Inflammation Clinical Trial
Official title:
Suppression of Postprandial Monocyte Activation by Fruit Rich in Anti-inflammatory Polyphenols or Docosahexaenoic Acid in Humans
| Verified date | October 2018 |
| Source | USDA, Western Human Nutrition Research Center |
| Contact | n/a |
| Is FDA regulated | No |
| Health authority | |
| Study type | Interventional |
The overall goal of the research study is to determine whether a high-fat meal causes postprandial (after meal) inflammation, and whether eating n-3 polyunsaturated fatty acids (PUFAs) or blueberries that are rich in anti-inflammatory polyphenols suppress the inflammation in healthy people.
| Status | Completed |
| Enrollment | 62 |
| Est. completion date | November 2017 |
| Est. primary completion date | November 2017 |
| Accepts healthy volunteers | Accepts Healthy Volunteers |
| Gender | All |
| Age group | 18 Years to 60 Years |
| Eligibility |
Inclusion Criteria: - Body Mass Index of 18-25 kg/m2 - Complete Blood Count (CBC) within normal limits - Blood chemistry panel within normal limits Exclusion Criteria: - following a vegetarian diet - smoke or use tobacco products - consume more than one alcoholic beverage per day (defined as 1 oz. distilled liquor, 3 oz. wine, or 12 oz. beer) - taking any cholesterol lowering - taking blood pressure medication - taking non-steroidal anti-inflammatory drugs (NSAIDS) more than once a week and for 3 days before each test day - taking steroids for asthma or other inflammatory states - taking thyroid-regulating drugs - taking over-the-counter weight loss products - allergies or sensitivities to foods or ingredients in the test meals, especially blueberries or DHA - taking fish or algae oil or other dietary supplements and unwilling to stop the supplements for the duration of the study (multivitamin is OK) - Women who are pregnant, lactating or planning a pregnancy - fasting blood cholesterol greater than 240 mg/dL - fasting blood triglyceride greater than 300mg/dL - hemoglobin less than 11.5 mg/dL - blood pressure greater than 140/90 mmHg - metabolic diseases such as diabetes mellitus, hypothyroidism, kidney disease, liver disease, bleeding disorders, autoimmune diseases, other inflammatory disease, or cancer unless greater than 5 years remission |
| Country | Name | City | State |
|---|---|---|---|
| United States | USDA, ARS, Western Human Nutrition Research Center | Davis | California |
| Lead Sponsor | Collaborator |
|---|---|
| USDA, Western Human Nutrition Research Center | University of California, Davis |
United States,
| Type | Measure | Description | Time frame | Safety issue |
|---|---|---|---|---|
| Primary | Change in Monocyte activation in whole blood | Change in monocyte activation using monocyte activation assay in whole blood. | Measured at 0, 1, 3, and 6 hours after high fat meal with blueberries, DHA or placebo | |
| Secondary | Change in surface markers for monocyte activation | Surface markers for monocyte activation will be measured by flow cytometry. Surface markers may include cluster of differentiation (CD) 14 (CD14), CD11c, CD11b and CD62 Ligand (CD62L) to assess monocyte activation and M1 and M2 macrophage marker proteins. | Measured at 0, 1, 3, and 6 hours after high fat meal with blueberries, DHA or placebo | |
| Secondary | Change in systemic inflammation | Inflammatory mediators measured in whole blood or blood plasma. Inflammatory mediators include cytokines such as Interleukin-1ß, Tumor Necrosis Factor-alpha, Interferon-gamma, Interleukin-6, Interleukin-8, Th1, Th2 and Th17. | Measured at 0, 1, 3, and 6 hours after high fat meal with blueberries, DHA or placebo | |
| Secondary | Change in systemic inflammation measured indirectly | The magnitude of the inhibition of cytokine production after 24 hour incubation of whole blood by endotoxin inhibitor, polymyxin B (PMB), is measured as an indirect assessment of endotoxin concentration. Cytokine concentrations in whole blood after 24 hour incubation with lipoprotein lipase and PMB is used to assess whether increased concentrations of non-esterified fatty acids (NEFA) and saturated fatty acids stimulate cytokine production. | Measured at 0, 3, and 6 hours after high fat meal with blueberries, DHA or placebo | |
| Secondary | Change in gene expression profile in whole blood | Gene expression measured using RNA sequencing | Measured at 0, 1, 3, and 6 hours after high fat meal with blueberries, DHA or placebo | |
| Secondary | Change in blood lipids | Lipids, total non-esterified fatty acids, and individual fatty acids measured in blood | Measured at 0, 1, 3, and 6 hours after high fat meal with blueberries, DHA or placebo | |
| Secondary | Change in endothelial function measurements | Endothelial function measurements will be made using the EndoPAT system, a noninvasive endothelial function assessment tool based on peripheral arterial tone (PAT) signal technology. The change in arterial tone is elicited by creating a hyperemic response induced by local ischemia (by occlusion of the brachial artery for five minutes). The endothelial function is expressed as a Reactive Hyperemia Index as described in the manufacturer's manual. | Measured at 0, 3, and 6 hours after high fat meal with blueberries, DHA or placebo |
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