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上海善然生物科技有限公司
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文献和实验).If you assume the efficiency of the cells is between 107 and 108/µg of DNA,then you need to dilute the plasmid to a concentration of 0.1 ng/µl.Then transform 1 ml (0.1 ng)and plate both high (90% of the transformation)and low (10% of the transformation
for every experiment (Bluescript is a nice control because it will turn blue on xgal/IPTG plates).If you assume the efficiency of the cells is between 107 and 108/µg of DNA,then you need to dilute the plasmid to a concentration of 0.1 ng/µl.Then transform 1 ml (0.1 ng
GTPγS-induced Inhibition of Binding
GTPγS-induced Inhibition of Binding 1. Chemicals and Equipment DB Buffer, PB, cAMP, cAMP [2, 8- 3H] (25 Ci/mmol, 1.0 mCi/ml, 32, 000 nM), 10 mM GTPγS, Wacker silicone AR-20, Reagiergefab test tubes (Sarstedt), millipore
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