Anti-Early Stage of Bacterial Recolonization

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This is an open access article distributed under the Creative Commons Attribution License, which permits unrestricted use, distribution, and reproduction in any medium, provided the original work is properly cited.

1. Introduction

Chronic periodontitis represents one of the most common bacterial infections and inflammatory diseases. Multibacterial colonization on supra- and subgingival tooth surfaces causes chronic destruction of the oral connective tissue and alveolar bone, which may result in tooth loss. The prevalence of several species of subgingival microorganisms has regularly been associated with periodontal diseases [1–4]. In dental plaque biofilm formation, Fusobacterium nucleatum (F. nucleatum) adhere to pellicles and early colonizers, while late colonizers, including Prevotella intermedia (P. intermedia), adhere to the outer surface of those microorganisms. While F. nucleatum is commonly detected in gingivitis and chronic periodontitis [5, 6], P. intermedia is detected in high frequency in lesions of chronic periodontitis, aggressive periodontitis, and acute necrotizing ulcerative gingivitis [5, 7–11]. Moreover, the presence of F. nucleatum in subgingival biofilm plays a significant role in coaggregation with other periodontal bacteria recolonization during the development of dental biofilms after eradication [12–14]. Additionally, some medical conditions such as pregnancy and poor glycemic control are associated with increased levels and frequencies of F. nucleatum and P. intermedia in sites with probing depth <5 mm [15, 16].

Mechanical debridement by scaling and root planing (SRP) is an essential method in the treatment of periodontal diseases by removing dental biofilm, bacterial products, and calculus [17]. However, the efficacy of SRP can be limited in cases with limited access to deep pockets, root anatomies, and tooth malalignment [18]. Thus, different adjunctive treatments, including local antiseptic and antibiotic, have been proposed to improve the clinical outcome of SRP or to reduce the numbers of pathogenic bacteria in those areas [19].

To avoid any unpleasant overdose or drug-resistant bacteria, our previous in vivo study considered the antibacterial effects of Curcuma longa extract against periodontal pathogen and its use as a photosensitizer in the gingival sulcus for additional photodynamic therapy (PDT) [20]. Thus, the objective of this study was to investigate the efficacy of subgingival application of 25 μg/mg Curcuma longa gel extract along with irradiation with blue LED light (energy density = 16.8 J/cm²) for 2 minutes as an adjunct to conventional scaling and root planing procedures.

2. Materials and Methods

2.1. Study Design and Participants

This randomized split-mouth controlled trial was approved by the University Center for Ethics in Human Research (HE-611065). Twelve patients with moderate chronic periodontitis (periodontitis stage II and stage III) were enrolled in this study after the study purpose was explained and their written consents were obtained. The inclusion criteria were ages between 35 and 65 years old and presence of clinically identical parameter on 2 posterior teeth with a probing pocket depth (PPD) >4 mm on the first and second quadrants. Patients with systemic diseases that could influence the outcomes, pregnancy, smoking, diabetes mellitus, periodontal treatment within the last six months, and systemic antibiotic therapy within the last three months were excluded.

2.2. Clinical Examination and Treatments

The following clinical parameters were assessed at baseline and 1, 2, 4, and 6 weeks after the treatment: plaque index (PI) [21], periodontal pocket depth (PPD), clinical attachment level (CAL), and bleeding on probing (BOP) [22]. Six sites per tooth on maxillary posterior teeth were measured and recorded by the same periodontist. The PI was expressed as scores of 0 to 3. PPD and CAL were recorded as the distances from the bottom of the pocket to the gingival margin and cementoenamel junction, respectively. BOP was recorded as “present” or “absent” within 30 seconds of probing. The treatment started by giving instructions on oral hygiene and full-mouth SRP with periodontal curettes and ultrasonic devices. One randomly chosen (by coin toss) clinically identical posterior teeth also received PDT following SRP. In the PDT group, Curcuma longa gel extract at a concentration of 25 μg/mg was applied to the gingival sulcus. Then, the chosen tooth was immediately irradiated with a 420–480 nm wavelength blue LED light source with a power output of 1000–1200 mW/cm². The blue LED was connected to a medical-grade quartz, periodontal probe-like shape, round end point with a diameter of 1 mm (energy density = 16.8 J/cm²). The tip was lightly run along the tooth surface on both buccal and palatal sides for 2 minutes without removing it from the gingival sulcus.

