Case Control Study Open Access
Copyright ©The Author(s) 2015. Published by Baishideng Publishing Group Inc. All rights reserved.
World J Gastroenterol. Dec 14, 2015; 21(46): 13064-13072
Published online Dec 14, 2015. doi: 10.3748/wjg.v21.i46.13064
Association between hepatocellular carcinoma and tumor necrosis factor alpha polymorphisms in South Korea
Suk Pyo Shin, Ju Hwan Kim, Ju Ho Lee, Hana Park, Kyu Sung Rim, Seong Gyu Hwang, Department of Internal Medicine, CHA Bundang Medical Center, CHA University, Seongnam 463-712, South Korea
Nam Keun Kim, Jung Oh Kim, Sung Hwan Cho, Department of Biomedical Science, College of Life Science, CHA University, Seongnam 463-400, South Korea
Nam Keun Kim, Jung Oh Kim, Sung Hwan Cho, Institute for Clinical Research, CHA Bundang Medical Center, CHA University, Seongnam 463-712, South Korea
Suk Pyo Shin, Ju Hwan Kim, Ju Ho Lee, Hana Park, Kyu Sung Rim, Seong Gyu Hwang, Institute of Gastroenterology, CHA Bundang Medical Center, CHA University, Seongnam 463-712, South Korea
Mi Na Kim, Department of Internal Medicine, CHA Gangnam Medical Center, CHA University, Seoul 135-913, South Korea
Author contributions: Shin SP and Kim NK contributed equally to this manuscript and considered as co-first author; Shin SP, Hwang SG and Kim NK designed research; Hwang SG and Rim KS contributed to acquisition of data; Shin SP, Kim NK, Kim JO and Cho SH performed research; Kim JH, Lee JH, Park H and Kim MN analyzed and interpreted data; and Shin SP wrote the manuscript.
Supported by Basic Science Research Program through National Research Foundation of Korea Grants funded by the Korean Government, No. NRF-2012R1A1A2007033 and No. 2009-0093821, South Korea.
Institutional review board statement: The present study was approved by the Institutional Review Board of CHA Bundang Medical Center, and written informed consent was obtained from all case and control subjects in the study.
Conflict-of-interest statement: The authors disclose no conflicts of interest.
Data sharing statement: All the dataset are available from the author at nkkim@cha.ac.kr
Open-Access: This article is an open-access article which was selected by an in-house editor and fully peer-reviewed by external reviewers. It is distributed in accordance with the Creative Commons Attribution Non Commercial (CC BY-NC 4.0) license, which permits others to distribute, remix, adapt, build upon this work non-commercially, and license their derivative works on different terms, provided the original work is properly cited and the use is non-commercial. See: http://creativecommons.org/licenses/by-nc/4.0/
Correspondence to: Seong Gyu Hwang, MD, PhD, Professor, Department of Internal Medicine, CHA Bundang Medical Center, CHA University, Yatapro 59, Bundang-gu, Seongnam 463-712, South Korea. sghwang@cha.ac.kr
Telephone: +82-31-7805213 Fax: +82-31-7805219
Received: June 29, 2015
Peer-review started: July 4, 2015
First decision: July 19, 2015
Revised: August 24, 2015
Accepted: October 17, 2015
Article in press: October 20, 2015
Published online: December 14, 2015

Abstract

AIM: To investigate associations between the tumor necrosis factor alpha (TNF-α) -1031 T>C, -863 C>A, -857 C>T, -308 G>A, and -238 G>A polymorphisms and HCC in Korea.

METHODS: Hepatocellular carcinoma (HCC) cases were diagnosed at CHA Bundang Medical Center from June 1996 to August 2008. The association between TNF-α polymorphisms and HCC was analyzed in 157 HCC patients and 201 controls using a polymerase chain reaction-restriction fragment length polymorphism assay. We investigated five TNF-α polymorphisms, which are TNF-α -1031 T>C, -863 C>A, -857 C>T, -308 G>A, and -238 G>A. The TNF-α genotype frequencies, genotype combinations and haplotypes were analyzed to disclose the association with HCC.

