Novel peptide toxins from the sea anemone Stichodactyla haddoni

Four peptide toxins, SHTX I-III with crab-paralyzing activity and SHTX IV with crab lethality, were isolated from the sea anemone Stichodactyla haddoni and their primary structures elucidated by protein sequencing and cDNA cloning. SHTX I (new toxin, 28 residues), II (analogue of SHTX I, 28 residues) and III (Kunitz-type protease inhibitor, 62 residues) are potassium channel toxins and SHTX IV (48 residues) is a member of the type 2 sea anemone sodium channel toxins. The precursor protein of SHTX IV is composed of a signal peptide, propart and mature peptide, while the propart is missing in that of SHTX III. In addition to these four toxins, an epidermal growth factor-like peptide was detected in S. haddoni by RT-PCR.     

Occurrence ofByronia Matthew andSphenothallus Hall in the Lower Cambrian of China

Rare phosphatic tubular fossils from the Lower-Middle Cambrian Kaili Formation of Guizhou Province, southern China were originally identified as non-calcified algae or ‘worms’ (ScoleciellusLiu). Re-examination of these fossils indicates that specimens identified as non-calcified algae areSphenothallus taijiangensis n. sp., while specimens identified asScoleciellus belong toByronia natus (Liu).Sphenothallus taijiangensis andByronia natus from Lower Cambrian strata in the Kaili Formation are the oldest known representatives of their genera. In addition,B. natus (Liu) is the only known species ofByronia with the exception ofB. annulata Matthew (Middle Cambrian, British Columbia). CambrovitusMao et al., a tubular fossil from Middle Cambrian strata in the Kaili Formation, originally was classified as a hyolithid. However, the discovery of a nearly complete specimen possessing an apical attachment disk shows thatCambrovitus, likeByronia andSphenothallus, probably was a thecate cnidarian polyp.     

Cytotoxicity of the nematocyst venom from the sea anemone Aiptasia mutabilis

Crude extracts of the coelenterate Aiptasia mutabilis (Anthozoa, Aiptasiidae) nematocysts have been tested for their cytotoxicity of Vero and HEp-2 cells monolayers. The results indicate that the nematocyte venom contains one or more toxins with an extremely powerful cytolytic activity. An extract containing the equivalent of as little as 0.6 nematocysts/microL is sufficient to induce significant cellular necrosis, and IC50 can be estimated to be ca. 2 nematocysts/microL on Vero cells. These values are 1-2 orders of magnitude lower than those reported so far for other sea anemone venoms. The extreme potency is accompanied by poor stability of the venom that is readily inactivated by moderate heat and by buffers at non-neutral pH values. The extract is unstable even when kept for short times at 4 degrees C, or after storage at -20 degrees C. Separation of crude venom by affinity chromatography on ConA-Sepharose allowed us to identify two main components with molecular masses of 95 and 31 kDa, respectively, as responsible for the cytolytic properties of A. mutabilis nematocyst extract.     

Modification of the neurotoxin RTX-III from the sea anemone Radianthus macrodactylus

The influence of chemical modification on neurotoxin RTX-III toxicity in mice has been studied. The toxicity was not affected by modification of Trp30 residue with 2-hydroxy-5-nitrobenzyl bromide but was diminished by a factor of 100 after reduction of the toxin's two disulfide bonds with 2-mercaptoethanol followed by derivatization with iodoacetamide. Blocking carboxyl groups with [3H]glycine methyl ester in the presence of 1-ethyl-3-(3-dimethylaminopropyl)carbodiimide led to only a two-fold drop in toxicity in the case of monocarboxylate-modified derivatives and a six-fold decrease for dimodified derivatives. A conception of multipoint attachment of the toxin to sodium channel is discussed.     

Primary structures of actinoporins from sea anemone Oulactis orientalis

Partial amino acid sequences of the actinoporins Or-A (136 aa) and Or-G (144 aa) isolated from the Sea of Japan sea anemone Oulactis orientalis were determined by sequencing the clones obtained by the amplification of genomic DNA and cDNA with specific primers to the N-terminal regions of the 0. orientalis actinoporin sequences and to the C-terminal region, which is known to be highly conservative in all the known actinoporin sequences. The complete structures of Or-A (165 aa) and Or-G (173 aa) were established by sequencing the cDNA clones obtained by the fast amplification of 3'-ends of cDNA. A comparative analysis of the amino acid sequences of the Oulactis actinoporins with those of actinoporins from tropical species revealed considerable differences in the structures of their N-terminal fragments and their membrane-binding sites. We believe that these differences could explain lower hemolytic activities of Or-A and Or-G than that of actinoporins from the tropical species.     

