Sensitive fluorescent hybridisation protocol development for simultaneous detection of microRNA and cellular marker proteins (in the retina)
Nowadays, increasing number of microRNAs are found to have crucial roles in various physiological processes through gene expression regulation via RNA silencing as a result of base pairing with complementary mRNA sequences. To reveal the spatial distribution of microRNA expression in tissues, in sit...
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Published in | Histochemistry and cell biology Vol. 150; no. 5; pp. 557 - 566 |
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Main Authors | , , , |
Format | Journal Article |
Language | English |
Published |
Berlin/Heidelberg
Springer Berlin Heidelberg
01.11.2018
Springer Nature B.V |
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Abstract | Nowadays, increasing number of microRNAs are found to have crucial roles in various physiological processes through gene expression regulation via RNA silencing as a result of base pairing with complementary mRNA sequences. To reveal the spatial distribution of microRNA expression in tissues, in situ hybridisation is the only method developed to date. This work aims to provide a novel approach to obtain information on the possible involvement of microRNA-s in regulatory processes under experimental conditions by enhancing fluorescent detection of microRNA labelling. Developing Wistar rats were used as a model system to analyse retinal microRNA expression in the first 3 postnatal weeks. Using cryosections, the crucial elements of optimal labels were (1) the concentration and duration of proteinase K treatment, (2) hybridisation temperature of microRNA probes and (3) temperature of stringency washes. Further improvements made possible to combine our in situ hybridisation protocol with double-label immunofluorescence allowing for the simultaneous detection of microRNA-s with high sensitivity and a neuronal cell marker and/or a synaptic marker protein. Thus, the regulatory microRNA-s can be localised in an identified cell type along with its potential target protein. We believe that our protocol can be easily adapted for a variety of tissues of different origins, developmental stages and experimental conditions. |
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AbstractList | Nowadays, increasing number of microRNAs are found to have crucial roles in various physiological processes through gene expression regulation via RNA silencing as a result of base pairing with complementary mRNA sequences. To reveal the spatial distribution of microRNA expression in tissues, in situ hybridisation is the only method developed to date. This work aims to provide a novel approach to obtain information on the possible involvement of microRNA-s in regulatory processes under experimental conditions by enhancing fluorescent detection of microRNA labelling. Developing Wistar rats were used as a model system to analyse retinal microRNA expression in the first 3 postnatal weeks. Using cryosections, the crucial elements of optimal labels were (1) the concentration and duration of proteinase K treatment, (2) hybridisation temperature of microRNA probes and (3) temperature of stringency washes. Further improvements made possible to combine our in situ hybridisation protocol with double-label immunofluorescence allowing for the simultaneous detection of microRNA-s with high sensitivity and a neuronal cell marker and/or a synaptic marker protein. Thus, the regulatory microRNA-s can be localised in an identified cell type along with its potential target protein. We believe that our protocol can be easily adapted for a variety of tissues of different origins, developmental stages and experimental conditions. |
Author | Kovács-Valasek, Andrea Gábriel, Robert Sétáló, György Szalontai, Bálint |
Author_xml | – sequence: 1 givenname: Andrea surname: Kovács-Valasek fullname: Kovács-Valasek, Andrea organization: Department of Experimental Zoology and Neurobiology, University of Pécs – sequence: 2 givenname: Bálint surname: Szalontai fullname: Szalontai, Bálint organization: János Szentágothai Research Centre, University of Pécs – sequence: 3 givenname: György surname: Sétáló fullname: Sétáló, György organization: Department of Medical Biology, University of Pécs – sequence: 4 givenname: Robert orcidid: 0000-0001-9323-8795 surname: Gábriel fullname: Gábriel, Robert email: gabriel@ttk.pte.hu organization: Department of Experimental Zoology and Neurobiology, University of Pécs, János Szentágothai Research Centre, University of Pécs |
BackLink | https://www.ncbi.nlm.nih.gov/pubmed/30088096$$D View this record in MEDLINE/PubMed |
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CitedBy_id | crossref_primary_10_1007_s00418_020_01944_z crossref_primary_10_3390_ijms22137078 crossref_primary_10_3390_ijms22052577 crossref_primary_10_1038_s41598_019_57194_0 |
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Keywords | MicroRNA mir-9 Tyramide signal amplification mir-23 In situ hybridisation Immunocytochemistry |
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SubjectTerms | Animals Biochemistry Biomarkers - analysis Biomedical and Life Sciences Biomedicine Cell Biology Developmental Biology DNA probes Endopeptidase K Gene expression Gene regulation Immunofluorescence Immunohistochemistry In Situ Hybridization, Fluorescence Labeling MicroRNAs MicroRNAs - analysis MicroRNAs - metabolism miRNA Neurons - chemistry Neurons - cytology Neurons - metabolism Original Paper Proteinase Proteins - analysis Proteins - metabolism Rats Rats, Wistar Retina Retina - chemistry Retina - cytology Retina - metabolism RNA-mediated interference Spatial distribution |
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