Cloning of the Gene Encoding Urease Subunit A in Helicobacter Pylori

Cloning of the Gene Encoding Urease Subunit A in Helicobacter Pylori

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摘要 The gene encoding urease subunit A (ureA) of Helicobacter pylori (H.pylori) was cloned from H.pylori isolate by polymerase chain reaction (PCR). Sterile distilled water instead of DNA served as negative control. The nucleotide sequence of the amplified product was determined. Homologous analysis of the ureA against that reported by Clayton CL and the GenBank and SwissProt databases were performed with the BLAST program at the Genome Net through the Internet. 0.8 kb PCR product was amplified from all H.pylori clinical isolators. The nucleotide sequence of the ureA was determined. The nucleotide sequence of the ureA began with ATG as the initiation codon and terminated in TAA as stop codon. The coding regions had a 44 % G+C content. The DNA sequence was 98 % homologous to that reported by Clayton CL (688 out of 702 residues were identical). The derived amino acid sequences of the ureA were 99 % homologous to that reported by Clayton CL (232 out of 234 residues were identical). The nucleotide sequence and the predicted protein showed significant homology to ureA of H.pylori in the NCBI Entrez database. The gene encoding urease subunit A (ureA) of Helicobacter pylori (H.pylori) was cloned from H.pylori isolate by polymerase chain reaction (PCR). Sterile distilled water instead of DNA served as negative control. The nucleotide sequence of the amplified product was determined. Homologous analysis of the ureA against that reported by Clayton CL and the GenBank and SwissProt databases were performed with the BLAST program at the Genome Net through the Internet. 0.8 kb PCR product was amplified from all H.pylori clinical isolators. The nucleotide sequence of the ureA was determined. The nucleotide sequence of the ureA began with ATG as the initiation codon and terminated in TAA as stop codon. The coding regions had a 44 % G+C content. The DNA sequence was 98 % homologous to that reported by Clayton CL (688 out of 702 residues were identical). The derived amino acid sequences of the ureA were 99 % homologous to that reported by Clayton CL (232 out of 234 residues were identical). The nucleotide sequence and the predicted protein showed significant homology to ureA of H.pylori in the NCBI Entrez database.

作者施理张宜俊陈劼候晓华

机构地区 Infective Disease Center Guangzhou Chinese Traditional Medical University Department of Digestive Disease

出处《Journal of Huazhong University of Science and Technology(Medical Sciences)》 SCIE CAS 2004年第1期22-24,共3页 华中科技大学学报（医学英德文版）

基金 ThisprojectwassupportedbyagrantfromNationalNaturalSciencesFoundationofChina (No.395 70 334)

关键词 Helicobacter pylori gene encoding urease subunit A CLONE PCR Helicobacter pylori gene encoding urease subunit A clone PCR

分类号 R346 [医药卫生—基础医学]

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Cloning of the Gene Encoding Urease Subunit A in Helicobacter Pylori

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