Aim, design and setting of the study
The aim of this study is to evaluate the clinical, microbiological and immunological effects of systemic probiotics as an adjunct to SRP alone or in combination with MTZ + AMX in the treatment of periodontitis. In order to address this aim, a double-blinded, four-armed, placebo-controlled and bicentric RCT was designed. This study is being conducted at Guarulhos University (UNG; Guarulhos, SP, Brazil) and Federal University of Parana (UFPR; Curitiba, PR, Brazil). The study protocol was developed according to the Standard Protocol Items: Recommendations for Interventional Studies (SPIRIT) guidelines and using the SPIRIT checklist (Additional file 1) (49) and was registered in the ClinicalTrials.gov (NCT03733379) database.
Ethical considerations
This trial is being conducted according to the principles of the Declaration of Helsinki for studies involving human subjects. The protocol was approved by the Institutional Review Board of UNG (Research Ethics Committee, CAAE: 74049717.7.1001.5506) and UFPR (Research Ethics Committee, CAAE: 74049717.7.3001.0102). All eligible volunteers are being informed about the nature, potential risks and benefits of their participation in this study and they sign a term of informed consent.
Subject population and inclusion/exclusion criteria
Systemically healthy volunteers with untreated generalized severe periodontitis (periodontitis Stages III or IV, generalized; (50)) are being selected from the Center for Clinical Trials of UNG and Periodontal Clinic of UFPR. Subjects are being selected according to the following inclusion criteria: presence of at least 15 teeth (excluding third molars and teeth indicated for extraction), at least 30% of the teeth with PD and CAL ≥ 4 mm and a minimum of 6 teeth with at least one interproximal site each with PD and clinical attachment level (CAL) ≥ 5 mm. Exclusion criteria are as follows: pregnancy, breastfeeding, current smoking and former smoking habit within the past 5 years, systemic diseases that could affect the progression of periodontitis (e.g. diabetes), SRP in the previous 12 months, antibiotic therapy in the previous 6 months, long-term intake of anti-inflammatory drugs, need for antibiotic pre-medication for dental treatment, use of orthodontic appliances, extensive prosthetic rehabilitation and allergy to MTZ and/or AMX.
Interventions
At baseline, all volunteers fulfill a structured questionnaire to collect information about demographic, oral and general health data. Subsequently, a complete periodontal clinical assessment and subgingival biofilm sampling are performed. One week later, gingival crevicular fluid (GCF) and peripheral blood samples are collected, and the patients receive oral hygiene instruction (OHI) and supragingival scaling using ultrasonic scaler (Cavitron® Select™ Ultrasonic Scaler, Denstply, New York, USA) and curettes (Millenium, GOLGRAN, São Caetano do Sul, SP, Brazil). The plaque index is repeated one week after OHI and supragingival plaque removal. Subsequently, each volunteer is randomly allocated to one of the following therapeutic groups: (i) Control: SRP + two antibiotic placebo pills three times a day (TID) for 14 days + two probiotic placebo lozenges a day for 90 days; (ii) Probiotic (Test 1): SRP + two antibiotic placebo pills TID for 14 days + two probiotic lozenges a day for 90 days; (iii) Antibiotic (Test 2): SRP + MTZ 400 mg and AMX 500 mg TID for 14 days + two probiotic placebo lozenges a day for 90 days; (iv) Antibiotic + probiotic (Test 3): SRP + MTZ 400 mg and AMX 500 mg TID for 14 days + two probiotic lozenges a day for 90 days (Fig. 1).
The administration of all medications (probiotic and antibiotics) and placebos starts immediately after the first SRP session. Antibiotics (or placebos) are given TID for 14 days and include two tablets, one of MTZ and one of AMX. Antibiotics and placebos are being specially prepared for this study by the same pharmacy (Gallen Pharmacy and Manipulation Ltda, Maringá, PR, Brazil). All tablets have the same color and size, and are stored in properly coded opaque plastic bottles, containing 22 capsules/lozenges. Volunteers, therapists and examiners are blind to the interventions applied.
Probiotic (or placebo) are administered two times per day for 90 days and include one lozenges every 12 hours after brushing and flossing. The second lozenge is administered just before going to sleep. The lozenges are slowly dissolved in the volunteer’s oral cavity. Probiotic and placebo are being prepared for this study by BioGaia AB (Stockholm, Sweden). Probiotic lozenges contain 2 different strains of Lactobacillus reuteri: L. reuteri DSM 17938 and L. reuteri ATCC (PTA 5289), each at a minimum amount of 1 × 108 CFU per lozenge. Placebo probiotic lozenges are identical to the active lozenges in taste, texture and shape, but they do not contain L. reuteri. All lozenges are kept refrigerated at a temperature below 25 °C until they are handed to the patient.
