Fig. 1

a Representative PCR profiles following electrophoresis on 1.5% agarose gel and staining with ethidium bromide, showing polymorphism among the Bacillus thuringiensis isolates. DNA amplification was performed using was carried out using repetitive extragenic palindromic PCR (rep-PCR) with primers ERIC (enterobacterial repetitive intergenic consensus), BOX, GTG (GTG₅) and Bc-Rep (Bacillus cereus-repetitive extragenic palindromic. Lanes M Molecular weight marker (100 bp) ladder, 1–15 B. thuringiensis isolates: 1 VLS64.1, 2 VLS64.2, 3 VLS64.3, 4 VLS64.4, 5 VLS21, 6 VLG15, 7 VLS72.1, 8 VLS72.2, 9 VLS72.3, 10 VRB1, 11 VL4b(i), 12 VL4b(ii), 13 VL126, 14 VL2d, 15 VL4C. b Unweighted pair grouping method with arithmetic mean dendrogram (UPGMA) resulting from rep-PCR patterns showing the genomic diversity among the 15 nodule endophytic B. thuringiensis isolates