A novel immunoassay based on monoclonal antibodies for the   detection of Helicobacter pylori antigens in human stool

K. Agha-Amiri; U. Peitz; D. Mainz; S. Kahl; A. Leodolter; P. Malfertheiner

doi:10.1055/s-2001-16629

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Z Gastroenterol 2001; 39(8): 555-560
DOI: 10.1055/s-2001-16629

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A novel immunoassay based on monoclonal antibodies for the detection of Helicobacter pylori antigens in human stool

Ein neuer Immunoassay, basierend auf monoklonalen Antikörpern, zum Nachweis von Helicobacter-pylori-Antigenen im menschlichen StuhlK. Agha-Amiri, U. Peitz, D. Mainz, S. Kahl, A. Leodolter, P. Malfertheiner

Department of Gastroenterology, Hepatology and Infectious Diseases, Otto-von-Guericke University, Magdeburg, Germany

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Publication History

20.11.2000

26.3.2001

Publication Date:
27 August 2001 (online)

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Abstract
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Summary

Background and Aim: With the Premier Platinum HpSA EIA™ a new enzyme immunoassay was developed for diagnosis of H. pylori infection, using polyclonal antibodies against H. pylori antigens in human stool. Here we evaluated FemtoLab H. pylori™ based on the use of monoclonal antibodies in comparison to established reference methods.

Methods: 53 consecutive patients (27male, 26 female, age: 17-85 years) undergoing routine upper gastrointestinal endoscopy were enrolled in this study. The H. pylori status was determined by 4 reference methods: Histology, rapid urease test (HUT), ¹³C-urea breath test (¹³C-UBT) and serology. Patients were considered to be infected with H. pylori if at least 2 of the 4 reference tests were positive. Stool samples were aliquoted after reception and stored frozen (-20 °C) until tested. The FemtoLab H. pylori™ (Connex GmbH, Germany) and the Premier Platinum HpSA EIA™ (Meridian, Connecticut, Ohio, USA) were performed according to the manufacturers protocols. Results: 26 of the 53 patients were H. pylori infected. 3 were false-negative by the FemtoLab H. pylori™ and one false-positive result was obtained (sensitivity 88,5 %, specificity 96,3 %). The concordance between the 2 stool tests was 94,3 % (50/53 cases). Conclusion: The diagnostic quality of the novel FemtoLab H. pylori™ Enzyme Immunoassay is comparable with the established Premier Platinum HpSA EIA™. The differences between positive and negative results obtained with the FemtoLab H. pylori™ are greater in comparison to the Premier Platinum HpSA EIA™ and therefore this test system allows a better distinction.

Ein neuer Immunoassay, basierend auf monoklonalen Antikörpern, zum Nachweis von Helicobacter-pylori-Antigenen im menschlichen Stuhl

Hintergrund und Ziel: Durch die Entwicklung des Premier Platinum HpSA EIA™, gelang der Nachweis spezifischer Helicobacter-pylori-(H. pylori)Antigene mittels polyklonaler Antikörper im Stuhl. In dieser Arbeit überprüften wir die diagnostische Treffsicherheit des FemtoLab H. pylori™, der auf der Verwendung monoklonaler Antikörper beruht, im Vergleich zu den etablierten Standardverfahren.

Methodik: 53 konsekutive Patienten (27 m, 26 w, Alter: 17-85 Jahre), die routinemäßig eine Ösophagogastroduodenoskopie erhielten, wurden in diese Untersuchung eingeschlossen. Der H.-pylori-Status wurde anhand der 4 Referenzmethoden - der Histologie, dem Helicobacter-Urease-Schnelltest (HUT), dem ¹³C-Harnstoff-Atemtest (¹³C-UBT) und der Serologie - ermittelt. Patienten gelten als mit H. pylori infiziert, wenn 2 von 4 Referenzmethoden positiv sind. Stuhlproben wurden portioniert und bei -20 ^°C bis zur Durchführung des Tests gelagert. Der FemtoLab H. pylori™ (Connex GmbH, Germany) und der Premier Platinum HpSA EIA™ (Meridian, Connecticut, Ohio, USA) wurden entsprechend der vom Hersteller angegebenen Anleitung durchgeführt. Ergebnisse: 26 der 53 Patienten waren mit H. pylori infiziert. 3 Ergebnisse waren falsch negativ im FemtoLab H. pylori™ und ein Ergebnis falsch positiv (Sensitivität 88,5 %, Spezifität 96,3 %). Die Qualität zwischen den beiden Stuhltests ergab 94,3 % (50/53 Proben). Schlussfolgerung: Die diagnostische Qualität des FemtoLab H. pylori™ (Connex GmbH, Germany) ist vergleichbar mit der des Premier Platinum HpSA EIA™. Die gemessenen Differenzen (OD₄₅₀) zwischen positiven und negativen Ergebnissen im FemtoLab H. pylori™ sind größer als beim HpSA-Enzym-Immunoassay™, sodass eine bessere Unterscheidung zwischen positiven und negativen Ergebnissen möglich ist.

