key: cord-0757035-a8yfi2wn
authors: Liu, Pengcheng; Lu, Lijuan; Xu, Menghua; Zhong, Huaqing; Jia, Ran; Su, Liyun; Cao, Lingfeng; Dong, Zuoquan; Dong, Niuniu; Zhou, Linfu; Xu, Jin
title: A novel multiplex PCR for virus detection by melting curve analysis
date: 2018-09-26
journal: J Virol Methods
DOI: 10.1016/j.jviromet.2018.09.010
sha: fb1727cba632fd315e7d816852f48456c60fd8df
doc_id: 757035
cord_uid: a8yfi2wn

BACKGROUND: Rapid and accurate laboratory diagnoses of viral infections are crucial for the management and treatment of patients with viral infections. Conventional methods for virus detection are labourious, time consuming, and only a single virus can be analysed in one assay. OBJECTIVES: The objective of this study was to develop a novel real-time PCR method for multiple virus detection by melting curve analysis using Taqman probes in a single reaction. STUDY DESIGN: As a model, six respiratory viruses were detected in one tube using three fluorophores. The specificity was assessed by cross-reaction tests with other common respiratory pathogens. The analytical sensitivity was assessed by testing the limit of detection of the assay using artificial plasmids as the positive template. The clinical evaluation of the established assay was evaluated for the detection of respiratory viruses in clinical samples, and the results were compared with direct fluorescent antibody testing (DFA). RESULTS: The six respiratory viruses were clearly distinguished by their respective melting temperature values in the corresponding fluorescence detection channels. No cross reactions were observed by cross reaction tests. The detection limits of this assay were 2 to 2 × 10(3) copies per reaction for each virus. The clinical evaluation of this assay was demonstrated by analysing 352 clinical samples, and 67(19.0%) samples were positive for at least one virus. The accordance rate between the established PCR and DFA testing was high, and ranged from 94.57% to 100%. CONCLUSIONS: Taqman probe-based melting curve analysis is well suited for detection of multiple viruses in clinical and research laboratories because of its high throughput, reliability, and cost savings.

Multiple virus detection can considerably improve the correct management of clinical viral infections and reduce unnecessary antibiotic prescriptions (Mayer et al., 2017) . A large number of different methods are currently available for the detection of viral infections in clinical laboratories. Traditional laboratory diagnostic methods include virus culture, rapid antigen tests and the direct fluorescent-antibody assay (DFA), but they are labourious, time consuming, and usually only a single virus can be analysed in one assay (Storch, 2000) .

With the advances of molecular techniques, real-time PCR has been developed and applied in clinical virology laboratories because of the high sensitivity, specificity and reproducibility. Real-time PCR is also easy to automate and relatively inexpensive. We can use different fluorophore-labeled probes to detect multiple viruses simultaneously in one tube. The combinatorial use of the fluorophore and melting temperature (Tm) as a 2D-label enables a magnitude increase in the number of targets in the real-time PCR platform.

TaqMan probes are widely used to monitor real-time PCR in clinical laboratories with the advantages of cost savings, multiplexing, and high flexibility in probe design. Recent studies have shown that the TaqMan probes can be used not only for monitoring PCR in real time but also for melting curve analysis under asymmetric PCR conditions (Huang et al., 2011) . Multicolor melting curve analysis using the TaqMan probe has been successfully applied in mutant gene detection and genotyping (Botezatu et al., 2017; Mou et al., 2016; Wang et al., 2017; Xia et al., 2016; Huang et al., 2016; Gao et al., 2015; Huang et al., 2017) . Nevertheless, the application to multiple virus detection has not yet been reported.

In this study, we sought to use this approach to establish a novel real-time PCR for multiple virus detection. influenza B (FluB), parainfluenza virus type 1 (PIV1), parainfluenza virus type 2 (PIV2) and parainfluenza virus type 3 (PIV3), were detected in one tube using three fluorophores.

Viral isolates for RSV, FluA, FluB and PIV3 were maintained in our laboratory. PIV1 (ATCC-VR94) and PIV2 (ATCC-VR92) were obtained from the Shanghai Medical College of Fudan University.

Plasmids containing specific viral target fragment sequences were synthesized by Sangon (Shanghai, China) on the basis of the sequences provided by the Genome Sequencing Project in GenBank. The concentration of each plasmid was quantified by the NanoVue spectrophotometer (GE, USA).

