2.1

Smear layer evaluation

2.1.1

Specimen preparation

Ethical clearance for the use of human teeth for the experiments performed in the present study was obtained from the institutional review board (IEC 166/2015) of Manipal University, India. Forty extracted human maxillary anterior teeth with straight root and single canal were selected. All the teeth were radiographed to verify the presence of a single canal with closed apex, and the absence of intra radicular resorption or root canal filling. Superficial soft tissues were removed with a curette and the teeth were stored in 0.2% sodium azide (Millipore Sigma, St. Louis, MO, USA) at 4 °C until use. The teeth were decoronated to standardise the root length to 15 mm longand the specimenswere randomly divided into three experimental groups and a control group (n = 10). Working length was established by inserting a size 10 K file (Mani Inc., Tochigi Ken, Japan) into each root canal until it was just visible at the apical foramen (observed using magnifying loupes) and by subtracting 1 mm from the recorded length. Chemomechanical preparation was performed using ProTaper ^® nickel titanium rotary instruments (Dentsply Maillefer, Ballaigues, Switzerland) and the canals wereinstrumented to size F3. Irrigation was performed with 2 mL of 2.5% of NaOCl (KMC Pharmacy, Manipal, India) after each instrument change.

2.2

Irrigation techniques

The final irrigation sequences were: (I) QMix group: 5 mL of 2.5% NaOCl for 1 min followed by 5 mL of QMix for 1 min; (II) MA group: 5 mL of 2.5% NaOCl for 1 min followed by 5 mL of 7% MA for 1 min; (III) EDTA group: 5 mL of 17% EDTA for 1 min; (IV) Negative control: 5 mL of 2.5% NaOCl for 1 min followed by 5 mL of 0.9% saline for 1 min. All the irrigating solutions were introduced into the canal using 29 gauge stainless steel needles (NaviTip ^® Tips, Ultradent Products Inc., South Jordan, UT, USA). The needle tip was inserted to 1 mm of the working length in each canal. After the use of the aforementioned irrigation protocols, each root canal was irrigated with 5 mL of deionised water to remove any precipitate that might have been formed. The canals were then dried with sterile paper points (Dentsply, Maillefer, Ballaigues, Switzerland). Longitudinal grooves werethen prepared on the buccal and lingual surfaces of each root using a diamond disc (Horico Dental, Berlin, Germany) at slow-speed without perforating the canal. The roots were then split into two halves using a chisel and stored in deionised water at 37 °C for scanning electron microscope (SEM) examination.

2.3

Scanning electron microscopy

The specimens were dehydrated using ascending grades of ethanol (25%, 50%, 75% and 100%), mounted on metal stubs, coated with gold/palladium using an ion-sputtering machine and examined with aJSM-6010 SEM (JEOL, Tokyo, Japan) for the presence or absence of the smear layer. Images were taken to observe the canal wall surface morphology at 500× magnification and 20 kV alongthe coronal (10–12 mm from apex), middle (6–7 mm from apex) and apical (1–2 mm from apex) thirds of each specimen. These areas were evaluated by two independent evaluators who were blind to the group designations. The images were scored according to the criteria reported by Torabinejad et al. : 1 = no smear layer (no smear layer on the surface of the canalwall; all dentinal tubules clean and open); 2 = moderate smear layer (no smear layer on the surface of the canal wall; tubules contain debris); and 3 = heavy smear layer (smear layer covering the canal wall and tubules).

2.4

Evaluation of mineral content

Twenty human maxillary central incisors extracted for periodontal reasons were selected and prepared using the previously described criteria, and stored in 0.2% sodium azide at 4 °C until use. The teeth were decoronated at the cementoenamel junction and the apical portions of the teeth were removed using a high speed diamond disc (Horico Dental, Germany) under water cooling. The length of each root was standardised to 10 mm long. The roots were then split longitudinally to obtain 40 root-halves; pulpal tissues present were removed with a fine brush. All specimens were dehydrated using Drierite for 14 days and weighed on a precision balance (AT 261, Mettler, Greifensee, Switzerland) so that each specimen weighed 0.20 g. Weight equality among the specimens was achieved by reducing the weight whenever necessary with silicon carbide abrasive paper from the cementum of the specimens. Thereafter, each specimen was covered with two consecutive layers of nail varnish, leaving the root canal surface exposed. The specimens were randomly divided into 4 groups (n = 10):

• (I)

  QMix group: treated with QMix for 1 min;

• (II)

  MA group: treated with 7% MA for 1 min;

• (III)

  EDTA group: treated with 17% EDTA for 1 min; and

• (IV)

  Negative control: treated with deionised water for 1 min.