RESULTS: None of the TNF-α polymorphisms was significantly associated with HCC. However, nine genotype combinations had associations with increased likelihood of HCC. Among them, TNF-α -1031/-857/-238 TT/CC/GA (AOR = 18.849, 95%CI: 2.203-161.246, P = 0.007), TNF-α -1031/-308/-238 TT/GG/GA (AOR = 26.956, 95%CI: 3.071-236.584, P = 0.003), and TNF-α -1031/-238 TT/GA (AOR = 21.576, 95%CI: 2.581-180.394, P = 0.005) showed marked association with HCC. There were five haplotypes of TNF-α polymorphisms which were significantly associated with HCC. They are TNF-α -1031/-863/-857/-308/-238 T-C-C-G-A (OR = 25.824, 95%CI: 1.491-447.223, P = 0.0005), TNF-α -1031/-857/-308/-238 T-C-G-A (OR = 12.059, 95%CI: 2.747-52.950, P < 0.0001), TNF-α -1031/-857/-238 T-C-A (OR = 10.696, 95%CI: 2.428-47.110, P = 0.0001), TNF-α -1031/-308/-238 T-G-A (OR = 7.556, 95%CI: 2.173-26.280, P = 0.0002) and TNF-α -1031/-238 T-A (OR = 10.865, 95%CI: 2.473-47.740, P = 0.0001). Moreover, HCC Okuda stage III cases with the TNF-α -1031 CC genotype had better survival than those with the TT genotype (AOR = 5.795, 95%CI: 1.145-29.323).

CONCLUSION: Although no single TNF-α polymorphism is associated with HCC in this study, some TNF-α genotype combinations and haplotypes are associated with HCC. In addition, HCC Okuda stage III cases with the TNF-α -1031 TT genotype may have a better prognosis than those with the CC genotype.

Key Words: Tumor necrosis factor-alpha, Polymorphism, Single nucleotide, Carcinoma, Hepatocellular

Core tip: We genotyped five single nucleotide polymorphisms [Tumor necrosis factor alpha (TNF-α) -1031T>C, -863C>A, -857C>T, -308G>A, and -238G>A] in hepatocellular carcinoma (HCC) patients and control subjects. A number of genotype combinations and some haplotypes had association with HCC. In addition, HCC Okuda stage III cases with the TNF-α -1031 TT genotype had a better prognosis than those with the CC genotype.
INTRODUCTION

Primary liver cancer is the fifth most common cancer (fourth in men, sixth in women) in South Korea, and the second most common cause of cancer-related deaths[1]. Hepatocellular carcinoma (HCC) is the most common type of primary liver cancer. HCC carcinogenesis is a multistep, multifactorial process. However, hepatitis B virus (HBV) and hepatitis C virus (HCV) are the best-known risk factors for HCC. Approximately 70%-80% of HCCs are related to these persistent viral infections[2-5]. Various inflammatory mediators related to chronic inflammation are known as cofactors in carcinogenesis[6]. Among these, tumor necrosis factor alpha (TNF-α) is the most important cytokine in inflammation-associated tumoriogenesis[7].

TNF-α is a potent, pleiotropic, proinflammatory cytokine. It is produced mainly by macrophages, but also by a broad variety of other cell types, including lymphoid cells, mast cells, endothelial cells, fibroblasts, and neurons[8]. The TNF-α gene lies in the class III region of the major histocompatibility complex (MHC) and is located on human chromosome 6p21.3[9]. Some single nucleotide polymorphisms (SNPs) in the TNF promoter have been identified, and they are thought to affect TNF-α production[10]. Past research has shown that the TNF-α -308 GG genotype[11] and TNF-α -857 T polymorphism[12] are associated with gastric cancer, the TNF-α -308 G>A polymorphism[13] is associated with vascular invasion of breast tumors, the TNF-α -308 G/A polymorphism[14] is associated with lung cancer, the TNF-α -308 G>A polymorphism[15] is associated with prostate cancer, the TNF-α -308 G>A polymorphism[16] is associated with oral squamous cell carcinoma, the TNF-α -238 G>A polymorphism[17] is associated with bone cancer, and the TNF-α -308 G>A polymorphism[18] is associated with invasive cervical cancer.

The results of past studies on the association between TNF-α polymorphisms and HCC have had conflicting results. A meta-analysis of 10 case-control studies reported that the TNF-α -308 GG genotype is associated with a modest decrease in HCC risk[19]. Similarly, a meta-analysis by Yang et al[20] reported that the TNF-α -308 G>A polymorphism is associated with increased HCC risk and that the TNF-α -238 G>A polymorphism is not associated with HCC. However, these meta-analyses did not investigate other TNF-α polymorphisms. Wei et al[21] performed a meta-analysis of 17 relevant studies and found that the TNF-α -308 G>A, -238 G>A, and -863 C>A polymorphisms are associated with HCC among Asians, while the TNF-α -857 C>T and -1031 T>C polymorphisms are not related to HCC risk. This meta-analysis did not investigate the association between TNF-α haplotypes and HCC risk, however.

