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Journal of Virology, May 2001, p. 4878-4888, Vol. 75, No. 10
Centre for Virus Research, Westmead
Millennium Institute of Health Research, University of Sydney, Sydney,
New South Wales, Australia1; Departments
of Pediatrics and Microbiology & Immunology, Stanford University School
of Medicine, Stanford, California2; and
Department of Pathology, Harvard Medical School, Boston,
Massachusetts3
Received 14 July 2000/Accepted 15 February 2001
We sought to examine the effects of varicella-zoster virus (VZV)
infection on the expression of major histocompatibility complex class I
(MHC I) molecules by human fibroblasts and T lymphocytes. By flow
cytometry, VZV infection reduced the cell surface expression of MHC I
molecules on fibroblasts significantly, yet the expression of
transferrin receptor was not affected. Importantly, when human fetal
thymus/liver implants in SCID-hu mice were inoculated with VZV, cell
surface MHC I expression was downregulated specifically on VZV-infected
human CD3+ T lymphocytes, a prominent target that sustains
VZV viremia. The stage in the MHC I assembly process that was disrupted
by VZV in fibroblasts was examined in pulse-chase and
immunoprecipitation experiments in the presence of endoglycosidase H. MHC I complexes continued to be assembled in VZV-infected cells and
were not retained in the endoplasmic reticulum. In contrast,
immunofluorescence and confocal microscopy showed that VZV infection
resulted in an accumulation of MHC I molecules which colocalized to the
Golgi compartment. Inhibition of late viral gene expression by
treatment of infected fibroblasts with phosphonoacetic acid did not
influence the modulation of MHC I expression, nor did transfection of
cells with plasmids expressing immediate early viral proteins. However, cells transfected with a plasmid carrying the early gene
ORF66 did result in a significant downregulation of MHC I
expression, suggesting that this gene encodes a protein with an
immunomodulatory function. Thus, VZV downregulates MHC I expression by
impairing the transport of MHC I molecules from the Golgi compartment
to the cell surface; this effect may enable the virus to evade
CD8+ T-cell immune recognition during VZV pathogenesis,
including the critical phase of T-lymphocyte-associated viremia.
Varicella-zoster virus (VZV) is a
human herpesvirus that causes varicella (chicken pox) as the primary
infection in susceptible individuals, establishes latency in sensory
nerve ganglia, and may reactivate as herpes zoster (shingles) (5,
6, 14). In healthy individuals, primary VZV infection induces
both innate and antigen-specific immune responses. Innate immunity may
limit the initial spread of VZV within the host, but VZV-specific
adaptive immunity plays a crucial role in recovery from varicella and
in the preservation of latency. Modulation of major histocompatibility complex class I (MHC I) expression may promote viral infection and
persistence in the host by enabling infected cells to evade the
CD8+ T-lymphocyte-mediated antiviral immune response. In
this respect, several viruses, including adenovirus, human
immmunodeficiency virus (HIV), murine and human cytomegalovirus (MCMV
and HCMV, respectively), Epstein-Barr virus, bovine herpesvirus,
pseudorabies virus, and herpes simplex virus (HSV), as well as VZV,
have been found to downregulate cell surface MHC I expression
(10, 15, 28, 29, 30, 31, 35, 42, 47, 49, 51). These
viruses have evolved various strategies for disrupting the MHC I
antigen presentation pathway, and some have been shown to coordinate
multiple mechanisms of interference (reviewed in references 19 and 44).
MHC I molecules are heterodimers consisting of a membrane-bound heavy
chain ( During primary VZV infection, both MHC I-restricted, CD8+ T
lymphocytes and MHC II-restricted, CD4+ T lymphocytes are
sensitized to VZV antigens (46). T-cell recognition of
infected cells is essential for terminating primary infection (7). Interestingly, VZV appears to evade host recognition
by T lymphocytes during a prolonged, 10- to 21-day incubation period following initial infection (6). Viral genes encoding
immunomodulatory proteins may allow VZV to escape immune surveillance
during this interval, permitting the virus to move from mucosal sites
of inoculation and to disseminate to skin via T lymphocytes.
The purpose of this study was to examine the effect of VZV infection on
cell surface expression of MHC I molecules by human fibroblasts and T
lymphocytes. We used flow cytometry to demonstrate that VZV reduced
cell surface MHC I expression on infected human fibroblasts and T
lymphocytes. We applied a combination of biochemical analyses and
confocal microscopy to show that VZV interferes with the transport of
MHC I molecules from the Golgi compartment to the cell surface.
Phosphonoacetic acid (PAA), an inhibitor of late viral gene synthesis,
did not alter the ability of the virus to downregulate MHC I
expression, suggesting that this function is not encoded by a late
viral gene product(s). Cells transfected with plasmids expressing
immediate early (IE) genes were not altered in the ability to express
MHC I molecules, but a plasmid carrying the early gene ORF66
did significantly downregulate MHC I expression on transfected cells.
