Rapid and specific detection of Helicobacter pylori macrolide resistance in gastric tissue by fluorescent in situ hybridisation

被引:108
|
作者
Trebesius, K
Panthel, K
Strobel, S
Vogt, K
Faller, G
Kirchner, T
Kist, M
Heesemann, J
Haas, R
机构
[1] Univ Munich, Max Von Pettenkofer Inst Hyg & Med Microbiol, D-80336 Munich, Germany
[2] Univ Freiburg, Inst Med Microbiol & Hyg, D-7800 Freiburg, Germany
[3] Humboldt Univ, Hosp Virchow, Dept Microbiol, Berlin, Germany
[4] Humboldt Univ, Charite, Berlin, Germany
[5] Univ Erlangen Nurnberg, Inst Pathol, D-8520 Erlangen, Germany
关键词
Helicobacter pylori; macrolide resistance; clarithromycin; in situ hybridisation; genotypic resistance;
D O I
10.1136/gut.46.5.608
中图分类号
R57 [消化系及腹部疾病];
学科分类号
摘要
Background-The development of macrolide resistance in Helicobacter pylori is considered an essential reason for failure of antibiotic eradication therapies. The predominant mechanism of resistance to macrolides, particularly clarithromycin, is based on three defined mutations within 23S rRNA, resulting in decreased binding of the antibiotic to the bacterial ribosome. Aim-To develop an rRNA based whole cell hybridisation method to detect Helicobacter species in situ within gastric tissue, simultaneously with its clarithromycin resistance genotype. Methods-A set of fluorescent labelled oligonucleotide probes was developed, binding either to H pylori 16S rRNA or 23S rRNA sequences containing specific point mutations responsible for clarithromycin resistance. After hybridisation and stringent washing procedures, labelling of intact single bacteria was monitored by fluorescence microscopy. The new approach was compared with PCR based assays, histology, and microbiological culture. Results-In comparison with the phenotypic resistance measurement by E test, the genotypic clarithromycin resistance correlated perfectly (100%) for 35 H pylori isolates analysed. In a set of gastric biopsy specimens (27) H pylori infection was confirmed by histology (17/27) and correctly detected by whole cell hybridisation. Five clarithromycin resistant strains were identified in gastric tissue specimens directly. Furthermore, non-cultivable coccoid forms of H pylori were easily detectable by whole cell hybridisation. Conclusions-Whole cell hybridisation of rRNA holds great promise for cultivation independent, reliable, and rapid (three hours) genotypic determination of clarithromycin resistance in H pylori. Compared with PCR techniques it is independent of nucleic acid preparations, not prone to inhibition, and allows semiquantitative visualisation of the bacteria within intact tissue samples.
引用
收藏
页码:608 / 614
页数:7
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