Key words

Helicobacter pylori - Diagnosis - Feces - EIA

Schlüsselwörter

Heliobacter pylori - Diagnostik - Stuhl - EIA

Literature

1 Rauws E A, Tytgat G N. Cure of duodenal ulcer associated with eradication of Helicobacter pylori. Lancet. 1990; 335 1233-1235

Search in Google Scholar
2 Borody T J, Cole P, Noonan S. et al . Recurrence of duodenal ulcer and Campylobacter pylori infection after eradication. Med J Aust. 1989; 151 431-435

Search in Google Scholar
3 Bayerdorffer E, Neubauer A, Rudolph B. et al . Regression of primary gastric lymphoma of mucosa-associated lymphoid tissue type after cure of Helicobacter pylori infection. MALT Lymphoma Study Group. Lancet. 1995; 345 1591-1594

Search in Google Scholar
4 Graham D Y, Lew G M, Klein P D. et al . Effect of treatment of Helicobacter pylori infection on the long-term recurrence of gastric or duodenal ulcer. A randomized, controlled study. Ann Intern Med. 1992; 116 705-708

Search in Google Scholar
5 Jones R, Tait C, Sladen G, Weston-Baker J. A trial of a test-and-treat strategy for Helicobacter pylori positive dyspeptic patients in general practice. Int J Clin Pract. 1999; 53 413-416

Search in Google Scholar
6 Joosen E A, Reininga J H, Manders J M, ten Ham J C, de Boer W A. Costs and benefits of a test-and-treat strategy in Helicobacter pylori-infected subjects: A prospective intervention study in general practice. Eur J Gastroenterol Hepatol. 2000; 12 319-325

Search in Google Scholar
7 Feldman R A, Deeks J J, Evans S J. Multi-laboratory comparison of eight commercially available Helicobacter pylori serology kits. Helicobacter pylori Serology Study Group. Eur J Clin Microbiol Infect Dis. 1995; 14 428-433

Search in Google Scholar
8 Logan R P. Urea breath tests in the management of Helicobacter pylori infection. Gut. 1998; 43 (Suppl. 1) S47-50

Search in Google Scholar
9 Makristathis A, Pasching E, Schutze K. et al . Detection of Helicobacter pylori in stool specimens by PCR and antigen enzyme immunoassay. J Clin Microbiol. 1998; 36 2772-2774

Search in Google Scholar
10 Chang M C, Wu M S, Wang H H, Wang H P, Lin J T. Helicobacter pylori stool antigen (HpSA) test - a simple, accurate and non-invasive test for detection of Helicobacter pylori infection. Hepatogastroenterology. 1999; 46 299-302

Search in Google Scholar
11 Vaira D, Malfertheiner P, Megraud F. et al . Diagnosis of Helicobacter pylori infection with a new non-invasive antigen-based assay. HpSA European study group. Lancet. 1999; 354 30-33

Search in Google Scholar
12 Fanti L, Mezzi G, Cavallero A. et al . A new simple immunoassay for detecting Helicobacter pylori infection: Antigen in stool specimens. Digestion. 1999; 60 456-460

Search in Google Scholar
13 Malfertheiner P, Enrique Dominguez-Munoz J J. et al . Modified rapid urease test for detection of Helicobacter pylori infection. Eur J Gastroenterol Hepatol. 1996; 8 53-56

Search in Google Scholar
14 Leodolter A, Dominguez-Munoz J E, von Arnim U, Manes G, Malfertheiner P. 13C-urea breath test for the diagnosis of Helicobacter pylori infection. A further simplification for clinical practice. Scand J Gastroenterol. 1998; 33 267-270

Search in Google Scholar
15 Dixon M F, Genta R M, Yardley J H, Correa P. Classification and grading of gastritis. The updated Sydney System. International Workshop on the Histopathology of Gastritis, Houston 1994. Am J Surg Pathol. 1996; 20 1161-1181

Search in Google Scholar
16 Genta R M, Gurer I E, Graham D Y. et al . Adherence of Helicobacter pylori to areas of incomplete intestinal metaplasia in the gastric mucosa. Gastroenterology. 1996; 111 1206-1211

Search in Google Scholar
17 Braden B, Teuber G, Dietrich C F, Caspary W F, Lembcke B. Comparison of new faecal antigen test with (13)C-urea breath test for detecting Helicobacter pylori infection and monitoring eradication treatment: prospective clinical evaluation. BMJ. 2000; 320 148

Search in Google Scholar
18 Vaira D, Malfertheiner P, Megraud F. et al . Noninvasive antigen-based assay for assessing Helicobacter pylori eradication: A European multicenter study. The European Helicobacter pylori HpSA Study Group. Am J Gastroenterol. 2000; 95 925-929

Search in Google Scholar
19 Ishihara S, Kaji T, Kawamura A. et al . Diagnostic accuracy of a new non-invasive enzyme immunoassay for detecting Helicobacter pylori in stools after eradication therapy. Aliment Pharmacol Ther. 2000; 14 611-614

Search in Google Scholar
20 Ni Y H, Lin J T, Huang S F, Yang J C, Chang M H. Accurate diagnosis of Helicobacter pylori infection by stool antigen test and 6 other currently available tests in children. J Pediatr. 2000; 136 823-827

Search in Google Scholar
21 Braden B, Posselt H G, Ahrens P. et al . New immunoassay in stool provides an accurate noninvasive diagnostic method for Helicobacter pylori screening in children. Pediatrics. 2000; 106 115-117

Search in Google Scholar

Prof. Dr. P. Malfertheiner

Klinik für Gastroenterologie, Hepatologie und Infektiologie
Otto-von-Guericke-Universität

Leipziger Straße 44, Haus 39

39120 Magdeburg

Fax: +49/391/6713105