Literature DB >> 28305154

Ultrastructural study of differentiation processes during aggregation of purified sponge archaeocytes.

Marco Buscema1, Danielle De Sutter1, Gysèle Van de Vyver1.   

Abstract

Archaeocytes from the spongeEphydatia fluviatilis were dissociated and then isolated on Ficoll density gradients. Their aggregation and reconstitution processes were studied by transmission electron microscopy to determine their capabilities for differentiation.Archaeocyte aggregates follow a well defined sequence of differentiation to generate the characteristic structures of a sponge. Pinacoderm is the first structure to be regenerated and appears progressively at the surface of the 12 h aggregates. Pinacocytes which have differentiated in archaeocyte aggregates are identical to native ones except that the nucleolus remains in most cells. The choanocytes appear only after 24 h by a two step process. First, small cells (choanoblasts) are formed from archaeocytes by mitosis. These cells then transform into fully differentiated choanocytes possessing collars and flagella. The early choanocyte chambers are small, irregular and randomly dispersed in the aggregates. Finally, collencytes and sclerocytes begin to appear just before the aggregates spread on the substrate.The differentiation of a suspension of pure archaeocytes is a unique model system to study sponge cell differentiation and has allowed us to demonstrate that archaeocytes isolated from developed sponges maintain the capacity to differentiate even though this capacity is not usually expressed.

Keywords:  Archaeocyte; Cell aggregation; Cell differentiation; Sponge

Year:  1980        PMID: 28305154     DOI: 10.1007/BF00848609

Source DB:  PubMed          Journal:  Wilehm Roux Arch Dev Biol        ISSN: 0340-0794


  13 in total

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Journal:  Wilehm Roux Arch Dev Biol       Date:  1977-12

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Authors:  D De Sutter; G Van de Vyver
Journal:  Wilehm Roux Arch Dev Biol       Date:  1977-06

5.  Isolation of a highly pure archeocyte fraction from the fresh-water spongeEphydatia fluviatilis.

Authors:  D De Sutter; M Buscema
Journal:  Wilehm Roux Arch Dev Biol       Date:  1977-06

6.  A low-viscosity epoxy resin embedding medium for electron microscopy.

Authors:  A R Spurr
Journal:  J Ultrastruct Res       Date:  1969-01

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Authors:  R M Bagby
Journal:  J Exp Zool       Date:  1972-05

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Journal:  Nat New Biol       Date:  1971-03-24

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Authors:  R Borojevic
Journal:  Dev Biol       Date:  1966-08       Impact factor: 3.582

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Authors:  J M Hurle; M Lafarga; J L Ojeda
Journal:  J Cell Sci       Date:  1978-10       Impact factor: 5.285

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  4 in total

1.  Cell separation of Tethya aurantia, an analytical study of embryonic and differentiated sponge cells.

Authors:  M P Zimmerman; M Hoberg; E Ayanoglu; C Djerassi
Journal:  Lipids       Date:  1990-07       Impact factor: 1.880

2.  The distribution of lipids and sterols in cell types from the marine sponge Pseudaxinyssa sp.

Authors:  M P Zimmerman; F C Thomas; J E Thompson; C Djerassi; H Streiner; E Evans; P T Murphy
Journal:  Lipids       Date:  1989-03       Impact factor: 1.880

3.  Intragenomic Profiling Using Multicopy Genes: The rDNA Internal Transcribed Spacer Sequences of the Freshwater Sponge Ephydatia fluviatilis.

Authors:  Liisi Karlep; Tõnu Reintamm; Merike Kelve
Journal:  PLoS One       Date:  2013-06-18       Impact factor: 3.240

4.  A pan-metazoan concept for adult stem cells: the wobbling Penrose landscape.

Authors:  Baruch Rinkevich; Loriano Ballarin; Pedro Martinez; Ildiko Somorjai; Oshrat Ben-Hamo; Ilya Borisenko; Eugene Berezikov; Alexander Ereskovsky; Eve Gazave; Denis Khnykin; Lucia Manni; Olga Petukhova; Amalia Rosner; Eric Röttinger; Antonietta Spagnuolo; Michela Sugni; Stefano Tiozzo; Bert Hobmayer
Journal:  Biol Rev Camb Philos Soc       Date:  2021-10-06
  4 in total

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