pLD-CTB-GAA

Protein Expression Eukaryotic cells - N. benthamiana CTB-GAA

Experiment
Protein Expression Eukaryotic cells - N. benthamiana CTB-GAA
Product
pLD-CTB-GAA from Henry Daniell, Department of Biochemistry, School of Dental Medi
Manufacturer
Henry Daniell, Department of Biochemistry, School of Dental Medi

Protocol tips

Protocol tips
Transformation of tobacco (Nicotiana tabacum cv. Petit Havana) chloroplasts with the expression vector pLD-CTB-GAA and PCR analysis of the transplastomic lines were performed according to the previously published protocols (Verma et al., 2008). The CTB-GAA transplastomic tobacco lines were selected and regenerated on spectinomycin (500 mg/L) selection media.

Publication protocol

Transformation of tobacco (Nicotiana tabacum cv. Petit Havana) chloroplasts with the expression vector pLD-CTB-GAA and PCR analysis of the transplastomic lines were performed according to the previously published protocols (Verma et al., 2008). The CTB-GAA transplastomic tobacco lines were selected and regenerated on spectinomycin (500 mg/L) selection media. Site-specific integration of the transgenes including the aadA selection cassette and the CTB-GAA expression cassette was first confirmed by PCR analysis with two primer sets 3P/3M and 5P/2M (Verma et al., 2008). The 3rd primer pair CTB-Fw (5′-CA TATGACACCTCAAAATATTACTGATT-3′) and GAA-Rv (the same primer used for overlap extension PCR) was also used to identify the integration of CTB-GAA expression cassette. Southern blot analysis was carried out essentially as described by Kumar and Daniell (2004). Total tobacco DNA (1 μg) was digested with AflIII, separated on a 0.8% agarose gel and then transferred to a nylon membrane. A 0.81-kb DNA probe was isolated from pUC-CT plasmid with BamHI and BglII digestion and labeled with 32P. After labeling, membrane hybridization was carried out by following the QUICK-HYB hybridization protocol (Stratagene, La Jolla, CA).

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