Shuttle cloning and nucleotide sequences of Helicobacter pylori genes responsible for urease activity

Labigne, Agnès; Cussac, V.; Courcoux, P.

doi:10.1128/jb.173.6.1920-1931.1991

Cited by 390 publications

(334 citation statements)

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“…Mycobacreriurn leprea (GenBank accession no. U00020), Helicobacrerpylori (Labigne et al, 1991). Escherichia coli (GlmM, Dallas et al, 1993;PGM, Lu & Kleckner, 1994).…”

Section: Isolation and Amino-terminal Sequence Analysis Of The 35-andmentioning

confidence: 99%

Archaeal phosphoproteins. Identification of a hexosephosphate mutase and the α‐subunit of succinyl‐CoA synthetase in the extreme acidothermophile Sulfolobus solfataricus

Solow¹,

Bischoff²,

Zylka³

et al. 1998

Protein Science

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When soluble extracts from the extreme acidophilic archaeon Sulfolobus solfataricus were incubated with [Y-'~P]ATP, several radiolabeled polypeptides were observed following SDS-PAGE. The most prominent of these migrated with apparent molecular masses of 14, 18, 35, 42, 46, 50, and 79 kDa. Phosphoamino acid analysis revealed that all of the proteins contained phosphoserine, with the exception of the 35-kDa one, whose protein-phosphate linkage proved labile to strong acid. The observed pattern of phosphorylation was influenced by the identity of the divalent metal ion cofactor used, Mg2+ versus Mn2+, and the choice of incubation temperature. The 35-and 50-kDa phosphoproteins were purified and their amino-terminal sequences determined. The former polypeptide's amino-terminal sequence closely matched a conserved portion of the a-subunit of succinyl-CoA synthetase, which forms an acid-labile phosphohistidyl enzyme intermediate during its catalytic cycle. This identification was confirmed by the ability of succinate or ADP to specifically remove the radiolabel. The 50-kDa polypeptide's sequence contained a heptapeptide motif, Phe/Pro-Gly-ThrAsp/Ser-Gly-Val/Leu-Arg, found in a similar position in several hexosephosphate mutases. The catalytic mechanism of these mutases involves formation of a phosphoseryl enzyme intermediate. The identity of p50 as a hexosephosphate mutase was confirmed by (1) the ability of sugars and sugar phosphates to induce removal of the labeled phosphoryl group from the protein, and (2) the ability of [32P]glucose 6-phosphate to donate its phosphoryl group to the protein.Keywords: Archaea; Archaebacteria; hexosephosphate mutase; phosphoprotein; succinyl-CoA synthetase Phosphate represents one of nature's most versatile and important chemical moieties (Westheimer, 1987). It comprises (1) the basic unit for the cell's energy currency, ( 2 ) a key chemical activator of organic functional groups in biocatalysis, (3) a charge-rich anchor for confining biomolecules within the cell membrane, (4) the linker that holds together the polymers that encode genetic information, and (5) a molecular switch for modulating the functional properties of key proteins. Although our general appreciation of the importance of phosphate in living organisms extends to the members of the Archaea-the third, most recent, phylogenetic domain to be recognized (Olsen & Woese, 1993)-in many areas, specific information is lacking. This is particularly true with regard to the interactions of phosphate with archaeal proteins. Only recently have archaeal phosphoproteins begun to be identified. The first was a CheA-like histidine kinase that functions as part of a twocomponent signal transduction cascade in Halobacterium salinarium Reprint requests to: Peter J. Kennelly, Department of Biochemistry, Virginia Polytechnic Institute and State University, 123 Engel Hall, Blacksburg, Virginia 24061-0308; e-mail: pjkennel@vt.edu. (Rudolph & Oesterhelt, 1995). The second was a methyltransferase activation protein from Methanosarcina...

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“…Mycobacreriurn leprea (GenBank accession no. U00020), Helicobacrerpylori (Labigne et al, 1991). Escherichia coli (GlmM, Dallas et al, 1993;PGM, Lu & Kleckner, 1994).…”

Section: Isolation and Amino-terminal Sequence Analysis Of The 35-andmentioning

confidence: 99%

Archaeal phosphoproteins. Identification of a hexosephosphate mutase and the α‐subunit of succinyl‐CoA synthetase in the extreme acidothermophile Sulfolobus solfataricus

Solow¹,

Bischoff²,

Zylka³

et al. 1998

Protein Science

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“…Forward primer (5'-TG GGACTGATGGCGTGAGGG-3') and reverse primer (5'-AAGGGCGTTTTTAGATTTTT-3') were prepared from the urease gene sequence according to the report of Labigne et al [14] . PCR amplification was carried out in a total volume of 50 μL containing 2 μL of 2 mmol/L dNTPs, 1 μL containing 50 ρmol of primer 1, 1 μL containing 50 ρmol of primer 2 (synthesized by ABI Automatic synthesizer), 1 unit of Taq DNA polymerase (Promega), 5 μL of 10 × PCR reaction buffer, 3 mmol/L of MgCl2, 2 μL of DNA template containing 0.5 ng of extracted DNA and total volume rounded to 50 μL by double distilled water.…”

Section: Extraction Of Dna From Gastric Biopsymentioning

confidence: 99%

Gastric juice for the diagnosis of H pylori infection in patients on proton pump inhibitors

