Abstract
Defects in Major Histocompatibility class I cell surface expression is thought to allow escape of tumor cells from immune surveillance. Hitherto, it is unclear whether this deficiency confers immune-independent survival advantage. We show here that class I cell surface expression deficiency due to defects in β2 microglobulin or the transporter-associated with antigen processing (TAP) results in resistance to apoptosis in response to various cytotoxic signals. Reduced apoptosis correlated with altered p53 activation, which was due to compromised nuclear translocation of p53. Binding of p53 to glycogen synthase kinase-3β (GSK3β), which is known to phosphorylate and lead to cytoplasmic sequestration of p53, was enhanced in these cells. Consistently, endoplasmic reticulum (ER) stress, which promotes binding of p53 to GSK3β was constitutively elevated in the absence of class I cell surface expression. Taken together, the results suggest a non-immunological causal role for defective class I cell surface expression in regulating cellular survival in a p53-dependent manner, through the upregulation of ER stress, which could be another mechanism leading to carcinogenesis.
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Main
The major histocompatibility complex (MHC) class I antigens are generally ubiquitously expressed and provide the identity to the host organism.1, 2 Expression of these antigens on the cell surface requires the concerted action of multiple proteins, which are part of the antigen processing machinery, including the transporters associated with antigen processing (TAP) 1 and 2, the low molecular mass polypeptide (LMP), tapasin, and so on,3, 4 which process the class I antigens in the endoplasmic reticulum (ER), after which the correctly folded heavy chain (class I molecules themselves) associates with the light chain (β2M molecules) and are together transported to the cell surface.5 The proper expression thus results in the eventual presentation of the self/foreign peptides at the cell periphery, facilitating T-lymphocyte recognition.
Correlation between levels of MHC class I expression and pathological conditions have been demonstrated. Hypoexpression of class I molecules on the cell surface have been observed in many tumor cells due to various mechanisms including methylation of the heavy chain genes, defects in β2M expression, defects in TAP or LMP expression, and so on, hence leading to their escape from immune surveillance by the cytotoxic T cells.6 Reintroduction of the missing MHC class I genes in many mouse tumor models resulted in the susceptibility of tumor cells to immune destruction,7 demonstrating a crucial role for the expression of MHC class I genes in enabling the recognition by T cells. On the contrary, elevated expression of the MHC class I antigens leads to recognition and destruction by the immune T cells, as demonstrated in autoimmune diseases.8 Transgenic overexpression of class I genes resulted in cellular defects such as developmental failure in chimeras; induction of insulin-dependent diabetes due to destruction of pancreatic β-cells; thyroid cell destruction; neural tube defects; disruption of lens development leading to cataract induction, and demyelination in oligodendrocytes.9, 10, 11, 12, 13 Although many of the phenotypes observed were dependent on activating the immune system, some were independent of immune activation and often resulted in tissue destruction, suggesting that MHC class I expression may have other non-immunological functions regulating cellular growth. However, whether changes in class I expression levels affect the proper functioning of a cell (independent on the immune system) has not been critically analyzed.
We therefore tested the hypothesis that modulation of class I expression could directly affect cellular survival independent of the immune system. Our data indicate that cells lacking class I expression on the cell surface were resistant to a variety of apoptotic insults and had compromised p53 activation. Defective p53 was due to its sequestration in the cytoplasm. Cells lacking class I expression on the cell surface had elevated ER stress, which led to cytoplasmic sequestration of p53. These data therefore suggest that defects in MHC class I expression in tumors may provide not only escape from immune surveillance, but also confer survival advantage on tumor cells through the elevation of ER stress.
