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Found 3 matching solutions for this experiment
Upstream tips |
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Typically, mtTEC DNA was digested by incubating mtTECs (5 mg of protein) with 5–20 U of appropriate restriction enzyme in a final volume of 30 μL for 30 min at 30°C as follows: 20 U of HhaI (NEB), 5 or 20 U of AvaII (NEB), 20 U of NspI (NEB), 5 U of RcaI (Roche), 5 U of XhoI, 5 U of XhoII, 5 U of PstI (NEB), 20 U of MspI (Roche), and 10 U of SacII (NEB). |
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Protocol tips |
Typically, mtTEC DNA was digested by incubating mtTECs (5 mg of protein) with 5–20 U of appropriate restriction enzyme in a final volume of 30 μL for 30 min at 30°C as follows: 20 U of HhaI (NEB), 5 or 20 U of AvaII (NEB), 20 U of NspI (NEB), 5 U of RcaI (Roche), 5 U of XhoI, 5 U of XhoII, 5 U of PstI (NEB), 20 U of MspI (Roche), and 10 U of SacII (NEB). |
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The purified DNA sample was treated in a 2-step reaction with a set of MREs in cocktail as RE1, including Cfr42I (SacII), PdiI (NaeI), Eco52I (EagI) and PteI (BssHII)(FastDigest enzyme from Thermal Scientific Inc.), called 4E collectively. |
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Protocol tips |
The purified DNA sample was treated in a 2-step reaction with a set of MREs in cocktail as RE1, including Cfr42I (SacII), PdiI (NaeI), Eco52I (EagI) and PteI (BssHII)(FastDigest enzyme from Thermal Scientific Inc.), called 4E collectively. |
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The pMD18-T-2B plasmid was digested with SacII (TaKaRa) and PacI (NEB), and 2B was inserted into the pGBHCupp-2A MCS site via the same restriction enzyme digestion and ligated to create the plasmid pGBHCupp-2A2B. |
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Protocol tips |
The pMD18-T-2B plasmid was digested with SacII (TaKaRa) and PacI (NEB), and 2B was inserted into the pGBHCupp-2A MCS site via the same restriction enzyme digestion and ligated to create the plasmid pGBHCupp-2A2B. |
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