Surgical procedure

The animals were anaesthetized with an intraperitoneal injection of 3.6% chloral hydrate (1 ml/100 g). The anaesthetized animals were placed in a supine position and the full thickness defects of 10 mm in diameter were demarcated and created by surgical incision using a standard surgical blade on the buccal mucosa under microscopic guidance. Figure 1 shows different views of wound creation. Sterilized polyporous silk fibroin scaffolds and crosslinking silk fibroin films were trimmed into round membranes with diameters of 10 mm and loaded onto single layered Vaseline gauze squares. The defects were covered with the gauze and secured by suturing to the adjacent mucosa with 7-0 silk suture. Two additional Vaseline gauze squares were placed on top and sutured with 1-0 silk suture.

Snapshots at different time spots during the surgical procedures for the creation of the wound (A–D).

At 5 days postoperatively, 10 rats were selected randomly from each group and anaesthetized with an intraperitoneal injection of 3.6% chloral hydrate (1 ml/100 g). The colour, exudation and healing of the wounds were observed and recorded. The diameter of the wounds was measured at three different locations using Vernier callipers. The selected rats were marked and macrographic observation and diameter measurements were made on the marked rats on days 10 and 15.

On days 10, 20 and 30 after surgery, 10 rats were selected from each group. 0.5 ml tail blood was obtained for peripheral blood T lymphocyte analysis under anaesthesia. These rats were killed and 5 mm × 5 mm newly grown mucosal tissues were harvested and fixed in 10% formalin, prior to haematoxylin–eosin (H–E) staining and subsequent histological and immunohistochemical analysis.

Histological study

Tissues were taken from the surgical area and fixed in 10% formalin for 48 h. H–E staining was done according to a standard protocol. Five microscopic views from each rat were randomly selected and the number of inflammatory cells and fibroblasts were counted by two independent pathologists using ×400 magnification.

Determination of newly formed blood vessels in the wounds was verified by CD34 staining . Briefly, the tissues were taken from the surgical area and fixed in 10% formalin for 48 h. Samples were cut into 3 mm × 3 mm × 3 mm cubes and embedded in paraffin and then sectioned to tissue slides with a thickness of about 3 μm. Immunohistochemical studies were performed using primary rabbit antibody against rat. Briefly, the tissue slides were deparaffinized and rehydrated, then submerged in hydrogen peroxide for peroxidase quenching. Before using the primary antibody, the slides were incubated with goat serum for 10 min to block non-specific binding. After 1 h incubation with the primary antibody, the secondary goat against rat antibody was added and incubated at room temperature for 10 min. Fifty microlitres streptovidin biotin complexes were incubated for 10 min at room temperature. Staining was performed by diaminobenze dinetetrahydrochloride (DAB) substrate and slides were counterstained with haematoxylin and mounted.

Endothelial cells of newly formed blood vessels were stained with anti-CD34 monoclonal antibody (Boster Biological Technology, Ltd, Wuhan, China). The positive cells appeared as clear brown in cytoplasm. Density of microvascular endothelia was expressed as the average cell numbers of 5 views at ×400 magnification.

Cytokeratin (CK) expression was determined to assess the density of newly formed oral epithelial cells in the wounds using immunohistochemistry described previously . Briefly, animals were killed and tissue samples were taken from the surgical area and fixed in 10% formalin for 48 h. Samples were cut into 3 mm × 3 mm × 3 mm cubes and embedded in paraffin and then sectioned to tissue slides with a thickness of about 3 μm. Immunohistochemical studies were performed using mouse against rat monoclonal CK antibody (Boster Biological Technology, Ltd, Wuhan, China). Briefly, the tissue slides were deparaffinized and rehydrated, then submerged in hydrogen peroxide for peroxidase quenching. Mouse against rat monoclonal antibody was added and kept overnight at 4 °C. Horseradish peroxidase conjugated goat anti-mouse polymer was added and incubated at 37 °C for 30 min. Staining was performed by DAB substrate and slides were counterstained with haematoxylin and mounted. The positive newly formed oral epithelial cells appeared as clear brown in cytoplasm. Magnification of ×100 was employed to assess the overall morphological features whilst ×400 was used for observations of the multi-layered epithelial cells with thick rete pegs .

