6533b86ffe1ef96bd12cdb05

RESEARCH PRODUCT

A chimeric ribozyme in Clostridium difficile combines features of group I introns and insertion elements

Christoph Von Eichel-streiberVeit BraunDavid E. MahonyMaja RupnikMichael MoosBettina KaltMarkus Mehlig

subject

GeneticsOpen reading framebiologyRNA splicingIntronRibozymebiology.proteinInterrupted geneGroup I catalytic intronGroup II intronORFSMolecular BiologyMicrobiology

description

CdlSt1, a DNA insertion of 1975 bp, was identified within tcdA-C34, the enterotoxin gene of the Clostridium difficile isolate C34. Located in the catalytic domain A1-C34, Cd/St1 combines features of two genetic elements. Within the first 434 nt structures characteristic for group I introns were found; encoding the two transposase-like proteins tlpA and tlpB nucleotides 435-1975 represent the remainder of a IS605-like insertion element. We show that the entire CdlSt1 is accurately spliced from tcdA-C34 primary transcripts and that purified TcdA-C34 toxin is of regular size and catalytic activity. A search for CdlSt1-related sequences demonstrates that the element is widespread in toxinogenic and non-toxinogenic C. difficile strains, indicating the mobility of CdlSt1. In strain C34, we characterize 10 CdlSt1 variants; all are highly homologous to CdlSt1 (> 93% identity), integrated in bacterial open reading frames (ORFs), show the typical composite structure of CdlSt1 and are precisely spliced from their primary transcripts. CdlSt1-like chimeric ribozymes appear to combine the invasiveness of an insertion element with the splicing ability of a group I intron, rendering transposition harmless for the interrupted gene.

yearjournalcountryeditionlanguage
2002-01-18Molecular Microbiology
https://doi.org/10.1046/j.1365-2958.2000.01965.x