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Clinical performance validation of Real-time fluorescence PCR for detection of HBV-DNA by magnetic beads extraction

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ã€Authorã€‘ SHI Ying;TIAN LÃ¼bo;FAN Xuejun;WANG Junxian;LONG Juan;Sichuan International Healthcare Center;

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ã€Abstractã€‘ Objective To evaluate the analytical performance and clinical value of Real-time fluorescent quantitative PCR reagents for HBV-DNA by nucleic acid magnetic beads extraction reagents,to help to select reagents.Methods According to the requirements of CNAS-CL36 capability verification,serum samples of hepatitis B patients from Sichuan Provincial Peopleâ€™s Hospital were collected,and methodological performance of the three(reagents A,B and C) nucleic acid extraction Real-time fluorescent quantitative PCR reagents by magnetic beads were verified and evaluated,including precision,accuracy,detection limit,reporting range and anti-interference ability. Results The LOD of reagents A and B met the performance parameters,the positive detection rate were all 100%,and the positive detection rate of reagent C was 83.3%,which was inconsistent with the lower limit of quantitative detection20 IU/ml announced by the manufacturer. The coefficient of variation(CV) of reagent A low-concentration and high-concentration specimens were lower than 5% in batches,reagent B low-concentration specimens was CVâ‰¥5%,high-concentration specimens was CV â‰¤5%,reagent C low-concentration and high-concentration specimens were CVâ‰¥5%. There was good correlation between the results of 3 reagents in the linear range. The interference test of the three reagents showed that severe hemolysis and lipid samples had an effect on the detection of HBV-DNA with low viral load,but were not affected by mild hemolysis and lipid samples. Conclusion Through the performance verification of the three reagents,it was found that one-step(magnetic bead method) quantitative detection reagent for HBV-DNA made by Daan Gene Co. Ltd had high sensitivity,and suitable for port and clinical routine detection.æ›´å¤š è¿˜åŽŸ