Cells.
The following cell lines were grown in tissue culture
medium (TCM) (Dulbecco's modified Eagle's medium; Gibco,
Gaithersburg, Md.) supplemented with heat-inactivated fetal calf serum,
2 mM L-glutamine (Gibco), 50 IU of penicillin, 50 mg of
streptomycin (Pen/Strep; ICN Biomedicals, Inc., Irvine, Calif.), and
0.5 mg of amphotericin B (Fungizone, Flow Laboratories, McLean, Va.): human fetal lung fibroblasts, MRC-5 (ATCC CCL 171), in passages 17 to
30; human foreskin fibroblasts (HFFs), in passages 5 to 25; human
melanoma (MeWo) cells; and Vero (African green monkey) cells.
Antibodies.
The monoclonal antibodies (MAbs) used were
specific for human MHC I (clone Tu149 recognizing complexed
SCID-hu mice.
Male homozygous C.B-17 scid/scid
mice were bred and maintained at SyStemix, Inc., Palo Alto, Calif. At 8 weeks of age, coimplants of human fetal thymus and liver (thymus/liver)
tissue from 18- to 23-week fetuses were introduced under the kidney
capsule as a cojoint implant (41). Human fetal tissues
were obtained with informed consent according to federal and state
regulations and were screened for HIV. The general care of these
animals was done in accordance with the guidelines of the
Administrative Panel on Laboratory Animal Care of Stanford University.
Viruses.
The VZV strain used in these studies was a
low-passage clinical isolate designated strain Schenke. For cell
infections, fibroblasts or melanoma cells were mixed with VZV-infected
cells (3+ to 4+ cytopathic effect), at a ratio of one infected cell to
five uninfected cells. Animal inoculations were done with VZV-infected
MRC-5 cells at 3+ to 4+ cytopathic effect. The VZV-infected monolayers
were trypsinized and washed once with phosphate-buffered saline (PBS), and the cells were counted and resuspended in TCM. Cells were briefly
stored on ice until they were injected into the SCID-hu thymus/liver
implants. Mock-infected implants were injected with an equal number of
uninfected MRC-5 cells prepared by the same method. The virus inoculum
was determined by plaque assay on Vero cell monolayers. The Oka vaccine
strain and a glycoprotein C (gC)-negative mutant of the Oka strain
were also tested for effects on MHC I expression (39).
Infection of thymus/liver implants.
Mice were anesthetized
by intraperitoneal injection with a solution of 5% ketamine (Aveco
Co., Fort Dodge, Iowa) and 2.5% xylazine (LyphoMed Inc., Rosemont,
Ill.) in PBS. The left kidney was surgically exposed, and the
thymus/liver implant was injected using a 27-gauge needle with
approximately 20 to 50 µl of cells. The peritoneal incision was
sutured, and the skin was stapled closed. Seven days after inoculation
the implants were removed and disrupted between ground glass slides.
Cell suspensions were filtered through a sterile nylon mesh to remove
large debris, and the released cells were washed, counted, and used for
fluorescence-activated cell sorting (FACS) analysis and virus titration.
FACS analysis.
Aliquots of approximately 106
cells obtained from uninfected and VZV-infected thymus/liver implants,
uninfected and VZV-infected MRC-5 cells, and HFF or MeWo cells or
transfected HFF cells were washed and resuspended in 100 µl of FACS
staining buffer (PBS with 1% fetal calf serum and 0.2% sodium azide).
The primary antibodies, VZV-immune or nonimmune polyclonal IgG, were
diluted 1:40. Secondary mouse MAbs anti-MHC I, anti-CD71, anti-CD3,
anti-CD4, anti-CD8, and anti-CD45 were diluted 1:50 with goat
anti-human FITC-conjugated F(ab')2 fragments (diluted
1:100). As a negative control cells were incubated with the appropriate
isotype control antibodies. All antisera were diluted in FACS staining
buffer, and all reactions were done in the dark on ice for 30 min. The
cells were washed between each antibody step by adding 2 ml of FACS
staining buffer, centrifuging, and aspirating the supernatant. After
the final wash cells were resuspended in orthofixative (PBS with 1%
electron microscopy grade formaldehyde), and cell suspensions were
analyzed with a Becton Dickinson FACScan apparatus.
Immunofluorescence and confocal microscopy.
