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ORIGINAL ARTICLE
Year : 2019  |  Volume : 8  |  Issue : 3  |  Page : 71-75

Influence of blood contamination and decontamination procedures on bond strength of a two-step etch and rinse adhesive system


1 Graduate Program in Dentistry, Department of Restorative Dentistry, School of Dentistry, Federal University of Pelotas, Pelotas, Rio Grande do Sul, Brazil
2 Department of Restorative Dentistry, Metropolitan Faculty of Grande Fortaleza, Fortaleza, Ceará, Brazil
3 Graduate Program in Dentistry, Department of Restorative Dentistry, School of Dentistry, Federal University of Pelotas, Pelotas, Rio Grande do Sul, Brazil; Dental Materials Laboratory, Academic Area of Dentistry, Autonomous University of Hidalgo State, Pachuca, Hidalgo, México

Date of Web Publication11-Sep-2019

Correspondence Address:
Prof. Rafael Guerra Lund
Department of Restorative Dentistry, Pelotas Dental School, Federal University of Pelotas, Gonçalves Chaves Street N. 457, Rm. 503, Centro District, 96015-560 Pelotas, Rio Grande do Sul
Brazil
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Source of Support: None, Conflict of Interest: None


DOI: 10.4103/ejgd.ejgd_57_19

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  Abstract 


Purpose: This study evaluated the effect of blood contamination and decontamination procedures performed at different stages of bonding, on the microtensile bond strength (μTBS) of an etch-and-rinse adhesive to dentin. Materials and Methods: Standardized cylindrical cavities were prepared in bovine incisors and were randomly divided into five groups, each one was treated using these experimental conditions – Control: etching-rinsing/bonding without blood contamination; Group 1: etching-rising/blood contamination/decontamination/bonding; Group 2: etching-rising/bonding/blood contamination/decontamination; Group 3: etching-rising/bonding/blood contamination/decontamination/etching-rising/bonding; and Group 4: etching-rising/blood contamination/decontamination/etching-rising/bonding. Specimens were prepared for μTBS and were evaluated both immediately and after 6 months of storage in distilled water. Results: Blood contamination significantly reduced the μTBS (P < 0.001). Groups 2 and 3 showed the lowest μTBS values, both for 24 h and 6 month aging. Conclusions: Blood contamination tested at any of the different stages of the bonding procedure showed a negative effect on the μTBS. Recovering adhesion of blood-contaminated dentin did not depend only on cleaning with distilled water.

Keywords: Contaminants, decontamination, dentin-bonding agents, microtensile, resin composite


How to cite this article:
Lund RG, Da Silveira IA, Ribeiro JS, Rubin D, Peralta SL, Cuevas-Suárez CE, Piva E. Influence of blood contamination and decontamination procedures on bond strength of a two-step etch and rinse adhesive system. Eur J Gen Dent 2019;8:71-5

How to cite this URL:
Lund RG, Da Silveira IA, Ribeiro JS, Rubin D, Peralta SL, Cuevas-Suárez CE, Piva E. Influence of blood contamination and decontamination procedures on bond strength of a two-step etch and rinse adhesive system. Eur J Gen Dent [serial online] 2019 [cited 2019 Nov 21];8:71-5. Available from: http://www.ejgd.org/text.asp?2019/8/3/71/266696




  Introduction Top


Current adhesive systems are applied using either an “etch-and-rinse,” “self-etch,” or “selective etch” technique, which differs in how the adhesives are applied and how they interact with tooth structures.[1] Etch-and-rinse systems comprise phosphoric acid to pretreat the dental hard tissues before rinsing and subsequent application of an adhesive. In the etch-and-rinse approach, adhesives are applied after phosphoric acid etching, whereas when using the self-etching technique, the acid-etching step is eliminated, simplifying the procedure.[2] The evidence available today suggests that the choice between etch-and-rinse or self-etch systems is often a matter of personal preference.[3] In general, the etch-and-rinse technique is frequently preferred for indirect restorations and when large areas of enamel are still present.[4]

