Cleavage of an engulfment peptidoglycan hydrolase by a sporulation signature protease in Clostridioides difficile

Diogo Martins; Hailee N. Nerber; Charlotte G. Roughton; Amaury Fasquelle; Anna Barwinska-Sendra; Daniela Vollmer; Joe Gray; Waldemar Vollmer; Joseph A. Sorg; Paula S. Salgado; Adriano O. Henriques; Mónica Serrano

doi:10.1111/mmi.15291

Cleavage of an engulfment peptidoglycan hydrolase by a sporulation signature protease in Clostridioides difficile

Diogo Martins, Hailee N. Nerber, Charlotte G. Roughton, Amaury Fasquelle, Anna Barwinska-Sendra, Daniela Vollmer, Joe Gray, Waldemar Vollmer, Joseph A. Sorg, Paula S. Salgado, Adriano O. Henriques, Mónica Serrano

Instituto de Tecnologia Química e Biológica António Xavier (ITQB)

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Abstract

In the model organism Bacillus subtilis, a signaling protease produced in the forespore, SpoIVB, is essential for the activation of the sigma factor σ^K, which is produced in the mother cell as an inactive pro-protein, pro-σ^K. SpoIVB has a second function essential to sporulation, most likely during cortex synthesis. The cortex is composed of peptidoglycan (PG) and is essential for the spore's heat resistance and dormancy. Surprisingly, the genome of the intestinal pathogen Clostridioides difficile, in which σ^K is produced without a pro-sequence, encodes two SpoIVB paralogs, SpoIVB1 and SpoIVB2. Here, we show that spoIVB1 is dispensable for sporulation, while a spoIVB2 in-frame deletion mutant fails to produce heat-resistant spores. The spoIVB2 mutant enters sporulation, undergoes asymmetric division, and completes engulfment of the forespore by the mother cell but fails to synthesize the spore cortex. We show that SpoIIP, a PG hydrolase and part of the engulfasome, the machinery essential for engulfment, is cleaved by SpoIVB2 into an inactive form. Within the engulfasome, the SpoIIP amidase activity generates the substrates for the SpoIID lytic transglycosylase. Thus, following engulfment completion, the cleavage and inactivation of SpoIIP by SpoIVB2 curtails the engulfasome hydrolytic activity, at a time when synthesis of the spore cortex peptidoglycan begins. SpoIVB2 is also required for normal late gene expression in the forespore by a currently unknown mechanism. Together, these observations suggest a role for SpoIVB2 in coordinating late morphological and gene expression events between the forespore and the mother cell.

Original language	English
Pages (from-to)	213-229
Number of pages	17
Journal	Molecular Microbiology
Volume	122
Issue number	2
DOIs	https://doi.org/10.1111/mmi.15291
Publication status	Published - 22 Jun 2024

Keywords

cortex
peptidoglycan
serine-protease
SpoIIP
SpoIVB

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10.1111/mmi.15291Licence: CC BY

Cleavage of an engulfment peptidoglycan hydrolase by asporulation signature protease in Clostridioides difficileFinal published version, 18.2 MBLicence: CC BY

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Martins, D., Nerber, H. N., Roughton, C. G., Fasquelle, A., Barwinska-Sendra, A., Vollmer, D., Gray, J., Vollmer, W., Sorg, J. A., Salgado, P. S., Henriques, A. O., & Serrano, M. (2024). Cleavage of an engulfment peptidoglycan hydrolase by a sporulation signature protease in Clostridioides difficile. Molecular Microbiology, 122(2), 213-229. https://doi.org/10.1111/mmi.15291

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title = "Cleavage of an engulfment peptidoglycan hydrolase by a sporulation signature protease in Clostridioides difficile",

