Abstract
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 × 101 copies/μL and 3.836 × 101 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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Introduction
Parvoviridae are mainly divided into two subfamilies: Parvovirinae and Densovirinae (Kailasan et al. 2015). Feline parvovirus (FPV) belongs to the Protoparvovirus genus of the Parvovirinae subfamily (Kailasan et al. 2015). FPV is the pathogen of feline panleukopenia, which is a highly contagious disease that primarily causes high fever, diarrhea, and other clinical symptoms (Barrs 2019). The virus is a positive, single-stranded, non-segmental and linear DNA virus. It is approximately 20–24 nm in diameter, the full genome of FPV is approximately 5000 nucleotide long (Pfankuche et al. 2018). FPV can infect both domestic and wild cats and is extremely harmful to them. Bocavirus belongs to the Bocaparvovirus genus of the Parvovirinae subfamily. Common bocaviruses include human bocavirus, bovine bocavirus, porcine bocavirus, canine bocavirus, and feline bocavirus (FBoV). FBoV is a single-stranded, non-enveloped, linear DNA virus with an icosahedral appearance and a diameter of approximately 25–26 nm (Zhai et al. 2017; Cotmore et al. 2014). The genome of FBoV is approximately 5500 nucleotides in length and has three open reading frames (ORFs), namely ORF1, ORF2, and ORF3. Among them, ORF1 encodes the nonstructural protein NS1, ORF2 encodes the viral nucleocapsid protein VP1/VP2, and ORF3 encodes the nuclear phosphoprotein NP1, respectively (Zhai et al. 2017; Amimo et al. 2017). Owing to the uniqueness of NP1 protein, bocavirus is significantly different from other members of the Parvoviridae family (Zou et al. 2016; Sun et al. 2013). FBoV can also cause diarrhea, which is possibly harmful to cats.
FPV was isolated in 1965 for the first time (Johnson et al. 1967). In 1977, American scholars Eugster and Nair found a variant of the FPV virus in fecal samples from a dog with diarrhea and named it canine parvovirus (CPV-2) (Wang et al. 2016). Subsequently, the virus was reported in several countries, such as Canada, France, Japan, and other countries. FPV is highly homologous to CPV-2 (McEndaffer et al. 2017), which is significantly different from the previously identified CPV. CPV-2 does not infect cats; however, three later discovered antigenic variants (CPV-2a, CPV-2b, and CPV-2c) were found to infect cats (Garigliany et al. 2016; Wang et al. 2016; Truyen and Parrish 1992). The mutation rate of CPV is higher than that of FPV. FBoV contains three genotypes: FBoV-1, FBoV-2, and FBoV-3. In 2012, a new bocavirus was first found in Hong Kong in the fecal, nasal, and serum samples of domestic cats and named FBoV-1 (Lau et al. 2012). Thereafter, FBoV-2 and FBoV-3 were discovered, in succession, in the fecal samples of cats using high-throughput sequencing technology (Zhang et al. 2014; Ng et al. 2014). Recently, researchers successfully isolated FBoV for the first time by collecting and analyzing the fecal samples from cats suffering from severe enteritis in mainland China (Liu et al. 2018). FBoV has been found in various countries, including Belgium, Japan, the United States (Ng et al. 2014; Takano et al. 2016; Zhang et al. 2014; Yi et al. 2018b). However, in China, the prevalence of FBoV remains unclear, and the genotype distribution is not well understood. Co-infection of the two viruses exacerbated the deterioration of the cat’s health (Piewbang et al. 2019). Moreover, co-infection increases the difficulty of treatment. So, there is an urgent need for a rapid, sensitive and reliable assay that can simultaneously detect the two viruses.
Rapid, sensitive, and reliable detection technologies play an extremely crucial role in the prevention and control of diseases. In contrast to various traditional diagnostic methods, such as the enzyme-linked immunosorbent assay (ELISA) and immuno-peroxidase monolayer assay (Okiro et al. 2019), real-time quantitative polymerase chain reaction (qPCR) is more flexible, rapid, and has good efficacy in terms of sensitivity, specificity, and reliability. A number of existing studies have used qPCR to detect FPV or FBoV (Yi et al. 2018b; Sun et al. 2019); however, to our best knowledge, there is no robust method to simultaneously detect the co-infection of FPV and FBoV-1. In this study, a SYBR Green I-based Duplex Real-time PCR assay was established to simultaneously detect FPV and FBoV in cat fecal samples, and the feasibility of applying this experimental model was evaluated. This method may be able to provide a certain reference value for the clinical diagnosis of other viral mixed infections, which will be a major progress in veterinary clinical diagnosis technology.