In each group, the specimens were immersed in a magnetic stirrer bath containing 10 mL of the respective experimental solution. After one min, all the specimens were removed from the stirrer bath, thoroughly rinsed with deionised water and dried using absorbent lint-free paper.The specimens were then mounted on metal stubs, sputtered with gold/palladiumand prepared for mineral content analysis. The levels of calcium (Ca), phosphorus (P), magnesium (Mg), carbon (C) and oxygen (O) in the canal wall dentine surface of each specimen were measured using SEM-energy dispersive X-ray spectrometry (EDS; JEOL, Japan) with a minimum detectable range of 1%. Each specimen was irradiated at the centre and at two other equidistant areas, at a voltage of 20 kV for 60 s. Changes in the mineral levels were recorded and differences among the groups were statistically analysed.

2.5

Statistical analyses

For smear layer evaluation, the inter-examiner’s reliability was rated using coefficient of Kappa test. The mean was used to summarize the smear scores of the photomicrographs taken at each level of each specimen to account for the clustered nature of the data. The Cochran–Mantel–Haenszel (CMH) test was then used to test for significant differences amongst treatment groups separately at each canal level. If a significant difference amongst treatment groups was found, the CMH method was used to test comparisons among the treatment groups, adjusting for the effect of canal level. For mineral content analysis, comparison was performed non-parametrically using Kruskal-Wallis analysis of variance. Post-hoc pairwise comparisons were performed using the Dunn’stest. For all analyses, the significance level was preset at α = 0.05.

2.1

Smear layer evaluation

2.1.1

Specimen preparation

Ethical clearance for the use of human teeth for the experiments performed in the present study was obtained from the institutional review board (IEC 166/2015) of Manipal University, India. Forty extracted human maxillary anterior teeth with straight root and single canal were selected. All the teeth were radiographed to verify the presence of a single canal with closed apex, and the absence of intra radicular resorption or root canal filling. Superficial soft tissues were removed with a curette and the teeth were stored in 0.2% sodium azide (Millipore Sigma, St. Louis, MO, USA) at 4 °C until use. The teeth were decoronated to standardise the root length to 15 mm longand the specimenswere randomly divided into three experimental groups and a control group (n = 10). Working length was established by inserting a size 10 K file (Mani Inc., Tochigi Ken, Japan) into each root canal until it was just visible at the apical foramen (observed using magnifying loupes) and by subtracting 1 mm from the recorded length. Chemomechanical preparation was performed using ProTaper ^® nickel titanium rotary instruments (Dentsply Maillefer, Ballaigues, Switzerland) and the canals wereinstrumented to size F3. Irrigation was performed with 2 mL of 2.5% of NaOCl (KMC Pharmacy, Manipal, India) after each instrument change.

2.2

Irrigation techniques

The final irrigation sequences were: (I) QMix group: 5 mL of 2.5% NaOCl for 1 min followed by 5 mL of QMix for 1 min; (II) MA group: 5 mL of 2.5% NaOCl for 1 min followed by 5 mL of 7% MA for 1 min; (III) EDTA group: 5 mL of 17% EDTA for 1 min; (IV) Negative control: 5 mL of 2.5% NaOCl for 1 min followed by 5 mL of 0.9% saline for 1 min. All the irrigating solutions were introduced into the canal using 29 gauge stainless steel needles (NaviTip ^® Tips, Ultradent Products Inc., South Jordan, UT, USA). The needle tip was inserted to 1 mm of the working length in each canal. After the use of the aforementioned irrigation protocols, each root canal was irrigated with 5 mL of deionised water to remove any precipitate that might have been formed. The canals were then dried with sterile paper points (Dentsply, Maillefer, Ballaigues, Switzerland). Longitudinal grooves werethen prepared on the buccal and lingual surfaces of each root using a diamond disc (Horico Dental, Berlin, Germany) at slow-speed without perforating the canal. The roots were then split into two halves using a chisel and stored in deionised water at 37 °C for scanning electron microscope (SEM) examination.

