Heterologous expression and characterisation of microcystinase

“…It was indicated previously that whole cells of E. coli BL21_MlrA exhibited approximately 250 times higher MlrA activity than Sphingomonas cells [14]. Furthermore, the use of IPTG to induct the MlrA expression in BL21_MlrA was not necessary, because the cells with and without induction exhibited a similar level of activity toward MC-LR (data not presented).…”

“…The crucial step in MC detoxification by bacteria is the linearization reaction catalyzed by metalloproteinase called microcystinase (MlrA). Such a decyclization results in a significant reduction of toxicity [14]. The pathway of MC degradation was confirmed independently, with small alteration due to the different strains.…”

“…coding for MlrA was amplified by PCR using primer pairs described earlier [14]. The amplified fragments were inserted into the pTZ57R/T cloning vector and the sequence was verified.…”

“…ACM-3962 and E. coli BL21_MlrA cells was measured as described earlier using the HPLC method [14]. The rate of MCs degradation was calculated by monitoring the level of linear MC-LR.…”

“…2). For example, better biochemical characterization of these important enzymes as well as the correction of their role in MCs degradation was possible [14] - [16]. Another option is to investigate the usefulness of such recombinant strains or recombinantly expressed MlrA enzyme in biotechnological application.…”

Genetically Engineered Bacteria Immobilized in Alginate as an Option of Cyanotoxins Removal

“…It was indicated previously that whole cells of E. coli BL21_MlrA exhibited approximately 250 times higher MlrA activity than Sphingomonas cells [14]. Furthermore, the use of IPTG to induct the MlrA expression in BL21_MlrA was not necessary, because the cells with and without induction exhibited a similar level of activity toward MC-LR (data not presented).…”

“…The crucial step in MC detoxification by bacteria is the linearization reaction catalyzed by metalloproteinase called microcystinase (MlrA). Such a decyclization results in a significant reduction of toxicity [14]. The pathway of MC degradation was confirmed independently, with small alteration due to the different strains.…”

“…coding for MlrA was amplified by PCR using primer pairs described earlier [14]. The amplified fragments were inserted into the pTZ57R/T cloning vector and the sequence was verified.…”

“…ACM-3962 and E. coli BL21_MlrA cells was measured as described earlier using the HPLC method [14]. The rate of MCs degradation was calculated by monitoring the level of linear MC-LR.…”

“…2). For example, better biochemical characterization of these important enzymes as well as the correction of their role in MCs degradation was possible [14] - [16]. Another option is to investigate the usefulness of such recombinant strains or recombinantly expressed MlrA enzyme in biotechnological application.…”

Genetically Engineered Bacteria Immobilized in Alginate as an Option of Cyanotoxins Removal

Biological Treatment for the Destruction of Cyanotoxins

Transformation Products (TPs) of Cyanobacterial Metabolites During Treatment