Open Access
Numéro
J Oral Med Oral Surg
Volume 26, Numéro 1, 2020
Numéro d'article 6
Nombre de pages 8
Section Revue de la littérature / Literature review
DOI https://doi.org/10.1051/mbcb/2019037
Publié en ligne 27 janvier 2020

© The authors, 2020

Licence Creative Commons
This is an Open Access article distributed under the terms of the Creative Commons Attribution License (https://creativecommons.org/licenses/by/4.0), which permits unrestricted use, distribution, and reproduction in any medium, provided the original work is properly cited.

Introduction

Periodontal disease is a major oral health problem with a multifactorial origin that affects a large number of people around the world whose origin is multifactorial. In Europe, >50% of the population is affected, with prevalence increasing to 70–85% in the 60–65 age group [1].

In 1999, Armitage [2] established a nosological classification splitting periodontal disease into seven distinct forms. Currently, this has been simplified by the terms acute periodontitis (AP) and chronic periodontitis (CP) [3].

Aggressive periodontitis, AP, is a very destructive form of periodontal disease. APs include precocious, prepubertal, juvenile, rapid progressive, and refractory periodontitis. They can be localized or generalized and affect 10–15% of the adult population around the world [4]. The earlier age of onset, faster progression rates, destruction patterns, clinical signs of inflammation, and lower relative plaque and calculus abundance [3] distinguish AP from CP.

CP is the most common form of periodontitis. It can begin at any time of life but is most often detected in adulthood. Periodontitis is localized when <30% of sites are affected and generalized when >30% of sites are affected. Its severity is assessed according to the loss of the attachment: light, 1–2 mm; moderate, 3–4 mm; and severe, >5 mm.

Specific clinical indices are used in epidemiological studies and daily practice to determine the degree of impairment and monitor the progress of patients' periodontal status. The aim is to evaluate gingival inflammation [5], the presence of dental plaque [6] and tartar, the clinical level of periodontal attachment, the pocket depth in mm, and mobility and/or tooth displacement and to look for bleeding on probing [7].

The initiation and progression of periodontal disease have been reported as the result of complex interactions between specific subgingival bacteria and the host's immunoreactive response [8,9]. This host response to periodontal disease consists of immune cells and their products (particularly cytokines) and complex interactions [10].

Immunocytes activated by exogenous bacteria destroy the bacteria and release myriads of substances, called inflammatory cytokines, which exert an antibacterial effect and contribute to the destruction of the periodontal tissues [11].

Therefore, considerable attention has been paid in establishing an association between periodontitis and certain inflammatory cytokines, such as leptin, which could modulate the host's response to infectious agents and play a role in certain inflammatory conditions because of its direct effect on innate and adaptive immune cells [11], including periodontal ligament cells, which are major resident cells of the periodontium [12].

The plasma levels of leptin increase in cases of acute inflammation and acute severe diseases such as sepsis. High plasma concentrations of leptin have been suggested as a risk factor for cardiovascular disease. The resolution of inflammation depends on the balance between pro- and anti-inflammatory cytokines [10].

These markers present in gingival crevicular fluid, saliva, and plasma have the potential to provide insight into the pathological process of periodontitis well beyond conventional clinical and radiographic findings. In addition, saliva is a noninvasively accessible biological fluid containing a set of locally produced biomolecules. Saliva has become a potential diagnostic fluid in the evaluation of oral and systemic diseases, particularly periodontal diseases [13,14].

There are two meta-analyses [15,16] evaluating the relationship between serum leptin concentrations and periodontal disease, but these do not rule out other adipokines, including adiponectin.

The aim of our study was to perform a qualitative and quantitative synthesis of the literature concerning the presence of leptin (salivary and serum) in patients with CP.

Materials and methods

Research strategy

Research studies were conducted using the PubMed and Web of science bibliographic databases.

Two computer queries were made using the following terms:

  • First request: [leptin and periodontal disease] [MeSH]

  • Second query: [leptin and periodontal disease] [MeSH major topic]

We then manually revised all bibliographic reference lists from previously selected studies to identify clinical trials evaluating leptin difference in patients with and without periodontitis.

