Saliva and tongue coating pH before and after use of mouthwashes and relationship with parameters of halitosis

Tolentino, Elen de Souza; Chinellato, Luiz Eduardo Montenegro; Tarzia, Olinda

doi:10.1590/S1678-77572011000200002

Abstract

OBJECTIVES: The aim of this work was to evaluate saliva and tongue coating pH in oral healthy patients with morning bad breath before and after use of different oral mouthrinses. MATERIAL AND METHODS: Saliva and tongue coating pH of 50 patients allocated in 5 groups were measured respectively by a digital pHmeter and color pH indicators, before, immediately after and 30 min after rinsing 5 different mouthrinses: cetilpiridine chloride associated with sodium chloride, triclosan, enzymatic solution, essential oil and distilled water. RESULTS: Only triclosan and essential oil increased salivary pH immediately after rising. The enzymatic solution decreased salivary and tongue coating pH immediately after rinsing. CONCLUSIONS: Salivary pH tended to be acidic while tongue coating pH tended to be alkaline, even after rising. Triclosan and essential oil mouthrinses increased salivary pH immediately after rinsing. Enzymatic solution decreased saliva and tongue coating pH immediately after rising.

Halitosis; Saliva; Tongue; Mouthwashes; pH

ORIGINAL ARTICLES

Saliva and tongue coating pH before and after use of mouthwashes and relationship with parameters of halitosis

Elen de Souza Tolentino^I; Luiz Eduardo Montenegro Chinellato^II; Olinda Tarzia^II

^IDDS, MSc, PhD student, Department of Stomatology, Bauru School of Dentistry, University of São Paulo, Bauru, SP, Brazil

^IIPhD, Professor, Department of Stomatology, Bauru School of Dentistry, University of São Paulo, Bauru, SP, Brazil

^IIIPhD, Assistant Professor, Department of Biological Sciences, Bauru School of Dentistry, University of São Paulo, Bauru, SP, Brazil

^{Corresponding address} Corresponding address: Elen de Souza Tolentino Rua: Campos Sales, nº 255 - apto 602 - Zona 07 87020-080 - Maringá - PR - Brasil e-mail: elen_tolentino@hotmail.com

ABSTRACT

OBJECTIVES: The aim of this work was to evaluate saliva and tongue coating pH in oral healthy patients with morning bad breath before and after use of different oral mouthrinses.

MATERIAL AND METHODS: Saliva and tongue coating pH of 50 patients allocated in 5 groups were measured respectively by a digital pHmeter and color pH indicators, before, immediately after and 30 min after rinsing 5 different mouthrinses: cetilpiridine chloride associated with sodium chloride, triclosan, enzymatic solution, essential oil and distilled water.

RESULTS: Only triclosan and essential oil increased salivary pH immediately after rising. The enzymatic solution decreased salivary and tongue coating pH immediately after rinsing.

CONCLUSIONS: Salivary pH tended to be acidic while tongue coating pH tended to be alkaline, even after rising. Triclosan and essential oil mouthrinses increased salivary pH immediately after rinsing. Enzymatic solution decreased saliva and tongue coating pH immediately after rising.

Key words: Halitosis. Saliva. Tongue. Mouthwashes. pH.

INTRODUCTION

The existence of an association between tongue microorganisms and those present in saliva has been reported⁶. The anaerobic microbiota of the tongue bioflm is one of the main responsible for the release of sulfur-containing compounds (VSC), which are directly involved in the occurrence of halitosis. The origin of halitosis has been localized in the oral cavity in up to 85% of people suffering from this condition. In most cases, it is produced in the mouth by the action of Gram-negative anaerobic bacteria on sulfur-containing proteinaceous substrates in the saliva, such as debris and plaque¹⁰.

The most common source of bad breath in individuals with good oral hygiene and healthy periodontal tissues is from the posterior dorsum of the tongue¹⁰, where the crypts are the favored sites for growth of the anaerobic bacteria responsible for halitosis. Several studies have implicated the dorsum of the tongue as the primary site of microfora putrefaction and the production of VSC^15,17.