SRP is performed using Gracey curettes (conventional and mini-fives) 5/6, 7/8, 11/12 and 13/14 under local anesthesia, and the treatment is completed in four to six sessions of approximately 1 h, distributed over a period of 14 days. At the end of each session, the clinical coordinator of each center evaluates the effectiveness of SRP using the outcome “smoothness of the scaled roots”. All volunteers will receive clinical monitoring at baseline, and at 3, 6 and 12 months post-therapies. In addition, all subjects will receive periodontal maintenance every 3 months post-treatment until the end of the study. These sessions include OHI and supragingival/subgingival biofilm/calculus removal, as necessary. If any participant shows periodontal attachment loss ≥ 2 mm in 3 or more sites during the maintenance phase they will be excluded from the study and referred for periodontal re-treatment.
Monitoring of compliance and adverse events
A study assistant in each clinical center is monitoring the compliance with intake of probiotic/antibiotics/placebos by calling the patients 2 times a week during the first three weeks of medication intake. After that, participants are monitored once a week for the next 9 weeks. Volunteers should take 21 antibiotics tablets in the first week and 21 in the second week. They are instructed to return the bottles at beginning of the second week of treatment and receive new bottles containing the same amount of medication to take during the second week. Volunteers are not informed about the total number of tablets in each bottle; therefore, at the end of each week, it is possible to confirm if any residual capsule (22nd ) is left in the bottle, to enable compliance to be monitored. Subjects are also asked to return the bottles at 45 days and 90 days post-SRP and the bottles are checked. On the 14th and at 90 days of the medication intake, subjects answer a questionnaire about any self-perceived side effects.
Clinical examination (baseline, 3, 6 and 12 months)
Two calibrated examiners, one from each center (UNG and UFPR), are performing the clinical evaluations and collection of biofilm, GCF and blood samples. The following periodontal parameters are being evaluated: visible plaque (51), gingival bleeding (0/1), BOP (0/1), SUP (0/1), PD (mm) and CAL (mm) at six sites per tooth (mesiobuccal, buccal, distobuccal, distolingual/palatal, lingual/palatal and mesiolingual/palatal) in all teeth, excluding third molars. PD and CAL measurements are rounded to the nearest millimeter using a North Carolina periodontal probe (Hu-Friedy, Chicago, IL, USA).
Investigator’ calibration
The two examiners (B.R.V. and G.M.S.S.) were trained and calibrated prior to the trial, in order to achieve maximum reproducibility in the measurements. The calibration exercise for both centers was conducted at UNG before the beginning of the study, as previously described (52). This exercise will be repeated once a year. Briefly, the standard error of measurement for continuous periodontal clinical parameters (PD and CAL) is evaluated. For the other clinical variables, the average level of agreement between the examiners is determined and considered satisfactory when the value is higher than 90% (Kappa test).
Microbiological monitoring (baseline, 3, 6 and 12 months)
Sample Collection
Nine subgingival samples are being collected per volunteer, three in each of the following categories: shallow (PD ≤ 3 mm), moderate (PD = 4–6 mm) and deep (PD ≥ 7 mm). The selected sites are located on non-contiguous interproximal teeth, preferably distributed across the four quadrants and subset according to baseline PD. Teeth with open margins and overhangs, furcation lesions, extensive caries and/or endo-periodontal lesions are not selected for sampling. After recording the clinical parameters, supragingival plaque is removed and the subgingival samples are collected with individual sterile mini-Gracey curettes #11–12, positioned at the most apical portion of the subgingival sulcus/pocket and with a single apical-coronal movement. The samples are immediately placed in separate Eppendorf tubes containing 150 ul of TE buffer solution (10 mM Tris-HCl, 1 mM EDTA, pH 7.6) and then 100 ul of 0.5M NaOH is added to each tube and the samples are dispersed using a vortex mixer. The samples are being stored at − 20 °C. The tubes containing the samples are previously identified with the volunteer’s code, date and site collected.
Processing of microbiological samples
Counts and proportion of 40 bacterial species will be determined in each sample, using the Checkerboard DNA–DNA hybridization technique (53, 54). The microbiological analysis will be entirely performed at the Laboratory of Microbiology of UNG. Briefly, the suspensions containing the bacterial biofilm samples will be boiled for 10 min and neutralized using 0.8 ml of 5 M ammonium acetate and the DNA is released in the solution. The released DNA will be then placed into the extended slots of a Minislot 30 apparatus (Immunetics, Cambridge, MA, USA) concentrated on a 15 × 15 cm positively charged nylon membrane (Boehringer Mannheim, Indianapolis, IN, USA) and fixed to the membrane by baking it at 1200C for 20 min. Subsequently, the membrane will be placed in a Miniblotter 45 (Immunetics, Cambridge, MA, USA) with the lanes of DNA at 900 to the lanes of the device. Digoxigenin-labeled whole genomic DNA probes for 40 bacterial species are hybridized in individual lanes of the Miniblotter 45. After hybridization, the membranes are washed in highly astringent solution and the DNA probes are detected using the antibody to digoxigenin conjugated with alkaline phosphatase and chemiluminescence detection. The last two lanes in each run contain standards at concentrations of 105 and 106 cells of each species. Signals will be evaluated visually by comparison with the standards for the test species on the same membrane by a calibrated examiner (k test = 93%). The sensitivity of this assay will be adjusted to allow detection of 104 cells of a given species by adjusting the concentration of each DNA probe (53–55).
