2.1. Drugs and chemicals
Umbelliferone (UMB) was purchased from Sigma Aldrich (USA). Acetic acid AA was purchased from El-Naser Pharmaceutical Chemicals Company (Egypt). Rats TNF-α and IL-6 ELISA kits for were purchased from Glory Science Company (USA). Trizol reagent was purchased from Invitrogen Inc, Grand Island, NY (USA). Complementary DNA (cDNA) was purchased from Thermo Scientific Revert Aid (USA). SYBR green master mix was purchased from Bioline, myBio (Ireland) PCR primers for NF-κB-p65, iNOS, TLR4, PPARγ, SIRT1, and β-actin genes were synthesized by Vivantis Technologies (Malaysia). The antibodies used were mouse monoclonal anti-NF-κB-p65, anti-iNOS, anti-TLR4, anti-PPARγ, anti-SIRT1 anti-p38MAPK, anti-ERK1, anti-VCAM-1, and anti-β-actin antibodies and were purchased from Santa Cruz (USA). BCIP/NBT substrate detection kit was purchased from Genemed Biotechnologies, (USA). Alkaline phosphatase (ALP)-conjugated secondary antibody was purchased from Santa Cruz (USA).
2.2. Animals
Adult male Wistar rats, weighing 190–210 g, were obtained from the animal house of the Faculty of Medicine, Assiut University, Egypt. The rats were maintained on a 12 h dark/light cycle at 24 ± 2 °C with free access to food and water ad libitum. Experimental procedure was conducted in accordance with the ethical standards and was approved by the Animal Ethics Committee, Faculty of Medicine, Assiut University, Egypt. Ethics Committee, approval No. (AUN/MED/20/123).
2.3. Induction of ulcerative colitis
Animals were starved for at least 24 hours prior to colitis induction, with free access to tap water. The water was held two hours before the procedure on the day of the experiment, then anaesthetized with ketamine (100 mg/kg, i.p.). Ulcerative colitis was induced by administering 2 ml of acetic acid (AA) (3% v/v in saline) by intrarectal route using an elastic catheter (outer diameter of 2 mm) under ketamine anesthesia. The catheter was inserted up to 8 cm rectally in the colon, then rats were kept in a straight position for two min to prevent the outflow of AA. Then to spread the AA totally in the colon, 2 ml of air were injected before removing the catheter. Using the same methods, control rats were given 2 ml of saline instead of acetic acid [25].
2.4. Experimental protocol
Forty rats were randomly allocated into four groups (10 rats per group). Group 1: Control group received the vehicle only (The same volume saline instead of AA and the vehicle was delivered only once a day for seven consecutive days). Group 2: (UMB) received UMB suspended in 0.5 % carboxymethyl cellulose (CMC) at a dose of (30 mg/kg/day, orally) [26]. once daily for seven days plus the same volume of saline instead of AA solution. Group 3: (AA): UC model (+ve control group) rats were administered the vehicle orally for seven days, and a rectal AA that was given at the end of the 5th day. Group 4: (UMB+AA) received UMB once daily for five days before AA and two days and served as UMB+AA group.
2.5. Samples preparation
Twenty-four hours after the last treatment, rats were sacrificed under ketamine anesthesia, and blood samples were collected via cardiac puncture. Blood samples were subjected to centrifugation for obtaining the sera. Sera were stored at −20 °C for determination of TNF-α and IL-6 levels using ELISA. The 8 cm distal colon portions of each rat were removed and longitudinally opened, cleaned with cold saline and observed for macroscopic colitis assessment, then cut into three small pieces. One part of the colon was used for histopathological examination and the determination of NF-κB-p65, iNOS, TLR4, PPARγ, and SIRT1 proteins expression using immunohistochemical staining. Another part was used for preparation of 20% (w/v) homogenates and the supernatants used for assays of NO2- content and MPO activity. Additionally, small part of colonic tissue was stored in RNAlater and used for assessment of NF-κB-p65, iNOS, TLR4, PPARγ, and SIRT1 genes using qRT-PCR. Finally, a small part stored in a lysis buffer for western blot analysis of p38MAPK, ERK1, and VCAM-1 proteins.