2.3. Microbial Samples

Subgingival plaque samples were collected from the clinically identical sites on quadrants 1 and 2 at the baseline and 1-, 2-, 4-, and 6-week follow-up visits by the same periodontist and then coded by a blinded assistant. In brief, the supragingival biofilm was removed by sterile cotton pellets; each site was dried and isolated from the saliva with sterile cotton rolls; 3 sterile paper points were inserted into the periodontal pocket to collect the subgingival biofilm and were immediately suspended in 0.5 mL of RNAlater storage solution (Sigma-Aldrich, St. Louis, United States) and stored at −20°C. In the next stage, DNA was isolated from the samples using commercial kits for DNA isolation, GeneJET (Fermentas). Quantification of F. nucleatum and P. intermedia was performed by using multicolored real-time polymerase chain reaction, TaqMan amplification, and ABI FAST 7500 sequence detection system. The primers, probes, and amplification conditions are shown in Table 1 [23]. F .nucleatum ATCC 25586 and P. intermedia ATCC 25611 were used as the standard references.

Table 1

Target primer/probe sequence and amplification condition for quantitative real-time PCR used in this study.

	Primer sequence (5′-3′)	Thermal program
Prevotella intermedia	F : CCACATATGGCATCTGACGTG	10 min at 95^°C, 40 cycles at 95^°C for 15 s, 58^°C for 60 s, 72^°C for 45 s, and a final extension at 72^°C for 5 min
	R : TCAATCTGCACGCTACTTGG
	P : FAM-ACCAAAGATTCTACGGTGGAGGATGGG-QSY
Fusobacterium nucleatum	F : CGCAGAAGGTGAAAGTCCTGTAT
	R : TGGTCCTCACTGATTCACACAGA
	P : ABY- ACTTTGCTCCCAAGTAACATGGAACAC GAG-QSY

F: forward primer; R: reverse primer; P: probe; FAM: 6-carboxyfluorescein.

2.4. Statistical Analysis

Statistical analysis was performed using SPSS ver. 19.0 (IBM Co., Armonk, NY, USA). The clinical parameters were calculated as means for each group and for each time point, before, and after the treatment protocols. Comparison of the baseline values was performed using the paired T-test. To assess the effects of the PDT on bacteria recolonization in the same periodontal pocket, the Friedman test and Wilcoxon signed-rank test were carried out. The level of significance was set at $p < 0.05$ .

3. Result

3.1. Clinical Outcomes

A total of 12 patients were included in the study, including 6 male and 6 female patients, with a mean age of 53.27 ± 7.47 years. No significant differences ( $p < 0.05$ ) were identified in the evaluated clinical parameters (PD, CAL, PI, and BOP) between the two study groups at baseline. The intergroup comparison showed no statistical significance in any of the follow-up periods throughout the study ( $p < 0.05$ ). In the PDT group, the mean difference in the reduction of PD and CAL was statistically significant in the intragroup comparison from the 1^st week up to 4^th week of follow-up. On the other hand, only a week after conventional treatment, a significant reduction in PD was observed. Analysis of BOP in PDT revealed a statistically significant reduction from baseline to 6 weeks, but in the conventional treatment, this reduction was significant only up to 4 weeks compared to the baseline. Clinical outcomes at baseline and 1, 2, 4, and 6 weeks after treatment are presented in Table 2.

Table 2

Mean clinical data from baseline through 6 weeks of follow-up of the study groups.

