Crystal Structure of an Uncommon Cellulosome-Related Protein Module from Ruminococcus flavefaciens That Resembles Papain-Like Cysteine Peptidases

Levy-Assaraf, Maly; Voronov-Goldman, Milana; Grinberg, Inna Rozman; Weiserman, Gloria; Shimon, Linda J. W.; Jindou, Sadanari; Borovok, Ilya; White, Bryan A.; Bayer, Edward A.; Lamed, Raphael; Frolow, Felix

doi:10.1371/journal.pone.0056138

Cited by 19 publications

(18 citation statements)

References 42 publications

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“…I1.2 is particularly intriguing, since biomass-modifying enzymes are directly involved in the deconstruction of lignocellulosic biomass. However, recent studies have suggested the presence of peptidases and proteases as members of Ruminococcus flavefaciens cellulossome, although the functional relevance of these enzymes is still not clear [27]. These observations are consistent with the detection of one Clostridium thermocellum serine protease and two serine proteases inhibitors (serpins), both containing one dockerin module [28,29].…”

Section: In Complexes C-[i] C-[ii] and C-[iii]supporting

confidence: 67%

Biochemical Characterization of Streptomyces sp. I1.2 Secretome Reveals the Presence of Multienzymatic Complexes Containing Cellulases and Accessory Enzymes

et al. 2016

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Two general strategies have been proposed for microbial cellulose degradation: filamentous fungi and aerobic bacteria secrete uncomplexed cellulases, while some anaerobic bacteria produce a cell-associated and large extracellular multienzymatic complex called cellulosomes. By using a combination of 1D-blue native (BN)-PAGE, 2D-BN/SDS-PAGE, zymography, and LC-MS/MS methods, we demonstrate here that Streptomyces sp. I1.2, an aerobic bacterium associated with the land snail Achatina fulica, is able to degrade both crystalline cellulose and sugarcane bagasse through the production of cellulolytic multienzymatic complexes containing different combinations of cellobiohydrolases, endo-glucanases, xylanases, lytic polysaccharide monooxygenases (LPMOs), and peptidases. The assembly and subunit composition of these complexes is specifically affected by the carbon source, while the multienzymatic complexes produced after growth in crystalline cellulose are composed mainly by one cellobiohydrolase and chitinase, in which the complexes produced in response to sugarcane bagasse are more heterogeneous and contain cellobiohydrolases, endo-glucanases, pectate lyases, one LPMO, β-1,3-glucanases, and one xylanase. Our results suggest that Streptomyces sp. I1.2 displays an alternative mechanism for deconstruction of cellulose that depends upon a noncellulosomic association of catalytic subunits into high molecular weight complexes in order to achieve higher catalytic efficiencies.

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Section: In Complexes C-[i] C-[ii] and C-[iii]supporting

confidence: 67%

Biochemical Characterization of Streptomyces sp. I1.2 Secretome Reveals the Presence of Multienzymatic Complexes Containing Cellulases and Accessory Enzymes

et al. 2016

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“…1 ). Sequence data and structural analysis have revealed that the dockerins of ScaB, CttA and a cysteine peptidase‐like scaffoldin [20] are different from the conventional symmetric dockerins, described earlier. They possess three insertions, one of which is positioned inside the second calcium‐binding loop [15].…”

Section: Introductionmentioning

confidence: 75%

Standalone cohesin as a molecular shuttle in cellulosome assembly

et al. 2015

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Edited by Wilhelm JustKeywords: Cohesin Type III Dockerin Cellulose degradation Cohesin-dockerin complex Rumen bacteria Ruminococcus flavefaciens a b s t r a c tThe cellulolytic bacterium Ruminococcus flavefaciens of the herbivore rumen produces an elaborate cellulosome system, anchored to the bacterial cell wall via the covalently bound scaffoldin ScaE. Dockerin-bearing scaffoldins also bind to an autonomous cohesin of unknown function, called cohesin G (CohG). Here, we demonstrate that CohG binds to the scaffoldin-borne dockerin in opposite orientation on a distinct site, relative to that of ScaE. Based on these structural data, we propose that the complexed dockerin is still available to bind ScaE on the cell surface. CohG may thus serve as a molecular shuttle for delivery of scaffoldins to the bacterial cell surface.