The research concerned literature published before March 2019.

Selection of studies and eligibility of criteria

Inclusion criteria

Type of study

Randomized trials, published in English or French before March 2019, were included. A clinical trial has been considered randomized if the author declares it as such or in the text the word “random, randomly, randomized, or randomization” appear [17].

Type of intervention

Studies evaluating salivary and/or serum leptin variations in CP and healthy subjects.

Judgment criteria

The diagnostic criteria for CP were established for each patient on the basis of the following clinical results: gingival index, probing depth ≥4 mm in 3–4 sites in >4 teeth in each quadrant, loss of clinical attachment >1 mm, and radiological evidence of bone loss without specifying the nature of the X-ray.

Exclusion criteria

The following cases have been excluded:

  • Therapeutic trials where the salivary and/or serum leptin dosage was not assessed in both healthy and patients with CP.

  • Studies conducted in animals or in humans in vitro.

  • Studies where chronic periodontal disease is associated with a general pathology when it is mentioned.

  • Factors that have been excluded are as follows:

    • Smoking

    • Alcoholism

    • Body mass index (BMI) >30

    • Pregnant and lactating women

    • Any antimicrobial, anti-inflammatory, or immunosuppressive treatment in the last 6 months known to affect periodontal status

    • Periodontal treatment in the last 12 months

    • All patients who did not provide their consent.

Nonrandomized cohort studies, nonrandomized trials, and studies not written in English or French were also excluded.

Data collection

The studies identified during the electronic research stages were listed in the chronological order of publication in a summary table indicating the principal author's name, publication year, journal review, study type, and exclusion criteria.

This information will be presented in the form of tables describing the selected studies.

After this census phase, a flow diagram that graphically represents the study selection process was created.

Extraction of data

The studies eligible for the analysis are presented in a summary table specifying the following:

  • The principal author, the journal, and the publication year

  • The description of the judgment criteria affected subjects/healthy subjects

  • Quantitative evaluation of the judgment criterion in each group

    • Number of subjects in recruitment and distribution of case/control subjects

    • The characteristics of the population studied in each group

      • Age

      • Sex ratio

      • BMI

      • The type of leptin studied (serum and/or salivary)

To obtain the relevant missing information from included studies for the meta-analysis, we attempted to contact the corresponding authors twice by e-mail without receiving a response from them.

Risk of bias in the evaluation

Case selection was done by two trained and qualified reviewers who considered a case adequate when a patient was representative for the defined type of periodontitis.

Selection of controls was appropriate when sampled from the same population as cases. The cases and controls were compared by sex, age, BMI, and group size.

Both reviewers included studies for which patients had a normal BMI, according to the 2002 World Health Organization table, and obesity influencing leptin levels present in serum.

Definition of the group

We divided case–control comparisons into three categories: patients with AP, subjects with CP, and healthy control subjects.

The healthy group consisted of people who showed no clinical sign of gingival inflammation or bone loss and who had good oral hygiene.

According to the articles, the dosage of leptin was present in saliva, gingival crevicular fluid, or in the blood.

Quantitative analysis

Quantitative data on serum and salivary leptin and the total number of patients with CP and control subjects were extracted to calculate, for each study, the standardized mean difference (SMD) and the 95% confidence interval (95% CI). All data were presented in the form of a data summary table. Statistical calculations were performed with the help of Review Manager 5.3.

SMD is used as a summary statistic in the meta-analysis when all studies evaluate the same result but measure it in various ways. In these circumstances, it is necessary to standardize the results of the studies on a uniform scale before they can be combined. SMD expresses the magnitude of the effect of the intervention in each study relative to the variability observed in this study.

Therefore, studies in which the mean difference between groups is of the same proportion as the standard deviation between the participants will have the same SMD, regardless of the actual scales used to perform the measurements.

Necessarily, the studies selected for a systematic review will not be identical and all the forms of variability within these studies will be grouped under the term of heterogeneity. The observed differences in the population recruited, the nature of the intervention performed, or the judgment criteria constitute the clinical variability. The methodological variability concerns the risk of bias and the design of each study. The variability in the measurement of the effect in the different studies results from the addition of clinical and methodological variability and can be quantified by measuring the statistical heterogeneity.