A total of 352 nasopharyngeal aspirates (NPA) were collected from children diagnosed with respiratory infection in the children's hospital of fudan university during January 2017 to February 2017. These samples were used to evaluate the multiplex PCR for its diagnostic capacity.

Viral nucleic acid was extracted from viral isolates or clinical samples using a kit (Mole, China) according to the protocol suggested by the manufacturer on the automated extraction platform (Tianlong, China).

Reverse transcription was performed in a reaction mixture consisting of 8 μl of extracted viral nucleic acid, 4 μl of 5×PrimeScritBuffer, 2 μl of Random 6mers, 1 μl of PrimeScript RT Enzyme Mix I, and 5 μl of nuclease-free water (TaKaRa, China). Reverse transcription was performed using a model 2720 thermal cycler (Applied Biosystems, USA) with amplification parameters as follows: incubation at 37°C for 30 min, followed by 85°C for 5 s.

The primers and probes for RSV, PIV1, PIV2, PIV3, FluA and FluB were designed using Primer Premier 5.0 (Primer Biosoft International, USA) based on the conserved regions of target genes and their specificity was confirmed by the Nucleotide BLAST search. The N gene of RSV, HN genes of PIV1, PIV2 and PIV3, M gene of FluA, and NS gene of FluB were selected as target genes for primer design. Three fluorophores were selected and probes with the same fluorophores were designed to have different Tm values. RSV and PIV2 probes were labelled with FAM; PIV1 and PIV3 probes were labelled with HEX; FluA and FluB probes were labelled with ROX. All primers and probes were synthesized and purified by Sangon, China. The sequences of the primers and probes are given in Table 1 .

In order to generate excess single-stranded amplicon for probe hybridization to generate sufficient melting curve signals, asymmetric PCR and 5′-nuclease-deficient mTaq DNA Polymerase (Kangwei Biotech, China) were introduced in this assay. The lack of the 5′-3′ exonuclease activity of mTaq DNA polymerase can avoid hydrolysing probes in the reaction. After optimization, PCR and melting curve analysis were performed on a LightCycler 480II real-time system (Roche Diagnostics, Switzerland) in a 25-μL reaction containing 1 × PCR buffer, 0.2 mM dNTPs, 3.0 mM MgCl 2 , 2.5 U mTaq DNA polymerase, primers and probes as listed in Table 1 , and 2 μL cDNA template. The final amplification program started with denaturation for 5 min at 95°C, followed by 50 cycles of denaturation at 94°C for 30 s, annealing at 55°C for 30 s, and extension at 72°C for 30 s. Melting curve analysis started with a denaturation step of 1 min at 95°C, a hybridization step of 5 min at 35°C, and an incremental temperature rise from 35°C to 85°C at a ramp rate of 0.01°C/s with fluorescence acquired from the FAM, HEX, and ROX channels 10 times per°C.

The specificity of the multiplex PCR assay was assessed by cross reaction tests with other common respiratory pathogens including respiratory viruses and bacteria. Clinical Samples positive for adenovirus (ADV), human rhinovirus/enterovirus (RV/EV), and human corona virus OC43 (hCoV-OC43) were confirmed by Filmarray, an automated nested multiplex PCR System (bioMérieux, France). Standard strains for influenza A/H1N1, influenza A/H3N2, influenza A/H7N9, influenza B/ Victoria, influenza B/Yamagata, measles virus, mumps virus, rubella virus, varicella zoster virus, E. coli, P. aeruginosa and S.aureus were obtained from the National Institutes for Food and Drug Control, China.

The analytical sensitivity of the multiplex PCR was assessed by testing the limit of detection (LOD) of the assay. The plasmids containing specific viral target fragment sequences were serially 10-fold diluted from 10 5 copies/μl to 10°copy/μl and analysed using the multiplex PCR. Each concentration of plasmid was analysed in triplicate. Water was used as a negative control.