Approximately
104 cells per well were seeded in four-chamber slides
(Lab-Tek, Inc., Naperville, Ill.). Adherent cells were infected with
VZV strain Schenke at a ratio of one infected cell to three uninfected
cells for 2 h at 37°C. The infected monolayers were washed three
times with PBS and incubated with TCM for 24 h. In certain
experiments, cells were fixed and permeabilized with acetone at 4°C
for 15 min and air dried for 1 h. Slides were washed once in PBS
and incubated with blocking buffer (1% bovine serum albumin [BSA] in
PBS) at room temperature for 15 min, washed three times with PBS, and
incubated with the primary antibodies diluted in blocking buffer for
1 h at 37°C. The primary antibodies used were mouse anti-human
HLA-A,B,C (PharMingen) and a VZV-immune polyclonal IgG fraction, at a
dilution of 1:10 and 1:100, respectively. An isotype control antibody
was used to control for nonspecific binding. Slides were washed three
times in the blocking solution, and the secondary antibodies were added
for 30 min in the dark at 37°C. Secondary antibodies included Texas
red-conjugated goat anti-human IgG (Jackson ImmunoResearch
Laboratories, West Grove, Pa.) (1:100) and FITC-conjugated goat
anti-mouse IgG (CalTag Laboratories) (1:100) diluted in blocking
solution. After three washes in PBS, slides were mounted with
Vectashield (Vector Laboratories, Inc., Burlingame, Calif.) and
examined using a Molecular Dynamics MultiProbe 2010 laser scanning
confocal microscope. The images were transferred to graphics software
(Adobe Photoshop, version 3.0) and printed with a Tektronix Phaser 440 dye sublimation printer.
0022-538X/01/$04.00+0 DOI: 10.1128/JVI.75.10.4878-4888.2001
Copyright © 2001, American Society for Microbiology. All rights reserved.
Varicella-Zoster Virus Retains Major
Histocompatibility Complex Class I Proteins in the Golgi Compartment of
Infected Cells
ABSTRACT
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Abstract
Introduction
Materials and Methods
Results
Discussion
References
INTRODUCTION
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Abstract
Introduction
Materials and Methods
Results
Discussion
References
C) and a light chain 
2 microglobulin
(2m) which present peptides derived from cytosolic
proteins to CD8+ T lymphocytes. Antigenic peptides
generated by cytosolic proteases are transported into the endoplasmic
reticulum (ER) by the ATP-dependent transporter associated with antigen
processing (TAP), where they associate with MHC I heterodimers. The
resulting trimolecular complex is transported from the ER through the
Golgi compartment to the cell surface where it presents the peptide to
cytotoxic T lymphocytes (34). Each step in the MHC I
biosynthesis and assembly pathway has been shown to be a potential
target for viral interference and the subsequent modulation of MHC I
expression on cell surfaces.
MATERIALS AND METHODS
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Abstract
Introduction
Materials and Methods
Results
Discussion
References
C/2m) (purified and R-phycoerythrin [PE]
conjugated); human transferrin receptor (CD71; clone T56/14) (purified
and PE conjugated); human CD3 (clone S4.1; tricolor conjugated); human
CD4 (clone S3.5; PE conjugated); human CD8 (clone 3B5; fluorescein
isothiocyanate [FITC] conjugated); goat anti-mouse immunoglobulin G
(IgG) F(ab')2 fragments, PE-conjugated goat anti-human IgG,
and FITC-conjugated goat anti-human IgG (CalTag Laboratories, South San
Francisco, Calif.); and human HLA-A,B,C (clone G46-2.6) and human
transferrin receptor (clone M-A712) (Pharmingen, San Diego, Calif.).
MAb W6/32 and rabbit antiserum specific for the human MHC I heavy chain
were provided by H. Ploegh (Harvard University, Boston, Mass.) and were
used in immunoprecipitation experiments. VZV-immune or nonimmune
polyclonal human serum (IgG purified) was used to identify VZV-infected cells.
Biochemical analysis and gel electrophoresis. Cells were incubated for 45 min in methionine- and cysteine-free TCM and labeled with [35S]methionine-cysteine (NEN, Boston, Mass.) for 30 min for pulse-chase experiments and for 1 h for coimmunoprecipitation experiments. If indicated, cells were chased for various times in regular TCM supplemented with nonradioactive methionine and cysteine to a final concentration of 1 mM. Aliquots of cells were spun down at each chase point, and the cell pellets were frozen before lysis and immunoprecipitation. Cell pellets were lysed in NP-40 lysis buffer (0.5% NP-40, 50 mM Tris-HCl [pH 7.4], 5 mM MgCl2) containing 1 mM phenylmethylsulfonyl fluoride for 15 min on ice. Total cell lysates were cleared of debris by centrifugation, and supernatants were precleared twice with protein A (70 µl), 3 µl of normal rabbit serum/ml, and 3 µl of normal mouse serum/ml and then immunoprecipitated with either W6/32 (3 µl/ml) or rabbit anti-MHC I heavy chain (3 µl/ml). Immunoprecipitated products were washed four times with ice-cold NET buffer (0.5% NP-40, 50 mM Tris [pH 7.4], 150 mM NaCl, 5 mM EDTA). Samples were boiled in sample buffer (62.5 mM Tris-HCl [pH 6.8], 5% 2-mercaptoethanol, 10% glycerol, 4% sodium dodecyl sulfate [SDS], and bromophenol blue) for 10 min before SDS-polyacrylamide gel electrophoresis (PAGE). In those experiments in which endoglycosidase H (endo H; New England Biolabs, Beverly, Mass.) was used, washed protein A-bound immune complexes were processed as follows. Immune complexes were boiled for 10 min in 30 µl of denaturation buffer (0.5% SDS, 1% 2-mercaptoethanol) and then incubated with endo H (1 µl) in 50 mM sodium citrate (pH 5.5) at 37°C for 1 h. Samples were then mixed in sample buffer and boiled for 10 min before SDS-PAGE. Samples were separated on SDS-12.5% PAGE gels, fixed, and washed prior to drying and autoradiography. Unlabeled samples prepared for coimmunoprecipitation experiments were prepared as described above, with the gel being Coomassie stained to reveal total protein before excision of the protein band of interest.