The Chi-square test proposed by Review Manager assesses whether the observed difference between studies is due to chance alone. A high Chi-square or low P value indicates heterogeneity in estimating the effect of an intervention.

The interpretation of these figures should be cautious, as it is highly dependent on the number of studies selected and the size of the samples from each of them, and small and few studies expose to under-screening for heterogeneity.

This means that even though a statistically significant result may indicate a problem of heterogeneity, a nonsignificant result should not be taken as evidence of the absence of heterogeneity. Thus, a P-value of 0.10 is sometimes used instead of the conventional 0.05 level to determine statistical significance.

Methods have been developed to quantify the inconsistency between studies that focus on assessing heterogeneity rather than assessing its impact on the meta-analysis.

Q = result of Chi-squared test and df = number of degrees of freedom of Chi-squared test; I2 is the percentage of variability in the measure of effect attributable to heterogeneity rather than sampling fluctuations.

The value of I2, according to the Cochrane Handbook for Systematic Review, will be interpreted as follows:

  • 0–40%: insignificant heterogeneity

  • 30–60%: moderately significant heterogeneity

  • 50–90%: heterogeneity to be considered

  • 75–100%: very significant heterogeneity

Results

Figure 1 describes the number of publications identified during the research strategy and details the process for selecting clinical trials. The manual revision of the bibliographic reference lists made it possible to select one additional publication that could be included in the analysis. The study characteristics are presented in Table I.

All the results of the qualitative analysis of the 14 studies were grouped together as a table (Tab. II). It groups together studies of leptin in its various forms in patients with CP with a BMI of ≤30 compared with healthy controls. All of these studies were not included in the quantitative analysis because they combined factors that we decided to exclude from our study.

Only four randomized trials were selected for quantitative analysis. They compared leptin dosages between the CP group and the control group. We decided not to include the Khorsand study [11] as the data collected on CP were too different from the other included studies and the definition criteria of the CP were not clearly specified in this publication.

thumbnail Fig. 1

Flowchart of the study selection process.

Table I

Risk of bias; N = number of studies considered adequate for the corresponding element.

Table II

Biological publications comparing leptin dosage in patients with periodontitis compared to healthy controls. ↑ : significantly high concentrations, ↓ : significantly decreased concentrations, N : number.

Description of selected studies for quantitative analysis

The four studies selected for quantitative analysis recruited a population of 186 patients from throughout India. The age of the patients included varies between 30 and 60 yr. All these studies analyzed the salivary and serum leptin dosage, except for the Karthikeyan study [18], which only studies the salivary leptin dosage.

In the two Purwar studies [20,21] and the Karthikeyan study [18], CP was defined for each patient by plaque index, gingival index, pocket depth, and clinical level of periodontal attachment that were scored on six sites (mesiovestibular, vestibular, distovestibular, mesiolingual, lingual, and distolingual) in each tooth, excluding the third molar, and the presence of bleeding during probing was evaluated using a sterile periodontal probe. All clinical parameters were recorded by one independent person.

The diagnosis of CP was established on the basis of clinical findings of gingival inflammation, clinical loss of periodontal attachment of >5 mm for Purwar [20,21] and only >1 mm for Karthikeyan [19], pocket depth of ≥4 mm in 3–4 sites in >4 teeth in each quadrant, and radiographic evidence of bone loss.

On examination, >30% of the sites examined were positive for the above criteria, and the patients were classified under generalized CP.

For Karthikeyan [18], CP was based on the clinical signs of gingival inflammation with loss of attachment, radiographic evidence of bone loss, and gingival index, as well as Ramfjord's Periodontal Disease Index.

The salivary samples for obtaining leptin concentrations in both media were performed according to two separate procedures specific to each of the two authors [1821].

Purwar [20,21] took nonstimulated whole salivary samples (approximately 2 ml) that were collected using a modified drainage method. Patients were asked to expectorate in disposable polypropylene tubes every 30 s over a period of 5 min. The desired volume (about 2 ml) of saliva was pipetted into an Eppendorf tube. Participants who were unable to expectorate the required saliva volume were excluded. The saliva samples were centrifuged at 4000× rpm for 10 min to remove cell debris, and 0.5 ml of the supernatant was stored in 1.5 ml aliquots at −80 °C until the analysis was performed.

