septal pores
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2020 ◽  
Vol 6 (4) ◽  
pp. 344
Author(s):  
Vasileios Vangalis ◽  
Ioannis A. Papaioannou ◽  
Emmanouil A. Markakis ◽  
Michael Knop ◽  
Milton A. Typas

Woronin bodies are membrane-bound organelles of filamentous ascomycetes that mediate hyphal compartmentalization by plugging septal pores upon hyphal damage. Their major component is the peroxisomal protein Hex1, which has also been implicated in additional cellular processes in fungi. Here, we analyzed the Hex1 homolog of Verticillium dahliae, an important asexual plant pathogen, and we report its pleiotropic involvement in fungal growth, physiology, stress response, and pathogenicity. Alternative splicing of the Vdhex1 gene can lead to the production of two Hex1 isoforms, which are structurally similar to their Neurospora crassa homolog. We show that VdHex1 is targeted to the septum, consistently with its demonstrated function in sealing hyphal compartments to prevent excessive cytoplasmic bleeding upon injury. Furthermore, our investigation provides direct evidence for significant contributions of Hex1 in growth and morphogenesis, as well as in asexual reproduction capacity. We discovered that Hex1 is required both for normal responses to osmotic stress and factors that affect the cell wall and plasma-membrane integrity, and for normal resistance to oxidative stress and reactive oxygen species (ROS) homeostasis. The Vdhex1 mutant exhibited diminished ability to colonize and cause disease on eggplant. Overall, we show that Hex1 has fundamentally important multifaceted roles in the biology of V. dahliae.


2020 ◽  
Author(s):  
Vasileios Vangalis ◽  
Ioannis A. Papaioannou ◽  
Emmanouil A. Markakis ◽  
Michael Knop ◽  
Milton A. Typas

AbstractWoronin bodies are membrane-bound organelles of filamentous ascomycetes that mediate hyphal compartmentalization by plugging septal pores upon hyphal damage. Their major component is the peroxisomal protein Hex1, which has also been implicated in additional cellular processes in fungi. Here, we analyzed the Hex1 homolog of Verticillium dahliae, an important asexual plant pathogen, and we report its pleiotropic involvement in fungal growth, physiology, stress response and pathogenicity. Alternative splicing of the Vdhex1 gene can lead to the production of two Hex1 isoforms, which are structurally similar to their Neurospora crassa homolog. We show that VdHex1 is targeted to the septum, consistently with its demonstrated function in sealing hyphal compartments to prevent excessive cytoplasmic bleeding upon injury. Furthermore, our investigation provides direct evidence for significant contributions of Hex1 in growth and morphogenesis, as well as in asexual reproduction capacity. We discovered that Hex1 is required both for normal responses to osmotic stress and factors that affect the cell wall and plasma membrane integrity, and for normal resistance to oxidative stress and ROS homeostasis. The Vdhex1 mutant exhibited diminished ability to colonize and cause disease on eggplant. Overall, we show that Hex1 has fundamentally important multifaceted roles in the biology of V. dahliae.


2020 ◽  
Vol 6 (3) ◽  
pp. 172 ◽  
Author(s):  
Guirong Tang ◽  
Yanfang Shang ◽  
Shiqing Li ◽  
Chengshu Wang

