ezh2 genetic variants affect risk of gastric cancer in the chinese han population
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MOLECULAR CARCINOGENESIS
EZH2 Genetic Variants Affect Risk of GastricCancer in the Chinese Han Population
Yuan Zhou,1,2 Wei-Dong Du,1,3,4,5* Qiang Wu,3 Yi Liu,6 Gang Chen,4 Jian Ruan,1,3 Song Xu,1,3
Feng Yang,3 Fu-Sheng Zhou,4 Xian-Fa Tang,4 Hua-Yang Tang,4 Xian-Bo Zuo,4 Feng-Yu Zhang,4
Liang-Dan Sun,4 and Xue-Jun Zhang4
1Key Lab of Genome Research of Anhui Province, Anhui Medical University, Hefei, China2Department of Biology, Anhui Medical University, Hefei, China3Department of Pathology, Anhui Medical University, Hefei, China4State Key Laboratory Incubation Base of Dermatology, Ministry of National Science and Technology, Anhui MedicalUniversity, Hefei, China5Sektion Experimentelle Anaesthesiologie, Universitaetsklinikum Ulm, Ulm, Germany6Department of Surgery, The First Affiliated Hospital of Anhui Medical University, Hefei, China
Enhancer of zeste 2 (EZH2) gene encodes a histone methyltransferase that constitutes the catalytic component ofthe polycomb repressive complex-2 (PRC2) to initiate epigenetic silencing of genes. It is reported that the expression
level of EZH2 in gastric cancer tissue was highly correlated with tumor progression, however, whether EZH2 geneticvariants were associated with the risk of gastric cancer remains yet unknown. In this study, we conducted a genotyp-ing analysis for EZH2 in 311 cases of gastric cancer and 425 controls from the Chinese Han population. We found fivesingle nucleotide polymorphisms (SNP; rs12670401, rs6464926, rs2072407, rs734005, and rs734004) of EZH2 gene
were significantly associated with the risk of gastric cancer. Of which, the rs12670401 with the minor allele C andrs6464926 with the minor allele T revealed strong associations with increased gastric cancer risk [P ¼ 0.009, adjustedodds ratio (aOR) ¼ 1.327, 95% CI ¼ 1.075–1.683 and P ¼ 0.012, aOR ¼ 1.310, 95% CI ¼ 1.059–1.619]. The other
three SNPs, rs2072407, rs734005, and rs734004 contributed to significantly reduced risk of gastric cancer (P ¼ 0.033,aOR ¼ 0.787, 95% CI ¼ 0.633–0.981, P ¼ 0.045, aOR ¼ 0.799, 95% CI ¼ 0.642–0.995 and P ¼ 0.048, aOR ¼0.803, 95% CI ¼ 0.645–0.999), respectively. We further found that rs12670401 and rs6464926 were in a strong LD
while rs2072407, rs734005, and rs734004 were in another. Haplotype analysis of the five SNPs showed that haplo-type CCTCT reduced the risk of gastric cancer (P ¼ 0.031 and aOR ¼ 0.784), while haplotype GTCTC significantlyelevated the risk of gastric cancer (P ¼ 0.011 and aOR ¼ 1.310). We concluded that EZH2 variants were significantly
associated with gastric cancer risk. Our results for the first time provided new insight into susceptibility factors ofEZH2 gene variants in carcinogenesis of gastric cancer of the Chinese Han population. � 2012 Wiley Periodicals, Inc.
