates the time (hour) at which TER was
measured. TER measurements are given for MDCK, MDCK-gE, MDCK-gI, and
MDCK-gE/gI cell lines in NC medium; measurements were also made
with MDCK (MDCK.LC) and MDCK-gE (MDCK-gE.LC) cell lines in LC medium.
The data are reported as the means ± standard deviations for
three assays. At the end of each experiment, filters were fixed and
stained with Hoechst 33342 to confirm the integrity of the monolayer.
|
|
Effect of VZV gE expression on TJ strand organization.
In
freeze fracture replicas of MDCK-gE cells, the TJ formed a network of
interconnected parallel strands present near the apex of the lateral
membranes (Fig. 6, lower panel). Its
appearance was similar to that in control MDCK cells (Fig. 6, upper
panel) (50, 51). These data suggest that the presence of gE
near TJ sites or its possible interactions with TJ proteins, such as ZO-1, did not affect TJ strand organization.
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|
FIG. 6.
Freeze fracture electron microscopy of TJ strand
organization in MDCK cells expressing VZV gE. The lower panel shows a
freeze fracture replica of an MDCK cell stably transfected with gE,
demonstrating an exoplasmic fracture face of a representative TJ. The
upper panel shows an exoplasmic fracture face of a representative TJ in
a nontransfected control MDCK cell. The appearance of the TJ is similar
in both cells. Magnification, ×62,500.
|
|
Effects of gE and gI on cell morphology, cytoskeletal proteins, and
cellular lipids.
MDCK-gE and MDCK-gE/gI cells were consistently
larger than the nontransfected controls (Fig. 2). The average number of
MDCK cells per microscopic field was 70, compared to 34 for MDCK-gE cells and 32 for MDCK-gE/gI cells. In order to assess whether this
difference in morphology was associated with changes in the distribution of cytoskeletal proteins, the cells were stained with
Oregon Green phalloidin, a dye specific for F-actin, and evaluated by
confocal fluorescence imaging (Fig.
7). The organization of F-actin filaments
in MDCK-gE, MDCK-gE/gI, or MDCK cells was scanned in apical to
basolateral sections. MDCK-gE cells appeared to be flattened on the
substratum compared with MDCK cells, based on the xz images
(Fig. 7). In contrast to MDCK cells, in which F-actin fibers were lined
up in the normal pattern next to cell-cell contacts, F-actin in MDCK-gE
cells was localized predominantly in stress fibers at the basolateral
regions of the cells and in thick cortical bundles at the periphery.
The cytoplasmic region of E-cadherin is anchored to cytoskeletal actin
microfilaments through catenins (46). To investigate whether
gE might disturb F-actin organization by an interaction with catenins,
MDCK-gE cells were examined for colocalization of gE with -catenin
and -catenin by confocal microscopy. VZV gE did not appear to
colocalize with catenin proteins, indicating that gE may alter F-actin
distribution by an indirect pathway (data not shown). F-actin
organization was similar in MDCK-gE/gI cells and MDCK cells, suggesting
that gI binding to gE diminished the disruption of cytoskeletal protein organization induced by gE.
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FIG. 7.
Effect of expression of gE on cell morphology and
F-actin filament distribution. After 24 h of incubation in NC
medium, MDCK, MDCK-gE, and MDCK-gE/gI cells were fixed, labeled with
0.165 µM phalloidin, and examined by confocal microscopy. The panels
show staining when cell monolayers were examined as xy
sections, showing the pattern detected at the apical (AP) level (upper
row) and the basolateral (BL) level (lower row). Arrow, actin stress
fibers; arrowhead, actin in thick cortical bundles. Bar, 5 µm. Narrow
panels at bottom show xz sections of cell monolayers.
|
|
Cellular lipids were stained with CM-DiI and anti-ZO-1 antibody (Fig.
4). At 10 h, staining by CM-DiI was extensive in plasma
membranes
of all cell lines (data not shown). By 23 h, lipid staining
remained somewhat more predominant in the plasma membrane of MDCK-gE
cells than in MDCK cells. The pattern of lipid localization in
MDCK-gE/gI cells was similar to that observed in MDCK cells; in
both
cases, lipids were shown to be evenly distributed throughout
the
cytoplasm (Fig.
4).
Sequence homologies with cadherins and MDCK desmocollin.