A total of 352 paediatric NPA samples described above were analysed using both the multiplex PCR assay and direct fluorescent antibody testing (DFA). DFA was performed for seven respiratory viruses: respiratory syncytial virus (RSV), influenza A (FluA), influenza B (FluB), parainfluenza viruses 1-3 (PIV 1-3) and adenovirus (ADV) using a panel of DFA assays (Diagnostic Hybrids, Athens, OH), a Food and Drug Administration (FDA) approved assay for respiratory virus detection. We were blinded to the DFA results while evaluating the NPA samples using the multiplex PCR assay. The results were compared for those viruses identified by both testing methods. Positive percent agreement is the percent of time that the multiplex PCR detected a virus when DFA detected it. Similarly, negative percent agreement is the percent of time that the multiplex PCR did not detect a virus when DFA did not detect it. The degree of agreement was measured by Cohen's kappa, which was performed as described previously (Watson and Petrie, 2010) . Statistical analyses were carried out using STATA 10 (College Station, TX, USA).

The samples detected positive only by the multiplex PCR were confirmed by independent PCR and sequencing. The sequencing was performed by Sangon (Shanghai, China) and compared with the sequences in GenBank for pathogen identification using BLAST. The samples detected positive only by DFA were confirmed by conventional real-time PCR assays (Mole, China).

To develop a melting curve-based multiplex PCR assay for the simultaneous detection of six human respiratory viruses in one tube, we designed 6 sets of primers and probes using three colour fluorophores. The actual Tm values of the probes ranged from 55.9°C to 72.6°C (Fig. 1) . Six viruses can be clearly distinguished from each other by Tm value and fluorophore. The corresponding Tm values were 63.2°C and 71.4°C for PIV2 and RSV, respectively, in the FAM channel (Fig. 1A) ; 55.9°C and 67.2°C for PIV1 and PIV3, respectively, in the HEX channel (Fig. 1B) ; 69.0°C and 72.6°C for FluA and FluB, respectively, in the ROX channel (Fig. 1C) . To verify the ability of established multiplex PCR to detect co-infection, a mixed template containing all six virus cDNAs was added to the reaction. Two distinguishable melting peaks with specific Tm values were generated in the FAM and HEX channels ( Fig. 1A and 1B, black line), which indicate the presence of PIV2, RSV, PIV1 and PIV3 target amplicons. However, the melting peaks of FluA and FluB were fused, and generated a wide melting peak with a Tm value between 69.0°C and 72.6°C (Fig. 1C, black line) .

The LOD of the multiplex PCR for RSV, PIV1, PIV2, PIV3, FluA and FluB were 2 × 10 3 , 2, 2 × 10 3 , 2, 2 × 10 2 , and 2 × 10 3 copies per reaction, respectively (Fig. 2) .

The specificity of the multiplex PCR was evaluated by cross reaction tests with other common respiratory pathogens as described above. Three common subtypes of influenza A (H1N1, H3N2, and H7N2) virus and two subtypes of influenza B (Yamagata and Victoria) virus can all be well detected using the multiplex PCR. There were no cross reactions observed against other common respiratory pathogens that were not involved in the detection profile. These results indicated that the multiplex PCR had good specificity for the detection of respiratory viruses.

Of the 352 clinical samples tested, 67 (19.0%) samples were positive by the multiplex PCR, which included 4 co-infections. DFA detected 46 (13.1%) positive samples of which 2 were co-infections.

The accordance rate between the multiplex PCR and DFA testing was high and ranged from 94.57% to 100% ( Table 2 ). Most of the discordant results were samples that were positive for virus by multiplex PCR but negative by DFA (+/-). Twenty-seven clinical samples positive by multiplex PCR but negative by DFA (+/-) were confirmed by sequencing. The sequencing results were in accordance with the multiplex PCR, except for one sample that was positive for PIV1 in the multiplex PCR but tested negative by sequencing.

Four clinical samples negative by multiplex PCR, but positive for RSV by DFA (-/+) were confirmed by the conventional PCR assay. Three samples were positive for RSV by the conventional PCR assay, and the other sample was negative (data not shown).

An increasing number of recent studies have focused on the development of molecular methods to solve the problem of multiple virus detection (Kishimoto et al., 2017; Boyd et al., 2015; Pripuzova et al., 2012; Choudhary et al., 2013) . In this study, we successfully developed a novel multiplex real-time PCR assay for the simultaneous identification of 6 respiratory viruses using probe-based melting curve analysis in a single reaction tube. The multiplex PCR developed and described here combined asymmetric PCR and multi-colour melting curve analysis techniques to achieve multiplex nucleic acid detection. This strategy uses the fluorophore and Tm as two measurable parameters (2D-label), which enables a magnitude increase in the number of targets that can be distinguished on the real-time PCR platform (Liao et al., 2013) .