PAA experiments. Cells were pretreated for 1 h in the presence of 300 µg of PAA (Sigma)/ml and then infected with VZV-infected cells. Following 2 h of adsorption of VZV-infected cells, cells were washed three times with PBS and then incubated with TCM containing PAA for a further 24 h. Cells were then harvested and analyzed by flow cytometry as described above, and cell lysates were tested by Western blot analysis for inhibition of late viral gene expression.
Western blot analysis. Cells were washed once in PBS, sonicated for 1 min in cell extract buffer containing protease inhibitors (50 mM Tris [pH 7.4], 240 mM NaCl, 0.5% NP-40, 10% glycerol, 0.1 mM EDTA, 1 mM dithiothreitol, 0.5 mM phenylmethylsulfonyl fluoride), and centrifuged (14,000 × g), and the supernatants were collected. The cell supernatants (5 × 104 cells/lane) were separated on SDS-7% PAGE gels, followed by electrotransfer to Immobilon-P polyvinylidene difluoride membranes (Millipore, Bedford, Mass.). Membranes were stained with amido black (1% amido black [naptho, blue black], 45% methanol, 10% acetic acid) to reveal total protein before Western blot analysis. Membranes were incubated in blocking solution (5% nonfat milk in PBS) for 1 h. gC proteins were detected with a rabbit polyclonal antibody diluted 1:500 in blocking solution. Secondary goat anti-rabbit IgG-horseradish peroxidase conjugate (Amersham, Buckinghamshire, England) was diluted 1:2,000 and used for enhanced chemiluminescence detection of bound antibodies according to the manufacturer's protocol (Amersham). Molecular masses of proteins were determined using protein reference standards (Bio-Rad, Richmond, Calif.).
Plasmid DNA and transient transfection. Plasmid pMS62 contains the IE62 coding sequence under the control of the HCMV IE promoter (43) and was kindly provided by J. Hay, State University of New York at Buffalo. Plasmid pON2345 contains the HCMV IE promoter without any VZV genes and was kindly provided by E. Mocarski, Stanford University. Plasmids encoding VZV ORF4 (pCMV4), ORF10 (pCMV10), ORF61 (pCMV61), ORF47 (pCMV47), ORF63 (pCMV63), and ORF66 (pCMV66) under the control of the HCMV IE promoter were kindly provided by P. Kinchington, University of Pittsburgh. These plasmids were transiently transfected into HFF cells using a calcium phosphate transfection protocol (12). Cells were harvested 48 h after transfection, stained for MHC I expression, and analyzed by flow cytometry.
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RESULTS |
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Abstract
Introduction
Materials and Methods
Results
Discussion
References
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VZV downregulates cell surface MHC I expression in primary and
transformed human cells.
Human fibroblasts and melanoma (MeWo)
cells were used to analyze the effects of VZV infection on MHC I
expression because these cells are optimal for VZV replication in vitro
(5). Due to the highly cell-associated nature of VZV, HFFs
were infected with VZV strain Schenke by mixing VZV-infected and
uninfected HFF cells at a ratio of 1:5. At 24 h postinfection,
cells were stained for VZV and MHC I expression using polyclonal
VZV-immune serum and a mouse MAb to MHC I antigens, respectively, and
were analyzed by flow cytometry (Fig. 1A and
B). Negative controls included
mock-infected cells and incubation of both mock- and VZV-infected cells
with isotype control antibodies. At 24 h postinfection, 20% of
the cells were VZV+ and 80% of the cells remained
VZV
as determined by flow cytometry. Of the
VZV cell population, 90% were MHC I+. In
contrast, only 25% of the VZV+ cells were MHC
I+ (Fig. 1C). To determine whether VZV downregulated MHC I
expression in a selective manner and did not have a general effect on
host cell surface molecules, these cells were also assessed by flow cytometry for transferrin receptor (CD71) expression using an anti-CD71
MAb (Fig. 1D and E). At 24 h postinfection, more than 98% of both
VZV+ and VZV cell populations expressed
transferrin receptor (Fig. 1F). Taken together, these data show that
VZV selectively downregulated cell surface MHC I expression on human
fibroblasts. In a further four replicate experiments, specific
downregulation of MHC I expression was also observed.
