Your search keyword '"Varossieau, Koen"' showing total 10 results

1. RNA targeting by the type III-A CRISPR-Cas Csm complex of Thermus thermophilus.

Author

Staals, Raymond HJ, Zhu, Yifan, Taylor, David W, Kornfeld, Jack E, Sharma, Kundan, Barendregt, Arjan, Koehorst, Jasper J, Vlot, Marnix, Neupane, Nirajan, Varossieau, Koen, Sakamoto, Keiko, Suzuki, Takehiro, Dohmae, Naoshi, Yokoyama, Shigeyuki, Schaap, Peter J, Urlaub, Henning, Heck, Albert JR, Nogales, Eva, Doudna, Jennifer A, Shinkai, Akeo, and van der Oost, John

Subjects

Thermus thermophilus, Endoribonucleases, Bacterial Proteins, RNA, Bacterial, Microscopy, Electron, Amino Acid Sequence, Base Sequence, Protein Structure, Quaternary, Protein Binding, Models, Molecular, Molecular Sequence Data, RNA Cleavage, Clustered Regularly Interspaced Short Palindromic Repeats, CRISPR-Associated Proteins, RNA, Bacterial, Microscopy, Electron, Protein Structure, Quaternary, Models, Molecular, Developmental Biology, Biological Sciences, Medical and Health Sciences

Abstract

CRISPR-Cas is a prokaryotic adaptive immune system that provides sequence-specific defense against foreign nucleic acids. Here we report the structure and function of the effector complex of the Type III-A CRISPR-Cas system of Thermus thermophilus: the Csm complex (TtCsm). TtCsm is composed of five different protein subunits (Csm1-Csm5) with an uneven stoichiometry and a single crRNA of variable size (35-53 nt). The TtCsm crRNA content is similar to the Type III-B Cmr complex, indicating that crRNAs are shared among different subtypes. A negative stain EM structure of the TtCsm complex exhibits the characteristic architecture of Type I and Type III CRISPR-associated ribonucleoprotein complexes. crRNA-protein crosslinking studies show extensive contacts between the Csm3 backbone and the bound crRNA. We show that, like TtCmr, TtCsm cleaves complementary target RNAs at multiple sites. Unlike Type I complexes, interference by TtCsm does not proceed via initial base pairing by a seed sequence.

Published

2014

2. Crystal structure of Brugia malayi venom allergen-like protein-1 (BmVAL-1), a vaccine candidate for lymphatic filariasis

Author

Darwiche, Rabih, Lugo, Fernanda, Drurey, Claire, Varossieau, Koen, Smant, Geert, Wilbers, Ruud H.P., Maizels, Rick M., Schneiter, Roger, and Asojo, Oluwatoyin A.

Published

2018

3. The root-knot nematode effector MiMSP32 targets host 12-oxophytodienoate reductase 2 to regulate plant susceptibility

Author

Verhoeven, Ava, Finkers-Tomczak, Anna, Prins, Pjotr, Valkenburg-van Raaij, Debbie R, van Schaik, Casper C, Overmars, Hein, van Steenbrugge, Joris Jm, Tacken, Wannes, Varossieau, Koen, Slootweg, Erik J, Kappers, Iris F, Quentin, Michaël, Goverse, Aska, Sterken, Mark G, Smant, Geert, Verhoeven, Ava, Finkers-Tomczak, Anna, Prins, Pjotr, Valkenburg-van Raaij, Debbie R, van Schaik, Casper C, Overmars, Hein, van Steenbrugge, Joris Jm, Tacken, Wannes, Varossieau, Koen, Slootweg, Erik J, Kappers, Iris F, Quentin, Michaël, Goverse, Aska, Sterken, Mark G, and Smant, Geert

