no products were observed

Insertion of the mgtc gene into the pKSII+ plasmid

Kamil

Tasks:

• Purification of the PCR product
• Plasmid assembly

Methods:

• The purification was carried out using Montage PCR Centrifugal Filter Device P36461 (Milipore) and according to the protocol supplied.

• Plasmid digest mix was prepared as fallows: 2ul Tango buffer (Fermentas), 1ul pKSII plasmid, 1ul XbaI enzyme, 1ul SmaI enzyme, the solution was topped up with H2O to the final volume of 20 ul.
• hly gene digest mix was prepared as fallows: 2ul Tango buffer (Fermentas), 2ul purified gene, 1ul XbaI enzyme, the solution was topped up with H2O to the final volume of 20 ul.
• The digest was kept for 3h at 37°C, and then the enzyme was inactivated for 15min. at 80°C.

• The ligation mix was prepared as follows: 2ul plasmid, 6ul gene, 2ul ligation buffer G (Fermentas), 2ul T4 DNA ligase (Fermentas) , the solution was topped up with H2O to the final volume of 20 ul. The ligation was carried out in 18°C overnight (~12h) and the inactivated for 10min. at 65°C.

• A 200ul batch of chemocompetent bacteria was transformed with 500ul of ligation mix and incubated on petri dishes containing LB medium supplemented with ampicilin, X-gal and IPTG.

Results:

Due to a technological error the bacteria used were electrocompetent rather than chemocompetent. This resulted in there being not a single colony on the petri dishes.