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Comparison of a new immunoassay and PCR-based method for quantification of microRNAs in whole blood. A pilot methodical study

The result's identifiers

  • Result code in IS VaVaI

    <a href="https://www.isvavai.cz/riv?ss=detail&h=RIV%2F61988987%3A17110%2F19%3AA2001YZL" target="_blank" >RIV/61988987:17110/19:A2001YZL - isvavai.cz</a>

  • Alternative codes found

    RIV/00843989:_____/19:E0107723

  • Result on the web

    <a href="https://biomed.papers.upol.cz/artkey/bio-201901-0005_comparison_of_a_new_immunoassay_and_pcr-based_method_for_quantification_of_micrornas_in_whole_blood_a_pilot_me.php" target="_blank" >https://biomed.papers.upol.cz/artkey/bio-201901-0005_comparison_of_a_new_immunoassay_and_pcr-based_method_for_quantification_of_micrornas_in_whole_blood_a_pilot_me.php</a>

  • DOI - Digital Object Identifier

    <a href="http://dx.doi.org/10.5507/bp.2018.080" target="_blank" >10.5507/bp.2018.080</a>

Alternative languages

  • Result language

    angličtina

  • Original language name

    Comparison of a new immunoassay and PCR-based method for quantification of microRNAs in whole blood. A pilot methodical study

  • Original language description

    Background. MicroRNAs (miRNAs) are new generation biomarkers used in oncology, cardiology, metabolic syndrome, obesity or in neurology. miRNAs are short non-coding RNA molecules that regulate gene expression in eukaryotes. Aim. To compare a new commercial method for establishing miRNA (imunoassay) with a commercial kit RT qPCR. Methods. RNA was isolated from whole blood samples obtained from four healthy volunteers. The isolates were liquated and miRNA-93-Sp and miRNA-23a-3p were measured independently with commercial hsa-miR-93-Sp miREIA and hsa-miR-23a-3p miREIA, and commercial RT-qPCR kits. Results. Both miRNAs had good analytical characteristics, very good correlation with RT qPCR. The results between immunoassay and RT qPCR did not statistically differ. A method based on ELISA was faster (2 h with ELISA vs. 3 h with qPCR) and had lower CV then a method based on RT qPCR (see more text). Conclusion. MicroRNAs from blood or derived fractions are particularly interesting candidates for routine laboratory applications.The immunoassay can be performed on any device that processes the ELISA plates and is therefore available in almost every laboratory.

  • Czech name

  • Czech description

Classification

  • Type

    J<sub>imp</sub> - Article in a specialist periodical, which is included in the Web of Science database

  • CEP classification

  • OECD FORD branch

    30500 - Other medical sciences

Result continuities

  • Project

  • Continuities

    V - Vyzkumna aktivita podporovana z jinych verejnych zdroju

Others

  • Publication year

    2019

  • Confidentiality

    S - Úplné a pravdivé údaje o projektu nepodléhají ochraně podle zvláštních právních předpisů

Data specific for result type

  • Name of the periodical

    BIOMEDICAL PAPERS-OLOMOUC

  • ISSN

    1213-8118

  • e-ISSN

    1804-7521

  • Volume of the periodical

    1

  • Issue of the periodical within the volume

    163

  • Country of publishing house

    CZ - CZECH REPUBLIC

  • Number of pages

    6

  • Pages from-to

    39-44

  • UT code for WoS article

    000458362500005

  • EID of the result in the Scopus database

    2-s2.0-85062361913

Similar results(10)

Evaluation of miRNA detection methods for the analytical characteristics necessary for clinical utilizationprototype of diagnostic multiplex immunochemical kit for the determination of selected microRNAs related to bladder cancerCirculating microRNA alternations in primary hyperuricemia and gout