Results
β2M−/− cells are resistant to cell death induced by genotoxic stress signals
Although sporadic reports have demonstrated that expression of MHC class I levels fluctuate during various physiological conditions, the relevance of such findings has not been fully understood. Hence, we first evaluated whether the absence of class I expression would affect cell death. As there are many class I antigens expressed in the cell, it is almost impossible to obtain cells devoid of all their expression. We therefore utilized primary mouse fibroblasts lacking β2M, in which surface expression of MHC class I antigens have been almost completely lost (Figure 1a).14 β2M−/− and β2M+/+ (wild type) primary embryonic fibroblast cells were derived from C57BL6/129 mouse embryos and tested for their sensitivity to nutrient deprivation and hypoxia, conditions prevalent in tumor masses in vivo. Cobalt chloride was used to induce hypoxia. Whereas wild-type cells were susceptible to apoptosis in both cases, as determined by annexin-V FITC and propidium iodide (PI) staining, β2M−/− cells were consistently more resistant (percentage viable cells – wild-type versus β2M−/− cells → untreated: 96 versus 97; 0.1% serum: 55 versus 77; 400 μ M CoCl2: 43 versus 67; 800 μM CoCl2: 7 versus 28) (Figure 1b, see bar chart for quantification), suggesting that the absence of β2M (and hence MHC class I expression) may confer survival advantage to cells. We therefore tested whether β2M−/− cells would be resistant to other forms of genotoxic stress signals. Treatment of wild-type fibroblasts with cytotoxic drugs such as cisplatin and vinblastine or UV irradiation invariably led to cell death, which was markedly reduced in β2M−/− cells (percentage viable cells – wild-type versus β2M−/− cells → untreated: 88 versus 89; vinblastine: 58 versus 78; cisplatin: 7 versus 52; UV: 33 versus 70) (Figure 1c, lower panel for quantification). Similar results were also obtained with other cytotoxic agents such as doxorubicin, camptothecin, hydrogen peroxide, and γ-irradiation, determined using similar methods and also by independent analysis of sub-G1 DNA content (data not shown), indicating that expression of β2M is essential for optimal cell death.
To evaluate whether the surface expression of MHC class I antigens was required for optimal cell death, we utilized the pan MHC blocking antibody, W6/32, which has the ability to block surface expression of MHC class I antigens by virtue of recognition of a non-polymorphic epitope common to all HLA class I molecules.15 Human primary fibroblastic cell line IMR90 was incubated with W6/32 antibody before UV irradiation. Incubation with W6/32 resulted in the loss of surface expression of the human MHC class I antigens, as detected with another pan HLA antibody (Figure 1d, leftmost upper panel). The UV irradiation resulted in cell death to similar extents in cells incubated with control or W6/32 antibodies (percentage dead cells: − versus + W6/32 → 50J UV: 23 versus 21; 150J: 33 versus 31) (Figure 1d), indicating the blocking MHC class I expression on the cellular surface (as opposed to inappropriate expression of MHC class I) does not affect sensitivity to cell death. Similar results were obtained with other genotoxic stresses (data not shown). Thus, the data together indicate that the absence of β2M affects the apoptotic process through mechanisms independent of surface exposure of the MHC class I antigens.
p53 activation is affected in β2M−/− cells
p53 is a major regulator of cellular death, and is often functionally inactivated in tumors.16 Thus, we envisaged that loss of MHC class I expression leading to p53 inactivation could be one mechanism through which tumor cells acquire resistance to death, and hence, survive. Therefore, we next investigated whether β2M−/− cells, which are resistant to cell death have compromised p53 activity. Immunoblot analysis indicated that whereas p53 protein was induced by various stress signals in wild-type mouse primary fibroblasts, it was severely compromised in β2M−/− cells (Figure 2a, left panel). Time course analysis after 80 J/m2 UV irradiation indicated that p53 was induced much later in the absence of β2M (Figure 1a, right panel), with delayed kinetics. Analysis of p53 mRNA levels indicated that it was not affected by the absence of β2M in fibroblasts as well as other tissues (Figure 2b). Examination of the half-life of p53, by treatment with the protein synthesis inhibitor cyclohexamide and subsequent pulse chase, indicated that lack of β2M did not lead to reduced-p53 stability (Figure 2c).
We therefore examined whether p53 activation was affected in the absence of β2M. Similar to earlier results, lower doses of UV irradiation (20 J/m2) also resulted in the delayed accumulation of p53 protein in β2M−/− cells (Figure 2d). While p53 accumulated at 1–2 h and reached the peak levels at 4–8 h post irradiation in wild-type cells, p53 was only visible at 4 h and reached peak levels at 24 h post irradiation in β2M−/− cells (Figure 2d; compare to loading controls and ratio of p53 to actin/tubulin). Analysis of posttranslation modifications such as phosphorylation at serines 18 and 389 (murine equivalent of serine 15 and 392, respectively) indicated that both these modifications were also delayed and compromised in β2M−/− cells (Figure 2d). However, phosphorylation of ataxia telangiectasia mutated (ATM) protein at serine 1981, a critical event for its activation and the eventual phosphorylation of mouse p53 on serine 18, and its activation was not affected after γ-irradiation in β2M−/− cells (data not shown). Consistent with the compromised activation of p53, the induction of p53 target genes such as PUMA, Cyclin G, MDM2, and p21 was reduced in β2M−/− cells (Figure 2d). Taken together, the data indicate that lack of β2M results in delayed and compromised activation of p53.
