Chronic Periodontitis Clinical Trial
Official title:
Grape Seeds Extract Gel as an Adjunct to Scaling and Root Planing for the Treatment of Chronic Periodontitis: A Pilot Clinical Study
The aim of this study was to formulate a mucoadhesive gel of grapes seed extract (GSE) followed by short-term clinical study for the effectiveness of this gel onto the pocket depth (PD), plaque index (PI), gingival index (GI), and bleeding on probing (BOP) when applied in periodontal pockets as an adjunct treatment for chronic periodontitis.
Before commencing with the study, the trial proposal was registered in the research center
and ethical clearance was taken from the ethical committee (FUGRP/2014/182)
Materials used in the study::
1. Pure Grape Seed Extract (GSE) supplied by pure bulk supplements (Bulksupplements, USA).
It contains natural ingredient of more than 180 mg of proanthocyanidins for every 200
mg of serving size of the powder. GSE has been considered safe by the National Center
for Complimentary and Integrative Health if used orally for up to 8 weeks of clinical
trials
2. Carbapol "CB 934" (Loba Chemie Pvt. Ltd., Mumbai)
3. Sodium- carboxy methly cellulose "Na-CMC" supplied (Loba Chemie Pvt. Ltd., Mumbai)
4. Sodium phosphate monobasic and sodium phosphate dibasic (Acros organic Ltd., Mumbai)
5. Parabens (Loba Chemie Pvt. Ltd., Mumbai)
Method of preparation:
GSE mucoadhesive gel preparation:
- Formula 1: 2% GSE mucoadhesive gel based on minimum inhibitory concentration (MIC) and
minimum toxic concentration (MTC) and depending on the concentration of adhesive polymers
that were added to the formula.
Weighed CB 934 was dissolved in 50 ml of phosphate buffer of pH 6.6 with a vigorous mixing
until it dissolved completely. Then, GSE and preservatives were dissolved in about 25 ml of
phosphate buffer of pH 6.6. After that, the GSE solution was slowly added into the solution
of CB 934 with a continuous stirring that was achieved by magnetic stirring at a speed of
100 rpm until a homogenous mixture was obtained. The gelling agent (Na-CMC) was added slowly
under a continuous magnetic stirring. Then, the volume was increased up to 100 ml with the
addition of phosphate buffer. Finally, the prepared gel was kept for 24 hours at room
temperature (25°C) for a complete polymer dissolution.
- Formula 2: controlled gel without GSE. A controlled mucoadhesive gel was used in the
clinical study to be compared with GSE gel. This control gel contained all above mentioned
substances except for the GSE.
Microbial limit test:
One gram of the gel was suspended in 2.9 ml of phosphate buffer at pH 7.2. Different sterile
media (Bismuth Sulfite Medium, Mannitol salt agar medium, Muller Hinton agar medium,
cetrimide agar medium and sabaroud agar medium) were inoculated with the gel, then,
incubated for 24 hours. After that, the media were examined to ensure no growth of bacterial
genera.
Subjects:
A random sample of 24 patients were screened and examined. Five patients with mean age 43.5
±7.9 years were found to comply with the study inclusion criteria
Baseline measurements and application of gels A total of 86 Sites of pocket depth (PD) of 5
mm and above were identified. Sites were divided randomly by split mouth technique into two
groups: Test group (GSE group) who will receive GSE mucoadhesive gel (N=48) and Control
group who will receive the control gel (N=38). The two prepared formulas were placed in
identical containers providing that neither the patient, nor the clinician were aware of
which was applied on which quadrant of the mouth "i.e. double blinded study".
In the first visit, an informed written consent was obtained from all patients. scaling and
root planing (SRP) were performed by the same calibrated examiner using an ultrasonic scaler
(miniPiezon, EMS, Switzerland) and Gracey curettes (Hu-Friedy Mfg, USA). Seven days after,
the patients were recalled for clinical examination and baseline measurement (T0) were taken
for Plaque index (PI), Gingival index (GI), Pocket depth (PD), and bleeding on probing (BOP)
by a single calibrated examiner. PD was measured using a manual probe (UNC 15). PI and GI
were assessed according to Silness and Loe (1964). BOP was assessed within 30 seconds after
probing. In the same visit, the examiner applied the two prepared formulas into two opposite
quadrants using a disposable syringe with a 23-gauge needle. Patients were given oral
hygiene instructions and were instructed not to drink or eat for a minimum of 3 hours, not
to brush the area for 24 hours and not to use mouth wash during the course of treatment.
