Transition state analogues in structures of ricin and saporin ribosome-inactivating proteins

Ho, M.; Sturm, Matthew B.; Almo, Steven C.; Schramm, Vern L.

doi:10.1073/pnas.0911606106

Cited by 59 publications

(85 citation statements)

References 44 publications

(69 reference statements)

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“…5). Previous studies have identified that Glu-177 is critical for the depurination activity of ricin (5,6,9,12). Taken together, these data suggested that the ␣-helix may modulate the enzymatic activity of ricin by controlling the side chain orientation of Glu-177.…”

Section: Discussionsupporting

confidence: 60%

“…Recently, the transition state analogues in structures of ricin and saporin ribosome-inactivating proteins were studied. The data confirmed that the invariant residues of RIPs in the catalytic active site of ricin were essential for the efficient catalysis by RTA (9). Although the biochemical properties of RIPs have been extensively studied, the enzymatic mechanism of RIPs is still elusive.…”

supporting

confidence: 67%

“…5B). Previous studies have demonstrated that there are four amino acids (Tyr-80, Tyr-123, Glu-177, and Arg-180) critical for the depurination activity of ricin (6,9,12,25). To investigate how the flexibility of the ␣-helix affects the enzyme activity of ricin, we performed a dihedral angle analysis.…”

Section: Rips With Very Low Similarity In Primary Structure Arementioning

confidence: 99%

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Identification of a Novel Functional Domain of Ricin Responsible for Its Potent Toxicity

Dai

Lei

Yang

et al. 2011

Journal of Biological Chemistry

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Ribosome-inactivating proteins (RIPs) are toxic N-glycosidases that depurinate the universally conserved ␣-sarcin loop of large rRNAs. They have received attention in biological and biomedical research because of their unique biological activities toward animals and human cells as cell-killing agents. A better understanding of the depurination mechanism of RIPs could allow us to develop potent neutralizing antibodies and to design efficient immunotoxins for clinical use. Among these RIPs, ricin exhibited remarkable efficacy in depurination activity and highly conserved tertiary structure with other RIPs. It can be considered as a prototype to investigate the depurination mechanism of RIPs. In the present study, we successfully identified a novel functional domain responsible for controlling the depurination activity of ricin, which is located far from the enzymatic active site reported previously. Our study indicated that ricin A-chain mAbs binding to this domain (an ␣-helix comprising the residues 99 -106) exhibited an unusual potent neutralizing ability against ricin in vivo. To further investigate the potential role of the ␣-helix in regulating the catalytic activity of ricin, ricin A-chain variants with different flexibility of the ␣-helix were rationally designed. Our data clearly demonstrated that the flexibility of the ␣-helix is responsible for controlling the depurination activity of ricin and determining the extent of protein synthesis inhibition, suggesting that the conserved ␣-helix might be considered as a potential target for the prevention and treatment of RIP poisoning. Ribosome-inactivating proteins (RIPs)3 are depurinating rRNA N-glycosidases (E.C. 3.2.2.22) that cleave a single bond between a specific adenine and ribose of rRNA in eukaryotes (1). They are generally divided into two classes (1-3). Type I RIPs such as trichosanthin and gelonin are monomeric enzymes of ϳ30 kDa. Type II RIPs are heterodimeric proteins with an approximate molecular mass of 60 kDa, in which one polypeptide with RIP activity (A-chain) is linked by a disulfide bridge to a galactose-binding lectin (B-chain). The B-chain is able to bind to a galactose-containing receptor on the surface of sensitive cells and mediate transport of the A-chain through the secretory pathways into the cytoplasm.Ricin (a type II RIP), which has emerged as a powerful catalyst for mammalian ribosomes, is a good prototype to investigate the N-glycosidase mechanism of RIPs. Ricin A-chain (RTA) is the catalytic subunit of ricin, which catalyzes the depurination of an invariant adenosine residue, A 4324 , within the GA 4324 GA tetraloop motif of the highly conserved sarcinricin loop of eukaryotic 28 S rRNA (4). Most previous studies have focused on the role of the active-site residues that are crucial for catalytic activity of RIPs. Day et al. (5) have presented the crystal structure of ricin, indicating that RTA has a prominent cleft able to recognize the target rRNA stem-loop. Sitedirected mutagenesis, as well as analysis by systematic deletion ...

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Section: Discussionsupporting

confidence: 60%

supporting

confidence: 67%

Section: Rips With Very Low Similarity In Primary Structure Arementioning

confidence: 99%

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Identification of a Novel Functional Domain of Ricin Responsible for Its Potent Toxicity

Dai

Lei

Yang

et al. 2011

Journal of Biological Chemistry

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“…The epitope mainly con-tains the residues Asp 96 -Thr 116 , which forms the substrate binding pocket together with the residues Gly 120 -Asn 136 and residues Asp 201 -Ser 221 (7). To investigate whether 6C2 binding to RTA will change its structure near the enzyme activity center and eliminate the rRNA depurination activity of RTA, we compared the apo-form RTA (PDB code 2AAI) with the RTA in complex with 6C2 and a substrate analog (PDB codes 4KUC and 3HIO).…”

Section: Resultsmentioning

confidence: 99%

“…Recently, the structure of ricin was solved with transition state analogues bound, confirming that these invariant residues of the RIPs in the catalytic active site of ricin were essential for efficient catalysis by RTA (7). Although the biochemical properties of RIPs have been extensively studied, the enzymatic mechanism of RIPs remains elusive.…”

mentioning

confidence: 99%

Structural Insights into the Neutralization Mechanism of Monoclonal Antibody 6C2 against Ricin

Zhu

Dai

Zhang

et al. 2013

Journal of Biological Chemistry

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Background:The antibody 6C2 exhibited an unusually potent neutralizing ability against ricin. Results: We determined the crystal structure of 6C2 Fab in complex with RTA and mapped the epitope on RTA. Conclusion: The binding of 6C2 hinders the interaction between RTA and the ribosome, thus inhibiting the activities of RTA. Significance: Our findings further confirm the role of ribosomal elements in ricin activity and specificity.

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The Structure and Action of Ribosome‐inactivating Proteins

Robertus

Monzingo

2014

Ribosome‐inactivating Proteins

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Transition state analogues in structures of ricin and saporin ribosome-inactivating proteins

Cited by 59 publications

References 44 publications

Identification of a Novel Functional Domain of Ricin Responsible for Its Potent Toxicity

Identification of a Novel Functional Domain of Ricin Responsible for Its Potent Toxicity

Structural Insights into the Neutralization Mechanism of Monoclonal Antibody 6C2 against Ricin

The Structure and Action of Ribosome‐inactivating Proteins

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