We investigated the association between the TNF-α -1031 T>C, -863 C>A, -857 C>T, -308 G>A, and -238 G>A polymorphisms and HCC in Korea.

MATERIALS AND METHODS
Study population

A total of 157 HCC cases diagnosed at CHA Bundang Medical Center from June 1996 to August 2008 were enrolled. The control group consisted of 201 individuals randomly selected from a health screening program with age and gender matched to HCC patients. Exclusion criteria included a history of other cancer or other severe medical conditions. Individuals with only hypertension and diabetes were not excluded. The grade of hepatic impairment was classified by Child-Pugh scores. HCC clinical stage was evaluated on the basis of TNM classification and Okuda stage. The present study was approved by the Institutional Review Board of CHA Bundang Medical Center, and written informed consent was obtained from all case and control subjects in the study.

DNA extraction and genotyping

Genomic DNA was extracted from leukocytes using a G-DEX II Genomic DNA Extraction Kit (iNtRON Biotechnology, Seongnam, South Korea). The TNF-α -238 G>A (rs361525), TNF-α -308 G>A (rs1800629), TNF-α -857 C>T (rs1799724), TNF-α -863 C>A (rs1800630), and TNF-α -1031 T>C (rs1799964) polymorphisms were analyzed using a polymerase chain reaction (PCR)-restriction fragment length polymorphism (RFLP) assay. The -238 G>A polymorphism was analyzed using the forward primer 5’-AGA AGA CCC CCC TCG GAA CC and the reverse primer 5’-ATC TGG AGG AAG CGG TAG TG, and PCR products were cut using the restriction enzyme MspI. Genotyping of the -308 G>A polymorphism was performed using the forward primer 5’-AGG CAA TAG GTT TTG AGG GCC AT and reverse primer 5’-TCC TCC CTG CTC CGA TTC CG, and PCR products were cut using the restriction enzyme Nco. Genotyping of the -857 C>T polymorphism was performed using the forward primer 5′- AAG TCG AGT ATG GGG ACC CCC CGT TAA and the reverse primer 5′- CCC CAG TGT GTG GCC ATA TCT TCT T, and PCR products were cut using the restriction enzyme MspA1 I. To genotype the -863 C>A polymorphism, the forward primer 5’-GGC TCT GAG GAA TGG GTT and the reverse primer 5’- CTA CAT GGC CCT GTC TTC GTT ACG were used, and PCR products were cut using the restriction enzyme TaiI. To genotype the -1031 T>C polymorphism, the forward primer 5’-AGC AAG AGC TGT GGG GAG AA and the reverse primer 5’-CCT GTA ACC CAT TCC TCA GAG CC were used, and PCR products were cut using the restriction enzyme BbsI. These primers and restriction enzymes are shown at Table 1.

Table 1 Used primer and restriction enzyme at each polymorphism.
PolymorphismsForward primerReverse primerRestriction enzyme1
-238 G>A5’-AGA AGA CCC CCC TCG GAA CC2-3’5’-ATC TGG AGG AAG CGG TAG TG-3'MspI
-308 G>A5’-AGG CAA TAG GTT TTG AGG GCC AT-3'5’-TCC TCC CTG CTC CGA TTC CG-3'NcoI
-857 C>T5′-AAG TCG AGT ATG GGG ACC CCC CGT TAA-3'5′-CCC CAG TGT GTG GCC ATA TCT TCT T-3'AseI
-863 C>A5'-GGC TCT GAG GAA TGG GTT5'-CTA CAT GGC CCT GTC TTC GTT ACG-3'MnlI
-1031 T>C5’-AGC AAG AGC TGT GGG GAG AA-3'5’-CCT GTA ACC CAT TCC TCA GAG CC-3'BbsI
1All of the restriction enzymes were available from New England Biolabs (MA, United States) and we used the reaction conditions recommended by the instructions;
2The underlined bases in the primer were mismatched with the wild-type sequence in order to introduce the restriction enzyme site.

The five polymorphic regions were amplified using the following PCR conditions: 95 °C for 5 min, 38 cycles of denaturing at 95 °C for 30 s, annealing at 60 °C for 30 s, extension at 72 °C for 30 s, and a final extension at 72 °C for 5 min. Digestion with the appropriate restriction enzymes was performed at 37 °C for 16 h, as described by the manufacturer (New England BioLabs, Beverly, MA, United States).

