Clinical Trial Details
— Status: Not yet recruiting
Administrative data
| NCT number |
NCT06430450 |
| Other study ID # |
ISMAILKMU |
| Secondary ID |
|
| Status |
Not yet recruiting |
| Phase |
|
| First received |
|
| Last updated |
|
| Start date |
July 15, 2024 |
| Est. completion date |
January 15, 2025 |
Study information
| Verified date |
May 2024 |
| Source |
Karamanoglu Mehmetbey University |
| Contact |
ismail tasdemir, assistant professor |
| Phone |
+905455694573 |
| Email |
drismailtasdemir[@]gmail.com |
| Is FDA regulated |
No |
| Health authority |
|
| Study type |
Observational [Patient Registry]
|
Clinical Trial Summary
The aim of this clinical study is; Comparatively comparing salivary Soluble Urokinase
Plasminogen Activator Receptor (SuPAR), Hypoxia-inducible factor-1 alpha (HIF-1α),
E-cadherin, galectin 3, IL-4, IL-10 and TNF-α levels in individuals with different
Periodontal Disease Degrees and to evaluate and analyze correlations with clinical
parameters. In our study, saliva samples will be taken from a total of 80 systemically
healthy volunteers, 20 of patients are periodontal healthy, 20 of patients have degree A
periodontitis, 20 of patients have degree B periodontitis and 20 of patients have degree C
periodontitis, along with the measurement of whole mouth clinical parameters. Soluble
Urokinase Plasminogen Activator Receptor (SuPAR), Hypoxia-inducible factor-1 alpha (HIF-1α),
E-cadherin, galectin 3, IL-4, IL-10 and TNF-α levels in the samples taken will be subjected
to enzyme-related immunoassay ( It will be determined by ELISA). Cytokine levels between
different groups will then be interpreted as a result of statistical analysis. Possible
significant differences shed light on future studies with Soluble Urokinase Plasminogen
Activator Receptor (SuPAR), Hypoxia-inducible factor-1 alpha (HIF-1α), E-cadherin, galectin
3, IL-4, IL-10 and TNF-α. These cytokines may help develop different diagnostic methods or
treatment strategies in future periodontal treatments.
Description:
The study included patients between the ages of 18 and 70 who applied to Karamanoğlu
Mehmetbey University Ahmet Keleşoğlu Faculty of Dentistry Department of Periodontology, were
non-smokers, had no systemic problems, had not used antibiotics, anti-inflammatory and
systemic corticosteroid drugs in the last 3 months, were not pregnant, had not received
periodontal treatment in the last 6 months, and having at least 20 teeth in its mouth; for
grade A periodontitis group; 20 individuals with a probing pocket depth of 5 mm or more in at
least 2 teeth in each quadrant of the jaw, attachment loss, and radiological bone loss
percentage/age ratio <0.25 in the tooth with the most bone loss; for grade B periodontitis
group; 20 individuals with a probing pocket depth of 5 mm or more in at least 2 teeth in each
quadrant jaw, attachment loss, and a radiological bone loss percentage/age ratio of 0.25-1.0
in the tooth with the most bone loss; for grade C periodontitis group; 20 individuals with a
probing pocket depth of 5 mm or more in at least 2 teeth in each quadrant of the jaw,
attachment loss, and radiological bone loss percentage/age ratio >1.0 in the tooth with the
most bone loss; For the healthy group; According to the evaluation made in 6 regions of each
tooth, including 20 individuals who show bleeding on probing in less than 20% of the area,
have a probing depth of less than 4 mm, and have no attachment loss. The healthy and
periodontal disease group will consist of 80 patients in total.Anamnesis will be taken from
individuals at the beginning of the interview, and individuals who meet the specified
criteria after the anamnesis will be included in the study. After being informed about the
study, an informed consent form will be obtained from the individuals.
After the anamnesis is taken, clinical periodontal evaluations will be performed on
individuals who are deemed to meet the inclusion criteria. Clinically, plaque index (Sillness
and Löe 1964), gingival index (Löe and Sillness 1963), pocket depth and bleeding on probing
index(Ainamo&Bay, 1975) will be recorded.
Saliva samples will be taken from individuals divided into groups for biochemical
examinations. Saliva samples will be taken from each patient, first frozen at -20ºC and than
stored at -28ºC until the day of analysis. Cytokine levels in the samples collected from the
patients will be determined by the enzyme-related immune test "Enzyme Linked-Immuno-Sorbent
Assay" (ELISA).
