remineralization effectiveness of mi paste plus - a clinical pilo
TRANSCRIPT
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University of IowaIowa Research Online
Theses and Dissertations
2011
Remineralization effectiveness of MI Paste Plus - aclinical pilot studySarah Elizabeth ClarkUniversity of Iowa
Copyright 2011 Sarah Clark
This dissertation is available at Iowa Research Online: http://ir.uiowa.edu/etd/939
Follow this and additional works at: http://ir.uiowa.edu/etd
Part of the Orthodontics and Orthodontology Commons
Recommended CitationClark, Sarah Elizabeth. "Remineralization effectiveness of MI Paste Plus - a clinical pilot study." master's Master's thesis, University ofIowa, 2011.http://ir.uiowa.edu/etd/939.
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REMINERALIZATION EFFECTIVENESS OF MI PASTE PLUSTM A CLINICAL
PILOT STUDY
by
Sarah Elizabeth Clark
A thesis submitted in partial fulfillment of the requirements for the Master of
Science degree in Orthodontics in the Graduate College of
The University of Iowa
May 2011
Thesis Supervisor: Professor Robert. N. Staley
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Graduate College The University of Iowa
Iowa City, Iowa
CERTIFICATE OF APPROVAL
_______________________
MASTER'S THESIS
_______________
This is to certify that the Master's thesis of
Sarah Elizabeth Clark
has been approved by the Examining Committee for the thesis requirement for the Master of Science degree in Orthodontics at the May 2011 graduation.
Thesis Committee: Robert. N. Staley, Thesis Supervisor
Clayton Parks
James Wefel
Fang Qian
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To my loving husband, Tanner
To my supportive parents, Dan and Karen
To my inspirational sister and brother, Kristin and John
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ACKNOWLEDGMENTS
I would like to thank Drs. Robert Staley, Clayton Parks, James Wefel, and Fang
Qian for serving on my thesis committee and for all the input and support during this project. I would also like to thank Jeff Harless for his patience, support, and insight into using the quantitative light-induced fluorescence unit.
I would also like to thank Dr. Tom Southard and the rest of the faculty at the
University of Iowa, Department of Orthodontics for giving me the opportunity to further
my education and pursue a career in orthodontics.
Lastly, I would like to thank Tanner for being an outstanding husband and friend,
I know you will make a wonderful father.
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TABLE OF CONTENTS
LIST OF TABLES ...............................................................................................................v
LIST OF FIGURES ......................................................................................................... viii
INTRODUCTION ...............................................................................................................1
Purpose of this Study ...............................................................................................3
LITERATURE REVIEW ....................................................................................................4
Development of a White Spot Lesion .....................................................................4 White Spot Lesions in Orthodontic Patients ...........................................................6 Methods to Decrease Demineralization during Orthodontic Treatment .................7 Mechanism of Action of Fluoride ...........................................................................9 Fluoride Dentrifice ................................................................................................10 Mechanism of Action of Casein Phosphopeptides ................................................11 Casein Phosphopeptide Amorphous Calcium Phosphate (CPP-ACP) ...............11 Quantitative Light-induced Fluorescence (QLF) ..................................................15
MATERIALS AND METHODS .......................................................................................18
Sample ...................................................................................................................18 Patient Inclusion Criteria .......................................................................................18 Clinical Procedure .................................................................................................18 Measurement of Data ............................................................................................21 Statistical Analysis ................................................................................................23 Reliability of Intra- and Inter-Examiner Measurement of Lesion Area ................24
RESULTS ..........................................................................................................................31
DISCUSSION ....................................................................................................................60
Experimental Design .............................................................................................60 Limitations of the Study ........................................................................................61 Clinical Application ..............................................................................................62 Future Projects .......................................................................................................63
SUMMARY AND CONCLUSIONS ................................................................................64
REFERENCES ..................................................................................................................65
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LIST OF TABLES
Table
1. Descriptive statistics of measurement differences for intra- and inter-examiner for tooth #6................................................................................................................24
2. Descriptive statistics of measurement differences for intra- and inter-examiner for tooth #7................................................................................................................25
3. Descriptive statistics of measurement differences for intra- and inter-examiner for tooth #8................................................................................................................26
4. Descriptive statistics of measurement differences for intra- and inter-examiner for tooth #9................................................................................................................26
5. Descriptive statistics of measurement differences for intra- and inter-examiner for tooth #10..............................................................................................................27
6. Descriptive statistics of measurement differences for intra- and inter-examiner for tooth #11..............................................................................................................27
7. Descriptive statistics of measurement differences for intra- and inter-examiner for antimere teeth #6 and #11 ...................................................................................28
8. Descriptive statistics of measurement differences for intra- and inter-examiner for antimere teeth #7 and #10 ...................................................................................28
9. Descriptive statistics of measurement differences for intra- and inter-examiner for antimere teeth #8 and #9 .....................................................................................29
10. Descriptive statistics of measurement differences for intra- and inter-examiner for all teeth ................................................................................................................29
11. Descriptive statistics of lesion area for tooth #6, control group. .............................33
12. Descriptive statistics of lesion area for tooth #7, control group ...............................33
13. Descriptive statistics of lesion area for tooth #8, control group ...............................33
14. Descriptive statistics of lesion area for tooth #9, control group ...............................34
15. Descriptive statistics of lesion area for tooth #10, control group .............................34
16. Descriptive statistics of lesion area for tooth #11, control group .............................34
17. Descriptive statistics of lesion area for tooth #6, treatment group ...........................35
18. Descriptive statistics of lesion area for tooth #7, treatment group ...........................35
19. Descriptive statistics of lesion area for tooth #8, treatment group ...........................35
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20. Descriptive statistics of lesion area for tooth #9, treatment group ...........................36
21. Descriptive statistics of lesion area for tooth #10, treatment group .........................36
22. Descriptive statistics of lesion area for tooth #11, treatment group .........................36
23. Descriptive statistics of lesion area for antimere teeth #6 and #11, control group ...37
24. Descriptive statistics of lesion area for antimere teeth #6 and #11,
treatment group .........................................................................................................37
25. Descriptive statistics of lesion area for antimere teeth #7 and #10, control group ...37
26. Descriptive statistics of lesion area for antimere teeth #7 and #10,
treatment group .........................................................................................................38
27. Descriptive statistics of lesion area for antimere teeth #8 and #9, control group .....38
28. Descriptive statistics of lesion area for antimere teeth #8 and #9,
treatment group .........................................................................................................38
29. Descriptive statistics of lesion area for all teeth, control group ................................39
30. Descriptive statistics of lesion area for all teeth, treatment group ............................39
31. Descriptive statistics of F values for tooth #6, control group.................................41
32. Descriptive statistics of F values for tooth #7, control group.................................41
33. Descriptive statistics of F values for tooth #8, control group.................................42
34. Descriptive statistics of F values for tooth #9, control group.................................42
35. Descriptive statistics of F values for tooth #10, control group ..............................42
36. Descriptive statistics of F values for tooth #11, control group ..............................43
37. Descriptive statistics of F values for tooth #6, treatment group .............................43
38. Descriptive statistics of F values for tooth #7, treatment group .............................43
39. Descriptive statistics of F values for tooth #8, treatment group .............................44
40. Descriptive statistics of F values for tooth #9, treatment group .............................44
41. Descriptive statistics of F values for tooth #10, treatment group ...........................44
42. Descriptive statistics of F values for tooth #11, treatment group ...........................45
43. Descriptive statistics of F values for antimere teeth #6 and #11, control group ....45
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44. Descriptive statistics of F values for antimere teeth #6 and #11, treatment group .........................................................................................................45
45. Descriptive statistics of F values for antimere teeth #7 and #10, control group ....46
46. Descriptive statistics of F values for antimere teeth #7 and #10, treatment group .........................................................................................................46
47. Descriptive statistics of F values for antimere teeth #8 and #9, control group ......46
48. Descriptive statistics of F values for antimere teeth #8 and #9, treatment group .........................................................................................................47
49. Descriptive statistics of F values for all teeth, control group .................................47
50. Descriptive statistics of F values for all teeth , treatment group ............................47
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LIST OF FIGURES
Figure
1. Example of white spot lesions (WSL) developed during orthodontic treatment ........2 2. Diagram illustrating the process of demineralization and remineralization ...............5
3. Horizontal and vertical measurements used to calculate the area of the WSL .........22
4. Photographic images illustrating remineralization in the treatment group, T0 and T4 respectively ..................................................................................................49
5. Photographic images illustrating remineralization in the control group, T0 and T4 respectively ..................................................................................................51
6. QLF images illustrating remineralization in treatment group (above) and control group (below), T0 and T4 respectively .....................................................................52 7. QLF images illustrating no significant remineralization in treatment group (above) and control group (below), T0 and T4 respectively ....................................53 8. Treatment group QLF (above) and photographic (below) images, T0 and T4 respectively ..........................................................................................................54
9. Control group QLF (above) and photographic (below) images, T0 and T4 respectively ..........................................................................................................57
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INTRODUCTION
Orthodontic treatment does more than just straighten teeth, it gives a person their unique smile and provides them with a positive sense of self-esteem. However, this smile
can be compromised by the development of demineralization around the brackets, bands,
and wires during orthodontic treatment. Upon removal of appliances at the termination
of treatment, the patient may exhibit straight, yet blemished teeth. These white, chalky
areas of demineralization are evidence of a loss of calcified tooth structure and are termed
white spot lesions (Figure 1). And if left untreated, further decalcification may cause these early lesions to develop into cavitations that will require tooth reduction or
permanent restoration (Mitchell, 1992). Even with advances in materials and techniques over the years, enamel
demineralization associated with fixed orthodontic appliances has been observed and
continues to be a problem (Farhadian et al., 2008). Historically, topical fluoride application has been the most common method to prevent development of white spot
lesions around orthodontic appliances. A study reported by Stratemann and Shannon
(1974) used a stannous fluoride gel. Only 2% of the subjects using the fluoride gel exhibited decalcification compared with the 58% of the control group. Another study
using a neutral sodium fluoride rinse reported a 25% reduction in the incidence of white
spot lesions (Geiger et al., 1992). More recently, Farhadian et al. (2008) observed a 40% decrease in the depth of demineralization among teeth treated with fluoride varnish
compared to untreated controls. Though the results of these studies are promising, it
takes a compliant patient to achieve such results and compliance with these patients is
difficult to attain. Unfortunately, patients with poor oral hygiene that could benefit the
most from fluoride preventive measures are also the same patients that are least likely to
comply with the required topical fluoride protocol.