Statistical analysis

We used χ2 tests to analyze baseline categorical variables and Mann-Whitney tests to analyze baseline continuous variables. Associations between TNF-α polymorphisms and HCC were estimated using adjusted odds ratios (AORs) and 95%CIs obtained from multiple logistic regression models adjusted for age, sex, hypertension, diabetes mellitus, body mass index, smoking status, and drinking status. The informations about hypertension, diabetes, smoking status and drinking status were obtained by questionnaires.

Survival time was calculated from the date of HCC diagnosis to the date of death or last follow-up. Survival analysis was performed using the Kaplan-Meier method, the log-rank test, and the Cox-proportional hazards regression model. The statistical significance level of all tests was set at P < 0.05. Analyses were performed using GraphPad Prism 4.0 (GraphPad Software Inc., San Diego, CA, United States) and Medcalc version 11.1.1.0 (Medcalc Software, Mariakerke, Belgium).

RESULTS
Study sample

Baseline characteristics of HCC cases and controls are shown in Table 2. The mean age of HCC cases was 56 years, and 120 were male (76.4%). HCC cases and controls were matched on age and sex (P = 0.069 and 0.570, respectively). Compared with controls, HCC cases were less likely to have hypertension (P = 0.002). However, no significant differences in obesity (BMI > 25 kg/m2) or in the prevalence of diabetes mellitus, smoking, or drinking were identified between cases and controls. HBV and HCV infections were identified in 125 (79.6%) and 16 (10.2%) HCC cases, respectively. Of the HCC cases, 12 (7.6%) underwent surgical resection. The Okuda stage distribution was as follows: stage I, 46 (29.3%); stage II, 68 (43.3%); and stage III, 43 (27.4%).

Table 2 Baseline characteristics of study sample n (%).
VariableCasesControlsP value1
n157201
Age (yr, mean ± SD)56.00 ± 11.0654.00 ± 11.220.061
Sex (male, %)120 (76.4)148 (73.6)0.871
Hypertension19 (12.1)50 (24.9)0.012
Diabetes mellitus30 (19.1)26 (12.9)0.195
BMI > 25 kg/m240 (25.5)51 (24.9)1.000
Smoking84 (53.5)78 (38.8)0.106
Drinking90 (57.3)93 (46.3)0.274
Tumor size
< 5 cm68 (43.3)--
≥ 5 cm89 (56.7)--
Portal vein thrombosis
No92 (58.6)--
Yes65 (41.4)--
Surgical resection
No145 (92.4)--
Yes12 (7.6)--
CTx/RTx
No27 (17.2)--
Yes130 (82.8)--
TNM stage
I34 (21.7)--
II37 (23.5)--
III51 (32.5)--
IV35 (22.3)--
Okuda stage
I46 (29.3)--
II68 (43.3)--
III43 (27.4)--
CTP class
A83 (52.9)--
B36 (22.9)--
C38 (24.2)--
1Derived from χ2 tests for categorical data and Mann-Whitney tests for continuous data. BMI: Body mass index; CTx: Chemotherapy; RTx: Radiotherpay; CTP: Chlid-Turcotte-Pugh.
Genotype frequencies of the TNF-α -1031 T>C, -863 C>A, -857 C>T, -308 G>A, and -238 G>A polymorphisms

The genotype distributions of the TNF-α -1031 T>C, -863 C>A, -857 C>T, -308 G>A, and -238 G>A polymorphisms in HCC cases, HCC cases with HBV, and controls are shown in Table 3. We found no significant differences in the genotype frequencies of the TNF-α -1031 T>C, -863 C>A, -857C>T, -308 G>A, or -238 G>A polymorphisms between cases and controls. We also found no significant difference in genotype frequencies of these polymorphisms between HCC cases with HBV and controls.

