DEN was obtained as 1 g solution in serum bottle diluted in 0.9% NaCl. 2-AAF was obtained as white powder, while cyan was obtained as black powder. Both 2-AAF and cyan were dissolved in 0.9% NaCl. All chemicals were purchased from Sigma-Aldrich, Cairo, Egypt.

All animal procedures were approved by the Institutional Animal Ethics Committee of Ain Shams University, Faculty of Medicine. Thirty male Wistar rats weighing 200-250 g were purchased from Nile Pharmaceuticals Company (Cairo, Egypt). Animals were housed in an animal room with temperature 25 ± 2 °C and 12 h light/dark cycle controls. An adaptation period of 1 wk was allowed before initiation of the experimental protocol.

Induction of hepatic PCL: DEN was injected intraperitoneally (i.p.) at a dose of 100 mg/kg once weekly for three consecutive weeks. One week after the last DEN injection, a single dose (300 mg/kg) of 2-AAF was injected.

Animal groups: Rats were divided into five groups (6 rats/each group), including: Naïve group: Rats were injected with a vehicle (0.9% NaCl), PCL group: Rats were injected with DEN and 2-AAF, and three cyan groups (cyan-10, cyan-15, and cyan-20 groups): Rats were injected with DEN and 2-AAF, and orally administered through gastric gavage with cyan in doses of 10, 15, and 20 mg/kg respectively, for four consecutive days per week for 16 wk[17].

Biochemical and molecular studies: After scarifying the animals, blood was withdrawn from each rat from the retro orbital vein and incubated for about half an hour for clotting. Then, the blood sample was centrifuged for 20 min at 5000 RPM to get serum samples. Livers were dissected. The right lobe of the livers was removed, cut into longitudinal sections 2-4 mm in thickness and kept in 10% formalin for histopathological and immunohistochemical examination. The other lobe was kept frozen at -80 °C for molecular analyses. The samples were analyzed for the following parameters: (1) alpha fetoprotein (AFP) levels: AFP level was analyzed using quantitative sandwich rat AFP ELISA kit purchased from MyBiosource Inc. (San Diego, United States) with a sensitivity range of 0.625-20 ng/mL; (2) serum alanine aminotransferase (ALT) levels: The serum ALT was measured according to method described by using kits purchased from Diamond Diagnostic (Cairo, Egypt). ALT catalyzes the transfer of amino groups from specific amino acids to ketoglutaric acid, yielding glutamic acid and oxaloacetic or pyruvic acid, respectively. Ketoacids were then determined calorimetrically after their reaction with 2, 4- dinitrophenylhydrazine; and (3) determination of serum total bilirubin and direct bilirubin: Alkaline methanolysis of bilirubin followed by chloroform extraction of bilirubin methyl esters, and later, separation of these esters by chromatography and spectrophotometric determination at 430 nm.

Quantitative determination of serum albumin level was quantified using rat albumin ELISA kit. The absorbance at 450 nm is a measure of the concentration of albumin in the test sample.

The RNA panel was chosen in three steps: (1) Tubulin, gamma 1 (TUBG1) was retrieved as a crucial player in microtubule formation and progression of the cell cycle through gene atlas expression database (available at https://www.ebi.ac.uk/gxa/home) alongside with verification of the chosen gene from protein Atlas database (available at https://www.proteinatlas.org/), followed by analysis of TUBG1 gene ontology to ensure that it is linked to G2-M transition and mitotic spindle assembly, which is closely linked to cancer development through gene card database (available at https://www.genecards.org/); (2) we selected miR-125b-1-3p targeting TUBG1 mRNA though) miRWALK database available at http://mirwalk.umm.uni-heidelberg.de/), followed by pathway enrichment, which revealed that miR-125b-1-3p is linked to MAP kinase and ubiquitin-mediated proteolysis (strongly correlated with mitotic assembly and cell cycle progression) through (Diana database available at http://diana.imis.athena-innovation.gr/DianaTools/index.php); and (3) lncRNA metastasis-associated lung adenocarcinoma transcript 1, lncRNA MALAT1, was obtained as a lncRNA specific to HCC and targeting miR-125b-1-3p using noncode database available at http://www.noncode.org/ and European Bioinformatics institute database available at https://www.ebi.ac.uk.