In our study, three fluorescence detection channels (FAM, HEX, and ROX) were introduced and two probes with discriminable Tm values were detected in each channel, thus six respiratory viruses could be detected simultaneously in a single reaction tube. This multiplex PCR accurately detected and discriminated multiple pathogens in one sample at the same time, which means this method has a good ability to detected co-infections. Because the Tm values of FluA and FluB are too close, their melting peaks are fused and generate a wide melting peak with a Tm value between them when they are positive at the same time. However, the melting peak can be well distinguished from single infection of FluA or FluB. Moreover, there are few co-infections of FluA and FluB (Ren et al., 2009) .

To evaluate the clinical utility of the multiplex PCR, 352 paediatric NPA samples were analysed, and the results demonstrate a successful real-world application of this method. When compared to DFA, the multiplex PCR showed a high percent agreement, which ranged from 94.57% to 100%. The most common reason for discordance was the detection of pathogens by multiplex PCR in DFA-negative samples. These discordant NPA samples were confirmed by sequencing, and most of the sequencing results were consistent with the multiplex PCR. We believe this is due to the increased sensitivity of PCR when compared to DFA.

Compared with other virus detection techniques, this novel multiplex PCR has many advantages. First, the number of detectable targets is significantly increased in our 2D-label multiplex PCR when compared with those multiplex PCR assays using a label that involves either Tm or fluorophore alone (Wan et al., 2016; Simmons et al., 2016) . In this study, 2 probes with discriminable Tm values were designed in each channel. It might be possible to design more probes in one channel, and then the number of targets detected in a single tube could be further enhanced. Second, this novel multiplex PCR is cost-effective. The cost of a probe-based real-time PCR assay primarily depends on the consumption of the fluorescence probe, and the TaqMan probe used in our study was easy to design and synthesize. The cost was lower than Fig. 2 . Sensitivity of the multiplex PCR using serially diluted templates (10 5 , 10 4 , 10 3 , 10 2 , 10, and 1 copies/μl). NC, negative control. probes with special modifications such as PNA and FRET. One peculiar requirement is asymmetric amplification, which is easy to perform without extra cost (Huang et al., 2011) . Third, this multiplex PCR can be performed with almost any real-time PCR machine, making it possible for wide application in the clinical laboratory for multiple virus detection. Similar to most other PCR methods, this novel multiplex PCR is fast and can be completed within 3 h. Therefore enabling results, including sample processing, nucleic acid extraction and analysis to be obtained within a single working day. However, there are some limitations of the multiplex PCR based on probe melting curve analysis. First, the TaqMan probes were designed based on the known sequence of conserved genes. As new variants of the virus continue to emerge, it might be possible that some variants could lead to mismatch of the probe against the target sequence, which could cause a Tm shift from the predefined values. In this regard, the established assay should be updated on an as needed basis. Second, as an end-point detection assay, melting curve analysis-based multiplex PCR is non-quantitative in nature and therefore restricts its application in virus quantitative detection. However, as shown in Fig. 2 , the signal of the melting curves increased with increasing template concentrations within a certain range. In some cases, we observed that when the concentration of template exceeds a certain standard, an increase of concentration does not result in the expected increase in the melt peaks, and sometimes they are even reduced (Fig. 2, PIV1 ). The reason is that after reaching the amplification plateau, complementary DNA strands rapidly anneal to one another and fall out of the reaction, whereas the excessive single-stranded DNA continues to be available to the primer and be converted into the double stranded form. As a result, the concentration of the single-stranded DNA in asymmetric PCR may be decreased after reaching plateau (Botezatu et al., 2015) . Third, the application of melting curve analysis increases the time required for analysis compared with standard real-time PCR. Another limitation is that the analytical sensitivity of the multiplex PCR is not high enough, especially for RSV, PIV2, and FluB. Further optimization of the reaction is needed.

In conclusion, we developed a novel multiplex PCR for the detection of six common respiratory viruses by melting curve analysis. This method is expected to be widely used in clinical and research laboratories due to its high throughput nature and easy application when compared with traditional methods such as DFA. Furthermore, this strategy can be modified and extended to detect additional pathogens responsible for many other infectious diseases, such as meningitis, gastrointestinal infections and bloodstream infections.

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None declared.

Not required.