PO Box 2345, Beijing 100023, China World J Gastroenterol 2006 January 28; 12(4): 625-629 www.wjgnet.com World Journal of Gastroenterology ISSN 1007-9327 wjg@wjgnet.com © 2006 The WJG Press. All rights reserved. RAPID COMMUNICATION Genetic alterations in benign lesions: Chronic gastritis and gastric ulcer Ana Cristina Gobbo César, Marília de Freitas Calmon, Patrícia Maluf Cury, Alaor Caetano, Aldenis Albaneze Borim, Ana Elizabete Silva Ana Cristina Gobbo César, UNESP - São Paulo State University, Campus São José do Rio Preto, SP, UNIP - Araçatuba, SP and Faculdades Católicas Salesianas, Araçatuba, SP, Brazil Marília de Freitas Calmon, Ana Elizabete Silva, UNESP - São Paulo State University, Department of Biology, Campus São José do Rio Preto, SP, Brazil Patrícia Maluf Cury, Alaor Caetano, Aldenis Albaneze Borim, FAMERP, School of Medicine, São José do Rio Preto, SP, Brazil This work was accomplished in the Cytogenetics and Molecular Biology Laboratory, Department of Biology, UNESP - São Paulo State University, São José do Rio Preto, SP, Brazil Supported by the Brazilian Agency FAPESP, No. 00/09413-6 Correspondence to: Dr. Ana Elizabete Silva, Departamento de Biologia, UNESP, Campus de São José do Rio Preto, Rua Cristóvão Colombo, 2265, Jardim Nazareth, CEP:15054-000 - São José do Rio Preto, SP-Brazil. anabete@ibilce.unesp.br Telephone: +55-17- 3221-2384 Fax: +55-17- 3221-2390 Received: 2005-04-12 Accepted: 2005-05-24 Abstract AIM: To investigate the occurrence of chromosome 3, 7, 8, 9, and 17 aneuploidies, TP53 gene deletion and p53 protein expression in chronic gastritis, atrophic gastritis and gastric ulcer, and their association with H pylori in- fection. METHODS: Gastric biopsies from normal mucosa (NM, n = 10), chronic gastritis (CG, n = 38), atrophic gastritis (CAG, n=13) and gastric ulcer (GU, n = 21) were studied using fl uorescence in situ hybridization (FISH) and im- munohistochemical assay. A modified Giemsa staining technique and PCR were used to detect H pylori . An as- sociation of the gastric pathologies and aneuploidies with H pylori infection was assessed. RESULTS: Aneuploidies were increasingly found from CG (21%) to CAG (31%) and to GU (62%), involving mainly monosomy and trisomy 7, trisomies 7 and 8, and triso- mies 7, 8 and 17, respectively. A signifi cant association was found between H pylori infection and aneuploidies in CAG (P = 0.0143) and GU (P = 0.0498). No TP53 dele- tion was found in these gastric lesions, but p53-positive immunoreactivity was detected in 45% (5/11) and 12% (2/17) of CG and GU cases, respectively. However, there was no signifi cant association between p53 expression and H pylori infection. CONCLUSION: The occurrence of aneuploidies in be- nign lesions evidences chromosomal instability in early stages of gastric carcinogenesis associated with H pylori infection, which may confer proliferative advantage. The increase of p53 protein expression in CG and GU may be due to overproduction of the wild-type protein related to an infl ammatory response in mucosa. © 2006 The WJG Press. All rights reserved. Key words: Aneuploidies; TP53 gene; p53 protein; Gas- tritis; Gastric ulcer Gobbo César AC, de Freitas Calmon M, Cury PM, Caetano A, Borim AA, Silva AE. Genetic alterations in benign lesions: Chronic gastritis and gastric ulcer. World J Gastroenterol 2006; 12(4): 625-629 http://www.wjgnet.com/1007-9327/12/625.asp INTRODUCTION Gastric carcinogenesis is considered a multi-step and multi- factorial process that proceeds from normal gastric mucosa with epithelial hyperproliferation to chronic gastritis with variable degrees of atrophy, intestinal metaplasia, dysplasia, and ultimately carcinoma[1]. In most cases, chronic gastritis, frequently associated with H pylori infection, precedes the formation of gastric cancer, and a great proportion of the clinical tumors occurs in connection with severe atrophic gastritis and extensive intestinal metaplasia[2]. Efforts have been made to identify changes of a precancerous nature in the gastric epithelium. The identifi cation of such changes may help to prevent the occurrence of gastric cancer[3]. Gastritis may also play a role in the pathogenesis of peptic ulcer disease by impairing the resistance of the gastric mucosa and consequently increasing the risk of ulcer[3]. In practice, the cancer risk in peptic ulcer disease applies