key: cord-0959928-uixv789m
authors: Wang, Yang; Xu, Huiren; Dong, Zaizai; Wang, Zhiying; Yang, Zhugen; Yu, Xinge; Chang, Lingqian
title: Micro/Nano biomedical devices for point-of-care diagnosis of infectious respiratory diseases
date: 2022-02-12
journal: Med Nov Technol Devices
DOI: 10.1016/j.medntd.2022.100116
sha: 467eebc82ce242b23b934c037bf058b625d32df6
doc_id: 959928
cord_uid: uixv789m

Corona Virus Disease 2019 (COVID-19) has developed into a global pandemic in the last two years, causing significant impacts on our daily life in many countries. Rapid and accurate detection of COVID-19 is of great importance to both treatments and pandemic management. Till now, a variety of point-of-care testing (POCT) approaches devices, including nucleic acid-based test and immunological detection, have been developed and some of them has been rapidly ruled out for clinical diagnosis of COVID-19 due to the requirement of mass testing. In this review, we provide a summary and commentary on the methods and biomedical devices innovated or renovated for the quick and early diagnosis of COVID-19. In particular, some of micro and nano devices with miniaturized structures, showing outstanding analytical performances such as ultra-sensitivity, rapidness, accuracy and low cost, are discussed in this paper. We also provide our insights on the further implementation of biomedical devices using advanced micro and nano technologies to meet the demand of point-of-care diagnosis and home testing to facilitate pandemic management. In general, our paper provides a comprehensive overview of the latest advances on the POCT device for diagnosis of COVID-19, which may provide insightful knowledge for researcher to further develop novel diagnostic technologies for rapid and on-site detection of pathogens including SARS-CoV-2.

The ongoing outbreak of COVID-19 has caused a global pandemic with considerable morbidity and mortality [1, 2, 3, 4] . Without timely diagnosis and treatment, some COVID-19 patients may develop into worse symptoms, including pneumonia and acute respiratory distress syndrome, even deaths, especially for the seniors above 50 years old [5, 6] . The fighting against COVID-19, among all infectious diseases caused by viruses, still remains challenging to the human beings, albeit 2 tremendous efforts and technical advances in public healthcare [7] . Although various medicines or vaccines have been proved to be effective to the disease [8, 9, 10] , advanced techniques for rapid and accurate detection of the virus still greatly contribute the control on viral spreading and early treatment [11, 12, 13] . SARS-CoV-2 is one of the beta coronavirus genera, which comprises a nucleocapsid (N) protein J o u r n a l P r e -p r o o f 3 associated single-stranded positive-sense RNA (29, 881 nucleotides, the genetic material) and three structural surface proteins, including the membrane (M), the spike (S) and the envelope (E) ( Figure  1a ) [14, 15, 16, 17, 18] . It has been demonstrated that SARS-CoV-2 is infectious in humans, animals, and herds [19] . Compared with the other emerging viruses that have caused wide epidemics in recent years, such as Middle East respiratory syndrome coronavirus (MERS), severe acute respiratory syndrome coronavirus (SARS-CoV), Ebola virus and Zika virus, SARS-CoV-2 is spreading with a significantly higher rate and wider range [20, 21, 22, 23, 24] , making even more difficult to control. The major symptoms of infected patients include neurological and respiratory diseases, such as fever, pain in the muscles and tiredness, cough and shortness of breath [25, 26, 27] . Unfortunately, these symptoms are not specific for the diagnosis of the infection [28] .