Toxins of the sea anemone Epiactis prolifera

Fe³⁺-EDTA chelates react with the superoxide radical at physiological pH values (k = 1.3 × 10⁶M^?1 s^?1 at pH 7 but is lower at more alkaline pH values) but do not appear to catalyze O₂^? dismutation at a significant rate. Complexes of Fe³⁺ with desferrioxamine, bathophenanthroline, or diethylenetriaminepentaacetic acid react much more slowly, if at all. Fe²⁺ complexes of EDTA, ATP, and diethylenetriaminepentaacetic acid also react with O₂^? at alkaline pH values. The significance of these reactions in the mechanism of the “iron-catalyzed Haber-Weiss reaction” is discussed.     

A cholesterol-inhibitable cytolytic from the sea anemone Metridium senile

The tissues of the common North Atlantic sea anemone, Metridium senile, contain an agent capable of lysing mammalian cells. The active substance, metridiolysin, was purified and found to be a protein of molecular weight approx. 80 000 and to be isoelectric at approx. pH 5.0. It is thermolabile and is inactivated by Pronase and subtilisin. The optimal pH for hemolysis is between 5 and 6, and at pH 8.0 or higher the lysin is inactive. It can be dissociated into two subunits of unequal size. Metridiolysin destroys blood platelets in vitro as well as cultured fibroblasts, and is lethal when injected intravenously into mice. It is not lytic for bacterial protoplasts and spheroplasts. Hemolysis is specifically prevented by cholesterol. Erythrocytes from the horse and dog are approx. 100 times as sensitive to lysis as those from the mouse, and erythrocytes from other animals tested are intermediate in sensitivity.     

Properties of allelic variants of phosphoglucomutase from the sea anemone Metridium senile

The phosphoglucomutase (Pgm) locus from populations of the sea anemone Metridium senile has three alleles in natural populations from the northeastern coast of North America. Two of the alleles exhibit clinal variation north of Cape Cod, suggesting a possible association of allele frequency with environmental temperature. This clinal pattern is reproducible and stable over at least brief periods of time. The allozymes encoded by each of the six Pgm genotypes have been partially purified and characterized. The symmetrical pH optimum for Vmax is pH 7.5; the apparent Km (Kmapp) of glucose-1-phosphate declines monotonically as the pH increases from 6.5 to 8.5. There are no pronounced differences in heat stabilities of PGM produced by various genotypes, nor are there significant differences in specific activities. There are no differences in the sensitivity of Vmax to temperature. Kmapp values are very low for all genotypes, ranging from about 2 to 12 microM, depending upon the temperature. Kmapp of glucose-1-phosphate declines as the temperature is raised for all genotypes, whether the pH is held constant or allowed to vary with the temperature. Under certain conditions, there are small significant differences among genotypes in Kappm values, but there is no systematic pattern to these differences. The present data provide no biochemical explanation for the maintenance of the Pgm cline by selection for functional differences under different thermal regimes.     

Cooperativity in the two-domain arginine kinase from the sea anemone Anthopleura japonicus

cDNAs of the two-domain arginine kinase (AK) (contiguous dimer; denoted by 2D/WT) and its separated domains 1 and 2 (denoted by D1/WT and D2/WT) from the sea anemone Anthopleura japonicus, were cloned into the plasmid pMAL, and recombinant enzymes were expressed in E. coli as MBP fusion proteins. The kinetic parameters kcat, Ka and Kia, were determined for all three AKs. All three enzymes showed distinct AK activity, and had high affinity for arginine (Ka Arg=0.25-0.48 mM). The catalytic efficiency, calculated by kcat/Ka ArgKia ATP, of the 2D/WT enzyme (182 mM(-2)s(-1), the value for one active 40 kDa domain) was two- to three-times higher than values for either D1/WT or D2/WT (80.2 and 86.4mM(-2)s(-1), respectively), suggesting the presence of domain-domain interactions (cooperativity) in the contiguous dimer. The Kia/Ka values of the three enzymes ranged from 0.88 to 1.32, indicating that there is no strong synergism in substrate binding, as seen in typical AKs. Asp62 and Arg193, which are conserved in most AKs and play a key role in stabilizing the substrate-bound structure, are also conserved in the two domains of Anthopleura AK. We replaced Asp62 in D2/WT with Glu or Gly. The catalytic efficiency and Kia/Ka for the D62E mutant were comparable to those of D2/WT, but catalytic efficiency for the D62G mutant was decreased to 13% of that of the D2/WT with a significantly increased value of Kia/Ka (1.92), indicating that Asp62 plays an important role in the expression of AK activity.     