abstract = "In the model organism Bacillus subtilis, a signaling protease produced in the forespore, SpoIVB, is essential for the activation of the sigma factor σK, which is produced in the mother cell as an inactive pro-protein, pro-σK. SpoIVB has a second function essential to sporulation, most likely during cortex synthesis. The cortex is composed of peptidoglycan (PG) and is essential for the spore's heat resistance and dormancy. Surprisingly, the genome of the intestinal pathogen Clostridioides difficile, in which σK is produced without a pro-sequence, encodes two SpoIVB paralogs, SpoIVB1 and SpoIVB2. Here, we show that spoIVB1 is dispensable for sporulation, while a spoIVB2 in-frame deletion mutant fails to produce heat-resistant spores. The spoIVB2 mutant enters sporulation, undergoes asymmetric division, and completes engulfment of the forespore by the mother cell but fails to synthesize the spore cortex. We show that SpoIIP, a PG hydrolase and part of the engulfasome, the machinery essential for engulfment, is cleaved by SpoIVB2 into an inactive form. Within the engulfasome, the SpoIIP amidase activity generates the substrates for the SpoIID lytic transglycosylase. Thus, following engulfment completion, the cleavage and inactivation of SpoIIP by SpoIVB2 curtails the engulfasome hydrolytic activity, at a time when synthesis of the spore cortex peptidoglycan begins. SpoIVB2 is also required for normal late gene expression in the forespore by a currently unknown mechanism. Together, these observations suggest a role for SpoIVB2 in coordinating late morphological and gene expression events between the forespore and the mother cell.",

keywords = "cortex, peptidoglycan, serine-protease, SpoIIP, SpoIVB",

author = "Diogo Martins and Nerber, {Hailee N.} and Roughton, {Charlotte G.} and Amaury Fasquelle and Anna Barwinska-Sendra and Daniela Vollmer and Joe Gray and Waldemar Vollmer and Sorg, {Joseph A.} and Salgado, {Paula S.} and Henriques, {Adriano O.} and M{\'o}nica Serrano",

note = "Funding Information: This work was supported by the European Union Marie Sklodowska Curie Innovative Training Networks (contract number 642068) to AOH and AF was the recipient of a PhD fellowship under that contract. This project was supported by award PTDC/BIA\u2010MIC/29293/2017 to MS. This work was also financially supported by Project LISBOA\u201001\u20100145\u2010FEDER\u2010007660 (\u201CMicrobiologia Molecular, Estrutural e Celular\u201D) funded by FEDER funds through COMPETE2020\u2014\u201CPrograma Operacional Competitividade e Internacionaliza\u00E7\u00E3o\u201D (POCI), by national funds through the FCT (\u201CFunda\u00E7\u00E3o para a Ci\u00EAncia e a Tecnologia\u201D). DM is the recipient of a PhD fellowship (PD/BD/143148/2019) within the scope of the PhD program INTERFACE funded by FCT. This project was supported by the Medical Research Council (grant number MR/V032151/1) awarded to PSS and ABS and the BBSRC (BB/W005557/1, BB/W013630/1) to WV. CGR is supported by a Barbour Foundation PhD Studentship from Faculty of Medical Science, Newcastle University. This project was also supported by awards R01AI116895 and R01AI172043 from the National Institute of Allergy and Infectious Diseases to JAS. The content is solely the responsibility of the authors and does not necessarily represent the official views of the NIAID. The funders had no role in study design, data collection, and interpretation, or the decision to submit the work for publication. Publisher Copyright: {\textcopyright} 2024 The Author(s). Molecular Microbiology published by John Wiley & Sons Ltd.",

year = "2024",

month = jun,

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doi = "10.1111/mmi.15291",

language = "English",

volume = "122",

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journal = "Molecular Microbiology",

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T1 - Cleavage of an engulfment peptidoglycan hydrolase by a sporulation signature protease in Clostridioides difficile

AU - Martins, Diogo

AU - Nerber, Hailee N.

AU - Roughton, Charlotte G.

AU - Fasquelle, Amaury

AU - Barwinska-Sendra, Anna

AU - Vollmer, Daniela

AU - Gray, Joe

AU - Vollmer, Waldemar

AU - Sorg, Joseph A.

AU - Salgado, Paula S.

AU - Henriques, Adriano O.