Key words: EZH2; gastric cancer; single nucleotide polymorphism
INTRODUCTION
Gastric cancer is a major health condition withlimited treatment options and poor prognosis. Itcauses about 800,000 deaths worldwide per year[1]. Despite the complexity of cancer development,both gene mutation and environment factor bearequally influential forces in carcinogenesis of thisentity.Polycomb group (PcG) proteins are epigenetic
chromatin modifiers that contribute to cancerdevelopment. Three PcG proteins, enhancer ofzeste 2 (EZH2), embryonic ectoderm development(EED), and suppressor of zeste 12 homolog(SUZ12), comprise the core of polycomb repressivecomplex-2 (PRC2) [2,3]. EZH2, also called histone–lysine N-methyltransferase (HKMT), is an enzymethat plays a crucial role in initiating silencing oftarget genes [4,5]. EZH2 contains a SET domainthat has histone methyltransferase (HMT) activity
and acts mainly as a gene silencer, adding threemethyl groups to lysine 27 of histone 3 (H3K27).The methylation of H3K27 by EZH2 results in therecruitment of PRC1. PCR1 and PCR2 cooperatewith each other in gene silencing [6–8]. Overex-pression of EZH2 is associated with poor prognosis
Abbreviations: PcG, Polycomb group; EZH2, enhancer of zeste 2;EED, embryonic ectoderm development; SUZ12, suppressor ofzeste 12 homolog; PRC2, polycomb repressive complex-2; HKMT,histone–lysine N-methyltransferase; HMT, histone methyltransfer-ase; H3K27, lysine 27 of histone 3; SNP, single nucleotide polymor-phism; HWE, Hardy–Weinberg equilibrium; OR, odds ratio; aOR,adjusted odds ratio; DNMT, DNA methyltransferase.
*Correspondence to: Key Lab of Genome Research of AnhuiProvince, Anhui Medical University, Meishan Road 81, Hefei230032, China.
Received 1 June 2011; Revised 9 December 2011; Accepted 12December 2011
DOI 10.1002/mc.21871
Published online in Wiley Online Library(wileyonlinelibrary.com).
� 2012 WILEY PERIODICALS, INC.
or increased cancer risk in a variety of epithelialcell-derived digestive tumors, such as oesophaguscancer [9], gastric cancer [2,10,11], colorectalcancer [12], hepatocellular carcinoma liver [13],pancreatic ductal adenocarcinoma [14], and blad-der cancer [15] in the both preclinical and clinicalmodels [16,17]. In gastric cancer, EZH2 acts as anoncogene. High EZH2 expression is correlated withKi-67 and p53 expressions and is significantlyassociated with distant metastases and non-signetring cells [2]. The single nucleotide polymorphisms(SNPs) associated with worse prognosis wouldbecome predictive of higher EZH2 expression.
The domain structure of EZH2 and mutationssites have been displayed in the previous investiga-tions [18,19]. Both the C-terminal SET domainand the adjacent cysteine-rich CXC domain arerequired for HMT activity [6,20,21]. Missense, in-frame deletion and splice mutation of the EZH2domain attribute to loss function of the gene.The EZH2 mutations might occur in monoallelicor biallelic states [22]. The truncating mutationsdistributed throughout the gene, whereas the mis-sense mutations mostly targeted evolutionarilyhighly conserved residues that were located indomain II and the CXC-SET domains. Thus, mostof the frame-shift and truncating mutations wereinactivating. Furthermore, Western blotting datarevealed an almost complete absence of H3K27me3in the EZH2-mutant ELF-153 and SKM-1 cell lines[18,22,23].
