4.7 Article

Whole-saliva Proteolysis and Its Impact on Salivary Diagnostics

Journal

JOURNAL OF DENTAL RESEARCH
Volume 90, Issue 11, Pages 1325-1330

Publisher

SAGE PUBLICATIONS INC
DOI: 10.1177/0022034511420721

Keywords

biochemistry; biomarkers; enzymology; proteolysis; saliva; salivary diagnostics

Funding

  1. NIH/NIDCR/NIAID [DE14950, DE17788, DE05672, DE07652, DE18132, AI087803]
  2. Canadian Institutes of Health Research (CIHR) [106657, 97577]

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There is growing interest in the use of human whole saliva for diagnostics and disease monitoring as an alternative to blood samples. In contrast to blood, whole saliva is a non-sterile body fluid. Proper hand-ling and storage are required to preserve the integrity of potential biomarkers. We investigated salivary autoproteolytic degradation using a variety of approaches. We determined inhibition of protease activities by monitoring the endogenous proteome. In addition, the stability of highly protease-susceptible proteins-histatin 5, statherin, and PRP1-was assessed. Experimental variables included (a) protease inhibitors, (b) salivary pH, (c) incubation temperatures, and (d) sample heating. A cocktail containing AEBSF, aprotinin, pancreatic trypsin inhibitor, leupeptin, antipain, and EDTA could not prevent histatin 5, statherin, or PRP1 degradation in whole saliva. Among the other treatments evaluated, short-term storage of freshly collected samples on ice was effective without interfering with the chemistry of the proteome. In conclusion, whole saliva contains a unique mixture of enzymes as evidenced from their resilience to protease inhibition. Analytical evidence on protein stability is needed to ensure the validity of salivary biomarker study outcomes. Analysis of the data presented will provide help and guidance for the use of saliva samples for diagnostic purposes.

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