Abstract

To establish persistent infections in host plants, herbivorous invaders, such as root-knot nematodes, must rely on effectors for suppressing damage-induced jasmonate-dependent host defenses. However, at present, the effector mechanisms targeting the biosynthesis of biologically active jasmonates to avoid adverse host responses are unknown. Using yeast two-hybrid, in planta co-immunoprecipitation, and mutant analyses, we identified 12-oxophytodienoate reductase 2 (OPR2) as an important host target of the stylet-secreted effector MiMSP32 of the root-knot nematode Meloidogyne incognita. MiMSP32 has no informative sequence similarities with other functionally annotated genes but was selected for the discovery of novel effector mechanisms based on evidence of positive, diversifying selection. OPR2 catalyzes the conversion of a derivative of 12-oxophytodienoate to jasmonic acid (JA) and operates parallel to 12-oxophytodienoate reductase 3 (OPR3), which controls the main pathway in the biosynthesis of jasmonates. We show that MiMSP32 targets OPR2 to promote parasitism of M. incognita in host plants independent of OPR3-mediated JA biosynthesis. Artificially manipulating the conversion of the 12-oxophytodienoate by OPRs increases susceptibility to multiple unrelated plant invaders. Our study is the first to shed light on a novel effector mechanism targeting this process to regulate the susceptibility of host plants.

Published

2023

4. The root-knot nematode effector MiMSP32 targets host 12-oxophytodienoate reductase 2 to regulate plant susceptibility

Author

Plant Stress Resilience, Sub Plant Stress Resilience, Verhoeven, Ava, Finkers-Tomczak, Anna, Prins, Pjotr, Valkenburg-van Raaij, Debbie R, van Schaik, Casper C, Overmars, Hein, van Steenbrugge, Joris Jm, Tacken, Wannes, Varossieau, Koen, Slootweg, Erik J, Kappers, Iris F, Quentin, Michaël, Goverse, Aska, Sterken, Mark G, Smant, Geert, Plant Stress Resilience, Sub Plant Stress Resilience, Verhoeven, Ava, Finkers-Tomczak, Anna, Prins, Pjotr, Valkenburg-van Raaij, Debbie R, van Schaik, Casper C, Overmars, Hein, van Steenbrugge, Joris Jm, Tacken, Wannes, Varossieau, Koen, Slootweg, Erik J, Kappers, Iris F, Quentin, Michaël, Goverse, Aska, Sterken, Mark G, and Smant, Geert

Published

2023

5. The root-knot nematode effector MiMSP32 targets host 12-oxophytodienoate reductase 2 (OPR2) to regulate plant susceptibility

Author

Verhoeven, Ava, Finkers‐Tomczak, Anna, Prins, Pjotr, Valkenburg‐van Raaij, Debbie R., Van Schaik, Casper C., Overmars, Hein, Van Steenbrugge, Joris J.M., Tacken, Wannes, Varossieau, Koen, Slootweg, Erik J., Kappers, Iris F., Quentin, Michaël, Goverse, Aska, Sterken, Mark G., Smant, Geert, Verhoeven, Ava, Finkers‐Tomczak, Anna, Prins, Pjotr, Valkenburg‐van Raaij, Debbie R., Van Schaik, Casper C., Overmars, Hein, Van Steenbrugge, Joris J.M., Tacken, Wannes, Varossieau, Koen, Slootweg, Erik J., Kappers, Iris F., Quentin, Michaël, Goverse, Aska, Sterken, Mark G., and Smant, Geert

Abstract

To establish persistent infections in host plants, herbivorous invaders, such as root-knot nematodes, must rely on effectors for suppressing damage-induced jasmonate-dependent host defenses. However, at present, the effector mechanisms targeting the biosynthesis of biologically active jasmonates to avoid adverse host responses are unknown.Using yeast-two-hybrid, in planta co-immunoprecipitation, and mutant analyses, we identified 12-oxophytodienoate reductase 2 (OPR2) as an important host target of the stylet-secreted effector MiMSP32 of the root-knot nematode Meloidogyne incognita. MiMSP32 has no informative sequence similarities with other functionally annotated genes but was selected for the discovery of novel effector mechanisms based on evidence of positive, diversifying selection.OPR2 catalyzes the conversion of a derivative of 12-oxophytodienoate to jasmonic acid (JA) and operates parallel to 12-oxophytodienoate reductase 3 (OPR3), which controls the main pathway in the biosynthesis of jasmonates. We show that MiMSP32 targets OPR2 to promote parasitism of M. incognita in host plants independent of OPR3-mediated JA biosynthesis.Artificially manipulating the conversion of the 12-oxophytodienoate by OPRs increases susceptibility to multiple unrelated plant invaders. Our study is the first to shed light on a novel effector mechanism targeting this process to regulate susceptibility of host plants

