5 mM MgSO4, 1.4 mM of dNTP mix, 20 mM Tris-HCl (pH 8.8), 10 mM KCl, 10 mM (NH4)2SO4, 0.1% Triton X-100 and 1.6 M betaine, in a final volume of 25 μL containing the template. This mixture was incubated
at 65°C for 30 minutes. Table 5 Sequences of primers used for CBC-LAMP assay Primer Name Type Sequence (5′-3′) Length XCC-F3 F3 GGTGGATCTACGCACGC 17 mer XCC-B3 B3 GCTGCGATCATGTCCTGAT 19 mer XCC-FIP FIP (F1c+F2) GGTGCTGCGCCACTGTCGAA – GCTACAGCCAGCAGCAACA 39 mer XCC-BIP BIP (B1c+B2) GCACTGGTCGGCCATGGGTA – GCGACGGTCCCTAACG 36 mer XCC-LF LF AACCTTCGGTTTGATCTTCTCC 22 mer XCC-LB LB TTACACACGCGCACATCGT 19 mer Figure 3 Localization of target sequences used for primer construction. Target sequences used for LAMP primer design are underlined and shadowed. The figure shows a portion Selleck Vadimezan of AZD5582 order pthA gene from Xcc 449 nucleotides downstream from the start codon. Analysis of LAMP products The amplified products were subjected to electrophoresis at 100V for 50 minutes on a 1.5% agarose gel, followed by ethidium bromide
staining. To confirm the specificity of the product some bands were cut and Nutlin-3a concentration sequenced (data not shown). The sequences obtained were used as queries to perform BLAST searches [36] in order to confirm identity. Direct analysis of LAMP products For direct analysis of LAMP products, generic LFD strips (Type I BEST™ TCL cassette, Biohelix Co, Beverly, MA, USA) were used. These strips are capable to detect an amplicon that is dual labelled with biotin and fluorescein. For this purpose we used 5′-biotin-labelled XCC-FIP primers and 5′-fluorescein-labelled XCC-BIP
primers in the amplification reactions. The labelled oligonucleotides were purchased from Integrated DNA Technologies™ requesting HPLC purification. After amplification reaction, the reaction tube is inserted in the detection chamber; the dual tagged amplicon is automatically mixed with the detection buffer, and directed by capillary flow to the strip. The amplicon is detected in the test zone (T) of the cassette whereas the control zone (C) serves as a control for the flow function. The complete detection process takes about 10 minutes. More information is available in the manufacturer web site http://www.biohelix.com/products/Type_I_&_Type_II_Cassettes.asp. The inspection for amplification was also performed through observation of colour change after addition of 1 μL of a 1:1000 dilution of SYBRGreen dye to the reaction tube. In the case of positive amplification the original orange color of the dye turns to green which can be examined in daylight. Sensitivity of LAMP In the sensitivity assay from pure DNA, 100 ng of Xcc DNA was 10-fold diluted and used as template for LAMP amplifications.