Health
Vol.6 No.4(2014), Article ID:43013,4 pages DOI:10.4236/health.2014.64038

The relationship between Helicobacter pylori disease and bacterial count in stomach

Sadegh Ghorbani-Dalini1, Mohammad Kargar2*, Abbas Doosti3, Akram Najafi4

1Department of Biology, University of Sistan and Baluchestan, Zahedan, Iran

2Department of Microbiology, Jahrom Branch, Islamic Azad University, Jahrom, Iran; *Corresponding Author: mkargar@jia.ac.ir

3Biotechnology Research Center, Shahrekord Branch, Islamic Azad University, Shahrekord, Iran

4Department of Marine Microbiology, The Persian Gulf Marine Biotechnology Research Center, Bushehr University of Medical Science, Iran

Copyright © 2014 Sadegh Ghorbani-Dalini et al. This is an open access article distributed under the Creative Commons Attribution License, which permits unrestricted use, distribution, and reproduction in any medium, provided the original work is properly cited. In accordance of the Creative Commons Attribution License all Copyrights © 2014 are reserved for SCIRP and the owner of the intellectual property Sadegh Ghorbani-Dalini et al. All Copyright © 2014 are guarded by law and by SCIRP as a guardian.

Received 4 November 2013; revised 10 December 2013; accepted 19 December 2013

ABSTRACT

Several studies showed significant relationships between bacterial counts and the severity and type of disease in patients. The aim of this study was to evaluate the relationship between Helicobacter pylori disease and bacterial count. In this study, 287 patients with dyspeptic symptoms were evaluated. Three variables including patient-reported data, clinical signs and bacterial load of gastric specimens were analyzed. Biopsy samples were collected from patients who were referred for endoscopies because of dyspeptic symptoms. Initially, the clinical status was evaluated and recorded by a questionnaire. DNA extraction was performed and H. pylori was analyzed for bacterial count by Real-time PCR assay and specific primers and probe. The variety range of bacteria in specimens was 104 to 1012. The results revealed that a greater relationships existed between 1012 and gastric cancer (p = 0.036), also 104 and acid reflux (p = 0.006) and vomiting (p = 0.047). Real-time PCR assay provides a highly accurate, rapid and precise method for detection of H. pylori and determination of progressive disease due to this bacterium.

KEYWORDS: Helicobacter pylori; Gastric Disorder; Quantitative Real-Time PCR; Stomach

1. INTRODUCTION

Helicobacter pylori is a microaerophilic, Gram-negative bacterium and is involved in the pathogenesis of peptic ulcer, gastritis, and gastric cancer [1]. Its prevalence ranges from 25% in developed countries to over 90% in developing areas [2-5]. Colonization by H. pylori is not a disease in itself, but as a condition that affects the relative risk of developing various clinical disorders of the upper gastrointestinal tract. It is important. Therefore, testing for the presence of H. pylori has no relevance to diseases but should be performed to find the cause of an underlying condition, such as peptic ulcer, or for the purpose of disease prevention, such as in subjects with a family history of gastric cancer. In these cases, a positive test result justifies treatment and a negative test result may indicate the need to search for other etiologic factors or preventive measures [3-7]. The aim of this study was to determine the H. pylori loads in gastric biopsy samples from patients with gastrointestinal disorders in Iran and to compare them with the severity and type of disease.

2. MATERIALS AND METHODS

287 H. pylori positive patients with gastrointestinal disorders in the southwest of Iran were enrolled in the study. Informed consent was taken from all patients at the beginning of endoscopy. Patient-reported symptoms and endoscopic findings by the pathologist were recorded at the time of the consultation.

For the purpose of analysis, three global variables were created: 1) patient-reported data, including age, gender and symptoms; 2) clinical signs; and 3) bacterial load as determined by PCR analysis.

Three biopsy specimens were collected from each patient (2 from antrum and 1 from corpus). All the samples were transported to the laboratory and stored in phosphate buffer saline (PBS) until the time of assay. A rapid urease test was performed with a Gastro urease kit (Baharafshan, Iran). The DNA was isolated from each biopsy, using a DNA extraction kit (CinnaGen, Iran) according to the manufacturer’s instructions and immediately used for the molecular analysis.

16S rRNA PCR analysis for the confirmation of H. pylori diagnosis was carried out in 25 µl reaction mixtures containing 2 µl of genomic DNA, 1.5 mM MgCl2, 200 mM concentrations of dNTPs, 1 U of smar Taq polymerase (CinnaGen, Iran) and 0.2 mM concentrations of primers HP-1 and HP-2 under previously reported conditions [8] (Table 1). The 109 bp fragment was visualized after electrophoresis on a 1.5% agarose gel stained with EtBr.

Bacterial quantification was performed applying the TaqMan probe technology of real-time PCR using a Corbett 6000 (Corbett research, Australia). Real-time PCR was performed using final solution of 25 µl containing 2 µl of extracted DNA, 200 mM dNTPs, 1.5 mM MgCl2, 1 U of smar Taq polymerase in PCR buffer 1X, 0.2 mM primers HP23S-1 and HP23S-2, and probes (Table 1) as previously reported under cycling conditions consisting of an initial denaturation at 95˚C for 5 min, followed by 45 cycles with denaturation at 95˚C for 30 s, annealing at 58˚C for 40 s [9,10]. All tests were performed three times on each sample. Data were analyzed with the Rotor-gene 6000 software ver1.7 (Corbett research).