Dry mouth is also related with oral malodor¹. A reduced saliva fow during sleep in healthy patients favors anaerobic bacterial putrefaction, giving rise to so-called "morning breath" or physiological halitosis, a transient condition resulting from decreased salivary fow and decreased activity of tongue and cheek muscles during sleep, which promotes the proliferation of bacteria of the oral cavity that are responsible for the emission of the VSC, which disappears after a meal¹⁰. Pathologic halitosis is more intense and is not easily reversible¹⁰.

The importance of halitosis has led to the formulation of different commercial products that are claimed to have anti-halitosis effect. The mechanisms of action of these solutions are in general due to their antimicrobial or oxidizing properties or their capacity to inhibit the formation of VSC, even in the presence of oral bacteria.Antibacterial components such as chlorhexidine, cetylpyridinium chloride, triclosan, essential oils, chlorine dioxide, zinc salts, benzalkonium chloride, hydrogen peroxide and sodium bicarbonate have been used in the treatment of halitosis, either alone or in combination, and either as a single mode of therapy or together with the mechanical treatment of tongue coating.

pH is the major regulating factor in the formation of bad breath⁶and the chemical control of bioflm with antimicrobial solutions may reduce the levels of microorganisms and VSC in patients with halitosis complaint. It is thus important to carry out new studies with these products and their actual infuence on salivary and tongue coating pH, as well as investigate the feasibility of the association of these aspects and the development of halitosis. The aim of this work was to evaluate saliva and tongue coating pH in oral healthy patients with physiological halitosis before and after use of different mouthrinses.

MATERIAL AND METHODS

This study was approved by the Human Research Ethics Committee of Bauru School of Dentistry, University of São Paulo (Process nº 008/2008). Fifty oral and systemic healthy dental students, aged over 18 years, from Bauru Dental School volunteered to participate in this study.

The exclusion criteria were subjects with medical disorders, such as diabetes mellitus, renal disease, gastrointestinal disorders, respiratory diseases¹³, evidence of recent bronchitis, sinusitis or tonsillitis³, pregnant women³, patients undergoing antibiotic or other antimicrobial therapy, smokers and those who, on pre-study clinical screening, presented a probing depth >4 mm, cavitated caries lesion, naso-pharyngeal alterations, mouth breathers and patients with prostheses, orthodontic or dental appliances.

Before examination, the patients received the following guidelines to improve standardization of data collection: avoid, 24 h before the second consultation, spicy and favored food, coffee, tea or alcoholic beverage; the night before perform oral hygiene as usual; be fasting for 8 h at the time of consultation; do not perform oral hygiene, use any kind of mint favoring or rinse solution or drink water before the consultation.

All patients attended two consultations, which were conducted by the same examinerr In the frst consultation, prior to the clinical examination, all subjects were asked to fll out a questionnaire⁴. Next, clinical examination was performed, mainly aiming the analysis of oral and systemic health of the patients. In the second consultation, all patients were seen in the morning, at 7 a.m., fasting for at least 8 h and without having performed any oral hygiene procedures on the day of consultation¹⁷, but having performed oral hygiene as usual the previous night at bedtime, with brushing and dental floss.

Each patient underwent three collections of saliva samples: at the beginning of the consultation, immediately after rising a specifc solution, and 30 min after rising (phases before, after, and 30 min, respectively). Each volunteer was submitted to a type of rinse with a specifc oral mouthrinse solution.

The patients were randomly assigned to 5 groups of 10 volunteers each, distributed as follows:

- SC Group: rinses with sodium chlorite combined with cetylpyridinium chloride - chlorine dioxide (Saúde Bucal^®; Embatek Technology in Cosmetics Ltd., São Paulo, SP, Brazil);

-TS Group: rinses with combined solution of triclosan (0r03%), sodium fuoride (225 ppm of fuorine) and copolymer PVMjMA (0r20%) Gantrez (Colgate Total Plax Classic^® 250 mL; Colgate-Palmolive and Industry Trade Ltd., São Bernardo do Campo, SP, Brazil);

-ES Group: rinses with enzyme solution - Lysozyme, Lactoferrin, Glucose Oxidase and Lactoperoxidase (Biotène Mouthwash^® 240 mL; Laclede, East University Drive, Rancho Dominguez, CA, USA);

-EO Group: rinses with essential oil (Listerine Cool Mint^®Oral antiseptic 1.5 L; Warner-Lambert Co., Morris Plains, NJ, USA);

-CTRL Group (control): rinses with distilled water (placebo).

