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Ligation high Ver.2 - Toyobo

Ligation high Ver.2 - Toyobo

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www.toyobo.co.jp/e/bioExample 5.TA Cloning using unpurified PCR productsT vector,(50 ng, 25 fmol)was mixed, at different ratios, with unpurified PCR products(500 bp from Taq DNA polymerase). An equal volume of <strong>Ligation</strong> <strong>high</strong> <strong>Ver.2</strong>, 7.5 μl, wasadded and incubated at 16℃ for 30 min. E. coli DH5α competent cells weretransformed using 10 μl of reaction mixture, and cultured on LB/Amp (X-Gal) platesO/N.Relative colony number1201008060402002 1 0.5BlueWhiteAmount of the added PCR products(μl)Fig. 7 TA cloning using unpurified productsColony number on the condition of adding 0.5 μl of the PCR product corresponds to 100.Example 6.Phage vector ligationλZAP ® II (500 ng), EcoRI digested, and pRheo/EcoRI test insert(225 ng, 2.8 kb), weremixed with half or with an equal volume of <strong>Ligation</strong> <strong>high</strong> <strong>Ver.2</strong>, 3.75 or 7.5 μl, andincubated at 16℃ for 30 min. in vitro packaging was performed with 1.5 μl ligationreaction using GIGAPACK ® III(Stratagene) followed by infection of E. coli XL-1 BlueMRF’. The E. coli cells were cultured O/N and plaques counted.Table 2. Reaction conditions and efficiencyDNA soln:<strong>Ligation</strong> reagent1 : 0.5 1 : 1Efficiency6.3×10 6 5.5×10 6(pfu/μg ZAP ® II)*λZAP ® and GIGAPACK ® are registered trademarks of STRATAGENE.JAPANTOYOBO CO., LTD.Tel(81)-6-6348-3888www.toyobo.co.jp/e/biotech_osaka@toyobo.jpCHINATOYOBO Bio-Technology, CO., LTD.Tel(86)-21-58794900.41405FOR RESEARCH USE ONLY. NOT FOR HUMAN OR DIAGNOSTIC USE.

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