Development of a duplex TaqMan real-time RT-PCR assay for simultaneous detection of newly emerged H5N6 influenza viruses

Liu, Lin; Zhang, Ying; Cui, Pengfei; Wang, Congcong; Zeng, Xianying; Wang, Xiurong

doi:10.1186/s12985-019-1229-2

Cited by 13 publications

(6 citation statements)

References 27 publications

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“…Multiplex TaqMan qPCR has been useful for the simultaneous detection of multiple viruses or genes in a single reaction [ 30 , 31 ]. This assay offers significant cost- and time-saving potential for the accurate detection of newly emerging viruses [ 32 , 33 ]. In this study, TaqMan qPCR was developed to target multiple genes such as the VP0, VP3, and 3C of HAV.…”

Section: Discussionmentioning

confidence: 99%

Molecular diagnosis of patients with hepatitis A virus infection using amplicon-based nanopore sequencing

et al. 2023

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High-throughput sequencing is a robust tool used for identifying and tracking pathogen outbreaks. Whole-genome sequencing of hepatitis A virus (HAV) remains poor due to ultra-low viral loads, limitations of next-generation sequencing technology, and its high costs in clinical applications. This study evaluated multiplex polymerase chain reaction (PCR)-based nanopore sequencing to obtain whole-genome sequences of HAV. The HAV genomes were obtained directly from patient specimens for a rapid molecular diagnosis of viral genotypes. Serum and stool samples were collected from six patients with hepatitis A infection. Amplicon-based nanopore sequencing was performed from the clinical specimens to identify HAV genotypes by acquiring nearly complete-genome sequences. TaqMan-based quantitative PCR (qPCR) was conducted to detect and quantify multiple HAV genes. Singleplex-based nanopore sequencing demonstrated high genome coverage rates (90.4–99.5%) of HAV within 8 h, at viral RNA loads of 10 to 105 copies/μL. TaqMan qPCR showed multiplex quantification of HAV genes namely, VP0, VP3, and 3C. This study provides useful insights into rapid molecular diagnosis during hepatitis A outbreaks and may ultimately augment public health disease surveillance in the hospital and epidemiology field.

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Section: Discussionmentioning

confidence: 99%

Molecular diagnosis of patients with hepatitis A virus infection using amplicon-based nanopore sequencing

et al. 2023

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“…To date, a variety of laboratory detection methods, including loop-mediated isothermal amplification (LAMP) (Wong et al 2018), TaqMan-based real-time PCR assay (Liu et al 2019), ELISA (Wischhusen and Padilla 2017), SYBR Green duplex real-time qPCR assay, and immunohistochemical analysis (Hai et al 2020), have been used to effectively detect viruses. Among them, LAMP does not require complicated equipment and provides visual experimental results; however, it is easy to show false positive due to the contamination of reagents, which will affect the experimental results.…”

Section: Discussionmentioning

confidence: 99%

Simultaneous detection of feline parvovirus and feline bocavirus using SYBR Green I-based duplex real-time polymerase chain reaction

Wang

Pan

et al. 2021

3 Biotech

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Since both feline parvovirus (FPV) and feline bocavirus (FBoV) can cause diarrhea in cats, it is difficult to distinguish them clinically. This study aimed to develop a SYBR Green I-based duplex real-time polymerase chain reaction (PCR) assay for distinguishing FPV and FBoV-1 on the basis of the melting temperature of the PCR product. A total of 132 fecal samples from different domestic and feral cats were collected, and the results of SYBR Green I-based duplex real-time PCR assay were compared with those of the traditional PCR assay for a comprehensive evaluation. The melting temperatures were found to be 86 °C and 77.5 °C for FBoV-1 and FPV, respectively, and no specific melting peaks for other non-targeted feline viruses were observed. The data obtained from this assay had a good linear relationship; the detection limits of FPV and FBoV-1 were 2.907 × 10 1 copies/μL and 3.836 × 10 1 copies/μL, respectively. In addition, the experiment exhibited high reproducibility. The positive detection rates of the SYBR Green I-based duplex real-time PCR assay for FPV and FBoV-1 were 16.67% (22/132) and 6.82% (9/132), respectively, and the positive detection rate for co-infection with FPV and FBoV-1 was 3.03% (4/132). This result was much more sensitive than that of the traditional PCR method. Thus, the developed SYBR Green I-based assay is a sensitive, rapid, specific, and reliable method for the clinical diagnosis of FPV and FBoV-1 and can provide technical support for the simultaneous detection of co-infection with these viruses in the future.

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“…Despite the low cost and mature nature of the technology (Table I), qPCR is prone to nucleic acid contamination, primer dimer formation, improper baseline setting and a number of other issues which can lead to false-positives. Furthermore, sample inhibitors, enzyme inactivation, insufficient enzyme concentration, a low template amount and/or an inappropriate annealing temperature may lead to false-negatives (25). In addition, qPCR is time-consuming, requires relatively complex and expensive instruments to achieve accurate (±0.5˚C) and rapid (>10˚C/s) thermal cycles, and requires knowledgeable operators, making this technology difficult to utilize in areas and hospitals with limited access to precision instruments (Table II) (26)(27)(28).…”

Section: Pcrmentioning

confidence: 99%

Advances in the application of molecular diagnostic techniques for the detection of infectious disease pathogens (Review)

et al. 2023

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Infectious diseases are a major global cause of morbidity and mortality, seriously affecting public health and socioeconomic stability. Since infectious diseases can be caused by a wide variety of pathogens with similar clinical manifestations and symptoms that are difficult to accurately distinguish, selecting the appropriate diagnostic techniques for the rapid identification of pathogens is crucial for clinical disease diagnosis and public health management. However, traditional diagnostic techniques have low detection rates, long detection times and limited automation, which means that they do not meet the requirements for rapid diagnosis. Recent years have seen continuous developments in molecular detection technology, which has a higher sensitivity and specificity, shorter detection time and increased automation, and performs an important role in the early and rapid detection of infectious disease pathogens. The present study summarizes recent progress in molecular diagnostic technologies such as PCR, isothermal amplification, gene chips and high-throughput sequencing for the detection of infectious disease pathogens, and compares the technical principles, advantages and disadvantages, applicability and costs of these diagnostic techniques.

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Development of a duplex TaqMan real-time RT-PCR assay for simultaneous detection of newly emerged H5N6 influenza viruses

Cited by 13 publications

References 27 publications

Molecular diagnosis of patients with hepatitis A virus infection using amplicon-based nanopore sequencing

Molecular diagnosis of patients with hepatitis A virus infection using amplicon-based nanopore sequencing

Simultaneous detection of feline parvovirus and feline bocavirus using SYBR Green I-based duplex real-time polymerase chain reaction

Advances in the application of molecular diagnostic techniques for the detection of infectious disease pathogens (Review)

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