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Recently, Recaldent, which is a complex of casein phosphopeptides and
amorphous calcium phosphate (CPP-ACP), has been proclaimed to prevent and even reverse white spot lesions. Casein phosphopeptides (CPP), which are products of milk protein casein, are thought to have the ability to increase the level of calcium phosphate
in dental plaque which would depress the demineralization process and raise the
remineralization process (Reynolds, 1998). Recaldent is the active ingredient in MI Paste and MI Paste Plus, which are preventive treatment products marketed by GC
America (Alsip, IL, USA) to provide a wide variety of benefits. The products are advertised to help prevent dry mouth, reduce tooth sensitivity, help fight acid imbalance,
prevent demineralization, and enhance remineralization. The FDA has approved the use
of MI PasteTM and MI Paste PlusTM as a prophy paste and for treating hypersensitivity.
Figure 1. Example of white spot lesions (WSL) developed during orthodontic treatment.
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Purpose of this Study
The purpose of this study is to evaluate the effectiveness of MI Paste Plus in
increasing remineralization and improving the esthetic appearance of white spot lesions
in patients who have been treated with fixed orthodontic appliances. Each patient must
meet specific criteria in order to be included in the study. Those patients who are eligible
and choose to participate in the study will undergo four in-office MI Paste PlusTM
treatments as well as three months of at-home MI Paste PlusTM applications. Initial,
progress and final photographs will be made, the area of the white spot lesions will be
measured and size comparisons will be conducted. Quantitative light-induced fluorescence (QLF) will also be used to quantitatively monitor the remineralization effects of MI Paste PlusTM after orthodontic treatment and three months post-treatment.
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LITERATURE REVIEW
Development of a White Spot Lesion
Dental caries, one of the most prevalent chronic diseases in adults and children
worldwide (Featherstone, 2000), affects nearly 90% of youth and 95% of adults within the United States (Garca-Godoy et al., 2008). Dental caries is a preventable, multi-factorial disease that involves bacteria (dental plaque), susceptible teeth (the host), and carbohydrates (the diet) (Keyes et al., 1963). These factors play a role in the dynamic demineralization-remineralization process that occurs at the surface of each tooth in the
oral environment.
As teeth erupt into the oral cavity, they are immediately covered by an acquired
enamel pellicle that consists of an acellular base layer of protective proteins. This
pellicle, which is continually present and immediately reforms after disruption from tooth
brushing or professional prophylactic cleaning, serves as the base on which dental plaque
builds (Garca-Godoy et al., 2008). Bacteria bind to the enamel pellicle and as dental plaque matures, additional bacteria adhere. Over 600 different bacteria colonize dental
plaque, with aerobic, facultative anaerobic and anaerobic organisms coexisting (Marsh, 2006). Acidogenic bacteria within dental plaque produce acid when fermentable carbohydrates are metabolized. Once this acid decreases the pH surrounding the teeth
past a critical level (pH = 5.5) it has the potential to diffuse into enamel and dissolve calcium phosphate mineral (Featherstone, 2000). During this demineralization process, less-soluble phases of dicalcium phosphate dihydrate (CaHPO42H2O) and fluoridated hydroxyapatite (Ca5(PO4)3(OH)xF(1-x)) precipitate out of the enamel surface and into the saliva. This process continues until equilibrium is reached between the enamel and the
oral environment. Demineralization can continue as long as the oral pH remains acidic
(Margolis et al., 1990).
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Once the oral pH rises above the acidic level and normalizes, the remineralization
process of the tooth surface can start. Calcium and phosphate are both minerals in saliva
and, with the help of fluoride, diffuse into the enamel and remineralize crystalline
structures in demineralized areas. Fluoridated hydroxyapatite and fluorapatite are the
constituents of the structures that are rebuilt and are much more resistant to acid attack
than the original structure (Selwitz et al., 2007). The processes of demineralization and remineralization occur several times throughout the day and if balanced, will not result in
carious lesions. If however, the multi-factorial disease is not kept in balance and the oral
environment becomes acidic, demineralization rather than remineralization occurs and
the lesion will progress and eventually become a frank cavitation (Featherstone, 2000). A diagrammatic representation of the demineralization and remineralization cycle is
shown in Figure 2.
Figure 2. Diagram illustrating the process of demineralization and remineralization.
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The primary clinical presentation of dental caries in enamel is a white spot lesion.
It is an area of demineralized enamel that usually develops because of prolonged plaque
accumulation (Guzman-Armstrong, 2010). The white spot lesions opaque appearance is a result of the loss of subsurface enamel, which results in the loss of enamel translucency
(Zero, 1999). Over time when plaque accumulates and aciduric bacteria colonize, active white spot lesions are produced. If left untreated, a cavitated carious lesion can develop.
The patients modifying factors can also impact the development of white spot lesions,
this includes medical, dental, and medication history; diet; levels of calcium, phosphate,
and bicarbonate in saliva; fluoride levels; and genetic susceptibility (Chalmers, 2006; Mount, 2005). A continuous process of enamel demineralization and remineralization occurs that can progress from initial demineralization, to noncavitated lesions, and finally
to cavitated lesions (Fejerskov, 2003).
White Spot Lesions in Orthodontic Patients
It is agreed upon that demineralization and the development of white spot lesions
is a problem during orthodontic treatment; however, published literature shows great
variation in the prevalence. Zachrisson et al. (1971) reported that 89% of patients developed white spot lesions, while Gorelick et al. (1982) observed that 49.6% of patients had white spot formation on at least one tooth at debanding. However, Sudjalim et al. (2006) reported overall prevalence of white spot lesions ranging widely between 2 and 96%. The differences in reported prevalence may be attributed to variation in incidence
geographically or to the difference in the definition of a white spot lesion. However
prevalent, it is established that white spot lesions may persist for years resulting in a
permanent, unaesthetic result with the potential of worsening to the point of requiring
permanent restoration (gaard, 1989; Sudjalim et al., 2006). Fixed orthodontic appliances create areas for plaque accumulation and make tooth
cleaning difficult. The irregular surfaces of brackets, bands, and wires limit the naturally
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occurring self-cleansing mechanisms of the oral musculature and saliva (Guzman-Armstrong, 2010), leading to increased plaque retention and subsequent white spot lesion formation. Due to the difficulty of effective daily cleaning around fixed appliances,
patients without fluoride supplementation (Ogaard et al., 1988), those with poor oral hygiene (Zachrisson et al,. 1971), and those patients with a high Streptococcus mutans count (Ogaard, 1989) are at higher risk for enamel demineralization and white spot lesion formation.
The degree of white spot lesion development is not completely apparent until the
fixed orthodontic appliances are removed. Upon removal of appliances, white, opaque
demarcations on the labial surface of the teeth where the brackets and bands once were
may be evident. These white, unesthetic demarcations of decalcification detract from the
smile and final esthetic result of straight teeth and good occlusion. Because these white
spot lesions most often occur on maxillary anterior teeth, they pose a significant esthetic
problem (Gorelick et al., 1982).
