Exclusive Amplification of cDNA Template (EXACT) RT-PCR to Avoid Amplifying Contaminating Genomic Pseudogenes | Zendy

Daron Smith | Zendy; Christopher Ogden | Zendy; Michelle A. Penny | Zendy

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Exclusive Amplification of cDNA Template (EXACT) RT-PCR to Avoid Amplifying Contaminating Genomic Pseudogenes

Author(s) -

Daron Smith,

Christopher Ogden,

Michelle A. Penny

Publication year - 2001

Publication title -

biotechniques

Language(s) - English

Resource type - Journals

SCImago Journal Rank - 0.617

H-Index - 131

eISSN - 1940-9818

pISSN - 0736-6205

DOI - 10.2144/01314st03

Subject(s) - pseudogene , genomic dna , complementary dna , biology , primer (cosmetics) , microbiology and biotechnology , rna , dna , reverse transcriptase , polymerase chain reaction , genetics , multiple displacement amplification , gene , rapid amplification of cdna ends , gene duplication , genome , dna extraction , molecular cloning , chemistry , organic chemistry

Genomic DNA contamination within RNA samples has important implications for RT-PCR, particularly if there is a pseudogene related to the gene under investigation, because amplification from pseudogenes and reverse-transcribed cDNA can be very difficult to distinguish. Methods to remove DNA contamination cannot guarantee the absolute absence of DNA from the sample without a loss of RNA quantity or quality, which can be crucial for small amounts of RNA or for the investigation of transcripts with a low level of expression. Here, we describe a general technique for RT-PCR that applies a sequence to the 5' tail of reverse-transcribed cDNA that is not present in genomic DNA and uses this for annealing the reverse PCR primer to exclude genomic DNA amplification in unmodified RNA samples.

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