A number of SNPs within the EZH2 gene are as-sociated with the susceptibility or outcomes tocancers. A recurring monoallelic EZH2 point muta-tion (Tyr641) in the SET domain was described inlymphoma [23]. The altered tyrosine correspondedto a key residue in the active site of the EZH2 pro-tein, leading to reduced enzymatic activity. Thisevidence was in consistence with the previousfunctional observation of a comparable mutationin the Drosophila E (z) ortholog [24]. PRC2 com-plexes containing mutated EZH2 protein reducedH3K27 trimethylation activity in vitro [23]. Thewild-type copy of EZH2 was present in all the sam-ples with Tyr641-altering mutations and presenceof both alleles was also detected in the mutantsamples profiled by transcriptome sequencing [23].Mutant and wild-type gene products cooperate toincrease H3K27trimeth in neoplastic cells [25].Increasing impression was in that variants of EZH2gene influenced development and consequenceof cancers. Breyer et al. [26] found rs2302427(D185H) of EZH2 had a minor allele frequency of3.7% in cases and 5.2% in controls, conferringsignificantly reduced risk of prostate cancer in aheterozygote manner (P ¼ 0.0085, OR ¼ 0.63).Bachmann et al. [27] conducted a mutation screenthrough EZH2 gene in hereditary prostate cancer.They observed 8 haplotypes with frequency of
>0.01, 1 of the haplotypes was significantly lessfrequent in familial cases than in controls[27].In addition, Yoon et al. [19] demonstratedEZH2 genetic polymorphisms rs6950683 andrs3757441 contribute to significant associationswith reduced lung cancer risk, indicating protec-tive effects of the variants on lung cancer risk. Sim-ilarly, EZH2 variants were associated with a poorprognosis of myeloid disorders [22] and myelodys-plastic syndromes [18]. More recently, one allelicgenotype of rs3757441 (C/C vs. C/T or T/T) ofEZH2 gene was observed being significantly associ-ated with shorter PFS and OS in colorectal cancer[28]. However, association study of genetic variantsin EZH2 and gastric cancer susceptibility remainsyet absent.We addressed the hypothesis that genetic varia-
tions in EZH2 might contribute to the susceptibili-ty to gastric cancer. Thus, we performed a geneticanalysis for the EZH2 variants in a case–control studyand investigated potential associations of thesevariants with biological behaviors of gastric cancer.
MATERIALS AND METHODS
Study Population
This study was a hospital-based case–controlstudy. Patients with gastric cancers (n ¼ 311) werecollected from the First Affiliated Hospital ofAnhui Medical University between March 2008and July 2009 and received no preoperative che-motherapy or radiotherapy before surgical gastrec-tomy. The patients were comprised 246 men and65 women with an average age of 60.4 � 10.4 yr(range, 24–83 yr). In addition, a total of 336 menand 89 women control subjects were matched withan average age of 60.6 � 8.4 yr (range, 30–86 yr).These control subjects without a history of cancerswere recruited from patients who visited hospitalfor a conventional cancer-screening program. In-formation on demographic characteristics, such asgender, age, smoking habits, alcohol consumption,and family history of cancer were obtained from apersonal interview administered by trained person-nel. Smoking habit was defined as non-smoker andsmoker. Individuals who smoked one cigarette perday for over 1 yr were defined as smokers. Alcoholconsumption was defined as non-drinker and drinker.Individuals who consumed more than 200 mL al-cohol per day were defined as drinker. There wasno significant difference in the distribution of age,gender, smoking, and drinking (P > 0.05, data notshown). All the subjects tested were Chinese Hanfrom the same geographic regions of China. In-formed consents were obtained from all the partic-ipants. This study was approved by the ethicscommittee for genome research of the Anhui Med-ical University of China and was conductedaccording to the Declaration of Helsinki Principles.
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METHODS
Extraction of Peripheral Blood DNA
Blood sample was collected from each subject inEDTA and stored at �808C.Genomic DNA wasextracted from peripheral blood by using QIAampDNA Blood Midi Kit (Qiagen Inc., Hilden, Germany)according to the manufacturer’s protocol. The con-centration of DNA was measured by the NanodropSpectrophotometer (ND-1000, Wilmington, DE) offull wavelength and standardized to 50 ng/mL.
SNP Selection and Sequenom Assay
We first checked the SNP genotype data of EZH2gene in the Chinese Han from InternationalHapMap Project website (http://hapmap.ncbi.nlm.nih.gov/). The data were then formatted by Haplo-view software. The SNPs rs6950683 and rs2303427of EZH2 with regard to the association with risk oflung [19] and prostate cancer [26] were excludedfor further analysis because the SNP rs6950683 wascompletely absent in the Chinese population,while the MAF of SNP rs2303427 was only up to0.011 in the Chinese population HapMap database.Thus, a total of 25 SNPs of the EZH2 gene werefinally selected in this study with the MAF > 0.05and were in Hardy–Weinberg equilibrium (HWE).
