An RNA synthesis inhibition assay for detecting toxic substances using click chemistry

Kametani, Yukiko; Iwai, Shigenori; Kuraoka, Isao

doi:10.2131/jts.39.293

Cited by 3 publications

(3 citation statements)

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“…Previously, we demonstrated that our in vivo method for visualizing transcription in mammalian cells can detect UV- and/or chemically (e.g., camptothecin, etoposide, 4NQO, cisplatin) induced damage in genomic DNA by inhibiting RNA polymerase during transcription elongation [ 20 , 22 , 23 ]. Here, we modified this in vivo method to establish a new in vitro method (Fig.…”

Section: Resultsmentioning

confidence: 99%

“…In our previous work, we established a method for detecting the effects of chemically induced DNA damage on transcription using the nucleotide analog 5-bromouridine and a anti-5-bromouridine antibody and/or the nucleotide analog 5-ethynyluridine [ 20 ] and a click chemistry reaction [ 21 , 22 ] without radioisotopes [ 23 ]. Our method is based on a model for transcription-coupled nucleotide excision repair (NER) triggered by blocked transcription at DNA lesions [ 24 , 25 ].…”

Section: Introductionmentioning

confidence: 99%

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An in vitro method for detecting genetic toxicity based on inhibition of RNA synthesis by DNA lesions

2015

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IntroductionA wide variety of DNA lesions such as ultraviolet light-induced photoproducts and chemically induced bulky adducts and crosslinks (intrastrand and interstrand) interfere with replication and lead to mutations and cell death. In the human body, these damages may cause cancer, inborn diseases, and aging. So far, mutation-related actions of DNA polymerases during replication have been intensively studied. However, DNA lesions also block RNA synthesis, making the detection of their effects on transcription equally important for chemical safety assessment. Previously, we established an in vivo method for detecting DNA damage induced by ultraviolet light and/or chemicals via inhibition of RNA polymerase by visualizing transcription.ResultsHere, we present an in vitro method for detecting the effects of chemically induced DNA lesions using in vitro transcription with T7 RNA polymerase and real-time reverse transcription polymerase chain reaction (PCR) based on inhibition of in vitro RNA synthesis. Conventional PCR and real-time reverse transcription PCR without in vitro transcription can detect DNA lesions such as complicated cisplatin DNA adducts but not UV-induced lesions. We found that only this combination of in vitro transcription and real-time reverse transcription PCR can detect both cisplatin- and UV-induced DNA lesions that interfere with transcription.ConclusionsWe anticipate that this method will be useful for estimating the potential transcriptional toxicity of chemicals in terminally differentiated cells engaged in active transcription and translation but not in replication.

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Section: Resultsmentioning

confidence: 99%

Section: Introductionmentioning

confidence: 99%

An in vitro method for detecting genetic toxicity based on inhibition of RNA synthesis by DNA lesions

2015

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“…RNA labeling has seen extensive use in imaging of infection by RNA viruses (e.g., 58 ). Another interesting application of RNA imaging has been to monitor transcription and this has been used, for example, to determine the toxicity of certain substances that inhibit transcription 59 .…”

Section: Conclusion: Current Applications and Outlookmentioning

confidence: 99%

Current techniques for visualizing RNA in cells

2016

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In vivo 5-ethynyluridine (EU) labelling detects reduced transcription in Purkinje cell degeneration mouse mutants, but can itself induce neurodegeneration

Sant

White

Hoeijmakers

et al. 2021

acta neuropathol commun

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Fluorescent staining of newly transcribed RNA via metabolic labelling with 5-ethynyluridine (EU) and click chemistry enables visualisation of changes in transcription, such as in conditions of cellular stress. Here, we tested whether EU labelling can be used to examine transcription in vivo in mouse models of nervous system disorders. We show that injection of EU directly into the cerebellum results in reproducible labelling of newly transcribed RNA in cerebellar neurons and glia, with cell type-specific differences in relative labelling intensities, such as Purkinje cells exhibiting the highest levels. We also observed EU-labelling accumulating into cytoplasmic inclusions, indicating that EU, like other modified uridines, may introduce non-physiological properties in labelled RNAs. Additionally, we found that EU induces Purkinje cell degeneration nine days after EU injection, suggesting that EU incorporation not only results in abnormal RNA transcripts, but also eventually becomes neurotoxic in highly transcriptionally-active neurons. However, short post-injection intervals of EU labelling in both a Purkinje cell-specific DNA repair-deficient mouse model and a mouse model of spinocerebellar ataxia 1 revealed reduced transcription in Purkinje cells compared to controls. We combined EU labelling with immunohistology to correlate altered EU staining with pathological markers, such as genotoxic signalling factors. These data indicate that the EU-labelling method provided here can be used to identify changes in transcription in vivo in nervous system disease models.

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An RNA synthesis inhibition assay for detecting toxic substances using click chemistry

Cited by 3 publications

References 16 publications

An in vitro method for detecting genetic toxicity based on inhibition of RNA synthesis by DNA lesions

An in vitro method for detecting genetic toxicity based on inhibition of RNA synthesis by DNA lesions

Current techniques for visualizing RNA in cells

In vivo 5-ethynyluridine (EU) labelling detects reduced transcription in Purkinje cell degeneration mouse mutants, but can itself induce neurodegeneration

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