The effectiveness of dentin bonding systems after suitable clinical application protocols is required to ensure the longevity of restorations. Clinically, many factors are known to impair adhesion and retention of resin-containing restorative materials such as the contamination of the operative field with oral fluids and microorganisms.[5],[6] To prevent this, the rubber dam is still the most important tool to use to guarantee moisture control.[7],[8] However, moisture control is difficult in some clinical situations, such as caries located at or near the gingival margin,[9] and contamination of the operative field with blood or saliva is likely to occur.[6]

Previous studies that have evaluated the effect of blood contamination during bonding procedures have shown that this could lead to premature failure of the bond of light-cured resin composites, even after several decontamination methods.[10],[11],[12] Contamination of operative field can occur at different critical times of the bonding procedure: before or after acid etching, after application of adhesive without light activation, after application of adhesive and light application, during insertion of a resin composite in increments, and after restoration placement.[10],[11],[13],[14],[15] Furthermore, few studies[16],[17],[18] have evaluated the effect of blood contamination in conventional adhesive systems.

Thus, this study aimed to evaluate the bond strength of a two-step etch-and-rinse adhesive system to dentin in the presence of blood contamination and to determine which decontamination protocol is capable of recovering adhesion. The null hypotheses to be tested were that (1) blood contamination will not impair the bond strength to dentin and that (2) the decontamination protocols tested will be able to recover the bond strength to dentin of a two-step etch-and-rinse adhesive.


  Materials and Methods Top


Twenty freshly extracted bovine incisors were collected and stored in 0.5% Chloramine-T solution for 7 days. Teeth were then kept in distilled water at 4°C until use.[19] The criteria for tooth selection included intact buccal enamel free of caries, cracks, and damage due to extraction. Each tooth was examined under a stereomicroscope to eliminate teeth with cracks or hypoplastic defects. All teeth were cleaned using hand scalers and scalpels, and then, their roots were sectioned using a low-speed diamond saw under water cooling, and their crowns were embedded in polyester resin (Resina cristal, Comfibras, Porto Alegre – Brasil), allowing the buccal enamel surface to be exposed. Then, the enamel was removed with an orthodontic grinder, and then, the exposed dentin surface was wet-ground with 400- and 500-grit SiC abrasive papers coupled to a universal polishing machine at a speed of 50 rpm, under constant water irrigation.

Standardized cylindrical cavities were prepared in the flat dentin using a round-wheel diamond bur (No. 3056, KG Sorensen, Alphaville, SP, Brazil) under water irrigation. Diamond bur was replaced after every five preparations to ensure efficient cutting. The cavity dimensions were 4.0 ± 0.1 mm in diameter and 1.0 ± 0.1 mm deep [Figure 1]. The teeth with the prepared cavities were divided into five experimental groups of six teeth each, and these were randomly assigned to one of the five blood contamination and decontamination protocols used [Figure 2]. Fresh human blood was collected from the fingertip of a volunteer (ethics committee approval protocol No. 41/11 Dentistry/UFPel) at the same time that the restoration processes were performed. In the blood contamination groups, the specimens were rinsed with distilled water and were dried with sterile paper towels.[20],[21]
Figure 1: Schematic representation of the microtensile bond strength process used. (a) Root sectioning. (b). Crown embedded in polyester resin. (c) Dentin surface exposed. (d) Cylindrical cavity preparation. (e) Bonding procedures. (f) Increments of micro-hybrid resin composite. (g) Specimens sectioning. (h) Microtensile bond strength beams

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Figure 2: Experimental groups and decontamination protocols