Yakoob¹,

Rasool²,

Abbas³

et al. 2008

WJG

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H pylori is a spiral gram negative microaerophilic bacterium that infects the human gastric mucosa and is associated with gastritis, gastroduodenal ulcer disease, gastric carcinoma and mucosal associated lymphoid tissue lymphoma [1,2] . The prevalence of H pylori is high in developing countries. A recent study revealed an early colonization/infection of infants with H pylori and a prevalence of 67% at 9 mo of age in a peri-urban community in Karachi, Pakistan [3] . H pylori serology was positive in 58% of our general population in a previous study but is likely to actually be higher [4] . Currently, several diagnostic tests of varying sensitivity and specificity are available for determining the presence of H pylori, which include rapid urease test (RUT), histology, culture, urea breath test (UBT), and serology. Isolation of H pylori from gastric biopsy specimens constitutes the most specific way to establish the diagnosis of infection and to study the genotype of the infecting strains, however, it is a time consuming process. RUT and histology are still commonly used for the diagnosis of H pylori infection in our country as other modalities of H pylori testing, such as UBT and facilities for H pylori stool antigen tests, are not widely available.In Pakistan, self-prescription is common and medications are available over the counter without prescriptions [5] . It is known that acid reducing drugs; e.g, proton pump inhibitor (PPI), histamine-2 receptor blocker (H2RB), antibiotics and bismuth compounds reduce the sensitivity and specificity of the diagnostic tests for H pylori [6,7] . In our previous studies, we demonstrated that histology is comparatively less affected by PPI than RUT [8,9] . Polymerase chain reaction (PCR) is a highly

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“…Variation at the ureA locus Genomic DNAs of all strains were digested with Hind III, which was predicted by analysis of the published nucleotide sequences [10,11] to lack a recognition site within the 411 bp internal fragment of the ureA gene of H. pylori. In genomic Southern blots, the ureA-411 probe hybridized to one Hind III fragment in each of the 64 strains.…”

Section: Resiultsmentioning

confidence: 99%

“…They are among four genes which are located in a 4-2 kb DNA region, which confers urease activity when genetically transferred to Campylobacter jejuni, a related species which lacks the enzyme. These four genes have been sequenced from H. pylori strain 85P [11] and their order in the chromosome is ure CDAB. This study examined strains isolated from patients with one of two major disease syndromes (gastroduodenal ulcer and gastritis), and asymptomatic subjects infected by H. pylori.…”

Section: Introductionmentioning

confidence: 99%

“…Similarly, a 1 7 kb fragment spanning the ureC and ureD genes (hereafter termed 'ureCD-1P7'), and corresponding to nt 521 to 2240 of the sequence of Labigne and co-workers [11], was amplified using the primers 5'-TGGGACTGATGGCGTGAGGG-3' and 5'-ATCATGACATCAG-CGAAGTTAAAAATGG-3' [14]. Amplification was carried out from 50 ng of genomic DNA of H. pylori NCTC 11637T.…”

Section: Introductionmentioning

confidence: 99%

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Molecular typing ofHelicobacter pyloriisolates from asymptomatic, ulcer and gastritis patients by urease gene polymorphism

et al. 1994

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SUMMARYThe gastric-adapted bacterium Helicobacter pylori plays an important role in gastritis and ulcer disease, but no phenotypic typing scheme presently exists for this organism. With a view to the development of genotypic typing, we have compared isolates of H. pytori from gastritis or ulcer patients with those from subjects exhibiting no disease. Variation was analysed at the urease genes, ureA and ureCD, by employing PCR-generated probes in genomic Southern blot hybridizations. Whilst ureA restriction fragments provided a fourfold subgrouping of strains, ureCD fragments were considerably more discriminatory. Twenty-four combined ureACD profiles were generated with Hind III, subdividing the 64 strains into 11 types and 13 single profiles. The most prevalent profile (UI) was found in 33 % of strains, almost all from gastritis or ulcer patients. On the other hand strains isolated from asymptomatic individuals had the most diverse ureACD profiles. A key finding from this set of isolates was that strains of H. pylori associated with general gastroduodenal disease were genetically more homogeneous than strains carried by people without disease symptoms. INTRODUCTIONThe Gram-negative bacterium Helicobacter pylori was first isolated in 1982 by Warren and Marshall [1]. Endoscopic and seroprevalence analyses indicate that this organism has a worldwide distribution, and is frequently isolated from asymptomatic persons [2]. By the age of 60 years, 40-60% of adult humans in developed countries show evidence of H. pylori infection without necessarily showing signs of disease [3]. The presence of the bacterium has however been causally associated with type B gastritis and is a contributing factor in peptic

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Shuttle cloning and nucleotide sequences of Helicobacter pylori genes responsible for urease activity

Cited by 390 publications

References 51 publications

Archaeal phosphoproteins. Identification of a hexosephosphate mutase and the α‐subunit of succinyl‐CoA synthetase in the extreme acidothermophile Sulfolobus solfataricus

Archaeal phosphoproteins. Identification of a hexosephosphate mutase and the α‐subunit of succinyl‐CoA synthetase in the extreme acidothermophile Sulfolobus solfataricus

Gastric juice for the diagnosis of H pylori infection in patients on proton pump inhibitors

Molecular typing ofHelicobacter pyloriisolates from asymptomatic, ulcer and gastritis patients by urease gene polymorphism

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