Total RNA was extracted from liver tissues using miRNeasy Mini kit (Cat No. 217004, Qiagen, United States) according to manufacturer’s protocol. The extracted RNA concentration and integrity were assessed using [(NanoDrop Technologies/Thermo Scientific, Wilmington, DE, United States)], with RNA purities were 1.8-2. The extracted total RNA was reverse transcribed into cDNA using a miScript II RT kit (Cat No. 218160, 218161, Qiagen, United States) on thermal cycler (Bio-Rad; Hercules, CA, United States), according to the manufacturer’s protocol.

The relative expression of TUBG1 mRNA and lncRNA-MALAT1 in liver tissue were measured using a Quantitect SYBR Green Master Mix kit and an RT2 SYBR Green ROX real time-polymerase chain reaction (qPCR) Mastermix (Qiagen), respectively, using a 7500 qPCR Systems (Applied Biosystems, Foster City, CA, United States) detection system) and specific primers (Accession: NM_001128148, NM_003234, NR_002819, and ENST00000534336, respectively) supplied by Qiagen. GAPDH (Accession NM_002046.7) was used as a housekeeping gene. MiR-3163 expression in liver tissue was quantified by PCR using a miScript SYBR Green kit (Qiagen), a miScript universal primer, and a miRNA-specific forward primer (mir-125b-1-3p miScript Primer Assay) (Accession: MIMAT0004592 (5'-ACGGGUUAGGCUCUUGGGAGCU). All steps followed the manufacturer’s suggested protocol, and SNORD68 was used as an internal control. Ct values more than 36 were considered as negative. The specificities of the amplicons for the SYBR Green−based PCR amplification were affirmed by the melting curves. The 2^−ΔΔCt technique was used to measure the relative expression of the HCC-specific RNA panel.

Liver sections were cut at 5-μm thickness and stained with H&E. Immunohistochemistry S-P method was used to detect GSTP and PCNA levels. Briefly, the protocol was as follows: (1) the tissues were treated with endogenous peroxidase blocking solution at room temperature for 10 min, and then, incubated in normal nonimmune serum at room temperature for 10 min; (2) mouse anti GSTP or PCNA antibody was added to adjacent tissue sections respectively and incubated overnight at 4 °C; (3) biotin-conjugated second antibody was added to the sections and incubated at room temperature for 10 min; and (4) S-P complex was added at room temperature for 10 min, and then, 2,4-diaminobutyric acid was used for the color reaction. The tissue sections were washed with Poly (butylene succinate) (PBS) (0.01 mol/L, pH 7.4) between each step. Positive and negative controls were simultaneously used to ensure specificity and reliability of the staining process. A positive section was taken as positive control. In negative control, PBS was used to replace the first antibody. GSTP-positivity was indicated by brown coloration of the cytoplasm. Morphometric analysis of the foci percent area was carried out using Leica Q win V.3 software after capturing the images using a Leica DM2500 microscope (Leica, Wetzlar, Germany). The PCNA labeling indices are represented as the expression of positively-stained nuclei (10 fields/slide at 400 ×) as shown below: +, positive expression found in 1-3 fields; ++, positive expression found in 4-6 fields; and +++, positive expression found in 7-10 fields. Rabbit monoclonal PCNA and GSTP antibodies were purchased from Abcam (San Francisco, United States).

All results were expressed as mean ± SD. Statistical analysis was carried out using GraphPad Prism version 6.01. Unpaired t-test was done to compare between naïve and PCL groups. One-way ANOVA, followed by Tukey’s test, was carried out to compare between all groups. P values < 0.05 were considered statistically significant.

As shown in Figure 1, following induction of PCL, rats exhibited a significant increase in AFP levels. AFP levels were significantly decreased in cyan-10, cyan-15, and cyan-20 groups compared to PCL group. There was no significant difference between the AFP levels of the three cyan groups. Liver function tests were affected after receiving DEN/2-AAF in which rats exhibited a significant increase in levels of ALT and total and direct bilirubin, and a significant decrease in the serum albumin (Figure 2). As shown in Figure 2A, rats received cyan. in different doses exhibited a significant decrease in serum ALT compared to PCL group. Cyan-15 group showed significant decrease in serum ALT compared to cyan-10 group. Moreover, cyan-20 group showed significant decrease in serum ALT compared to cyan-10 group. In As depicted in Figure 2B, compared to PCL group, the rats in the three cyan groups exhibited a significant decrease in serum total bilirubin. Furthermore, cyan-20 group showed significant decrease in serum total bilirubin compared to cyan-10 group. Figure 2C: Serum direct bilirubin was significantly decreased in the three cyan groups compared to the PCL group. Moreover, cyan-20 group showed significant decrease in serum direct bilirubin compared to cyan-10 group. Administration of cyan in doses 5, 10 and 20 mg/kg/d produced a significant increase in serum albumin compared to PCL group. However, there was no significant difference between the serum albumin levels of the three cyan groups (Figure 2D).