Table 3 Genotype frequencies and hepatocellular carcinoma adjusted odd ratios for the TNF-α -1031 T>C, -863 C>A, -857 C>T, -308 G>A, and -238 G>A polymorphisms in hepatocellular carcinoma cases and controls n (%).
CharacteristicsControls, n = 201HCC cases
HCC cases with HBV
Cases, n = 157AOR (95%CI)1P-valueFDR-P-valueCases, n = 125AOR (95%CI)1P-valueFDR-P-value
TNF-α -1031 T>C, rs1799964
TT121 (60.2)99 (63.1)1.000 (reference)73 (58.4)1.000 (reference)
TC70 (34.8)47 (29.9)0.796 (0.487-1.301)0.3620.58642 (33.6)0.922 (0.550-1.544)0.7560.960
CC10 (5.0)11 (7.0)1.308 (0.498-3.436)0.5860.58610 (8.0)1.724 (0.628-4.729)0.2900.580
Dominant (TT vs TC + CC)0.860 (0.540-1.369)0.5240.5861.013 (0.622-1.650)0.9600.960
Recessive (TT + TC vs CC)1.393 (0.540-3.595)0.4930.5861.745 (0.649-4.693)0.2700.580
HWE-P0.9760.1120.268
TNF-α -863 C>A, rs1800630
CC129 (64.2)98 (62.4)1.000 (reference)74 (59.2)1.000 (reference)
CA62 (30.8)53 (33.8)1.154 (0.709-1.878)0.5650.67246 (36.8)1.284 (0.767-2.150)0.3410.750
AA10 (5.0)6 (3.8)0.784 (0.255-2.414)0.6720.6725 (4.0)0.825 (0.253-2.690)0.7500.750
Dominant (CC vs CA + AA)1.109 (0.695-1.768)0.6660.6721.226 (0.749-2.007)0.4180.750
Recessive (CC + CA vs AA)0.734 (0.243-2.222)0.5840.6720.760 (0.238-2.428)0.6430.750
HWE-P0.4770.7230.513
TNF-α -857 C>T, rs1799724
CC142 (70.6)116 (73.9)1.000 (reference)92 (73.6)1.000 (reference)
CT53 (26.4)35 (22.3)0.841 (0.493-1.432)0.5230.69729 (23.2)0.840 (0.477- 1.478)0.5450.893
TT6 (3.0)6 (3.8)1.816 (0.428-7.714)0.4190.6974 (3.2)1.110 (0.226- 5.438)0.8980.893
Dominant (CC vs CT + TT)0.930 (0.558-1.548)0.7800.780.888 (0.516-1.531)0.6700.893
Recessive (CC + CT vs TT)2.091 (0.494-8.860)0.3170.6971.500 (0.312-7.203)0.6120.893
HWE-P0.6980.1200.371
TNF-α -308 G>A, rs1800629
GG181 (90.0)133 (84.7)1.000 (reference)108 (86.4)1.000 (reference)
GA18 (9.0)23 (14.6)1.949 (0.940- 4.040)0.0730.17817 (13.6)1.779 (0.821-3.853)0.1440.430
AA2 (1.0)1 (0.6)0.936 (0.075-11.646)0.9590.9590 (0.0)N/A0.9950.995
Dominant (GG vs GA + AA)1.841 (0.911-3.720)0.0890.1781.610 (0.758-3.419)0.2150.430
Recessive (GG + GA vs AA)0.861 (0.069-10.734)0.9080.959N/A0.9950.995
HWE-P0.0570.9960.415
TNF-α -238 G>A, rs 361525
GG180 (89.6)130 (82.8)1.000 (reference)104 (83.2)1.000 (reference)
GA20 (10.0)26 (17.6)1.634 (0.821-3.251)0.1620.32420 (16.0)1.491 (0.713-3.117)0.2880.576
AA1 (0.5)1 (0.6)N/A0.9930.9941 (0.8)N/A0.9930.993
Dominant (GG vs GA + AA)1.732 (0.876-3.424)0.1150.3241.614 (0.780-3.340)0.1970.576
Recessive (GG + GA vs AA)N/A0.9940.994N/A0.9930.993
HWE-P0.5870.8070.972
1Adjusted for age, sex, hypertension, diabetes mellitus, drinking status, and smoking status. HCC: Hepatocellular carcinoma; AOR: Adjusted odd ratios; HBV: Hepatitis B virus.
Associations between combinations of TNF-α polymorphisms and HCC

Next, we evaluated the combined effect of TNF-α polymorphisms on HCC risk. Using multiple logistic regression models, we found nine combined TNF-α genotypes associated with increased likelihood of HCC, as shown in Table 4. Some combinations showed marked association with HCC. The combinations were TNF-α -1031/-857/-238 TT/CC/GA (AOR = 18.849, 95%CI: 2.203-161.246, P = 0.007) TNF-α -1031/-308/-238 TT/GG/GA (AOR = 26.956, 95%CI: 3.071-236.584, P = 0.003) and TNF-α -1031/-238 TT/GA (AOR = 21.576, 95%CI: 2.581-180.394, P = 0.005).