In the past few months, numerous scientific teams and companies have reported methods for COVID-19 detection [29, 30, 31, 32, 33] . In terms of their working principle, the major diagnostics methods include: immunoassay-based methods for detection of antibodies in blood serums [34, 35, 36, 37] and nucleic acid testing (NAT) for direct determination of the virus in nasal/throat swabs ( Figure 1b) [38, 39] . The characteristics of some frequently used NAT methods and immunoassaybased methods are summarized in Table 1 . Thanks to the advantages of robust and sensitive assay, NAT has gained tremendous development with the technical innovation in molecular biology and biomedical engineering, and currently it is a gold standard for COVID-19 diagnosis [40, 41] . They can identify and detect trace amounts of the specific viral genomic sequence with various amplification, e.g. reverse transcript -polymerase chain reaction (RT-PCR). In terms of the mechanism underlying the routes for identifying and amplifying the targeted nucleic acids, three methods are currently adopted, including thermo-cycling-based amplification, isothermal amplification methods and CRISPR-based methods ( Figure 1c ) [42, 43, 44] . NAT is generally very sensitive, but it needs a central laboratory and well-trained technical to operate experiments and interpret the data. Alternatively, immunoassays can provide the information concerning any active viral infections as well as past exposures [45] . The basic mechanism of immunoassay was to detect the specific antibodies against SARS-CoV-2 produced by the immune response in blood serums [46] , particularly immunoglobulin M (IgM) and immunoglobulin G (IgG) [47] . As a result, detecting the existence of IgG and IgM antibodies against SARS-CoV-2 is a feasible way to indicate infection [48] . Furthermore, due to the reason that there are a large portion of the population that have been vaccinated, it is important to distinguish between actual infection and vaccination. According to the suggestions of China Food and Drug Administration (CFDA), a combination test of IgM antibodies against the S protein and the N protein can help. Specifically, the people who has a positive IgM antibody test against the S protein needs to take an extra test against the N protein. If both tests were positive, it means that the antibodies are induced from an actual infection. Otherwise, the antibodies are induced from vaccination. Usually, SARS-CoV-2 triggered antibodies could be detected as early as on the 3rd day and decrease gradually as immune responses go on in patients' body. The antibodies generally become undetectable in about two weeks (Figure 1d ) [49] . Typically, IgM antibodies appear in the serum samples in an earlier stage than IgG does. To date, a wide variety of immunoassays have been developed to detect SARS-CoV-2 antibodies, including enzyme-linked immunosorbent assay, chemiluminescent immunoassay [50] and even a lateral flow immunoassay (Figure 1e ) [51] . Compared with NAT, these immunoassays can provide more convenient and rapid detection of SARS-CoV-2 antibodies in human serum or blood without needing biosafety laboratories, which can also be suitable for the epidemiological of COVID-19. Clinically, chest computed tomography (CT) [52, 53] and transmission electron microscopy (TEM) [54] also assist in the evaluation and diagnosis of the symptomatic patients. Nevertheless, these instruments are unaffordable in most undeveloped countries. So far, noticeable reviews about SARS-CoV-2 have been provided, with special focus on the origin [55, 56] , transmission [57, 58] , clinical features [59, 60, 61] , and even treatment methods [62, 63, 64] . However, a timely review comprehensively summarizing the advancements of rapid diagnostics platforms for point-of-care testing (POCT) of SARS-CoV-2 remains open, especially for those with improved performance by involving micro and nanotechnologies. In this review, we summarize the emerging micro-/nanoscale biomedical devices applied for detecting SARS-CoV-2 in the last two years, which can provide a fast turn-around and sample-to-answer assay. In particular, those micro-nano devices may provide a point-of-care testing and home diagnosis to release the burden of central hospital [65] . We hope this review offers an insight on the methodologies used in developing advanced devices for pointof-care detection of COVID-19 and inspires novel diagnostic technologies in clinical trials in the future.

Detection mechanism of SARS-CoV-2

Polymerase chain reaction (PCR) offers ultra-high sensitivities and sequence specificities in medical and biological applications, including DNA sequencing [66] , functional genes analysis [67] and infectious diseases identification [68] . Especially during the current period, a great number of J o u r n a l P r e -p r o o f 5 efforts have been made to improve the performances of PCR systems, which have boosted the whole market. With an additional reverse transcription (RT) process that transfers RNA into complementary DNA (cDNA) strands, RT-PCR can be used for direct detection of RNA-viruses [69] . In the past few years, RT-PCR has achieved a considerable achievement that speeded up its practical applications. Basically, a standard RT-PCR test takes about 3 hours from RNA extraction to the final amplification ( Figure 1c ) [70] . It uses specific primer sets to hybridize and amplify the target genomic sequence [71] . With the designed primers, it is possible to test the presence of SARS-CoV-2 with a real-time PCR instrument in a Biosafety Level II Laboratory [38] . However, as the gold-standard method, RT-qPCR requires central laboratory and skilled person to operate and interpret the data. The time-consuming and high-cost facts of the thermal-cycling instruments limit their applications in most of on-site, point-of-care circumstances [72] . Moreover, the dependence on the specialized reagents further limits its universally available in those resource-limited regions [73] . Presently, the existing regents and enzymes for the PCR reactions typically require specific refrigeration for storage and transport [74] . As a result, the reagents and medical professionals may be easily constrained in those low and middle-income countries during the pandemic. To improve the testing capabilities in remote locations or at the point-of-care applications, more attention should be given to the innovations of low-cost and stable reagents for PCR with the consideration of roomtemperature stable reagents [26, 75] . In most scenarios where the expensive thermal cycling instruments are not affordable, isothermal amplification methods, including loop-mediated isothermal amplification (LAMP) [40] , recombinase polymerase amplification (RPA) [76] , nicking enzyme amplification reaction (NEAR) [77] and rolling circle amplification (RCA) [78] have been developed for the point-of-care testing of SARS-CoV-2. These isothermal amplification methods, conducted with a fixed temperature [79] , are independent of expensive thermal cycling units that a PCR amplification needs. Each of these methods has its unique strategy or mechanism to initiate and recycle a new round of dsDNA separation, extension and synthesis ( Figure 2 ). Among them, LAMP and RPA are initiated by a DNA target while NEAR enables direct RNA identification and amplification [40] . In addition to the above advantages, there are also actually known issues for isothermal amplification such as nonspecific or non-template amplification.