Each volunteer rinsed with 20 mL of the solution for 30 s followed by gargling for 10 s.

Before saliva collection, patients were kept seated for 5 min, relaxed and without talking¹². Unstimulated saliva was collected over a period of 5 min. Before collection, the mouth was emptied by an initial swallow⁹. The examinator asked the subjects to spit out the produced saliva each 30 s in a plastic container (J-10; Injeplast^®, São Paulo, SP, Brazil)¹⁴. This procedure was performed before and after rising, and after 30 min.

Salivary pH was measured by a digital pH meter (Sentron Model 1001 pH System; Sentron Incorporated, 33320, USA), calibrated with standard solutions of pH 4.0 and 7.0. The electrode was washed with distilled water and dried with absorbent paper after each analysis⁸.

In the same consultation, tongue coating pH was measured using pH indicator strips (pH 0-14; Merck, Darmstadt, Germany). One strip was placed on posterior tongue region, with the patient with the mouth opened, for 1 min. The color change in the strip indicated tongue coating pH. The measurements were performed before, immediately and 30 min after rising.

Data were analyzed statistically by two-way ANOVA and Tukey's testr A signifcance level of 5% was set for all analyses.

RESULTS

The measurements of salivary and tongue coating pH in the 5 groups are presented in Tables 1 and 2. There was no statistically signifcant difference (p>0.05) in the salivary pH between the groups in the before and 30 min phases. In the after phase, the ES group presented mean values smaller than the EO and TS groups (Table 3). In the groups CTRL and SC there was no statistically signifcant difference (p>0.05) in salivary pH between the 3 phases. In the TS and EO groups, the mean pH values in the after phase were higher than the mean values obtained in the before and 30 min phases. In the ES group, the mean pH values in the before phase were higher than in the after phase (Table 4).

Thumbnail

In the tongue coating pH analysis, there was no statistically significant difference (p>0.05) between groups in the before and 30 min phases. In the after phase, the ES group presented smaller mean values than all other groups (Table 5). In the SC, TS, EO and CTRL groups, there were no statistically signifcant difference (p>0r05) between the 3 phases. In the ES group, average values in the after phase were smaller than the average in the phases before and 30 min (Table 6).

Thumbnail

DISCUSSION

The reduction in salivary fow during sleep and consequent increase in the number of epithelial cells scaled from oral mucosa lead to tongue coating formation and therefore in halitosis, even in healthy pacients²⁰. Several masking and antimicrobial agents have been proposed to control both physiological and pathological halitosis. Their clinical effcacy has often been tested on morning breath^4,11 rather than in real clinical situations for evident ethical reasons. It has been postulated that a decrease in salivation during sleep promotes proliferation of the oral bacteria responsible for the release of the offending gases in morning bad breath^4,11. Strong evidence that morning breath odor can be used as a model for investigation of other offensive odors is still lacking but universally accepted¹⁸r This fact justifes the use of oral healthy patients with morning breath odor in this research.

Saliva of individuals with "dry mouth" (common situation after a night of sleep) often presents acidic pH^5,16. However, there is a tendency that salivary pH becomes more alkaline during the day, by the act of talking or chewing. Salivary pH is slightly acidic before its secretion in oral cavity. It becomes alkaline at the time of gland's secretion due to loss of carbon dioxide (CO₂) and increase of saliva's bicarbonate concentration when salivary fow is increased²⁰r Hypothetically, body fuid pHs remain relatively constant because of buffering systems, fact that is not different in the saliva, which, many times, keeps its pH constant, even after rising with acidic solutions, for example. In the present study, the most notable changes in pH were observed immediately after rising, but were stabilized after 30 min. Moreover, salivary pH remained slightly acidic in all stages in all groups, possibly due to the effect of mouthrinses or the buffer capacity of saliva.

To discuss these fndings of this study, we put in question whether salivary pH, considered acidic after sleeping, would have a direct infuence in halitosis or whether morning breath odor is only due to increased mucosa desquamation and formation of tongue coating. According to McNamara, et al.¹²(1972), pH is the major regulating factor in the formation of bad breath and is clearly established that acidity inhibits the production of odors while neutrality and alkalinity favor it¹². The same context is applied to tongue coating pH, which has alkaline pH due to the production of odorivetores during proteolysis²⁰r Among the fnal products of proteolysis are amines, ammonia and urea, which have alkaline pH, characteristic of physiological or pathological halitosis²⁰. It is also questioned whether the use of mouthrinses could change these pH values and thus infuence, in the reduction of halitosis after their use. For that reason, it would be logical that mouthrinses provide reduction of saliva and tongue coating pH in order to reduce halitosis.

