Basic Study Open Access
Copyright ©The Author(s) 2015. Published by Baishideng Publishing Group Inc. All rights reserved.
World J Gastroenterol. Mar 14, 2015; 21(10): 2905-2911
Published online Mar 14, 2015. doi: 10.3748/wjg.v21.i10.2905
Prevalence of human papillomavirus in esophageal carcinoma in Tangshan, China
Mohammadreza Mohammadzad Mehryar, Fan Li, Fang Zhang, Yu-Bai Zhou, Yi Zeng, Jin-Tao Li, Beijing Key Laboratory of Environmental and Viral Oncology, College of Life Science and Bio-Engineering, Beijing University of Technology, Beijing 100124, China
Mohammadreza Mohammadzad Mehryar, Fan Li, Fang Zhang, Yu-Bai Zhou, Yi Zeng, Jin-Tao Li, Collaborative Innovation Center for Biotherapy, West China Hospital, Sichuan University, Chendu 610041, Sichuan Province, China
Shu-Ying Li, Department of Pathogenic Biology, College of Basic Medicine, Hebei United University, Tangshan 063000, Hebei Province, China
Hong-Wei Liu, Key Laboratory of Southwest China Wildlife Resources Conservation, Ministry of Education, College of Life Sciences, China West Normal University, Nanchong 637000, Sichuan Province, China
Yi Zeng, Jin-Tao Li, National Institute for Viral Disease Control and Prevention, Chinese Center for Disease Control and Prevention, and State Key Laboratory for Infectious Disease Prevention and Control, Beijing 100052, China
Author contributions: Li JT and Zeng Y designed the study; Mehryar MM and Li SY performed the majority of the experiments and contributed equally to this work; Liu HW, Li F and Zhang F performed the research; Zhou YB analyzed the data and wrote the paper.
Supported by Chinese Center for Disease Control and Prevention and the State Key Laboratory for Infectious Disease Prevention and Control, No. 2011SKLID103; Beijing Key Laboratory of Environmental and Viral Oncology, College of Life Science and Bio-Engineering, Beijing University of Technology (Grant sponsor: State 863 projects, No. 2012AA02A404, No. 2014ZX10005002 and No. PXM2014_014204_07_000046).
Ethics approval: Approval Letter of Ethics Committee of Hebei United University
Conflict-of-interest: The authors report no conflict of interest.
Data sharing: No additional data are available.
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: Jin-Tao Li, PhD, Beijing Key Laboratory of Environmental and Viral Oncology, College of Life Science and Bio-Engineering, Beijing University of Technology, No. 100 Pingleyuan, Chaoyang District, Beijing 100124, China. ljt2000593@163.com
Telephone: +86-1067392780 Fax: +86-1067392780
Received: May 8, 2014
Peer-review started: May 9, 2014
First decision: June 10, 2014
Revised: June 27, 2014
Accepted: October 15, 2014
Article in press: October 15, 2014
Published online: March 14, 2015

Abstract

AIM: To study the prevalence of human papillomavirus (HPV) in esophageal carcinoma in Tangshan, China, a high-incidence area.

METHODS: Formalin-fixed, paraffin-embedded tissue specimens from 198 patients who were pathologically diagnosed with esophageal squamous cell carcinoma from 2011 to 2013 were obtained from a pathology department in Tangshan. DNA was extracted from all 198 specimens to detect HPV by polymerase chain reaction (PCR). β-globin PCR was performed to check the quality of the DNA extraction procedure. PCR was performed to detect a wide range of HPV types, and type-specific PCR was performed to detect HPV types 16 and 18. Negative and positive controls were used for HPV 16 and 18 detection.