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cells.
These data indicate that VZV isolates, whether fresh clinical isolates
or tissue culture-passaged virus, specifically downregulate MHC I
expression in primary and transformed human cells.
MHC I downregulation in human T lymphocytes infected with VZV.
VZV causes a mononuclear cell-associated viremia and tropism for T
lymphocytes, which is a critical event for VZV pathogenesis during
primary infection (5, 38). We therefore sought to determine whether VZV infection altered cell surface MHC I expression on human T lymphocytes using the SCID-hu thymus/liver mouse model (38). Human fetal thymus/liver implanted under the kidney
capsules of five SCID-hu mice was inoculated with HFF cells infected
with VZV strain Schenke. Mock-infected implants were injected with an
equal number of uninfected cells. Seven days after inoculation, total
cells from the implants were collected and stained with antibodies to
CD3 (a T-cell marker) and MHC I and VZV proteins. Flow cytometry was
performed whereby CD3+ T lymphocytes were gated and
analyzed for MHC I and VZV antigen expression (Fig. 2A and
B). In all five mice inoculated with
VZV-infected cells, VZV+ cells were readily detectable
(11.5 to 23%) (Fig. 2C). There was a significant decrease in the
percentage of MHC I+ cells in the CD3+
VZV+ population when compared to the CD3+
VZV population in all animals (Fig. 2D). These data
indicate that VZV infection of human CD3+ T lymphocytes
modulates cell surface MHC I expression.
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cell populations (data not
shown). These data indicate that VZV infection specifically
downregulated cell surface MHC I expression on human T lymphocytes.
Retention of MHC I molecules in VZV-infected cells.
To further
examine VZV-mediated downregulation of MHC I expression, we evaluated
the intracellular localization of MHC I molecules by immunofluorescence
and confocal microscopy on uninfected and VZV-infected cells. HFFs were
infected with VZV strain Schenke by mixing infected and uninfected HFFs
at a ratio of 1:3. At 24 h postinfection, cells were fixed and
permeabilized with acetone and incubated with antibodies against MHC I
and VZV antigens, followed by secondary antibodies conjugated with
either FITC or Texas red. Negative controls included mock-infected
cells and staining of VZV- and mock-infected cells with isotype control antibodies. VZV+ cells were readily detected in infected
cell populations (Fig. 3A). In contrast
to VZV cells, which displayed diffuse cytoplasmic MHC I
staining, VZV+ cells exhibited a significant accumulation
of MHC I molecules in the perinuclear region (Fig. 3B and C). No
staining was detected in VZV- or mock-infected cell populations when
isotype control antibodies were used. These data suggest that MHC I
molecules were retained within VZV-infected cells.
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MHC I molecules are not retained in the ER of VZV-infected
cells.
To determine the stage in the MHC I assembly process that
was disrupted by VZV in fibroblasts, we used pulse-chase and
immunoprecipitation experiments in the presence of endo H to examine
the synthesis and cell surface transport of MHC I complexes. HFFs were
infected with VZV strain Schenke by mixing VZV-infected and uninfected cells at a ratio of 1:2. These cells and mock-infected cells were labeled at 24 h postinfection with
[35S]methionine-cysteine for 30 min, chased for 1, 2, and
3 h before immunoprecipitation of MHC I molecules using W6/32 MAb,
and digested with endo H. Correctly assembled MHC I molecules enter the
medial Golgi compartment, where they acquire endo H resistance, whereas unassembled or ER-retained MHC I molecules remain endo H sensitive. In
mock-infected cells, MHC I molecules acquired endo H resistance by the
3-h chase period. Similarly, in VZV-infected cells the MHC I molecules
became resistant to endo H at the 3-h chase period (Fig.
4). Furthermore, the transferrin receptor
was efficiently converted to endo H-resistant forms during the
pulse-chase period in infected and uninfected cells (data not shown).
These data demonstrate that MHC I protein synthesis is unaltered in
infected cells and that MHC I complexes are not retained in the ER of
VZV-infected cells.
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) endo H. The MHC I endo H-resistant (R) and
-sensitive (S) forms are indicated.
Localization of MHC I molecules in the Golgi compartment of
VZV-infected cells.