In the present study, there was no statistically signifcant difference in salivary pH between the groups, in the phases before and after 30 min of rinsing. In the after phase, the ES group presented smaller mean values than the TS and EO groups. In the CTRL and SC groups, there was no statistically signifcant difference in salivary pH between the 3 phases. In the TS and EO groups, the mean pH values in the phase after were higher than those recorded before and after 30 min of rinsing. In the ES group, the mean pH values before rinsing was higher than immediately after rinsing. According to the present research, rinsing with mouthwashes based on triclosan and essential oils lead to an increase in salivary pH, both lasting for 30 min. This can be explained by the fact that mouthrinses that cause mouth burning (fact reported by the volunteers of the groups TS and EO) stimulate salivation and thus increase salivary pH²⁰. For the ES group, there was a pH decrease immediately after its use; however, there was no information in literature about pH decreasing caused by enzymatic solutions.

In the control group, in which the volunteers rinsed with distilled water, there was an increase in salivary pH during the measurements. It can be explained because of the increase in the saliva's bicarbonate concentration when salivary fow is increased, a condition that is common over time: salivary pH increases with the increase of fow². In the study of Suarez, et al.¹⁹(2000), patients with complete oral health were submitted to measurements of bad breath after any kind of oral hygiene and water only when necessary. The authors observed that the concentrations of each gas tended to decrease in the frst hour after waking. After this period the concentration tended to remain stable or increase in the next 7 h.

In our research, the analysis of tongue coating pH showed no statistically signifcant difference between the groups, in the phases before and after 30 min of rising. In the after phase, the ES group presented smaller mean values than all other groups. In the SC, TS, EO and CTRL groups, there was no signifcant difference between the three phases. In the ES group, the mean values of the after phase were lower than those obtained before and after 30 min of rinsing. It is known that tongue coating is the main cause of oral halitosis^5,11,20-22and that its pH tends to be alkaline. Only risings with enzymatic solution (ES group) provided pH decrease immediately after its use; however, the mechanism of action is not clearly described in the literaturer The benefcial impact of oral mouthrinses on the bacterial load on the dorsum tongue is clearly demonstrated in the study of Steenberghe, et al.¹⁸(2001).

This study was conducted in oral healthy patients, which is a factor of extreme importance to avoid the development of chronic halitosis, since bad breath is closely associated to poor oral hygiene. The measurements of saliva and tongue coating pH in healthy patients with physiological halitosis homogenized the method. Patients should be aware that some bacteria are inevitably left behind after mechanical plaque control, even with an optimal technique. If the oral hygiene is not performed properly, gingivitis, caries, periodontitis and eventually halitosis may develop. The dental professional could explain that antiseptic rinsing kills additional bacteria and helps controlling plaque. For absolute clarity, rinsing should be described as an adjunct to an established daily oral-care routine, rather than a substitute for brushing and interdental cleaning⁷.

CONCLUSIONS

According to the methodology applied in this study, it may be concluded that:

-In a situation of physiological halitosis, salivary pH tended to be acidic while tongue coating pH tended to be alkaline, even after the use of mouthrinses;

-Only triclosan and essential oil mouthrinses increased salivary pH immediately after rising;

-The enzymatic solution was able to decrease saliva and tongue coating pH immediately after rising.

ACKNOWLEDGEMENTS

The authors would like to thank Ovídio dos Santos Sobrinho, Thelma Lopes Silva and José Roberto Lauris for the support of this study. This investigation was supported by CAPES.