2.3

Scanning electron microscopy

The specimens were dehydrated using ascending grades of ethanol (25%, 50%, 75% and 100%), mounted on metal stubs, coated with gold/palladium using an ion-sputtering machine and examined with aJSM-6010 SEM (JEOL, Tokyo, Japan) for the presence or absence of the smear layer. Images were taken to observe the canal wall surface morphology at 500× magnification and 20 kV alongthe coronal (10–12 mm from apex), middle (6–7 mm from apex) and apical (1–2 mm from apex) thirds of each specimen. These areas were evaluated by two independent evaluators who were blind to the group designations. The images were scored according to the criteria reported by Torabinejad et al. : 1 = no smear layer (no smear layer on the surface of the canalwall; all dentinal tubules clean and open); 2 = moderate smear layer (no smear layer on the surface of the canal wall; tubules contain debris); and 3 = heavy smear layer (smear layer covering the canal wall and tubules).

2.4

Evaluation of mineral content

Twenty human maxillary central incisors extracted for periodontal reasons were selected and prepared using the previously described criteria, and stored in 0.2% sodium azide at 4 °C until use. The teeth were decoronated at the cementoenamel junction and the apical portions of the teeth were removed using a high speed diamond disc (Horico Dental, Germany) under water cooling. The length of each root was standardised to 10 mm long. The roots were then split longitudinally to obtain 40 root-halves; pulpal tissues present were removed with a fine brush. All specimens were dehydrated using Drierite for 14 days and weighed on a precision balance (AT 261, Mettler, Greifensee, Switzerland) so that each specimen weighed 0.20 g. Weight equality among the specimens was achieved by reducing the weight whenever necessary with silicon carbide abrasive paper from the cementum of the specimens. Thereafter, each specimen was covered with two consecutive layers of nail varnish, leaving the root canal surface exposed. The specimens were randomly divided into 4 groups (n = 10):

• (I)

  QMix group: treated with QMix for 1 min;

• (II)

  MA group: treated with 7% MA for 1 min;

• (III)

  EDTA group: treated with 17% EDTA for 1 min; and

• (IV)

  Negative control: treated with deionised water for 1 min.

In each group, the specimens were immersed in a magnetic stirrer bath containing 10 mL of the respective experimental solution. After one min, all the specimens were removed from the stirrer bath, thoroughly rinsed with deionised water and dried using absorbent lint-free paper.The specimens were then mounted on metal stubs, sputtered with gold/palladiumand prepared for mineral content analysis. The levels of calcium (Ca), phosphorus (P), magnesium (Mg), carbon (C) and oxygen (O) in the canal wall dentine surface of each specimen were measured using SEM-energy dispersive X-ray spectrometry (EDS; JEOL, Japan) with a minimum detectable range of 1%. Each specimen was irradiated at the centre and at two other equidistant areas, at a voltage of 20 kV for 60 s. Changes in the mineral levels were recorded and differences among the groups were statistically analysed.

2.5

Statistical analyses

For smear layer evaluation, the inter-examiner’s reliability was rated using coefficient of Kappa test. The mean was used to summarize the smear scores of the photomicrographs taken at each level of each specimen to account for the clustered nature of the data. The Cochran–Mantel–Haenszel (CMH) test was then used to test for significant differences amongst treatment groups separately at each canal level. If a significant difference amongst treatment groups was found, the CMH method was used to test comparisons among the treatment groups, adjusting for the effect of canal level. For mineral content analysis, comparison was performed non-parametrically using Kruskal-Wallis analysis of variance. Post-hoc pairwise comparisons were performed using the Dunn’stest. For all analyses, the significance level was preset at α = 0.05.