To confirm a post-ER retention of MHC I
molecules and to demonstrate the intracellular localization of MHC I
molecules in VZV-infected cells, intracellular probes for the ER or the
Golgi compartment were used in conjunction with MHC I- and VZV-specific antibodies in immunofluorescence and confocal microscopy. HFF cells
were infected with VZV and incubated with either BODIPY-Texas red-ceramide to label the Golgi compartment or with Texas
red-conjugated ConA to label the ER 24 h after infection. Fixed and
permeabilized cells were then stained with an antibody to MHC I antigen
which was detected with a secondary antibody conjugated to FITC.
Negative controls included mock-infected cells and staining of VZV- and mock-infected cells with isotype control antibodies. The individual scans of ConA-derived fluorescence (Fig.
5A) and MHC I antibody stains (Fig. 5B)
on VZV-infected cells were electronically merged into one image (Fig.
5C). The dual-color image did not reveal any colocalization of these
molecules in VZV-infected cells. The images of ceramide labeling of the
Golgi complex (Fig. 5D) and the MHC I staining (Fig. 5E) of
VZV-infected cells were similarly superimposed into a dual fluorescence
image (Fig. 5F). The yellow color designates colocalization of the
ceramide and MHC I molecules and was found only in VZV-infected cells.
The colocalization of MHC I molecules with ceramide labeling in virally
infected cells demonstrates the retention of MHC I molecules in the
Golgi complex of VZV-infected cells.
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Immunoprecipitation of proteins from VZV-infected cells with MHC I
antibodies.
To determine whether a viral protein specifically
interacts with a component of the MHC I complex, thereby causing
retention of MHC I molecules, we used immunoprecipitation with MHC I
antibodies to assess whether any coprecipitating proteins could be
detected in VZV-infected cell lysates. HFFs were infected with VZV
strain Schenke by mixing VZV-infected and uninfected cells at a ratio of 1:2. These cells and mock-infected cells were labeled at 24 h
postinfection with [35S]methionine-cysteine for 1 h
before immunoprecipitation using W6/32 MAb and rabbit anti-heavy chain
antibody and digestion with endo H. In mock- and VZV-infected cells,
MHC I heavy chain and light chain (2 microglobulin) were detected
and showed similar endo H-resistant and -sensitive forms (Fig.
6). An ~40-kDa protein that
coprecipitated with MHC I molecules was detected in VZV-infected cell
samples but not in mock-infected cell lysates. This protein was
detected in four separate experiments and was detected only in
VZV-infected cells. In order to identify this protein,
immunoprecipitation was done in which half of the VZV-infected cell
sample was radiolabeled and the other half was not; cell lysates were
then immunoprecipitated with W6/32 and separated by SDS-12.5% PAGE.
The ~40-kDa protein was detected in the radiolabeled samples; the gel
containing unlabeled sample was Coomassie stained, and the ~40-kDa
protein band was excised, trypsin digested, and analyzed by mass
spectrometry. By sequence analysis, the ~40-kDa protein belonged to
MHC I as HLA class I alpha chain (data not shown), suggesting that
VZV-infected cells have an unusual cleaved form of MHC I protein.
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Late viral gene products do not affect cell surface MHC I expression. During productive VZV infection, viral genes are likely to be expressed in an ordered cascade which can be divided into three categories, the IE, early, and late genes characteristic of other herpesviruses (26). To identify the phase of viral gene expression responsible for MHC I modulation in VZV-infected cells, PAA, an inhibitor of viral DNA replication and thus late gene expression, was added to infected and mock-infected cells, and the cells were assessed for cell surface MHC I expression by flow cytometry.
HFFs were pretreated with 300 µg of PAA/ml for 1 h prior to infection and then infected by mixing VZV-infected cells with uninfected, PAA-treated cells at a ratio of 1:5 and incubated in the presence of PAA for a further 24 h. Cells were then harvested and stained with antibodies to MHC I and VZV for flow cytometric analysis or prepared for Western blot analysis. As predicted, the expression of the late gene gC was reduced more than 50-fold after the addition of PAA compared to untreated cells (Fig. 7A). Treatment with PAA did not change the reduction in MHC I expression. In the absence of PAA, 46% of VZV+ cells expressed cell surface MHC I molecules. In the presence of PAA, 54% of VZV+ cells expressed cell surface MHC I molecules (Fig. 7B). The observation that gC expression did not influence MHC I expression was confirmed using a VZV gC-negative mutant strain to infect fibroblasts (39); the percentage of cells that were VZV+ and MHC I+ was 50%, compared to 80% for VZV cells. Constitutive expression of VZV gE or
gK in melanoma cells also had no effect on cell surface MHC I
expression (data not shown). These data suggest that a VZV IE or early
gene product(s) or a virion component(s) is involved in reducing cell
surface MHC I expression on infected cells.
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Effects of VZV IE and early genes on MHC I expression.
