Comparison of PCR-restriction fragment length polymorphism analysis and PCR-direct sequencing methods for differentiating Helicobacter pylori ureB gene variants
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Tanahashi, T
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机构:Kyoto Prefectural Univ Med, Dept Internal Med 3, Kamigyo Ku, Kyoto 6028566, Japan
Tanahashi, T
Kita, M
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机构:Kyoto Prefectural Univ Med, Dept Internal Med 3, Kamigyo Ku, Kyoto 6028566, Japan
Kita, M
Kodama, T
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机构:Kyoto Prefectural Univ Med, Dept Internal Med 3, Kamigyo Ku, Kyoto 6028566, Japan
Kodama, T
Sawai, N
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机构:Kyoto Prefectural Univ Med, Dept Internal Med 3, Kamigyo Ku, Kyoto 6028566, Japan
Sawai, N
Yamaoka, Y
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机构:Kyoto Prefectural Univ Med, Dept Internal Med 3, Kamigyo Ku, Kyoto 6028566, Japan
Yamaoka, Y
Mitsufuji, S
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机构:Kyoto Prefectural Univ Med, Dept Internal Med 3, Kamigyo Ku, Kyoto 6028566, Japan
Mitsufuji, S
Katoh, F
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机构:Kyoto Prefectural Univ Med, Dept Internal Med 3, Kamigyo Ku, Kyoto 6028566, Japan
Katoh, F
Imanishi, J
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机构:Kyoto Prefectural Univ Med, Dept Internal Med 3, Kamigyo Ku, Kyoto 6028566, Japan
Imanishi, J
机构:
[1] Kyoto Prefectural Univ Med, Dept Internal Med 3, Kamigyo Ku, Kyoto 6028566, Japan
[2] Kyoto Prefectural Univ Med, Dept Microbiol, Kamigyo Ku, Kyoto 6028566, Japan
[3] Nippon Shinyaku Co Ltd, Res Labs, Kyoto 6018550, Japan
A method utilizing PCR-restriction fragment length polymorphism (RFLP) in the Helicobacter pylori genes is widely used to differentiate strains. However, with this typing method only a single base change at a specific restriction site can be detected. In addition, it is unclear whether the nucleotide base change recognized by RFLP is related to a substitution of encoded amino acid. To examine the validity of the PCR-RFLP method, 933-bp PCR products mere obtained from 41 different clinical H. pylori isolates and were digested with Sau3A restriction endonuclease. Furthermore, the nucleotides of the same region in the ureB gene were directly sequenced and compared. PCR-RFLP confirmed that there was genetic diversity within the ureB gene with three distinct types, one being well conserved and the other two being variations. However, the direct sequencing method revealed that there,vas no difference at the nucleotide level among these RFLP types. Base substitutions recognized by Sau3A occurred in the third-base position and did not change the encoded amino acid. In addition, many nucleotide mutations, which could not be recognized by Sau3A,were frequently found. These results suggest that the PCR-RFLP method pro,ides for an easy typing scheme of isolates, but does not reveal the true extent of genetic diversity. It is proposed that careful observation is required for the interpretation of results when clinical isolates are differentiated.
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Univ Int La Rioja UNIR, ESIT, Logrono 26006, SpainUniv Int La Rioja UNIR, ESIT, Logrono 26006, Spain
Garcia-Suarez, Maria del Mar
Gonzalez-Rodriguez, Irene
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IPLA, Villaviciosa 33300, SpainUniv Int La Rioja UNIR, ESIT, Logrono 26006, Spain
Gonzalez-Rodriguez, Irene
Cima-Cabal, Maria Dolores
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Univ Int La Rioja UNIR, ESIT, Logrono 26006, SpainUniv Int La Rioja UNIR, ESIT, Logrono 26006, Spain
Cima-Cabal, Maria Dolores
Yuste, Jose Enrique
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Inst Salud Carlos III, Ctr Nacl Microbiol, Madrid 28220, Spain
CIBERES, CIBER Enfermedades Resp, Madrid 28029, SpainUniv Int La Rioja UNIR, ESIT, Logrono 26006, Spain