exclusively to gastric ulcer. Epidemiological data on the incidence of peptic ulcer disease with gastric cancer suggest that ulcer disease may not be an important precursor of gastric cancer. However, possible links between these two are suggested by a similar relationship with chronic gastritis[2]. H pylori infection is accepted as the major causal factor for the histological features leading to severe gastroduodenal disease, including chronic gastritis, peptic www.wjgnet.com ulcer disease, intestinal-type gastric cancer and gastric MALT lymphoma. Only a small proportion of the infected cases will develop clinically signifi cant disease. About one in 5-6 individuals will develop peptic ulcer disease during their lifetime, and <1% will develop gastric cancer[4]. It is particularly important to recognize and define the characteristics of benign and pre-malignant lesions for application to studies of carcinogenesis and cancer prevention. Hence, in this study, we aimed to verify the occurrence of aneuploidies of chromosomes 3, 7, 8, 9, and 17, and of TP53 gene deletions using the FISH technique, besides p53 expression, in benign lesions such as chronic gastritis, atrophic gastritis and gastric ulcer. The results were associated with H pylori infection and other clinicopathological features, such as sex, age, smoking and alcohol consumption. MATERIALS AND METHODS Samples Chronic gastritis (CG), atrophic gastritis (CAG) and gastric ulcer (GU) samples were obtained, respectively, from 38 (13 males and 25 females), 13 (7 males and 6 females) and 21 patients (15 males and 6 females) without gastric cancer by biopsy performed during endoscopic evaluation. The mean age of these patients was 53 years (range, 2-89 years). Biopsies of histologically confirmed normal and H pylori-negative mucosa (NM) were obtained from 10 healthy individuals (2 males and 8 females) with a mean age of 43 years (range, 19-75 years). All specimens were collected at the Hospital de Base of São José do Rio Preto, SP, Brazil. All biopsies of normal mucosa and gastric ulcer were collected from the antral region of the stomach, whereas those of chronic gastritis and atrophic gastritis were mainly collected from the antrum and corpus. Clinicopathological data were collected using a standard interviewer-administered questionnaire and a review of the patients’ medical records. The study was approved by the National Research Ethics Committee, and written informed consent was obtained from all subjects. Histology Hematoxylin-eosin (H&E) staining was used for the diagnosis and classification of gastritis[5]. A modified Giemsa staining technique was used to visualize H pylori. DNA extraction and PCR for H pylori diagnosis DNA was extracted by the phenol-chloroform method after digestion with proteinase K[6]. PCR assays were performed separately with approximately 100 ng of total DNA, using three different sets of oligonucleotides. One of them amplifies a 312-bp segment of the gene CYP1A[7] as a DNA quality control, the other amplifies a 298-bp product of the gene encoding species-specific H pylori antigen[8], and the last one amplifies a 411-bp fragment corresponding to the urease A gene[9]. Positive and negative controls were used in all experiments. PCR products were separated on 75 g/L polyacrylamide-gel electrophoresis, followed by silver nitrate staining. The assay was considered positive when at least one of the bacterial PCR products was present[10]. Fluorescence in situ hybridization (FISH) Nuclear suspensions from all samples were obtained by mechanical and enzymatic disaggregation[11]. After washes in 600 mL/L acetic acid, the resulting nuclear suspension was dropped onto microscope slides and stored at -70 ℃ until use for FISH assay. FISH analysis was performed on interphase nuclei using centromere probes (CEP) for chromosomes 3, 7, and 8 directly labeled with Spectrum Green, and for chromosome 9 labeled with rhodamine (Vysis, Inc., Downers Grove, IL, USA). Dual-color FISH assays were performed using TP53 probe kits (Vysis), including the LSI TP53 sequence labeled in Spectrum Orange, with the centromere probe for chromosome 17 labeled in Spectrum Green. The hybridization and detection protocols followed the manufacturer’s instructions. For each probe, signals of about 300 intact and non- overlapping nuclei were evaluated by two