key: cord-1045207-5rep8wlv authors: Ding, Sheng; Chen, Gangyi; Wei, Yinghua; Dong, Juan; Du, Feng; Cui, Xin; Huang, Xin; Tang, Zhuo title: Sequence-specific and multiplex detection of COVID-19 virus (SARS-CoV-2) using proofreading enzyme-mediated probe cleavage coupled with isothermal amplification date: 2021-01-28 journal: Biosens Bioelectron DOI: 10.1016/j.bios.2021.113041 sha: 9e6efd744687b72679b1c0e0625d7a682f07b8d7 doc_id: 1045207 cord_uid: 5rep8wlv The outbreak of COVID-19 caused by severe acute respiratory syndrome coronavirus 2 (SARS-CoV-2) has been challenging human health worldwide. Loop-mediated isothermal amplification (LAMP) has been promptly applied to the detection of SARS-CoV-2 owing to its high amplification efficacy and less requirement of the thermal cycler. However, the vast majority of these LAMP-based assays depend on the non-specific detection of LAMP products, which can not discern the undesirable amplificons, likely to yield unreliable results. Herein, a sequence-specific LAMP assay was reported to detect SARS-CoV-2 using proofreading enzyme-mediated probe cleavage (named Proofman), which could realize real-time and visual detection without uncapping. This assay, introducing a proofreading enzyme and the fluorogenic probe to reverse-transcription LAMP (RT-Proofman-LAMP), can specifically detect the SARS-CoV-2 RNA with a detection limit of 100 copies. In addition to the real-time analysis, the assay is capable of endpoint visualization under a transilluminator within 50 min, providing a convenient reporting manner under the setting of point-of-care testing (POCT). In combination with different fluorophores, the one-pot multiplex assay was successfully achieved to detect multiple targets of SARS-CoV-2 and inner control simultaneously. In summary, the development of RT-Proofman-LAMP offers a versatile and highly-specific method for fast field screening and laboratory testing of SARS-CoV-2, making it a promising platform in COVID-19 diagnosis. Over the past two decades, the world has faced several infectious disease outbreaks. Ebola, Influenza A (H1N1), SARS, MERS and Zika virus have had a massive global impact in terms of economic disruption, the strain on local and global public health resources and, above all, human health. Most recently, the pandemic of COVID-19, which caused more than one million deaths based on the Weekly Epidemiological Updates of WHO in October 2020, has been challenging the global public health system since December 2019 (Wang et al. 2020a ). The high risk posed by the transmission of infectious agents like SARS-CoV-2 requires an efficient response mechanism in which rapid and accurate diagnostic methods are urgently demanded. Nucleic acid detection techniques providing fast and reliable diagnosis could fulfill the requirement and play a critical role in the surveillance and prevention of infectious diseases. The reverse transcription polymerase chain reaction (RT-PCR) has been developed as a gold standard method to diagnose COVID-19 (Wang et al. 2020b ). However, the strong reliance on thermal-cycler, as well as the time-consuming process, limit its broad use in some regions where the fast and on-site screening of potential infection cases are direly needed. Isothermal nucleic acid amplification (INAA) is widely used in detecting causative pathogens, which can provide a fast detection platform under constant temperature (Yan et al. 2014 ). Among the INAA methods, loop-mediated isothermal amplification (LAMP) is the most prevailing method as its high amplification efficiency and the good tolerance to crudely-processed biological samples (Kaneko et al. 2007; Notomi et al. 2000) . Facing the challenge of COVID-19, many LAMP-based assays have been successfully applied to detect the SARS-CoV-2 virus, demonstrating LAMP is a robust and perspective method in COVID-19 detection (Lu et al. 2020; Yan et al. 2020) . These LAMP-based assays, however, mainly rely on the non-specific reporters, such as DNA intercalating dyes, metal ion indicators, reaction turbidity and labeled primers; that is to say, the non-specific analytic methods cannot discern the non-specific amplificon which would be problematic for some cases, especially in the case of detecting the samples sharing high homology in genetic sequence. Moreover, as a result of that LAMP is hard to perform multiplex detection in one-pot, many LAMP-based methods lack inner control to ensure sample collection procedure and avoid false positive. Most recently, two