In [18,19] the CP group, Karthikeyan collected the site with the highest gingival index, pocket depth, and clinical level of periodontal attachment (range, 1–4 mm) for gingival crevicular fluid sampling. The site chosen for sampling was isolated with a cotton roll, and the supragingival plaque was removed with a curette, without touching the marginal gingiva. Crystalline gingival fluid specimens were obtained before probing the site by placing micro capillary pipettes. At each test site, a standard volume of 1 ml was collected using micropipette calibration. Any trial site that did not express any volume of gingival crevicular fluid and/or a micropipette that was contaminated with blood and saliva was excluded from the study. The gingival crevicular fluid collected was immediately transferred to a plastic vial and stored at −70 °C until the time of testing.

The serum samples were taken, identically for the two authors Karthikeyan and Purwar [1821] by peripheral venipuncture. After 1 h, the serum was separated from the blood by centrifugation. Each tube was designated by a tracking number and stored at −80 °C until further analysis could be performed.

The two authors [1821] performed the same technical procedure for leptin analysis using highly sensitive enzyme-linked immunosorbent assay (ELISA) kits to detect leptin levels in saliva and serum. Each plate was checked prior to use to ensure that the standard curve measured leptin standards (0–1000 µg/ml) within the indicated range of the dosage. The absorption of the colored reaction of the substrate was read on the ELISA reader using 405 nm as the primary wavelength. Each patient was used as the unit of analysis. Total leptin was determined in picograms (µg), and calculation of the concentration in each sample was performed by dividing the amount of leptin by the sample volume (µg/ml).

The characteristics of the included studies are detailed in Table III.

Table III

Studies included in the quantitative analysis M/F: Male/Female.

Analysis of the risk of bias in studies

Power bias

Among the four studies, three studies [1921] obtained a result with p < 0.05, and one study with p < 0.003 corresponded to a highly significant study.

Sampling bias

From the available cohort descriptions, the four studies recruited cases and controls from the same population. For the four studies, it was explicitly stated that the witnesses did not have a personal history of periodontitis in the 12 months preceding recruitment. In addition, all studies are comparable by age, sex, and BMI (Tab. I).

Most studies on periodontitis applied adequate diagnostic criteria; the criteria for CP and Armitage periodontitis classification were applied by all four studies.

Sampling and measurement methods were adequate and described in all studies. With regard to the serum and saliva collection procedure, all studies applied the same protocol.

The main technique for analyzing leptin concentration was done using the ELISA test in all studies.

Heterogeneity bias

The main bias of our study is represented by the heterogeneity of the samples that were prepared differently (in total saliva or gingival crevicular fluid). As a result, we chose to analyze SMD rather than relative risk to correct this bias. We also ensured certain homogeneity in the four selected final studies with regard to the populations studied, the main endpoint, and the absence of systemic diseases associated with CP.

Quantitative analysis

We conducted two series of comparative analyses:

  • Analysis 1: salivary leptin dosage in CP vs. control

  • Analysis 2: serum leptin dosage in CP vs. control.

The results of each analysis (SMD, 95% CI) are presented using Review Manager 5.3.

  • 1.

    Regarding the comparison of salivary leptin, we measured an SMD of −2.27, 95% CI [−2.68, −1.86]. The difference is highly significant, but we detected significant heterogeneity in this dataset (I2 = 94%) (Fig. 2).

    thumbnail Fig. 2

    Forest plot of salivary leptin concentrations in patients with chronic periodontitis versus controls. The squares represent the effect sizes of the individual studies (the size reflects the weight of the study) and the horizontal lines indicate the 95% confidence intervals (CI). The filled diamonds represent the total size of the effect (the horizontal width indicates the 95% CI).

  • 2.