independent observers according to the criteria described by Eastmond et al[12]. Cutoff levels for aneuploidies were based on the upper-limit mean +4 SD of the normal gastric mucosa biopsies. By defi nition, for monosomy of chromosomes 3, 7, 8, 9, and 17, the cutoff values were set at 10.0%, 11.0%, 11.0%, 8.5%, and 7.5%, respectively, and, for trisomy of the same chromosomes, at 10.0%, 9.0%, 8.0%, 8.5%, and 7.0%, respectively. Tetrasomy and pentasomy were absent in the normal mucosa samples; thus, 2% was arbitrarily taken as cutoff value. The TP53 gene scores were taken together with those of the chromosome 17 centromere. For TP53 gene deletion analysis, the gene-to-centromere ratio (G/C) was calculated for each case, that is, the total number of gene signals observed was divided by the total number of centromere signals. Immunohistochemical analysis To assess p53 protein accumulation, the commercially available monoclonal antibody DO-7 (Novocastra, Newcastle, UK) was used in combination with the anti- Ig second-stage antibody and the ABC kit (Novocastra) on paraffi n-embedded sections. This antibody recognizes both mutant and wild types of p53 protein. The slides were counterstained with Harris hematoxylin. As positive controls, sections from gastric adenocarcinoma were processed, previously shown to express high levels of p53 protein. For each sample, 500 epithelial cells were counted. Statistical analysis Data were analyzed using χ2 and Fisher’s exact tests. P values less than 0.05 were considered statistically signifi cant. RESULTS Analysis by the FISH technique showed that 89% to 99% of the nuclei of the H pylori-negative normal mucosa cases were disomic for chromosomes 3, 7, 8, 9, and 17, so they were considered to have no aneuploidy. The gene-to-centromere ratio (G/C) for the TP53 gene deletion ranged from 0.97 to 0.99 (mean of 0.98), so, in the cases of benign lesions with a G/C ratio < 0.90, 626 ISSN 1007-9327 CN 14-1219/ R World J Gastroenterol January 28, 2006 Volume 12 Number 4 www.wjgnet.com gene deletion was assumed. Low-intensity nuclear p53 protein immunoreactivity was observed only in 4 of the 8 evaluated cases of normal gastric mucosa, ranging from 0.2% to 4.0% of the immunostained nuclei. The positivity index was defined as >10% of cells showing nuclear staining, according to a previous report by Gobbo-César et al[11]. Table 1 shows the results regarding aneuploidies of chromosomes 3, 7, 8, 9, and 17, TP53 gene deletion, p53 expression, and clinicopathological data only of those cases with benign lesions (chronic gastritis, atrophic gastritis and gastric ulcer) which showed some genetic alteration. Increasing frequencies of aneuploidies were detected in the CG, CAG and GU cases: 21% (8/38), 31% (4/13), and 62% (13/21), respectively. The samples also showed an increasing complexity of the alterations with mainly monosomy and trisomy of chromosome 7 in CG, trisomy of chromosomes 7 and 8 in CAG, and more frequent trisomy of chromosomes 7, 8 and 17 in GU. About 75% (6/8) of CG, 100% (4/4) of CAG and 69% (9/13) of GU with aneuploidies were H pylori-positive. However, a significant association between the presence of aneuploidies and H pylori infection was found only in CAG (P = 0.0143) and GU (P = 0.0498), while parameters such as sex, age, smoking and alcohol consumption did not show any association with the occurrence of aneuploidies. No TP53 gene deletion was found in the cases evaluated, whether in CG, in CAG or in GU, but low- intensity nuclear p53-positive immunoreactivity was present in 45% (5/11) and 12% (2/17) of the CG and GU cases, respectively, ranging from 12% to 47.2% of p53- positive nuclei, as compared to over-expression of the p53 protein in positive controls from gastric adenocarcinoma (Figure 1). No significant association was found either between p53 expression and H pylori infection or with the other clinicopathological features investigated. DISCUSSION The development of gastric carcinoma is considered as a multistage progressive process due to alterations in onco- genes, tumor suppressor genes, cell-adhesion molecules, telomerase, as well as to a genetic instability at several mi- crosatellite loci, possibly related to H pylori infection[13,14]. The mechanisms leading to mutations, hyperproliferation Table 1 Aneuploidy, TP53 gene deletion and expression, and