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The restorative procedures were performed using a two-step etch-and-rinse adhesive system (Single Bond; 3M ESPE, St Paul, MN, USA) applied in accordance with the manufacturer's recommendations. Phosphoric acid gel (Scotchbond etchant; 3M ESPE, St Paul, MN, USA) was applied during 15 s and then rinsed for 10 s. Excess water was removed using sterile paper towels, leaving dentin moist. Then, two consecutive coats of adhesive were applied to the etched dentin using a microbrush. A stream of air was applied for 5 s between each coat. The adhesive was light cured using a light-emitting diode (LED) photopolymerization unit (Radii Cal, SDI Limited, Victoria, Australia) with a light irradiance of 900 mW/cm2. After light curing the adhesive, a microhybrid resin composite (Filtek Z-250; 3M ESPE, St. Paul, MN, USA) was applied in four increments of approximately 1.0 mm thick. Each increment was light cured for 20 s with a light polymerizing unit equipped with a LED visible light source (Radii Cal; SDI, Bayswater, Victoria, Australia).

After storage in distilled water at 37°C for 24 h, the specimens were sectioned perpendicular to the bond interfaces in the mesiodistal and buccolingual directions, using a slow-speed diamond saw (Isomet Saw 1000 Precision, Buehler Ltd., Lake Bluff, IL, USA) to obtain resin-dentin beams with a cross-sectional area of approximately 0.5 mm2. Six beams from each tooth were obtained, providing 30 sticks per group for the microtensile bond strength (μTBS) test. Half of the beams were tested after 24 h and the other half, after 6 months of storage in distilled water at 37°C (n = 15). The beams were attached to a microtensile testing device with cyanoacrylate glue (Super Bonder Gel, Loctite® Corp., Henkel Technologies, Diadema, SP, Brazil), and the μTBS was tested in a universal mechanical testing machine (DL 500, EMIC®, Pinhais, PR, Brazil), at a crosshead speed of 0.5 mm/min and a load cell of 100 N.

The μTBS values were expressed in MPa by dividing the load (N) applied at the time of the fracture by the cross-sectional area of the bonded interface (μTBS = F/A). The fracture modes were evaluated by a single observer, using a light microscope (Mobiloskop; Renfert, Hilzingen, Germany) at ×100 and ×500. Failure modes were classified as adhesive, cohesive within dentin, and cohesive within resin composite or mixed failure.

The data were analyzed to check normality (Shapiro–Wilk test) and homoscedasticity (Levene's test). Two-way analysis of variance (ANOVA) was used to evaluate the effect of contamination step and storage time on the μTBS. Multiple comparison procedures were performed using Tukey's test (α = 5%). Data were analyzed and plotted with SigmaPlot 12 software (Systat Software Inc., San Jose, CA, USA).


  Results Top


The results of the μTBS test are summarized in [Figure 3]a. The two-way ANOVA test revealed that μTBS was influenced by both the decontamination protocol and storage time (P< 0.05); however, the interaction between these two variables was not significant (P = 0.529).
Figure 3: Microtensile bond strength (a) and distribution of failure modes (b). Columns under the same horizontal line indicate no differences between aging times for each group. Different capital or lowercase letters indicate differences between groups within 24 h and 6 months, respectively

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In the μTBS test at 24 h, the highest bond strength values were observed for the Control Group, followed by Group 1; the lowest μTBS values were observed for Group 3. After 6 months of storage in distilled water, the μTBS values decreased in all groups; the Control Group showed the highest values, while the Group 2 showed the lowest μTBS values; however, these differences were not statistically significant. The intergroup analysis revealed that μTBS values for Groups 3 and 4 remained stable.

The numbers and percentages of failure modes in each group are shown in [Figure 3]b. The results of failure mode analysis after 24 h demonstrated that adhesive type failure mode was predominant in all groups, followed by mixed-type failure. After 6 months of aging, the results of failure mode analysis demonstrated that the adhesive type failure mode remained predominant in all groups, followed by the cohesive in dentin failure type.