Materials and methods
Fecal samples collection
From June 2019 to September 2020, a total of 132 domestic cat fecal samples were collected from Shanghai, Hefei, Nan**g, Maanshan, and other places in China, including 92 samples from cats with diarrhea and 40 samples from cats without diarrhea. After confirmation, the tissue samples were homogenized, diluted with phosphate-buffered saline at a ratio of 1:10, and then centrifuged at 8000×g for 3 min. The supernatant was used for nucleic acid extraction or stored at – 40 °C for subsequent use; All the other viral groups used extracted nucleic acid from clinical samples stored at -40° C in our laboratory that had previously been identified, including feline astrovirus (FAstV), feline calicivirus (FCV), feline herpesvirus (FHV), and feline coronavirus (FCoV).
Viral DNA extraction
All nucleotides were extracted using the TIANamp Virus DNA/RNA Kit (Tiangen, Bei**g, China); according to the manufacturer’s instructions. The samples were stored at − 20 °C until using. All RNA viruses were reverse transcribed into cDNA using the Prime Script™ RT Reagent Kit with gDNA Eraser (Takara, Dalian, China), and operated according to the manufacturer’s instructions, and stored at − 20 °C until use.
Primer design
The nucleotide sequences for FPV and FBoV-1 were downloaded from GenBank. The MegAlign software was used to compare the nucleotide sequences of FPV and FBoV-1 to obtain a highly conserved sequence. A pair of primers for constructing the recombinant plasmid and a pair of specific primers for detection were designed using the Primer Premier 5.0 software (Table 1). The location and size of the specific primers for each target gene and the length of each amplified fragment are shown in Table 1. The primers were synthesized by a commercial corporation (General Biological System [Anhui] Co., Ltd., Chuzhou, China).
Preparation of standard plasmids
The extracted DNA was used as the template, and the target fragments of FPV and FBoV-1 were amplified using the above-mentioned primers (Table 1). The positive amplification products were recovered and purified using the TIANgel Midi purification Kit (Tiangen) according to the manufacturer’s instructions. Then, it was verified with electrophoresis on a 1% agarose gel. The purified products were cloned into the pMD19-T vector (Takara) and verified using commercial sequencing [General Biological System (Anhui) Co., Ltd.]. The recombinant plasmids were named pMD19-FPV and pMD19-FBoV and quantified by measuring the optical density at 260 nm (OD260) and OD280 using a Nanodrop 2000 spectrophotometer (Thermo Fisher Scientific, Waltham, MA, USA). The copy number of each plasmid was calculated according to the following formula: amount (copies/μL) = (6.02 × 1023) × (concentration in ng × 10–9) / (plasmid length × 660 Da/bp) (Yu et al. 2020). Concentrations of the recombinant plasmids pMD19-FPV and pMD19-FBoV were 2.907 × 1011 ng/μL and 3.836 × 1011 ng/μL, respectively. The plasmids were continuously diluted tenfold for subsequent amplification and stored at − 40 °C until use.
Optimization of the FPV/FBoV-1 duplex SYBR Green real-time PCR assay
The parameters of FPV/FBoV-1 duplex SYBR Green real-time PCR assay were optimized with plasmid template of 108 copies/μL to obtain the best experimental results, including the PCR program, primer concentration, and annealing temperature (Supplementary Table S1).
Singular and duplex real-time qPCR
After optimization of the reaction parameters, both the singular qPCR and duplex real-time qPCR assays were performed on a CFX96 Real-Time PCR Detection System (Bio-Rad, Hercules, CA, USA). For the singular qPCR assay for FPV, the reaction volume was 20 μL, comprising 0.6 μL each of forward and reverse primers, 10 μL of 2 × SuperReal Premix Plus (Tiangen), 1 μL of DNA template, and RNase-free H2O (to make up final volume). The singular qPCR assay for FBoV-1 had the same reaction components as the reaction for FPV. The reaction volume for the duplex real-time qPCR assay was 40 μL, containing 0.2 μL of each primer for FBoV-1, 0.8 μL of each primer for FPV, 1 μL of FPV DNA template, 1 μL of FBoV-1 DNA template, and 20 μL of 2 × SuperReal Premix Plus (Tiangen). RNase-free H2O was added to make up final volume. The reaction conditions for both singular and duplex qPCR were as follows: 15 min at 95 °C, followed by 40 cycles of 10 s at 95 °C and 30 s at 60 °C. The annealing/extension temperature was then optimized. The reaction without template and the negative reference samples were used as negative controls.
Establishment of standard curves
In the real-time qPCR assay, the recombinant plasmid DNA was continuously diluted tenfold from 108 copies/μL to 101 copies/μL. The logarithm of the initial template number was plotted on the x-axis, and the cycle threshold was plotted on the y-axis to establish a standard curve.
