Production of recombinant urease for screening of helicobacter pylori infection

Production of recombinant urease for screening of helicobacter pylori infection

Helicobacter pylori establishes infection inside human stomach lining and causing duodenal diseases, such as peptic ulcer and potentially into gastric cancer. The invasive diagnostic methods require unpleasant endoscopic procedure for H. pylori detection. Preferably, the noninvasive diagnostic me...

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Main Author: Che Wan Sharifah Robiah, Mohamad
Format: Thesis
Language:English
Subjects:
Helicobacter pylori
Recombinant urease
Online Access:http://dspace.unimap.edu.my:80/xmlui/bitstream/123456789/44263/1/p.1-24.pdf
http://dspace.unimap.edu.my:80/xmlui/bitstream/123456789/44263/2/full%20text.pdf
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spelling my-unimap-442632016-12-01T01:13:44Z Production of recombinant urease for screening of helicobacter pylori infection Che Wan Sharifah Robiah, Mohamad Helicobacter pylori establishes infection inside human stomach lining and causing duodenal diseases, such as peptic ulcer and potentially into gastric cancer. The invasive diagnostic methods require unpleasant endoscopic procedure for H. pylori detection. Preferably, the noninvasive diagnostic methods would make suspected patients less stressful to procedure for H. pylori detection. The two most preferable noninvasive diagnostic methods are antibody detection (serology) and antigen detection (from fecal) with their own advantages and drawbacks. H. pylori urease is one of the antigens found in H. pylori with strong immunogenic property. Thus, urease was chosen for the development of H. pylori dot-EIA test strip which could be used in a serology based detection system for H. pylori infection. Cloning of urease A gene fragment (pET32ureA3), urease B gene fragment (pET32ureB2) and the whole of urease operon (pET32UOA6) produced biologically active recombinant urease A (UreA), recombinant urease B (UreB) and recombinant urease enzyme complex (UreA/UreB) verified by immune functioning assay using commercial antibody H. pylori urease-α and commercial antibody H. pylori urease-β from Santa Cruz, Inc, USA. The production of recombinant UreA/UreB complex indicates that a fully functional urease operon or a urease replicon was successfully constructed. Purifications of the recombinant ureases were successful and the purified recombinant ureases were still biologically active. The purified recombinant ureases were coated onto membranes in preparation of dot-EIA test strips. The prepared dot- EIA test strips gave brown colour dots indicating positive reactions when probed with commercial antibodies against ureases (Santa Cruz, Inc, USA). Nine rabbits were used to assess the immunogenicity properties of the recombinant ureases. Sera from the challenged animals gave positive detections on the prepared test strips, similar to detections using commercial antibodies, indicating the recombinant ureases could act as immunogens comparable to native ureases. Three groups containing three rabbits each were challenged with purified recombinant UreA, UreB or UreA/UreB respectively showed the presence of ureases antibodies in their sera on dot-EIA test strips. One rabbit that served as a negative control, challenged with bovine serum albumin (BSA), did not give positive reaction on dot-EIA test strip. To conclude, this study was successfully achieving all the objectives: cloning, expression and purification of functioning recombinant ureases, as well as, developing dot-EIA test strip. With the intention to develop user friendly, easy, cheap and fast detection; this dot-EIA test strip provides a foundation for further urease enzyme-linked serology based assay development as a mean for early screening. In addition, the constructed H. pylori urease replicon opened an opportunity for developing a genetically modified animal model to study H. pylori pathogenesis. Universiti Sains Malaysia (USM) 2014-09 Thesis en http://dspace.unimap.edu.my:80/xmlui/handle/123456789/44263 http://dspace.unimap.edu.my:80/xmlui/bitstream/123456789/44263/1/p.1-24.pdf ea4399b749bccc847e69145191402c47 http://dspace.unimap.edu.my:80/xmlui/bitstream/123456789/44263/2/full%20text.pdf 8089e2a8409ded1b4235a008917f2c26 http://dspace.unimap.edu.my:80/xmlui/bitstream/123456789/44263/3/license.txt 8a4605be74aa9ea9d79846c1fba20a33 Helicobacter pylori H. pylori urease H. pylori Recombinant urease School of Biological Sciences