Methods to Decrease Demineralization During Orthodontic Treatment
Depending on the patients risk factors, a number of suitable agents and therapies
can be used to help prevent white spot lesions in orthodontic patients: fluoride
toothpastes, gels, varnishes, and mouth rinses; antimicrobials; xylitol gum; diet
counseling; and casein derivatives (Guzman-Armstrong, 2010). The critical component in preventing demineralization is patient compliance
along with good oral hygiene. Reinforcing oral hygiene habits throughout orthodontic
treatment has been shown to be effective in reducing demineralization (Artun et al., 1986). Exhaustive tooth brushing, daily flossing, and routine prophylactic cleanings will minimize the amount of dental plaque, thereby decreasing the probability of developing
areas of decalcification (gaard, 1989).
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Decreasing the amount of Streptococcus mutans has also been shown to limit the
caries process (van Houte, 1994). Chlorhexidine is an antimicrobial agent that is effective at reducing levels of Streptococcus mutans (Ribeiro, 2007). Therefore, a before bedtime protocol utilizing a chlorhexidine rinse, gel, or varnish may assist in preventing
demineralization. A drawback of the chlorhexidine products is their tendency to stain the
teeth.
Xylitol gum has been shown to be effective as a caries preventive agent. Xylitol
is a polyol (a type of carbohydrate) that is not a metabolizable substrate for Streptococcus mutans and can be used as a low-calorie sugar substitute. It is noncariogenic and
appears to have antimicrobial properties that help to inhibit the attachment of
Streptococcus mutans to the teeth, decreasing the bacterial count. Makinen et al (1995) showed that the systematic use of xylitol chewing gum can significantly reduce the risk
of caries. The consumption of chewing gum has also increased production of stimulated
saliva containing more calcium and phosphate ionic concentrations when compared to
non-stimulated saliva.
Increasing the levels of topical fluoride in the oral cavity is fundamental in
minimizing the risk of decalcification. Fluoride can be introduced via dentifrice, mouth
rinses, foams, gels, varnishes, bonding agents, cements, and even elastomers. Several of
these delivery systems are intended for home use, relying on patient cooperation. Patient
compliance with these products is essential for these products to have a significant
preventive effect. For instance, Geiger et al. (1992) reported that only 42% of patients rinsed with sodium fluoride mouth rinse at least every other day, but patients who were
more compliant had fewer white spot lesions. It is difficult to have a high percentage of
patients willing and able to follow hygiene instruction for an extended period of time.
Due to the unpredictability of patient cooperation, fluoride products that do not
rely on patient compliance have gained popularity. Brackets and bands can be cemented
with fluoride-releasing materials, sealants can be placed to cover the facial surface of
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each tooth, and a fluoride varnish containing high amounts of fluoride can be applied at
office visits at least twice per year (Schmit et al., 2002; Todd et al., 1999; Ashcraft et al., 1997; Vorhies et al., 1998).
Mechanism of Action of Fluoride
Fluoride has the ability to aid in the prevention of dental caries. Topical fluoride
has three principal mechanisms of action: 1) inhibiting bacterial metabolism, 2) inhibiting demineralization, and 3) enhancing remineralization (Featherstone, 2000). To inhibit bacterial metabolism, acidulated fluoride ions in the form HF are able to cross the cell
wall and membrane of cariogenic bacteria, such as Streptococcus mutans (Whitford et al., 1977; Van Loveren et al., 1990). Once inside the cell, HF dissociates, acidifying the cell and inhibiting enzyme activity with the fluoride ion F-. Enolase, an enzyme involved in
carbohydrate metabolism, is affected by such inhibitory activity. This activity limits the
cariogenic potential of the cell (Featherstone, 2000). Fluoride also has the ability to protect the enamel surface from demineralization
during an acid attack. If topical fluoride is present in the plaque fluid when the pH drops
below the critical level (pH = 5.5), it will travel with the acid into the subsurface layer, absorb to the crystal surface of carbonated hydroxyapatite (CAP) and protect it from being dissolved (Featherstone, 2000). Thus, low levels of fluoride surrounding the enamel during an acid attack are able to inhibit demineralization.
The third mechanism of action of fluoride is enhancing the remineralization
process. Following the acid attack and the pH rising above 5.5, available calcium and
phosphate are able to be attracted into the crystal structure by the presence of absorbed
fluoride. Calcium and phosphate ions enhance and are required for this remineralization
process. These three minerals are able to create a new crystalline structure between
hydroxyapatite (HAP) and fluorapatite (FAP), which is stronger and more acid-resistant
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than the previous structure (Featherstone, 2000; Moreno et al., 1977; ten Cate et al., 1991).
Fluoride Dentifrice
Fluoridated dentifrice is the most common method of topical fluoride delivery
worldwide and is recognized as a major factor in reducing the prevalence of caries in many developed countries (Zero, 2006). In a meta-analysis of seventy studies by Marinho et al. (2003) and in a systematic review of fifty-four published studies by Twetman et al. (2003), it was concluded that there was clear evidence that fluoridated toothpastes are effective in preventing dental caries.
Fluoride concentrations in dentifrice range from low (below 600 ppm) to high (5000 ppm), with the majority between 1000-1100 ppm. The low and high concentrations of fluoride are intended for patients under the age of six and those with
high caries risk, respectively (Ammari, 2003). Twetman et al. (2003) reported a superior preventive effect with toothpastes containing 1,500 ppm fluoride compared with those
containing 1,000 ppm fluoride. Sources of fluoride in dentifrice include stannous
fluoride (SnF2), monofluorophosphate (MFP), and sodium fluoride (NaF). Of these, the majority of dentifrice marketed in the United States is in the form of NaF or MFP (Zero, 2006). High-fluoridated dentifrice, such as PreviDent 5000 Plus (Colgate-Palmolive Co., New York City, NY, USA), have few studies demonstrating efficacy over traditional 1,100 ppm fluoride dentifrice. Baysan et al. (2001) compared the ability of two fluoridated dentifrices, one containing 5,000 ppm (PreviDent 5000 Plus) and the other 1,100 ppm (Winterfresh Gel), to reverse primary root caries lesions. They concluded that the 5,000 ppm fluoride dentifrice was significantly better at preventing the lesions
than the 1,100 ppm fluoride dentifrice.
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Mechanism of Action of Casein Phosphopeptides
Dairy products such as milk, milk concentrates, powders, and cheeses have been
demonstrated to have anticariogenic properties (Reynolds et al., 1981; Rosen et al., 1984; Harper et al., 1986, 1987; Krobicka et al., 1987; Silva et al., 1987). Using in vitro, animal, and in situ caries models, the components responsible for this significant attribute
have been identified as casein, calcium, and phosphate (Schweigert et al., 1946, Shaw, 1950; Bavetta et al., 1957; Holloway et al., 1961, Reynolds et al., 1984, 1987, 1989;
Reynolds, 1987). A soluble form of casein, or caseinate, was shown to have anticariogenic potential in rats; however, due to the high amount required for effective
caries control this form of casein was not ideal for commercial use (Reynolds et al., 1984).
Researchers later discovered that digesting caseinate with trypsin did not destroy
the proteins ability to prevent subsurface enamel demineralization (Reynolds, 1989). The resultant tryptic peptides were shown to be incorporated within dental plaque along
with elevated concentrations of calcium and phosphate (Reynolds, 1998). The major tryptic peptides associated with the anticariogenic nature of casein are casein
phosphopeptides (CPP). Through multiple phosphoseryl residues, CPP has the unique ability to stabilize calcium phosphate in a CPP-amorphous calcium phosphate (ACP) complex (Azarpazhooh et al., 2008).