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Figure 1 Effect of cyanidin 3-glucoside at different doses (10, 15 and 20 mg/kg/d) on alpha fetoprotein in the serum of rats. Values are mean ± SEM; number of animals = 6 rats/each group. ^aP < 0.05 significant differences compared to naïve group, unpaired t test; ^bP < 0.05 significant differences compared to precancerous lesion group. PCL: Precancerous lesion; Cyan: Cyanidin-3-O-glucoside; AFP: Alpha fetoprotein.

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Figure 2 Effect of cyanidin 3-glucoside at different doses (10, 15 and 20 mg/kg/d) in rats. A: Alanine aminotransferase; B: Total bilirubin; C: Direct bilirubin; D: Serum albumin. Values are mean ± SEM; number of animals = 6 rats/each group. ^bP < 0.05 significant differences compared to precancerous lesion group; ^cP < 0.05 significant differences between the 2 selected groups, One-way ANOVA followed by Tukey’s test. PCL: Precancerous lesion; Cyan: Cyanidin-3-O-glucoside; ALT: Alanine aminotransferase.

As shown in Figure 3, induction of PCL resulted in significant increase of lncRNA MALAT a significant decrease in RQ miR-125b and significant increase in RQ TUBG1 expressions in comparison to naïve group. RQ of lncRNA MALAT1 in the liver tissue was significantly decreased in cyan -10,15 and cyan-20 groups compared to PCL group. Furthermore, cyan-20 group showed significant decrease in RQ of lncRNA MALAT1 in the liver tissue compared to cyan-10 group (Figure 3A). On the contrary, RQ of miR-125b in the liver tissue was significantly increased in cyan -10, cyan-15 and cyan-20 groups compared to PCL group. In addition, cyan-20 group showed significant increase in RQ of miR-125b in the liver tissue compared to cyan-10 group (Figure 3B). Furthermore, RQ of TUBG1 in the liver tissue was significantly decreased in cyan-10, cyan-15 and cyan-20 groups compared to PCL group. Also, cyan-20 group showed significant decrease in RQ of TUBG1 in the liver tissue compared to cyan-10 group (Figure 3C).

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Figure 3 Effect on expression of of long non-coding RNA, MALAT1, miR-125b and tubulin 1 (G2/M transition of mitotic cell cycle) in the liver tissue. A: RQ of long non-coding RNA MALAT1; B: RQ miR-125b; C: RQ TUBGI . Values are mean ± SEM; number of animals = 6 rats/each group. ^aP < 0.05 significant differences compared to naïve group; ^bP < 0.05 significant differences compared to precancerous lesion group; ^cP < 0.05 significant differences between the 2 selected groups, One-way ANOVA followed by Tukey’s test. PCL: Precancerous lesion; Cyan: Cyanidin-3-O-glucoside; TUBG: Tubulin gamma 1; lncRNA: Long non-coding RNA.

Light microscopic examination of H&E-stained sections of naïve rats’ liver showed normal hepatic architecture, cords of hepatocytes radiating from central vein, portal triads present in between, polygonal hepatocytes with centrally rounded vesicular nuclei, and hepatic sinusoid in between (Figure 4A and B). Liver sections obtained from rats received DEN/2-AAF (Figure 4C-E) showed disruption of normal hepatic lobular architecture along with presence of large, discriminated dysplastic nodules compressing the surrounding liver tissue, with high-grade dysplastic cells displaying increased nuclear: Cytoplasmatic ratio (Figure 4E), nuclear hyperchromatosis, and basophilic cytoplasm. Liver sections of rats treated with different doses of cyanidin (10, 15, and 20 mg/kg) respectively, showed small and less discriminated dysplastic nodules (Figure 4F-H).