Fifteen nanograms of genomic DNA was used togenotype each sample. Locus-specific PCR and de-tection primers were designed using the MassAR-RAY Assay Design 3.0 software (Sequenom, SanDiego, CA) at the Key Laboratory of Dermatologyat Anhui Medical University, Ministry of Educa-tion, China, following the manufacturer’s instruc-tions. The DNA samples were amplified bymultiplex PCR reactions, and the PCR productswere then used for locus-specific single-base exten-sion reactions. The resulting products weredesalted and transferred to a 384-element Spectro-CHIP array. Genotyping analysis of the SNPs forfast-track validation analysis was performed usingthe Sequenom MassArray system with MALDI-TOFMS for allele detection. Genotyping quality wasexamined by a detailed QC procedure consistingof >95% successful call rate, duplicate calling ofgenotypes, internal positive control samples,and HWE testing. The mass spectrograms were an-alyzed by the MassARRAY Typer software (Seque-nom, San Diego, CA).
Data Analysis
We used a logistic regression model while con-trolling for age and gender as covariates to analyze(1) association of EZH2 polymorphisms with the
Table 1. Analysis of EZH2 Polymorphisms Associated With the Risk of Gastric Cancer
SNPNo. SNP rs# Alleles Position
HWE MAF
P-value OR (95% CI)Controls Cases Controls Cases
22 rs12670401 T ! C 148193868 1.000 0.134 0.392 0.461 0.009 1.327 (1.075,1.683)14 rs6464926 C ! T 148149944 0.836 0.246 0.383 0.449 0.012 1.310 (1.059–1.619)6 rs2072407 C ! T 148139766 0.677 0.433 0.372 0.318 0.033 0.787 (0.633–0.981)2 rs734005 T ! C 148136797 0.678 0.303 0.376 0.325 0.045 0.799 (0.642–0.995)1 rs734004 G ! C 148136393 0.918 0.199 0.380 0.330 0.048 0.803 (0.645–0.999)7 rs2072408 C ! T 148139130 0.677 0.362 0.372 0.323 0.053 0.805 (0.646–1.003)3 rs740949 G ! A 148136997 0.755 0.436 0.370 0.323 0.063 0.812 (0.653–1.012)4 rs1544571 A ! G 148172594 0.605 0.159 0.377 0.330 0.065 0.815 (0.655–1.014)19 rs10274535 G ! A 148174458 0.680 0.158 0.378 0.332 0.069 0.817 (0.657–1.016)11 rs3779038 T ! C 148173755 0.605 0.159 0.377 0.331 0.072 0.819 (0.659–1.019)10 rs3779037 C ! T 148170256 0.757 0.126 0.376 0.331 0.074 0.820 (0.659–1.020)15 rs6959647 C ! T 148161651 0.919 0.129 0.379 0.334 0.076 0.822 (0.661–1.021)16 rs6975291 G ! C 148179326 0.678 0.202 0.376 0.331 0.076 0.821 (0.660–1.022)12 rs3807450 A ! C 148153202 0.677 0.199 0.372 0.329 0.083 0.824 (0.663–1.026)18 rs9691534 C ! T 148175852 0.757 0.126 0.376 0.332 0.085 0.826 (0.665–1.027)13 rs3807451 C ! T 148169555 0.678 0.159 0.376 0.332 0.088 0.827 (0.665–1.029)20 rs10274701 T ! C 148183389 0.759 0.127 0.377 0.342 0.162 0.856 (0.688–1.065)8 rs3735219 G ! A 148144400 0.785 0.021 0.232 0.202 0.167 0.837 (0.649–1.078)21 rs10488070 T ! C 148159803 0.505 0.091 0.241 0.217 0.284 0.873 (0.681–1.119)25 rs17171127 C ! T 148172919 0.684 0.060 0.235 0.212 0.301 0.876 (0.682–1.126)23 rs17171118 C ! T 148148237 0.356 0.191 0.244 0.222 0.346 0.888 (0.694–1.136)9 rs3757441 T ! C 148155685 0.126 0.348 0.257 0.238 0.399 0.902 (0.708–1.148)5 rs1880357 G ! C 148208543 0.681 0.059 0.231 0.212 0.400 0.898 (0.699–1.154)24 rs17171119 T ! G 148148389 0.295 0.109 0.246 0.229 0.454 0.911 (0.714–1.163)17 rs7785022 T ! C 148164317 0.534 0.011 0.379 0.370 0.730 0.961 (0.765–1.207)
The ORs (95% CI) and corresponding P-values were derived from an age and gender adjusted logistic regression. P-values <0.05were indicated in bold font.
