Маркетинговые исследования
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The amplified 5LTR promoter was cloned to the

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 The amplified 5LTR promoter was cloned to the  Empty The amplified 5LTR promoter was cloned to the

Сообщение  qq123456 Пн Дек 14, 2015 10:44 am

The amplified 5LTR promoter was cloned to the ABT-888 臨床試験 pGL3 Luciferase standard vector applying KpnI and Hin dIII sites. The CMV promoter was eliminated from pCDNA3. 1 hygro vector applying MluI and NheI and inserted into the pGL3 Luciferase standard vector together with the exact same restric tion web sites to create the CMV reporter construct. Web page directed mutagenesis on MCT one 3 PCR primer sets had been designed to produce the mutant strands of MCT 1 on Serine 118 residue. The primer set for S118A included the forward primer Following the suppliers protocol for that GeneEditor in vitro internet site directed mutagenesis system, the insertion of wild style MCT 1 constructed on pGEX 5X 1 plasmid was utilised because the mutagenesis tem plate.<br><br> The plasmid DNA was denatured, phosphorylated, annealed together with the mutagenic oligonucleotides, and incu bated with T4 DNA polymerase and T4 DNA ligase at 37 C for 90 min. Mutant plasmids have been transformed into BMH 71 18 mutS competent cells オーダー Afatinib and selected using the GeneEditor antibiotic assortment mix, and subsequently transformed into high efficiency JM109 competent cells followed from the selection of the ampicillin and GeneEditor antibiotic choice mix. For long lasting storage, the mutants had been transformed to the DH5a competent cells. Wild variety MCT 1 cDNA was digested from pLXSN MCT one plasmid by EcoRI XhoI. Stage mutant inserts had been digested from pGEX 5X 1 MCT 1 mutant plasmid by EcoRI and BamHI. Inserts have been amplified by pfu DNA polymerase. PCR goods were digested with HpaI and ClaI just before con structing into pLHCX vector.<br><br> The recombinant plasmids were transformed into OneShot MachI 価格 AG-1478 T1 cells, followed by col ony PCR, enzyme digestion, and sequencing evaluation. Three copies of FLAG Tag was PCR priming from pCMV3Tag8 vector together with the FLAG Tag primer set, i. e. forward primer. The PCR products of 3 copies of Flag Tag was cloned in to the NotI internet site of pLHCX MCT one plasmid. MOCK control and FLAG tagged pLHCX MCT 1 plasmids were individually transfected into PT67 packaging cell line using a Lipofectamine agent. Transfectants were picked by a hundred ugml hygro mycin. The viral supernatants were collected in the hygromycin no cost medium after which infected MCF 10A cells. Luciferase activity assay To analyze the luciferase activity, 0. five ug reporter plas mid, 0.<br><br> one ug b galactosidase plasmid, and one ul JetPEI reagent have been mixed with 75 mM NaCl solution for 30 min just before transfection into H1299 or MCF 10A cells. After 48 h, the cells have been washed with 1X PBS and incubated with 200 ul lysis buffer for 30 min at 80 C. Cell extracts have been extra into 96 properly microtiter plates and mixed with thirty ul luciferase assay reagent. The reaction was detected that has a Hidex Chameleon machine, then analyzed with Mikro Win2000 soft ware. To analyze b galactosidase activity, thirty ul lysates have been incubated with 22 ul 1X ONPG, 47 mM sodium phosphate, and 1 mM MgCl2 answer. Reactions have been incubated at 37 C for 10 min and measured together with the spectrophotometer at OD 420 nm. Chromatin immunoprecipitation assay ChIP experiments have been performed in accordance towards the man ufacturers protocol.

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