RESULTS: The DNA extraction method in this study appeared to be more effective than other previously reported methods. After DNA extraction, more than 98% of the tissue specimens had an acceptable result in the DNA qualification test (β-globin PCR). The overall prevalence of HPV in tumor tissues by GP6+/GP5+ PCR was 79.79%, and the prevalence of HPV types 16 and 18 was 40.40% and 47.47%, respectively. PCR demonstrated the presence of HPV, and direct sequencing confirmed the HPV genotypes. All HPV-positive PCR products were checked by DNA sequence analysis using DNAman and compared with the known HPV sequences listed in the Basic Local Alignment Search Tool database to evaluate the HPV types. This analysis confirmed the presence of HPV types 16 and 18.

CONCLUSION: DNA of high-risk HPV types 16 and 18 is present in esophageal tumors, implicating HPV as a possible etiologic factor for esophageal squamous cell carcinoma.

Key Words: Esophageal carcinoma, Formalin-fixed, paraffin-embedded tissue, Esophageal squamous cell carcinoma, Human papillomavirus, Polymerase chain reaction

Core tip: China is considered to have a high incidence of esophageal cancer. Many etiologic factors for esophageal cancer have been described; in China, human papillomavirus (HPV) infection could be an important cause of esophageal cancer. Tangshan in Hebei, China has a high incidence of esophageal cancer. However, no large-sample analyses of the prevalence of HPV in this area have been performed. We analyzed the prevalence and types of HPV in 198 esophageal cancer specimens in this area of China. These findings have important significance for analysis of the various causes of local esophageal cancer.
INTRODUCTION

Esophageal cancer is the eighth most common cancer and sixth most common cause of cancer death worldwide[1]. Human papillomavirus (HPV) belongs to a group of nonenveloped, double-stranded DNA viruses, more than 100 genotypes of which have been recognized. Many molecular and epidemiologic studies have confirmed that HPV, especially high-risk HPV types, has an important role in the development of cervical cancer[2,3]. HPV DNA must be integrated into the host cell genome for malignant transformation of the cervical epithelium to occur[4]. Several studies have evaluated the role of HPV in extragenital cancers, but have produced conflicting results regarding the involvement of HPV[5,6].

In 1982, Syrjänen[7] was the first to report the probable involvement of HPV in esophageal squamous cell carcinoma (ESCC). Many researchers subsequently became interested in HPV infection as a possible cause of the development of ESCC. A comprehensive review in 2002 reported that HPV was positive in 22.9% of 1485 ESCC specimens evaluated by in situ hybridization and in 15.2% of 2020 ESCC specimens evaluated by PCR[8]. Esophageal cancer usually begins in the epithelial layer of the esophagus. Approximately 90% of esophageal cancers are squamous cell carcinomas. In some countries, such as the United States, the frequency of ESCC is almost identical to that of adenocarcinoma[9]. Different studies around the world have shown that, for unknown reasons, the incidence of esophageal cancer differs among various countries, as well as among different regions within the same country. According to the World Health Organization, West Africa is considered to be of low risk for ESCC, while China is considered to be of high risk[10]. Among North American countries, Peru and Mexico have the lowest mortality rates for esophageal carcinoma, and Argentina, Chile, and Brazil have the highest rates[11]. Many studies have been performed in different areas of China, but their results are conflicting. Studies on HPV in the Anyang, Shandong, and Gansu areas of China have confirmed the presence of the HPV genome, especially the high-risk types, in esophageal cancer[12]. However, this finding was not supported by another study conducted in Linxian, China[13].

Studies on HPV involvement in esophageal cancer have reported conflicting results, with prevalence rates ranging from 0 to 71%[14]. Variations in the specificity and sensitivity of the evaluation techniques used are a probable cause of these differences. Polymerase chain reaction (PCR) is the most rapid and sensitive method for detecting DNA in any type of sample; however, the use of PCR with a suitable pair of primers is critical[15].

Collection of fresh cancerous tissues on a large scale is difficult. On the other hand, examination of fresh tissues allows samples to be evaluated in a short period of time. Therefore, formalin-fixed, paraffin-embedded (FFPE) archived tissue specimens were used in this study. Various methods are available to examine paraffin-embedded tissues, such as immunohistochemistry or other techniques for extraction and examination of DNA or RNA. Among these different methods, PCR has been confirmed to be a rapid and particularly sensitive method for examining DNA from paraffin-embedded tissues. Adequate storage of samples and the production of high-quality extracted DNA are important factors in obtaining accurate PCR results.