p53 nuclear translocation is affected in β2M−/− cells
One mechanism by which p53 activation can be compromised is due to the cytoplasmic sequestration of p53, as has been demonstrated in neuroblastoma cells and in cells undergoing endoplasmic reticulum stress.17, 18 Hence, we evaluated whether cytoplasmic nuclear localization of p53 is affected in β2M−/− cells. To this end, both wild-type and β2M−/− cells were UV irradiated and the location of endogenous p53 was monitored by immuno fluorescence after staining with p53-specific antibodies. p53, which was generally diffuse and almost undetectable in untreated wild-type cells was localized to the nucleus, starting at about 6 h and peaked at around 18 h post irradiation (Figure 3a, top panel). Whereas only 1.75% of the cells had p53 in the nucleus in untreated state, irradiation resulted in about 57–59% of the wild-type cell population containing nuclear p53 (Figure 3b). Consistent with published findings, treatment of wild-type cells with tunicamycin (TM), an ER stress-inducing agent, did not result in nuclear accumulation of p53 (Figure 3a, top panel).18 However, irradiation of β2M−/− cells did not result in substantial nuclear accumulation of p53 at both the time points, leading only to about 12–16% of the β2M−/− cells containing nuclear p53 (Figure 3a, middle panel). These results thus indicate that p53 localization to the nucleus might be affected in β2M−/− cells, which could contribute to the defects in p53 activation in these cells.
To confirm this, we performed fractionation of cellular lysates and analyzed the p53 status in the cytoplasmic and nuclear fractions. As shown in Figure 3c, UV irradiation resulted in an increase in p53 levels in cytoplasm from 2–8 h and a consequent accumulation in the nucleus between 4–16 h in wild-type cells. By contrast, although p53 accumulated later in β2M−/− cells (between 16–24 h), there was a distinct absence of accumulation in the nuclear fraction (Figure 3c, compare with loading controls). These data, together with the immunofluorescence results suggest that p53 translocation to the nucleus upon exposure to genotoxic stress such as UV irradiation is affected in the absence of β2M.
β2M−/− cells display constitutively elevated ER stress
Sequestration of p53 in the cytoplasm could be due to several mechanisms, one of which is elevated ER stress, as has been recently demonstrated.18 As the absence of β2M results in the improper folding of the MHC class I antigens (leading to defects in surface expression), we envisaged that this would lead to ER stress in these cells. We therefore tested whether the β2M−/− cells were subjected to constitutive ER stress. To this end, we employed several assays to determine the ER stress status. Firstly, the status of GRP78, which is activated by ER stress19 was evaluated. Untreated wild-type cells did not express GRP78, which was induced by treatment with TM or another ER inducer, thapsigargin (TG) (Figure 4a). By contrast, GRP78 expression was already detected in untreated β2M−/− cells, which were further robustly induced upon TM or TG treatment (Figure 4a), suggesting that the β2M−/− cells are subjected to ER stress even in the absence of drug treatment. Next, we determined the status of XBP-1, which is also induced by ER stress.20 Similar to GRP78, untreated β2M−/− cells expressed significantly higher basal levels of XBP-1 compared to their wild-type counterparts (Figure 4b, top panel). In both cell types, XBP-1 expression was induced upon treatment with TG or TM. XBP-1 is generally found in an unprocessed state and is processed by splicing of a small intron upon ER stress, giving rise to bands of different sizes upon Pst1 restriction enzyme digestion.21 Analysis upon Pst1 digestion also revealed elevated levels of processed product from untreated β2M−/− cells compared to wild-type cells (Figure 4b, lower panel).
ER stress has also been shown to result in the phosphorylation and activation of the ER-resident kinase, PERK.22 Analysis of phosphorylation status of PERK indicated that it was constitutively and robustly phosphorylated in β2M−/− cells compared to wild-type cells (Figure 4c). The levels of total PERK was not affected, and treatment with TM or TG resulted in phosphorylation of PERK in wild-type cells, confirming its role in ER stress activation (Figure 4c).