Clinical parameters	Conventional treatment					PDT
	Baseline	After treatment (weeks)				Baseline	After treatment (weeks)
	Baseline	1	2	4	6	Baseline	1	2	4	6
Pocket depth (mm)	4.38 ± 0.61	3.88 ± 0.41 $^{*}$	3.96 ± 0.52	4.08 ± 0.55	4.08 ± 0.55	4.46 ± 0.68	4.00 ± 0.63 $^{*}$	4.00 ± 0.79 $^{*}$	4.17 ± 0.56 $^{*}$	4.29 ± 0.57
Clinical attachment loss (mm)	4.00 ± 1.08	3.46 ± 1.24	3.58 ± 1.08	3.75 ± 1.09	3.83 ± 0.98	4.38 ± 1.42	3.75 ± 1.53 $^{*}$	3.92 ± 1.48 $^{*}$	4.04 ± 1.42 $^{*}$	4.17 ± 1.38
Plaque index	1.04 ± 0.33	0.79 ± 0.16	0.79 ± 0.20	0.92 ± 0.29	0.96 ± 0.36	1.04 ± 0.28	0.85 ± 0.18	0.75 ± 0.22 $^{*}$	0.81 ± 0.21	0.88 ± 0.29
Bleeding on probing (%)	85.42 ± 20.58	56.25 ± 10.54 $^{*}$	58.33 ± 16.87 $^{*}$	58.33 ± 12.08 $^{*}$	68.75 ± 16.87	85.42 ± 20.83	54.17 ± 15.02 $^{*}$	58.33 ± 11.02 $^{*}$	60.42 ± 12.50 $^{*}$	66.67 ± 13.18 $^{*}$

Repeated ANOVA was used to compare within-group differences ( $^{*} p < 0.05$ ). All data are presented in mean ± SD.

3.2. Bacterial Profile

Microbiological data are shown in Table 3. All groups showed a significant reduction in the amount of F. nucleatum and P. intermedia after 1 week of treatment ( $p < 0.02$ ). When compared to 1 week after treatment, the conventional treatment group showed significantly lower reducing effects of F. nucleatum ( $p < 0.02$ ) and P. intermedia ( $p = 0.03$ ) from the 2 and 4 weeks after treatment, respectively. In contrast, there was no statistically significant increase in the amount of F. nucleatum and P. intermedia after treatment with PD throughout the entire study period. The median, mean, 25th to 75th percentiles, maximum, minimum, and maximum outlier of F. nucleatum and P. intermedia from baseline through 6 weeks of follow-up are presented in Figure 1. Effect of conventional and photodynamic treatments on the amount of F. nucleatum copy unit and P. intermedia copy unit from each site of all 12 chronic periodontitis patients at baseline, a week, and 6 weeks following nonsurgical periodontal treatment is shown in Figure 2.

Table 3

Median and interquartile range of bacterial unit from baseline through 6 weeks of follow-up of the study groups.

		Baseline	After treatment (weeks)
		Baseline	1	2	4	6
F. nucleatum	Conventional treatment	420.94 (181–955)	102.75 (54–314) $^{#}$	513.46 (197–895) $^{*}$	394.63 (191–953) $^{*}$	655.56 (346–1568) $^{*}$
F. nucleatum	PDT	561.54 (215–1109)	243.65 (44–616) $^{#}$	254.22 (70–1053)	238.14 (90–832)	433.10 (91–631)

P. intermedia	Conventional treatment	44.10 (28.9–302)	14.03 (0.2–35) $^{#}$	20.40 (0.3–87)	63.55 (0.2–228) $^{*}$	104.73 (0.3–355) $^{*}$
P. intermedia	PDT	141.17 (30.85–378)	13.34 (0.1–52) $^{#}$	28.21 (0.1–436)	13.08 (0.1–67)	15.79 (0.2–252)

All data are presented in median (quartile 1–quartile 3).