Reverse transcription loop-mediated isothermal amplification (RT-LAMP) is one of the most common isothermal methods for RNA-based pathogen diagnosis [80, 81] , which consists of a reverse transcriptase process and a one-step amplification reaction where RNA plays a part as the final template (Figure 2a ). It can recognize and amplify a specific nucleic acid fragment at a constant temperature (60-65 °C) in less than one hour with high sensitivity by utilizing a set of four to six primers and a strand-displacement polymerase [82] . The stem-loop DNAs as the final products include multiple inverted repeats of the target and exhibit a cauliflower-like appearance. In comparison with the real-time RT-PCR assay, a single protocol-based LAMP is a more straightforward method that can fade the dependence on thermocycler as well as energy consumption [83] . The RT-LAMP results from viral RNA amplification are usually read out colorimetrically or fluorescently, by adding colorimetric pH indicators or fluorescence dyes [84] .

In addition, LAMP could also be integrated with sequencing infrastructures [85] . Up to now, LAMP assay kits have already been commercially available. Davidson et al. used paper basedstrategy and RT-LAMP to develop an instant device, which visually detected SARS-CoV-2 in saliva in 60 min, with a detection limit of up to 200 copies/μl [86] . However, it does not show absolute superiorities over PCR in clinical scenarios due to the fact that there are limited suitable devices which can do sample processing and RNA extraction on-site [80] . Moreover, there are four to six primers used during LAMP reactions, as a result, the primers need to be strictly designed to avoid potential cross-interactions. Moreover, LAMP may cause false positive detection of samples as well as the carry-over contaminations.

Compared with LAMP, RPA is a relatively new isothermal amplification method reported firstly in 2006 [87] . However, it has experienced an exponential growth in terms of popularity and applications due to the advantages of fast reaction speed and high sensitivity [88] . During amplification, recombinases are combined with primers to form protein-DNA complexes that can bind specifically to the target genes, initiating chain exchange reactions and DNA replications. It is capable of amplifying as low as 1 ~ 10 DNA target copies within 10 min with minimal sample preparation [89] . The amplification is under control from a specific combination of enzymes and proteins below 37 °C (Figure 2b ). With a reverse transcription process, RT-RPA based assays could 7 be easily adapted for detecting SARS-CoV-2 [90, 91] . The developed assay produced 100% diagnostic sensitivity and specificity with a total run time between 15 and 20 min when compared to RT-qPCR (n=20), indicating a viable alternative detection method [76] . Thomas et al. developed an RPA-LF based on test strips that detected 35.4 copies /μl of SARS-COV-2 cDNA nucleocapsid (N) gene [91] . However, the prices of RPA kits are relatively high, which limits its clinical applications. Moreover, the flexibility in the kit formulation, as well as the application, are highly limited compared to other isothermal methods [92] .

NEAR belongs to the family of isothermal amplification detection methods, which is mainly used for detection of short oligonucleotide sequences [40] . With the help of a DNA polymerase, the primer will extend in the presence of a target template (Figure 2c ). The extended primer will be cut by the nicking endonuclease, releasing the short oligonucleotides due to insufficiently stable duplex under 55 °C. Subsequently, the primers are regenerated and undergo another round of extension and cleavage. Based on the NEAR isothermal amplification technique, a rapid detector called ID NOW has been manufactured by Abbott. Co (Chicago, IL, USA) and authorized [93, 94] .