state-of-the-art techniques have been reported to solve the issues by using nanoparticle-based lateral flow biosensor (Zhu et al. 2020) or fluorogenic oligonucleotide strand exchange (OSD) probes (Bhadra et al. 2020) . However, these two methods required J o u r n a l P r e -p r o o f uncapping operation or extra oligonucleotide strand, which enhances the risk of carry-over contamination or the complexity of probe design. The enzymatic cleavage-based probes are highly popular in specific molecular diagnosis (Juskowiak 2011) . Owing to the isothermal DNA polymerase lacks 5' → 3' exonuclease activity, enzymatic cleavage-mediated probes are hardly used in INAA. The inclusion of endonuclease IV to recombinase polymerase reaction (RPA) provided a strategy of sequencespecific detection based on enzymatic cleavage-mediated probes (Piepenburg et al. 2006 ). However, the probe requires the incorporation of tetrahydrofuran abasic-site mimic, complicating the probe preparation. In previous research, we briefly introduced the proofreading enzyme-mediated probe cleavage (termed Proofman) as developing recombinase assisted loop-mediated isothermal amplification (RALA) . When using Proofman probe, an additional DNA polymerase (Pfu) with proofreading activity was involved to cleave the probe from 3' end, producing a fluorescent signal. In this study, we developed a sequence-specific detection platform for SARS-CoV-2 nucleic acid using LAMP coupled with the Proofman probe. In addition to real-time monitoring, visual detection could be realized under a transilluminator, providing a convenient amplification-to-result assay for rapid on-site detection. Furthermore, we evaluated the feasibility of multiplex detection, proving the Proofman-based LAMP could be an appealing choice for accurate diagnosis of COVID-19. The plasmid containing the SARS-CoV-2 gene N cDNA sequence was purchased from Sangon Biotech Company Limited (Shanghai, China). The SARS-CoV-2 gene Orf1ab cDNA was artificially synthesized through reverse transcription-PCR using pseudovirus (purchased from Yeasen Biotech Co., Ltd.) as the template, then conventional PCR was conducted followed by gel extraction and purification using commercial kit (Vazyme, China). The primers used were described below. To obtain the RNA sequence, the corresponding target sequences were amplified through PCR with the T7 promoter-tagged primers (as depicted in Figure S4 ). Then the PCR products were verified by sanger sequencing and thereafter, transcribed by RNA transcription kit (New England Biolabs, English). The transcribed RNA was purified and recycled using denaturing polyacrylamide gel electrophoresis. The final RNA quality and concentration were measured by the NanoDrop UV-Vis spectrophotometer J o u r n a l P r e -p r o o f (Thermo Fisher Scientific Corporation, USA). Then the transcribed RNA was verified via RT-PCR kit (TaKaRa Bio Inc, Japan) The primers for LAMP (FIP, BIP, F3, B3, LF, LB) were designed according to the SARS-CoV-2 (GenBank accession number: MN985325.1) genome target sequences gene N (location: 28274 to 29533) and Orf1ab (location: 13051 to 13282). The Proofman probes were designed based on primer LB sequence, with the fluorophore and the quencher labeled at the end of 3' end mismatch nucleotide and 5' end nucleotide, respectively. The primers used for reverse transcription-PCR, conventional PCR were designed according to relative sequences. All sequences used in this study were presented in Tables S1. For PCR reaction, it was performed in 50 μL condition containing 5 U EasyTaq® DNA Polymerase, 5 μL 10 × EasyTaq® buffer (TransGen Biotech, Beijing, China), 0.2 mM deoxyribonucleoside triphosphates (dNTP), and 0.4 μM each of forward and reverse primer. The PCR reaction was incubated in a C1000TM Thermal Cycler PCR (Bio-Rad Laboratories, USA) for a total of 30 cycles (94 ℃ for 1 min, followed by 30 cycles of 15 sec at 94 ℃, 10 sec at 55 ℃ and 20 sec at 72 ℃. A final elongation step at 72 ℃ for 5 min). For RT-PCR, the One Step PrimeScript RT-PCR kit (TaKaRa Bio Inc, Japan) was used. The reaction was carried out in 25 μL condition according to the manufacturer's instructions with the exception that the concentration of forward and reverse primers was 0.64 μM and the 0.4 × SYBR Green I was used to monitor the real-time amplification. The RT-PCR reaction was incubated in PikoReal 24 RealTime PCR System (Thermo Fisher Scientific Corporation, USA) at 42 ℃ for 5 min, 95 ℃ for 10 sec and then 50 cycles of 5 sec