MHC class II associated stomach cancer mutations correlate with lack of subsequent tumor development
- Authors:
- Published online on: September 29, 2017 https://doi.org/10.3892/mco.2017.1432
- Pages: 1119-1121
Abstract
Introduction
The potential impact of MHCII expression on solid tumor cells received increased interest when it became apparent over two decades ago that mutations specific to tumorigenesis interfered with MHCII induction by interferon-γ (IFN-γ) (1–9). As one example, a lack of retinoblastoma tumor suppressor protein leads to over expression of the pro-proliferative protein, YY1, which in turn is part of a repressive complex that maintains histone deacetylase activity at the MHCII promoter, thereby blocking the assembly of MHCII enhanceosome proteins, including the highly specific MHCII enhanceosome proteins, RFXANK, RFXAP, RFX5 and CIITA (10,11). In addition, Ostrand-Rosenberg and colleagues (12,13) have established the negative impact of tumor cell-MHCII expression on tumor development, although there remain questions about whether such a negative impact occurs in a natural state, where there is the expectation of CLIP expression blocking endogenous MHCII tumor-peptide loading, or in the absence of tumor cell expression of conventional co-stimulatory molecules. The apoptotic mechanisms of tumor cell MHCII expression provide another possible ‘anti-tumor’ role (14,15).
Data collection methods
Clinical and primary tumor specimen mutation Microsoft Excel files for the stomach adenocarcinoma (STAD), skin cutaneous melanoma (SKCM), lung adenocarcinoma (LUAD), colon adenocarcinoma (COAD), head and neck squamous cell carcinoma (HNSC) and bladder urothelial carcinoma (BLCA) cancer sets was downloaded from the TCGA data portal (dbGaP project approval number 6300). The ‘new tumor event after initial treatment’ column of the TCGA clinical follow up file for each cancer dataset was used to categorize barcodes based on the development of a new tumor or not (Table I, New Tumor and No Subsequent Tumor, respectively). To obtain matching barcodes, for the clinical and somatic mutation files, the barcodes from the primary tumor specimen mutation file were truncated to contain the following characters, TCGA-##-####. Mutation data, including truncated tumor sample barcodes, human genome organization symbols and mutation type (nonsynonymous or silent) for HLA-DRA and the set of transcription factors (CIITA, RFX5, RFXANK and RFXAP) associated with MHC Class II were collected for each cancer dataset. Mutations were assessed using the PROVEAN web tool (16) The Excel COUNTIF function was used to obtain the number of MHC Class II coding region mutations per barcode for the New Tumor and No Subsequent Tumor groups for each cancer dataset and a statistical comparison between the groups was conducted. t-tests were used to obtain P-values. P<0.05 was considered to indicate a statistically significant difference. P-values were obtained using Microsoft Excel (Microsoft Corporation, Redmond, WA, USA).
All procedures performed in studies involving human participants were in accordance with the ethical standards of the institutional and national research committee and with the 1964 Helsinki declaration and its later amendments or comparable ethical standards. The present study is exempt from IRB approval and was approved via the National Institutes of Health, Database of Phenotypes and Genotypes (dbGaP), project no. 6,300; approval granted to George Blanck.
Results and discussion
TCGA provides a wealth of information regarding mutagenesis in many cancer datasets. To obtain an indication of mutations that may impact MHCII expression, TCGA was searched for mutations in RFXAP, RFXANK, RFX5, CIITA and HLA-DRA. Other MHCII structural genes were excluded due to the potential confusion caused by the high level of polymorphisms. Overall, the nonsynonymous mutation rate for the following TCGA datasets, for the above collection of MHCII specific proteins, was ~8–9%: STAD, SKCM, LUAD, COAD, HNSC and BLCA.
The opportunities for linking TCGA clinical information, particularly negative vs. positive outcomes, to particular mutations remains limited, largely owing to the minimal overlap of barcodes (patient samples) for mutation results and clinical information. However, it is possible to attempt to correlate mutation results with either no-subsequent tumor or new-tumor for the above cancer datasets, particularly due to the relatively high number of barcodes available representing this distinction (Table I). Of the six TCGA datasets representing a substantial number of mutations and no-subsequent tumor and new-tumor cases, only the stomach cancer datasets (STAD) demonstrated a correlation with the MHCII specific mutations, namely an association of more mutations with no-subsequent tumor (Table II). Of thirty-one mutations that were in the STAD no-subsequent tumor group, 21 were assessable by the PROVEAN (17) web tool, of which 9 were deleterious and 12 were neutral. The two mutations that were in the new-tumor group were assessable by PROVEAN, revealing that 1 was deleterious and 1 was neutral.
Table II.The average number of mutations per barcode and statistical comparison of the New Tumor and No Subsequent Tumor sets |
As aforementioned, solid tumor cell expression of MHCII has led to contradictory impressions as to whether MHCII facilitates or inhibits solid tumor development. The above data support the former possibility, but no doubt there are a number of circumstances in which the impact of solid tumor expression of MHCII may have varying effects on tumor progression. For example, varied solid tumors may be affected differently by constitutive MHCII expression or MHCII induction by IFN-γ. Furthermore, MHCII expression may have different impacts at different stages of tumorigenesis. The issue of the variable impacts of immune function spans the consideration of the role of the immune system in tumor development. Immune checkpoint inhibitors have had great positive benefits for at least a subset of patients (18), yet in other settings, evidence indicates that inflammation, particularly chronic inflammation, is associated with tumor development (19,20).
The negative impact of MHCII expression on solid tumor cells may include induction of T-cell anergy (21), due to lack of costimulatory molecules, but a previous study indicates that non-professional antigen presenting cells, including solid tumor cells, are able to employ substitute co-stimulatory molecules such as ICAM1 (22). Another potential explanation for a negative impact of MHCII expression is the possibility that MHCII facilitates T-cell engulfment by solid tumor cells (23,24).
In conclusion, the current study indicates that, at least in certain situations, the expression of MHCII on tumor cells may represent a negative prognosis. Such a conclusion calls into question scenarios where MHCII-based interactions with the immune system would facilitate an anti-tumor immune response.
Acknowledgements
The authors would like to acknowledge the support of the Anna Valentine Program and the taxpayers of the State of Florida.
Glossary
Abbreviations
Abbreviations:
MHC |
major histocompatibility complex |
STAD |
stomach adenocarcinoma |
TCGA |
the cancer genome atlas |
CIITA |
class II transactivator |
RFX |
regulatory factor-X |
SKCM |
skin cutaneous melanoma |
LUAD |
lung adenocarcinoma |
COAD |
colon adenocarcinoma |
BLCA |
bladder carcinoma |
HNSC |
head and neck cancer |
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