    For the results of the serum leptin comparison, we measured an SMD of 2.18, 95% CI [1.75, 2.61]. The difference was highly significant. The heterogeneity measured in this dataset was also too large (I2 = 95%) (Fig. 3).

    thumbnail Fig. 3

    Forest plot of serum leptin concentrations in patients with chronic periodontitis versus controls. The squares represent the effect sizes of the individual studies (the size reflects the weight of the study) and the horizontal lines indicate the 95% confidence intervals (CI). The filled diamonds represent the total size of the effect (the horizontal width indicates the 95% CI).

Discussion

For several years, the literature on the influence of leptin on systemic and periodontal diseases has been steadily increasing and becoming controversial. Data from the first meta-analysis suggest that serum leptin levels are significantly higher and salivary leptin levels are lower in patients with CP than in healthy subjects. The results of our analysis show similar trends.

We performed an electronic and manual literature review ensuring an exhaustive character of our selection. Our selection criteria were different from those of Zhu [15] and Jain [16] as we included only randomized case-control trials for CP, both salivary and serum leptin dosages. Our study selection criteria ensured certain homogeneity in the study populations (in terms of age, sex distribution, group size, and BMI), the primary endpoint, and the lack of systemic diseases associated with CP.

We chose to exclude patients whose BMI was >30 because an increase in BMI results in an increase in serum leptin; it is the obese (ob) gene that appears to be involved in this mechanism, with a greater amount of ob mRNA found in adipocytes of obese subjects than in those of subjects with normal weight.

The populations studied are also homogeneous in the definition of CP, serum data collection, and independent operators.

In agreement with Zhu [15] (I2 = 91.6%), we also measured an excessive heterogeneity during the serum leptin comparison of subjects with CP versus healthy subjects.

The significant heterogeneity modifies the interpretation of our results and presents one of the weak points of our study.

However, strict adherence to the inclusion and exclusion criteria limited the sample size of the study. Further longitudinal interventional studies with larger samples are needed to potentiate the role of salivary and serum leptin as a reliable biomarker in patients with periodontitis. It might be interesting to compare AP and CP in later studies as well.

Only Zhu's meta-analysis of [15] serum leptin can be compared to our study because Jain's [16] meta-analysis does not present precise data on leptin dosages and does not exclude systemic diseases from the study. Zhu et al. [15] obtained similar results in our study, favoring an increase in serum leptin levels in patients with periodontitis compared with those in controls in the population with a BMI of <30.

The role of leptin as a potential biomarker of periodontitis is suggested in different meta-analyses and [15,16] deserves to be emphasized. In fact, monitoring the adipokine profile may allow clinicians to predict risk factors of periodontitis. Future research should be focused on distinguishing what comes first and what is the cause and effect; recognizing bilateral relationships between periodontitis and systemic diseases will encourage endocrinologists and odontologists to collaborate closely in the future for treatment of patients with diabetes, obesity, atherosclerosis, and periodontal disease.

Conclusion

We can conclude that the current level of evidence is insufficient to assert that there is definitely an increase in serum leptin and a decrease in salivary leptin in patients with CP compared with healthy control subjects.

Further research could evaluate the influence of leptin levels on the response to periodontal disease treatment in a large patient population in randomized trials with rigorous methodology.

Conflict of interest

The authors declare that they have no conflicts of interest in relation to this article.