institution Universiti Malaysia Perlis
collection UniMAP Institutional Repository
language English
topic Helicobacter pylori
Helicobacter pylori
Helicobacter pylori
Recombinant urease
spellingShingle Helicobacter pylori
Helicobacter pylori
Helicobacter pylori
Recombinant urease
Che Wan Sharifah Robiah, Mohamad
Production of recombinant urease for screening of helicobacter pylori infection
description Helicobacter pylori establishes infection inside human stomach lining and causing duodenal diseases, such as peptic ulcer and potentially into gastric cancer. The invasive diagnostic methods require unpleasant endoscopic procedure for H. pylori detection. Preferably, the noninvasive diagnostic methods would make suspected patients less stressful to procedure for H. pylori detection. The two most preferable noninvasive diagnostic methods are antibody detection (serology) and antigen detection (from fecal) with their own advantages and drawbacks. H. pylori urease is one of the antigens found in H. pylori with strong immunogenic property. Thus, urease was chosen for the development of H. pylori dot-EIA test strip which could be used in a serology based detection system for H. pylori infection. Cloning of urease A gene fragment (pET32ureA3), urease B gene fragment (pET32ureB2) and the whole of urease operon (pET32UOA6) produced biologically active recombinant urease A (UreA), recombinant urease B (UreB) and recombinant urease enzyme complex (UreA/UreB) verified by immune functioning assay using commercial antibody H. pylori urease-α and commercial antibody H. pylori urease-β from Santa Cruz, Inc, USA. The production of recombinant UreA/UreB complex indicates that a fully functional urease operon or a urease replicon was successfully constructed. Purifications of the recombinant ureases were successful and the purified recombinant ureases were still biologically active. The purified recombinant ureases were coated onto membranes in preparation of dot-EIA test strips. The prepared dot- EIA test strips gave brown colour dots indicating positive reactions when probed with commercial antibodies against ureases (Santa Cruz, Inc, USA). Nine rabbits were used to assess the immunogenicity properties of the recombinant ureases. Sera from the challenged animals gave positive detections on the prepared test strips, similar to detections using commercial antibodies, indicating the recombinant ureases could act as immunogens comparable to native ureases. Three groups containing three rabbits each were challenged with purified recombinant UreA, UreB or UreA/UreB respectively showed the presence of ureases antibodies in their sera on dot-EIA test strips. One rabbit that served as a negative control, challenged with bovine serum albumin (BSA), did not give positive reaction on dot-EIA test strip. To conclude, this study was successfully achieving all the objectives: cloning, expression and purification of functioning recombinant ureases, as well as, developing dot-EIA test strip. With the intention to develop user friendly, easy, cheap and fast detection; this dot-EIA test strip provides a foundation for further urease enzyme-linked serology based assay development as a mean for early screening. In addition, the constructed H. pylori urease replicon opened an opportunity for developing a genetically modified animal model to study H. pylori pathogenesis.
format Thesis
author Che Wan Sharifah Robiah, Mohamad
author_facet Che Wan Sharifah Robiah, Mohamad
author_sort Che Wan Sharifah Robiah, Mohamad
title Production of recombinant urease for screening of helicobacter pylori infection
title_short Production of recombinant urease for screening of helicobacter pylori infection
title_full Production of recombinant urease for screening of helicobacter pylori infection
title_fullStr Production of recombinant urease for screening of helicobacter pylori infection
title_full_unstemmed Production of recombinant urease for screening of helicobacter pylori infection
title_sort production of recombinant urease for screening of helicobacter pylori infection
granting_institution Universiti Sains Malaysia (USM)
granting_department School of Biological Sciences
url http://dspace.unimap.edu.my:80/xmlui/bitstream/123456789/44263/1/p.1-24.pdf
http://dspace.unimap.edu.my:80/xmlui/bitstream/123456789/44263/2/full%20text.pdf
_version_ 1747836830929125376

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