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_6
Snippet: The next key step is the cloning and modification of a partial-or full-length JEV cDNA in BAC, which is a relatively straightforward procedure that uses standard recombinant DNA techniques. 69 Figure 3 presents a representative outcome for the purification of the BAC clone containing a fulllength cDNA of JEV SA 14 -14-2 by banding in a CsCl-EtBr gradient. In this experiment, after centrifugation for 16 hr at 401,700 × g, two distinct bands, i.e......
Document: The next key step is the cloning and modification of a partial-or full-length JEV cDNA in BAC, which is a relatively straightforward procedure that uses standard recombinant DNA techniques. 69 Figure 3 presents a representative outcome for the purification of the BAC clone containing a fulllength cDNA of JEV SA 14 -14-2 by banding in a CsCl-EtBr gradient. In this experiment, after centrifugation for 16 hr at 401,700 × g, two distinct bands, i.e., the E. coli chromosomal DNA above and the supercoiled BAC plasmid DNA below, are visible in the middle of the tube under longwave ultraviolet light. A minimal volume (~400 µl) of the lower BAC DNA band was carefully collected by poking a hole with a syringe on the side of the tube. Subsequently, the EtBr was extracted from the BAC DNA by butanol extraction, and the EtBr-free BAC DNA was concentrated by ethanol precipitation.
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