EZH2 GENETIC VARIANTS AFFECT GASTRIC CANCER RISK 3
Molecular Carcinogenesis
Table
2.EZH2GenotypeDistributionsin
theControlandin
theGastricCancer
SNP
Genotype
Frequency
CodominantModel
DominantModel
RecessiveModel
Controls
GC
OR(95%
CI)
P-value
OR(95%
CI)
P-value
OR(95%
CI)
P-value
rs12670401
TT
157
96
11
1TC
202
138
1.117(0.800–1.560)
0.515
1.101(0.817–1.479)
0.121
CC
65
71
1.786(1.172–2
.723)
0.007
1.676(1.152–2
.437)
0.007
rs6464926
CC
161
98
11
1CT
196
140
1.173(0.842–1.635)
0.345
1.307(0.958–1.783)
0.092
TT
63
66
1.721(1.123–2
.638)
0.013
1.571(1.072–2
.303)
0.020
rs2072407
CC
164
146
11
1TC
202
128
0.712(0.520–0
.975)
0.034
0.710(0.527–0
.955)
0.024
TT
56
35
0.702(0.435–1.132)
0.147
0.835(0.532–1.310)
0.432
rs734005
TT
162
144
11
1TC
203
128
0.709(0.518–0
.972)
0.033
0.714(0.530–0
.961)
0.026
CC
57
37
0.730(0.456–1.169)
0.191
0.871(0.560–1.356)
0.541
rs734004
GG
161
142
11
1CG
201
126
0.711(0.518–0
.976)
0.035
0.717(0.532–0
.966)
0.029
CC
60
39
0.737(0.464–1.170)
0.195
0.978(0.569–1.353)
0.556
TheORs(95%
CI)andP-valueswere
derivedfrom
anageandgenderadjustedlogisticregression.P-values<0.05were
indicatedin
bold
font.DominantModel:(DD,Dd)versusdd.Recessive
Model:DDversus(Dd,dd).Dwastheminorallele
anddwasthemajorallele.
4 ZHOU ET AL.
Molecular Carcinogenesis
risk of gastric cancer; (2) comparison of EZH2genotypes; and (3) haplotype distributions in 311gastric cancers and 425 normal controls. Thosewith the frequency of <0.05 were ignored in theanalysis. Hardy–Weinberg proportion was tested incontrol samples to ensure genotyping quality. Forthe stratified association analysis, chi-squared testwas used through case-only logistic regressionanalyses, while if there was a number of genotype�5, Fisher’s exact test was used. All analyses forP-values were two-sided. The statistical softwareplink v1.07 (http://pngu.mgh.harvard.edu/purcell/plink/) and Stata/SE version 10 were used for statis-tical analyses (StataCorp LP, College Station, TX).The Haploview 4.2 was used to calculate the link-age disequilibrium.