Table 4 TNF-α genotype combinations in hepatocellular carcinoma cases and controls1n (%).
GenotypeHCC cases, n = 157Controls, n = 201AOR (95%CI)2P-value
TNF-α -1031/-857/-238
TT/CC/GG56 (35.7)81 (40.3)1.000 (reference)
TT/CC/GA11 (7.0)2 (1.0)18.849 (2.203-161.246)0.007
TNF-α -1031/-308/-238
TT/GG/GG68 (43.3)103 (51.2)1.000 (reference)
TT/GG/GA13 (8.3)2 (1.0)26.956 (3.071-236.584)0.003
TT/GA/GG17 (10.8)14 (7.0)2.712 (1.085-6.778)0.033
TNF-α -863/-308/-238
CC/GG/GG68 (43.3)99 (49.3)1.000 (reference)
CC/GA/GG16 (10.2)13 (6.5)2.533 (1.007-6.371)0.048
CA/GG/GA13 (8.3)5 (2.5)4.242 (1.243-14.473)0.021
TNF-α -1031/-238
TT/GG86 (54.8)119 (59.2)1.000 (reference)
TT/GA13 (8.3)2 (1.0)21.576 (2.581-180.394)0.005
TNF-α -863/-238
CC/GG85 (54.1)114 (56.7)1.000 (reference)
CA/GA13 (8.3)5 (2.5)3.669 (1.098-12.253)0.035
TNF-α -308/-238
GG/GG107 (68.2)160 (79.6)1.000 (reference)
GA/GG23 (14.6)18 (9.0)2.283 (1.078-4.836)0.031
GA+AA/GG24 (15.3)20 (10.0)2.150 (1.041-4.441)0.039
1Only combinations significantly associated with HCC are presented in the table;
2Adjusted for age, sex, hypertension, diabetes mellitus, drinking status, and smoking status. HCC: Hepatocellular carcinoma.
Haplotype frequencies of TNF-α polymorphisms

We then calculated haplotype frequencies to attain more comprehensive information about the association between TNF-α and HCC. TNF-α -1031 T>C, -863 C>A, -857 C>T, -308 G>A, and -238 G>A haplotype frequencies in HCC cases and controls are shown in Table 5. The TNF-α -1031/-863/-857/-308/-238 T-C-C-G-A haplotype was significantly associated with HCC (OR = 25.824, 95%CI: 1.491-447.223, P = 0.0005). Other haplotypes significantly associated with HCC included TNF-α -1031/-857/-308/-238 T-C-G-A (OR = 12.059, 95%CI: 2.747-52.950, P < 0.0001), TNF-α -1031/-857/-238 T-C-A (OR = 10.696, 95%CI: 2.428-47.110, P = 0.0001), TNF-α -1031/-308/-238 T-G-A (OR = 7.556, 95%CI: 2.173-26.280, P = 0.0002), and TNF-α -1031/-238 T-A (OR = 10.865, 95%CI: 2.473-47.740, P = 0.0001).

Table 5 TNF-α -1031 T>C, -863 C>A, -857 C>T, -308 G>A, and -238 G>A haplotypes in hepatocellular carcinoma cases and controls1.
HaplotypeOverallControlCaseOR (95%CI)P-value
TNF-α -1031/-863/-857/-308/-238
T-C-C-G-G0.52660.53990.51391.000 (reference)
T-C-C-G-A0.01190.00000.028925.824 (1.491-447.223)0.0005
T-C-C-A-G0.05820.04860.06471.428 (0.749-2.723)0.320
T-C-T-G-G0.13340.14350.12320.891 (0.564-1.407)0.645
T-C-T-A-G0.00560.00400.00721.360 (0.190-9.764)1.000
T-A-C-G-G0.01710.02100.00000.080 (0.005-1.396)0.023
T-A-C-G-A0.01090.00250.02264.761 (0.976-23.230)0.043
T-A-C-A-G0.00100.00000.00666.796 (0.324-142.621)0.181
T-A-T-G-G0.01230.01210.01331.088 (0.288-4.118)1.000
T-A-T-A-G0.00090.00220.00000.453 (0.018-11.201)1.000
C-C-C-G-G0.01330.01030.01622.176 (0.699-6.778)0.254
C-C-C-G-A0.04140.04980.03180.605 (0.257-1.425)0.306
C-C-T-G-A0.00420.00090.00666.796 (0.324-142.600)0.181
C-A-C-G-G0.16310.16380.16461.088 (0.717-1.652)0.749
TNF-α -1031/-857/-308/-238
T-C-G-G0.54300.56370.51051.000 (reference)
T-C-G-A0.02350.00600.053112.059 (2.747-52.950)< 0.0001
TNF-α -1031/-857/-238
T-C-G0.60260.61280.58541.000 (reference)
T-C-A0.02310.00600.051710.696 (2.428-47.110)0.0001
TNF-α -1031/-308/-238
T-G-G0.68850.71870.64881.000 (reference)
T-G-A0.02380.00630.05187.556 (2.173-26.280)0.0002
TNF-α -1031/-238
T-G0.75460.77380.72971.000 (reference)
T-A0.02330.00620.050510.865 (2.473- 47.740)0.0001
1Only data for haplotypes significantly associated with hepatocellular carcinoma are presented in the table. Haplotypes with frequencies of less than zero among cases or controls are not shown.
Cox regression analysis of HCC case survival