clinicopathological data in CG, CAG and GU cases Cases Sex/age Smoking/alcohol consumption H pylori L TP53 deletion (G/C<0.9) p53 IHC (>10%) Aneuploidy Chronic gastritis CG03 M/32 No/No - A ND ND -7, +8a CG06 M/02 No/No - A 0.97 15.6 CG13 F/56 Yes/No + C 0.95 31.4 CG14 F/36 Yes/No + A 0.94 0 -7 CG16 M/89 Yes/Yes + C 0.98 12.0 CG19 F/54 No/Yes - A 0.90 15.0 +7 CG30 F/41 Yes/No + A ND ND +7a CG31 M/44 Yes/No + A 0.95 ND +9 CG33 F/57 No/No + A 0.96 12.8 CG34 F/34 Yes/Yes + A ND ND +7 CG35 M/54 Yes/Yes + A ND ND +3, +7, +17 CG36 F/58 No/No + A 0.96 0.8 -7 Atrophic gastritis CAG05 F/84 No/No + A ND ND +8a CAG07 M/65 Yes/Yes + A ND ND +7, +8 CAG08 M/57 No/Yes + A ND ND +7 / +7+7 CAG13 M/77 Yes/No + A ND ND +9 Gastric ulcer GU02 M/73 Yes/Yes - A ND 0.8 +17 GU03 M/52 Yes/Yes - A ND 47.2 +9 / +9+9 GU04 M/78 Yes/Yes - A ND 9.6 +7, +8a GU05 M/64 Yes/Yes - A ND 0.8 -7a GU06 M/43 Yes/No + A ND 0 +7 / +7+7, +8, –9, +17 / +17+17 GU07 F/51 Yes/Yes + A ND 1.2 +3 / +3+3 GU09 F/72 No/No + A 0.97 14.6 GU12 M/28 Yes/Yes + A ND 3.2 -7, -9, -17 GU14 F/83 No/No + A ND 1.2 -9 GU15 M/43 Yes/Yes + A ND 6.4 -7, -8 GU16 F/82 No/No + A ND 0 -8 GU18 M/58 Yes/Yes + A ND ND +7 / +7+7 GU19 F/62 Yes/No + A ND ND +7 / +7+7, +8, +17 / +17+17 GU20 M/63 Yes/Yes + A ND ND +9 / +9+9a M: male; F: female; L:location; - : H pylori negative; +: H pylori positive; A: antrum; C: corpus; ND: not done; a: chromosome 17 not analyzed. Gobbo César AC et al. Genetic alterations in gastritis and ulcer 627 www.wjgnet.com and apoptosis of the epithelial cells are triggered very early in the H pylori gastritis cascade, resulting in atrophic gastri- tis, intestinal metaplasia and gastric cancer[2,13]. The identifi cation of genetic alterations in biopsies of the epithelium of patients with gastric dyspepsia may be helpful in early diagnosis of gastric cancer. FISH is an ac- curate and sensitive technique for the detection of aneu- ploidies in interphase nuclei from biopsies, making it pos- sible to identify changes in early stages of benign lesions, such as gastritis and gastric ulcer. Such changes may be used as markers for estimating the risk of gastric cancer. A few studies have evaluated aneuploidy in epithelial lesions of the stomach using DNA flow cytometry. In chronic and atrophic gastritis, Weiss et al[15] found DNA aneuploidy in 5.2% and in 8.5% of the cases, respectively. Teodori et al[16] observed aneuploidy in 45% (9/20) chronic atrophic gastritis specimens, whereas Abdel-Wahab et al[3] detected quantitative DNA alterations in 18.8% of atro- phic gastritis cases. To our knowledge, studies about aneuploidy in gastric ulcer are not available in the literature. Our study using the FISH technique showed increasing aneuploidy and com- plexity of the alterations from chronic gastritis (21%) to- wards atrophic gastritis (31%) and gastric ulcer (62%). The more frequent aneuploidies were monosomy and trisomy 7 in CG, trisomies 7 and 8 in CAG, and trisomies 7, 8, and 17 in GU. Moreover, in CAG and GU, these aneuploidies occurred more frequently in the H pylori-positive cases, probably being responsible for the chromosomal instability observed. Chromosomes 7, 8 and 17 carry several important genes involved in the control of cell proliferation, such as EGFR (7p12-13), c-myc (8q24), HER-2/neu (17q21), and TP53 (17p13). Therefore, the presence of trisomy of these chro- mosomes in precancerous gastric lesions leading to gene imbalance may confer proliferative advantage, increasing the risk of developing into gastric cancer. The development of carcinoma in cases of gastric ulcer disease during long-term H2-blocker treatment is slowly increasing, and ulcers that require such treatment exhibit the characteristics of intractable conditions, including linear ulcers, simultaneous gastric and duodenal ulcers, immature intestinal metaplasia of the gastric epithelium, and atrophic gastritis accompanied by multiple ulcer cica- trices[17]. Hence, especially in these cases of gastric ulcer, it is suggested that a genetic study should be performed to allow early detection of malignant transformation. Inactivation of the TP53 gene by mutation or deletion occurs as an initial event in gastric tumorigenesis, possibly associated with H pylori infection[14,18,19]. Using the FISH technique, Gomyo et al[20] detected a TP53 deletion in 77% (10/13) cases of gastric carcinoma. In the