RESULTS
Association Analysis of 25 SNPs of EZH2
The minor allele, P-values, and the estimatedodds ratios (OR) of the 25 SNPs of EZH2 gene inpatients with gastric cancer and in controls wereshown in Table 1. Five SNP polymorphisms(rs12670401, rs6464926, rs2072407, rs734005, andrs734004) of EZH2 were identified to be signifi-cantly associated with the risk of gastric cancer. Ofwhich, the rs12670401 with the minor allele Cand rs6464926 with the minor allele T showed
strong associations with increased gastric cancerrisk [P ¼ 0.009, adjusted OR (aOR) ¼ 1.327, 95%CI ¼ 1.075–1.683; and P ¼ 0.012, aOR ¼ 1.310,95% CI ¼ 1.059–1.619], while the rs2072407,rs734005 and rs734004 polymorphisms presentedsignificantly reduced risk of gastric cancer(P ¼ 0.033, aOR ¼ 0.787, 95% CI ¼ 0.633–0.981;P ¼ 0.045, aOR ¼ 0.799, 95% CI ¼ 0.642–0.995;and P ¼ 0.048, aOR ¼ 0.803, 95% CI ¼ 0.645–0.999, respectively). The effects of the five SNPswere further analyzed using alternative models,such as codominant, dominant, and recessivemodels (Table 2). The homozygous genotype CCof rs12670401 and homozygous genotype TT ofrs6464926 accounted for higher proportion incases and significantly elevated the risk of gastriccancer (P ¼ 0.007, aOR ¼ 1.786, 95% CI ¼ 1.172–2.723; and P ¼ 0.013, aOR ¼ 1.721, 95% CI ¼1.123–2.638), respectively. Conversely, the frequen-cies of heterozygous genotypes TC (rs2072407), TC(rs734005), and CG (rs734004) were significantlyhigher in controls, leading to reduced risk of gas-tric cancer (P < 0.05).
The Linkage Disequilibrium and Haplotypes Analysis
We performed linkage disequilibrium analysisand showed the LD plot in Figure 1. The SNPsrs12670401 and rs6464926 were in a strong LDand the SNPs rs2072407, rs734005, and rs734004
Figure 1. Pairwise linkage disequilibrium (r2) in the study population.
EZH2 GENETIC VARIANTS AFFECT GASTRIC CANCER RISK 5
Molecular Carcinogenesis
were within another. A haplotype analysis wasperformed further (Table 3). We found that thehaplotypes of EZH2 genes affected susceptibility togastric cancer. The haplotypes with either minoralleles of rs12670401 and rs6464926 or majoralleles of rs2072407, rs734005 and rs734004 signif-icantly elevated risk of gastric cancer, while thehaplotypes with either major alleles of rs12670401and rs6464926 or minor alleles of rs2072407,rs734005, and rs734004 conferred reduced risk ofgastric cancer. In combination with the 25 SNPs,we found Ht3 and Ht4 exhibited statistically signif-icant differences. Ht3 represented elevated riskof gastric cancer (P ¼ 0.049, aOR ¼ 1.230). Ht4reduced the risk of gastric cancer (P ¼ 0.050,aOR ¼ 0.701, Table 3), instead.
Association Analysis of the Five SNPs by ClinicalCharacteristics
We performed the stratified association analysiswith regard to the five SNPs in different clinicalvariables by gender, age, tumor location, tumorsize, histologic subtype, depth of invasion, lymphnode metastasis, TNM stage, smoking, alcoholdrinking, family history, and salted food. Theresults were summarized in Table 4. However,there were no associations of the five SNPs withthe clinical characteristics.
DISCUSSION
In this study, we performed a genetic associationanalysis of EZH2 variants with gastric cancer.We demonstrated that the five SNPs, rs12670401,rs6464926, rs2072407, rs34005, and rs734004,were significantly associated with gastric cancersusceptibility. To the best of our knowledge, thiswas the first study addressing EZH2 variants mightbe novel susceptibility markers linked to gastriccancer.
