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. 2008 Jul 23;82(19):9409–9416. doi: 10.1128/JVI.00428-08

TABLE 2.

Characteristics of the HDV RNA species-specific RT-PCR procedures

Protocol RNA detected RNAs transfected RT primera Reverse transcriptase enzyme Temp of RT reaction (°C) PCR primera (F/R)b Sensitivity Specificityc (discrimination)
mI-S mRNA-I G-RNA and mRNA-I/II Oligo(dT)20 SuperScript III 55 Tagm-T20-F/mI-R 103 6 log10
mI/II-S mRNA-I/II G-RNA and mRNA-I/II Oligo(dT)20 SuperScript III 55 mII-R/mI-F d
G-S G-RNA AG-RNA and mRNA-I/II Tagged GS rTth 70 TagG-F/GS-R 103 5 log10
AG-S AG-RNA G-RNA and mRNA-I/II Tagged AGS rTth 70 TagAG-F/AGS-R 103 5 log10
a

The sequences of the RT-PCR primers are listed in Table 1.

b

F, forward primer; R, reverse primer.

c

The specificity for the mI-S protocol is defined as the log difference between the titer at which the mRNA-I was detectable and the titer at which the G-RNA or AG-RNA generated the first positive signal. The specificity for the G-S protocol is defined as the log difference between the titer at which the G-RNA was detectable and the titer at which the AG-RNA generated the first positive signal. The specificity for AG-S protocol is defined as the log difference between the titer at which the AG-RNA was detectable and the titer at which the G-RNA generated the first positive signal.

d

—, not determined.