[figures omitted; refer to PDF]

4. Discussion

Several studies have shown that access limitations during scaling root planing and unfavorable clinical response to conventional treatment appeared to be a consequence of subgingival ecological changes associated with increased gingival inflammation and clinical attachment loss [15, 24, 25]. In the present clinical study, periodontal examinations showed improvement in the inflammatory reactions, and there was a >10% reduction in pocket depth following one complete SRP. While these reductions gradually rebound back, we observed continual beneficial effects of Curcuma longa extract-mediated photodynamic therapy for up to 6 weeks.

In a classical study, recolonization of the subgingival microflora after 7 days of SRP was similar to that of periodontal healthy sites [26]. Even though cultural and dark‐field examination data have detected a nonspecific recolonization of bacteria at the 21‐day sampling point, our TaqMan quantitative DNA examination revealed a significant reemergence of subgingival F. nucleatum and P. intermedia after 14 and 21 days of the conventional SRP. Interestingly, this gradual accumulation of two target subgingival bacteria was found only in conventional treatment but not in the photodynamic therapy group. Our findings are in accordance with the previous photodynamic therapy study which reported antiperiopathogenic bacteria and F. nucleatum from the gingival sulcus [27]. However, the previous report was limited to only young adults with mild to moderate gingivitis.

In recent decades, many reports have proposed different wavelengths and light energies against biofilm growth in vitro [28–30]. In our previous study, we have established the optimal concentration of Curcuma longa extract solution and the use of blue light energy as an effective photosensitizer in PDT against periodontal bacteria [20]. It was also noted that the same dose of photosensitizer in gel form and blue light from periodontal probe-like quartz (subgingival 25 μg/mg Curcuma longa extract irradiated with blue LED light energy density = 16.8 J/cm²) can be used to attain significant therapeutic effects without any local and systemic adverse effects in mild to moderate chronic periodontitis patients with healthy medical condition.

We conclude that Curcuma longa gel extract and blue LEDs can be used in the gingival sulcus for photodynamic adjunctive therapy to suppress subgingival recolonization of F. nucleatum and P. intermedia following conventional mechanical debridement with no detectable damage to the adjacent areas.

Wilcoxon signed-rank test was used to compare within-group differences ( $^{#} p < 0.05$ , compared with baseline; $^{*} p < 0.05$ , compared with 1 week after treatment).

The median (solid bar), mean (cross), 25th to 75th percentiles (box), maximum and minimum (whisker), and maximum outlier (dot) were indicated. The black and red asterisks indicate a statistically significant difference of bacterial unit when compared with baseline and the first week of follow-up, respectively ( $p < 0.05$ ).

Acknowledgments

This work was supported by IRD9-906-62-12-11 from Suranaree University of Technology Research and Development Fund. We would like to thank Associate Professor Yasuo Takeuchi, Tokyo Medical and Dental University, for his generous preparation of all target bacteria, Center for Research and Development of Herbal Health Products for providing Curcuma longa gel extract, and Research Group of Chronic Inflammatory Oral Diseases and Systemic Diseases Associated with Oral Health for the research equipment.

References

[1] T. Okuda, E. Kokubu, T. Kawana, A. Saito, K. Okuda, K. Ishihara, "Synergy in biofilm formation between fusobacterium nucleatum and prevotella species," Anaerobe, vol. 18 no. 1, pp. 110-116, DOI: 10.1016/j.anaerobe.2011.09.003, 2012.

[2] B. Signat, C. Roques, P. Poulet, D. Duffaut, "Role of Fusobacterium nucleatum in periodontal health and disease," Current Issues in Molecular Biology, vol. 13 no. 2, pp. 25-36, DOI: 10.21775/cimb.013.025, 2011.

[3] A. Ashimoto, C. Chen, I. Bakker, J. Slots, "Polymerase chain reaction detection of 8 putative periodontal pathogens in subgingival plaque of gingivitis and advanced periodontitis lesions," Oral Microbiology and Immunology, vol. 11 no. 4, pp. 266-273, DOI: 10.1111/j.1399-302X.1996.tb00180.x, 1996.

