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Found 5 matching solutions for this experiment
| Upstream tips |
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The microsatellite-enriched cDNA PCR products was digested with SalI and NotI using the following protocol: 20 μl (ca. 500 ng) cleaned cDNA, 3 μl 10 × SalI buffer, 1 μl (20 units) SalI (NEB) and 1 μl (10 units) NotI (NEB) at 37°C for 2 hours. |
After digestion, the cDNA was electrophoresed on 1% low melt gel (BIO-RAD). Fragments between 500 bp and 1200 bp were excised and cleaned using glassmilk (Gen 101). Approximately 50 ng cDNA was ligated to 25 ng pCMV-SPORT-6 vector (Invitrogen) which was used to transform XL-blue supercompetent cells (Stratagene). Schematic presentation of the method for microsatellite enrichment from normalized cDNA is shown in Figure Figure11. |
| Protocol tips |
| The microsatellite-enriched cDNA PCR products was digested with SalI and NotI using the following protocol: 20 μl (ca. 500 ng) cleaned cDNA, 3 μl 10 × SalI buffer, 1 μl (20 units) SalI (NEB) and 1 μl (10 units) NotI (NEB) at 37°C for 2 hours. |
| Downstream tips |
| After digestion, the cDNA was electrophoresed on 1% low melt gel (BIO-RAD). Fragments between 500 bp and 1200 bp were excised and cleaned using glassmilk (Gen 101). Approximately 50 ng cDNA was ligated to 25 ng pCMV-SPORT-6 vector (Invitrogen) which was used to transform XL-blue supercompetent cells (Stratagene). Schematic presentation of the method for microsatellite enrichment from normalized cDNA is shown in Figure Figure11. |
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The thereby assembled complementation cassette was gel-purified, verified by sequencing and further cleaved by EagI-HF (NEB) and SalI-HF (NEB) following manual’s instructions. Analogously, respective pENTRY-miniCR-constructs (see above) were cleaved by the same enzymes, respectively, as a EagI and a SalI restriction site are sequentially located 5 bp upstream of the truncated leader promoter (cf. Fig. 2a). |
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| Protocol tips |
| The thereby assembled complementation cassette was gel-purified, verified by sequencing and further cleaved by EagI-HF (NEB) and SalI-HF (NEB) following manual’s instructions. Analogously, respective pENTRY-miniCR-constructs (see above) were cleaved by the same enzymes, respectively, as a EagI and a SalI restriction site are sequentially located 5 bp upstream of the truncated leader promoter (cf. Fig. 2a). |
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The 3 DNA fragments were digested with 4 kinds of FastDigest restriction enzymes (KpnI, HindIII, BamHI, and SalI) in FastDigest Buffer (Thermo Fisher Scientific, Waltham, MA, USA), and ligated to the KpnI-SalI sites of the pUC19 vector (Takara Bio) to yield a plasmid, pAYA1, carrying the ΔrodZ::hph mutation. |
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| Protocol tips |
| The 3 DNA fragments were digested with 4 kinds of FastDigest restriction enzymes (KpnI, HindIII, BamHI, and SalI) in FastDigest Buffer (Thermo Fisher Scientific, Waltham, MA, USA), and ligated to the KpnI-SalI sites of the pUC19 vector (Takara Bio) to yield a plasmid, pAYA1, carrying the ΔrodZ::hph mutation. |
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The purified PCR products were then digested with NdeI (Promega) and SalI (Promega) at 37°C for 1 h. |
The restriction digests were purified as described above with a Qiagen QIAquick PCR purification kit and eluted in 30 μl ddH2O. |
| Protocol tips |
| The purified PCR products were then digested with NdeI (Promega) and SalI (Promega) at 37°C for 1 h. |
| Downstream tips |
| The restriction digests were purified as described above with a Qiagen QIAquick PCR purification kit and eluted in 30 μl ddH2O. |
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This T2A-NeoR fragment was digested with XhoI (Thermo Scientific), HSVtk fragment was digested with SalI (Thermo Scientific), fragments were ligated and the fragment of predicted length was gel purified again. |
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| Protocol tips |
| This T2A-NeoR fragment was digested with XhoI (Thermo Scientific), HSVtk fragment was digested with SalI (Thermo Scientific), fragments were ligated and the fragment of predicted length was gel purified again. |
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