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. 2011 May;85(10):5091–5104. doi: 10.1128/JVI.02565-10

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Fig. 2. — Schematic representation of constructs built and used in this study. Each clone has the same pJL89-derived backbone, where double StuI/SmaI restriction digestion allows insertion of blunt-end PCR fragments derived from RT-PCR of full-length genomic segments between the double 35S promoter (2-35S) and the hepatitis delta virus ribozyme (Rz) followed by a Nos terminator. Arrow directions indicate the orientation of the viral transcripts obtained for each of the described clones. The arrows indicate each ORF encoded by the genome.