A stepwise Cox regression analysis of HCC-related survival is shown in Table 6. Survival in HCC cases was associated with sex, history of chemotherapy or radiotherapy, portal vein thrombosis, and TNF-α -1031 polymorphism status.

Table 6 Results of stepwise Cox regression analysis of hepatocellular carcinoma survival.
CovariateβSEMHR (95%CI)P value
Sex-1.3180.4800.268 (0.105-0.682)0.006
Chemotherapy or radiotherapy-1.9140.5000.148 (0.056-0.391)0.0001
Portal vein thrombosis1.3340.4783.795 (1.495-9.631)0.005
TNF-α -1031 TT vs CC1.7720.7335.881 (1.408-24.554)0.016
TNF-α polymorphisms and HCC case survival stratified by stage

TNF-α polymorphism-related survival was analyzed in HCC cases stratified by TNM and Okuda stage. Survival of cases with the TNF-α -1031 wild type (TT) genotype or a single T>C polymorphism was significantly better than those with the CC genotype (regression coefficient = 1.772, HR = 5.881, 95%CI: 1.408-24.554, P = 0.016), as shown in Figure 1 and Table 7. Other TNF-α polymorphisms did not affect HCC case survival at any TNM or Okuda stage.

Figure 1
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Figure 1 Survival curves for hepatocellular carcinoma Okuda stage III cases with the TNF-α-1031 (rs1799964) TT genotype (reference) and the CC genotype.
Table 7 TNF-α genotypes and survival in Okuda stage III hepatocellular carcinoma cases.
GenotypeValidation set
Adjusted HR (95%CI)1P-value
Cases (n = 43)Deaths (n = 41)
TNF-α -1031 T>C, rs1799964
TT29 (67.4)27 (65.9)1.000 (reference)
TC11 (25.6)11 (26.8)1.314 (0.448-3.856)0.621
CC3 (7.0)3 (7.3)5.795 (1.145-29.323)0.035
Dorminant model (TT vs TC + CC)1.805 (0.733-4.442)0.201
Recessive model (TT + TC vs CC)3.761 (0.869-16.265)0.078
1Adjusted for age, sex, hypertension, diabetes mellitus, drinking status, smoking status, portal vein thrombosis, tumor size, surgical resection, and chemotherapy or radiotherapy.
DISCUSSION

We performed this case-control study to investigate the associations between the TNF-α -1031 T>C, -863 C>A, -857 C>T, -308 G>A, and -238 G>A polymorphisms and HCC. Furthermore, we analyzed TNF-α polymorphism combinations and haplotypes. In this study, the TNF-α -1031 T>C, -863 C>A, -857 C>T, -308 G>A, and -238 G>A polymorphisms were not associated with HCC risk. This result is inconsistent with the findings of previous meta-analyses. An insufficient number of HCC cases and controls in our study could be the reason for this discordance; for example, we were able to analyze only 18 TNF-α -308 GA controls and 23 cases and 2 TNF-α -308 AA controls and 1 HCC case.

Past studies have analyzed combined genotypes or haplotypes to attain a more comprehensive understanding of the association between various polymorphisms and diseases[22,23]. In this study, we found significant associations between some TNF-α genotype combinations and HCC risk. All of the statistically significant genotype combinations included the GA genotype at TNF-α -238 or -308. The TNF-α -863 CA genotype accompanied by the TNF-α -238 GA genotype was also associated with increased HCC risk in some combinations. This result suggests that the TNF-α -238 GA and -308 GA genotypes increase HCC risk in specific genotype combinations. The TNF-α -863 CA genotype accompanied by the TNF-α -238 GA genotype was associated with increased HCC risk, but the TNF-α -863 CA genotype was not associated with increased HCC risk when accompanied by other genotype combinations. This suggests that the TNF-α -863 polymorphism increases the risk of HCC only in the presence of the TNF-α -238 GA genotype.