VZV
encodes several genes which have been reported to be expressed under IE
conditions (32). To test whether these IE proteins might
mediate MHC I downregulation, human fibroblasts were transfected with
the plasmids expressing ORF62, ORF63, ORF4, and ORF61 (pMS62, pCMV63,
pCMV4, and pCMV61, respectively). In addition, we also tested plasmids
encoding the early gene products ORF10, ORF47, and ORF66 (pCMV10,
pCMV47, and pCMV66, respectively). After 48 h, transfected cells
were stained for cell surface MHC I expression and analyzed by flow
cytometry. Negative controls included cells transfected with the
parental plasmid (pON2345) and incubation of transfected cells with an
isotype control antibody. The mean fluorescence intensity of cell
surface MHC I staining was determined for each transfected population
of HFF cells (Fig. 8). Compared to the
parental plasmid, those expressing ORF4, -10, -47, -61, -62, and -63 did not significantly alter cell surface MHC I expression. In contrast,
the mean fluorescence intensity of cell surface MHC I staining was
significantly decreased for cultures transfected with the
ORF66-expressing plasmid. Similar results were obtained in two
replicate experiments, indicating that ORF66 plays a role in
downregulating MHC I.
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DISCUSSION |
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Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
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These experiments demonstrate that VZV expresses a protein(s) with an immunomodulatory function that interferes with the transport of MHC I molecules through the Golgi complex of infected cells and thereby inhibits the cell surface expression of MHC I molecules. VZV pathogenesis is characterized by cellular tropisms for T lymphocytes, skin, and dorsal root ganglia (5, 14). The capacity of VZV to regulate cell surface MHC I expression on human fibroblasts and, importantly, on human T lymphocytes provides a mechanism by which the virus can limit the consequences of immunosurveillance by CD8+ T lymphocytes. Impaired CD8+ T-cell recognition of VZV-infected cells, which involves the T-cell receptor recognition of viral peptides complexed with MHC I molecules, may allow infected T lymphocytes to harbor VZV during the viremic phases of pathogenesis. VZV cell-associated viremia is necessary for viral dissemination to mucocutaneous sites, and infection at these sites is required to achieve VZV transmission to susceptible contacts and its persistence in the human population. During latency, VZV differs from HSV in its ability to persist in satellite cells as well as in neurons and in the synthesis of viral gene transcripts and proteins in these latently infected cells (14). While neurons do not usually express MHC I molecules, interference with MHC I expression may help the virus to survive in nonneuronal cells within the ganglia. It is interesting that MHC I expression was downregulated by the recombinant Oka vaccine strain, which has been passaged in guinea pig embryo fibroblasts and in tissue culture cells and is attenuated for replication in skin (39), as well as by a low-passage clinical isolate.
In investigations of the mechanism of cell surface MHC I downregulation, we found that VZV infection does not alter MHC I protein synthesis and that complexes are not retained in the ER compartment. However, MHC I molecules accumulate in the Golgi complex of VZV-infected cells. These observations indicate that the pathway by which VZV infection reduces MHC I cell surface expression is novel, differing from the effects of the other human herpesviruses, HSV and HCMV (24). HSV has been shown to induce the retention of MHC I molecules in the ER through a specific interaction of a viral protein (ICP47) with the TAP complex, resulting in the prevention of TAP-mediated antigen transport (4, 19, 21, 25, 48, 50). In contrast, HCMV has been demonstrated to use several viral immunomodulatory proteins that affect various stages of the MHC I assembly pathway, including prevention of TAP-mediated antigen transport, retention of MHC I molecules in the ER, and dislocation of retained complexes to the cytosol for degradation (2, 3, 22, 23, 29, 30, 36, 49). Interestingly, MCMV encodes a protein that disrupts the transport of MHC I molecules past the ERGIC/cis-Golgi compartment (51). Therefore, the human herpesviruses, VZV, HSV, and HCMV, all employ unique strategies to downmodulate cell surface MHC I expression. VZV resembles MCMV in that both viruses cause the retention of MHC I molecules in the post-ER compartment.
Despite the sequence similarities between the genomes of VZV and HSV, VZV does not encode an ICP47 homolog. In addition, VZV does not contain any identifiable homologs to the gene products of the other herpesviruses known to alter cell surface MHC I expression. Nonetheless, experiments using PAA to inhibit viral DNA replication suggest that an IE or early VZV gene product(s) is involved in the downmodulation of cell surface MHC I molecules, whereas late genes were not required. Expression of gC was not required for MHC I modulation, and melanoma cell lines that expressed gE or gK had no alteration in cell surface MHC I expression, which was consistent with the results of the PAA experiments. Further, the transient transfection experiments described in the present study provide evidence that IE gene products do not modulate MHC I expression but that an early gene product encoded by ORF66 is able to downregulate MHC I expression on HFF cells. ORF66 is a putative serine/threonine protein kinase which is dispensable for viral replication in tissue culture. However, ORF66 is required for T-cell infectivity, since deletion of ORF66 was associated with decreased virus replication in thymus/liver implants in the SCID-hu mouse (40). Additional genetic studies using recombinant viruses will further define the function(s) of ORF66 during VZV infection. It is also possible that other viral genes may encode proteins with the ability to downregulate MHC I expression, as another herpesvirus, HCMV, encodes no fewer than four viral genes which function to downregulate MHC I expression (20).
