Abstract
BackgroundMore than 200 Scyphozoa species have been described, but few have been properly studied regarding their chemical and genetic characteristics. Catostylus tagi, an edible Scyphozoa and the sole European Catostylidae, occurs in summer at Tagus and Sado estuaries. Neither a systematic comparison between the two Catostylus communities nor a chemical approach on their nematocytes had been carried out yet.MethodsIn order to achieve these purposes, optimisation of DNA extraction and of histochemical staining procedures were developed. Catostylus specimens from Tagus and Sado estuaries were compared by ribosomal 18S, 28S, and ITS1 partial sequencing. The morphochemistry of nematocytes was studied by optical and electronic microscopy.ResultsMacroscopic and molecular results indicated that both communities belong to the same species, C. tagi. The hematoxylin and eosin staining allowed the visualisation of nematocyst genesis and indicated a basic character for the macromolecules on the shaft of euryteles and on the tubule of isorhizae and birhopaloids. By Masson’s trichrome procedure, the basic properties of the tubules were confirmed and a collagenous profile for the toxins was suggested. Results of the alcian blue staining showed that the outer membrane of nematocyte may consist of macromolecules with acidic polysaccharides, consistent with NOWA and nematogalectin glycoproteins detected in Hydra, but also with poly-gamma-glutamate complex, chitin-like polysaccharides and hyaluronic acids. Through the von Kossa assays, calcium was detected; its position suggested interactions with polysaccharides of the membrane, with proteins of the contractile system or with both.ConclusionsThe optimisation of sample preparation for DNA extraction may facilitate further studies on little known jellyfish species. The improvement of the smear procedure simplified the use of stained reactions in zooplankton. Moreover, it was shown that good slide images might be acquired manually. The development of specific reactions, with traditional dyes and others, can give important contributions to clarify the chemical nature of the components of nematocytes. The characterisation of nematocyst toxins by staining tests is a goal to achieve.
Highlights
More than 200 Scyphozoa species have been described, but few have been properly studied regarding their chemical and genetic characteristics
The present study proposes two optimisation procedures, one for genomic DNA extraction and another one for the histochemical staining of some structural compounds of nematocytes, which were applied to the scyphozoan Catostylus tagi (Haeckel, 1869), the sole European specie of Catostylidae family
The observations by optical microscopy indicated no significant variances in Catostylus samples from Tagus and Sado
Summary
More than 200 Scyphozoa species have been described, but few have been properly studied regarding their chemical and genetic characteristics. Neither a systematic comparison between the two Catostylus communities nor a chemical approach on their nematocytes had been carried out yet. In the case of cnidarians, the primary commonality is the occurrence of cnidocyte (mostly known as nematocyte), a specialized cell which synthesizes an organelle named cnidocyst (usually referred as nematocyst). The nematocyst consists of a capsule with a coiled tubule inside containing toxins. The capsule opens, through the operculum, and the tubule and toxins are rapidly ejected to outside, in attack or defense actions. About 30 types of nematocysts are recognized, mainly based on Weill’s morphological classification of the tubule and the capsule [3]
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