Associations between TNF-α haplotypes and various medical conditions, such as polycystic ovary syndrome (PCOS)[24], bladder cancer[25], gastric carcinoma[26,27], peptic ulcer[28], and anemia[29] have been reported. Chen et al[30] reported that the TNF-α -1031/-863/-857/-308/-238 T-C-C-G-A haplotype may account for decreased susceptibility to HCC. However, we found this haplotype was more common in HCC patients. All haplotypes significantly associated with HCC contained the TNF-α -238 A allele, suggesting it may play a role in HCC development. The HCC odds ratio for TNF-α haplotype -1031/-863/-857/-308/-238 T-A-C-G-G was 0.080, while the OR for haplotype T-A-C-G-A, in which the -238 allele changed from G to A, was 4.716. This result supports the hypothesis that the -238 A allele is associated with HCC risk, though the HCC odds ratio for haplotype T-A-C-G-A was not statistically significant.

To the best of our knowledge, no study has reported an association between HCC prognosis and TNF-α polymorphisms. TNF-α acts like a double-edged sword via its two distinct receptors: TNF receptor 1 (TNFR-1) and receptor 2 (TNFR-2)[31,32]. The major difference between the two receptors is the death domain in TNFR-1 absent in TNFR-2. On the one hand, TNFR-1 plays an important role in apoptotic cell death. On the other hand, TNF-α can stimulate the growth, proliferation, and angiogenesis of cancer cells by activating nuclear factor NF-κB[32]. Nakazaki et al[33] reported higher levels of TNF-α in patients with recurrent HCC than in patients without HCC recurrence or patients with metastatic liver carcinoma or gastrointestinal carcinoma. Liu et al[34] have reported that TNF-α overexpression is related to poor differentiation and microvascular invasion in HCC. Our study raises the possibility that specific TNF-α polymorphisms are related to HCC patient prognosis. The TNF-α polymorphism associated with treatment outcomes in our study (TNF-α -1031) may potentially be used in the clinic as a surrogate biomarker of prognosis.

In conclusion, although we found no direct association between TNF-α polymorphisms and HCC risk, some TNF-α genotype combinations and haplotypes were associated with HCC. In addition, HCC patients with the TNF-α -1031 TT genotype had a better prognosis than those with the CC genotype. An important limitation of our study was the small sample size, which prevents us from drawing definitive conclusions. Therefore, our results should be interpreted cautiously. However, to the best of our knowledge, ours is the first study to analyze the association between these five TNF-α polymorphisms, as well as their combinations and haplotypes, and HCC case status and prognosis. Our findings provide a more comprehensive understanding of TNF-α polymorphisms and HCC. Further studies with sufficient sample size are needed to clarify the role of TNF-α polymorphisms in HCC risk and prognosis.

COMMENTS
Background

Tumor necrosis factor alpha (TNF-α) is a pro-inflammatory cytokine that plays a role in inflammatory pathways leading to tumorigenesis. Some TNF-α polymorphisms have been found to be associated with hepatocellular carcinoma (HCC) susceptibility.

Research frontiers

Some TNF-α polymorphisms have been considered to have association with the susceptibility of HCC in many studies. But not all the five TNF-α polymorphisms are sufficiently studied and some of them are controversial. Thus to elucidate accurate genetic risk factors for HCC is important. Genetic factors affecting prognosis in patients with HCC is also important research area.

Innovations and breakthroughs

As far as I know, this study is first that analyzed the association between all the five TNF-α polymorphisms, as well as their combinations and haplotypes, and HCC. So it can provides more comprehensive understandings of TNF-α polymorphisms and HCC. Furthermore, our study raises the possibility that specific TNF-α polymorphisms are related to HCC patient prognosis.

Applications

Analyzing TNF-α polymorphisms in patients with hepatitis or cirrhosis may help predicting the risk of HCC in individual patient. And TNF-α -1031 may potentially be used in the clinic as a surrogate biomarker of prognosis.

Peer-review

It’s a case-control study investigating the associations between the TNF-α polymorphisms and HCC with analysis of TNF-α polymorphism combinations and haplotypes. In this study, although no direct association between TNF-α polymorphisms and HCC risk was found, some TNF-α genotype combinations and haplotypes were associated with HCC. A significant association was find between some TNF-α genotype combinations and HCC risk particularly the TNF-α -238GA and -308GA genotypes, and the TNF-α -863 polymorphism increases the risk of HCC only in the presence of the TNF-α -238 GA genotype.

Footnotes

P- Reviewer: Berkane S S- Editor: Ma YJ L- Editor: A E- Editor: Zhang DN

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