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The fungal CCAAT-binding complex and HapX display highly variable but evolutionary conserved synergetic promoter-specific DNA recognition

  • Takanori Furukawa
  • , Mareike Thea Scheven
  • , Matthias Misslinger
  • , Can Zhao
  • , Sandra Hoefgen
  • , Fabio Gsaller
  • , Jeffrey Lau
  • , Christoph Jöchl
  • , Ian Donaldson
  • , Vito Valiante
  • , Axel A. Brakhage
  • , Michael J. Bromley
  • , Hubertus Haas
  • , Peter Hortschansky

Research output: Contribution to journalArticlepeer-review

Abstract

To sustain iron homeostasis, microorganisms have evolved fine-tuned mechanisms for uptake, storage and detoxification of the essential metal iron. In the human pathogen Aspergillus fumigatus, the fungal-specific bZIP-type transcription factor HapX coordinates adaption to both iron starvation and iron excess and is thereby crucial for virulence. Previous studies indicated that a HapX homodimer interacts with the CCAAT-binding complex (CBC) to cooperatively bind bipartite DNA motifs; however, the mode of HapX-DNA recognition had not been resolved. Here, combination of in vivo (genetics and ChIP-seq), in vitro (surface plasmon resonance) and phylogenetic analyses identified an astonishing plasticity of CBC:HapX:DNA interaction. DNA motifs recognized by the CBC:HapX protein complex comprise a bipartite DNA binding site 5ʹ-CSAATN12RWT-3ʹ and an additional 5ʹ-TKAN-3ʹ motif positioned 11–23 bp downstream of the CCAAT motif, i.e. occasionally overlapping the 3ʹ-end of the bipartite binding site. Phylogenetic comparison taking advantage of 20 resolved Aspergillus species genomes revealed that DNA recognition by the CBC:HapX complex shows promoter-specific cross-species conservation rather than regulon-specific conservation. Moreover, we show that CBC:HapX interaction is absolutely required for all known functions of HapX. The plasticity of the CBC:HapX:DNA interaction permits fine tuning of CBC:HapX binding specificities that could support adaptation of pathogens to their host niches.

Original languageEnglish
Pages (from-to)3567-3590
Number of pages24
JournalNucleic Acids Research
Volume48
Issue number7
DOIs
Publication statusPublished - 22 Feb 2020
Externally publishedYes

Bibliographical note

Publisher Copyright:
© The Author(s) 2020.

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