As ER stress was shown to inactivate p53 function due to the physical interaction with GSK-3β, leading to sequestration of p53 in the cytoplasm,18 we tested whether p53 was constitutively bound to GSK-3β in β2M−/− cells. Immunoprecipitation with anti-p53 antibodies and subsequent immunoblot with anti-GSK-3β antibodies indicated that GSK-3β was only bound to p53 upon ER stress induced by TG in wild-type cells (Figure 4d). However, GSK-3β was found to be bound to p53 in the untreated state in β2M−/− cells (Figure 4d), indicative of elevated ER stress in these cells. The total levels of GSK-3β were equal in both cell types, thereby excluding any alterations in GSK-3β levels in β2M−/− cells that may have contributed to the observations (Figure 4d, lower panel).
To further confirm these observations, we performed immunofluorescence studies to evaluate the localization of GSK-3β, which was shown to be enriched upon ER stress.18 Consistently, we found that GSK-3β was diffused in untreated cells and was enriched in the nucleus upon TG treatment in wild-type cells (Figure 4e, left panel). However, GSK-3β was found both in the nucleus and the cytoplasm of untreated β2M−/− cells to a higher extent (Figure 4e, right panel). To substantiate this observation, we utilized nuclear and cytoplasmic fractions from cells of both genotypes and found that GSK-3β levels were indeed elevated in the nuclear fraction of β2M−/− cells compared to wild-type cells (Figure 4f; compared with loading control). As expected, more p53 was seen in the nuclear fraction of wild-types cells in contrast to β2M−/− cells after UV irradiation (Figure 4f). Thus, the data together suggest that the absence of β2M results in constitutively elevated ER stress, thereby probably leading to the sequestration of p53 in the cytoplasm.
Loss of MHC class I expression due to TAP deficiency also results in defects in apoptosis, p53 activation and elevated ER stress
To evaluate whether the lack of class I expression due to other defects in the MHC processing pathway would also result in a similar phenotype, we employed the mouse RMA and RMAS isogenic tumor cells that are proficient or deficient in TAP expression, respectively.23 TAP has been demonstrated to be required for the efficient expression of MHC class I on the cellular surface.24 Flow cytometric analysis confirmed that RMAS cells have a significant reduction of surface expression of the H-2kb antigen (Figure 5a). Cell death analysis indicated that whereas RMA cells were sensitive to a variety of cellular stress insults such as cisplatin, γ- and UV irradiation, RMAS cells were significantly more resistant to cell death (percentage dead cells → RMA versus RMAS – untreated: 2.5 versus 3.5; cisplatin: 52.7 versus 24.3; IR: 38.5 versus 23.5; UV: 67.1 versus 29.2) (Figure 5b), similar to the observation with β2M−/− cells. Moreover, p53 levels after γ-irradiation was also compromised in RMAS cells compared to RMA cells (Figure 5c). Analysis of ER stress markers such as XBP-1 levels indicated that untreated RMAS cells contained higher levels of XBP-1 compared to RMA cells (Figure 5d, left top panel). Moreover, Pst1 restriction digestion experiments indicated that RMAS cells contained significantly higher levels of processed products even in unstressed state (Figure 5d, left middle panel). In addition, western blot analysis confirmed that RMAS cells expressed higher XBP-1 protein even without any ER stress inducers (Figure 5d, right panel). Taken together, the data indicate that absence of MHC class I expression due to defects in various mechanisms result in elevated ER stress and consequently, defective p53 activation and resistance to apoptosis.
Discussion
The data presented here demonstrate that the defects in MHC class I surface expression result in elevated ER stress and defective p53 activation. This leads to resistance to multiple apoptotic stimuli, therefore conferring cellular survival advantage. These results thus identify a novel role for defects in MHC class I antigen expression in promoting cellular growth and survival by allowing escape from apoptotic pressure.
Although sporadic reports have demonstrated that expression of MHC class I levels fluctuate during various physiological conditions, the relevance of such findings has not been fully understood. The data presented here show that reduced class I expression confers survival advantage in response to growth factor deprivation, hypoxia, and a variety of genotoxic stresses. It is to be noted that oncogene-mediated cellular transformation and subsequent tumorigenesis – in which conditions of hypoxia and nutrient deprivation prevail – are also associated with reduction in class I expression.25, 26, 27 Conversely, treatment with genotoxic agents leading to cell cycle arrest was associated with increased class I expression. Supporting evidence comes from pathological conditions in which cells undergoing arrest or cell death have also been associated with increased MHC class I expression. For example, motoneurons and nigral dopaminergic neurons in the brainstem of adult rat which were vulnerable to neurodegeneration in diseases such as Parkinson's disease (PD) and amyotrophic lateral sclerosis display high levels of both MHC class I heavy chain and β2M mRNAs.28 Moreover, MHC class I expression was elevated in microglia upon both ischemia and axonal degeneration.29 Similarly, we have noted that overexpression of MHC class I molecules also lead to p53-dependent apoptosis in fibroblasts (data not shown). Thus, these evidences from physiological settings correlate surface MHC class I levels with cellular survival, supporting our observations using cultured cells.