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“…Examples of frequent components include an N-terminal signal peptide, a MurNAc amidase, and one or multiple targeting domains, such as the LysM domain, the peptydoglycan binding domain (PGBD), the choline binding domain (CGD), and the bacterial SH3b domain34. Recently, the crystal structure of a CHAP domain has been characterized as a cellulosome-related module, indicating that this family of cysteine peptidases might modulate processes other than cell-wall hydrolysis46. CHAP domains have been unified under the peptidase families C40 and C51 in the MEROPS database23, under Pfam47 domains NlpC/P60 (PF00877) and CHAP (PF05257), and under the COG database48 entries COG0791 ‘cell-wall-associated hydrolases (invasion-associated proteins)’ and COG3942 ‘surface antigen’.…”

Section: Resultsmentioning

confidence: 99%

“…CHAP superfamily members also share structural similarities that cannot be detected at the sequence level46. Beyond the catalytic core, the structures are highly divergent through deletions and insertions of structural elements.…”

Section: Resultsmentioning

confidence: 99%

“…In this regard, the PGBD and SH3 domain from PCP may form a bridge between the bacterial cell wall and the cell wall of plant substrates via their respective binding to these organelles. This correlation is also strengthened by the discovery of a CHAP domain acting as module in a cellulosome46. Recently, Xu and coworker have shed a light on the differences between substrate specificity of one turnover and two recycling cysteine proteases64.…”

Section: Discussionmentioning

confidence: 95%

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Functional and structural characterization of a novel putative cysteine protease cell wall-modifying multi-domain enzyme selected from a microbial metagenome

Faheem

Martins-de-Sa

Vidal

et al. 2016

Sci Rep

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A current metagenomics focus is to interpret and transform collected genomic data into biological information. By combining structural, functional and genomic data we have assessed a novel bacterial protein selected from a carbohydrate-related activity screen in a microbial metagenomic library from Capra hircus (domestic goat) gut. This uncharacterized protein was predicted as a bacterial cell wall-modifying enzyme (CWME) and shown to contain four domains: an N-terminal, a cysteine protease, a peptidoglycan-binding and an SH3 bacterial domain. We successfully cloned, expressed and purified this putative cysteine protease (PCP), which presented autoproteolytic activity and inhibition by protease inhibitors. We observed cell wall hydrolytic activity and ampicillin binding capacity, a characteristic of most bacterial CWME. Fluorimetric binding analysis yielded a Kb of 1.8 × 105 M−1 for ampicillin. Small-angle X-ray scattering (SAXS) showed a maximum particle dimension of 95 Å with a real-space Rg of 28.35 Å. The elongated molecular envelope corroborates the dynamic light scattering (DLS) estimated size. Furthermore, homology modeling and SAXS allowed the construction of a model that explains the stability and secondary structural changes observed by circular dichroism (CD). In short, we report a novel cell wall-modifying autoproteolytic PCP with insight into its biochemical, biophysical and structural features.

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Crystal Structure of an Uncommon Cellulosome-Related Protein Module from Ruminococcus flavefaciens That Resembles Papain-Like Cysteine Peptidases

Cited by 19 publications

References 42 publications

Biochemical Characterization of Streptomyces sp. I1.2 Secretome Reveals the Presence of Multienzymatic Complexes Containing Cellulases and Accessory Enzymes

Biochemical Characterization of Streptomyces sp. I1.2 Secretome Reveals the Presence of Multienzymatic Complexes Containing Cellulases and Accessory Enzymes

Standalone cohesin as a molecular shuttle in cellulosome assembly

Functional and structural characterization of a novel putative cysteine protease cell wall-modifying multi-domain enzyme selected from a microbial metagenome

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