MATERIALS AND METHODS
Tissue collection

ESCC specimens were obtained from a pathology department in Tangshan from 2011 to 2013. The samples comprised 198 FFPE tissue blocks of histologically confirmed ESCC.

DNA extraction

The FFPE tissue blocks were cut into 20-μm sections and dewaxed by incubation for 2 h in pure xylene with remixing of the tube contents every 45 min. The remixing was repeated seven times, and the dewaxed samples were then washed and dehydrated with 100% ethanol six times. They were then dried at room temperature. The deparaffinized samples were digested with 600 μL of lysis buffer [10 mmol/L Tris-HCL (pH 8.0), 0.1 mol/L EDTA, 0.5% SDS, and 20 μg/mL RNase A]. Next, 20 μL of 20 μg/mL proteinase was added. After mixing, the tubes were incubated at 55 °C for 12 h with remixing of the tube contents every 2 h. After complete digestion, DNA was extracted by phenol/chloroform precipitation. This process was performed twice for every sample and then followed by one phenol/chloroform precipitation. The DNA was precipitated with 100% ethanol and incubated at -20 °C overnight. After precipitation of the DNA, the tubes were centrifuged at 13000 rpm for 15 min, rewashed with 75% ethanol, and dried at room temperature. Finally, 80 μL of TE buffer was added to every tube, and tubes were incubated at 4 °C for a few hours to dissolve the precipitated DNA.

PCR

The obtained DNA was amplified for the β-globin gene using a Takara PCR kit (Takara Inc., Otsu, Shiga, Japan) and PC04/GH20 primers to evaluate the performance of the DNA extraction (Table 1). A GP5+/GP6+ primer set was used with a low annealing temperature and small PCR product of 150 bp to detect a wide range of HPV types[16-18]. Two sets of primers were used for specific detection of HPV types 16 and 18. The annealing temperature and PCR products of these two sets are mentioned in Table 1. In each batch, water was used as the negative control and the genome of HPV-positive cervical cells was used as the positive control. The PCR products were checked on a 1.0% agarose gel and visualized by ethidium bromide staining.

Table 1 Primers used in PCR amplification of human papillomavirus DNA.
PrimerSequence, 5’-3’Annealing temperature,°CPCR product, bp
PC04CAACTTCATCCACGTTCACC62150
GH20GAAGAGCCAAGGACAGGTAC
GP5+TTTGTTACTGTGGTAGATACTAC55150
GP6+CTTATACTAAATGTCAAATAAAAAG
HPV16E6FCAACAAGACATACATCGACC60350
RCAACAAGACATACATCGACC
HPV18E6FCACTTCACTGCAAGACATAGA55350
RGTTGTGAAATCGTCGTTTTTCA
Sequencing of PCR products

All PCR-positive products were sequenced and analyzed using the T7 sequence version 2.0 DNA PCR product sequencing kit (Affymetrix, Santa Clara, CA, United States) to identify the HPV types and any sequence variations. The nucleotide sequences were subsequently confirmed using the Basic Local Alignment Search Tool (BLAST).

RESULTS

All PCR processes were performed twice to confirm the presence of the PCR products of interest. The products of the first PCR process were used as the template for the second PCR process. During the second PCR process, the amounts of all PCR mixture materials excluding the 8-μL template were similar to those in the first PCR process. Table 2 summarizes the results of every PCR process of all 198 ESCC specimens examined in this study. All results shown in Table 2 are those of the second PCR process.