Data were statistically analyzed by SPSS version 17 (SPSS Inc., Chicago, IL, USA). Statistical analysis χ2 test was used to analyze the data obtained. P-values less than 0.05 were considered to indicate statistical significance.

3. RESULTS

287 patients, with a median age of 51.5 (ranging from 15 to 88 years) were divided into 8 age groups from 10 to 90 years. 4.77% (137) of them were male and 52.3% (150) were female. Pain was present in 173 patients, nausea in 74, anorexia in 68, acid reflux in 55, heaviness after meals in 51, early satiety in 46, vomiting in 51 and flatulence in 70 (Table 2). The main endoscopic findings are depicted in Table 3. Chi-square analysis revealed a greater correlation between gastritis and the age group 30 - 40 (p = 0.007), NUD and 40 - 50 (p = 0.001), early satiety and 10 - 20 (p = 0.05), flatulence and 10-20 (p = 0.038), vomiting and 20 - 30 (p = 0.001), pain and 50 - 60 (p = 0.003), heaviness after a meal and 50 - 60 (p = 0.018) and early satiety and 60 - 70 (p = 0.05) (Table 2).

Both 16S rRNA PCR and real-time PCR assays confirmed the presence of H. pylori in all of these 287 biopsy samples (100%).

Mucosal bacterial quantification was performed by TaqMan real-time-PCR. The bacterial density by this technique could be evaluated for all 287 H. pylori-positive patients and ranged from 1.53 × 104 to 5.89 × 1012 CFU. In order to evaluate the relationship between bacterial concentration and other variables, patients were divided into 9 groups from 1 × 104 to 6 × 1012 CFU (Table 3). The statistical analysis revealed a greater relationship between group 1012 and gastric cancer (p = 0.036), also 104 and acid reflux (p = 0.006) and vomiting (p = 0.047). There was no correlation between bacterial load and age or gender.

Table 1. Sequences of oligonucleotides used in this study.

Table 2. Distribution of symptoms and age groups.

Table 3. Interview data and endoscopic findings according to bacterial count of H. pylori.

4. DISCUSSION

In the present study, we have developed a real-time PCR assay based on the amplification of a fragment of the 23S rRNA gene with the TaqMan technology aimed at detecting H. pylori directly from gastric biopsy specimens, quantifying the bacterial density, and evaluating the relationship between bacterial load and disease severity. This assay provides formal statistical proof that the concentration of H. pylori in the gastric system is extremely high in gastric cancer patients.

The quantitative sensitivity of our assay was 400 bacteria per reaction tube, i.e., 800 copies of the 23S rRNA gene. As few as 40 bacteria (80 copies of the gene) could be detected but not accurately quantified. Therefore, our real-time PCR can accurately quantify the gastric mucosal density of H. pylori. Other techniques can be employed for quantification; however, each technique has its weaknesses. A bacterial culture is only semiquantitative and time-consuming. Histology is also semiquantitative, but its accuracy is relatively low because of great interobserver variation. The urea breath test has been shown to be uncorrelated to culture-determined bacterial density [11].

Several studies demonstrate that there are significant correlations between bacterial counts and the severity and type of disease in patients infected with S. enterica serovar typhi [12], Orientia tsutsugamushi [13], and M. Tuberculosis [14], but so far not enough results regarding H. pylori have been reported.

H. pylori infection results in a sequence of events, ultimately resulting in the development of some gastrointestinal disorders. The initial acute gastritis is followed by active chronic gastritis, which lasts for life if the infection is not treated. Nevertheless, H. pylori-positive subjects are mostly unaware of this inflammation due to the lack of clinical symptoms. The ongoing presence of H. pylori and the resulting cellular damage initiates the histological cascade including gastric atrophy, intestinal metaplasia, dyspepsia and finally gastric cancer [4,6]. Our study was consistent with these findings: the bacterial load was 105 to 106 in biopsies from patients with chronic active gastritis, 107 to 108 in gastric atrophy and 1012 in gastric cancer. In this study, we found a correlation between a bacterial count of 104 and some symptoms including vomiting and acid reflux. The simultaneous presence of these symptoms may indicate infection by H. pylori and the possible development of the H. pylori disease cascade.

In conclusion, we show that disease severity and clinical symptoms are dependent on the bacterial load. H. pylori-positive patients are often described as being “completely well”. When the H. pylori load in gastric mucosa increases, the first clinical symptoms occur, including pain, anorexia, heaviness after meal, early satiety, nausea and flatulence. Finally, when a bacterial load of 104 is reached, vomiting and acid reflux are induced. After bacterial colonization, when the bacterial count reaches 105, the first grade of disease is observed. This induces an inflammatory response which leads to some lesions and consequently to acute gastritis, which is followed by active chronic gastritis when bacterial counts reach 106. This lasts for life if the infection is not treated. The ongoing inflammation and cellular damage due to more colonization with H. pylori lead to the second grade of disease severity with bacterial counts of 107 that induce gastric atrophy. When the bacterial density reaches high levels, gastric cancer appears. These data were collected from our findings and those of other investigators. We believe more researches in other regions of the world are needed to confirm the relationship between the number of bacteria and different stages of gastric disease.

Lower frequency of sever diseases such as gastric cancer and atrophy in our samples is a limitation of this study. Therefore, it is suggested that this evaluation should conduct on large samples with a higher number of sever disorders and in different areas.

ACKNOWLEDGEMENTS

All authors are grateful to the Islamic Azad University, Jahrom and Shahrekord Branches and staff of Biotechnology Research Center, for their executive support of this project.

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