Computer-assisted amino acid similarity searches (CLUSTALW and
Swissprot BestFit) were used to determine relationships between VZV gE
and HSV-1 gE and the cell adhesion molecules E-cadherin and MDCK
desmocollin (9, 13). The multiple-amino-acid sequence alignment by CLUSTALW and Swissprot BestFit indicated that the extracellular segments of VZV gE, E-cadherin, and desmocollin were
similar in size and that these segments had regions of similarity and
identity not found in comparing their cytoplasmic components. Two
regions of the VZV gE ectodomain, amino acids 278 to 330 and 467 to
498, were shown to have high degrees of similarity (43.4 and 37.5%)
and identity (22.6 and 19%) with regions of the cell adhesion
molecules E-cadherin and desmocollin. In contrast, HSV-1 gE amino acids
198 to 256 and 403 to 444 had similarities of 25.0 and 11.9% and
identities of 10.7 and 4.8% (Fig. 8).
The Genetics Computer Group (GCG) GAP program was used to evaluate the
significance of the alignment. This program generated the average
alignment score ± standard deviation, based on repeated
randomized alignments, and this average quality score was compared to
the quality score of the actual alignment. VZV gE amino acids 278 to
330 had a significantly higher quality score than E-cadherin by this
test (30 versus 15.4 ± 5.6). We speculate that the gE 278-to-330
amino acid sequence might be a functional domain of VZV gE that
enhances cell-cell contact, which we observed as partial TJ formation
under LC conditions and enhanced maximum TER in gE- and
gE/gI-expressing MDCK cells. VZV gE, consistent with a capacity to
enhance cell-cell contacts under LC conditions (45), has
none of the calcium binding motifs PENE, LDRE, DQNDN, and DAD,
which are common in cell adhesion molecules (Fig. 8).
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FIG. 8.
Comparisons of amino acid sequences of VZV gE
ectodomains and HSV-1 gE extracellular region with those of cell
adhesion molecules E-cadherin and MDCK desmocollin. Sequences were
compared by CLUSTALW multiple-sequence alignment using the DeCypher
bioinformatics supercomputer (Center for Molecular and Genetic
Medicine, Stanford University). Two domains from the extracellular
region of VZV gE and HSV-1 gE were compared to regions of the
ectodomains of E-cadherin and MDCK desmocollin. Symbols: *, amino
acid conserved among three proteins; :, amino acid conserved between gE
and one of the adhesion proteins; -, gap that was introduced to
maintain maximal alignment. Underlined amino acids correspond to the
calcium binding motif.
|
|
| |
DISCUSSION |
This investigation of gE and gI expression in MDCK cells provides
initial information about how these VZV proteins may affect the
structure and function of polarized epithelial cells. VZV gE expression
was associated with the translocation of the TJ protein ZO-1 to cell
membranes under LC conditions, whether expressed with or without gI.
This effect of gE and gE/gI on the formation of MDCK cell-cell contacts
was Ca2+ independent, in contrast to the requirement for
Ca2+ when it is mediated by E-cadherin. While most VZV gE
was intracellular in its distribution, evidence of gE colocalization
with the TJ protein ZO-1 with or without concomitant expression of gI
was suggested by confocal microscopy. In contrast, the homologous HSV
gE protein localized with -catenin and the glycoprotein encoded by
Us9 in the human CMV short unique region were found with E-cadherin when expressed in epithelial cells (15, 16, 33, 34).
Experiments assessing TJ gate function demonstrated that VZV gE, gI,
and gE/gI expression also accelerated the kinetics of induction and
maximum TER in MDCK cells.
Epithelial cell junction proteins move from the ER to form complexes at
the plasma membrane that include occludin, ZO-1, ZO-2, cadherins, and
catenins (8, 22, 26, 27, 39). When epithelial cells are
plated at confluence in calcium-sufficient medium, they adhere to the
substrate and form E-cadherin-rich adherens junctions, while occludin
and ZO-1 localize to the subapical sites on lateral membranes, forming
TJ. As the most apical segment of the intercellular junctions within an
epithelial layer, TJ form a regulated seal that restricts paracellular
diffusion of ions and solutes and intramembrane diffusion of lipids
(21, 32). The E-cadherin-catenin complex is a
Ca2+-regulated cell-cell adhesion complex; E-cadherin
transport from the ER to lateral membranes is mediated by -catenin
binding to its cytoplasmic domain (10), and catenins anchor
E-cadherin to the cytoskeletal protein F-actin (46). ZO-1
mRNA transcription in MDCK cells is also regulated by calcium
(22). We found that VZV gE enhanced ZO-1 translocation to
cell membranes in the absence of Ca2+ triggering, which was
observed as partial TJ formation when MDCK-gE cells were tested in
calcium switch experiments performed at low cell density. This effect
on ZO-1 was maintained when gE was expressed in the presence of gI. The
mechanisms by which gE may affect ZO-1 trafficking under LC conditions
remain to be determined. Whether gE functions as a PKC agonist like
diC8 to facilitate the translocation of ZO-1 or is directly involved in
TJ formation, or both, is not certain. Some additional evidence that
VZV gE or gE/gI may alter ZO-1 trafficking was provided by the tendency
of this TJ protein to appear on cell membranes at the free margin of
the monolayer after the calcium switch, while it was rarely found in
confluent monolayers of control MDCK cells.