In this study, we observed that the rs12670401with the minor allele C and rs6464926 withthe minor allele T showed strong associations withincreased gastric cancer risk (P ¼ 0.009, aOR ¼1.327, 95% CI ¼ 1.075–1.683; P ¼ 0.012, aOR ¼1.310, 95% CI ¼ 1.059–1.619). The SNP rs12670401located near the transcriptional start position ofEZH2, according to the web-based SNP analysistool, TF search 1.3 [29]. The T to C change ofrs12670401 might affect predicted GATA-X tran-scription factors binding, resulting in directly acti-vating or repressing the expression of target genes.GATA family includes essential regulators, whichshare two highly conserved zinc fingers of theC2H2 type that mediate not only DNA bindingbut also the great majority of protein interactions.GATA factors typically bind to the elementA/TGATA A/G [30]. T allele may create a bindingsite for the GATA-X factors. Patients carrying theC/C genotype are lack of binding sites for this fac-tor. In patients carrying one T allele, EZH2 expres-sion may be inhibited by GATA-X factors. In C/Chomozygotes, EZH2 expression could be deregu-lated. We supposed that C allele of rs12670401failed to be targeted by GATA factors and attribut-ed to the development of gastric cancer. The SNPrs6464926 located in the intron region betweenexons 8 and 9, C to T change of the SNPrs6464926 may affect the binding activity of TFIID,which serves as the scaffold for assembly of the re-mainder of the transcription complex, and acts asa channel for regulatory signals [31]. In this study,we found that the minor allele T of rs6464926 con-ferred susceptibility with gastric cancer. We sup-posed that the effect of T allele might contributeto higher EZH2 expression. EZH2 and DNA meth-yltransferases (DNMTs) are physiologically andfunctionally linked to each other. EZH2 is neces-sary for DNMT binding and CpG methylation of
Table 3. Haplotype Distributions in 311 Gastric Cancers and 425 Controls
SNPs
Frequency
Haplotype OR P-valueControls Cases
snp14,22 0.385 0.450 TC 1.290 0.018snp14,22 0.614 0.549 CT 0.770 0.015snp1,2,6 0.375 0.321 CCT 0.788 0.034snp1,2,6 0.624 0.678 GTC 1.250 0.042snp1,2,6,14,22 0.387 0.458 GTCTC 1.310 0.011snp1,2,6,14,22 0.375 0.321 CCTCT 0.784 0.031snp1,2,6,14,22 0.238 0.220 GTCCT 0.897 0.404snp1-25 (Ht1) 0.258 0.242 CCAGGTTGCTCCTCTCCTACTTCTC 0.895 0.360snp1-25 (Ht2) 0.228 0.205 GTGACCCATCTACCCGTCGTCTTGT 0.840 0.194snp1-25 (Ht3) 0.391 0.459 GTGAGCCGTCTACTCGTCGTTCCTC 1.230 0.049snp1-25 (Ht4) 0.122 0.092 CCAGGTTGTTCCTCTCCTACTTCTC 0.701 0.050
The ORs and corresponding P-values were derived from an age and gender adjusted logistic regression. P-values <0.05 were indicat-ed in bold font.
6 ZHOU ET AL.
Molecular Carcinogenesis
Table
4.StratifiedAssociationAnalysisoftheFive
SNPsbyClinicalSubgroups
Parameter
rs734004
rs734005
rs2072407
rs6464926
rs12670401
CC
CG
GG
P-value
CC
TC
TT
P-value
CC
TC
TT
P-value
CC
CT
TT
P-value
CC
TC
TT
P-value
Gender
0.266
0.289
0.149
0.152
0.660
Male
29
98
116
28
99
118
119
99
27
73
113
55
60
110
72
Female
10
28
26
929
26
27
29
825
27
11
11
28
24
Age
0.178
0.521
0.403
0.305
0.986
�55
29
95
110
27
97
112
114
97
25
74
109
48
54
106
73
<55
10
31
32
10
31
32
32
31
10
24
31
18
17
32
23
Tumorlocation
0.530
0.414
0.599
0.423
0.478
Cardia
923
22
17
47
63
63
47
17
42
54
29
32
52
41
Antrum
627
35
627
35
35
27
621
32
14
15
33
20
Corpus
18
46
61
923
22
23
23
819
25
10
10
25