Published

2023

6. The root‐knot nematode effector MiMSP32 targets host 12‐oxophytodienoate reductase 2 to regulate plant susceptibility

Author

Verhoeven, Ava, primary, Finkers‐Tomczak, Anna, additional, Prins, Pjotr, additional, Valkenburg‐van Raaij, Debbie R., additional, van Schaik, Casper C., additional, Overmars, Hein, additional, van Steenbrugge, Joris J. M., additional, Tacken, Wannes, additional, Varossieau, Koen, additional, Slootweg, Erik J., additional, Kappers, Iris F., additional, Quentin, Michaël, additional, Goverse, Aska, additional, Sterken, Mark G., additional, and Smant, Geert, additional

Published

2023

7. β-Hexosaminidases Along the Secretory Pathway of Nicotiana benthamiana Have Distinct Specificities Toward Engineered Helminth N-Glycans on Recombinant Glycoproteins

Author

Alvisi, Nicolò, Noort, Kim, van, Dwiani, Sarlita, Geschiere, Nathan, Sukarta, Octavina, Varossieau, Koen, Nguyen, Dieu-Linh, Strasser, Richard, Hokke, Cornelis H., Schots, Arjen, Wilbers, Ruud H.P., Alvisi, Nicolò, Noort, Kim, van, Dwiani, Sarlita, Geschiere, Nathan, Sukarta, Octavina, Varossieau, Koen, Nguyen, Dieu-Linh, Strasser, Richard, Hokke, Cornelis H., Schots, Arjen, and Wilbers, Ruud H.P.

Abstract

Secretions of parasitic worms (helminths) contain a wide collection of immunomodulatory glycoproteins with the potential to treat inflammatory disorders, like autoimmune diseases. Yet, the identification of single molecules that can be developed into novel biopharmaceuticals is hampered by the limited availability of native parasite-derived proteins. Recently, pioneering work has shown that helminth glycoproteins can be produced transiently in Nicotiana benthamiana plants while simultaneously mimicking their native helminth N-glycan composition by co-expression of desired glycosyltransferases. However, efficient “helminthization” of N-glycans in plants by glyco-engineering seems to be hampered by the undesired truncation of complex N-glycans by β-N-acetyl-hexosaminidases, in particular when aiming for the synthesis of N-glycans with antennary GalNAcβ1-4GlcNAc (LacdiNAc or LDN). In this study, we cloned novel β-hexosaminidase open reading frames from N. benthamiana and characterized the biochemical activity of these enzymes. We identified HEXO2 and HEXO3 as enzymes responsible for the cleavage of antennary GalNAc residues of N-glycans on the model helminth glycoprotein kappa-5. Furthermore, we reveal that each member of the HEXO family has a distinct specificity for N-glycan substrates, where HEXO2 has strict β-galactosaminidase activity, whereas HEXO3 cleaves both GlcNAc and GalNAc. The identification of HEXO2 and HEXO3 as major targets for LDN cleavage will enable a targeted genome editing approach to reduce undesired processing of these N-glycans. Effective knockout of these enzymes could allow the production of therapeutically relevant glycoproteins with tailor-made helminth N-glycans in plants.

Published

2021

8. β-Hexosaminidases Along the Secretory Pathway of Nicotiana benthamiana Have Distinct Specificities Toward Engineered Helminth N-Glycans on Recombinant Glycoproteins

Author

Alvisi, Nicolò, primary, van Noort, Kim, additional, Dwiani, Sarlita, additional, Geschiere, Nathan, additional, Sukarta, Octavina, additional, Varossieau, Koen, additional, Nguyen, Dieu-Linh, additional, Strasser, Richard, additional, Hokke, Cornelis H., additional, Schots, Arjen, additional, and Wilbers, Ruud H. P., additional

