Multiplex qPCR for serodetection and serotyping of hepatitis viruses: A brief review
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  • 英文篇名:Multiplex qPCR for serodetection and serotyping of hepatitis viruses: A brief review
  • 作者:Mohammad ; Irshad ; Priyanka ; Gupta ; Dhananjay ; Singh ; Mankotia ; Mohammad ; Ahmad ; Ansari
  • 英文作者:Mohammad Irshad;Priyanka Gupta;Dhananjay Singh Mankotia;Mohammad Ahmad Ansari;Clinical Biochemistry Division, Department of Laboratory Medicine, All India Institute of Medical Sciences;
  • 英文关键词:Co-infection;;Viral genome;;Quantitative real-time polymerase chain reaction;;Genotyping techniques;;Serotyping;;Hepatitis viruses
  • 中文刊名:ZXXY
  • 英文刊名:世界胃肠病学杂志(英文版)
  • 机构:Clinical Biochemistry Division, Department of Laboratory Medicine, All India Institute of Medical Sciences;
  • 出版日期:2016-05-28
  • 出版单位:World Journal of Gastroenterology
  • 年:2016
  • 期:v.22
  • 语种:英文;
  • 页:ZXXY201620006
  • 页数:11
  • CN:20
  • 分类号:49-59
摘要
The present review describes the current status of multiplex quantitative real time polymerase chain reaction(q PCR) assays developed and used globally for detection and subtyping of hepatitis viruses in body fluids. Several studies have reported the use of multiplex q PCR for the detection of hepatitis viruses, including hepatitis A virus(HAV), hepatitis B virus(HBV), hepatitis C virus(HCV), hepatitis D virus(HDV), and hepatitis E virus(HEV). In addition, multiplex q PCR has also been developed for genotyping HBV, HCV, and HEV subtypes. Although a single step multiplex q PCR assay for all six hepatitis viruses, i.e., A to G viruses, is not yet reported, it may be available in the near future as the technologies continue to advance. All studies use a conserved region of the viral genome as the basis of amplification and hydrolysis probes as the preferred chemistries for improved detection. Based on a standard plot prepared using varying concentrations of template and the observed threshold cycle value, it is possible to determine the linear dynamic range and to calculate an exact copy number of virus in the specimen. Advantages of multiplex q PCR assay over singleplex or other molecular techniques in samples from patients with co-infection include fast results, low cost, and a single step investigation process.
        The present review describes the current status of multiplex quantitative real time polymerase chain reaction(q PCR) assays developed and used globally for detection and subtyping of hepatitis viruses in body fluids. Several studies have reported the use of multiplex q PCR for the detection of hepatitis viruses, including hepatitis A virus(HAV), hepatitis B virus(HBV), hepatitis C virus(HCV), hepatitis D virus(HDV), and hepatitis E virus(HEV). In addition, multiplex q PCR has also been developed for genotyping HBV, HCV, and HEV subtypes. Although a single step multiplex q PCR assay for all six hepatitis viruses, i.e., A to G viruses, is not yet reported, it may be available in the near future as the technologies continue to advance. All studies use a conserved region of the viral genome as the basis of amplification and hydrolysis probes as the preferred chemistries for improved detection. Based on a standard plot prepared using varying concentrations of template and the observed threshold cycle value, it is possible to determine the linear dynamic range and to calculate an exact copy number of virus in the specimen. Advantages of multiplex q PCR assay over singleplex or other molecular techniques in samples from patients with co-infection include fast results, low cost, and a single step investigation process.
引文
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