AU - Serrano, Mónica

N1 - Funding Information: This work was supported by the European Union Marie Sklodowska Curie Innovative Training Networks (contract number 642068) to AOH and AF was the recipient of a PhD fellowship under that contract. This project was supported by award PTDC/BIA\u2010MIC/29293/2017 to MS. This work was also financially supported by Project LISBOA\u201001\u20100145\u2010FEDER\u2010007660 (\u201CMicrobiologia Molecular, Estrutural e Celular\u201D) funded by FEDER funds through COMPETE2020\u2014\u201CPrograma Operacional Competitividade e Internacionaliza\u00E7\u00E3o\u201D (POCI), by national funds through the FCT (\u201CFunda\u00E7\u00E3o para a Ci\u00EAncia e a Tecnologia\u201D). DM is the recipient of a PhD fellowship (PD/BD/143148/2019) within the scope of the PhD program INTERFACE funded by FCT. This project was supported by the Medical Research Council (grant number MR/V032151/1) awarded to PSS and ABS and the BBSRC (BB/W005557/1, BB/W013630/1) to WV. CGR is supported by a Barbour Foundation PhD Studentship from Faculty of Medical Science, Newcastle University. This project was also supported by awards R01AI116895 and R01AI172043 from the National Institute of Allergy and Infectious Diseases to JAS. The content is solely the responsibility of the authors and does not necessarily represent the official views of the NIAID. The funders had no role in study design, data collection, and interpretation, or the decision to submit the work for publication. Publisher Copyright: © 2024 The Author(s). Molecular Microbiology published by John Wiley & Sons Ltd.

PY - 2024/6/22

Y1 - 2024/6/22

N2 - In the model organism Bacillus subtilis, a signaling protease produced in the forespore, SpoIVB, is essential for the activation of the sigma factor σK, which is produced in the mother cell as an inactive pro-protein, pro-σK. SpoIVB has a second function essential to sporulation, most likely during cortex synthesis. The cortex is composed of peptidoglycan (PG) and is essential for the spore's heat resistance and dormancy. Surprisingly, the genome of the intestinal pathogen Clostridioides difficile, in which σK is produced without a pro-sequence, encodes two SpoIVB paralogs, SpoIVB1 and SpoIVB2. Here, we show that spoIVB1 is dispensable for sporulation, while a spoIVB2 in-frame deletion mutant fails to produce heat-resistant spores. The spoIVB2 mutant enters sporulation, undergoes asymmetric division, and completes engulfment of the forespore by the mother cell but fails to synthesize the spore cortex. We show that SpoIIP, a PG hydrolase and part of the engulfasome, the machinery essential for engulfment, is cleaved by SpoIVB2 into an inactive form. Within the engulfasome, the SpoIIP amidase activity generates the substrates for the SpoIID lytic transglycosylase. Thus, following engulfment completion, the cleavage and inactivation of SpoIIP by SpoIVB2 curtails the engulfasome hydrolytic activity, at a time when synthesis of the spore cortex peptidoglycan begins. SpoIVB2 is also required for normal late gene expression in the forespore by a currently unknown mechanism. Together, these observations suggest a role for SpoIVB2 in coordinating late morphological and gene expression events between the forespore and the mother cell.

AB - In the model organism Bacillus subtilis, a signaling protease produced in the forespore, SpoIVB, is essential for the activation of the sigma factor σK, which is produced in the mother cell as an inactive pro-protein, pro-σK. SpoIVB has a second function essential to sporulation, most likely during cortex synthesis. The cortex is composed of peptidoglycan (PG) and is essential for the spore's heat resistance and dormancy. Surprisingly, the genome of the intestinal pathogen Clostridioides difficile, in which σK is produced without a pro-sequence, encodes two SpoIVB paralogs, SpoIVB1 and SpoIVB2. Here, we show that spoIVB1 is dispensable for sporulation, while a spoIVB2 in-frame deletion mutant fails to produce heat-resistant spores. The spoIVB2 mutant enters sporulation, undergoes asymmetric division, and completes engulfment of the forespore by the mother cell but fails to synthesize the spore cortex. We show that SpoIIP, a PG hydrolase and part of the engulfasome, the machinery essential for engulfment, is cleaved by SpoIVB2 into an inactive form. Within the engulfasome, the SpoIIP amidase activity generates the substrates for the SpoIID lytic transglycosylase. Thus, following engulfment completion, the cleavage and inactivation of SpoIIP by SpoIVB2 curtails the engulfasome hydrolytic activity, at a time when synthesis of the spore cortex peptidoglycan begins. SpoIVB2 is also required for normal late gene expression in the forespore by a currently unknown mechanism. Together, these observations suggest a role for SpoIVB2 in coordinating late morphological and gene expression events between the forespore and the mother cell.

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KW - peptidoglycan

KW - serine-protease

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DO - 10.1111/mmi.15291

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SN - 0950-382X

VL - 122

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JO - Molecular Microbiology

JF - Molecular Microbiology

IS - 2

ER -

Cleavage of an engulfment peptidoglycan hydrolase by a sporulation signature protease in Clostridioides difficile

Abstract

Keywords

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