Published

2021

9. RNA Targeting by the Type III-A CRISPR-Cas Csm Complex of Thermus thermophilus

Author

Sub Biomol.Mass Spectrometry & Proteom., Sub Biomol.Mass Spect. and Proteomics, Biomolecular Mass Spectrometry and Proteomics, Molecular Pharmacy, Staals, Raymond H J, Zhu, Yifan, Taylor, David W, Kornfeld, Jack E, Sharma, Kundan, Barendregt, Arjan, Koehorst, Jasper J, Vlot, Marnix, Neupane, Nirajan, Varossieau, Koen, Sakamoto, Keiko, Suzuki, Takehiro, Dohmae, Naoshi, Yokoyama, Shigeyuki, Schaap, Peter J, Urlaub, Henning, Heck, Albert J R, Nogales, Eva, Doudna, Jennifer A, Shinkai, Akeo, van der Oost, John, Sub Biomol.Mass Spectrometry & Proteom., Sub Biomol.Mass Spect. and Proteomics, Biomolecular Mass Spectrometry and Proteomics, Molecular Pharmacy, Staals, Raymond H J, Zhu, Yifan, Taylor, David W, Kornfeld, Jack E, Sharma, Kundan, Barendregt, Arjan, Koehorst, Jasper J, Vlot, Marnix, Neupane, Nirajan, Varossieau, Koen, Sakamoto, Keiko, Suzuki, Takehiro, Dohmae, Naoshi, Yokoyama, Shigeyuki, Schaap, Peter J, Urlaub, Henning, Heck, Albert J R, Nogales, Eva, Doudna, Jennifer A, Shinkai, Akeo, and van der Oost, John

Published

2014

10. Crystal structure of Brugia malayi venom allergen-like protein-1 (BmVAL-1), a vaccine candidate for lymphatic filariasis

Author

Darwiche, Rabih, Lugo, Fernanda, Drurey, Claire, Varossieau, Koen, Smant, Geert, Wilbers, Ruud H. P., Maizels, Rick M., Schneiter, Roger, Asojo, Oluwatoyin A., Darwiche, Rabih, Lugo, Fernanda, Drurey, Claire, Varossieau, Koen, Smant, Geert, Wilbers, Ruud H. P., Maizels, Rick M., Schneiter, Roger, and Asojo, Oluwatoyin A.

Abstract

Brugia malayi is a causative agent of lymphatic filariasis, a major tropical disease. The infective L3 parasite stage releases immunomodulatory proteins including the venom allergen-like proteins (VALs), which are members of the SCP/TAPS (Sperm-coating protein/Tpx/antigen 5/pathogenesis related-1/Sc7) superfamily. BmVAL-1 is a major target of host immunity with >90% of infected B. malayi microfilaraemic cases being seropositive for antibodies to BmVAL-1. This study is part of ongoing efforts to characterize the structures and functions of important B. malayi proteins. Recombinant BmVAL-1 was produced using a plant expression system, crystallized and the structure was solved by molecular replacement and refined to 2.1 Å, revealing the characteristic alpha/beta/alpha sandwich topology of eukaryotic SCP/TAPS proteins. The protein has more than 45% loop regions and these flexible loops connect the helices and strands, which are longer than predicted based on other parasite SCP/TAPS protein structures. The large central cavity of BmVAL-1 is a prototypical CRISP cavity with two histidines required to bind divalent cations. The caveolin-binding motif (CBM) that mediates sterol binding in SCP/TAPS proteins is large and open in BmVAL-1 and is N-glycosylated. N-glycosylation of the CBM does not affect the ability of BmVAL-1 to bind sterol in vitro. BmVAL-1 complements the in vivo sterol export phenotype of yeast mutants lacking their endogenous SCP/TAPS proteins. The in vitro sterol-binding affinity of BmVAL-1 is comparable with Pry1, a yeast sterol transporting SCP/TAPS protein. Sterol binding of BmVAL-1 is dependent on divalent cations. BmVAL-1 also has a large open palmitate-binding cavity, which binds palmitate comparably to tablysin-15, a lipid-binding SCP/TAPS protein. The central cavity, CBM and palmitate-binding cavity of BmVAL-1 are interconnected within the monomer with channels that can serve as pathways for water molecules, cations and small molecules.