Literature DB >> 15771557

Comparison of three PCR assays for the evaluation of interferon-beta biological activity in patients with multiple sclerosis.

Francesca Gilli1, Fabiana Marnetto, Guglielmo Stefanuto, Valentina Rinaldi, Federica Farinazzo, Simona Malucchi, Marco Capobianco, Marzia Caldano, Arianna Sala, Antonio Bertolotto.   

Abstract

BACKGROUND: The gene expression of the myxovirus-resistant protein A (MxA) gene is a sensitive measure of the biological response of therapeutically applied interferon-beta (IFNbeta) and of its reduced bioavailability due to inhibiting factors such as IFNbeta-induced neutralizing antibodies (NAbs).
METHODS: We compared three methods for MxA mRNA quantification in 826 peripheral blood mononuclear cell (PBMC) samples obtained from patients with multiple sclerosis (MS). MxA mRNA measurements were performed using quantitative-competitive (qc)-PCR, real time-PCR, and the new semi-quantitative (sq)-PCR assay (MxA IBRIDOGEN).
RESULTS: According to the treatment status (untreated samples versus NAb-negative treated samples), real time-PCR gave the highest specificity (93%). Slightly lower specificities were obtained with qc-PCR and sq-PCR (both 91%). qc-PCR showed the highest sensitivity (97%) compared with both real time-PCR (94%) and sq-PCR (95%). A positive correlation was found between qc-PCR and real time-PCR measurements (rspearman=0.776; p<0.0001), which also showed 90% agreement based on a statistically calculated threshold. Likewise, sq-PCR evaluations showed 84% and 79% agreement with qc-PCR and real time-PCR measurements, respectively. In addition, we showed a concordance of 89% between three sq-PCR kits.
CONCLUSIONS: All three methods displayed high specificity for MxA gene expression analysis, allowing the detection of patients in whom IFNbeta did not have any biological action. qc-PCR and real time-PCR are both useful during clinical trials demanding quantitative data of biological activity, whereas sq-PCR could prove useful for routine screening purposes because it is easy to perform and can be done in not specialized laboratories.

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Year:  2004        PMID: 15771557     DOI: 10.1007/BF03260063

Source DB:  PubMed          Journal:  Mol Diagn        ISSN: 1084-8592


  29 in total

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5.  Evaluation of IFNalpha bioavailability by MxA mRNA in HCV patients.

Authors:  F Gilli; A Sala; C Bancone; P Salacone; M Gallo; E Gaia; A Bertolotto
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6.  Improved quantitation of minimal residual disease in multiple myeloma using real-time polymerase chain reaction and plasmid-DNA complementarity determining region III standards.

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7.  PRISMS-4: Long-term efficacy of interferon-beta-1a in relapsing MS.

Authors: 
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8.  Evaluation of bioavailability of three types of IFNbeta in multiple sclerosis patients by a new quantitative-competitive-PCR method for MxA quantification.

Authors:  A Bertolotto; F Gilli; A Sala; L Audano; A Castello; U Magliola; F Melis; M T Giordana
Journal:  J Immunol Methods       Date:  2001-10-01       Impact factor: 2.303

9.  The human intracellular Mx-homologous protein is specifically induced by type I interferons.

Authors:  P von Wussow; D Jakschies; H K Hochkeppel; C Fibich; L Penner; H Deicher
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10.  Increased levels of antiviral MxA protein in peripheral blood of patients with a chronic disease of unknown etiology.

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Journal:  J Med Virol       Date:  2001-10       Impact factor: 2.327

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  1 in total

1.  One-year evaluation of factors affecting the biological activity of interferon beta in multiple sclerosis patients.

Authors:  Simona Malucchi; Francesca Gilli; Marzia Caldano; Arianna Sala; Marco Capobianco; Alessia di Sapio; Letizia Granieri; Antonio Bertolotto
Journal:  J Neurol       Date:  2010-12-12       Impact factor: 4.849

  1 in total

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