References

  1. Kavanagh DA. The incidence of periodontal disease and its impact on future dental practice. Dent Update 1998;25:435–440. [PubMed] [Google Scholar]
  2. Armitage GC. Development of a classification system for periodontal diseases and conditions. Ann Periodontol 1999;4:1–6. [CrossRef] [PubMed] [Google Scholar]
  3. Armitage GC, Cullinan MP. Comparison of the clinical features of chronic and aggressive periodontitis. Periodontology 2000;53:12–27. [CrossRef] [PubMed] [Google Scholar]
  4. Calas-Bennasar I, Jame O, Orti V, Gibert P. Classification des maladies parodontales. Datatraitesmb28-54762 [Internet]. 23 déc 2016 [cité 30 juin 2019]; Disponible sur: http://emvmsa1a.jouve-hdi.com/article/1098272 [Google Scholar]
  5. Loe H, Silness J. Periodontal disease in pregnancy. I. Prevalence and severity. Acta Odontol Scand 1963;21:533–551. [CrossRef] [PubMed] [Google Scholar]
  6. Silness J, Loe H. Periodontal disease in pregnancy. II. Correlation between oral hygiene and periodontal condtion. Acta Odontol Scand 1964;22:121–135. [CrossRef] [PubMed] [Google Scholar]
  7. Muhlemann HR. [Measurement of dental mobility as a diagnostic and prognostic aid in paradontology]. Paradentologie 1950;4:110–119. [PubMed] [Google Scholar]
  8. Zambon JJ. Periodontal diseases: microbial factors. Ann Periodontol 1996;1:879–925. [CrossRef] [PubMed] [Google Scholar]
  9. Gemmell E, Carter CL, Grieco DA, Sugerman PB, Seymour GJ. P. gingivalis-specific T-cell lines produce Th1 and Th2 cytokines. J Dent Res 2002;81:303–307. [CrossRef] [PubMed] [Google Scholar]
  10. Ahima RS, Flier JS. Leptin. Annu Rev Physiol 2000;62:413–437. [CrossRef] [PubMed] [Google Scholar]
  11. Khorsand A, Bayani M, Yaghobee S, Torabi S, Kharrazifard MJ, Mohammadnejhad F. Evaluation of Salivary Leptin Levels in Healthy Subjects and Patients with Advanced Periodontitis. J Dent Tehran Iran 2016;13:1–9. [Google Scholar]
  12. Li W, Huang B, Liu K, Hou J, Meng H. Upregulated Leptin in Periodontitis Promotes Inflammatory Cytokine Expression in Periodontal Ligament Cells. J Periodontol 2015;86:917–926. [CrossRef] [PubMed] [Google Scholar]
  13. Miller CS, King CP, Langub MC, Kryscio RJ, Thomas MV. Salivary biomarkers of existing periodontal disease: a cross-sectional study. J Am Dent Assoc 2006;137:322–329. [CrossRef] [PubMed] [Google Scholar]
  14. Miller CS, Foley JD, Bailey AL, Campell CL, Humphries RL, Christodoulides N, et al. Current developments in salivary diagnostics. Biomark Med 2010;4:171–189. [Google Scholar]
  15. Zhu J, Guo B, Gan X, Zhang L, He Y, Liu B, et al. Association of circulating leptin and adiponectin with periodontitis: a systematic review and meta-analysis. BMC Oral Health [Internet]. 29 juin 2017 [cité 30 juin 2019];17. Disponible sur: https://www.ncbi.nlm.nih.gov/pmc/articles/PMC5492908/ [Google Scholar]
  16. Jain H, Mulay S. Relationship between periodontitis and systemic diseases: leptin, a new biomarker? Indian J Dent Res Off Publ Indian Soc Dent Res 2014;25:657–661. [CrossRef] [Google Scholar]
  17. Jadad AR, Moore RA, Carroll D, Jenkinson C, Reynolds DJ, Gavaghan DJ, et al. Assessing the quality of reports of randomized clinical trials: is blinding necessary? Control Clin Trials 1996;17:1–12. [CrossRef] [PubMed] [Google Scholar]
  18. Karthikeyan BV, Pradeep AR. Leptin levels in gingival crevicular fluid in periodontal health and disease. J Periodontal Res 2007;42:300–304. [CrossRef] [PubMed] [Google Scholar]
  19. Karthikeyan BV, Pradeep AR. Gingival crevicular fluid and serum leptin: their relationship to periodontal health and disease. J Clin Periodontol 2007;34:467–472. [CrossRef] [PubMed] [Google Scholar]
  20. Purwar P, Khan MA, Mahdi AA, Pandey S, Singh B, Dixit J, et al. Salivary and serum leptin concentrations in patients with chronic periodontitis. J Periodontol 2015;86:588–594. [CrossRef] [PubMed] [Google Scholar]
  21. Purwar P, Khan MA, Gupta A, Mahdi AA, Pandey S, Singh B, et al. The effects of periodontal therapy on serum and salivary leptin levels in chronic periodontitis patients with normal body mass index. Acta Odontol Scand 2015;73:633–641. [CrossRef] [PubMed] [Google Scholar]
  22. Gangadhar V, Ramesh A, Thomas B. Correlation between leptin and the health of the gingiva: a predictor of medical risk. Indian J Dent Res Off Publ Indian Soc Dent Res 2011;22:537–541. [CrossRef] [Google Scholar]
  23. Ay S, Ağar U, Biçakçi AA, Köşger HH. Changes in mandibular third molar angle and position after unilateral mandibular first molar extraction. Am J Orthod Dentofacial Orthop 2006;129:36–41. [CrossRef] [PubMed] [Google Scholar]
  24. Zimmermann GS, Bastos MF, Dias Gonçalves TE, Chambrone L, Duarte PM. Local and circulating levels of adipocytokines in obese and normal weight individuals with chronic periodontitis. J Periodontol 2013;84:624–633. [CrossRef] [PubMed] [Google Scholar]
  25. Gundala R, Chava VK, Ramalingam K. Association of leptin in periodontitis and acute myocardial infarction. J Periodontol 2014;85:917–924. [CrossRef] [PubMed] [Google Scholar]
  26. Thanakun S, Watanabe H, Thaweboon S, Izumi Y. Association of untreated metabolic syndrome with moderate to severe periodontitis in Thai population. J Periodontol 2014;85:1502–1514. [CrossRef] [PubMed] [Google Scholar]
  27. Mendoza-Azpur G, Castro C, Peña L, Guerrero M-E, De La Rosa M, Mendes C, et al. Adiponectin, leptin and TNF-α serum levels in obese and normal weight Peruvian adults with and without chronic periodontitis. J Clin Exp Dent 2015;7:e380–e386. [CrossRef] [PubMed] [Google Scholar]
  28. Zeigler CC, Wondimu B, Marcus C, Modéer T. Pathological periodontal pockets are associated with raised diastolic blood pressure in obese adolescents. BMC Oral Health [Internet]. 24 mars 2015 [cité 30 juin 2019];15. Disponible sur: https://www.ncbi.nlm.nih.gov/pmc/articles/PMC4373518/ [Google Scholar]
  29. Leira Y, Ameijeira P, Domínguez C, Leira R, Blanco J. The role of leptin as a biomarker in the relationship between periodontitis and chronic migraine. J Clin Periodontol 2017;44:1208–1214. [CrossRef] [PubMed] [Google Scholar]
  30. Sete MRC, Júnior RL, Fischer RG, Figueredo CMS. Serum adipokine levels and their relationship with fatty acids in patients with chronic periodontitis. Braz Dent J 2015;26:169–174. [CrossRef] [PubMed] [Google Scholar]