present study, no TP53 deletion was found in ei- ther chronic gastritis (15 cases), atrophic gastritis (3 cases) or gastric ulcer (3 cases), although it was observed in 60% (3/5) of the intestinal metaplasia and 110% (3/3) of the adenocarcinoma cases in a previous study conducted by our group[11], thereby corroborating the hypothesis that these pathologies share genetic alterations and progress jointly. The p53 gene products are known to regulate cell growth and proliferation. Wild-type p53 protein sup- presses cell growth by controlling the G1 checkpoint, and has several additional physiological functions, including control of the G2 cell checkpoint, as well as mediation of apoptosis[21]. The products of wild-type p53 can hardly be detected in normal cells by immunohistochemical assays because of their short half-life. However, TP53 gene al- terations induced by many missense mutations may modify the conformation and stabilize the proteins, leading to their accumulation[22]. Therefore, over-expression of a p53 protein is a useful marker for detecting a mutated TP53 gene[23,24]. In this study, an increase of detectable low-intensity p53 was observed in 45% (5/11) of chronic gastritis and 12% (2/17) of gastric ulcer cases. These positive immunostaining fi ndings may be a consequence of point mutations or small deletions. However, these changes are not detected by FISH, so were not tested in the current study. Alternatively, such alterations are more likely to be due to over-expression of the wild-type protein related to a physiological response brought about by the infl ammatory process of the gastric epithelium. The lack of association between p53 expression and H pylori infection may be related to the reduced number of specimens from benign lesions evaluated. Although some studies have described p53 protein accumulation in benign gastric lesions[13,25-28], its association with H pylori infection in gastric carcinogenesis is not yet clear. Whereas some authors reported over-expression of p53 protein in H pylori-positive chronic gastritis and intestinal metaplasia[13,25,27,28], Craanen et al [29] did not observe p53 protein accumulation in either atrophic gastritis or intestinal metaplasia and suggested that this process may be a late event in gastric carcinogenesis. On Figure 1 p53 protein expression on paraffi n-embedded sections (400X original magnification). Low-intensity nuclear p53 protein immunoreactivity in chronic gastritis (A) and gastric ulcer (B) in comparison with p53 over-expression in the positive controls from gastric adenocarcinoma of intestinal type (C) and diffuse type (D). A B DC 628 ISSN 1007-9327 CN 14-1219/ R World J Gastroenterol January 28, 2006 Volume 12 Number 4 www.wjgnet.com the other hand, Lan et al[13] reported that H pylori infection might first cause severe imbalance of proliferation and apoptosis in the precancerous lesions, leading to p53- Rb tumor suppressor system mutation and telomerase reactivation, and fi nally causing gastric cancer. In conclusion, our study has clearly shown the occurrence of aneuploidies, which increases with the progression of lesions from chronic gastritis to atrophic gastritis and to gastric ulcer, is frequently associated with H pylori infection, evidencing chromosomal instability in benign gastric lesions that may play an important role in gastric carcinogenesis. We observed no TP53 gene deletion in the benign gastric lesions, whereas p53 protein over- expression was detected in some cases of chronic gastritis and gastric ulcer, thus suggesting that an accumulation of wild-type p53 protein occurs, probably due to an infl ammatory response. REFERENCES 1 Correa P. Human gastric carcinogenesis: a multistep and multifactorial process--First American Cancer Society Award Lecture on Cancer Epidemiology and Prevention. Cancer Res 1992; 52: 6735-6740 2 Sipponen P, Hyvarinen H, Seppala K, Blaser MJ. Review article: Pathogenesis of the transformation from gastritis to malignancy. Aliment Pharmacol Ther 1998; 12 Suppl 1: 61-71 3 Abdel-Wahab M, Attallah AM, Elshal MF, Eldousoky I, Zalata KR, el-Ghawalby NA, Gad el-Hak N, el-Ebidy G, Ezzat F. Correlation between endoscopy, histopathology, and DNA fl ow cytometry in patients with gastric dyspepsia. Hepatogastroenterol 1996; 43: 1313-1320 4 Go MF. 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