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      Fission yeast meu14+ is required for proper nuclear division and accurate forespore membrane formation during meiosis II.

      Journal of Cell Science
      Amino Acid Sequence, genetics, Base Sequence, Cell Compartmentation, Cell Cycle Proteins, isolation & purification, metabolism, Cell Nucleus, ultrastructure, Cells, Cultured, DNA, Complementary, analysis, Fungal Proteins, Genes, Regulator, Giant Cells, cytology, Intracellular Membranes, Meiosis, physiology, Microscopy, Electron, Microtubules, Molecular Sequence Data, Schizosaccharomyces, Schizosaccharomyces pombe Proteins, Spindle Apparatus, Spores, Fungal

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          Abstract

          Using a meiosis-specific subtracted cDNA library of Schizosaccharomyces pombe, we identified meu14+ as a gene whose expression is upregulated during meiosis. Transcription of meu14+ is induced abruptly after the cell enters meiosis. Its transcription is dependent on the meiosis-specific transcription factor Mei4. In meu14Delta cells, the segregation and modification of the SPBs (spindle pole bodies) and microtubule elongation during meiosis II were aberrant. Meiotic meu14Delta cells consequently produced a high frequency of abnormal tetranucleate cells harboring aberrant forespore membranes and failed to produce asci. In wild-type cells harboring the integrated meu14+-gfp fusion gene, Meu14-GFP first appeared inside the nuclear region at prophase II, after which it accumulated beside the two SPBs at metaphase II. Thereafter, it formed two ring-shaped structures that surrounded the nucleus at early anaphase II. At post-anaphase II, it disappeared. Meu14-GFP appears to localize at the border of the forespore membrane that later develops into spore walls at the end of sporulation. This was confirmed by coexpressing Spo3-HA, a component of the forespore membrane, with Meu14-GFP. Taken together, we conclude that meu14+ is crucial in meiosis in that it participates in both the nuclear division during meiosis II and the accurate formation of the forespore membrane.

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