  Discussion Top


In this study, the influence of blood contamination on the bond strength of a two-step etch-and-rinse adhesive to dentin was investigated. Besides, the decontamination protocol that would be capable of recovering the bond strength of this adhesive system was determined. Since the statistical analysis revealed that blood contamination impaired the bond strength of a resin composite to dentin and that none of the decontamination protocols tested were able to recover the bond strength, the null hypotheses tested in this study were rejected.

In this study, freshly drawn blood, collected at the same time that the experiment was being performed, was used to contaminate the dentin surfaces. No anticoagulants were used since studies in the literature have shown that the addition of an anticoagulant may reduce the bond strength.[10],[22] Considering this variable, and other factors such as the adhesive system used, the step when contamination occurs, and substrate type, it was difficult to make comparisons with previous studies that investigated the blood contamination of adhesive restorations.

The results obtained in this study proved that when compared with the control group, any blood contamination at any of the stages of adhesive system application decreased the μTBS, both in 24 h and after 6 months. The literature has shown that the blood is capable of interacting with the dentin surface, and the content of proteins, macromolecules of fibrinogen, and platelets may form a thin film on the dentin surface, which may make it difficult for the adhesive to infiltrate into the treated dentin, thereby weakening the bond strength.[23] Furthermore, residual blood proteins could remain on the polymerized bond surface and eliminate an oxygen-inhibited layer, which has the potential of preventing copolymerization between the successive increments of resin composite material.[24]

Among the decontamination protocols, when the contamination occurred after the application of acid and before the application of the adhesive system (Group 1), the bond strength values were higher than those in the other contaminated groups, both in 24 h and after 6 months. These results could be explained by the cleaning processes performed after blood contamination, which were able to eliminate a large part of the blood proteins deposited on the dentin surfaces. In addition, it could be hypothesized the application of primer cleaned or hydrolyzed blood on the dental surface.[25] However, as no values equal to those of the control group were obtained, rinsing with water was shown to be insufficient to achieve complete decontamination of the dentin surface.

When the contamination occurred after the application of the adhesive system (Groups 2 and 3), the decrease in bond strength could be attributed to the degradation of the adhesive components of the contaminated adhesive layer, rather than to its removal. Furthermore, the presence of excessive humidity trapped in the degraded components in the dentinal tubules may have impaired bonding between the subsequent resin composite layers (increments).[26]

Moreover, in this study, it could be demonstrated that after the dentin surface had been contaminated, it was not recommendable to re-etch the contaminated surface. In Groups 3 and 4, in which a re-etching procedure was performed after blood contamination, lower μTBS values were also observed. A possible explanation for this could be that re-etching the dentin surface could produce an excessive layer of demineralized dentin, which could be not totally penetrated by the adhesive system, allowing the formation of a fragile adhesive area.[27]

This study showed the negative effect that blood contamination has on the bond to dentin when using a two-step etch-and-rinse adhesive system. Besides, it could be established that recovering the bond to blood contaminated dentin surfaces did not depend only on careful cleaning with distilled water, and other cleaning agents should be tested in further studies.


  Conclusions Top


The findings of this study proved that blood contamination significantly impaired the bond strength of two-step etch-and-rinse adhesives to dentin. In addition, none of the decontamination protocols tested were capable of recovering the bond strength. Therefore, when the dentin surface has been contaminated with blood during the restoration bonding procedures with the use of two-step etch-and-rinse adhesives, the dentin surface should be re-prepared with a rotary cutter to prevent impairment of the bond efficiency of the adhesive system.

Acknowledgments

This work was supported by the Research Support Foundation of Rio Grande do Sul – Brazil (FAPERGS APE 12/05783 and PRONEX 16.0471-4). This study was also financed in part by the Coordenação de Aperfeiçoamento de Pessoal de Nível Superior – Brasil (CAPES) – Finance Code 001, Brazil. The author, Carlos Enrique Cuevas Suárez, would like to thank PRODEP, México (DSA/103.5/15/6615).

Financial support and sponsorship

Nil.

Conflicts of interest

There are no conflicts of interest.



 
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