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Found 3 matching solutions for this experiment
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Using the same primers and thermal cycling conditions described above, genotyping of g.52734272 in unrelated ABDs and other breeds was carried out through a restriction enzyme digest with 5 µL PCR product and either BfaI CutSmart (New England Biolabs, Ipswich, MA, USA) or FspBI FastDigest (Thermo Scientific) for total reaction volumes of 25 and 15 µL, respectively. BfaI (FspBI) recognizes and cleaves (^) the following sequence: 5′-C^TAG-3′. Digests were visualized on a 1.2 % agarose gel, where wild-type alleles are uncut (489 bp) and mutant alleles are cut once (248 and 241 bp). |
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Protocol tips |
Using the same primers and thermal cycling conditions described above, genotyping of g.52734272 in unrelated ABDs and other breeds was carried out through a restriction enzyme digest with 5 µL PCR product and either BfaI CutSmart (New England Biolabs, Ipswich, MA, USA) or FspBI FastDigest (Thermo Scientific) for total reaction volumes of 25 and 15 µL, respectively. BfaI (FspBI) recognizes and cleaves (^) the following sequence: 5′-C^TAG-3′. Digests were visualized on a 1.2 % agarose gel, where wild-type alleles are uncut (489 bp) and mutant alleles are cut once (248 and 241 bp). |
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Restriction digestion of 1 μg of custom-designed DNA was carried out at 37°C for 4 h using 30U AluI, 80U BfaI, 30U HaeIII, 15U HpyCH4V, 10U MluCI, 10U MseI, and 10U MspI. Restriction products were size separated in 2% agarose. |
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Protocol tips |
Restriction digestion of 1 μg of custom-designed DNA was carried out at 37°C for 4 h using 30U AluI, 80U BfaI, 30U HaeIII, 15U HpyCH4V, 10U MluCI, 10U MseI, and 10U MspI. Restriction products were size separated in 2% agarose. |
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Protocol tips |
Downstream tips |
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The restriction enzymes RsaI and FspBI (Fermentas, York, UK) discriminated the respective genotypes. |
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Protocol tips |
The restriction enzymes RsaI and FspBI (Fermentas, York, UK) discriminated the respective genotypes. |
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