Saliva Altered Clinical Trial
Official title:
Astringency Perception and Oral Health
Verified date | March 2024 |
Source | Rutgers, The State University of New Jersey |
Contact | n/a |
Is FDA regulated | No |
Health authority | |
Study type | Interventional |
The perception of astringency is thought to involve the interaction between tannins and salivary proteins. However, the mechanisms underlying this interaction are poorly understood. The tannins' subclass known as type A proanthocyanidins seems to have a positive effect on human health. Despite that, humans show large individual differences in the sensory perception and acceptance of astringent foods such as tea, wine and chocolate suggesting that this variation may have a genetic basis. Salivary proteins play an essential role both in affecting oral taste perception and in maintaining a healthy oral environment. Diverse microorganisms inhabit the oral cavity. The interactions between oral microbiota, host and environmental factors influence microbial homeostasis and ultimately human oral health. Understanding individual differences in salivary proteins, oral microbiome and the mechanisms by which tannins evoke the perception of astringency could provide important insights into the role of these compounds in human nutrition and health.
Status | Completed |
Enrollment | 49 |
Est. completion date | November 14, 2023 |
Est. primary completion date | November 14, 2023 |
Accepts healthy volunteers | Accepts Healthy Volunteers |
Gender | All |
Age group | 18 Years to 50 Years |
Eligibility | Inclusion Criteria: - PROP insensitive individuals (PROP non-tasters; homozygous recessive for TAS2R38 gene) - PROP high-sensitive individuals (PROP super-tasters; homozygous dominant for TAS2R38 gene) - Overall healthy; good oral health and hygiene routine - Current on a routine checkup by a oral/dental health professional - Recently underwent dental/cleaning by a oral/dental health professional - No ongoing oral health problems - Agree to use intervention material as prescribed - Agree to refrain from using any other oral rinse material during the term of the study Exclusion Criteria: - PROP medium-taster individuals (heterozygous for TAS2R38 gene) - Taste or smell dysfunction - Pregnant or nursing - Oral piercings - Smoking - Use of medications other than birth control |
Country | Name | City | State |
---|---|---|---|
United States | Rutgers University, Department of Food Science | New Brunswick | New Jersey |
Lead Sponsor | Collaborator |
---|---|
Rutgers, The State University of New Jersey |
United States,
Type | Measure | Description | Time frame | Safety issue |
---|---|---|---|---|
Primary | Change from Baseline Taste and Flavor Intensity Ratings after 11 days | Taste and flavor intensity ratings of cranberry juice and aronia juice samples will be collected 3 days after control intervention and then at the end of the experimental intervention. An end-anchored (None, Very Strong) 15 cm line scale will be used with taste and key flavor attributes. | Baseline measure 3 days after control intervention; Post intervention measure 11 days after experimental intervention | |
Primary | Change from Baseline Levels of Salivary Proteins after 11 days | Saliva will be collected 3 days after control intervention and then at the end of the experimental intervention. Samples will be analyzed via dot blot analysis and LC-MS (liquid chromatography-mass spectrometry) to establish proteomic composition before and after the intervention. Specifically, area of the ion current peaks (XIC peaks) generated will be used as a relative quantity of the salivary protein levels. The XIC peaks are proportional to the concentration of salivary proteins under constant conditions and will be used to understand the effect of the intervention on salivary protein levels. | Baseline measure 3 days after control intervention; Post intervention measure 11 days after experimental intervention | |
Primary | Change from Baseline Composition of Oral Microbiome after 11 days | Salivary samples will be collected 3 days after control intervention and then at the end of the experimental intervention. Samples will be analyzed for microbial composition via Whole Genome Sequencing and data used to understand changes in microbial diversity before and after the intervention. Specifically operational taxonomic units will be identified and classified at the species level. | Baseline measure 3 days after control intervention; Post intervention measure 11 days after experimental intervention |
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