at 95 ℃, 30 sec at 55 ℃ followed by a signal collection. For LAMP reaction, the reaction was performed in 25 μL mixture containing 2.5 μL Bsm DNA polymerase and AMV reverse transcriptase were doubled compared to singleplex assay. The sensitivity was evaluated by using 10-fold serial dilutions of the RNA templates. The specificity of the assay was measured by using the extracted genomics from 5 common Table S2 . The saliva samples were collected from consent informed healthy persons through published saliva specimen collection procedure. Then the pseudovirus (purchased from Yeasen Biotech Co., Ltd.) were spiked into the collected samples and taken as contrived real-life samples. The contrived samples were processed either by viral RNA isolation kit (Foregene, Chengdu, China) or cellular direct lysis buffer (Sigma-Aldrich, USA). 3.1 The principle of Proofman coupled with LAMP. The schematic strategy was shown in Figure 1A , the primers used for LAMP amplification were designed according to the target sequence. LAMP could produce the dumbbell structure in the initial amplification phase (step J o u r n a l P r e -p r o o f 1). After the initial phase, the products containing single-strand loop were generated during the exponential amplification phase (step 2). Then the Proofman probe, respectively labeled with fluorophore and quencher at 3' end and 5' end, together with a thermostable proofreading DNA polymerase (Pfu) were introduced to realize the sequence-specific detection ( Figure 1B ). Of note was that a deliberate mismatch at the 3' end of the Proofman probe was necessary to trigger the 3' → 5' exonuclease activity of the proofreading enzyme Pfu. Upon the binding of the Proofman probe to the target segment in the loop domain, the mismatched nucleotide would be cleaved by Pfu, releasing the fluorophore. Since then, the cleaved probe can further serve as an extendable primer which enhances the isothermal amplification efficiency (step 3). Based on the Proofman probe, the LAMP amplification products can be detected specifically through the increase of fluorescence intensity as the amplification reaction is proceeding. In our strategy, the sequence-specific detection of LAMP products was achieved by the binding and cleavage of the Proofman probe, thus enhancing the accuracy of LAMP reaction. Figure. 1 The schematic of specific detection of LAMP products using the Proofman probe. According to the genome information of SARS-CoV-2 from Global Initiative on Sharing All Influenza Data (GISAID, https://www.gisaid.org) and WHO guidance for laboratory testing of COVID-19 (https://www.who.int/publications-detail/laboratory-testing-for-2019-novelcoronavirus-in-suspected-human-cases-20200117), SARS-CoV-2 gene N (nucleocapsid phosphoprotein) was a conservative target in COVID-19 diagnosis (Corman et al. 2020) . To J o u r n a l P r e -p r o o f develop a specific detection platform for COVID-19 using the Proofman probe combined with LAMP, the same region of gene N was chosen to design LAMP primer sets (Figure 2A) . The plasmid containing the SARS-CoV-2 gene N cDNA sequence was successfully amplified by the conventional LAMP reaction in the absence of the probe (Figure S1A and S1B). Then the Proofman probe (labeled with FAM and BHQ1, Figure 2A ) was designed based on the loop domain of LAMP products and verified to be cleavable by proofreading enzyme Pfu under LAMP condition ( Figure S1C) . Next, the probe was introduced to the developed LAMP assay. As shown in Figure 2B , the reaction tube showed an increase in fluorescence intensity with 0.4 μM of Proofman probe, while reactions without the probe or template remained no change in fluorescence intensity. When verified with gel electrophoresis, as expected, all of the reactions except negative controls (without target template) presented characterized product bands on the gel electrophoresis ( Figure 2C , bottom). These results confirmed that the Proofman system was compatible with the established LAMP reactions and able to monitor the LAMP reaction real-timely. Moreover, we found that visualized detection could be realized under the 475 nm blue light (Figure 2C, upper), indicating that the assay was capable of end-point detection without uncapping operation or adding extra dyes. Due to the fluorescence intensity derives from the cleavage of the Proofman probe, we further investigated the concentration of the probe and Pfu to obtain the optimal condition. As shown in Figure S2A , increasing the concentration of