Casein Phosphopeptide-Amorphous Calcium Phosphate (CPP-ACP)
The CPP-ACP complex was patented by the University of Melbourne, Australia,
and the Victorian Dairy Industry Authority, Abbotsford, Australia. Bonlac Foods
Limited (an Australian company owned by 2,300 dairy farmers in Victoria and Tasmania) has retained exclusive manufacturing and marketing rights for CPP-ACP and is the owner of the trademark Recaldent (Azarpazhooh et al., 2008). CPP-ACP
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complexes have been shown to exhibit anticariogenic activity in laboratory, animal, and
human in situ caries models (Morgan et al., 2008; Oshiro et al., 2007; Ramlingam et al., 2005; Reynolds et al., 1987, 1991, 1995, 1997, 1998, 1999, 2003; Shen et al., 2001). The anticariogenic mechanism of CPP-ACP is the localization of amorphous calcium
phosphate at the tooth surface, where it buffers free calcium and phosphate ion activity
during an acid challenge, and maintaining a state of supersaturation of calcium and
phosphate ions on the enamel surface (ElSayad, 2009). This process results in a decrease in demineralization during a cariogenic challenge and an increase in the subsequent
remineralization of the enamel (Azarpazhooh et al., 2008; Reynolds, 1987, 1991, Pulido et al., 2008). One of the benefits of this peptide compound is that it has been shown to incorporate well into the salivary pellicle thereby reducing the adherence of cariogenic
bacteria, specifically S. sobrinus and S. mutans (Schupbach, 1996). In addition to reducing the amount of acid-producing bacteria within dental plaque, the incorporation of
CPP-ACP within dental plaque is able to provide a reservoir of additional bio-available
calcium and phosphate ions. These ions help buffer acidic challenges to the enamel and
aid in rebuilding enamel structure (Aimutis, 2004). It has been shown that enamel remineralized by CPP-ACP is relatively more acid-resistant than normal tooth enamel
(Yengopal, 2009). The most commonly tested (and used) mode of CPP-ACP application in the human oral environment is via sugar-free sorbitol or xylitol-based chewing gum.
Other vehicles include milk, mouth rinses, lozenges, and dental cream/ MI Paste/Tooth
Mousse (Yengopal, 2009). Morgan et al. (2008) compared the progression and regression of interproximal caries in adolescent subjects chewing a sugar-free gum containing 54 mg CPP-ACP to subjects chewing identical gum without CPP-ACP. The investigators reported a significantly slowed progression and enhanced regression of the lesions relative to the
control group over a 24 month period. Similarily, Cai et al. (2007) showed that gum containing 18.8 mg and 56.4 mg of the CPP-ACP nanocomplexes, chewed for 20 minutes
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four times per day for 14 days, increased enamel subsurface remineralization by 102%
and 152%, respectively, relative to the control sugar-free gum.
In a randomized, controlled trial Reynolds et al. (2003) observed an increase in plaque calcium and inorganic phosphate levels of 118% and 57%, respectively, using a
2% CPP-ACP mouth rinse. The increase of calcium and phosphate ions within dental
plaque was consistent with the proposed anticariogenic mechanism of CPP-ACP by
maintaining the supersaturated state of remineralizing ions on the enamel surface. The
investigators also reported that mouth rinses containing ACP without CPP did not exhibit
increased calcium and inorganic phosphate levels. This is significant in that it
demonstrates that CPP is essential in stabilizing and delivering ACP to the tooth surface
(Reynolds et al., 2003). Currently, CPP-ACP (Recaldent) is commercially available in the United States
in the form of sugar-free gum, Trident White (Cadbury North America, Parsippany, NJ), MI Paste, and MI Paste Plus (containing 900 ppm fluoride) (GC America, Alsip, IL, USA). The FDA has approved MI Paste for use primarily as an abrasive prophylactic paste, secondarily as treatment for dentin hypersensitivity, and thirdly for
dry mouth. However, its use as a caries preventive and remineralization agent is
considered off-label. Outside the United States, MI Paste and MI Paste Plus is
marketed as GC Tooth Mousse and Tooth Mousse Plus (GC Europe N.V., Leuven, Belgium) (Azarpazhooh et al., 2008).
While several articles have been published on the evidence of CPP-ACP as an
anti-caries agent in its pure form, quality studies involving commercially-available MI
Paste and MI Paste Plus (or Tooth MousseTM and Tooth Mousse PlusTM ) are limited. The majority of reviews are found in abstracts presented at International Association for Dental Research (IADR) conferences and funded by GC Corporation (Paterson, 2008; Sakaguchi, 2005, 2006; Sato, 2003). Although CPP-ACP is the main active ingredient in these products (5-10% w/v) it is uncertain whether incorporation into the form of a paste
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alters its effective ability. An IADR abstract presented by Sato et al., (2003) confirmed the ability of Tooth Mousse to prevent the formation of caries in a bovine tooth model.
Using Knoop Hardness measurements to evaluate treatment groups, those treated with
Tooth Mousse displayed a significantly less change in hardness reduction compared to
a placebo paste and to a fluoridated paste. In addition, Sakaguchi et al., (2005) reported the ability of MI Paste to prevent acid-inducted demineralization in bovine tooth
enamel compared with a placebo paste, a 900 ppm fluoride paste, and water. Samples
were imaged using quantitative light-induced fluorescence (QLF) as well as x-ray CT. Researchers concluded that there was a significant protective effect of MI Paste in
preventing the demineralization of enamel. Sakaguchi et al., (2006) later described a synergistic effect of CPP-ACP and fluoride, as found in Tooth Mousse Plus (MI Paste Plus), in remineralizing subsurface enamel lesions in bovine teeth. Tooth Mousse Plus was compared with Tooth Mousse, a placebo containing no CPP-ACP or
fluoride, and a paste containing 950 ppm fluoride. The remineralization potential of
Tooth Mousse Plus (Tooth Mousse with 900 ppm fluoride) was greater than the additive effect of the Tooth Mousse and the 950 ppm fluoridated paste groups. It is
important to note that GC Corporation appears on each of the author reference lists.
Studies not associated with GC Corporation prove to be a bit more contradictory.
For instance, a study attempting to remineralize subsurface enamel lesions on extracted
human teeth using MI Paste, MI Paste with Crest toothpaste, Crest toothpaste
alone, and PreviDent 5000 Plus reported no significant difference between groups
except for the PreviDent 5000 Plus treatment group (Eberle, 2006). In addition, a recent study examining the ability of MI Paste in preventing the progression of
artificial carious lesions in human enamel revealed no significant effect of the product
(Pulido et al., 2008). The authors reported that no significant difference between MI Paste, 1100 ppm NaF, or a combined application of both products was detected from
the study. On the other hand, Guilio et al. (2009) reported greater demineralization
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15
resistance in teeth coated with Tooth Mousse than a control group after enamel
stripping. In a clinical trial conducted by Bailey et al. (2009), 92% of white spot lesions had regressed or stabilized after using a remineralizing cream (Tooth Mousse TM) containing 10% w/v CPP-ACP. Over 12 weeks, there were significantly (31%) more post-orthodontic white spot lesions regressed with the remineralizing cream compared
with an identical cream not containing CPP-ACP. CPP-ACP promotes remineralzation of
enamel subsurface lesion, restoring the white opaque appearance of the lesions to
translucency, even in the presence of fluoride (Reynolds et al., 2003, 2008). A dentifrice formulation containing 2% CPP-ACP nanocomplexes plus 1100 ppm
F (CPP-ACPF) has been shown to be superior (2.6 times) to a dentifrice containing only 1100 ppm F in remineralization of enamel subsurface lesions in situ with mineral that
was more resistant to acid challenge (Reynolds et al., 2008). The CPP-ACP nanocomplexes-plus-fluoride dentifrices resulted in significantly greater incorporation of
fluoride into the subsurface enamel as fluorapatite. These results indicate that the CPP is
an excellent delivery vehicle to co-localize bioavailable calcium, fluoride, and phosphate
ions at the tooth surface to remineralize subsurface enamel lesions with fluorapitite
(Reynolds, 2009).
Quantitative Light-induced Fluorescence (QLF) The quantitative light-induced fluorescence (QLF) method for quantitative
assessment of early enamel lesions provides a fluorescence image of a smooth surface
carious lesion that quantifies the mineral loss and size of the lesion. Accordingly, the
method is suitable for quantitative assessment of early enamel lesions in visually
accessible surfaces. It may be used for quantitative monitoring of mineral changes
(regression or progression) over just a few months (Angmar-Mansson, 2001). QLF is based on fluorescent light which is induced by visible or near-ultraviolet radiation. There is an uncertainty regarding the cause of the decreased fluorescence of
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16
incipient lesions. The generally accepted explanation is that the light scattering in the
lesion, which is much stronger than in sound enamel, causes the light path in the lesion to
be much shorter than in sound enamel, thus the light absorption per volume is much
smaller in the lesion and thus the fluorescence is less strong. A second explanation is that
the light scattering in the lesion is a barrier for excitation light to reach the underlying
fluorescing dentin, and a barrier for fluorescence light from dentin to reach the surface
(Angmar-Mansson, 2001). QLF is non-destructive and thus a suitable method for quantitative assessment of one and the same lesion at different times. This involves making a series of images at
different times. Most often, the first image in the series is made of the sound tooth which
serves as the baseline for all later images. A comparison of images yields values of the
fluorescence decrease as a function of position (x,y) on the tooth surface at the location of the lesion, expressed as a percentage of the fluorescence in the sound situation (Angmar-Mansson, 2001).