Defects in MHC class I expression were found to result in ER stress, which led to defects in p53 activation due to cytoplasmic sequestration of p53. p53 is a known mediator of cell death, and functional inactivation often occurs in tumors.16 Thus, loss of MHC class I expression leading to p53 inactivation may thus be one mechanism through which tumor cells acquire resistance to death, and hence survive. A recent report shows that downregulation of MHC class I expression correlated with poor prognosis in colon cancers is supporting this idea.30 Besides, several reports have suggested a positive correlation between elevated ER stress and resistance to apoptosis, and between an increase in ER markers and carcinogenesis. Overexpression of GRP78 was shown to result in reduced apoptosis and higher colony survival upon genotoxic challenges, and has been associated with hepatocarcinogenesis and malignant breast lesions, and very recently, to be a predictor of chemoresistance.31, 32, 33, 34 Moreover, PERK function was shown to be essential for cell survival following the exposure of cells to ER stress.35 Furthermore, XBP-1 was also shown to be essential for survival under hypoxic conditions and is required for tumor growth.36 Finally, reduction of expression of ER proteins correlated with lower viability after ionophore treatment.37 Taken together, the evidence supports our proposal that defects in cell-surface MHC class I expression lead to resistance to apoptosis by elevating ER stress.
As p53 nuclear localization and consequently its activity is compromised due to lack of MHC class I expression, we also investigated whether lack of class I in β2M−/− mice would affect tumorigenicity. However, β2M−/− mice did not succumb to spontaneous tumors up to over 3 years unlike their p53−/− counterparts (data not shown). This suggested that although p53 activation (such as apoptosis) is compromised in β2M−/− cells, it was not sufficient to allow the formation of spontaneous tumors in mice. This could be due to the requirement for a threshold of p53 activity that has to be maintained for tumor suppression (which was not breached in the β2M−/− mice) – implying that although p53 activity is compromised in β2M−/− mice, it is not sufficient enough to inhibit p53's tumor suppressive function. In this respect, we noted that not all p53-dependent functions, such as ras-mediated senescence of primary fibroblasts as well as basal cellular proliferation rates, were compromised by lack of β2M (data not shown). Thus, although the defects in MHC class I surface expression is not sufficient to promote tumorigenicity, its absence leading to resistance to apoptosis probably contributes to the tumorigenic process.
In conclusion, the data presented here suggest that defects in MHC class I expression often found in cancer cells may not only provide an avenue for escape from immune surveillance, but also directly result in their resistance to apoptotic stimuli, thereby allowing enhanced growth. Thus, the status of surface MHC class I levels in tumors may provide information on whether the tumors may respond well to cytotoxic drugs, and be of prognostic significance. In addition, future efforts aimed at identifying regulators of ER stress may have potential utility in treating class I deficient tumors.
Materials and Methods
Cell lines, transfections, treatment conditions, and plasmids
All cell lines used in this study were cultured in 10% fetal bovine serum containing DMEM. IMR90 human diploid fibroblasts were obtained from ATCC. RMA and RMAS cells were obtained from Dr. Hideo Yagita and grown as non-adherent cells in culture. Murine embryonic fibroblasts (MEFs) were isolated from E12.5 p53−/− and β2M−/− embryos and as described and immortalized spontaneously according to the 3T3 protocol.38 Cells were starved by culturing in medium containing 0.5% serum for 48 h, and subsequently, 20% FCS (final concentration) was added directly onto the dishes to release them into the cell cycle. Nutrient deprivation was achieved by culturing cells 0.1% serum containing medium without other amino acids and nutrients.
Cells were treated with the following stress signals for cell death and MHC class I analysis: UV irradiation (as indicated); γ-irradiation (20 Gy); cobalt chloride (400 and 800 μM); vinblastine (15–30 μM); cisplatin (50–80 μM); TM (10 μg/ml), and TG (1 μM), for indicated time periods. Cells were treated with 25 μg/ml cyclohexamide to inhibit protein synthesis for the indicated time periods.
