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Dive into the research topics where Chiyome Ichinose is active.

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Featured researches published by Chiyome Ichinose.


Molecular Cell | 1998

Cell Cycle–Dependent Duplication and Bidirectional Migration of SeqA-Associated DNA–Protein Complexes in E. coli

Sota Hiraga; Chiyome Ichinose; Hironori Niki; Mitsuyoshi Yamazoe

Using immunofluorescence microscopy, we have found that SeqA protein, a regulator of replication initiation, is localized as discrete fluorescent foci in E. coli wild-type cells. Surprisingly, SeqA foci were observed also in an oriC deletion mutant. Statistical analysis revealed that a SeqA focus is localized at midcell in newborn cells. The SeqA focus is duplicated and tethered at midcell until an FtsZ ring is formed. Subsequently, these foci migrate in opposite directions toward cell quarter sites and remain tethered there until the cell divides. The cell cycle-dependent bidirectional migration of SeqA-DNA complexes is quite different from the migration pattern of oriC Dna copies. MukB protein is required for correct localization of SeqA complexes by an unknown mechanism.


Genes to Cells | 2000

Bidirectional migration of SeqA‐bound hemimethylated DNA clusters and pairing of oriC copies in Escherichia coli

Sota Hiraga; Chiyome Ichinose; Toshinari Onogi; Hironori Niki; Mitsuyoshi Yamazoe

We previously found that SeqA protein, which binds preferentially to newly replicated hemimethylated DNA, is localized as discrete fluorescent foci in Escherichia coli cells. A single SeqA focus, localized at midcell, separates into two foci and these foci migrate abruptly in opposite directions.


Journal of Bacteriology | 2000

Null mutation of the dam or seqA gene suppresses temperature-sensitive lethality but not hypersensitivity to novobiocin of muk null mutants.

Toshinari Onogi; Mitsuyoshi Yamazoe; Chiyome Ichinose; Hironori Niki; Sota Hiraga

Escherichia coli mukF, mukE, and mukB null mutants have common phenotypes such as temperature-dependent colony formation, anucleate cell production, chromosome cutting by septum closure, and abnormal localization of SeqA-DNA clusters. We show here that the associated muk null mutations cause hypersensitivity to novobiocin. Null mutation of either dam or seqA suppressed partially the temperature-sensitive lethality but failed to suppress the anucleate cell production and the hypersensitivity to novobiocin caused by muk null mutations.


Journal of Bacteriology | 1989

Chromosome partitioning in Escherichia coli: novel mutants producing anucleate cells.

Sota Hiraga; Hironori Niki; Teru Ogura; Chiyome Ichinose; Hirotada Mori; Bunichi Ezaki; A Jaffé


Journal of Biological Chemistry | 1989

Purification and characterization of SopA and SopB proteins essential for F plasmid partitioning.

Hirotada Mori; Y Mori; Chiyome Ichinose; Hironori Niki; Teru Ogura; A Kato; Sota Hiraga


Journal of Bacteriology | 1990

Positioning of replicated chromosomes in Escherichia coli.

Sota Hiraga; Teru Ogura; Hironori Niki; Chiyome Ichinose; Hirotada Mori


Journal of Bacteriology | 1988

Chromosomal genes essential for stable maintenance of the mini-F plasmid in Escherichia coli.

Hironori Niki; Chiyome Ichinose; Teru Ogura; Hirotada Mori; M Morita; M Hasegawa; N Kusukawa; Sota Hiraga


Journal of Bacteriology | 1990

Identification and characterization of gyrB mutants of Escherichia coli that are defective in partitioning of mini-F plasmids.

Teru Ogura; Hironori Niki; Hirotada Mori; M Morita; M Hasegawa; Chiyome Ichinose; Sota Hiraga


Archive | 1989

Chromosome Partitioning inEscherichia coli: NovelMutants Producing Anucleate Cells

Sota Hiraga; Hironori Niki; Teru Ogura; Chiyome Ichinose; Hirotada Mori; Bunichi Ezaki; Aline Jaffé


Archive | 1990

Identification andCharacterization ofgyrBMutants ofEscherichia coli ThatAreDefective inPartitioning ofMini-FPlasmids

Chiyome Ichinose; Sota Hiraga

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Hironori Niki

National Institute of Genetics

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