The accuracy of any measurement technique is affected by the equipment used
and the skill of the operator. Ideally, the equipment should be able to compensate for any
deficiencies in the operator. With the QLF equipment, the operator adjusts the camera to view the region of interest on a monitor screen and the light guide is attached to the
camera requiring no separate adjustment. The camera amplifier is automatically adjusted and an image can be grabbed and stored by pressing a foot pedal.
There is on-screen guidance for the operator to perform image analysis.
Reference points that are seen on subsequent images, such as a cusp tip or gingival
margin, are used and assist for correction due to irradiation geometry changes. After
these adjustments, the program is able to analyze both images and calculate the ^F (fluorescence loss) for each image (Angmar-Mansson). The ^F % is used to calculate the change between the images.
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17
The repeatability and reproducibility of QLF have been tested in vivo. The image-capturing stages were tested by three operators, each captured images of 15
incipient smooth surface lesions in vivo. The analytical stage of the method was also
tested. The same three operators analysed the images of 15 in vivo incipient smooth
surface lesions. For the image-capturing stage, interexaminer reliability showed an
interclass correlation coefficient, r, between 0.95 and 0.99. For the analytical stage,
intra-examiner reliability for all three analysts showed an intraclass correlation
coefficient, r, between 0.93 and 0.99. Interexaminer reliability showed an interclass
correlation coefficient, r, between 0.95 and 0.99. It was concluded that the in vivo
repeatability and reproducibility of the QLF method is excellent (Angmar-Mansson). An in vivo application of the QLF method of measurement of mineral changes in natural enamel lesions on smooth surfaces was demonstrated in a 12-month study
monitoring remineralization of carious lesions, which had developed around orthodontic
brackets during fixed appliance therapy. Removal of the orthodontic brackets and bands
had disclosed active carious lesions, and caries preventive measures were intensified.
The carious lesions were monitored with the QLF method immediately after removal of the orthodontic brackets and once a month thereafter. During a 1-year follow-up period,
the areas of the lesions decreased, and the lost enamel fluorescence was partly regained,
indicating remineralization. It was concluded that QLF is appropriate for in vivo monitoring of mineral changes in incipient enamel lesions and is useful for the evaluation
of preventive measures in caries-susceptible individuals, such as orthodontic patients
(Mattousch, 2007).
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18
MATERIALS AND METHODS
The study protocol was reviewed and approved by the Institutional Review Board
at the University of Iowa.
Sample
A total of twelve subject participants aged twelve to twenty years were selected in this pilot study. All participants were recruited from patients treated with fixed edgewise
orthodontic appliances in the Department of Orthodontics at the University of Iowa,
College of Dentistry. The sample was comprised of 6 control and 6 treatment subjects. All 12 subjects were Caucasian, 7 were female and 5 were male.
Patient Inclusion Criteria
The patients must have been age 12 years or older, been in good general health
with no proven or suspected milk protein allergy and/or with a sensitivity or allergy to
benzoate preservatives, had a treatment period with fixed appliances of at least 1 year at
the debonding appointment, had at least 1 clinically visible white spot lesion on the facial
surface of a maxillary anterior tooth, had not undergone any type of
remineralization/demineralization regimen, and have not had more than 2 failed
appointments during orthodontic treatment. The patient could not have been a consent
debond, and must have had an informed consent signed by the participant and for those
under 18 years, signed in addition by their parents or guardians.
Clinical Procedure
The purpose of the clinical study was to evaluate the effectiveness of CPP-ACPF,
MI Paste Plus (GC America, Alsip, Illinois, USA) to remineralize and improve the esthetic appearance of white spot lesions (WSL) after orthodontic treatment.
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19
Twelve patients were selected based on the inclusion criteria and were randomly
assigned to the treatment and control groups (n=6 per group). The first six patients who met the study criteria were selected for the treatment group. The following six patients
who again met the study criteria were selected to be the control subjects. One to two weeks after fixed orthodontic appliances were removed (T0), both the treatment and control subjects returned for photographs. These photographs consisted of five intra-oral photos of the six maxillary anterior teeth made at a higher magnification
than standard photographs. A standard intra-oral photographic camera was utilized and
the photos were taken in a light controlled environment with pre-set photographic
protocol. The first photo was centered on the maxillary central incisors, the second and
third on the right and left lateral incisors, and the remaining two on the right and left
canines. The treatment and control subjects also had initial QLF images made at this appointment.
Initial QLF images were made of the facial surface of all six maxillary anterior teeth. The images were examined visually for signs of demineralization, which appears
as dark areas surrounded by bright green fluorescing tooth structure. Once the
photographs and QLF images were made, the treatment subjects only started their first round of the in-office MI Paste PlusTM application.
Appropriate isolation was achieved with cheek retractors. A 35% phosphoric acid
etch was applied to only the white spot lesions for 1 minute. The etch was rinsed off
thoroughly after 1 minute. A small amount of MI Paste PlusTM was applied directly onto
the WSL with an application swab. The MI Paste PlusTM was left undisturbed for 5
minutes. After the 5 minutes had expired, the patient was instructed to use their tongue to
spread the remaining paste throughout the mouth. The patient was requested to avoid
expectoration for an additional 1-2 minutes. The patient was then advised not to eat or
drink for 30 minutes following application. They were instructed to return in three weeks
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20
for their second in-office application. At-home application instruction and oral hygiene
guidance were given to the patient at the end of the appointment.
Both the control group and treatment group were given a 6.4 oz tube of cavity
protection toothpaste (Colgate or Crest depending on patient preference) to use during morning and evening brushing for the next three months. They were both given identical
oral hygiene instruction. The subjects were advised to brush with a soft toothbrush both morning and night with the toothpaste provided. They were encouraged to floss once
daily. They also received their invisible retainers along with full time wear instructions.
The treatment group retainers were made with a thin reservoir area around the WSL for
the MI Paste PlusTM to settle during the overnight application.
The treatment group was given additional instruction for their at-home application
of the MI Paste PlusTM (provided for patient). After brushing their teeth in the evening, each patient applied a pea-sized amount of the paste to the facial surface of the maxillary
six teeth with a clean dry finger. The patient immediately inserted their invisible retainer
which remained in place overnight and was not removed until the next morning. In the
morning when the tray was removed, the patient was allowed to expectorate, rinse and
complete their regular morning brush. The invisible retainer was rinsed, brushed and
reinserted for full time daily wear. Both groups were instructed to return to the office in
three weeks.
Upon return (T1), a set of progress photographs were made of both groups and the treatment subjects received their in-office application of the MI Paste PlusTM. The clinical trial ran for a total of 12 weeks (3 months). T0 (initial appointment) and four retention visits were scheduled; 3 weeks (T1), 6 weeks (T2), 9 weeks (T3), and 12 weeks/ 3 months or final appointment (T4). At each visit, the treatment subjects were given an at-home diary card. The card detailed at-home MI Paste PlusTM application instruction and oral hygiene guidance.
There was a column in the table where the patient was able to write in how many hours
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21
the retainer was worn overnight. A separate section was available for comments. On the
final 3 month in-office visit (T4), the treatment group did not have an MI Paste PlusTM application, but both groups had their final photographs and QLF images made. T4 photographs were made in the same manner as T0 photographs. T4 QLF images were captured using the softwares video-repositioning technique.
Measurement of Data
The remineralization effectiveness of MI Paste PlusTM was quantitively measured
in two ways, photographs (Area in mm2) and quantitative light-induced fluorescence (fluorescence loss in per cent). Five standard photographs were made at each three week interval, but only the initial and final photographs and QLF images were used for calculation. Each photograph was made with the same Nikon D1X/105mm/SB29
camera. The focal distance and magnification ratio were standardized at 1:2 and the
aperture maintained at an f equal to 40. The first photo was centered on the two central
incisors, the second and third on the left and right lateral incisors, and the fourth and fifth
on the left and right canines. Each photograph was downloaded into Dolphin Imaging 11
orthodontic imaging software. From the models made at the debond appointment, actual
mesial/distal measurements were made for each of the six maxillary anterior teeth with
Mitutoyo Absolute Digimatic calipers. These measurements were used to calibrate the
photographic image in order to be able to measure the white spot lesions accurately. Two
measurements were made, one horizontal (mesial/distal) and one vertical (incisal/gingival). The maximum lesion dimensions in both directions were measured in millimeters. The area of the lesion was calculated and compared. Figure 3 illustrates the
horizontal and vertical measurements which were made for each individual white spot
lesion on the calibrated photo in order to calculate the area.
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22
Figure 3. Horizontal and vertical measurements used to calculate the area of the WSL.
