Cloning and Expression of Cecropin Gene in E.Coli JM109
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Q78

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    Abstract:

    Five 50-70 bp DNA fragments were synthesized first and then proceeding to 3-step PCR amplification using fragment piecing-together method to get the final full sequence. The fragment was cloned into vector PUC19 and then transformed into E. Coli JM109. Re

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LI Qi-hui, LE Guo-wei, SHI Yong-hui, WANG Shu-ying. Cloning and Expression of Cecropin Gene in E. Coli JM109[J]. Journal of Food Science and Biotechnology,2004,23(6).

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