the probe from 0.2 μM to1.2 μM produced increasing fluorescence intensity, while the reaction rate remained unchanged. However, changing the concentration of Pfu did not influence the fluorescence intensity ( Figure S2B) . Thus, the final concentration of the probe and Pfu used for the following study were 0.4 μM and 0.1 U, respectively. To investigate the feasibility of Proofman-LAMP in the detection of SARS-CoV-2 RNA, we artificially synthesized the RNA template of gene N by in vitro transcription and verified it with RT-PCR ( Figure S4 ). Avian Myeloblastosis Virus (AMV) reverse transcriptase was chosen to amplify the RNA template because it keeps active even under the LAMP temperature (60 ℃, Figure S5A) . We explored the effect of AMV reverse transcriptase on the Proofman-LAMP reaction and found that the 1 U of AMV reverse transcriptase was enough to develop the reverse transcription Proofman-LAMP, namely RT-Proofman-LAMP ( Figure S5B) . Then, the RT-Proofman-LAMP reactions were carried out with the target template and non-target template parallelly. As illustrated in Figure 2D , only the reaction containing the target template displayed an increase in fluorescence intensity. In contrast, the signal change in reactions containing nontarget template or negative control was undetectable. Additionally, the end-point detection J o u r n a l P r e -p r o o f showed a clear visual difference between positive reactions and other reactions ( Figure 2E) . These results demonstrated that the Proofman-coupled LAMP was successfully applied to the detection of the targeted sequence of SARS-CoV-2. To determine the sensitivity of the assay, the serially diluted synthetic SARS-CoV-2 RNA templates were taken as input samples for RT- Figure 3A , the RT-Proofman-LAMP could efficiently detect as low as 100 copies of gene N RNA in less than 1 hour. A quantification time Tq, which is similar to the Cq in quantitative PCR, was introduced to the real-time RT-Proofman-LAMP assay as the reaction time when fluorescence intensity exceeds an arbitrary threshold. Figure 3B , the Tq values of the assay were in linear correlation to the concentration of the target, suggesting the assay has the potential for quantitative analysis. The end-point visual outcome also presented unambiguous distinguishment between positive and negative reactions after 50 min incubation, confirming the assay was a sensitive method ( Figure S6) . The reported viral load of infected patients at the onset of symptom could be 10 5 -10 7 copies per milliliter of sputum specimen ), which indicates that the limit of detection for the RT-Proofman-LAMP was sufficient to realize the detection at the early phase of COVID-19. Next, we sought to verify the specificity of the RT-Proofman-LAMP. We conducted an assay using RT-Proofman-LAMP to discern the SARS-CoV-2 from 5 different pathogens, which are closely related to pathogenic infection. The results illustrated in Figure 3C that the RT-Proofman-LAMP correctly discerned different pathogens and showed no cross-reactivity. The visualized results under the blue light also confirmed the high specificity of the assay (Figure 3D) . It is worth mentioning that the SARS-CoV-2 is extremely high homology to SARS-CoV at the nucleotide level 17 . The results demonstrated J o u r n a l P r e -p r o o f that RT-Proofman-LAMP could efficiently distinguish these two homologous sequences ( Figure 3C and 3D) . Therefore, the RT-Proofman-LAMP assay could be a sensitive method for SARS-CoV-2 detection with high specificity. Proofman-coupled LAMP assay was theoretically accessible to realize multiplex detection which could be helpful to improve the accuracy of the COVID-19 detection. Gene Orf1ab (ORF1ab polyprotein), another conservative domain in SARS-CoV-2 genome, was also recommended as a target for COVID-19 diagnosis according to the standard testing guideline published by WHO and Chinese Center for Disease Control and Prevention (Jung et al. 2020; Prevention 2020) . Thus, we also sought to develop a Proofman-based assay for the detection of gene Orf1ab. In this case, the Proofman probe used for Orf1ab was labeled by another fluorophore HEX. After the establishment of singleplex detection of gene Orf1ab using RT-Proofman-LAMP (Figure S9) , we investigated the feasibility of multiplex detection of RT-Proofman-LAMP by combining two sets of primers and probes in one tube to detect SARS-CoV-2 gene N and gene Orf1ab concurrently. As shown in Figure 4A and 4B, only the reaction tube