The induction of membrane adhesion between gE- or gE/gI-expressing MDCK
cells incubated at low density and under LC conditions suggests that
VZV gE may have the capacity to function as a
Ca2+-independent adhesion protein to enhance cell-cell
contact. Since gE has a large extracellular domain like E-cadherin, one
hypothesis is that gE may bind to a cell membrane ligand on uninfected
cells in proximity to the infected cell, which could assist viral
transport from infected cells. Alternatively or in addition, gE could
contribute to the fusion of neighboring cells that were infected
independently, since it forms homodimers as well as heterodimers with
gI (31, 42); this mechanism would mimic dimer formation by
the extracellular domains of E-cadherin (57). Residues 278 to 330 and 467 to 498 in the ectodomain of gE have identities of 22.6 and 18.8% and similarities of 43.4 and 37.5%, respectively, with the
corresponding regions of E-cadherin and the MDCK cell adhesion protein
desmocollin, but predicted Ca2+ binding residues are absent
in VZV gE. These similarities between the amino acid sequences of
extracellular segments of gE and cell adhesion molecules are only
suggestive; whether they actually represent functional domains of gE
will require analysis in mutagenesis experiments. However, this
possibility is of interest because VZV gE is a substantially larger
molecule than its counterparts in other herpesviruses, and its
multifunctional nature is becoming well documented (1, 12,
43).
The change in kinetics of induction and peak TER in MDCK cells was a
notable and reproducible effect of VZV gE, gI, or gE/gI expression.
Although the claudins and occludin are known to be the critical
molecules, how they are arranged to form TJ strands is not clear; the
molecular mechanisms that account for the gate functions of TJ remain
unresolved, but the regulation of paracellular solute transport is an
active process that continues after TJ formation (54).
Similar effects on TER were reported with overexpression of occludin or
a COOH-terminal truncation of occludin in MDCK cells (7).
However, it is not likely that gE or gI has any direct occludin-like
functions, since gE and gI are type I transmembrane proteins. By
contrast, occludin and the 18 known claudins are all tetraspan integral
membrane proteins with both N and C termini in the cytoplasm
(49). Extracellular domains of occludin are unique in that
they have unusually high tyrosine and glycine content (37).
The unusual TER kinetics in MDCK cells expressing gE, gE/gI, or gI is
intriguing and indicates that viral proteins may affect TJ regulation
of paracellular ion diffusion, but specific pathways cannot be
suggested from current information.
In contrast to VZV, HSV-1 gE and gI accumulated at lateral membranes
and colocalized with -catenin in endometrial epithelial (HEC-1A)
cells and MDCK cells (17). The human CMV glycoprotein Us9
colocalized with E-cadherin in a basolateral distribution and with
F-actin (33). Other differences were that VZV gE trafficked to cell membranes with or without gI in MDCK cells, albeit in limited
amounts relative to intracellular concentrations, whereas HSV gE
required gI for its translocation to plasma membranes and no
colocalization of HSV proteins with ZO-1 was observed. While these
various patterns suggest virologic differences, interpretations must be
tempered by the fact that these experiments were done using different
expression systems and different cellular substrates. Although the
effects of VZV gE on ZO-1 localization and TER could be observed in the
absence of gI, their occurrence in the presence of gI is important if a
functional role in virus-infected cells is to be considered, because gE
typically forms heterodimers with gI during VZV replication.