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Figure 4 Photomicrographs of liver sections stained with H&E staining. A and B: Naïve group liver sections showed normal hepatic architecture, cords of hepatocytes radiating from central vein and portal triads present in-between and polygonal hepatocytes with central rounded vesicular nuclei, and hepatic sinusoid in-between; C-E: Liver sections of rats received diethylnitrosamine/2-acetylaminofluorene (DEN/2-AAF) showed larger, discriminated dysplastic nodules (doted shapes) compressing the surrounding liver tissue with disruption of normal hepatic lobular architecture; D: Liver sections of rats received DEN/2-AAF showed eosinophilic foci of cellular alteration consisting of enlarged hepatocytes with increased acidophilic staining and vaculated nuclei (arrow head); E: Liver sections of rats received DEN/2-AAF showed foci of Clear cell formed of hepatocytes showing variable degrees of cytoplasmic vacuolations and ballooning with pyknotic nuclei (arrow); F-H: Liver sections of rats treated with different doses of cyanidin (10, 15, 20 mg/kg) respectively, showing small and less discriminated dysplastic nodules (doted shapes). (Magnification: A, C, F, G, H × 1000; B, D, E × 400). CV: Central vein; PV: Portal vein; Pt: Portal triads; S: Sinusoid; H: Hepatocytes.

Immunohistochemical examination with GSTP antibody appeared as large hyperplastic nodules were demonstrated by the brown color. Figure 5A and B shows the liver sections of naïve group, while Figure 5C shows large-positively stained GSTP foci demonstrated in PCL group. Liver sections from rats of all cyan-treated groups exhibited small GSTP-positive small hepatic foci of different sizes scattered in-between negatively-stained hepatic parenchyma (Figure 5D-F). The percent area of GSTP foci was significantly increased in the PCL group compared to naïve group, while all cyan-treated groups showed significant decrease in the GSTP percent area. Furthermore, cyan-15 and -20 showed significant decrease in the GSTP percent area over cyan-10 (Table 1). PCNA immunohistochemical analysis showed an elevated expression of PCNA in the group that received DEN/2-AAF as compared to naïve group (Figure 6A and B). Liver sections obtained from rats received cyan. in its three doses showed decrease in PCNA-positively stained nuclei (Figure 6C-E and Table 1).

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Figure 5 Photomicrographs of liver sections of rats immunohistochemical stained with glutathione S-transferase placental antibody. A and B: Naive group; C: Precancerous lesion group showing multiple glutathione S-transferase placental (GSTP)-positive large hepatic nodules (brown stained nodules) occupying most of section; D-F: Liver sections of rats treated with different doses of cyanidin (10, 15, 20 mg/kg) showing GSTP positive small hepatic foci (brown stained cells = arrow) of different size scattered in-between negatively stained hepatic parenchyma. (Magnification: × 40)

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Figure 6 Photomicrographs of liver sections Immunohistochemical stained with proliferating cell nuclear antigen. A: Negative reaction of control group; B: Diethylnitrosamine + 100 mg 2-acetylaminofluorene group showing positive stained nuclei scattered all over the field; C-E: Liver sections of rats treated with different doses of cyamidine (10, 15, 20 mg/kg) respectively, show few positive hepatocytes sporadically distributed over the field (arrow). (Magnification × 100).

Several regulatory RNA networks are important in regulation of liver cell cycle progression.

Cyanidin-3-glucoside (cyan) is a potential chemotherapeutic and chemo-protective agent.

The present study aimed to investigate the effect of cyan administration on cell cycle in hepatic precancerous lesion induced by diethylnitrosamine/2-acetylaminofluorene in Wistar rats.

We used bioinformatic analysis followed by experimental validation.

Cyan dose dependently decreased the long non-coding RNA-MALAT1 and tubulin gamma 1 mRNA expressions and increased the hsa-miR-125b expression which participate in cell cycle and mitotic spindle assembly. Cyan administration decreased alpha-fetoprotein and improved liver function. Cyan decreased glutathione S-transferase placental foci percent area and proliferating cell nuclear antigen positively stained nuclei.

Cyanidin may offer a natural molecule to unravel the mystery a cytotoxic pharmacy for the future.

Further larger in vitro and in vivo studies are needed to elucidate the mechanism of cyanidin cytotoxicity in hepatocellular carcinoma.