[4] P.-M. Jervoe-Storm, M. Koltzscher, W. Falk, A. Dörfler, S. Jepsen, "Comparison of culture and real-time PCR for detection and quantification of five putative periodontopathogenic bacteria in subgingival plaque samples," Journal of Clinical Periodontology, vol. 32 no. 7, pp. 778-783, DOI: 10.1111/j.1600-051X.2005.00740.x, 2005.

[5] W. E. C. Moore, L. V. H. Moore, "The bacteria of periodontal diseases," Periodontology 2000, vol. 5, pp. 66-67, DOI: 10.1111/j.1600-0757.1994.tb00019.x, 1994.

[6] R. P. Teles, A. D. Haffajee, S. S. Socransky, "Microbiological goals of periodontal therapy," Periodontology 2000, vol. 42, pp. 180-218, DOI: 10.1111/j.1600-0757.2006.00192.x, 2006.

[7] A. D. Haffajee, S. S. Socransky, M. R. Patel, X. Song, "Microbial complexes in supragingival plaque," Oral Microbiology and Immunology, vol. 23 no. 3, pp. 196-205, DOI: 10.1111/j.1399-302X.2007.00411.x, 2008.

[8] G. A. Weijden, M. F. Timmerman, E. Reijerse, G. N. Wolffe, A. J. Winkelhoff, U. Velden, "The prevalence of A. actinomycetemcomitans , P. gingivalis and P. intermedia in selected subjects with periodontitis," Journal of Clinical Periodontology, vol. 21 no. 9, pp. 583-588, DOI: 10.1111/j.1600-051X.1994.tb00747.x, 1994.

[9] J. M. Albandar, L. J. Brown, H. Löe, "Putative periodontal pathogens in subgingival plaque of young adults with and without early-onset periodontitis," Journal of Periodontology, vol. 68 no. 10, pp. 973-981, DOI: 10.1902/jop.1997.68.10.973, 1997.

[10] S. Nakagawa, H. Fujii, Y. Machida, K. Okuda, "A longitudinal study from prepuberty to puberty of gingivitis. Correlation between the occurrence of Prevotella intermedia and sex hormones," Journal of Clinical Periodontology, vol. 21 no. 10, pp. 658-665, DOI: 10.1111/j.1600-051X.1994.tb00783.x, 1994.

[11] W. J. Loesche, S. A. Syed, B. E. Laughon, J. Stoll, "The bacteriology of acute necrotizing ulcerative gingivitis," Journal of Periodontology, vol. 53 no. 4, pp. 223-230, DOI: 10.1902/jop.1982.53.4.223, 1982.

[12] D. J. Bradshaw, P. D. Marsh, G. K. Watson, C. Allison, "Role of Fusobacterium nucleatum and coaggregation in anaerobe survival in planktonic and biofilm oral microbial communities during aeration," Infection and Immunity, vol. 66 no. 10,DOI: 10.1128/iai.66.10.4729-4732.1998, 1998.

[13] Y.-J. Jung, H.-K. Jun, B.-K. Choi, "Porphyromonas gingivalis suppresses invasion of Fusobacterium nucleatum into gingival epithelial cells," Journal of Oral Microbiology, vol. 9 no. 1,DOI: 10.1080/20002297.2017.1320193, 2017.

[14] Y. Li, H. Guo, X. Wang, Y. Lu, C. Yang, P. Yang, "Coinfection with Fusobacterium nucleatum can enhance the attachment and invasion of Porphyromonas gingivalis or Aggregatibacter actinomycetemcomitans to human gingival epithelial cells," Archives of Oral Biology, vol. 60 no. 9, pp. 1387-1393, DOI: 10.1016/j.archoralbio.2015.06.017, 2015.

[15] P. V. Borgo, V. A. A. Rodrigues, A. C. R. Feitosa, K. C. B. Xavier, M. J. Avila-Campos, "Association between periodontal condition and subgingival microbiota in women during pregnancy: a longitudinal study," Journal of Applied Oral Science, vol. 22 no. 6, pp. 528-533, DOI: 10.1590/1678-775720140164, 2014.