containing the mixed template (equal mixing of SARS-CoV-2 gene N and Orf1ab RNA) presented the fluorescence curves both in FAM and HEX channels, while the reaction tube containing one kind of templates (SARS-CoV-2 gene N or Orf1ab) presented fluorescence curve just in one fluorescence collection channel, demonstrating the duplex was J o u r n a l P r e -p r o o f available using RT-Proofman-LAMP. Given that inner control plays an important role in clinical detection, we aimed to develop a triplex assay in which the human glyceraldehyde-3phosphate dehydrogenase (GAPDH) gene mRNA was taken as inner control. As illustrated in Figure S10 , when adding triple-mixed template (containing SARS-CoV-2 gene N, gene Orf1ab and human GAPDH mRNA) to the reaction comprising three sets of corresponding primers and probes, the fluorescence curves appeared both in three fluorescence collection channels (FAM, HEX and ROX), suggesting the triplex assay was successfully conducted. Although multiplex detection is a favorable method in molecular detection, few LAMP-based methods are capable of multiplex detection in one pot due to the lack of suitable reporters. The Proofman-based LAMP assay provided a good alternative to achieve multiplex detection in a single step, which could further strengthen the specificity of the assay. Moreover, the inclusion of the inner control in one pot could guarantee the quality of specimen processing, decreasing the false-positive results. 3.5 Evaluation of the assay using contrived samples. After the development of the assay, we sought to evaluate the performance of the RT-Proofman-LAMP to detect real-life samples. The saliva specimen has been proposed as a reliable tool for the diagnostic of SARS-CoV-2 (Azzi et al. 2020) , which is easy to collect and highly appreciated in POCT. Based on the RT-Proofman-LAMP, a general workflow was proposed to realize the rapid detection of SARS-CoV-2 ( Figure 5A) . Due to the lacking of clinical samples from infected patients, the pseudovirus containing the SARS-CoV-2 virus partial genome and the retrovirus envelope was spiked to saliva samples from informed individuals to simulate real-life samples. The spiked saliva samples were processed either by viral RNA extraction kit or commercial direct lysis buffer. Then 1 μL of processed samples were inputted to the RT-Proofman-LAMP assays. We first checked the ability of the assay to detect the pseudovirus in the presence of genomic RNA (RNA extraction Kit) or cellular lysate (lysis buffer). The results demonstrated J o u r n a l P r e -p r o o f that RT-Proofman-LAMP was able to detect the target viral RNA without cross-reaction with genomic RNA or cellular lysate ( Figure S11) . Then the spiked samples were used to evaluate the singleplex and multiplex RT-Proofman-LAMP assay. For the singleplex assay, as shown in Figure 5B , after 50 min incubation only the tube with spiked samples showed an increased fluorescence under the blue light, indicating the RT-Proofman-LAMP could be a qualitative method through visual results. Additionally, the method was compared to conventional RT-PCR and showed comparable analytical performance ( Figure S12A) . Afterward, the duplex assay was examined. When using a duplex assay that simultaneously detects SARS-CoV-2 gene N and the inner control, both the fluorescence signals in FAM and ROX channel were detected in the tube containing spiked samples ( Figure 5C ). Another duplex detection targeting gene Orf1ab and inner control was also successfully achieved ( Figure S12B ). Next, the triplex assay that includes both two targets of the viral genome and the inner control was tested. As can be seen from Figure 5D , three corresponding fluorescence signals of FAM (blue curve), HEX (red curve) and ROX (green curve) were concurrently appeared in one tube containing spiked samples, verifying the accessibility of the triplex assay. These results validated that the RT-Proofman-LAMP was capable of detecting the contrived samples in the way of the singleplex or multiplex assay. Facing the challenge of COVID-19, varied diagnostic requirements are needed under different settings. Based on the above results, we provided three solutions to meet diverse diagnostic demands. The simplest singleplex assay could be readily used to fast pre-screening of suspected cases in some resource-limited regions where the sophisticated instrument is out of reach. To improve the diagnostic accuracy, the duplex assay established above was a convenient one that