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Clinical Trial Details — Status: Terminated

Administrative data

NCT number NCT03297008
Other study ID # BIO-MK-001
Secondary ID
Status Terminated
Phase N/A
First received September 26, 2017
Last updated March 9, 2018
Start date March 11, 2015
Est. completion date December 31, 2017

Study information

Verified date December 2017
Source Danone Asia Pacific Holdings Pte, Ltd.
Contact n/a
Is FDA regulated No
Health authority
Study type Observational

Clinical Trial Summary

To collect saliva and stool samples using the salimetrics swab and self-stool collection kit, process and store samples in a standardized manner. Following this, perform immunological assays such as enzyme-linked immunosorbent assay, multiplex bead assay and Immunocap to correlate the salivary and fecal levels of biomarkers in healthy donors. As this method is non-invasive, we believe that more people will be willing to donate samples.


Description:

Many soluble factors found in blood can be detected in saliva and stool. Often levels of these factors are found to correlate between body fluids, though the exact relationship between systemic (blood) and local (saliva and stool) immunity is not well established yet. Saliva- and stool-associated factors are produced in the oral cavity and in the gut, which represent mucosal sites that potentially come in direct contact with pathogens. Thus, the levels of mucosal-associated soluble factors can better represent the local immune response at these sites.

It is becoming clear now that saliva and stool can be used to analyze inflammatory responses as well. In a recent study, 20 possible salivary biomarkers related to obesity were surveyed and the authors found four biomarkers that exhibit significant change with increasing body weight in a pediatric population. Salivary C-reactive protein (CRP), salivary insulin, leptin and adiponectin were found to be different in obese children compared to healthy normal weight children. This data suggests that saliva could be a useful blood surrogate for the study of metabolic complications of obesity in children, where repeated blood sampling can be both traumatic and difficult. The results of this study also provide insight into the early development of metabolic disease in children. (Goodson, Kantarci et al. 2014). In another study, cytokines-chemokines-growth factors (CCGFs) were measured using multiplex bead assays and compared between plasma, saliva and urine collected from 20 male and female healthy volunteers. By analyzing more than one sample types from the same subject would increase the possibility of identifying biomarker(s) for any inflammatory disease. In this study, gender-specific CCGFs were also observed and concentrations of some CCGFs varied between genders. This information is also valuable for biomarker discovery that by combining male and female subjects in a clinical trial would eliminate false discovery of biomarkers (Khan 2012).

The mucosal immune system can be also understood by analyzing stool samples. In a recent study, it is shown that a particular bacterial predominance, such as Bifidobacterium sp., may enhance thymic development and immune responses to both oral and parenteral vaccines early in infancy, whereas a deviation from this pattern, resulting in greater bacterial diversity, may cause systemic inflammation (neutrophilia) and lower vaccine responses. Thus, vaccine responsiveness may be improved by promoting intestinal Bifidobacteria sp. and minimizing dysbiosis early in infancy (Huda, Lewis et al. 2014). Of note, the hallmark of adequate mucosal immune responses is the production of secretory immunoglobulin A (SIgA), which can prevent infection and remove antigen crossing the mucosal barrier.SIgAis also imperative to establish mutualism between host and the intestinal microbiota (Maynard, Elson et al. 2012). Hence measurement of SIgA can help to assess the mucosal immunity.

Despite saliva and stool samples are increasingly studied in order to assess mucosal immune response and/or clinical outcomes, there is still a lack of established methodology to be routinely used in diagnostic laboratories and clinical trials. Therefore our aim is to collect saliva and stool samples using the salimetrics swab and self-stool collection kit from a cohort of 60 volunteers, process and store samples in a standardized manner. Following this, we intend to perform immunological assays such as enzyme-linked immunosorbent assay, multiplex bead assay and Immunocap to correlate the salivary and fecal levels of biomarkers in healthy donors. As this method is non-invasive, we believe that more people will be willing to donate samples. It is also easy to self-collect and it is cost efficient.


Recruitment information / eligibility

Status Terminated
Enrollment 86
Est. completion date December 31, 2017
Est. primary completion date December 31, 2017
Accepts healthy volunteers Accepts Healthy Volunteers
Gender All
Age group N/A to 60 Years
Eligibility Inclusion Criteria:

• Healthy volunteers of age 0-60 years old

Exclusion Criteria:

- Volunteers with any known infectious diseases, such as HIV and Hepatitis B

- Volunteers with any acute or chronic illness, such as chronic inflammatory bowel disease (e.g. Crohn's disease or ulcerative colitis)

- Volunteers with oral diseases/ulcers

Study Design


Related Conditions & MeSH terms


Intervention

Other:
No internvetion
No intervention, this is an observational study

Locations

Country Name City State
Singapore Danone Nutricia Research Singapore

Sponsors (1)

Lead Sponsor Collaborator
Danone Asia Pacific Holdings Pte, Ltd.

Country where clinical trial is conducted

Singapore, 

Outcome

Type Measure Description Time frame Safety issue
Other Establish methods to detect immune markers in non-invasive samples: Saliva and stool in healthy volunteers ELISA RSV specific Immunoglobulin in stool 1 year after completion of primary outcome
Other Establish methods to detect immune markers in non-invasive samples: Saliva and stool in healthy volunteers ELISA Rotavirus specific Immunoglobulin in saliva 1 year after completion of primary outcome
Primary Establish methods to detect immune markers in non-invasive samples: Saliva and stool in healthy volunteers ELISA RSV specific Immunoglobulin in saliva 1 year after completion of recruitment
Primary Establish methods to detect immune markers in non-invasive samples: Saliva and stool in healthy volunteers ELISA Rotavirus specific Immunoglobulin in stool 1 year after completion of recruitment
Secondary Difference in RSV-specific Immunoglobulins between age groups. Correlation between age and RSV-specific Immunoglobulins in saliva 1 year after completion of primary outcome
Secondary Difference in RSV-specific Immunoglobulins between age groups. Correlation between age and rotavirus-specific Immunoglobulins in stool 1 year after completion of primary outcome
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