Immunoblot analysis
Immunoblot analysis was performed as described.38 Cellular fractionation was performed using NE-PER nuclear and cytoplasmic extractions reagents (Pierce Biotech), according to the manufacturer's protocol. The following antibodies were used for immunoblot analysis: p53 (CM5 – Novocastra) and (IC12 – Cell Signaling), phospho-ser18, -ser 315, and -389 p53, GSK-3β (Cell Signaling), phospho-PERK (US Biologicals), MDM2, Puma, Cyclin G, XBP-1, PERK, p21, Tubulin (Santa Cruz), Lamin (Cell Signaling), and Actin (Sigma).
Immunoprecipitations were carried out using anti-p53 antibody (mixture of Ab-3 and Ab-4, Oncogene Sciences), and immunoblotted using anti-p53 (CM5 or IC12) or anti-GSK3β antibodies.
Flow cytometry and cell death assays
Flow cytometric analysis was performed to determine MHC class I surface expression, using either the anti-H-2Kb or H-2Kk (Pharmingen) antibodies. Cell-surface MHC class I expression was blocked by incubated with the anti-pan HLA-blocking antibody (W6/32) for 1 h, before analysis of HLA surface expression using another anti-pan HLA antibody (clone G46-2.6, Pharmingen).
Two independent cell death assays were employed in this study, namely PI staining of sub-G1 populations, and annexin-V staining. Sub-G1 population analysis representing dead cells was performed as for cell cycle status analysis. To detect annexin-V+ cells, cells were incubated with FITC-conjugated annexin-V (BD biosciences) and 50 μg/ml PI in binding buffer, and cells were analyzed by flow cytometry.
RNA analysis
Total RNA was extracted and utilized for reverse transcriptase-PCR (RT-PCR) analysis as described39 using the following primers: GRP78 – for: 5′- TTGCTGGACTCCTAAGACTC-3′; rev: 5′ –AGCAGATCAGTGCACCTACA-3′ (expected size: approximately 2.0 Kb); XBP-1 – For: 5′- AAACAGAGTAGCAGCGCAGACTGC-3′; Rev: 5′-GGATCTCTAAAACTAGAGGCTTGGTG-3′ (600 bp); p53 – For: 5′- GCAATTCGCCATGGAGGAGTCACAGTCG-3′; rev: 5′- CCCAAGCTTCAGTCTGAGTCAGGCCCCAC-3′ (1.2 Kb); Tubulin – For: 5′- CCACGTCAAGACGGCCGTGTG-3′; Rev: 5′- GACAGAGGCAAACTGAGCACC-3′ (436 bp); gapdh – For: 5′- ATCTTCTTGTGCAGTGCCAG-3′; rev: 5′-GTAGTTGAGGTCAATGAAGG-3′ (140 bp). XBP-1 product was digested with Pst-1 restriction enzyme to determine the amount of processed or unprocessed products of 300 and 600 bp, respectively, as described.21
Northern blot was performed using mouse p53 cDNA as a probe as described.38
Immunofluorescence
Cells grown on cover slips were fixed in 4% paraformaldehyde/PBS and incubated with anti-p53 (mixture of Ab-3 and Ab-4), or anti-GSK3β antibodies, followed by incubation with the secondary antibody (FITC or PE-conjugated anti-mouse/rabbit IgG) before being mounted in mounting medium containing DAPI. Cells were counted by eye, and compared to negative controls such as those without primary antibody as well as with p53−/− cells stained with anti-p53 antibody. Cells with signals above these negative controls were counted as positive events. Between 150 and 200 cells were counted per field, and at least three independent fields were analyzed per experiment. The experiments were repeated at least four independent times.
Abbreviations
- ATM:
-
ataxia telangiectasia mutated
- ER:
-
endoplasmic reticulum
- GSK:
-
glycogen-synthase kinase
- MHC:
-
major histocompatibility complex
- TAP:
-
transporter-associated with antigen processing
- TM:
-
tunicamycin
- TG:
-
thapsigargin
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Acknowledgements
We thank Tan YT for technical assistance during the early phase of the project, Dr. Hideo Yagita for the RMA/RMAS cells, and Dr. Hui KM for the W6/32 antibody. This work was supported by the generous funding by the National Medical Research Council of Singapore (NMRC) and Nippon Boehringer Ingelheim, Japan, to KS.
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Sabapathy, K., Nam, S. Defective MHC class I antigen surface expression promotes cellular survival through elevated ER stress and modulation of p53 function. Cell Death Differ 15, 1364–1374 (2008). https://doi.org/10.1038/cdd.2008.55
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DOI: https://doi.org/10.1038/cdd.2008.55
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