QLF images were captured at the initial appointment and at the final three month appointment using an intraoral fluorescence camera (InspektorTM Pro) on a personal computer using the image capturing software (QLF Patient version 2.0.0.30). The mineral change and size of the lesion was quantified. The fluorescence change between
initial and final appointment was compared. To ensure that the images of the tooth
surface are always captured with the same camera position and from the same angle, the
software uses video-repositioning techniques. The video-repositioning technique
displays the baseline and live image simultaneously and computes their correlation based
on similar geometry of the fluorescence intensities. Images are stored in a list when the
correlation is higher than 0.90 and the system automatically stops grabbing when the
correlation reaches 0.98. In this way, the images from the T0 and T4 should show the
tooth surface from the same angle and at the same magnification. The systems analysis
software determined the lesion extent. A patch was drawn surrounding the lesion site
with its borders on sound enamel. Inside the patch, the fluorescent levels of sound tissue
were reconstructed using the fluorescence radiance of the surrounding sound enamel.
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23
The T0 stored patch was overlayed around the T4 lesion. The percentage difference
between the reconstructed (T4) and original fluorescence levels was calculated. To ensure that the same area of a tooth surface was analyzed at each time point, the analysis
patch and surface contour were copied and then matched for size, orientation, and
location to this tooth surface in the final image.
Statistical Analysis
The two-sample t-test and nonparametric Wilcoxon rank-sum test were used to
detect the differences in lesion area and in F values between control and treatment
groups at baseline and at 3-month follow-up, as appropriate.
Within each group, the paired samples t-test and nonparametric Wilcoxon signed
rank test were used to assess the differences in change of lesion area and change in F
values from baseline to three-month follow-up under different situations.
The paired sample t-test was also used to assess the mean differences between
pairs of measurements for intra- and inter- examiner. Additionally, intraclass correlation
coefficients were computed as a measure of agreement between two measurements which
were taken either by a single evaluator or two evaluators on the same tooth for each
subject. The following is an approximate guide for interpreting an agreement between two measurements that corresponds to an intraclass and interclass correlation coefficient:
1) 1.0 = perfect agreement 2) 0.8 = strong agreement 3) 0.5 = moderate agreement 4) 0.2 = weak agreement 5) 0.0 = no agreement
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24
All tests employed a 0.05 level of statistical significance. SAS for Windows
(v9.2, SAS Institute Inc, Cary, NC, USA) was used for the data analysis.
Reliability of Intra- and Inter-Examiner Measurements of Lesion Areas
Each patients teeth were evaluated by two examiners. To eliminate the possible
bias, examiner A took two measurements on each tooth in two sessions with an interval
of 7 days, and examiner B only took one measurement. Therefore, 3 recordings were
obtained on each tooth for each subject. The intra- and inter-examiner measurement reliability was assessed for each
tooth, for antimere teeth, and for all teeth. The descriptive statistics of mean
measurement differences for intra- and inter-examiner are summarized in Tables 1-10.
Based on the paired samples t-test, intra-examiner duplicate measurements for
examiner A showed no significant differences, whereas inter-examiner differences (i.e. differences between measurements made by examiner A and examiner B) were also not statistically significant. This is true for teeth numbers 6, 7, 8, 9, and 10; antimere teeth #6
and #11, #7 and #10, #8 and #9; and for all teeth. For tooth #11, the data showed
significant difference (between 1st measurements of examiner A and measurements of examiner B (p=0.0312) (Table 6). Additionally, intra- and inter-class correlation coefficients were computed to
assess intra- and inter-observer agreement in measurements of lesion areas. All
correlation coefficients ranged from 0.80 to 0.99. These indicated a strong agreement
between two measurements with a single evaluator and with two evaluators, except for
one case, in which the corresponding values between measurements examined by A and
B (inter-examiner) were r = 0.62 and r = 0.60 for 1st and 2nd measurements of examiner A vs. examiner B, respectively. The correlation coefficients of 0.62 and 0.60 indicated a
moderate agreement between two measurements.
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25
Table 1: Descriptive statistics of measurement differences for intra- and inter-examiner for tooth #6.
Table 2: Descriptive statistics of measurement differences for intra- and inter-examiner for tooth #7.
Variable N Mean Std Dev Min Max
Median
P-value
Lesion 12 21 0.05 0.50 -0.78 1.36
0.00
0.6313
Lesion 13 21 0.88 3.02 -2.82 12.04
0.10
0.1946
Lesion 23 21 0.83 3.02 -2.48 12.04
-0.02
0.2220
Variable N Mean Std Dev Min Max
Median
P-value
Lesion 12
21
0.14
0.34
-0.41
1.18
0.08
0.0806
Lesion 13
21
-0.80
2.70
-11.38
1.32
-0.08
0.1880
Lesion 23
21
-0.94
2.89
-11.94
1.28
-0.14
0.1506
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26
Table 3: Descriptive statistics of measurement differences for intra- and inter-examiner for tooth #8.
Table 4: Descriptive statistics of measurement differences for intra- and inter-examiner for tooth #9.
Variable N Mean Std Dev Min Max
Median
P-value
Lesion 12
9
-0.05
0.26
-0.49
0.48
0.00
0.6109
Lesion 13
9
-0.31
0.53
-1.61
0.00
-0.08
0.1160
Lesion 23
9
-0.26
0.59
-1.61
0.37
-0.06
0.2124
Variable N Mean Std Dev Min Max
Median
P-value
Lesion 12
11
0.02
0.33
-0.82
0.48
0.06
0.8303
Lesion 13
11
-0.07
1.24
-2.25
1.80
0.03
0.8603
Lesion 23
11
-0.09
1.26
-2.21
2.08
-0.03
0.8190
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27
Table 5: Descriptive statistics of measurement differences for intra- and inter-examiner for tooth #10.
Table 6: Descriptive statistics of measurement differences for intra- and inter-examiner for tooth #11.
Variable N Mean Std Dev Min Max
Median
P-value
Lesion 12
19
-0.12
0.53
-1.60
0.50
0.00
0.3438
Lesion 13
19
-0.64
1.19
-2.96
1.12
-0.36
0.0312**
Lesion 23
19
-0.52
1.33
-3.09
2.72
-0.36
0.1033
** Significantly different (a paired-sample t-test).
Variable N Mean Std Dev Min Max
Median
P-value
Lesion 12
19
-0.11
0.88
-2.85
1.38
0.00
0.5948
Lesion 13
19
0.16
1.44
-2.36
3.12
0.18
0.6321
Lesion 23
19
0.27
1.34
-2.13
4.05
0.04
0.3932
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28
Table 7: Descriptive statistics of measurement differences for intra- and inter-examiner for antimere teeth #6 and #11.
Variable N Mean Std Dev Min Max
Median
P-value
Lesion 12
40
-0.03
0.52
-1.60
1.36
0.00
0.7329
Lesion 13
40
0.16
2.43
-2.96
12.04
-0.07
0.6803
Lesion 23
40
0.19
2.44
-3.09
12.04
-0.14
0.6293
Table 8: Descriptive statistics of measurement differences for intra- and inter-examiner for antimere teeth #7 and #10.
Variable N Mean Std Dev Min Max
Median
P-value
Lesion 12
40
0.02
0.66
-2.85
1.38
0.02
0.8426
Lesion 13
40
-0.35
2.22
-11.38
3.12
0.00
0.3311
Lesion 23
40
-0.37
2.34
-11.94
4.05
-0.07
0.3285
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29
Table 9: Descriptive statistics of measurement differences for intra- and inter-examiner for antimere teeth #8 and #9.
Variable N Mean Std Dev Min Max
Median
P-value
Lesion 12
20
-0.01
0.30
-0.82
0.48
0.00
0.8933
Lesion 13
20
-0.18
0.97
-2.25
1.80
-0.06
0.4237
Lesion 23
20
-0.17
0.99
-2.21
2.08
-0.04
0.4584
Table 10: Descriptive statistics of measurement differences for intra- and inter-examiner for all teeth.
Variable N Mean Std Dev Min Max
Median
P-value
Lesion 12
100
0.00
0.54
-2.85
1.38
0.00
0.9308
Lesion 13
100
-0.11
2.12
-11.38
12.04
-0.06
0.6065
Lesion 23
100
-0.11
2.18
-11.94
12.04
-0.07
0.6313
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30
Note: Lesion 1 = first measurements of Examiner A
Lesion 2 = second measurements of Examiner A
Lesion 3 = measurements of Examiner B
Lesion 12 = first measurements of Examiner A minus second measurements of
Examiner A
Lesion 13 = first measurements of Examiner A minus measurements of Examiner
B
Lesion 23 = second measurements of Examiner A minus measurements of
Examiner B
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31
RESULTS
The average lesion areas of two measurements of examiner A on the same tooth
for the same patient were used for the statistical analysis in this study. Tables 11-22
report descriptive statistics of lesion area by each tooth for each time period.