Table 2 Polymerase chain reaction detection frequency of human papillomavirus using different primers.
Primer setTested cases, nPositive cases, nPositive cases
PC04/GH20198196> 98.00%
GP5+/GP6+19815879.79%
HPV 161988040.40%
HPV 181989447.47%
GP+ and HPV16/18-1198136.50%
HPV 16 and 181985527.77%
HPV 16 or 1819811960.10%
GP and HPV 16 and 181984824.24%
GP+/HPV16+/HPV18+219818593.00%
1GP5+/GP6+ positive but human papillomavirus (HPV) 16/18 negative;
2GP5+/GP6+ positive or HPV 16 positive or HPV 18 positive.
β-globin PCR (PC04/GH20)

The DNA extraction method seemed to be more effective than other previously reported methods. After DNA extraction, all samples were subjected to β-globin PCR to test the quality of the extracted DNA. The DNA quality was good in 190/198 (> 98%) of the ESCC specimens. PCR using the PC04/GH20 primer pair resulted in clearly differentiated DNA fragments of 150 bp (Figure 1).

Figure 1
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Figure 1 β-globin PCR results. Clearly differentiated DNA fragments of 150 bp are evident.
General HPV PCR (GP5+/GP6+)

After β-globin PCR, all 198 specimens were examined using the GP5+/GP6+ primer set to visualize the HPV-positive cases on an agarose gel. PCR using the GP5+/GP6+ primer pair resulted in clearly differentiated DNA fragments of 150 bp (Figure 2). In total, 158/198 (79.79%) specimens were positive for HPV as indicated by the presence of the 150-bp PCR product.

Figure 2
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Figure 2 GP5+/GP6+ PCR. Clearly differentiated DNA fragments of 150 bp are evident.
Type-specific PCR (HPV types 16/18)

All samples were amplified using the primer sets specific for HPV 16 (JHPV16E6F/JHPV16E6R) and HPV 18 (X18E6F/X18E6R) with the sequences listed in Table 1. These two PCR processes yielded an intense band of the correct size (350 bp) for both HPV types 16 and 18 (Figure 3). Of all 198 specimens, 80 (40.40%) were positive for HPV 16, and 94 (47.47%) were positive for HPV 18 as indicated by the presence of the corresponding PCR products (Table 2).

Figure 3
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Figure 3 Human papillomavirus PCR results. DNA fragments of 350 bp are evident. A: Human papillomavirus (HPV) 16; B: HPV 18.
Sequencing PCR products

The DNA sequences of all HPV-positive PCR products were analyzed with DNAman software, and the results were compared with the known HPV sequences in the DNA database using BLAST to identify the various HPV types. The specimens contained DNA of both HPV types 16 and 18. The DNA software analysis results confirmed the presence of HPV DNA with a few mutations in the viral DNA (Figure 4).

Figure 4
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Figure 4 Human papillomavirus sequencing results. A: Human papillomavirus (HPV) 16E6 in three specimens with some mutations; B: HPV 18E6 in three specimens with one mutation.
DISCUSSION

ESCC has one of the highest mortality rates worldwide. In some countries with a low prevalence of ESCC, tobacco and alcohol use may be the main causative factors of ESCC. However, in regions with a high incidence of ESCC, including China and northern Iran, only a small portion of ESCC cases are related to smoking or alcohol consumption. Therefore, other risk factors should be considered to help explain the high incidence of ESCC in these areas. Probable factors that could be responsible for this high incidence include a low intake of fruits and vegetables, drinking of hot tea, consumption of opium products and tobacco, Helicobacter pylori infection, contaminated water sources, and genetic susceptibility[19]. Polycyclic aromatic hydrocarbons and N-nitroso compounds are the most important mutagens that cause esophagus cancer[20]. Since the first study by Syrjänen in 1982[7], several studies have been performed in different countries and in different parts of the same country to identify and confirm the involvement of HPV in the development of ESCC. Many studies have shown the presence of the HPV genome in DNA isolated from esophageal cancer tissues; however, their results are conflicting[21-28]. On the other hand, there are differences in the HPV prevalence rates from the same areas. For example, although Chang et al[29] and Lu et al[30] reported a high incidence (36.8%) of HPV infection in patients with ESCC in northern Iran, another study found no HPV infection in 92 patients with ESCC in another Iranian city (Shiraz). Similarly, studies from Australia using the same evaluation method reported different HPV infection rates of 50% and 23% in patients with esophageal cancer[31,32]. Using molecular methods, the majority of these studies have shown the presence of high-risk HPV types in a variable proportion of cases[33-35]. However, HPV has not been identified as an etiologic agent of esophageal cancer, even in highly prevalent regions[13,36].

