Comparison between the Amount of Environmental Change and the Amount of Transcriptome Change

Ogata, Naoya; Kozaki, Toshinori; Yokoyama, Takeshi; Hata, Tamako; Iwabuchi, Kikuo

doi:10.1371/journal.pone.0144822

Cited by 17 publications

(21 citation statements)

References 19 publications

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“…This is thought to be re-differentiation to construct new plants and reprogramming can be explained as an integration of dedifferentiation and regeneration. Callus may be regarded as dedifferentiated cells which holding down the redifferentiation process; using callus and plant tissue culture, bi-/multi-stability of transcriptome [8,9] could be demonstrated in plant. If their re-differentiation process is caused by the determination of intercellular division of labor based on cell-tocell communication [10], it will be possible to examine them in a test that separates cultured cells.…”

Section: Resultsmentioning

confidence: 99%

Transcriptome Dedifferentiation Observed in Animal Primary Cultures is Essential to Plant Reprogramming

Ogata¹

2019

Preprint

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Tissue culture environment liberate cells from ordinary laws of multi-cellular organisms. This liberation enables cells several behaviors, such as growth, dedifferentiation, acquisition of pluripotency, immortalization and reprogramming. Each phenomenon is relating to each other and hardly to determine. Recently, dedifferentiation of animal cell was determined and quantified in increasing information entropy of transcriptome. The increasing information entropy of transcriptome induced by tissue culture may reappear in plant cells too. Here we corroborated it. Measuring information entropies of transcriptomes during reprogramming of plant cells suggested that reprogramming is a combined phenomenon of dedifferentiation and re-differentiation.

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Section: Resultsmentioning

confidence: 99%

Transcriptome Dedifferentiation Observed in Animal Primary Cultures is Essential to Plant Reprogramming

Ogata¹

2019

Preprint

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“…RNA samples were readily obtained from cultured tissues in the present study thus avoiding such variable factors; in this way, biologically significant differentially expressed genes were realized. Drug concentration is also an important factor in comparative transcriptomics as has been reported 7,18,19 . Such methods, predicting NCR toxins using comparative transcriptomics, would be useful not only in pest control but also in research fields affected by biological drug resistance, e.g., antibiotics and cancer research.…”

Section: Fig 1 Probabilities Of Survival Of the Permethrin Survivor mentioning

confidence: 95%

“…Total RNA was extracted using TRIzol LS (Invitrogen) and the RNeasy Lipid Tissue Mini Kit (Qiagen, Hilden, Germany) following the manufacturers' instructions as previously described 7 . Silkworm fat bodies (30 mg) soaked in 300 µL TRIzol LS were homogenized.…”

Section: Rna Isolationmentioning

confidence: 99%

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Synergic Interaction between Permethrin and Bt toxins discovered using RNA-seq

Sakamoto

Kozaki

Ogata³

2019

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Acting against the development of resistance to antibiotics and insecticides, involving negatively correlated cross-resistance (NCR) is an alternative to use-and-discard approach. It is termed NCR that toxic chemicals interact with each other and resistance of target organisms to one chemical is sometimes associated with increased susceptibility to a second chemical when; an allele confers resistance to one toxic chemical and hyper-susceptibility to another, NCR occurs. However, only 11 toxin pairs have been revealed to cause NCR in insects. Finding novel NCRs is needed for integrated pest management. We analyzed permethrin, an insecticide, induced transcriptomes of cultured fat bodies of the silkworm Bombyx mori, a lepidopteran model insect. Differentially expressed gene analyses suggested Bacillus thuringiensis (Bt) toxin was an NCR toxin of permethrin. NCR to permethrin and Bt toxins inThysanoplusia intermixta, the agricultural pest moth, was examined; the children of permethrin survivor T. intermixta had increased susceptibility to Bt toxin. A novel NCR toxin pair, permethrin and Bt toxin, was discovered. The screening and developmental method for negatively correlated cross-resistance toxins established in this study was effective, in vitro screening using model organisms and in vivo verification using agricultural pests.

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“…Transcriptome diversity also used for measurement of cellular dedifferentiation [6]. Our Previous study compared transcriptome diversity between cells cultured in vitro in media supplemented with several concentrations of phenobarbital, to investigate how the amount of environmental change (in terms of drug concentration) affects the amount of transcriptome change and multi-stability of the genome expression system was indicated by an observation of hysteretic phenomenon of transcriptome diversities [7].…”

Section: Introductionmentioning

confidence: 99%