No significant differences between control and treatment groups were found at
baseline for teeth numbers 6, 7, 8, 9, 10, and 11; all antimere teeth; and for all teeth
(p>0.05 in each instance). Similarly, no significant difference in the lesion area were found between control
and treatment groups at 3-month follow-up for teeth numbers 6, 7, 8, 10, and 11; all
antimere teeth; and for all teeth (p>0.05 in each instance). Due to insufficient data, a statistical test was unable to be conducted for tooth #9.
To compare the change in lesion area from baseline to 3-month follow-up
between control and treatment group, a new variable called Lesion_area_change was
created, and this new variable is defined as lesion area at baseline minus lesion area at 3-
month follow-up. Based on the two-sample t-test, there were no significant differences
between control and treatment groups for the mean lesion area change from baseline to
follow-up for teeth numbers 6, 7, 8, 10, and 11; all antimere teeth; and for all teeth
(p>0.05 in each instance). Due to insufficient data, a statistical test was unable to be conducted for tooth #9.
Within the control group, the data showed there were no significant differences in
the lesion area measured between baseline and 3-month follow-up for teeth numbers 6, 7,
8, 10, and 11; antimere teeth #7 and #10, #8 and #9; and for all teeth (p>0.05 in each instance). Due to insufficient data, a statistical test was unable to be conducted for tooth #9. The data showed there was a significant difference in the lesion area measured
between baseline and 3-month follow-up for antimere teeth #6 and #11 (p=0.0235) in the
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32
control group. It revealed that the mean lesion measured at baseline was significantly
greater than that at follow up (Table 23). Within the treatment group, the data showed that there were no significant
differences in the lesion area measured between baseline and 3-month follow-up for teeth
numbers 7, 8, 9, 10, 11 and antimere teeth #7 and #10. The data also showed there was a
significant difference in the lesion area measured between baseline and 3-month follow
up for tooth #6 (p=0.0434). It revealed that the mean lesion measured for tooth #6 at baseline was significantly greater than that at follow up (Table 17). The data also showed there was a significant difference in the lesion area measured between baseline and 3-
month follow-up for antimere teeth #6 and #11 (p=0.0181) in treatment group. It revealed that the mean lesion measured at baseline was significantly greater than that at
follow up (Table 24). Based on the Wilcoxon signed-rank test, the data showed there was a significant difference in the lesion area measured between baseline and 3-month follow-
up for antimere teeth #8 and #9 (p=0.0331) in treatment group. It revealed that the mean lesion measured at baseline was significantly greater than that at follow up (Table 28). Additional analysis was conducted for combining all teeth. The results showed that there
was a significant difference in the lesion areas measured between baseline and follow-up
for all teeth (p=0.0219). It revealed that the mean lesion measured at baseline was significantly greater than that at follow-up for treatment group (Table 30).
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33
Table 11: Descriptive statistics of lesion area for tooth #6, control group.
Variable
N
Mean
Std Dev
Min
Max
Median
Lesion Area - Baseline
6
10.26
9.30
2.88
26.64
5.56
Lesion Area 3 Months
5
10.07
10.48
0.84
25.19
4.48
Table 12: Descriptive statistics of lesion area for tooth #7, control group.
Variable
N
Mean
Std Dev
Min
Max
Median
Lesion Area - Baseline
5
4.98
1.99
1.68
6.89
5.52
Lesion Area 3 Months
4
5.93
1.14
4.34
6.94
6.21
Table 13: Descriptive statistics of lesion area for tooth #8, control group.
Variable
N
Mean
Std Dev
Min
Max
Median
Lesion Area - Baseline
3
3.17
2.63
0.81
6.00
2.70
Lesion Area 3 Months
2
4.06
5.27
.034
7.79
4.06
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34
Table 14: Descriptive statistics of lesion area for tooth #9, control group.
Variable
N
Mean
Std Dev
Min
Max
Median
Lesion Area - Baseline
2
3.26
3.11
1.06
5.46
3.26
Lesion Area 3 Months
1
0.53
0.53
0.53
0.53
Table 15: Descriptive statistics of lesion area for tooth #10, control group.
Variable
N
Mean
Std Dev
Min
Max
Median
Lesion Area - Baseline
5
5.38
7.14
1.68
18.11
2.04
Lesion Area 3 Months
4
6.21
6.62
1.62
16.03
3.59
Table 16: Descriptive statistics of lesion area for tooth #11, control group.
Variable
N
Mean
Std Dev
Min
Max
Median
Lesion Area - Baseline
6
5.14
6.21
0.72
17.40
3.41
Lesion Area 3 Months
5
5.45
5.99
1.45
15.92
3.08
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35
Table 17: Descriptive statistics of lesion area for tooth #6, treatment group.
Variable
N
Mean**
Std Dev
Min
Max
Median
Lesion Area - Baseline
5
5.50
5.27
0.26
12.07
5.22
Lesion Area 3 Months
5
4.99
5.06
0.23
11.56
4.23
** Significantly different (p=0.0434, a paired-sample t-test).
Table 18: Descriptive statistics of lesion area for tooth #7, treatment group.
Variable
N
Mean
Std Dev
Min
Max
Median
Lesion Area - Baseline
6
7.25
6.60
2.15
16.57
3.57
Lesion Area 3 Months
6
7.12
3.30
4.57
11.79
5.28
Table 19: Descriptive statistics of lesion area for tooth #8, treatment group.
Variable
N
Mean
Std Dev
Min
Max
Median
Lesion Area - Baseline
3
4.18
4.07
0.69
8.66
3.20
Lesion Area 3 Months
3
1.02
1.76
0.00
3.05
0.00
-
36
Table 20: Descriptive statistics of lesion area for tooth #9, treatment group.
Variable
N
Mean
Std Dev
Min
Max
Median
Lesion Area - Baseline
3
1.42
0.39
1.05
1.83
1.38
Lesion Area 3 Months
3
0.55
0.95
0.00
1.65
0.00
Table 21: Descriptive statistics of lesion area for tooth #10, treatment group.
Variable
N
Mean
Std Dev
Min
Max
Median
Lesion Area - Baseline
5
8.20
8.79
0.90
22.09
4.14
Lesion Area 3 Months
5
6.00
9.73
0.00
22.59
0.48
Table 22: Descriptive statistics of lesion area for tooth #11, treatment group.
Variable
N
Mean
Std Dev
Min
Max
Median
Lesion Area - Baseline
4
15.32
14.21
1.94
28.14
15.61
Lesion Area 3 Months
4
14.25
13.83
0.70
27.68
14.32
-
37
Table 23: Descriptive statistics of lesion area for antimere teeth #6 and #11, control group.
Variable
N
Mean**
Std Dev
Min
Max
Median
Lesion Area - Baseline
12
7.70
8.00
0.72
26.64
4.77
Lesion Area 3 Months
10
7.76
8.41
0.84
25.19
3.78
** Significantly different (p=0.0235, a paired-sample t-test). *** Comparison was based on the available measurements on both baseline and follow-up. In this case, the mean difference between baseline and 3-month follow-up is 0.93 (std = 1.09).
Table 24: Descriptive statistics of lesion area for antimere teeth #6 and #11, treatment group.
Variable
N
Mean
Std Dev
Min
Max
Median
Lesion Area - Baseline
9
9.86
10.79
0.26
28.14
5.22
Lesion Area 3 Months
9
9.11
10.41
0.23
27.68
4.23
** Significantly different (p=0.0181, a paired-sample t-test).
Table 25: Descriptive statistics of lesion area for antimere teeth #7 and #10, control group.
Variable
N
Mean
Std Dev
Min
Max
Median
Lesion Area - Baseline
10
5.18
4.94
1.68
18.11
4.00
Lesion Area 3 Months
8
6.07
4.40
1.62
16.03
5.12
-
38
Table 26: Descriptive statistics of lesion area for antimere teeth #7 and #10, treatment group.
Variable
N
Mean
Std Dev
Min
Max
Median
Lesion Area - Baseline
11
7.68
7.28
0.90
22.09
3.65
Lesion Area 3 Months
11
6.61
6.60
0.00
22.59
5.24
Table 27: Descriptive statistics of lesion area for antimere teeth #8 and #9, control group.
Variable
N
Mean
Std Dev
Min
Max
Median
Lesion Area - Baseline
5
3.21
2.42
0.81
6.00
2.70
Lesion Area 3 Months
3
2.88
4.25
0.34
7.79
0.53
Table 28: Descriptive statistics of lesion area for antimere teeth #8 and #9, treatment group.