Immunological monitoring (baseline and 12 months)
Serum and GCF sampling
Peripheral blood samples and GCF are being collected one week after clinical examination. Two non-contiguous diseased sites (i.e. PD and CAL > 5 mm, BoP and no furcation involvement) and two non-contiguous healthy sites (i.e. PD and CAL < 4 mm without BOP and/or gingival bleeding) are being randomly chosen per patient for GCF sampling (among the same sites selected for microbiological sampling). After removal of the supragingival biofilm, the selected sites are isolated with cotton rolls and gently dried with an air syringe to eliminate saliva. GCF is collected by inserting standard paper strips (Periopaper, Oraflow Inc., Smithtown, NY, USA) up to approximately 2 mm into the sulcus/pocket for 30 s. Strips visually contaminated with blood are discarded. The GCF volume is measured in a calibrated device (Periotron 8000, Proflow Inc., Amityville, NY, USA) and the readings are converted into an actual volume (microliter, µl) by reference to a standard curve. Strips from the four selected sites are immediately placed into separate microcentrifuge tubes and stored at -800C for subsequent assays. Peripheral blood samples are into an appropriate tube (Serum BD Vacutainer Plus Plastic Serum Tubes, BD, Franklin Lakes, NJ). Fasted samples are obtained in the morning for all patients. Immediately after blood collection, the serum is separated from blood by centrifugation (10 min at 1,300 rpm) and stored in aliquots at -80 °C.
Processing of serum and GCF samples
The tubes containing the samples will be vortexed for 15 s and centrifuged for 5 min at 1,500xg in order to elute. Samples will be analyzed using a Multiplex Bead Immunoassay (MAGPIX® System, Merck Millipore, Billerica, MA, USA) by means of a multiplex fluorescent bead-based immunoassay for 17 cyto/chemokines (eotaxin, GCSF, GM-CSF, interferon (IFN)-γ, IL-1β, IL-2, IL-6, IL-7, IL-8, IL-10, IL-12, protein chemoattractant monocyte [MCP]-1, MIP-1α and tumor necrosis factor [TNF]-α) using commercially available kits (Milliplex Human Cytokine/Chemokine, EMD Millipore, Billerica, MA, USA) and a plate reader (Luminex. 100TM, EMD Millipore, Billerica, MA, USA), in accordance with the manufacturer’s recommendations. The amount of protein in each sample will extrapolate from standards using an appropriate software (Beadview EMD Millipore, Billerica, MA, USA). The minimum detectable concentrations for eotaxin, G-CSF, GM-CSF, IFN-γ, IL-1β, IL-2, IL-6, IL-7, IL-8, IL-10, IL-12, MCP-1, MIP-1α and TNF-α are: 1.2 pg/ml, 0.5 pg/ml, 9.5 pg/ml, 0.1 pg/ml, 0.4 pg/ml, 0.3 pg/ml, 0.3 pg/ml, 1.8 pg/ml, 0.2 pg/ml, 0.3 pg/ml, 10.5 pg/ml, 0.9 pg/ml, 3.5 pg/ml and 0.1 pg/ml, respectively. The results will be reported as total amount (pg/site/30 sec) and concentrations of cyto/chemokines per volume of GCF (pg/µl) and serum (pg/ml).
Primary and secondary outcome variables
The primary outcome variable is the difference among groups for the percentage of volunteers achieving the clinical endpoint for therapy (≤ 4 sites with PD ≥ 5 mm) at 1 year post-treatment (56).
Secondary outcome variables is: difference between baseline and 12 months post-therapy for mean CAL gain and PD reduction (in the full mouth and in different PD categories), mean number and percentage of volunteers with 0, 1–2 or ≥ 3 sites with different thresholds of residual pockets (e.g. PD ≥ 6 and ≥ 7 mm) at 12 months post-therapy; mean number (and mean reductions) of different thresholds of residual pockets at all post-treatment time points; difference among groups for the percentage of volunteers achieving different thresholds of BOP (e.g. ≤10%, 20% and 30% of bleeding sites in the mouth) at 1 year post-treatment; differences in the occurrence of adverse events among therapeutic groups; differences in the counts and proportions of 40 bacterial species in the biofilm samples at all post-treatment time-points and in the levels of 17 chemokines in the GCF and peripheral blood samples at 1 year post-therapy.