The intracellular localization of MHC I molecules to the Golgi complex in VZV-infected cells suggests that a viral protein interacts specifically with a component of the MHC I complex, thereby preventing efficient MHC I transport to the cell surface. In this respect, other herpesviruses, including HSV, HCMV, and MCMV, have been shown to encode immunomodulatory proteins that directly associate with components of the MHC I biosynthesis pathway (2, 19, 21, 25, 29, 33, 36, 45, 48, 49, 50). Immunoprecipitation of radiolabeled MHC I molecules in VZV- and mock-infected cells did not reveal binding of a viral protein, but a modified, ~40-kDa MHC I molecule was detected consistently in VZV-infected cells, which may reflect accelerated degradation of MHC I molecules retained in the Golgi complex.
VZV and other viruses that modulate cell surface MHC I expression may evade cytotoxic T-lymphocyte (CTL) recognition, but by reducing the overall surface levels of MHC I expression, these cells may also become more sensitive to natural killer (NK) cell lysis. HCMV and MCMV have mechanisms to combat NK cell as well as CTL recognition (8, 9, 11, 17, 18, 33). Although an MHC I homolog has yet to be identified in the VZV genome, it is possible that VZV does encode a gene product to avoid NK cell lysis while maintaining immune evasion of CTL. Alternatively, as shown in HIV-infected cells, decreasing the cell surface concentration of certain MHC I alleles and not others may result in evasion of NK cell lysis (13). Our preliminary results suggest that VZV may also cause an allele-specific downmodulation of MHC I molecules (unpublished data).
In order to cause primary infection and to establish latency, VZV must be able to evade both MHC I- and MHC II-restricted immune responses with some efficiency. VZV memory immunity is characterized by the presence of equivalent numbers of antigen-specific CD4+ and CD8+ T lymphocytes (6). Our previous studies have shown that VZV has evolved a mechanism to minimize recognition of infected cells by CD4+ T lymphocytes by inhibiting gamma interferon-stimulated expression of MHC II molecules (1). Delayed induction of CD4+ T-lymphocyte responses to VZV antigens is accompanied by a longer period of formation of new skin lesions, which provide a reservoir for VZV spread to susceptible individuals (7). In addition, VZV reactivation and replication in skin cause herpes zoster, despite the presence of memory T lymphocytes that can produce high concentrations of gamma interferon when exposed to VZV antigens (27), as well as memory CD8+ CTL that recognize viral glycoproteins and structural and regulatory proteins. Thus, immunomodulatory mechanisms that limit the initial presentation of VZV peptides by MHC I or MHC II presentation pathways are likely to provide the virus with a transient advantage during primary and recurrent VZV infections.
In summary, we have demonstrated that VZV infection causes downregulation of MHC I molecules in human fibroblasts and T lymphocytes. The analysis of VZV-infected human T lymphocytes provides a novel demonstration of MHC I downregulation on a human cell type that is instrumental for viral pathogenesis. These experiments indicate that VZV encodes a protein(s) with an immunomodulatory function which does not affect biosynthesis of MHC I molecules but interferes with the transport of MHC I molecules through the cell, causing retention in the Golgi compartment. Immunomodulatory mechanisms that enhance the transport of VZV to skin and a period of viral replication before immunologic clearance in individuals with varicella or herpes zoster ensure opportunities for transmission to susceptible individuals and have allowed the virus to persist in the human population for millions of years.
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ACKNOWLEDGMENTS |
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This work was supported by a grant from the National Institute of Allergy and Infectious Diseases, AI20459.
We thank Jennifer Moffat for help with the SCID-hu experiments, Hideto Kaneshima, SyStemix, Inc., for supplying the SCID-hu mice, Chengjun Mo in our laboratory for providing the gE- and gK-expressing melanoma cells, and Frank Masiarz, Chiron Corporation, Emeryville, Calif., for the mass spectrometry analysis.
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FOOTNOTES |
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* Corresponding author. Mailing address: 300 Pasteur Dr., Rm. G312, Stanford University School of Medicine, Stanford, CA 94305-5208. Phone: (650) 723-5682. Fax: (650) 725-8040. E-mail: aarvin{at}stanford.edu.
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REFERENCES |
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Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
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Journal of Virology, May 2001, p. 4878-4888, Vol. 75, No. 10
0022-538X/01/$04.00+0 DOI: 10.1128/JVI.75.10.4878-4888.2001
Copyright © 2001, American Society for Microbiology. All rights reserved.
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