Received: June 9, 2009

Modifcation: August 7, 2009,

Accepted: October 14, 2009

1- Almas K, Al-Hawish A, Al-Khamis W. Oral hygiene practices, smoking habits, and self-perceived oral malodor among dental students. J Contemp Dent Pract. 2003;4(4):77-90.
2- Bartlett DW, Bureau GP, Anggiansah A. Evaluation of the pH of a new carbonated soft drink beverage: an in vivo investigation. J Prosthodont. 2003;12(1):21-5.
3- Borden LC, Chaves ES, Bowman JP, Fath BM, Hollar GL. The effect of four mouthrinses on oral malodor. Compendi Contin Educ Dent. 2002;23(6):531-46.
4- Bornstein MM, Stocker BL, Seemann R, Burgin WB, Lussi A. Prevalence of halitosis in young male adults: a study in Swiss army recruits comparing self-reported and clinical data. J Periodontol. 2009;80(1):24-31.
5- Bosy A, Kulkarni GV, Rosemberg M, McCulloch CA. Relationship of oral malodor to periodontitis: evidence of independence in discrete subpopulations. J Periodontol. 1994;65(1):37-46.
6- Casemiro LA, Martins CH, Carvalho TC, Panzeri H, Lavrador MA, Pires-de-Souza FC. Effectiveness of a new toothbrush design versus a conventional tongue scraper in improving breath odor and reducing tongue microbiota. J Appl Oral Sci. 2008;16(4):271-4.
7- Claffey N. Essential oil mouthwashes: a key component in oral health management. J Clin Periodontol. 2003;30(Suppl 5):22-4.
8- Delbem AC, Sassaki KT, Castro AM, Pinto LM, Bergamaschi M. Assessment of the fluoride concentration and pH in different mouthrinses on the Brazilian market. J Appl Oral Sci. 2003;11(4):319-22.
9- Gavião MB, Van der Bilt A. Salivary secretion and chewing: stimulatory effects from artifcial and natural foodsr J Appl Oral Sci. 2004;12(2):159-63.
10- Messadi DV, Younai FS. Halitosis. Dermatol Clin. 2003;21(1):147-55.
11- McDowell JD, Kassebaum DK. Diagnosing and treating halitosis. J Am Dent Assoc. 1993;124:55-64.
12- McNamara TF, Alexander JF, Lee M. The role of microorganisms in the production of oral malodor. Oral Surg Oral Med Oral Pathol. 1972;34(1):41-8.
13- Nalçaci R, Sönmez IS. Evaluation of oral malodor in children. Oral Surg Oral Med Oral Pathol Oral Radiol Endod. 2008;106(3):384-8.
14- Nikolopoulou F, Tzortzopoulou E. Salivary pH in edentulous patients before and after wearing conventional dentures and implant overdentures: a clinical study. Implant Dent. 2007;16(4):397-402.
15- Rosenberg M. Clinical assessment of bad breath: current concepts. J Am Dent Assoc. 1996;127(11):475-82.
16- Rosenberg M, Kulkarni GV, Bosy A, McCulloch CA. Reproducibility and sensitivity of oral malodor measurements with a portable sulphide monitor. J Dent Res. 1991;70(11):1436-40.
17- Rosenberg M, McCulloch CA. Measurement of oral malodor: current methods and future prospects. J Periodontol. 1992;63(9):776-82.
18- Van Steenberghe D, Avontroodt P, Peeters W, Pauwels M, Coucke W, Lijnen A, et al. Effect of different mouthrinses on morning breath. J Periodontol. 2001;72(9):1183-91.
19- Suarez FL, Furne JK, Springfield J, Levitt MD. Morning breath odor: infuence of treatments on sulfur gasesr J Dent Resr 2000;79(10):1773-7.
20- Tarzia O. Halitose. 1^st ed. Rio de Janeiro: EPUB; 2003.
21- Tonzetich J. Production and origin of oral malodor: a review of mechanisms and methods of analysis. J Periodontol. 1977;48(1):13-20.
22- Yaegaki K, Sanada K. Biochemical and clinical factors infuencing oral malodor in periodontal patientsr J Periodontolr 1992;63(9):783-9.

Corresponding address:

Elen de Souza Tolentino

Rua: Campos Sales, nº 255 - apto 602 - Zona 07

87020-080 - Maringá - PR - Brasil

e-mail:

elen_tolentino@hotmail.com

Publication Dates

Publication in this collection
02 May 2011
Date of issue
Apr 2011

History

Received
09 June 2009
Reviewed
07 Aug 2009
Accepted
14 Oct 2009

This work is licensed under a Creative Commons Attribution 4.0 International License.