To assess T lymphocyte subsets in peripheral blood, 0.5 ml tail blood samples were collected from 10 randomly selected rats in each group. Each blood sample was divided and heparinized into four tubes (three for test, one for control) for T lymphocyte subsets analysis. Ten microlitres anti-rat CD3, CD4 and CD 8 fluorescein isothiocyanate (FITC) conjugated monoclonal antibody were added to each of the test tubes (eBioscience, Shanghai Laizee Biotech Co., Ltd, Shanghai, China) . Rat IgG1 was added to the control tube as negative controls to define background staining. An aliquot of whole blood (50 μl) was added to the test tube, mixed, and then left in the dark for 20 min at room temperature. Two hundred fifty microlitres haemolysin was added to each tube, mixed thoroughly and left for 10 min at room temperature. Two millilitres phosphate buffered saline (PBS) was used to rinse the samples twice with centrifugation at 1200 rpm for 5 min. Supernatant was discarded and 0.5 ml PBS was added before flow cytometry (FCM) analysis (Beckman-Coulter USA). FCM and scattering distribution were obtained and analysed using SYSTEMT M II software. The percentage of CD3 ⁺ , CD4 ⁺ and CD8 ⁺ was calculated.

Statistical analysis

Statistical calculations were performed with SAS8.1 software (SAS Institute Inc., Cary, NC, USA). Student’s t -test was used to determine the significance of the differences between group means. Statistical significance was defined as P < 0.05.

Histology and immunohistochemistry

Newly generated buccal mucosa specimens were sectioned for H–E staining and CD34, CK immunohistochemical analysis to inspect the distribution of the inflammatory cells, fibroblasts and microvascular endothelia in three groups.

On postoperative day 10, newly generated multi-layered epithelia were found at the wound margin with thick rete pegs in group A. Inflammatory cells and fibroblasts appeared on the polyporous silk fibroin scaffolds. Newly formed capillaries were visible with a small cavity ( Fig. 3 – HE ). Compared to group A, there were fewer epithelia layers with small and sparse distributed rete pegs in group B. A swelling band between the silk fibroin and tissue surface was noticeable surrounded by dense inflammatory cells and fibroblasts, with blood vessels infiltrating into the membrane ( Fig. 3 – CK). In contrast, a significant accumulation of inflammatory cells, fibroblasts, new capillaries with large cavities in granular tissue was observed in the control group ( Fig. 3 – Cd34). The epithelium in this group had fewer layers of cells compared to the other two groups and the continuity of epithelium remained intact.

Representative histology and immunohistology microphotographs (×100) of buccal mucosa from silk fibroin scaffold, silk fibroin film and control groups (10 days postoperative). Arrows indicate the newly formed capillaries. Bar is 50 μm.

By day 20, similar observations were found in the three groups including an increased number of epithelial rete pegs, reduced cellular swelling, decreased inflammatory infiltrates and increased number of fibroblasts as well as capillary endothelia. Partial degradation of silk fibroin with short and sparse fibroin fibres was also readily detectable.

By day 30, the silk fibroin in tissue almost disappeared, inflammatory cells decreased and fibroblasts increased. The number of capillaries increased and the cavity of blood vessels enlarged. Comparison of inflammatory cells, fibroblasts and density of endothelia is demonstrated in Fig. 4 .

Comparison of neutrophils, fibroblasts and capillary endothelia in the buccal wounds amongst three groups.

Peripheral T lymphocyte subsets

There were no significant differences in the percentages of CD3 ⁺ , CD4 ⁺ , and CD8 ⁺ in rat peripheral blood amongst the three groups on days 10, 20 and 30 after surgery ( Fig. 5 ).

Distribution of peripheral lymphocyte subgroups in the three groups after buccal surgery <SPAN role=presentation tabIndex=0 id=MathJax-Element-1-Frame class=MathJax style="POSITION: relative" data-mathml='(x¯±S,n=10)’>(x¯±S,n=10)(x¯±S,n=10)
( x ¯ ± S , n = 10 )
.

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