19
Tumorsize
(cm)
0.453
0.503
0.435
0.949
0.982
�521
51
61
20
52
62
62
53
19
47
55
30
32
58
45
<5
12
54
57
12
54
58
59
54
11
37
63
22
25
60
37
Histologictype
0.195
0.185
0.213
0.081
0.142
Tubularor
papillary
34
96
110
33
97
112
113
98
31
79
114
45
51
111
77
Others
213
18
212
18
18
12
28
13
11
11
13
8Depth
ofinvasion
0.828
0.559
0.667
0.801
0.797
T1
311
14
322
14
15
10
37
14
67
11
8T2
719
21
719
22
22
20
613
29
57
28
12
T3
26
74
89
25
75
90
90
76
24
65
80
43
45
83
63
Lymphnode
metastasis
0.372
0.302
0.229
0.202
0.202
N0
13
37
55
12
38
56
57
38
11
31
52
22
24
49
31
N1
17
50
50
17
50
51
51
51
16
38
48
29
32
49
36
N2
615
19
615
19
19
15
616
20
44
20
16
TNM
stage
0.447
0.388
0.328
0.867
0.661
Iþ
II15
49
62
14
50
63
64
50
13
38
63
24
28
60
37
IIIþ
IV21
57
65
21
57
66
66
58
20
49
62
31
32
64
48
Smoking
0.425
0.317
0.309
0.658
0.717
Nooroccasionally
14
62
67
13
63
69
70
63
12
42
69
31
33
68
41
Yes
22
60
68
22
60
68
69
60
21
48
69
31
34
68
47
Alcoholdrinking
0.854
0.956
0.794
0.751
0.674
Nooroccasionally
20
66
73
19
67
74
76
67
17
51
71
34
36
72
50
Yes
16
56
62
16
56
63
63
56
16
39
67
28
31
64
38
Family
history
0.103
0.114
0.138
0.621
0.762
No
36
111
119
35
112
121
123
112
33
82
127
54
59
125
80 (Continued)
EZH2 GENETIC VARIANTS AFFECT GASTRIC CANCER RISK 7
Molecular Carcinogenesis
target genes. Hyper-methylation of the GATA fam-ily promoter made the GATA gene expression si-lenced [32]. Candidate target genes of these GATAfactors were commensurately decreased in their ex-pression and also displayed methylated promoters[30]. On the other hand, we found that EZH2 SNPsrs2072407, rs734005, and rs734004 presented pro-tective effort on the gastric cancer progression(P ¼ 0.033, aOR ¼ 0.787; P ¼ 0.045, aOR ¼ 0.799;P ¼ 0.048, aOR ¼ 0.803), respectively. The SNPsrs2072407, rs734005, and rs734004 showed astrong LD located in the intron region betweenexons 15 and 19. The G to C change of SNPrs734004 might affect the binding of poly A down-stream elements and further the transcription ofgene terminated [33]. Furthermore, we found thathaplotypes of the EZH2 SNPs conferred variablesusceptibility to gastric cancer. The mechanismwith regard to effect of EZH2 SNPs on biologicalphenotypes of gastric cancer needs to be investi-gated further.In conclusion, we found the five SNPs of EZH2
gene were significantly associated with gastric can-cer susceptibility. Our findings might provide in-sight into the genetic basis of gastric cancer. Theeffect of EZH2 variants on recruitment of PRC1and PRC2 components and state of methylation ofgenes would warrant further investigation of thepotential mechanism in gastric cancer of the Chi-nese Han population.
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able4.(Continued)
Parameter
rs734004
rs734005
rs2072407
rs6464926
rs12670401
CC
CG
GG
P-value
CC
TC
TT
P-value
CC
TC
TT
P-value
CC
CT
TT
P-value
CC
TC
TT
P-value
Yes
111
16
111
16
16
11
19
11
88
11
9Saltedfood
0.516
0.460
0.315
0.975
0.795
Nooroccasionally
20
63
65
20
63
67
67
65
18
45
71
31
35
68
44
Yes
17
58
70
16
59
70
72
57
14
45
67
31
32
68
44
Thenumberof1genotypewas�5
,Fisher’sexact
test
wasused.Forothers,chi-squaredtest
wasused.
8 ZHOU ET AL.
Molecular Carcinogenesis
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EZH2 GENETIC VARIANTS AFFECT GASTRIC CANCER RISK 9
Molecular Carcinogenesis
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