Assessment of sensitivity, specificity and reproducibility
The recombinant plasmid was successively diluted from 108 copies/μL to 101 copies/μL as a positive control to determine the minimum detection limits of FPV and FBoV-1. The sensitivity of single and duplex qPCR detection of the recombinant plasmid was compared to that of the conventional PCR assay. Specificity for the detection of FPV and FBoV-1 was evaluated with duplex real-time qPCR using the above-mentioned DNA or RNA virus samples as templates and RNase-free H2O as the negative control. Three plasmid templates with different concentrations (107, 105, and 103 copies/μL) were selected to simultaneously carry out three parallel tests under the same amplification conditions. The coefficient of variation (CV) was calculated to evaluate the reproducibility of the inter/intra-assay values.
Evaluation of clinical samples with real-time and conventional PCR assays
DNA was extracted from 132 clinical samples (fecals) and detected using conventional and real-time PCR. The positive samples were all verified with 1% agarose gel electrophoresis, and the positive samples were sequenced again to confirm the reliability.
Results
Construction of FPV and FBoV-1 standard curves
Using standard plasmids from 2.907 × 108 copies/μL to 2.907 × 101 copies/μL as the standard templates for FPV, a linear standard curve was plotted with the logarithm of the initial template number as the x-axis and the cycle threshold as the y-axis. The standard curve was defined as y = –3.226x + 36.155, with an R2 value (square of the correlation coefficient) of 0.999 (Fig. 1a). A linear standard curve was plotted with viral genomes from 3.836 × 108 copies/μL to 3.836 × 101 copies/μL as the standard templates for FBoV-1; the curve was defined as y = − 3.295x + 38.133, with an R2 value of 0.998 (Fig. 1b).
Optimization of duplex qPCR assay
To obtain stable fluorescence signal, the subsequent optimization experiments showed that the optimal amount of primers for FPV and FBoV-1 is 0.8 μL and 0.2 μL, respectively. And the optimal temperature is 60 ℃. The CV values obtained under these conditions were minimal, so the subsequent duplex real-time PCR was performed according to these reaction conditions. After the primer concentration and annealing temperature were optimized, the fluorescence signals of FPV and FBoV-1 were detected with singular qPCR. The lowest cycle threshold was recorded and a melting curve was established. Melting curve analysis revealed that the melting temperature of FPV was 77.5 °C and that of FBoV-1 was 86 °C (Fig. 2a and b). The results of the duplex qPCR assay showed that FPV and FBoV-1 could be easily distinguished based on their different melting temperatures (Fig. 3).
Sensitivity of duplex qPCR assay
Sensitivity was assessed using the standard plasmids of FPV or/and FBoV-1 as templates and a tenfold dilution with RNase-free H2O (2.907 × 108 copies/μL to 2.907 × 101 copies/μL for FPV and 3.836 × 108 copies/μL to 3.836 × 101 copies/μL for FBoV-1) to determine the limit of detection. The detection limits were 2.907 × 101 copies/μL and 3.836 × 101 copies/μL for FPV and FBoV-1, respectively, and the Sensitivity of duplex qPCR is also 101 copies/μL (Fig. 4a, b and c).
Specificity of duplex qPCR assay
In the specificity assessment, a total of six viral genomes (FAstV, FCV, FHV, FCoV, FPV, and FBoV-1) were simultaneously detected, among which only FPV and FBoV-1 showed specific melting peaks (77.5 °C for FPV and 86 °C for FBoV-1; Fig. 5).
Reproducibility of the duplex real-time qPCR assay
To determine the reproducibility of the experiment, three parallel tests were carried out independently by three individuals using three different concentrations (107 copies/μL, 105 copies/μL, and 103 copies/μL) of standard plasmids, and comparisons of the intra-assay and inter-assay CVs were made. The results showed that the intra-assay CV was 0.81–1.32% for FPV and 0.15–0.89% for FBoV-1. The inter-assay CV was 1.35–1.54% for FPV and 0.39–1.71% for FBoV-1 (Table 2). These results indicate that the duplex qPCR has the advantages of low variability and high reproducibility.
Evaluation of the duplex real-time qPCR assay using clinical samples
Fecal samples from 132 cats were collected for the individual detection of FPV and FBoV-1 using real-time qPCR. The results showed that 22 samples were positive for FPV, and the detection rate was 16.67% (22/132). Nine samples were positive for FBoV-1, with a detection rate of 6.82% (9/132). Four samples were positive for FPV and FBoV-1 co-infection, and the positive detection rate for co-infection was 3.03% (4/132). The positive samples were sequenced again to determine the reliability of real-time qPCR. Single real-time qPCR and conventional PCR were also used to detect these samples; The results of the conventional PCR showed that 18 samples were positive for FPV, with a detection rate of 13.64% (18/132). Seven samples were positive for FBoV-1, with a detection rate of 5.30% (7/132). The positive detection rate for co-infection with FPV and FBoV-1 was 1.52% (2/132). And the results of the single real-time qPCR were same as the duplex qPCR (Table 3). All the positive results were reliable by sequencing. Thus, the samples that tested positive using conventional PCR also tested positive using real-time qPCR.
