{"title":"Detection of the babA2 adhesin protein gene in Helicobacter pylori clinical isolates.","authors":"A V Svarval, D A Starkova, R S Ferman","doi":"10.51620/0869-2084-2022-67-9-538-543","DOIUrl":null,"url":null,"abstract":"<p><p>The study compared the effectiveness of two different primer sets for detecting and evaluating the prevalence of the babA2 gene in 52 H. pylori clinical isolates from patients with chronic gastritis (n=32), duodenal ulcer (n=16) and stomach cancer (n=4) in St. Petersburg, Russia. The PCR was used for detection of the babA2 gene with 271 bp and 832 bp primer sets followed by sequencing of the PCR-amplicons. The largest proportion of babA2-positive strains - 90.4% (47/52) was detected using a 271 bp PCR primer set. Detection of the 832 bp PCR positive samples was observed only in 51.9% of cases (27/52). The largest proportion of babA2-positive strains - 90.4% (47/52) was detected using 271 bp PCR primer set; detection of 832 bp PCR product was observed only in 51.9% cases (27/52), however, there were no significant differences in the babA2 gene detection rates (p>0.05). Bioinformatic analysis revealed a homology of Sanger sequenced PCR products 271 bp and 832 bp of babA2 gene with regions of the babA2, babA1, and chimeric babA/B genes of H. pylori strains annotated in the NCBI database. Regardless of the primer set used, the presence of babA2 was not significantly associated with duodenal ulcer nor gastric cancer (p>0.05). The combination of the three babA2, cagA, and vacAs1 genes did not reveal any association between the presence of babA2 gene and cagA/vacAs1 genes in H. pylori strains (p>0.05). Thus, none of the two primer sets (271 bp and 832 bp) appears sufficiently informative for detecting the babA2 gene to assess virulence of H. pylori Russian strains.</p>","PeriodicalId":52451,"journal":{"name":"Klinichescheskaya Laboratornaya Diagnostika","volume":"67 9","pages":"538-543"},"PeriodicalIF":0.0000,"publicationDate":"2022-09-12","publicationTypes":"Journal Article","fieldsOfStudy":null,"isOpenAccess":false,"openAccessPdf":"","citationCount":"0","resultStr":null,"platform":"Semanticscholar","paperid":null,"PeriodicalName":"Klinichescheskaya Laboratornaya Diagnostika","FirstCategoryId":"1085","ListUrlMain":"https://doi.org/10.51620/0869-2084-2022-67-9-538-543","RegionNum":0,"RegionCategory":null,"ArticlePicture":[],"TitleCN":null,"AbstractTextCN":null,"PMCID":null,"EPubDate":"","PubModel":"","JCR":"Q4","JCRName":"Health Professions","Score":null,"Total":0}
引用次数: 0
Abstract
The study compared the effectiveness of two different primer sets for detecting and evaluating the prevalence of the babA2 gene in 52 H. pylori clinical isolates from patients with chronic gastritis (n=32), duodenal ulcer (n=16) and stomach cancer (n=4) in St. Petersburg, Russia. The PCR was used for detection of the babA2 gene with 271 bp and 832 bp primer sets followed by sequencing of the PCR-amplicons. The largest proportion of babA2-positive strains - 90.4% (47/52) was detected using a 271 bp PCR primer set. Detection of the 832 bp PCR positive samples was observed only in 51.9% of cases (27/52). The largest proportion of babA2-positive strains - 90.4% (47/52) was detected using 271 bp PCR primer set; detection of 832 bp PCR product was observed only in 51.9% cases (27/52), however, there were no significant differences in the babA2 gene detection rates (p>0.05). Bioinformatic analysis revealed a homology of Sanger sequenced PCR products 271 bp and 832 bp of babA2 gene with regions of the babA2, babA1, and chimeric babA/B genes of H. pylori strains annotated in the NCBI database. Regardless of the primer set used, the presence of babA2 was not significantly associated with duodenal ulcer nor gastric cancer (p>0.05). The combination of the three babA2, cagA, and vacAs1 genes did not reveal any association between the presence of babA2 gene and cagA/vacAs1 genes in H. pylori strains (p>0.05). Thus, none of the two primer sets (271 bp and 832 bp) appears sufficiently informative for detecting the babA2 gene to assess virulence of H. pylori Russian strains.
本研究比较了两种不同引物组在俄罗斯圣彼得堡慢性胃炎(n=32)、十二指肠溃疡(n=16)和胃癌(n=4)患者的52株幽门螺杆菌临床分离株中检测和评估babA2基因流行率的有效性。分别用271 bp和832 bp引物对babA2基因进行PCR检测,并对扩增产物进行测序。271 bp PCR引物检出的baba2阳性菌株比例最高,为90.4%(47/52)。832 bp PCR阳性标本检出率仅为51.9%(27/52)。271 bp PCR引物检出baba2阳性菌株比例最高,为90.4% (47/52);832 bp PCR产物检出率仅为51.9%(27/52),而babA2基因检出率差异无统计学意义(p>0.05)。生物信息学分析显示,Sanger测序的PCR产物babA2基因271 bp和832 bp与NCBI数据库中注释的幽门螺杆菌菌株babA2、babA1和嵌合babA/B基因区域同源。无论使用哪种引物,babA2的存在与十二指肠溃疡和胃癌均无显著相关性(p>0.05)。在幽门螺杆菌中,babA2、cagA和vacAs1基因与babA2基因和cagA/vacAs1基因的组合不存在相关性(p>0.05)。因此,这两组引物(271 bp和832 bp)都不足以检测babA2基因以评估俄罗斯幽门螺杆菌菌株的毒力。
期刊介绍:
The journal deals with theoretical and practical problems of clinical laboratory diagnosis, publishes editorial articles, reviews of literature, original articles, short reports, discussions, book reviews, current events, materials which may assist the practitioners, methods of laboratory investigations used in medicine, materials on the results of practical application of new methods of investigation in the following fields of clinical laboratory diagnosis: hematology, cytology, coagulation, biochemistry, immunology.