All Tables

Table I

Risk of bias; N = number of studies considered adequate for the corresponding element.

Table II

Biological publications comparing leptin dosage in patients with periodontitis compared to healthy controls. ↑ : significantly high concentrations, ↓ : significantly decreased concentrations, N : number.

Table III

Studies included in the quantitative analysis M/F: Male/Female.

All Figures

thumbnail Fig. 1

Flowchart of the study selection process.

In the text
thumbnail Fig. 2

Forest plot of salivary leptin concentrations in patients with chronic periodontitis versus controls. The squares represent the effect sizes of the individual studies (the size reflects the weight of the study) and the horizontal lines indicate the 95% confidence intervals (CI). The filled diamonds represent the total size of the effect (the horizontal width indicates the 95% CI).

In the text
thumbnail Fig. 3

Forest plot of serum leptin concentrations in patients with chronic periodontitis versus controls. The squares represent the effect sizes of the individual studies (the size reflects the weight of the study) and the horizontal lines indicate the 95% confidence intervals (CI). The filled diamonds represent the total size of the effect (the horizontal width indicates the 95% CI).

In the text

Les statistiques affichées correspondent au cumul d'une part des vues des résumés de l'article et d'autre part des vues et téléchargements de l'article plein-texte (PDF, Full-HTML, ePub... selon les formats disponibles) sur la platefome Vision4Press.

Les statistiques sont disponibles avec un délai de 48 à 96 heures et sont mises à jour quotidiennement en semaine.

Le chargement des statistiques peut être long.