[16] T. S. Miranda, M. Feres, B. Retamal-Valdés, "Influence of glycemic control on the levels of subgingival periodontal pathogens in patients with generalized chronic periodontitis and type 2 diabetes," Journal of Applied Oral Science, vol. 25 no. 1, pp. 82-89, DOI: 10.1590/1678-77572016-0302, 2017.

[17] F. Duarte, D. Karapetsa, B. Alonso, D. Herrera, "Nonsurgical and surgical treatment of periodontitis: how many options for one disease?, " , Periodontology 2000, vol. 75 no. 1, pp. 152-188, DOI: 10.1111/prd.12201, 2017.

[18] A. D. Haffajee, M. A. Cugini, S. Dibart, C. Smith, R. L. Kent, S. S. Socransky, "The effect of SRP on the clinical and microbiological parameters of periodontal diseases," Journal of Clinical Periodontology, vol. 24 no. 5, pp. 324-334, DOI: 10.1111/j.1600-051X.1997.tb00765.x, 1997.

[19] K. Cugini, S. Jepsen, "Antibiotics/antimicrobials: systemic and local administration in the therapy of mild to moderately advanced periodontitis," Periodontology 2000, vol. 71 no. 1, pp. 82-112, DOI: 10.1111/prd.12121, 2016.

[20] D. Saitawee, A. Teerakapong, N. P. Morales, P. Jitprasertwong, D. Hormdee, "Photodynamic therapy of Curcuma longa extract stimulated with blue light against Aggregatibacter actinomycetemcomitans," Photodiagnosis and Photodynamic Therapy, vol. 22, pp. 101-105, DOI: 10.1016/j.pdpdt.2018.03.001, 2018.

[21] J. Silness, H. Löe, "Periodontal disease in pregnancy II. Correlation between oral hygiene and periodontal condition," Acta Odontologica Scandinavica, vol. 22 no. 1, pp. 121-135, DOI: 10.3109/00016356408993968, 1964.

[22] J. Ainamo, I. Bay, "Problems and proposals for recording gingivitis and plaque," International Dental Journal, vol. 25 no. 4, pp. 229-235, 1975.

[23] E. Gaetti-Jardim, S. L. Marcelino, A. C. R. Feitosa, G. A. Romito, M. J. Avila-Campos, "Quantitative detection of periodontopathic bacteria in atherosclerotic plaques from coronary arteries," Journal of Medical Microbiology, vol. 58 no. 12, pp. 1568-1575, DOI: 10.1099/jmm.0.013383-0, 2009.

[24] A. Mombelli, "Microbial colonization of the periodontal pocket and its significance for periodontal therapy," Periodontology 2000, vol. 76 no. 1, pp. 85-96, DOI: 10.1111/prd.12147, 2018.

[25] M. Feres, M. Bernal, F. Matarazzo, M. Faveri, P. Duarte, L. Figueiredo, "Subgingival bacterial recolonization after scaling and root planing in smokers with chronic periodontitis," Australian Dental Journal, vol. 60 no. 2, pp. 225-232, DOI: 10.1111/adj.12225, 2015.

[26] L. Sbordone, L. Ramaglia, E. Gulletta, V. Iacono, "Recolonization of the subgingival microflora after scaling and root planing in human periodontitis," Journal of Periodontology, vol. 61 no. 9, pp. 579-584, DOI: 10.1902/jop.1990.61.9.579, 1990.

[27] A. Alqerban, "Efficacy of antimicrobial photodynamic and photobiomodulation therapy against treponema denticola, fusobacterium nucleatum and human beta defensin-2 levels in patients with gingivitis undergoing fixed orthodontic treatment: a clinic-laboratory study," Photodiagnosis and Photodynamic Therapy, vol. 29,DOI: 10.1016/j.pdpdt.2020.101659, 2020.