Variable
N
Mean
Std Dev
Min
Max
Median
Lesion Area - Baseline
6
2.80
3.00
0.69
8.66
1.61
Lesion Area 3 Months
6
0.78
1.29
0.00
3.05
0.00
** Significantly different (p=0.0331, a Wilcoxon signed-rank test).
-
39
Table 29: Descriptive statistics of lesion area for all teeth, control group.
Variable
N
Mean
Std Dev
Min
Max
Median
Lesion Area - Baseline
27
5.94
6.29
0.72
26.64
4.76
Lesion Area 3 Months
21
6.42
6.57
0.34
25.19
4.34
Table 30: Descriptive statistics of lesion area for all teeth, treatment group.
Variable
N
Mean
Std Dev
Min
Max
Median
Lesion Area - Baseline
26
7.31
8.22
0.26
28.14
3.57
Lesion Area 3 Months
26
6.13
7.91
0.00
27.68
4.15
** Significantly different (p=0.0219, a paired-sample t-test).
Based on the two-sample t-test, the data showed that there was no significant
difference in F value between control and treatment groups at baseline for teeth
numbers 7, 8, 10, 11 and all antimere teeth (p>0.05 in each instance), except for tooth number 6. The significant difference in F values between control and treatment groups
was found at baseline for tooth #6 (p=0.0240). Data showed that mean F values were significantly less negative in treatment group than control group (mean F: -7.23 vs. 17.07, respectively) (Table 31-42). Due to insufficient data, a statistical test was unable to be conducted for tooth #9.
-
40
Considering all the teeth at baseline, there was a significant difference in F
values between control and treatment groups (p=0.0268, a Wilcoxon rank-sum test). Data showed that median or mean F values was significantly less negative in treatment
group than control group (median F: -7.4 vs. -10.0, respectively) (Table 49 and 50). At 3-month follow-up, no significant differences were found for teeth numbers 6,
7, 8, 10, 11, and all antimere teeth (p>0.05 in each instance). Due to insufficient data, a statistical test was unable to be conducted for tooth #9. The data showed that there was a
significant difference in F values between control and treatment groups at 3-month
follow-up for all teeth (p=0.0332, Wilcoxon rank-sum test). Data showed that median or mean F values were significantly less negative in treatment group than control group
(median F: -6.80 vs. -9.51, respectively) (Table 49 and 50). To compare the changes in F values from baseline to 3-month follow-up
between the two groups, a new variable called F_value_change was created, and this
new variable is defined as F values at baseline minus F values at 3-month follow-up.
Based on the two-sample t-test, there were no significant differences between control and
treatment groups for the mean change in F values from baseline to 3-month follow-up
for teeth numbers 6, 7, 8, 10, and 11; all antimere teeth; and for all teeth (p>0.05 for each instance) . Due to insufficient data, a statistical test was unable to be conducted for tooth #9.
For the control group, the data showed there was no significant difference in F
values between baseline and 3-month follow-up for teeth numbers 6, 7, 8, 10, 11, and all
antimere teeth (p>0.05 in each instance). Due to insufficient data, a statistical test was unable to be conducted for tooth #9. The results indicated that there was a significant
difference in F values between baseline and 3-month follow-up for all teeth (p=0.0013, a Wilcoxon signed-rank test). Data showed that mean or median F values was significantly less negative at 3-month follow-up than at baseline (mean or median F: -9.17 or -9.51 vs. -12.00 or -10.00, respectively) (Table 49).
-
41
For the treatment group, no significant differences in F values between baseline
and 3-month follow-up were found for teeth numbers 6, 7, 8, 9, 10, 11; and all antimere
teeth (p>0.05 in each instance). The results indicated that there was a significant difference in F values between baseline and 3-month follow-up for all teeth (p=0.0288, a Wilcoxon signed-rank test). Data showed that median F values was significantly less negative at 3-month follow-up than at baseline (mean or median F: -10.07 or -6.80 vs. -12.06 or -7.40, respectively) (Table 50).
Table 31: Descriptive statistics of F values for tooth #6, control group.
Variable
N
Mean
Std Dev
Min
Max
Median
F Value - Baseline
5
-17.07
6.56
-24.50
-8.15
-15.50
F Value 3 Months
5
-10.03
4.26
-14.90
-6.30
-7.85
Table 32: Descriptive statistics of F values for tooth #7, control group.
Variable
N
Mean
Std Dev
Min
Max
Median
F Value - Baseline
4
-12.12
4.64
-16.30
-7.06
-12.56
F Value 3 Months
4
-9.87
2.40
-12.10
-6.47
-10.45
-
42
Table 33: Descriptive statistics of F values for tooth #8, control group.
Variable
N
Mean
Std Dev
Min
Max
Median
F Value - Baseline
2
-11.10
6.23
-15.50
-6.69
-11.10
F Value 3 Months
2
-6.45
9.12
-12.90
0.00
-6.45
Table 34: Descriptive statistics of F values for tooth #9, control group.
Variable
N
Mean
Std Dev
Min
Max
Median
F Value - Baseline
1
-8.66
-8.66
-8.66
-8.66
F Value 3 Months
1
-6.72
-6.72
-6.72
-6.72
Table 35: Descriptive statistics of F values for tooth #10, control group.
Variable
N
Mean
Std Dev
Min
Max
Median
F Value - Baseline
4
-11.22
4.36
-16.80
-6.27
-10.90
F Value 3 Months
4
-10.20
2.94
-13.00
-6.36
-10.72
-
43
Table 36: Descriptive statistics of F values for tooth #11, control group.
Variable
N
Mean
Std Dev
Min
Max
Median
F Value - Baseline
5
-8.50
1.37
-10.00
-6.48
-9.06
F Value 3 Months
5
-8.49
1.05
-9.73
-7.48
-7.98
Table 37: Descriptive statistics of F values for tooth #6, treatment group.
Variable
N
Mean
Std Dev
Min
Max
Median
F Value - Baseline
5
-7.23
4.43
-13.20
-0.81
-7.46
F Value 3 Months
5
-5.05
4.58
-10.40
-0.09
-6.82
Table 38: Descriptive statistics of F values for tooth #7, treatment group.
Variable
N
Mean
Std Dev
Min
Max
Median
F Value - Baseline
6
-17.28
14.10
-40.10
-3.55
-11.60
F Value 3 Months
6
-18.06
21.80
-52.30
-1.74
-7.12
-
44
Table 39: Descriptive statistics of F values for tooth #8, treatment group.
Variable
N
Mean
Std Dev
Min
Max
Median
F Value - Baseline
3
-4.66
3.95
-8.57
-0.68
-4.74
F Value 3 Months
3
-4.65
4.40
-8.80
-0.04
-5.11
Table 40: Descriptive statistics of F values for tooth #9, treatment group.
Variable
N
Mean
Std Dev
Min
Max
Median
F Value - Baseline
3
-5.18
3.53
-7.80
-1.16
-6.57
F Value 3 Months
3
-2.90
5.00
-8.67
0.00
-0.02
Table 41: Descriptive statistics of F values for tooth #10, treatment group.
Variable
N
Mean
Std Dev
Min
Max
Median
F Value - Baseline
5
-11.04
8.51
-25.70
-5.44
-6.41
F Value 3 Months
5
-4.68
4.32
-10.60
0.00
-3.65
-
45
Table 42: Descriptive statistics of F values for tooth #11, treatment group.
Variable
N
Mean
Std Dev
Min
Max
Median
F Value - Baseline
4
-22.27
34.13
-73.30
-1.39
-7.19
F Value 3 Months
4
-20.36
29.43
-64.10
-0.54
-8.40
Table 43: Descriptive statistics of F values for antimere teeth #6 and #11, control group.
Variable
N
Mean
Std Dev
Min
Max
Median
F Value - Baseline
10
-12.79
6.35
-24.50
-6.48
-9.58
F Value 3 Months
10
-9.26
3.04
-14.90
-6.30
-7.92
Table 44: Descriptive statistics of F values for antimere teeth #6 and #11, treatment group.
Variable
N
Mean
Std Dev
Min
Max
Median
F Value - Baseline
9
-13.91
22.57
-73.30
-0.81
-7.34
F Value 3 Months
9
-11.85
20.01
-64.10
-0.09
-6.82
-
46
Table 45: Descriptive statistics of F values for antimere teeth #7 and #10, control group.
Variable
N
Mean
Std Dev
Min
Max
Median
F Value - Baseline
8
-11.67
4.20
-16.80
-6.27
-10.90
F Value 3 Months
8
-10.03
2.49
-13.00
-6.36
-10.45
Table 46: Descriptive statistics of F values for antimere teeth #7 and #10, treatment group.
Variable
N
Mean
Std Dev
Min
Max
Median
F Value - Baseline
11
-14.44
11.79
-40.10
-3.55