Dingwell and Johnson have suggested that targeting of certain
herpesvirus glycoproteins to regions of epithelial cell contact and
their interaction with cell junction proteins facilitate the movement
of virions into uninfected cells by creating membrane fusion or enable
virion release into intercellular spaces, followed by fusion of the
viral envelope to the uninfected cell membrane (17). A
second hypothesis, which was suggested for human CMV Us9, is that the
viral glycoproteins destabilize the cellular proteins that constitute
adherens junction complexes, enhancing access to adjacent cells in
epithelial tissues by disruption of basolateral membranes
(33). We showed that VZV gE and gE/gI complexes did not
disturb TJ gate function, as measured by TER. TJ gate function was also
preserved in epithelial cells expressing HSV-1 gE and gI
(17). Our experiments further demonstrated that TJ strands
were structurally intact by freeze fracture electron microscopy. Thus,
the evidence is that neither VZV nor HSV-1 gE or gE/gI complexes
disrupt the plasma membrane contacts that are generated by cellular
proteins. Our experiments indicate that VZV gE and gE/gI actively
promoted adhesion of epithelial cell membranes and the establishment of
TJ gate function. Although ZO-1 is at the apex of the lateral membrane
and -catenins move to lateral membrane segments below the TJ when
MDCK cells are confluent, trafficking of particular herpesvirus
glycoproteins to either of these sites could fit the functional model
that gE and gI enhance membrane fusion or local release of virions into intercellular spaces next to uninfected cells, as illustrated by
Dingwell and Johnson (17). The small-plaque phenotype
observed with deletion of VZV gI (11, 35) or with HSV-1 and
PRV gE and gE/gI deletion mutants (3, 17, 29, 30) could
occur if either fusion or release was impaired. In addition to having pathogenic effects on epithelial cells, the alphaherpesviruses are
neurotropic and neuronal cells are also polarized (48). Studies of HSV and PRV gE mutants or mutants that block the formation of gE/gI heterodimers demonstrate that gE and the gE/gI complex make a
critical contribution to central nervous system spread in animal
models, and recent PRV experiments demonstrate that this effect is
independent of the gE endocytosis motif (3, 4, 16, 29, 30, 53,
56).
In cellular adherens junctions, cadherins and actin filaments are
aligned in bundles with the plasma membrane (38, 52). Viral
pathogens, especially poxviruses, have been shown to manipulate cellular cytoskeletal components during replication (14). In contrast to human CMV Us9 protein, VZV gE did not colocalize with E-cadherin or F-actin (33). Nevertheless, VZV gE expression appeared to disrupt the prominent bundles of actin filaments that encircle the lateral membranes in association with adherens junctions and induced the formation of "stress" fibers. Since actin fibers are anchored to cadherins by catenins, gE expression appears to disrupt
this complex along the lateral membrane (47). Of note, these
changes in actin were independent effects in gE-expressing cells and
were not associated with any altered ZO-1 localization, TJ gate
function as measured by TER, or TJ structure as visualized by freeze
fracture electron microscopy. These marked changes in the cellular
cytoskeleton may explain why it has been difficult to generate and
maintain VZV gE-expressing cell lines. The yield of MDCK gE-expressing
clones was much lower than that of MDCK-gE/gI clones in our
experiments. Although gI is dispensable for VZV replication in Vero and
melanoma cells, its deletion resulted in a significant decrease in
infectious-virus yields, which may reflect the toxic effects of gE on
cells when it is not modulated by binding to gI (11, 35). In
contrast, the MDCK-gE/gI clones exhibited morphology, F-actin
organization, and lipid distribution patterns like those of control
MDCK cells. Thus, our experiments suggest that under the normal
conditions of VZV infection in which both gE and gI are expressed,
their synthesis and intracellular trafficking are associated with
preservation rather than with disorganization of the links between
membrane cadherins and the actin cytoskeleton in epithelial cells.
Cell-cell spread of VZV is associated with the formation of distinctive
"viral highways" that disappear when gI is deleted (18,
35). Maintaining membrane and/or cytoskeletal connections through
dual expression of gE and gI might be important during the early stages
of VZV infection.
This analysis of VZV gE and gI in MDCK cells adds to the accumulating
evidence that some herpesvirus glycoproteins may function to enhance
contacts between epithelial cells and suggests that these viral
proteins have the capacity to facilitate cell adhesion by pathways
distinct from those of the Ca2+-dependent
E-cadherin-like molecules.
| |
ACKNOWLEDGMENTS |
We are grateful to our colleagues who provided necessary
reagents and valuable advice, including W. James Nelson, Stanford University; Charles Grose, University of Iowa; and Bagher Forghani, California Department of Health Services. We thank members of the
Nelson and Arvin laboratories for their helpful discussions and
criticisms and Lee Kozar of the Bioinformatics Resource at Stanford
University Medical Center for sequence alignment analysis. We thank Jay
Lee for excellent technical assistance.
This work was supported by Public Health Service grant AI20459 to
A.M.A. C.M. is the recipient of a postdoctoral fellowship from the
VZV Research Foundation.
| |
FOOTNOTES |
*
Corresponding author. Mailing address: G-312, Stanford
University School of Medicine, 300 Pasteur Dr., Stanford, CA 94305. Phone: (650) 725-6555. Fax: (650) 725-8040. E-mail:
cmo{at}cmgm.stanford.edu.
| |
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Journal of Virology, December 2000, p. 11377-11387, Vol. 74, No. 23
0022-538X/00/$04.00+0
Copyright © 2000, American Society for Microbiology. All rights reserved.
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Abstract
Introduction