RCA is an efficient isothermal enzymatic process that simulates the rolling circle replication process of natural microbial circular DNA ( Figure 2d ) [33, 95] . With a DNA polymerase, a single primer can trigger the strand displacement synthesis along the circular DNA template to achieve isothermal linear amplification. Owing to its isothermal nature, it is an ideal method with a simple and efficient process. Up to now, RCA-based detection systems or platforms have been successfully applied to test various types of targets [96] . Typically, in a circle-to-circle amplification process, amplicons of the first round RCA will be converted into multiple circles by monomerization (endonuclease digestion) and ligation. Subsequently, newly formed circles will act as templates for the following round RCA, thus reaching an ultra-low limit of detection [97] . To further improve the efficiency of amplification, some exponential or quadratic amplification formats are developed and combined with RCA-based approaches. As a result, it will achieve a detection limit up to subfemtomolar level [98] . Moreover, it significantly simplifies the operation without the dependence on the time-consuming and labor-intensive operations. Tian et al. reported a typically RCA-based amplification method for quick and ultra-sensitive detection of SARS-CoV-2, achieving a limit of detection of 0.4 fM [78] . Generally, the amplification template for RCA is required to be circular DNA or a linear DNA circularized firstly. In addition, the results of RCA do not have ideal quality control goals up to now, which greatly limit their wide applications.

CRISPR/Cas-based nucleic acid detection technologies were recently developed for COVID-19 detection [99] , by using a unique group of Cas-nucleases, which demonstrated noticeable advantages of sensitivity, specificity, rapidity and simplicity for detection ( Figure 2e ). By using extracted nucleic acids as input, both CRISPR Cas13-and Cas12-based assays have been developed for SARS-CoV-2 detection [100] . Cas12, as an RNA guided DNase, can cleave ssDNA indiscriminately upon binding its target sequence [101] . In normal conditions, it will be combined with isothermal amplification to achieve high detection sensitivity and specificity. Broughton et al. proposed a CRISPR-Cas12-based assay, which performed RT-LAMP at 62 °C for 20 ~ 30 min followed by Cas12 detection at 37 °C for 10 min of predefined coronavirus sequences and visualized on a lateral flow strip [102] . Other isothermal amplification methods, such as recombinase aided amplification (RAA) have also been used to amplify the extracted RNAs before a CRISPR/Cas12a reaction. When SARS-CoV-2 presents in the system, a quenched green fluorescent molecule J o u r n a l P r e -p r o o f 8 labelled ssDNA reporter will be cleaved by Cas12a, resulting in the motivation of green fluorescence, which can be observed directly with a naked eye under 485 nm light [103] .

In comparison, Cas13a is a non-specific RNase that remains inactive until it binds its programmed RNA target [104] . Cas13a-based detection is highly programmable and specific, as it relies on complementary based pairing between the target RNA and the CRISPR RNA sequence [105] . A CRISPR-Cas13a-based tool named SHERLOCK (Specific High-sensitivity Enzymatic Reporter unLOCKing) was recently designed by Feng Zhang group specifically for SARS-CoV-2 diagnosis. This protocol involves an RPA and T7 transcription, followed with method Cas13mediated collateral cleavage of a single-stranded RNA reporter. Combining with colorimetric or fluorescent readouts, the assay enabled detection of 10 copies/μL of synthetic RNA [106] . In the pursuit of less time and labor-intensive, Arizti-Sanz et al. finalize detection by combining isothermal amplification, T7 transcription and Cas13-based detection into a single step. Compared to the twostep assay, this single-step SHERLOCK assay could diagnose SARS-CoV-2 with reduced sampleto-answer time and equal sensitivity with optimized conditions [107] . Zhang et al. combined RPA with SHERLOCK to detect the S gene and Orf1ab gene of SARS-COV-2 [108] .

The CRISPR-based molecular diagnostics has great potential towards POCT, quantitation and digital analysis of SARS-CoV-2 with detection sensitivity comparable to real-time RT-PCR assay. If coupled with lateral flow readouts, they will be an attractive option for easy, at-home testing scenarios. However, as newly-emerged methods, more efforts should be taken to guarantee its accuracy and prevent the issues of aerosol contamination and false positive rate in clinical trials.

Serological testing of antibodies is another common method for detection of COVID-19. Compared to nucleic acid methods, it offers advantageous turn-around time, throughput and workload [109, 110] . Although a wide range of doctors and experts have marked that the results from immunological methods may not be considered for the final diagnosis since they only indicate the previous infection, it does not mean that the IgM/IgG serological tests are useless since the immune status of individuals is still important to be acknowledged by the doctors in the following step of treatment (Table 2 ) [111] . The clinical interpretation of all possible scenarios that can be encountered when testing a patient with both RT-qPCR and IgM/IgG immunoassay are illustrated in Table. 2. Based on the current knowledge about the rise and fall of SARS-CoV-2, the correlation of IgM level and IgG level varies during the initial time of infection, the onset of symptoms and recovery phase. The key takeaway is that the results of nucleic-acid tests and IgM/IgG serological tests do not necessarily need to agree [49] . A disagreement between the two tests, if any, can often be traced to the after-infection time points at which the tests were performed. Since the exact time of infection is often unknown, combining these two testing can further improve the accuracy of COVID-19 diagnosis [112, 113] .