The patients were recalled again after 3, 6, and 9 days to reapply the two formulas in the
examined sites by the same examiner.
Revaluation The first re-evaluation visit (T1) was after 28 days from the baseline
measurements (T0). During this visit, the calibrated clinician measured and recorded PI, GI,
PD, BOP for all examined sites.
The second re-evaluation visit (T2) was after 6 months from the baseline measurements (T0)
and the same measurements were retaken for all sites.
Statistical Package for the Social Sciences (SPSS) v20 package (IBM Corp) was used for
statistical analysis. Significance of the change in PI, GI, and PD within each group were
determined using paired t-test while the significance of difference in the change between
the two groups was determined using the independent t-test. The difference was considered
statistically significant at p < 0.05.
;
Allocation: Randomized, Intervention Model: Parallel Assignment, Masking: Double Blind (Subject, Caregiver, Outcomes Assessor), Primary Purpose: Treatment
Status | Clinical Trial | Phase | |
---|---|---|---|
Not yet recruiting |
NCT06400069 -
Role of NLRP6 in Chronic Periodontitis
|
||
Completed |
NCT05231096 -
Comparison of the Effect of Gingival Massage of Aloe-vera Gel and Sidr Honey on Chronic Periodontitis
|
N/A | |
Completed |
NCT03203746 -
Gingival Crevicular Fluid Levels of Protein Carbonyl Following the Use of Lycopene in Chronic Periodontitis
|
Phase 1/Phase 2 | |
Active, not recruiting |
NCT03354338 -
Amoxicillin to Prevent Bacteria and Inflammatory Biomarkers After Intensive Periodontal Therapy
|
Phase 2 | |
Completed |
NCT02516111 -
Comparison of Autologous PRF, 1% Alendronate and 1.2% Atorvastatin Gel in Chronic Periodontitis Treatment
|
Phase 2/Phase 3 | |
Completed |
NCT02174146 -
Leptin and Visfatin in Diabetic Patients With Periodontitis Before and After Periodontal Therapy
|
N/A | |
Terminated |
NCT02568163 -
Influence of Stress on Non Surgical Periodontal Treatment
|
N/A | |
Completed |
NCT02430519 -
Benefits of Platelet Rich Fibrin In Mandibular Molar Furcation Defects
|
N/A | |
Completed |
NCT01438333 -
Efficacy of INERSAN in Patients With Chronic Periodontitis as Adjunctive to Full Mouth Disinfection
|
N/A | |
Completed |
NCT01233765 -
Analysis of Neutrophil Response in Chronic Periodontitis
|
N/A | |
Completed |
NCT02218515 -
Treatment of Intrabony Periodontal Defects With Enamel Matrix Derivatives and Autogenous Bone Graft
|
Phase 4 | |
Completed |
NCT02197260 -
Antimicrobial Therapy as Adjunct to Periodontal Treatment: Effect of Timing
|
Phase 4 | |
Not yet recruiting |
NCT03270280 -
Comparison of Salivary Interleukin-1β and Matrix Metalloproteinase-8 Levels in Individuals With Chronic Periodontitis
|
Phase 2 | |
Not yet recruiting |
NCT04026828 -
Evaluation of Possible Genes in Periodontal Diseases by Genetic Methods
|
||
Completed |
NCT04697199 -
The Adjunctive Effect of Probiotics to Non Surgical Treatment of Chronic Periodontitis
|
Phase 1 | |
Completed |
NCT04643288 -
Nanocrystalline Hydroxyapatite Bone Substitute for Treating Periodontal Intrabony Defects
|
N/A | |
Completed |
NCT03039244 -
Evaluation of Antimicrobial Photodynamic Therapy as an Adjunct to Periodontal Treatment in Smokers
|
N/A | |
Completed |
NCT02851823 -
Combined Use of Er:YAG and Nd:YAG Laser
|
N/A | |
Completed |
NCT02898675 -
Advantages of Autologous Platelet-Rich Fibrin Membrane on Growth Factor Levels and Periodontal Healing
|
N/A | |
Completed |
NCT02518152 -
Platelet Rich Fibrin+1% Alendronate in Treatment of Chronic Periodontitis
|
Phase 2/Phase 3 |