Cytotoxicity was determined through a WST-8 assay (Cell Counting Kit-8, Beyotime, Shanghai, China) [38, 39]. The number of viable cells was then determined by absorbance measured at 450 nm on an automated plate

reader. The potential off-target effects of siRNA were evaluated by monitoring the IFN response. Huh7 cells were transfected with 1 μg of shRNA plasmids. Non-transfected cells treated or untreated with 500 IU of IFNα-2a (Anfulong, Huadali Company, China) for 24 h served as a positive control [40]. Expression profile of four major interferon-stimulated (STAT1, OAS1, GBP1 and MX1) were analyzed by a quantitative RT-realtime PCR using the previously reported primers while the GAPDH level served as a control[41]. Mice Experiments To evaluate the anti-viral effects of siRNA in vivo, an HBV hydrodynamic injection was conducted in BALB/c mice. Briefly, 50 μg Silmitasertib cell line of purified HBV plasmid and 10 μg shRNA plasmids were diluted to 2 mL with physiological saline and then injected into the tail vein within 5-10 s. Mice sera were assayed every day for HBsAg and HBeAg from Day 0 to Day

9. For each group, five mice aging from 4-6 weeks were used [42]. All animals received humane care and the study protocol complied HKI 272 with the institution’s ethics guidelines. Measurement of HBV RNA and DNA For detection of the cytoplasmic HBV RNA, total RNA was extracted from cells using Tripure Isolation Reagent (Roche Applied Science, Switzerland) according to the manufacturer’s instructions. Potential residual DNA contamination of RNA preparations were excluded by DNase I digestion. Ten nanograms of RNA were analysed by AccessQuick realtime RT-PCR buy Bromosporine System (Promega, USA) on a CFX96 instrument (Bio-Rad, USA). The HBV pg/pc (pregenomic/preCore) RNA level was detected by primers PGP (-CACCTCTGCCTAATCATC, nt1826-nt1843) and BC1 (GGAAAGAAGTCAGAAGGCAA, nt1974-nt1955) [43] using probe Rucaparib in vivo CP2 (HEX-ATGTTCATGTCCTACTGTTCAAGCC-BHQ2). The

transcript copy number was normalized to those of GAPDH. For the HBV DNA assay, 100 μL of supernatant was pre-heated at 50°C for 20 minutes and then treated with 1 U DNase I for 2 hours to eliminate residual plasmids. The reaction was terminated by EDTA at a final concentration of 10 mM. The mixture was then incubated at 70°C for 10 min and the HBV DNA was extracted using QIAamp DNA blood kits (QIAGEN, Hilden, Germany). HBV DNA quantification assays were performed using a commercial real-time PCR kit (Kehua, Shanghai, China). Determination of HBV Antigens HBsAg, HBeAg and HBcAg levels were determined by chemiluminescence using commercial assay kits (Wantai, Beijing, China). The relative level of each antigen was expressed as an S/CO (signal/cutoff) value, on a linear range from 1 to 1000 for all three assays. The lower detection limit was 10 pg/mL for the HBsAg and HBeAg assays, and 50 pg/ml for the HBcAg assay.