Purification and pharmacological properties of eight sea anemone toxins from Anemonia sulcata, Anthopleura xanthogrammica, Stoichactis giganteus and Actinodendron plumosum

Schweitz, Hugues; Vincent, Jean Pierre; Barhanin, Jacques; Frelin, Christian; Linden, G.; Hugues, Michel; Lazdunski, Michel

doi:10.1021/bi00521a023

Cited by 131 publications

(72 citation statements)

References 38 publications

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“…ATX I was extracted from the venom of Anemoniu sulcata and purified as described elsewhere [27]. In a further purification step the two polypeptides with either Ala (ATX Ia) or Pro (ATX Ib) in position 3 ( Fig.…”

Section: Sample Preparationmentioning

confidence: 99%

The secondary structure of the toxin ATX Ia from Anemonia sulcata in aqueous solution determined on the basis of complete sequence‐specific ¹H‐NMR assignments

Widmer¹,

Wagner²,

Schweitz³

et al. 1988

European Journal of Biochemistry

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The toxin preparations ATX I, ATX Ia and ATX Ib from Anemonia sulcata were investigated by proton nuclear magnetic resonance (NMR). High-resolution phase-sensitive two-dimensional NMR experiments were used to monitor the separation by high-performance liquid chromatography of the two isoproteins ATX Ia and ATX Ib. For ATX Ia complete sequence-specific resonance assignments were obtained and the secondary structure was determined. To obtain the NMR assignments we used a variant of the sequential assignment technique which relied extensively on cross-peak fine-structure analysis in phase-sensitive spectra, using spectrum simulations based on density matrix calculations with the program SPHINX. These procedures, which resulted in extensive amino acid spin system identifications prior to the sequential assignments, should be generally applicable for small proteins with relatively narrow 'H-NMR lines. The secondary structure of ATX I includes a / 3 sheet consisting of four strands. No evidence was found for the presence of regular helical segments. The four p strands are connected by two extended loops and a tight turn, for which further characterization has to await the complete determination of the three-dimensional structure.The venom of sea anemones contains several polypeptides with neurotoxic and cardiotoxic activities [l], which affect the duration of the action potential in the course of the nerve impulse. The sodium channel inactivation is slowed down and thus the force of the cardiac contraction is increased by these toxins. Purification procedures and the amino acid sequences of four different polypeptide toxins from Anemonia sulcata are known, i.e. ATX I, ATX 11, ATX 111, and ATX V [2 -81. These proteins consist of 46, 47, 27, and 46 amino acid residues, respectively, with a high degree of sequence homology between ATX I, ATX 11, and ATX V. Each toxin has three disulfide bridges, of which the positions were directly determined only for ATX I1 [9]. Fig. 1 shows the sequence and the disulfide bridges of ATX I. When the different toxins are tested on mammals, ATX I1 is 50 -100-fold more toxic than ATX I, but five times less toxic than ATX V [S].Correspondence to K. Wuthrich, Institut fur Molekularbiologie und Biophysik, Eidgenossische Technische Hochschule ZurichHonggerberg, CH-8093 Zurich, SwitzerlandAbbreviations. 1 D, one-dimensional; 2D, two-dimensional; COSY, 2D correlated spectroscopy; 2QF-COSY, two-quantum filtered COSY; NOESY, two-dimensional nuclear Overhauser enhancement spectroscopy; RELAYED-COSY, two-dimensional relayed coherence transfer spectroscopy; DOUBLE-RELAYED-COSY, two-dimensional double-relayed coherence transfer spectroscopy; SPHINX, program for the simulation of high-resolution 2D NMR experiments; LINSHA, line shape simulation program; dAB (i, j ) , distance between the proton types A and B located, respectively, in the amino acid residues i and j , where N, GI, and B denote the amide proton, aH, and BH, with the following abbreviations for The physiological activities of the sea anem...

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Section: Sample Preparationmentioning

confidence: 99%

The secondary structure of the toxin ATX Ia from Anemonia sulcata in aqueous solution determined on the basis of complete sequence‐specific ¹H‐NMR assignments

Widmer¹,

Wagner²,

Schweitz³

et al. 1988

European Journal of Biochemistry

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“…It may be that the toxin is more active on Ca2+ channels of animals of marine origin. Affinities for other polypeptide toxins on Na+ channels are also known to be very dependent on the animal species [28,29].…”

Section: Resultsmentioning

confidence: 99%

A polypeptide toxin from the coral Goniopora

et al. 1986

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A polypeptide toxin has been isolated from Goniopora coral with an M r of 19000. Goniopora toxin has the following properties: (i) it induces contraction of guinea pig ileum and this contraction is prevented by Ca2+‐channel blockers; (ii) it stimulates 45Ca2+ influx in cardiac cells in culture and this stimulation is abolished by Ca2+‐channel blockers; (iii) it prevents binding of (+)‐[3H]PN 200‐110 to the Ca2+‐channel protein of skeletal muscle T‐tubule membranes. All these results taken together suggest that Goniopora toxin is a Ca2+‐channel activator.