The Woronin body (WB) is a peroxisome-derived dense-core vesicle, a self-assembling hexagonal crystal of a single protein Hex1. This organelle is specific to the ascomycete fungi belonging to the Pezizomycotina subphylum by functioning in sealing septal pores in response to mycelium damage and the control of cell heterogeneity. We retrieved all available Hex1-domain containing proteins of different fungi from the GenBank database and found considerable length variations among 460 obtained Hex1 proteins. However, a highly conserved Hex1 domain containing 75 amino acid residues with a specific S/A-R/S-L consensus motif for targeting peroxisome is present at the carboxy-terminus of each protein. A homologous Hex1 gene, named MrHex1, was deleted in the entomopathogenic fungus Metarhizium robertsii. It was found that MrHex1 was responsible for WB formation in M. robertsii and involved in sealing septal pores to maintain cell integrity and heterogeneity. Different assays indicated that, relative to the wild-type (WT) strain, ∆Mrhex1 demonstrated a growth defect on a solid medium and substantial reductions of conidiation, appressorium formation and topical infectivity against insect hosts. However, there was no obvious virulence difference between WT and mutants during injection of insects. We also found that ∆MrHex1 could tolerate different stress conditions like the WT and the gene-rescued mutant of M. robertsii, which is in contrast to the reports of the stress-response defects of the Hex1 null mutants of other fungal species. In addition to revealing the phenotypic/functional alterations of the Hex1 deletion mutants between different pathotype fungi, the results of this study may benefit the understanding of the evolution and WB-control of fungal entomopathogenicity.


2019 ◽  
Vol 132 ◽  
pp. 103259 ◽  
Author(s):  
Sofia Dimou ◽  
Anezia Kourkoulou ◽  
Sotiris Amillis ◽  
Riccardo Percudani ◽  
George Diallinas

2018 ◽  
Author(s):  
Lianhu Zhang ◽  
Dongmei Zhang ◽  
Yunyun Chen ◽  
Wenyu Ye ◽  
Qingyun Lin ◽  
...  

ABSTRACTMagnaporthe oryzae (Mo) is a model pathogen causing rice blast resulting in yield and economic losses world-wide. CK2 is a constitutively active, serine/threonine kinase in eukaryotes, having a wide array of known substrates and involved in many cellular processes. We investigated the localization and role of MoCK2 during growth and infection. BLAST search for MoCK2 components and targeted deletion of subunits was combined with protein-GFP fusions to investigate localization. We found one CKa and two CKb subunits of the CK2 holoenzyme. Deletion of the catalytic subunit CKa was not possible and might indicate that such deletions are lethal. The CKb subunits could be deleted but they were both necessary for normal growth and pathogenicity. Localization studies showed that the CK2 holoenzyme needed to be intact for normal localization at septal pores and at appressorium penetration pores. Nuclear localization of CKa was however not dependent on the intact CK2 holoenzyme. In appressoria, CK2 formed a large ring perpendicular to the penetration pore and the ring formation was dependent on the presence of all CK2 subunits. The effects on growth and pathogenicity of deletion of the b subunits combined with the localization indicate that CK2 can have important regulatory functions not only in the nucleus/nucleolus but also at fungal specific structures as septa and appressorial pores.


2017 ◽  
Vol 109 ◽  
pp. 53-55 ◽  
Author(s):  
Gero Steinberg ◽  
Nicholas J. Harmer ◽  
Martin Schuster ◽  
Sreedhar Kilaru
Keyword(s):  

2017 ◽  
Vol 19 (11) ◽  
pp. e12764 ◽  
Author(s):  
Gero Steinberg ◽  
Martin Schuster ◽  
Christian Hacker ◽  
Sreedhar Kilaru ◽  
Ana Correia

2014 ◽  
Vol 36 (5) ◽  
pp. 11-15
Author(s):  
Jacob O. Brunkard ◽  
Anne M. Runkel ◽  
Patricia C. Zambryski

Multicellularity is central to the stunning diversity of biological forms on earth today. In multicellular species, individual cells become dependent on each other, differentiate to specialize their functions, and may even undergo cell death as the whole organism develops. This developmental process requires intense co-ordination of genetic programs and physiology across the organism, relying on communication between cells. There are only a handful of lineages of obligate multicellular eukaryotes – animals, a few groups of fungi, certain algal lineages, and land plants – but each arose independently, and each employs a distinct mechanism of intercellular communication1. Direct physical cell–cell communication between animal cells occurs via gap junctions, which transport only very small molecules, and via tunnelling nanotubes, which permit exchange of larger molecules. Fungal cells never fully separate after cell division, in a sense, because they leave behind septal pores that connect adjacent cytoplasts. In plants, intercellular communication is primarily facilitated by plasmodesmata (PD).


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