Conservation and specificity in Bacillus biofilm dynamics: on structure and function of B. cereus Camelysins

Diehl, Anne; Lindemann, Florian; Cremer, Nils; Roske, Yvette; Hiller, Matthias; van Rossum, Barth; Leidert, Martina; Turgay, Kürşad; Oschkinat, Hartmut

Conservation and specificity in Bacillus biofilm dynamics: on structure and function of B. cereus Camelysins

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Item Type:	Article
Title:	Conservation and specificity in Bacillus biofilm dynamics: on structure and function of B. cereus Camelysins
Creators Name:	Diehl, Anne, Lindemann, Florian, Cremer, Nils, Roske, Yvette, Hiller, Matthias, van Rossum, Barth, Leidert, Martina, Turgay, Kürşad and Oschkinat, Hartmut
Abstract:	The B. cereus family comprises members highly pathogenic for mammals or insects, with B. anthracis and B. thuringiensis respectively as notable examples. The biofilm operon of these bacteria encodes two TasA-like proteins, the 60% identical Camelysins CalY1 and CalY2. In this study, we observed that at neutral pH CalY2 alone polymerizes readily into filaments, whereas CalY1 forms a polydispersed mixture of oligomers without filament formation. However, at basic or acidic pH CalY1 also modestly polymerizes. CalY2 polymerization into filaments involves ß-sheet remodeling via donor strand complementation, as demonstrated here by a combination of NMR and AlphaFold studies. In contrast to TasA of B. subtilis, this process is spontaneous and does not require initiation by a TapA homolog. NMR studies show that the functionally relevant region (β1-β2-β3) of the CalY2 monomer structure closely resembles that of B. subtilis TasA, and differs from AlphaFold models. A survey of AlphaFold 2 predictions on 12 homologous B. cereus group Camelysins yielded only four correctly predicted β1-β2-β3 segments, which decreased to one when using AlphaFold 3. Since crucial residues in the protomer contact region are conserved among TasA-like proteins, we investigated whether family members of different species could form mixed filaments. NMR revealed features in CalY2 filaments that are structurally conserved with TasA filaments but sequentially different, promoting specificity. These interactions and differences, respectively, involve the C-terminus and the beginning of β3, which most likely hinder joint TasA and CalY1 copolymerization. A protease activity could not be observed for the heterologously expressed B. cereus Camelysins. SIGNIFICANCE: The B. cereus group includes extremely harmful and surprisingly benign bacterial strains. The Anthrax-toxin-producing B. anthracis is one of the most toxic bacterial threats to man, whereas B. thuringiensis toxin is used as a biological insecticide. Other B. cereus strains pose problems in food production and medical implant usage. These bacteria can exist as biofilms allowing them to survive and proliferate, an essential feature of which are protein filaments. Here we characterize the B. cereus Camelysins CalY1 and CalY2 and compare their structure and filament formation with B. subtilis filaments to understand principles determining patterns of conservation and specificity. This investigation provides the basis for developing novel means to suppress or enhance biofilms with potential benefits for plant protection.
Keywords:	Bacillus Subtilis, Bacillus Cereus, Biofilm, CalY, TasA, TapA, Structure, Filaments, AUC, Protease Activity
Source:	Journal of Molecular Biology
ISSN:	0022-2836
Publisher:	Elsevier
Page Range:	169661
Date:	27 January 2026
Official Publication:	https://doi.org/10.1016/j.jmb.2026.169661
PubMed:	View item in PubMed
Related to:	URL URL Type http://gwagner.med.harvard.edu/intranet/hmsIST Software

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