2.1

Materials

Na-polyP with an average chain length of ≈40 phosphate units was obtained from Chemische Fabrik Budenheim (Budenheim, Germany).

2.2

Preparation of amorphous Ca-polyP microparticles

The microparticles, composed of Ca-polyP (termed aCa-polyP-MP), were prepared as described . By application of Fourier transform infrared spectroscopy the polymer characteristics of polyP within the microparticles was verified; X-ray diffraction analysis was used to prove that the material is amorphous . The average size of the particles is 300 nm and they vary within the size range of 100–600 nm ( Fig. 1 A and B).

2.3

In vitro incubation of teeth

In order to determine the efficacy of the aCa-polyP-MP to reseal the dentin layer and to check for the potency of the microparticles to occlude the dentinal tubules human teeth were used. They came from 20- to 50-years-old individuals of the Department of Oral and Maxillofacial Surgery of the University Medical Center of the University Mainz; Germany (gift of Prof. Dr. Bilal Al-Nawas; the permission to collect human teeth was obtained from the Ethical Committee of the “University Medical Center of the Johannes Gutenberg University Mainz” – No. 12-05-2015). Prior to use the teeth were mechanically cleaned from soft tissue, treated for 5 h in 3% Na-hypochlorite to remove tissue remains and then stored at 4 °C in a 100% relative humidity chamber.

Teeth specimens were submersed in saline (0.90% [w/v] NaCl) which contained, as mentioned in the text, either 10 mg/mL of aCa-polyP-MP or Na-polyP, stoichiometrically complexed with Ca ²⁺ (molar ratio of 2:1/phosphate monomer: Ca ²⁺ ; ). Incubation was performed at 25 °C. Then the samples were sliced by cutting 1–2 mm thick discs inwards to the pulp as described ; where indicated, the dentin or enamel regions, as well as the cement layer, were included in the measurements.

2.4

Microscopic analyses

Scanning electron microscopy (SEM) was performed with a HITACHI SU 8000 (Hitachi High-Technologies Europe GmbH, Krefeld, Germany), equipped with a low voltage (<1 kV; analysis of near-surface organic surfaces ) detector. Where mentioned the samples have been cut . Digital light microscopy was performed with a VHX-600 Digital Microscope (Keyence, Neu-Isenburg; Germany) equipped with a VH-Z100 zoom lens.

2.5

Energy dispersive X-ray spectroscopy

Energy dispersive X-ray (EDX) spectroscopy was performed with an EDAX Genesis EDX System attached to a scanning electron microscope (Nova 600 Nanolab; FEI, Eindhoven, the Netherlands) operating at 10 kV with a collection time of 30–45 s. Areas of approximately 10 μm ² were analyzed.

2.6

Mechanical-nanoindentation determinations

The surfaces of either the untreated or the polyP-coated teeth specimens were evaluated at 25 °C by depth-sensing indentation, using a NanoTest Vantage system (Micro Materials Ltd., Wrexham; UK). The methods used have been published previously . In one series of experiments the surfaces of the teeth were brushed using an electric toothbrushes (Braun Oral-B PRO 6000; Procter & Gamble, Cincinnati, OH) at 8000 rpm and 100 g force for 3 min at room temperature, as described .

2.7

Reverse transcription-quantitative real-time PCR analyses

To quantify the expression level of the gene encoding the ALP in the hMSC, the technique of reverse transcription-quantitative real-time polymerase chain reaction (qRT-PCR) was applied. After incubating the cells for 1, 3 and 7 d in the presence of 30 μg/mL either of Na-polyP [Ca ²⁺ ] or of aCa-polyP-MP they were harvested, RNA was isolated and qRT-PCR was performed . The primer pairs, matching with the human ALP gene (accession number NM_000478.4 ) Fwd: 5′-TGCAGTACGAGCTGAACAGGAACA-3′ [nt ₁₁₄₁ to nt ₁₁₆₄ ] and Rev: 5′-TCCACCAAATGTGAAGACGTGGGA-3′ [nt ₁₄₁₈ to nt ₁₃₉₅ ; PCR product length 278 bp], as well as the COL1A1 gene (NM_000088.3) Fwd: 5′-GACTGCCAAAGAAGCCTTGCC-3′ [nt ₅₀₇₃ to nt ₅₀₉₃ ] and Rev: 5′-TTCCTGACTCTCCTCCGAACCC-3′ [nt ₅₁₁₉₆ to nt ₅₁₇₅ ; PCR product length 124 bp] and with the reference gene GAPDH ( glyceraldehyde 3-phosphate dehydrogenase ; NM_002046.3) using the primer pair Fwd: 5′-CCGTCTAGAAAAACCTGCC-3′ [nt ₈₄₅ to nt ₈₆₃ ] and Rev: 5′-GCCAAATTCGTTGTCATACC-3′ [nt ₁₀₅₉ to nt ₁₀₇₈ ; 215 bp], were used. The amplification was performed in an iCycler (Bio-Rad, Hercules; CA) with the respective iCycler software.

2.8

Cultivation of the human multipotent stromal cells

The human multipotent stromal cells (hMSC) differentiate into odontoblasts in the presence of conditioned medium from developing tooth germ cells; the conditioned medium was prepared as described . The description of the cultivation procedure for the hMSCs was given recently .

2.9

Statistical analysis

After finding that the values follow a standard normal Gaussian distribution, the results were statistically evaluated using paired Student’s t -test .

