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Ice nucleation proteins self-assemble into large fibres to trigger freezing at near 0 ℃

  1. Thomas Hansen
  2. Jocelyn C. Lee
  3. Naama Reicher
  4. Gil Ovadia
  5. Shuaiqi Guo
  6. Wangbiao Guo
  7. Jun Liu
  8. Ido Braslavsky
  9. Yinon Rudich
  10. Peter L. Davies author has email address
  1. Department of Biomedical and Molecular Sciences, Queen’s University, Kingston, ON Canada K7L 3N6
  2. Department of Earth and Planetary Sciences, The Weizmann Institute of Science, Rehovot 7610001, Israel
  3. The Robert H. Smith Faculty of Agriculture, Food and Environment, Institute of Biochemistry, Food Science, and Nutrition, The Hebrew University of Jerusalem, Rehovot 7610001, Israel
  4. Department of Microbial Pathogenesis, Yale University School of Medicine, New Haven, CT 06536

Peer review process

Not revised: This Reviewed Preprint includes the authors’ original preprint (without revision), an eLife assessment, and public reviews.

Read more about eLife’s peer review process.

Editors

  • Reviewing Editor
    Hannes Neuweiler
    University of Würzburg, Würzburg, Germany
  • Senior Editor
    David Ron
    University of Cambridge, Cambridge, United Kingdom

Reviewer #1 (Public Review):

Summary: Hansen et al. dissect the molecular mechanisms of bacterial ice nucleating proteins mutating the protein systematically. They assay the ice nucleating ability for variants changing the R-coils as well as the coil capping motifs. The ice nucleation mechanism depends on the integrity of the R-coils, without which the multimerization and formation of fibrils are disrupted.

Strengths: The effects of mutations are really dramatic, so there is no doubt about the effect. The variants tested are logical and progressively advance the story. The authors identify an underlying mechanism involving multimerization, which is plausible and compatible with EM data. The model is further shown to work in cells by tomography.

Weaknesses: The theoretical model presented for how the proteins assemble into fibrils is simple, but not supported by much data.

Reviewer #2 (Public Review):

Summary:
This paper further investigates the role of self-assembly of ice-binding bacterial proteins in promoting ice-nucleation. For the P. borealis Ice Nucleating Protein (PbINP) studied here, earlier work had already determined clearly distinct roles for different subdomains of the protein in determining activity. Key players are the water-organizing loops (WO-loops) of the central beta-solenoid structure and a set of non-water-organizing C-terminal loops, called the R-loops in view of characteristically located arginines. Previous mutation studies (using nucleation activity as a read-out) had already suggested the R-loops interact with the WO loops, to cause self-assembly of PbINP, which in turn was thought to lead to enhanced ice-nucleating activity. In this paper, the activities of additional mutants are studied, and a bioinformatics analysis on the statistics of the number of WO- and R-loops is presented for a wide range of bacterial ice-nucleating proteins, and additional electron-microscopy results are presented on fibrils formed by the non-mutated PbINP in E coli lysates.

Strengths:
-A very complete set of additional mutants is investigated to further strengthen the earlier hypothesis.
-A nice bioinformatics analysis that underscores that the hypothesis should apply not only to PbINP but to a wide range of (related) bacterial ice-nucleating proteins.
-Convincing data that PbINP overexpressed in E coli forms fibrils (electron microscopy on E coli lysates).

Weaknesses:
-The new data is interesting and further strengthens the hypotheses put forward in the earlier work. However, just as in the earlier work, the proof for the link between self-assembly and ice-nucleation remains indirect. Assembly into fibrils is shown for E coli lysates expressing non-mutated pbINP, hence it is indeed clear that pbINP self-associates. It is not shown however that the mutations that lead to loss of ice-nucleating activity also lead to loss of self-assembly. A more quantitative or additional self-assembly assay could shine light on this, either in the present or in future studies.

-Also the "working model" for the self-assembly of the fibers remains not more than that, just as in the earlier papers, since the mutation-activity relationship does not contain enough information to build a good structural model. Again, a better model would require different kinds of experiments, that yield more detailed structural data on the fibrils.

Reviewer #3 (Public Review):

Summary: in this manuscript, Hansen and co-authors investigated the role of R-coils in the multimerization and ice nucleation activity of PbINP, an ice nucleation protein identified in Pseudomonas borealis. The results of this work suggest that the length, localization, and amino acid composition of R-coils are crucial for the formation of PbINP multimers.

Strengths: The authors use a rational mutagenesis approach to identify the role of the length, localisation, and amino acid composition of R-coils in ice nucleation activity. Based on these results, the authors hypothesize a multimerization model. Overall, this is a multidisciplinary work that provides new insights into the molecular mechanisms underlying ice nucleation activity.

Weaknesses: Several parts of the work appear cryptic and unsuitable for non-expert readers. The results of this work should be better described and presented.

  1. Howard Hughes Medical Institute
  2. Wellcome Trust
  3. Max-Planck-Gesellschaft
  4. Knut and Alice Wallenberg Foundation