Sample size calculation
The ideal sample size to assure adequate power for this study was based on the percentage of volunteers achieving “≤4 sites with PD ≥ 5 mm” at 1 year post-treatment (56). Considering a difference of 44 percentage points between groups for volunteers achieving this clinical endpoint at 1 year post-treatment (5) and a significance level of 5%, 17 subjects per group would be necessary to provide a power of 80%. Considering an attrition of 25%, it was established that at least 22 subjects should be included in each treatment group. Considering a difference of 30 percentage points between groups for volunteers achieving this clinical endpoint at 1-year post-treatment and a significance level of 5% 37 subjects per group would be necessary to provide a power of 80%. Considering an attrition rate of 15%, it was established that 44 volunteers should be included in each treatment group (total 176 subjects).
Randomization
The study coordinator (M.Fe.), who is not involved in the inclusion and treatment of patients, assigned the study participants to one of the four treatment groups by means of a computer-generated random sequence (Random Allocation Software, http://random-allocation-software.soft). Randomization was stratified by center using permuted blocks of 4, 8 and 12. The study coordinator also organizes the bottles with the antibiotics tablets in opaque plastic bags labeled with the volunteer’s number. In addition, one clinical investigator and the study coordinator sent the randomization list to the BioGaia AB Company (Stockholm, Sweden). The company made and packed the probiotic (and placebo) lozenges in boxes labeled with each volunteer's number. The bags are handed directly to the volunteer by the study coordinator. This sequence of procedures assures allocation concealment.
Data collection and management
Clinical data are entered directly onto electronic spreadsheets (Microsoft® Excel 2011®, version 14.4.8, Copyright © 1990, Microsoft, Santa Rosa, California, USA), at the time of clinical examination, by a single investigator in each center. Data quality will be validated by checking missing data, out-of-range values and invalid responses. The analyses will be conducted using a statistical program developed by Sigmund Socransky (Forsyth, USA), as well as SAS and GraphPad Prism (version 7.0) software.
Statistical analysis
Clinical monitoring
The Chi-square test will be used to compare the differences in the frequency of gender, and to compare the differences in the frequency of subjects achieving the clinical endpoint for treatment (≤ 4 sites with PD ≥ 5 mm) at 1-year (primary outcome variable) and of self-perceived adverse effects. Each individual continue/categorical variable will be computed per subject and then across subjects in each group. The significance of clinical differences over the course of the study will be sought using repeated measures ANOVA or Friedman multiple comparison tests (and their respective post-hoc tests, when necessary); and at each time point (among groups), using either ANOVA or Kruskal-Wallis multiple comparison tests (and their respective post-hoc tests when necessary) or ANCOVA with adjustments for the baseline values. Parametric or non-parametric tests will be chosen based on the normality of the data. A stepwise forward logistic regression analysis will be performed to investigate the impact of predictor variables on the clinical endpoint for treatment, i.e., “presence of ≤ 4 sites with PD ≥ 5 mm at 1-year post-therapy (yes/no)”. The Number Needed to Treat (NNT) with each treatment protocol in order to obtain treatment success (≤ 4 sites with PD ≥ 5 mm) will be calculated using the formula: NNT = 1/ARR, where ARR = |CER - EER| and CER = control group event rate and EER = experimental group event rate (http://ktclearinghouse.ca/cebm/glossary/nnt). The level of significance will be set at 5%. The data will be evaluated using intention-to-treat analysis with last observation carried forward.
Microbiological and immunological monitoring
Microbiological data will be expressed in counts (levels) and proportion counts of DNA probes. Mean counts will be expressed as counts × 105. Microbial data will be calculated at each site for each volunteer and then across volunteers within each group, at each time-point. The sum of the mean proportions of individual bacterial species will be computed for each microbial complex described by Socransky et al. (57). The concentration and total amount of each cytokine/chemokine in the GCF will be assessed per volunteer and then per volunteer within each group at each study time-point. Immunological data will be calculated at each site for each volunteer and then across volunteers within each group, at each time-point. The significance of differences in microbiological and immunological parameters over the course of the study will be sought using repeated measures ANOVA or Friedman multiple comparison tests (and their respective post-hoc tests, when necessary); and at each time point (among groups) using either ANOVA or Kruskal-Wallis multiple comparison tests (and their respective post-hoc tests when necessary) or ANCOVA with adjustments for the baseline values. Parametric or non-parametric tests will be chosen based on the normality of the data.