| HOME | HELP | FEEDBACK | SUBSCRIPTIONS | ARCHIVE | SEARCH | TABLE OF CONTENTS |
|
|
|
|||||||
|
|||||||||
Journal of Dental Research, Vol 69, 1839-1846, Copyright © 1990 by International & American Associations for Dental Research Online Journals
ARTICLES |
B. Mansson-Rahemtulla, F. Rahemtulla and M. G. Humphreys-Beher
Department of Community and Public Health Dentistry, University of Alabama School of Dentistry, Birmingham 35294.
Peroxidases are abundant in nature, and the primary function of mammalian peroxidases is to catalyze the peroxidation of halides and pseudohalides. Previous studies have shown that antibodies raised against bovine lactoperoxidase moderately cross-react with human salivary peroxidase, a feature that has been used in the present study to examine epitopes common to the antigen and human salivary peroxidase. Polyclonal antibodies against a highly purified preparation of bovine lactoperoxidase were raised in rabbits, and their properties were examined. In double-immunodiffusion experiments, the two enzymes showed partial identity, and in competitive radioimmunoassay and enzyme-linked immunosorbent assay, lactoperoxidase replaced the labeled and coated antigen, while salivary peroxidase did not. However, salivary peroxidase from human and rat saliva samples and the purified enzyme in its non-reduced, reduced, and de-glycosylated forms were recognized by these antibodies, as analyzed by Western blot analysis and immunodetection. The major activity of these antibodies was directed against the protein core of the antigen. Immunodetection of the peptide fragments of bovine lactoperoxidase and human salivary peroxidase revealed structural differences in the two enzymes. These antibodies also precipitated an in vitro translation product from rat-parotid-gland cell lysate that, on SDS-PAGE, compared favorably with the expected molecular weight of a de-glycosylated peroxidase. The antibodies partly inhibited the enzyme activity of salivary peroxidase and the peroxidase in rat parotid gland lysate, but the enzyme activity of lactoperoxidase was not affected by addition of anti-lactoperoxidase IgG between 25 and 400 micrograms/mL. The enzyme activity remained unchanged in all samples when pre-immune IgG was used.
This article has been cited by other articles:
|
|
 |
|
  K. Shin, H. Hayasawa, and B. Lonnerdal Purification and quantification of lactoperoxidase in human milk with use of immunoadsorbents with antibodies against recombinant human lactoperoxidase Am. J. Clinical Nutrition, May 1, 2001; 73(5): 984 - 989. [Abstract] [Full Text] [PDF]
|
|
|
|
 |
|
 J. E. Heath, F. Rahemtullah, and W. D. Fine Case Report: Carcinoma of the Extraorbital Lacrimal Gland in a Female Fischer 344 Rat Toxicol Pathol, November 1, 2000; 28(6): 824 - 826. [Abstract] [PDF]
|
|
|
|
 |
|
 C. Gerson, J. Sabater, M. Scuri, A. Torbati, R. Coffey, J. W. Abraham, I. Lauredo, R. Forteza, A. Wanner, M. Salathe, et al. The Lactoperoxidase System Functions in Bacterial Clearance of Airways Am. J. Respir. Cell Mol. Biol., June 1, 2000; 22(6): 665 - 671. [Abstract] [Full Text]
|
|
| HOME | HELP | FEEDBACK | SUBSCRIPTIONS | ARCHIVE | SEARCH | TABLE OF CONTENTS |
| IADR Journals | Advances in Dental Research ® |
| Journal of Dental Research ® | Critical Reviews (1990-2004) |
