Real time PCR quantification of frataxin mRNA in the peripheral blood leucocytes of Friedreich ataxia patients and carriers

L Pianese; M Turano; M S Lo Casale; I De Biase; M Giacchetti; A Monticelli; C Criscuolo; A Filla; S Cocozza

doi:10.1136/jnnp.2003.028605

Real time PCR quantification of frataxin mRNA in the peripheral blood leucocytes of Friedreich ataxia patients and carriers

J Neurol Neurosurg Psychiatry. 2004 Jul;75(7):1061-3. doi: 10.1136/jnnp.2003.028605.

Authors

L Pianese¹, M Turano, M S Lo Casale, I De Biase, M Giacchetti, A Monticelli, C Criscuolo, A Filla, S Cocozza

Affiliation

¹ BioGeM Consortium, c/o Department of Molecular and Cellular Biology and Pathology, Frederico II University, Naples, Italy. pianese@biogen.it

Abstract

The most common causative mutation of Friedreich ataxia (FRDA) is the unstable hyperexpansion of an intronic GAA triplet repeat that impairs frataxin transcription. Using real time quantitative PCR, we showed that FRDA patients had residual levels of frataxin mRNA ranging between 13% and 30% and that FRDA carriers had about 40% of that of controls. Asymptomatic carriers also showed reduced frataxin mRNA levels. We found an inverse correlation between the number of GAA repeats and frataxin mRNA levels. Real-time quantitative PCR may represent an alternative assay for FRDA molecular diagnosis.

Publication types

Research Support, Non-U.S. Gov't

MeSH terms

DNA Primers / genetics
DNA, Complementary / genetics
Female
Frataxin
Friedreich Ataxia / genetics*
Friedreich Ataxia / metabolism*
Humans
Introns / genetics
Iron-Binding Proteins / genetics*
Leukocytes / metabolism*
Male
Peripheral Nervous System / metabolism*
Point Mutation / genetics
Polymerase Chain Reaction / methods*
RNA, Messenger / genetics*
Trinucleotide Repeats / genetics

Substances

DNA Primers
DNA, Complementary
Iron-Binding Proteins
RNA, Messenger