can guarantee the sureness of a test and avoid the uncertain test results caused by improper sample processing. As an evolving virus, SARS-CoV-2 may generate some latent mutants in its genome, thus the triplex assay that detects two targets of SARS-CoV-2 genome could be an efficient way to prevent the situation. Taken together, the RT-Proofman-LAMP was a versatile method that embraces the potential to realize accurate POCT. J o u r n a l P r e -p r o o f In summary, this work combined the proofreading-based detection method with the LAMP condition for the first time, which realizes the sequence-specific detection of LAMP amplicon. With the Proofman probe, the multiplex detection can be achieved in one pot, which bypasses the uncapping operation. In addition to real-time monitoring, colorimetric detection was also realized under blue light, which can give fast qualitative results. Unlike many reported LAMP-based methods that achieved the fast colorimetric SARS-CoV-2 detection with non-specific reporters, the RT-Proofman-LAMP assay could improve the diagnostic accuracy by providing a sequence-specific colorimetric result. Based on the visualized singleplex assay, the fast pre-screening of suspected individuals could be finished in 50 min using direct lysed samples, which is highly suitable for POCT. Using multiple fluorogenic probes, the one-pot multiplex assay could provide a robust laboratory testing platform for accurate diagnosis of COVID-19. All in all, the Proofman-based LAMP offers a highly specific platform for the detection of SARS-CoV-2, promising in enhancing the accuracy of the COVID-19 diagnosis. Sichuan Science and Technology Program (grant numbers 18PTDJ0083, 2019ZDZX0048, 20ZDYF2224 and 2019YFS0331); and China Postdoctoral Science Foundation (grant number Saliva is a reliable tool to detect SARS-CoV-2 High-surety isothermal amplification and detection of SARS-CoV-2, including with crude enzymes Recombinase assisted loop-mediated isothermal DNA amplification Comparative Analysis of Primer-Probe Sets for Causative Virus (SARS-CoV-2) Nucleic acid-based fluorescent probes and their analytical potential Tolerance of loop-mediated isothermal amplification to a culture medium and biological substances Viral Load Kinetics of SARS-CoV-2 Infection in First Two Patients in Korea A Novel Reverse Transcription Loop-Mediated Isothermal Amplification Method for Rapid Detection of SARS-CoV-2 Development of Reverse Transcription Loop-Mediated Isothermal Amplification Assays Targeting Severe Acute Respiratory Syndrome Coronavirus 2 (SARS-CoV-2) DNA detection using recombination proteins A novel coronavirus outbreak of global health concern Limits of Detection of 6 Approved RT-PCR Kits for the Novel SARS-Coronavirus-2 (SARS-CoV-2) Rapid and visual detection of 2019 novel coronavirus (SARS-CoV-2) by a reverse transcription loopmediated isothermal amplification assay Isothermal amplified detection of DNA and RNA Multiplex reverse transcription loop-mediated isothermal amplification combined with nanoparticle-based lateral flow biosensor for the diagnosis of COVID-19 copies to 10 2 copies of SARS-CoV-2 gene N synthetic RNA. The error bars are the standard deviation of three repetitive measurements. (C) The specificity of RT-Proofman-LAMP in the detection of SARS-CoV-2 gene N synthetic RNA. (D) The visual image of specific detection of SARS-CoV-2 gene N synthetic RNA after 50 min incubation. The amount of Pseudomonas aeruginosa, Escherichia coli, Klebsiella pneumoniae, Staphylococcus aureus, Candida tropicalis and SARS-CoV-gene N was 26 ng A) The real-time fluorescence in the FAM channel of duplex assay using different templates. (B) The real-time fluorescence in the HEX channel of duplex assay using different templates. The mixed template comprised an equal amount (1×10 6 copies) of SARS-CoV-2 gene N and gene Orf1ab RNA. The gene Orf1ab RNA template was obtained by in vitro transcription and Evaluation of RT-Proofman-LAMP using spiked saliva samples. (A) The general workflow to detect saliva samples using Proofman-coupled LAMP. (B) Visual detection of singleplex RT-Proofman-LAMP. The spiked sample contained 50 copies of pseudovirus Duplex assay of RT-Proofman-LAMP using spiked saliva sample (containing 50 copies of pseudovirus). (D) Triplex assay of RT-Proofman-LAMP using spiked saliva sample This work was supported by the National Natural Science Foundation of China (grant numbers 21907090, 21708037, and 21877108); the Innovative Team of Sichuan Province