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“…In spite of its hydrophobic character, and it most probable overall rigidity, ATX I11 is immunogenic. From a pharmacological point of view ATX I, I1 and I11 are highly toxic to crabs [26] and ATX I1 binds specifically to receptor sites at the level of the sodium channel and can displace Androctonus australis Hector scorpion a-toxin I1 from its receptor sites. There is, however, no sequence similarity between ATX I11 and ATX 11.…”

Section: Discussionmentioning

confidence: 99%

Specificity of antibodies to sea anemone toxin III and immunogenicity of the pharmacological site of anemone and scorpion toxins

Bahraoui

Ayeb

Granier

et al. 1989

European Journal of Biochemistry

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Toxin I11 (ATX 111) of the sea anemone (Anemonia sulcata) is a polypeptide containing 27 amino acid residues.It has no sequence similarity with other toxins (ATX I and 11) from the same species, or with scorpion toxins, although they apparently act in a similar manner by prolonging action potentials. The specificity of ATX I11 antibodies was characterized using ATX 111, ATX I, native and chemically modified ATX 11, and scorpion atoxins. The results obtained suggest that a region of ATX 111, partially or totally overlapping the pharmacological site shared with ATX I and ATX 11, is immunogenic. It includes a guanidino and at least two carboxylate groups. The corresponding region is not immunogenic in ATX I and ATX 11. Anti-(ATX 111) antibodies recognize the similar regions of ATX I and ATX I1 and apparently do not recognize scorpion toxins.The voltage-sensitive Na' -channel plays a major role in nerve and muscle action potentials. One group of neurotoxins causes repetitive action potentials and persistent nerve depolarization: (a) tetrodotoxin and saxitoxin block Na' entry through the Na' channel (0 ciguatoxin and brevetoxin depolarize excitable membranes by selectively opening one class of sodium channels [13, 141. Sea anemone and scorpion a-toxins apparently act in a similar manner by prolonging action potentials. They seem to bind to a common site and can maintain the Na+ channel open by decreasing its rate of inactivation [9-111. Possible structural similarities that may explain this similar mode of action have not yet been defined; X-ray crystallography [15] and chemical modification studies [16 -181 have suggested that a conserved and hydrophobic, but accessible, surface may constitute the receptor-binding site of scorpion toxins, but no such data are available for anemone toxins.Previous immunochemical studies of the anemone toxin system showed a cross-antigenicity between ATX I and I1 from Anemonia sulcata. On the other hand, there was no crossantigenicity with ATX 111, a polypeptide containing 27 amino acid residues, or with scorpion a-toxins when anti-(ATX I) or anti-(ATX 11) antibodies were used [19]. Assuming these molecules share some common functional structure enabling them to bind to a common receptor site, the absence of immunological cross-reactivity suggests that the pharmacological site(s) of ATX I, ATX I1 and scorpion a-toxins is not immunogenic. The purpose of the present work was to prepare anti-(ATX 111) antibodies and characterize their specificity towards ATX 111, ATX I and ATX I1 and its chemical derivatives, and scorpion a-toxins. MATERIALS AND METHODS MATERIALSLactoperoxidase was obtained from Sigma. CNBrSepharose-C14B, Sephadex G-25 and protein-A -Sepharose were purchased from Pharmacia. Bio-Gel P2 and P6 were obtained from Bio-Rad. Na "' I (13-17 mCi/g was obtained from Amersham. Donkey RDI7 anti-(rabbit immunoglobulin) serum was purchased from Wellcome. Non-immune rabbit serum was prepared in the laboratory. Reagents for chemical modification were from Roche (fluorescamine), Fluka...

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Purification and pharmacological properties of eight sea anemone toxins from Anemonia sulcata, Anthopleura xanthogrammica, Stoichactis giganteus and Actinodendron plumosum

Cited by 131 publications

References 38 publications

The secondary structure of the toxin ATX Ia from Anemonia sulcata in aqueous solution determined on the basis of complete sequence‐specific ¹H‐NMR assignments

The secondary structure of the toxin ATX Ia from Anemonia sulcata in aqueous solution determined on the basis of complete sequence‐specific ¹H‐NMR assignments

A polypeptide toxin from the coral Goniopora

Specificity of antibodies to sea anemone toxin III and immunogenicity of the pharmacological site of anemone and scorpion toxins

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Purification and pharmacological properties of eight sea anemone toxins from Anemonia sulcata, Anthopleura xanthogrammica, Stoichactis giganteus and Actinodendron plumosum

Cited by 131 publications

References 38 publications

The secondary structure of the toxin ATX Ia from Anemonia sulcata in aqueous solution determined on the basis of complete sequence‐specific 1H‐NMR assignments

The secondary structure of the toxin ATX Ia from Anemonia sulcata in aqueous solution determined on the basis of complete sequence‐specific 1H‐NMR assignments

A polypeptide toxin from the coral Goniopora

Specificity of antibodies to sea anemone toxin III and immunogenicity of the pharmacological site of anemone and scorpion toxins

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The secondary structure of the toxin ATX Ia from Anemonia sulcata in aqueous solution determined on the basis of complete sequence‐specific ¹H‐NMR assignments

The secondary structure of the toxin ATX Ia from Anemonia sulcata in aqueous solution determined on the basis of complete sequence‐specific ¹H‐NMR assignments