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. 2022 Nov 26;2:100105. doi: 10.1016/j.crpvbd.2022.100105

Table 1.

PCR conditions which differed between the published protocol by Sulaiman et al. (2003) and the modified protocol.

Primer name Primer sequence (5′-3′) Product length (bp) Buffera No. of cycles Annealing T (°C) Total reaction volume (μl) Template DNA per reaction (μl) dNTP (μM)a MgCl2 (mM)a Taq (U) per reaction Primer (nM)a
AL3543 (Outer forward) AAATIATGCCTGCTCGTCG 605 1x 35 50.0 100 0.25–2.00 200 each 3 5 200
AL3546 (Outer reverse) CAAACCTTITCCGCAAACC 200
AL3544 (Inner forward) CCCTTCATCGGIGGTAACTT 530 1x 35 50.0 100 2.50 200 each 3 5 200
AL3545 (Inner reverse) GTGGCCACCACICCCGTGCC 200
AL3543Mod (Outer forward)b AAATYATGCCTGCTCGTCG 605 10x 40 54.2 20 3.00 50 each 15 (incorporated into buffer) 0.5 500
AL3546Mod (Outer reverse)b TGGCCACCACRCCCGTGCC 2000
AL3544Mod (Inner forward)b CAAACCTTYTCYGCAAACC 531 10x 40 57.8 20 3 ​at 1:1000 dilution of first round PCR product 50 each 15 (incorporated into buffer) 0.5 500
AL3545Mod (Inner reverse)b CCCTTCATCGGYGGTAACTT 500

Abbreviation: T, temperature.

a

Concentration.

b

New primers.