Discussion
FPV is a common virus that causes diarrhea in cats and can be fatal in severe cases. FBoV is a newly discovered virus belonging to the same family of Parvoviridae as FPV. Several studies have shown that FBoV can cause diarrhea via concurrent infection with other viruses (Piewbang et al. 2019; Yi et al. 2018a; Lu et al. 2018). Recently, it was reported that the detection rate of FBoV in cats with diarrhea was as high as 33.3% in Northeast China (Niu et al. 2019; Yi et al. 2018b). In cats with diarrhea, co-infection with FPV and FBoV adds significant complications to proper clinical diagnosis and treatment. At present, there is no suitable detection method for the quantitative and simultaneous detection of FPV and FBoV in a sample. The lack of effective diagnostic methods is very disadvantageous to the epidemiological investigation and prevention and control of the diseases. Therefore, a reliable, sensitive, and rapid detection method is urgent needed to simultaneously detect FPV and FBoV in epidemiological and clinical diagnostic studies.
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. Immunohistochemical analysis and ELISA require a long operation time, and cannot be used to estimate the number of copies of viral DNA/cDNA. TaqMan-based real-time PCR assay has good specificity and sensitivity, but is not cost-effective. The SYBR Green duplex real-time qPCR assay is a widely used detection method with good specificity, sensitivity, highly reproducible, and cost-effective. Compared to the conventional PCR, the SYBR Green duplex real-time qPCR assay has more obvious advantages, such as simplicity, efficiency, and sensitivity, which enables high-throughput screening and quantification of viral vectors using only a small amount of virus. In this study, a SYBR Green duplex real-time qPCR method was established for the simultaneous detection of FPV and FBoV-1 in 132 fecal samples. The positive detection rates of FPV and FBoV-1 were 16.67% (22/132) and 6.82% (9/132), respectively, and the detection rate of the co-infection was 3.03% (4/132). In contrast, using conventional PCR, the positive detection rates of FPV and FBoV-1 were 13.64% (18/132) and 5.30% (7/132), respectively, and the co-infection rate was 1.52% (2/132). This indicates that the developed SYBR Green duplex real-time qPCR assay was more sensitive than the conventional PCR.
In this study, a conserved sequence from FPV and FBoV-1 was amplified using a SYBR Green duplex real-time qPCR assay, and different melting peak values were obtained. The melting peak values of FPV and FBoV-1 were 77.5 °C and 86 °C, respectively, and the two viruses could be easily distinguished by their specific melting temperature values. In addition, standard curves for FPV and FBoV-1 were established. The correlation coefficient of the standard curve of FPV was 0.999, and the standard formula was y = –3.226x + 36.155. The standard curve correlation coefficient of FBoV-1 was 0.998, and the standard formula was y = –3.295x + 38.133. Detection limits of the two viruses were 2.907 × 101 copies/μL and 3.836 × 101 copies/μL, respectively, which were 100 times higher than those of the conventional PCR method used in a previous study (Zhang et al. 2019). In addition, the positive detection rate of the SYBR Green real-time duplex qPCR assay was higher than that of the conventional PCR; the samples that were negative with conventional PCR and positive with the SYBR Green duplex real-time qPCR assay were confirmed to be positive by DNA sequencing, which indicated that the SYBR Green duplex real-time qPCR assay had a high sensitivity for detection at low viral load levels. In addition, to determine the feasibility of the assay, we carried out repeatability verification. The results showed that the intra-assay and inter-assay CVs were 0.81–1.32% for FPV and 0.15–0.89% for FBoV-1, and 1.35–1.54% for FPV and 0.39–1.71% for FBoV-1, respectively. Both sets of which were less than 2%, indicating that the assay had good repeatability.
In summary, the SYBR Green-based duplex real-time PCR assay established in this study is a rapid, sensitive, and reliable laboratory testing method to detect FPV and FBoV-1 simultaneously. It is suitable for high-throughput screening of a low level of viral genome, which exhibits potential adaptability and stability for the differential diagnosis of FPV and FBoV-1 in field samples.
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We would like to thank Editage (www.editage.cn) for English language editing.
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This study was supported by the Ningbo Health Branding Subject Fund (No. ppxk2018-10).
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YP, JW, and XT were involved in performing experiments. JS, and FX were involved in data analysis, experimental design. YW, BC, and TZ wrote the manuscript. All authors read and approved the final manuscript.
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Wang, Y., Pan, Y., Wu, J. et al. Simultaneous detection of feline parvovirus and feline bocavirus using SYBR Green I-based duplex real-time polymerase chain reaction. 3 Biotech 11, 400 (2021). https://doi.org/10.1007/s13205-021-02947-w
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DOI: https://doi.org/10.1007/s13205-021-02947-w