Two millilitres of CMC overlay were added to each well Plates we

Two millilitres of CMC overlay were added to each well. Plates were incubated at 37°C in a humidified 5% CO2 incubator for 48 hours. After that, CMC overlay

was aspirated and cells were washed with PBS. Plaques were visualized by staining with crystal violet. Entry assay To determine HSV-1 entry, confluent monolayers of HOG cells plated in 96-well tissue culture dishes were infected with serial dilutions of recombinant HSV-1 (KOS) gL86, which expresses β-galactosidase upon entry into cells. After 6 h p.i., β-galactosidase assays were performed using a soluble substrate ONPG assay. The enzymatic activity was measured at 410 nm using a Benchmark microplate reader (Bio Rad). HSV-1 resistant CHO-K1 cells were used as control. Real-time Rucaparib research buy quantitative RT-PCR assay Total RNA from triplicate samples of HOG cells cultured in 60-mm dishes under growth or differentiation conditions was extracted using RNeasy Qiagene Mini kit (Qiagen, Valencia, CA, USA). RNA integrity was evaluated on Agilent 2100 Bioanalyzer (Agilent Technologies, Santa Clara, CA). Then, RNA was quantified

in a Nanodrop ND-1000 spectrophotometer (Thermo Fisher Scientific). All the click here samples showed 260/280 ratio values around 2, which correspond to pure RNA. Yield range was between 405 and 639 ng/μl. RNA Integrity Number (RIN) values were between 9.3 and 9.8, corresponding to RNA samples with high integrity. Genomic DNA contamination was assessed by amplification of representative samples without retrotranscriptase (RT). RT reactions were performed using the High Capacity RNA-to-cDNA Master Mix with No-RT Control (Applied Biosystems PN 4390712) following manufacturer’s instructions. Briefly, 1 μg of total RNA from each sample

was combined with 4 μl of master mix (including all necessary reagents among which a mixture of random primers and oligo-dT for priming). RT- controls were obtained by using the No-RT master mix included in the master mix pack. The reaction volume was completed up to 20 μl with DNAse/RNAse free distilled water (Gibco PN 10977). Thermal conditions consisted of the following steps: 5’ × 25°C, this website 30’ × 42°C and 5’ × 85°C. RT- amplifications of the representative samples were either negative or delayed more than 5 cycles compared to the corresponding RT + reactions. Intron-spanning assays were designed using Probe Finder software (Roche Applied Science). Primer sequences were as follows: 5’-AGGCCAGAGAATCCACCTG-3’ (forward), and 5’-GCATCTCTGAAGAACGCTGTC-3’ (reverse). Manufacturer of oligonucleotides was Sigma Aldrich. Oligo design, RT-qPCR and data analysis was performed by the Genomics Core Facility at Centro de Biología Molecular Severo Ochoa (CSIC-UAM). In order to know the most suitable genes for the normalization, the stability of four candidates –β-Actin, GAPDH, 18S and UBQ– were assayed using the NormFinder algorithm. Given its exceptionally high stability, 18S was chosen as the most appropriate.

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