Chemical synthesis of a neurotoxic polypeptide from the sea anemone Stichodactyla helianthus

The sea anemone Stichodactyla helianthus neurotoxin I, a 48-residue polypeptide, was synthesized by automated solid phase methodology. The fully reduced polypeptide was subsequently refolded in the presence of a glutathione oxidoreduction buffer to the biologically active species containing three disulfide bonds. The overall yield after rigorous purification was 12.5%. The circular dichroism (CD), and proton nuclear magnetic resonance (1H NMR) spectra of the HPLC-purified synthetic toxin were indistinguishable from those obtained concurrently with the natural toxin. A subtilisin digest of the synthetic neurotoxin generated peptide fragments identical to that of a sample of the natural toxin subjected to the same treatment. The toxicity of the synthetic polypeptide was identical to that of the natural toxin (crab LD50, 3.1 micrograms/kg). The equilibrium dissociation constant (28 nM) for interaction of the synthetic toxin with crab axolemma vesicles was nearly identical to that of the natural toxin (25 nM).     

Pharmacological effects of two cytolysins isolated from the sea anemone Stichodactyla helianthus

Sticholysins I and II (St I/II) are cytolysins purified from the sea anemone Stichodactyla helianthus. In this study, we show their pharmacological action on guinea-pig and snail models in native and pH-denatured conditions in order to correlate the pharmacological findings with the pore-forming activity of both isoforms. In guinea-pig erythrocytes (N = 3), St II possessed higher haemolytic activity in comparison with St I and this activity was lost at an alkaline pH. In molluscan central neurons (N = 30), they irreversibly decreased the amplitude of the cholinergic response; St I (EC ₅₀ 0.6 µmolL^?1) was more potent than St II (EC₅₀ >6.6 µmolL^?1) and they both increased the duration of the action potential; these effects were absent at an alkaline pH. In guinea-pig isolated atrium (N = 25), both increased the amplitude of the contraction force, but St II was more potent than St I (EC₅₀ 0.03 µmolL^?1 and 0.3 µmolL^?1, respectively) and this effect persisted at an alkaline pH. In summary, both cytolysins have neuroactive and cardioactive properties. The main mechanism in molluscan neurons seems to be associated with the cytolytic activity of these molecules, whereas in guinea-pig atrium, the existence of an additional pharmacological mechanism might be contributing to the observed effect.     

Embryonic and larval development of the sea anemone Haliplanella lineata from Japan

The development of Haliplanella lineata, following fertilization in the laboratory, was studied by light and electron microscopy. Spawned ova were spherical, magenta in color and about 120–150 µm in diameter. Cleavage was holoblastic and radial. Gastrulation occurred by immigration and invagination. Eighteen hours after fertilization, the embryo became a swimming planula larva with an apical organ and ciliary tuft at the aboral end. In the laboratory, planulae lived for about 2 weeks in the swimming state but in no case was there any settlement by larvae in this study. The structural study of planulae concentrated on the development of the aboral ectoderm, because of the functional significance of its cellular organization in larval settlement.     

Cloning of a novel G-protein-coupled receptor from the sea anemone nervous system

We describe the cloning and analysis of genomic and cDNA copies of a gene from sea anemones that encodes a new member of the G-protein-coupled receptor family. The receptor shows similarity to previously described receptors for biogenic amines such as adrenaline, serotonin, and octopamine, as well as a variety of small molecule agonists and peptides, although we have been unable to determine which ligand is the natural agonist. Antibodies generated against the recombinant receptor protein identify a single protein with a molecular weight of 66 kDa in membrane preparations. Immunofluorescence studies using the same antibody have enabled localization of the receptor in the nervous system. Western blotting and RT-PCR analysis reveal that a homologue of this receptor is expressed in jellyfish and soft coral. We suggest that the receptor plays a role in neurotransmission in the sea anemone and other members of the phylum Cnidaria.     

Amino acid sequence of neurotoxin II from the sea anemone Radianthus macrodactylus

Amino acid sequence of neurotoxin II isolated from the sea anemone Radianthus macrodactylus was determined by analysis of peptides obtained after its digestion with trypsin and staphylococcal proteinase. It is shown that the polypeptide chain of the toxin consists of 48 amino acid residues, including six cysteines.     

Conformational stability of serine proteinase inhibitor from the sea anemone Heteractis crispa

The influence of different environmental values of the pH and temperature on the spatial organization of serine proteinase inhibitor from the sea anemone Heteractis crispa (=Radianthus macrodactylus) on the level of tertiary and secondary structure was studied by CD spectroscopy. The molecule InhVJ was shown to possess a high conformational thermo- and pH-stability. We determined the point of conformational thermotransition of polypeptide (70 degrees C) after which the molecule gets denaturational stable state with conservation of 80% proteinase inhibitory activity. The significant partial reversible changes of molecule spatial organization were established to occur at the level of tertiary structure in the process of acid-base titration in the range of pH 11.0-13.0. This can be explained by of ionization of tyrosine residues. The molecule InhVJ is conformationally stable at the low pH values (2.0). The quenching of tyrosine residues by acrylamide showed that two of these residues are accessible to the quencher in full, while the third part is available.