Literature DB >> 9387935

Self-sustained sequence replication (3SR): an alternative to PCR.

J D Mueller1, B Pütz, H Höfler.   

Abstract

The amplification of target nucleic acids before hybridization is one of the most powerful approaches for the detection of low copy number RNA and DNA. The best known amplification reaction is PCR which has many applications. However, certain drawbacks of the PCR reaction provide a role for alternative amplification methods. One of these methods is the self-sustained sequence replication (3SR) reaction, which is an isothermal method for RNA amplification depending on the action of three enzymes. 3SR has been used in several in vitro applications and has also been modified for in situ use (IS-3SR). We have studied IS-3SR with the measles virus as a model and have found that it can significantly amplify the amount of intracellular RNA. Such a level of amplification could raise the amount of single copy RNA to the level of detection by conventional in situ hybridization. Although careful controls to insure its specificity must be carried out, IS-3SR has several advantages, including ease of use, preserved cell morphology, and specificity for RNA amplification, which make it an attractive alternative to the in situ PCR method.

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Year:  1997        PMID: 9387935     DOI: 10.1007/s004180050183

Source DB:  PubMed          Journal:  Histochem Cell Biol        ISSN: 0948-6143            Impact factor:   4.304


  3 in total

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2.  Primer fabrication using polymerase mediated oligonucleotide synthesis.

Authors:  Murray J Cairns; Torsten Thomas; Carolina E Beltran; Daniel Tillett
Journal:  BMC Genomics       Date:  2009-07-31       Impact factor: 3.969

3.  Polymerase Spiral Reaction Assay for Rapid and Real Time Detection of West Nile Virus From Clinical Samples.

Authors:  Priyanka Singh Tomar; Jyoti S Kumar; Sapan Patel; Shashi Sharma
Journal:  Front Cell Infect Microbiol       Date:  2020-08-27       Impact factor: 5.293

  3 in total

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