2.1

Materials

Na-polyP with an average chain length of ≈40 phosphate units was obtained from Chemische Fabrik Budenheim (Budenheim, Germany).

2.2

Preparation of amorphous Ca-polyP microparticles

The microparticles, composed of Ca-polyP (termed aCa-polyP-MP), were prepared as described . By application of Fourier transform infrared spectroscopy the polymer characteristics of polyP within the microparticles was verified; X-ray diffraction analysis was used to prove that the material is amorphous . The average size of the particles is 300 nm and they vary within the size range of 100–600 nm ( Fig. 1 A and B).

2.3

In vitro incubation of teeth

In order to determine the efficacy of the aCa-polyP-MP to reseal the dentin layer and to check for the potency of the microparticles to occlude the dentinal tubules human teeth were used. They came from 20- to 50-years-old individuals of the Department of Oral and Maxillofacial Surgery of the University Medical Center of the University Mainz; Germany (gift of Prof. Dr. Bilal Al-Nawas; the permission to collect human teeth was obtained from the Ethical Committee of the “University Medical Center of the Johannes Gutenberg University Mainz” – No. 12-05-2015). Prior to use the teeth were mechanically cleaned from soft tissue, treated for 5 h in 3% Na-hypochlorite to remove tissue remains and then stored at 4 °C in a 100% relative humidity chamber.

Teeth specimens were submersed in saline (0.90% [w/v] NaCl) which contained, as mentioned in the text, either 10 mg/mL of aCa-polyP-MP or Na-polyP, stoichiometrically complexed with Ca ²⁺ (molar ratio of 2:1/phosphate monomer: Ca ²⁺ ; ). Incubation was performed at 25 °C. Then the samples were sliced by cutting 1–2 mm thick discs inwards to the pulp as described ; where indicated, the dentin or enamel regions, as well as the cement layer, were included in the measurements.

2.4

Microscopic analyses

Scanning electron microscopy (SEM) was performed with a HITACHI SU 8000 (Hitachi High-Technologies Europe GmbH, Krefeld, Germany), equipped with a low voltage (<1 kV; analysis of near-surface organic surfaces ) detector. Where mentioned the samples have been cut . Digital light microscopy was performed with a VHX-600 Digital Microscope (Keyence, Neu-Isenburg; Germany) equipped with a VH-Z100 zoom lens.

2.5

Energy dispersive X-ray spectroscopy

Energy dispersive X-ray (EDX) spectroscopy was performed with an EDAX Genesis EDX System attached to a scanning electron microscope (Nova 600 Nanolab; FEI, Eindhoven, the Netherlands) operating at 10 kV with a collection time of 30–45 s. Areas of approximately 10 μm ² were analyzed.

2.6

Mechanical-nanoindentation determinations

The surfaces of either the untreated or the polyP-coated teeth specimens were evaluated at 25 °C by depth-sensing indentation, using a NanoTest Vantage system (Micro Materials Ltd., Wrexham; UK). The methods used have been published previously . In one series of experiments the surfaces of the teeth were brushed using an electric toothbrushes (Braun Oral-B PRO 6000; Procter & Gamble, Cincinnati, OH) at 8000 rpm and 100 g force for 3 min at room temperature, as described .

2.7

Reverse transcription-quantitative real-time PCR analyses

To quantify the expression level of the gene encoding the ALP in the hMSC, the technique of reverse transcription-quantitative real-time polymerase chain reaction (qRT-PCR) was applied. After incubating the cells for 1, 3 and 7 d in the presence of 30 μg/mL either of Na-polyP [Ca ²⁺ ] or of aCa-polyP-MP they were harvested, RNA was isolated and qRT-PCR was performed . The primer pairs, matching with the human ALP gene (accession number NM_000478.4 ) Fwd: 5′-TGCAGTACGAGCTGAACAGGAACA-3′ [nt ₁₁₄₁ to nt ₁₁₆₄ ] and Rev: 5′-TCCACCAAATGTGAAGACGTGGGA-3′ [nt ₁₄₁₈ to nt ₁₃₉₅ ; PCR product length 278 bp], as well as the COL1A1 gene (NM_000088.3) Fwd: 5′-GACTGCCAAAGAAGCCTTGCC-3′ [nt ₅₀₇₃ to nt ₅₀₉₃ ] and Rev: 5′-TTCCTGACTCTCCTCCGAACCC-3′ [nt ₅₁₁₉₆ to nt ₅₁₇₅ ; PCR product length 124 bp] and with the reference gene GAPDH ( glyceraldehyde 3-phosphate dehydrogenase ; NM_002046.3) using the primer pair Fwd: 5′-CCGTCTAGAAAAACCTGCC-3′ [nt ₈₄₅ to nt ₈₆₃ ] and Rev: 5′-GCCAAATTCGTTGTCATACC-3′ [nt ₁₀₅₉ to nt ₁₀₇₈ ; 215 bp], were used. The amplification was performed in an iCycler (Bio-Rad, Hercules; CA) with the respective iCycler software.

2.8

Cultivation of the human multipotent stromal cells

The human multipotent stromal cells (hMSC) differentiate into odontoblasts in the presence of conditioned medium from developing tooth germ cells; the conditioned medium was prepared as described . The description of the cultivation procedure for the hMSCs was given recently .

2.9

Statistical analysis

After finding that the values follow a standard normal Gaussian distribution, the results were statistically evaluated using paired Student’s t -test .