Author: Yun, Sang-Im; Song, Byung-Hak; Kim, Jin-Kyoung; Lee, Young-Min
Title: Bacterial Artificial Chromosomes: A Functional Genomics Tool for the Study of Positive-strand RNA Viruses Document date: 2015_12_29
ID: 2se4d1yp_5
Snippet: Step 4, modification of the cloned cDNAs for in vitro run-off transcription with SP6 RNA polymerase, i.e., placing an SP6 promoter sequence immediately upstream of the viral 5'-end (pBAC/F1 Step 5, assembly of a full-length SA 14 -14-2 cDNA BAC, pBAC/SA 14 -14-2 ( Figure 1E) . Table 1 lists the oligonucleotides used in this cloning procedure. 28 For the construction of a functional JEV cDNA, the first important step is the synthesis of the four o.....
Document: Step 4, modification of the cloned cDNAs for in vitro run-off transcription with SP6 RNA polymerase, i.e., placing an SP6 promoter sequence immediately upstream of the viral 5'-end (pBAC/F1 Step 5, assembly of a full-length SA 14 -14-2 cDNA BAC, pBAC/SA 14 -14-2 ( Figure 1E) . Table 1 lists the oligonucleotides used in this cloning procedure. 28 For the construction of a functional JEV cDNA, the first important step is the synthesis of the four overlapping cDNA fragments using the purified viral RNA as a template for RT-PCR. Figure 2 provides a representative result for the four RT-PCR products that were electrophoresed on a 0.8% agarose gel. This gel demonstrates clearly that a full-length JEV cDNA is amplified into four overlapping cDNA fragments. Occasionally, RT-PCR reactions might yield one or more additional virus-specific or nonspecific products that are mostly smaller than the expected product, because of the nonspecific annealing of primers during cDNA synthesis/amplification. On the other hand, little or no expected RT-PCR product would be amplified because of accidental RNase contamination during the viral RNA isolation or improper RT-PCR performance.
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