Strategy for the Detection of Helicobacter Species by Amplification of 16S RRNA Genes and Identification of H. Felis in a Human Gastric Biopsy

Overview

Journal Res Microbiol

Publisher Elsevier

Specialty Microbiology

Date 1997 May 1

PMID 9765810

Citations 34

Authors

Y Germani

C Dauga

P Duval

M Huerre

M Levy

G Pialoux

P Sansonetti

P A Grimont

Affiliations

Soon will be listed here.

Abstract

The aim of the present work was to develop polymerase chain reactions (PCRs) based on the conserved nucleotide sequence of the 16S rRNA gene for detection of bacteria of the Helicobacter genus in human antral biopsy samples. The assay for Helicobacter spp was developed by amplifying a 399-bp 16S rRNA gene sequence specific to the genus Helicobacter. The identity of the amplicon was confirmed by hybridization with an internal probe and by restriction by endonuclease VspI showing two expected fragments of 295 and 104 base pairs. A total of 65 dyspeptic patients from France and New Caledonia were screened for Helicobacter spp infection through the use of the following diagnostic assays on biopsy specimens collected through endoscopy: direct detection of bacteria in histological sections by Giemsa and Warthin Starry staining, urease test and bacterial isolation, PCR for Helicobacter pylori ureC/glmM gene, and PCR targeted to 16S rRNA genes. The 16S rRNA gene PCR assay was able to detect down to 680 bacterial cells, as assessed by agarose gel electrophoresis, and down to 4 bacterial cells by hybridization of amplicon with the internal probe. The 16S rRNA PCR test was 100% specific and sensitive; results obtained with this test were in agreement with the visualization of bacteria by histology. Urease test and culture were 86.4% and 22.7% sensitive, and 96.5 and 100% specific, respectively. The H. pylori ureC/glmM gene-based PCR was 100% specific and only 95.4% sensitive, since one biopsy from a Melanesian patient contained a Helicobacter strain other than H. pylori. For this Melanesian patient, a branch-specific PCR targeting the epsilon branch of Proteobacteria was used to amplify a 967-bp amplicon. This amplicon was sequenced and matched with the H. felis sequence. This was confirmed using an H. felis-specific urease PCR test.

Citing Articles

Modulation Effects of Extract on Hyperglycemia and Hyperlipidemia in Type 2 Diabetic Mice.

Xie X, Chen C, Fu X Foods. 2023; 12(24).

PMID: 38137213 PMC: 10742466. DOI: 10.3390/foods12244409.

Effect of a Probiotic Mixture in Captive Cheetahs () with Gastrointestinal Symptoms-A Pilot Study.

Mangiaterra S, Schmidt-Kuntzel A, Marker L, Cerbo A, Piccinini R, Guadagnini D Animals (Basel). 2022; 12(3).

PMID: 35158716 PMC: 8833592. DOI: 10.3390/ani12030395.

DNA diagnostics for reliable and universal identification of .

Sulo P, Sipkova B World J Gastroenterol. 2021; 27(41):7100-7112.

PMID: 34887630 PMC: 8613642. DOI: 10.3748/wjg.v27.i41.7100.

A report of nonexistence of the non-Helicobacter pylori Helicobacter species in Iranian patients suffering from inflammatory bowel disease.

Pirmanesh S, Mirzaei N, Azimirad M, Yadegar A, Kao J, Aghdaei H Folia Microbiol (Praha). 2021; 66(5):751-759.

PMID: 34101130 DOI: 10.1007/s12223-021-00883-z.

Evidence of spp. in Saliva and Gastric Mucosa of Domestic Dogs in the Central Region of Rio Grande do Sul, Brazil.

Guerra Segundo D, Mello C, Cargnelutti J, Flores M, Pedrotti L, Antunes B Vet Med Int. 2021; 2021:8857231.

PMID: 33575024 PMC: 7864744. DOI: 10.1155/2021/8857231.