2.6. Macroscopic scoring:
2.6.1. Evaluation of Disease activity index (DAI):
Evaluation of the clinical severity of colitis was done through calculation of DAI according previously described method with criteria provided in Table 1[27]. It was calculated according to this equation:
2.6.2 Colon mucosal injury score (CMIS):
Furthermore, the percentage of the affected area for which 8 cm of colon area proximal to the anus with criteria provided in Table 2 [28].
2.7. Histopathological study
Histopathological evaluation was done following the method described by Bancroft and Gamble, (2008) [30]. Colon biopsies were fixed with 10% neutral buffer formalin and embedded in paraffin. The specimens were washed, dehydrated by alcohol, cleared in xylene and embedded in paraffin. For histopathological assessment, 3μm thickness sections were cut and stained with hematoxylin and eosin (H&E). Histopathological assessment of specimens was performed by an experienced pathologist blindly under the light microscope to the identity of the tested samples.
2.8. Biochemical assessments
2.8.1. Assessment of serum cytokines; TNF-α and IL-6
Following the manufacturer's instructions and depend on the previously described principles, biochemical estimations of serum TNF-α and IL-6 levels were performed using ELISA kits [31].
2.8.2. Assessment of NO2- content and MPO activity
Determination of NO2- content and MPO enzymatic activity were done by methods described by Tasikas (2007) [32] and Krawisz et al. (1984) [33] respectively.
2.9. Western blot analysis
Colon tissues were homogenized in Tris lysis buffer and protease inhibitor cocktail (Biospes, China) at 4°C for 30 minutes. The residual tissue was discarded by centrifugation at 12000 xg for 10 min at 4 ° C for 10 minutes. The amount of total protein in each sample was measured according to Bradford's method [34]. A total 50 µg of total protein was loaded in each lane and resolved by 10% SDS-polyacrylamide gel electrophoresis at 150 V for 50 minutes. SDS-gel was transferred to a PVDF membrane after the completion of the electrophoresis using semi-dry transfer methods [35]. The membranes were blocked with 5% skimmed milk in TBST buffer at room temperature for 1 hour. The membranes were then incubated at 4 °C with primary antibodies overnight. The membranes were then incubated with the ALP-conjugated secondary antibody for 1 hour. Bands were visualized by BCIP/NBT detection kit. The produced bands were subjected to analysis using image J® software (National Institutes of Health, Bethesda, USA) related to β-actin.
2.10. Immunohistochemical study
For immunohistochemical investigation, multiple consecutive sections were used. Tissue sections were deparaffinized then treated with 3% H2O2 for 10 minutes. Heated in 10 mM citrate buffer at 121 ° C for 30 minutes for antigen retrieval in order to inactivate endogenous peroxidases, then blocked by 5 percent BSA in Tris-buffered saline. Then samples incubation with primary antibodies against NF-κB-p65, iNOS, TLR4, PPARγ, and SIRT1 overnight were done. After incubation with HRP-conjugated secondary antibodies for 30 minutes at room temperature, the slides were washed and stained with DAB staining and hematoxylin counterstaining. It was observed that the positive staining of brown color by light microscopy [36]. Using Image J® software, the percentage of area occupied by brown colour was evaluated and the mean area for each slide was obtained.
2.11. Real-time PCR analysis
Genes expression estimation of NF-κB-p65, iNOS, TLR4, PPARγ, and SIRT1 (Primers sequences were listed in Table (3)) by qRT-PCR. Briefly, Using the Trizol reagent, RNA was extracted from rat colon tissues, and subsequent RNA was transcribed in reverse to cDNA as instructed by the manufacturer. SYBR green was used to assay target genes' expression as previously described [37]. The β-actin is employed as a reference gene. After PCR amplification, according to the method described by Livak and Schmittgen (2001), the data obtained was analyzed to represent a fold change using the 2-ΔΔCT equation [38].
2.12. Statistical Analysis
All data are expressed as mean ± SEM (standard error of the mean). Statistical analysis was performed using the Graph Pad Prism Software Version 6.00 (GraphPad Software, Inc. La Jolla, CA, USA). One-way analysis of variance (ANOVA), followed by Tukey's test, was used to evaluate the statistical significance of differences in each parameter among the different groups, and a P-value of < 0.05 was considered statistically significant.