| Abstract: | Bacillus thuringiensis has been used as a bioinsecticide to control agricultural insects. Bacillus cereus group genomes were found to have a Bacillus enhancin-like (bel) gene, encoding a peptide with 20 to 30% identity to viral enhancin protein, which can enhance viral infection by degradation of the peritrophic matrix (PM) of the insect midgut. In this study, the bel gene was found to have an activity similar to that of the viral enhancin gene. A bel knockout mutant was constructed by using a plasmid-free B. thuringiensis derivative, BMB171. The 50% lethal concentrations of this mutant plus the cry1Ac insecticidal protein gene were about 5.8-fold higher than those of the BMB171 strain. When purified Bel was mixed with the Cry1Ac protein and fed to Helicoverpa armigera larvae, 3 μg/ml Cry1Ac alone induced 34.2% mortality. Meanwhile, the mortality rate rose to 74.4% when the same amount of Cry1Ac was mixed with 0.8 μg/ml of Bel. Microscopic observation showed a significant disruption detected on the midgut PM of H. armigera larvae after they were fed Bel. In vitro degradation assays showed that Bel digested the intestinal mucin (IIM) of Trichoplusia ni and H. armigera larvae to various degrading products, similar to findings for viral enhancin. These results imply Bel toxicity enhancement depends on the destruction of midgut PM and IIM, similar to the case with viral enhancin. This discovery showed that Bel has the potential to enhance insecticidal activity of B. thuringiensis-based biopesticides and transgenic crops.Bacillus thuringiensis is a ubiquitous gram-positive, spore-forming soil bacterium and produces insecticidal crystal proteins during the sporulation phase of its growth cycle. Because these insecticidal crystal proteins have activity against certain insect species, B. thuringiensis has been extensively used as a biopesticide to control crop pests in commercial agriculture and forest management. It is also a key source of genes for transgenic expression and provides pest resistance in plants (2, 20, 30).The viral enhancin protein was originally described for granuloviruses (GVs) as a 126-kDa protein that showed an ability to enhance the infectivity of nucleopolyhedroviruses (NPVs) (36, 37, 39). It has also been found in several other GVs (13) and NPVs (19, 27). Considered a pathogenicity factor, it is not essential for growth of viruses in cell culture or infected insects but has the function of facilitating GV and NPV infection and decreasing larval survival time (14, 17, 19, 27).The widely accepted action mode of the viral enhancin protein, which has been identified as a metalloprotease (17), is that it can disrupt the protective peritrophic matrix (PM), allowing virion access to the underlying epithelial cells of the insect gut (17). The PM has a lattice structure formed by chitin and insect intestinal mucin (IIM), and the viral enhancin protein targets the IIM for degradation (33).Enhancin-like genes with 24 to 25% nucleotide identity to viral enhancin genes have been found in Yersinia pestis, Bacillus anthracis, Bacillus thuringiensis, and Bacillus cereus genome sequences (16, 25, 28). When B. cereus enhancin-like protein was expressed in recombinant Autographa californica multicapsid nucleopolyhedrovirus (AcMNPV) budded viruses and polyhedral inclusion bodies, it was found to be cytotoxic compared to viral enhancin protein. However, larval bioassays indicated that this enhancin-like protein did not enhance infection (8). Hajaij-Ellouze et al. (12) isolated a B. thuringiensis enhancin-like gene from a 407 crystal-minus strain and found that this enhancin-like protein has a typical metalloprotease zinc-binding domain (HEIAH) and belongs to the PlcR regulon. When the enhancin-like mutant was fed to Galleria mellonella larvae, no significant reduction in virulence was observed.In the present study, we report a B. thuringiensis enhancin-like gene (bel) encoding a protein (Bel) that has 20 to 30% identity to the viral enhancin protein and 95% identity to bacterial enhancin-like proteins. Therefore, Bel function may have a synergistic action similar to that of the virus enhancin protein. To understand the biochemical activity of this novel bacterial gene, bel was knocked out in the plasmid-free strain BMB171. We expected that this bel mutant would have no significant reduction in toxicity according to the reports of Galloway et al. (8) and Hajaij-Ellouze et al. (12). However, the bel mutant surprisingly resulted in dramatically reduced Cry1Ac toxicity to Helicoverpa armigera larvae. To further confirm this result, purified Bel was fed together with the Cry1Ac protein to H. armigera larvae. We found that Bel can function as a synergist of Cry1Ac toxicity against H. armigera. In vivo and in vitro observations showed that Bel can disrupt the insect midgut PM and degrade IIM of insect midgut PM. The target of Bel is the IIM of PM, similar to the results found with viral enhancin. |