In the present study, we examined tissue specimens from 198 patients with a pathologic diagnosis of ESCC and found a high prevalence of HPV DNA (approximately 67% of all specimens). These rates are clearly higher than in some previous studies in other regions of the same country (China). In another study, although the evaluation methods, PCR processes, and samples (paraffin-embedded cancerous tissues) were almost identical, the rates in Shandong and Gansu were lower than in Shantou[12]. In the present study, 19.0% of the specimens were HPV-positive in contrast to 77.2% reported in a previous evaluation in Shantou[10,37]. Previous studies performed throughout the world, including China, have shown a high incidence of HPV DNA in almost all samples examined. These results implicate HPV as a suspected causative agent of esophageal cancer in addition to other etiologies (environmental or genetic). Several factors may contribute to the controversial results among different countries or among different regions of the same country: sample preparation (including all processes from intraoperative cutting of the suspected tissue by the surgeon to DNA extraction and analysis for the viral genome), sensitivity of the evaluation method (any item related to analysis of the HPV genome, including instrument sensitivity and the use of high-quality materials during DNA analysis in the PCR procedure), and regional diet habits or other special customs.

In conclusion, a potential role of HPV in the development of ESCC has emerged as evidenced by the HPV-like histologic changes in the mucosa of patients with esophageal cancer and the presence of HPV antigens and HPV DNA in cancerous tissues. Although various types of HPV have been detected by PCR amplification and other methods, clear evidence of the etiologic significance of HPV in ESCC is still lacking. Considering that no studies on the relationship between HPV and esophageal cancer have been performed in Tangshan, China, we hope that the present study promotes further efforts to confirm the etiologic significance of HPV in the development of ESCC.

COMMENTS
Background

Human papillomavirus (HPV) was introduced as a possible causative agent in the development of esophageal squamous cell carcinoma (ESCC) in 1982. Many studies have since been performed to prove this relationship; however, the results have been controversial.

Research frontiers

Many recent studies have focused on the relationship between many cancers and high-risk HPV infection. In this study, we focused on Tangshan, China, one area characterized by a high incidence of ESCC. HPV may be an important cause of the occurrence of ESCC. The authors anticipate that the results of this study will encourage researchers to launch new studies in other regions of China with a high incidence of ESCC to confirm this relationship. Their findings will also provide new ideas for additional studies on potential vaccines for HPV infection-induced ESCC.

Innovations and breakthroughs

In this study, 79.79% of all ESCC specimens were positive for HPV. Differentially, 40.40% and 47.47% were positive for HPV 16 and 18, respectively. Conflicting results from different regions of China have also been reported, with HPV positive rates ranging from 0 to 71%.

Applications

One possible reason for the variability in HPV infection rates is the use of different evaluation methods. In this study, the most sensitive and common method (PCR) was used to evaluate cancerous tissues. The use of other complementary methods to confirm the PCR results is ideal.

Terminology

More than 150 types of HPV exist, and they may be divided into two groups: high risk and low risk. Both groups can induce growth of abnormal cells, but only the high-risk types, specifically types 16 and 18, lead to malignant transformation.

Peer-review

This study introduced HPV as a probable cause of esophageal carcinoma. However, for confirmation of this causative relationship, other studies using different methods should be performed in other geographic areas. One limitation of this study was the lack of an ideal negative control; normal esophageal tissue is too difficult to obtain. This study can promote research using other methods or further research in other regions to clarify the etiologic significance of HPV in ESCC.

Footnotes

P- Reviewer: Tovey FI S- Editor: Ma YJ L- Editor: Wang TQ E- Editor: Ma S

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