quantitative RT PCR. Viral RNA was e tracted from each sample of the viral preparations using the QIAamp Viral RNA Mini Kit. The e tracted RNA, along with a known amount of standard this website HAstV1 RNA, was reverse transcribed into cDNA using the Superscript III system with oligo dT as the primer. For quantitating the copy number of the viral genome, cDNA was amplified using viral cDNA Inhibitors,Modulators,Libraries specific primers, S3988 4008 and AS4193 4171 with the Thunderbird q PCR Kit. Amplification proceeded through 40 cycles of denaturation at 94 C for 15 s, annealing at 62 C for 20 s, and e tension at 72 C for 20 s in either a LightCycler 2. 0 or a CF 96. The cDNA copy number, derived from the fluorescence signals of the amplification products, was then converted into particle number.
Standard HAstV1 RNA was prepared by in vitro tran scription Inhibitors,Modulators,Libraries using a T7 RiboMa E press Large Scale RNA Production System and the template DNA pAVIC V, which harbors a molecular clone of HAstV1. Infectious titer was determined using the method de scribed by Mendez et al. In our study, infection with 100 particles per Caco 2 cell yielded appro imately 20% Inhibitors,Modulators,Libraries of the cells positive for anti HAstV1 antibody at 24 hpi. From this value, the multiplicity of infection was calculated to be appro imately 0. 22. Infection and drug treatment Prior to infection, confluent Caco 2 cells maintained in EMEM were washed with PBS thrice and starved of serum for 1 h by incubation in EMEM supplemented with sodium pyruvate, non essential amino acids, and 20 mM HEPES.
Inhibitors,Modulators,Libraries HAstV1 stock was pretreated with 10 ug mL trypsin IV for 15 min at 37 C, and then applied to the cells along with trypsin at appro imately 100 particles per cell. The mi ture was then incubated for 1 h at 4 C, which was intended to allow the virus to bind the cells, but not proceed further in the entry process. We noted that this procedure has been described in Moser and Schulz Cherry and that incubation at 4 C for 1 h did not substantially alter the infectious events seen when incu bating at 37 C, judged by the number of cells positive for viral antigen after staining with mouse anti HAstV1 antibody. After removal of the cul ture medium and washing with EMEM, incubation Batimastat of the cells was continued in EMEM supplemented with 10 ug mL trypsin IV until the time of harvest. For e periments involving pharmacological inhibitors, the infection of Caco 2 cells was carried out in the presence of a specified drug for a designated time period.
Genistein, U0126, JNK inhibitor II, H 89, Akt inhibi tor V, and Y 27632 were high throughput screening purchased from Merck. Wortmannin and staurosporine were from Sigma Aldrich. SB203580 and LY294002 were obtained from Promega. NSC23766 and MK 2206 were from Santa Cruz Biotechnology and Selleckchem, respectively. All drugs were sol ubilized in dimethyl sulfo ide. Initial drug con centrations were selected after consulting the following references staurosporine, genistein, U0126, SB205830, JNK inhibitor II, LY294003, wortmannin, triciribine, MK 2206, NSC237