[28] S. Eick, G. Markauskaite, S. Nietzsche, O. Laugisch, G. E. Salvi, A. Sculean, "Effect of photoactivated disinfection with a light-emitting diode on bacterial species and biofilms associated with periodontitis and peri-implantitis," Photodiagnosis and Photodynamic Therapy, vol. 10 no. 2, pp. 156-167, DOI: 10.1016/j.pdpdt.2012.12.001, 2013.

[29] C. R. Fontana, A. D. Abernethy, S. Som, "The antibacterial effect of photodynamic therapy in dental plaque-derived biofilms," Journal of Periodontal Research, vol. 44 no. 6, pp. 751-759, DOI: 10.1111/j.1600-0765.2008.01187.x, 2009.

[30] D. Park, M. Kim, J. W. Choi, J. H. Baek, S. H. Lee, K. Baek, "Antimicrobial photodynamic therapy efficacy against specific pathogenic periodontitis bacterial species," Photodiagnosis and Photodynamic Therapy, vol. 30,DOI: 10.1016/j.pdpdt.2020.101688, 2020.

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Objective. To evaluate the amount of Fusobacterium nucleatum (F. nucleatum) and Prevotella intermedia (P. intermedia) on subgingival recolonized plaque after mechanical debridement and photodynamic treatment by using blue light-emitting diodes (LEDs) in combination with topical Curcuma longa gel extract. Methods. A total of 12 subjects with stage III grade B periodontitis were recruited for the study. Maxillary posterior teeth with periodontal pocket >4 mm were selected. These teeth were examined for periodontal clinical data at baseline and at 1, 2, 4, and 6 weeks after treatment. All remaining teeth were treated by scaling and root planing (SRP). Then, the teeth were bilaterally divided using randomized split-mouth design with and without photodynamic adjunctive therapy (PDT). Samples of the subgingival microbiota were obtained in each visit. All samples were analyzed by multicolor TaqMan real-time polymerase chain reaction (PCR) for the presence of target bacteria. Results. Throughout the six-week follow-up, long-term improvement of probing depth and bleeding on probing was revealed on the PDT group. The number of subgingival F. nucleatum and P. intermedia also significantly reduced, compared to the baseline. There was a statistically significant recolonization in F. nucleatum and P. intermedia number after 2 and 4 weeks of conventional SRP, respectively. Our quantitative PCR method showed no significant recolonization of those subgingival bacteria on PDT sites throughout the 6-week study duration. Conclusion. The results showed that adjunctive photodynamic treatment by using blue LEDs in combination with topical Curcuma longa gel extract was effective to alter the recolonization patterns of F. nucleatum and P. intermedia after conventional debridement.

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Title

Anti-Early Stage of Bacterial Recolonization Effect of Curcuma longa Extract as Photodynamic Adjunctive Treatment

Author

Hormdee, Doosadee¹

; Rinsathorn, Weena²

; Puasiri, Subin³

; Jitprasertwong, Paiboon⁴

¹ Division of Periodontology, Department of Oral Medical Science, Faculty of Dentistry and Research Group of Chronic Inflammatory Oral Diseases and Systemic Diseases Associated with Oral Health, Khon Kaen University, Khon Kaen, Thailand
² Division of Periodontology, Department of Oral Medical Science, Faculty of Dentistry, Khon Kaen University, Khon Kaen 40002, Thailand
³ Division of Community Dentistry, Department of Oral Prevention Faculty of Dentistry, Khon Kaen University, Khon Kaen 40002, Thailand
⁴ Institute of Dentistry, Suranaree University of Technology, Nakhon Ratchasima, Thailand

Editor

Caren Bavaresco

Publication year

2020

Publication date

2020

Publisher

John Wiley & Sons, Inc.

ISSN

16878728

e-ISSN

16878736

Source type

Scholarly Journal

Language of publication

English

DOI

https://doi.org/10.1155/2020/8823708

ProQuest document ID

2474858045

Anti-Early Stage of Bacterial Recolonization Effect of Curcuma longa Extract as Photodynamic Adjunctive Treatment

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