Validation of a nested PCR assay UMELOSA®HCV CUALITATIVO for the detection of Hepatitis C virus

Biologicals ◽  
2003 ◽  
Vol 31 (1) ◽  
pp. 55-61 ◽  
Author(s):  
Idania Gonzalez-Perez ◽  
Yaimé Josefina González González ◽  
Anny Armas Cayarga ◽  
Ariel Vina-Rodrı́guez ◽  
Ariel Medina Concepción ◽  
...  
1991 ◽  
Vol 13 ◽  
pp. S165 ◽  
Author(s):  
J Ruiz ◽  
JI Cuende ◽  
B Sangro ◽  
JI Herrero ◽  
O Belogui ◽  
...  

2014 ◽  
Vol 60 (1) ◽  
pp. S324
Author(s):  
M. Mukaide ◽  
M. Sugiyama ◽  
M. Korenaga ◽  
K. Murata ◽  
T. Kanto ◽  
...  

Author(s):  
Jens Mueller ◽  
Matthias Gessner ◽  
Anja Remberg ◽  
Jochen Hoch ◽  
Gerold Zerlauth ◽  
...  

AbstractNucleic acid amplification testing for hepatitis C virus (HCV) RNA has become an essential tool for the prevention and clinical management of hepatitis C. We describe the development, validation and evaluation of a homogenous reverse transcriptase-initiated HCV-PCR assay with competitive internal control that is applicable to both the quantitative detection of HCV genomes in single patient samples and the screening of blood donations by mini-pool testing. For the implementation of a positive run control, a HCV RNA-positive plasma sample was calibrated against an international HCV RNA standard preparation. For quantification purposes, an in vitro-transcribed RNA calibrator sequence was used. The detection limit of the assay (95% positive cut-off) was determined by probit analysis and was calculated as 114IU/mL. Comparable sensitivity to different HCV template sequences was verified for HCV genotypes 1–5. Quantitative test results correlated well with viral loads that had been previously determined by the Bayer VERSANT HCV RNA 3.0 bDNA assay (n=53, R=0.943, p<0.001). During more than 5years of blood donation testing, the specificity of the assay was found to be 99.51%. All assay components showed constant performance during this time period. In conclusion, we introduce a well-proven method that allows fast and reliable quantification of HCV genomes.


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