[1] 1- Almas K, Al-Hawish A, Al-Khamis W. Oral hygiene practices, smoking habits, and self-perceived oral malodor among dental students. J Contemp Dent Pract. 2003;4(4):77-90.

[2] 2- Bartlett DW, Bureau GP, Anggiansah A. Evaluation of the pH of a new carbonated soft drink beverage: an in vivo investigation. J Prosthodont. 2003;12(1):21-5.

[3] 3- Borden LC, Chaves ES, Bowman JP, Fath BM, Hollar GL. The effect of four mouthrinses on oral malodor. Compendi Contin Educ Dent. 2002;23(6):531-46.

[4] 4- Bornstein MM, Stocker BL, Seemann R, Burgin WB, Lussi A. Prevalence of halitosis in young male adults: a study in Swiss army recruits comparing self-reported and clinical data. J Periodontol. 2009;80(1):24-31.

[5] 5- Bosy A, Kulkarni GV, Rosemberg M, McCulloch CA. Relationship of oral malodor to periodontitis: evidence of independence in discrete subpopulations. J Periodontol. 1994;65(1):37-46.

[6] 6- Casemiro LA, Martins CH, Carvalho TC, Panzeri H, Lavrador MA, Pires-de-Souza FC. Effectiveness of a new toothbrush design versus a conventional tongue scraper in improving breath odor and reducing tongue microbiota. J Appl Oral Sci. 2008;16(4):271-4.

[7] 7- Claffey N. Essential oil mouthwashes: a key component in oral health management. J Clin Periodontol. 2003;30(Suppl 5):22-4.

[8] 8- Delbem AC, Sassaki KT, Castro AM, Pinto LM, Bergamaschi M. Assessment of the fluoride concentration and pH in different mouthrinses on the Brazilian market. J Appl Oral Sci. 2003;11(4):319-22.

[9] 9- Gavião MB, Van der Bilt A. Salivary secretion and chewing: stimulatory effects from artifcial and natural foodsr J Appl Oral Sci. 2004;12(2):159-63.

[10] 10- Messadi DV, Younai FS. Halitosis. Dermatol Clin. 2003;21(1):147-55.

[11] 11- McDowell JD, Kassebaum DK. Diagnosing and treating halitosis. J Am Dent Assoc. 1993;124:55-64.

[12] 12- McNamara TF, Alexander JF, Lee M. The role of microorganisms in the production of oral malodor. Oral Surg Oral Med Oral Pathol. 1972;34(1):41-8.

[13] 13- Nalçaci R, Sönmez IS. Evaluation of oral malodor in children. Oral Surg Oral Med Oral Pathol Oral Radiol Endod. 2008;106(3):384-8.

[14] 14- Nikolopoulou F, Tzortzopoulou E. Salivary pH in edentulous patients before and after wearing conventional dentures and implant overdentures: a clinical study. Implant Dent. 2007;16(4):397-402.

[15] 15- Rosenberg M. Clinical assessment of bad breath: current concepts. J Am Dent Assoc. 1996;127(11):475-82.

[16] 16- Rosenberg M, Kulkarni GV, Bosy A, McCulloch CA. Reproducibility and sensitivity of oral malodor measurements with a portable sulphide monitor. J Dent Res. 1991;70(11):1436-40.

[17] 17- Rosenberg M, McCulloch CA. Measurement of oral malodor: current methods and future prospects. J Periodontol. 1992;63(9):776-82.

[18] 18- Van Steenberghe D, Avontroodt P, Peeters W, Pauwels M, Coucke W, Lijnen A, et al. Effect of different mouthrinses on morning breath. J Periodontol. 2001;72(9):1183-91.

[19] 19- Suarez FL, Furne JK, Springfield J, Levitt MD. Morning breath odor: infuence of treatments on sulfur gasesr J Dent Resr 2000;79(10):1773-7.

[20] 20- Tarzia O. Halitose. 1^st ed. Rio de Janeiro: EPUB; 2003.

[21] 21- Tonzetich J. Production and origin of oral malodor: a review of mechanisms and methods of analysis. J Periodontol. 1977;48(1):13-20.

[22] 22- Yaegaki K, Sanada K. Biochemical and clinical factors infuencing oral malodor in periodontal patientsr J Periodontolr 1992;63(9):783-9.