Enzyme-linked immunosorbent assay (ELISA) is one of the most widely used methods for the detection of protein-based biomarkers [114, 115] . Briefly, the ELISA for total antibodies detection is developed based on double-antigens sandwich immunoassay, using mammalian cell-expressed recombinant antigens contained the receptor binding domain (RBD) of the spike protein of SARS-CoV-2 as the immobilized and HRP-conjugated antigen. According to statistics, compared with a single PCR test, the positive detection rate is significantly increased from 51.9 % to 98.6 % by combining the PCR with the ELISA assay for each patient [116] . Srivatsa et al. used aptamerfunctionalized gold nanoparticles to identify SARS-CoV-2 spike proteins, limit of detection can up to 3540 genome copies/μl [117] . However, the cross-reactivity and low antibodies titers are among common factors that limited the detection efficacy of ELISA. It is also critical to executing the procedures of serial washings and incubation with reagents in ELISA to reduce the background noise and amplify the signal. In clinical, their results are used as an assistant to diagnose the infection.

Usually, the timing of requests for serological assays and the interpretation of antibody results are pre-requisites of crucial importance in their efficacy [118] . Combining with chemiluminescence and the immunoreactions, chemiluminescent immunoassay (CLIA) can quantitatively determine the concentrations of corresponding antigens or antibodies through the intensity of luminescence with high sensitivity and specificity [119] . Based on automatic platforms, CLIA enables high throughput detection, making an outstanding contribution to the early screening. Lyu et al. used ABEI/Co2+ dual-functionalized magnetic beads to perform rapid CLIA detection of SARS-CoV-2 nucleocapsid protein (NP) [120] .

Compared with ELISA and CLIA, lateral flow immunoassay (LFI) enables direct test without extraction, which made it well fit for the large-scope, on-site screening [121] . LFI typically contain sample pad, conjugation pad, nitrocellulose membrane, test line, control line and plastic cassette [122] . The mechanism of LFI is based on the hydration and transport of reagents as the specimen across the strip via chromatographic lateral flow. If anti-SARS-CoV-2 IgG and IgM antibodies present in the sample, they will be bound by the corresponding antigen labelled gold colorimetric reagent fixed on the conjugate pad. With samples continuing to travel up the strip, the IgM antibodies are bound on the M (IgM) line, and the IgG are bound to the G (IgG) line, presenting a reddish-purple line at the test zone [112] . During the performance of all valid tests, a control line will appear whether the sample is positive or negative, demonstrating the fluid has migrated adequately through the device. In normal conditions, the detection takes at most 15 min to obtain results with one drop of various specimens such as sera, plasma of venous blood and finger stick blood. Chen et al. developed a LFIA strip based on SERS for anti-SARS-COV-2 IgM and IgG [123] . However, when the concentration of antibodies is none or at a low level, there is a risk of missed detection by the false negative results.

10 Table 2 . The clinical significance of IgM/IgG serological test results. ("+" means "Positive", "-" means "Negative").

Recent advances in microfluidic technology and nanotechnology have brought us closer than ever to the realization of simple yet highly sensitive and specific devices that could be used in complicated environments without central lab. Based on either nucleic acid testing or immunoassay, the micro/nano devices significantly enrich the toolset of POCT of SARS-CoV-2, which have the potential to rapidly diagnose pathogens or antibodies and efficiently monitor the infection transmission by self-tests even at home. They can act as a bridge between laboratory-based testing and home detection. Presently, more and more these devices are transformed by the companies as promising platforms for COVID-19 detection. Especially those miniaturized devices, which integrated all the steps (nucleic acid extraction, amplification and detection) by fluidic manipulation, are conducive to complex real-time diagnosis. Moreover, the introduction of nanomaterials could also significantly increase the detection sensitivity of immunoassays. In this section, we summarize the very recent progresses on the micro/nano technologies in the field of POCT, hoping to provide useful information and insight for the further researches in the area.

J o u r n a l P r e -p r o o f In a typical diagnostic test, there are two types of inaccuracy, including the false-negative result (FNR) and the false-positive result (FPR) [124, 125] . Statistically, RT-PCR assay based on nasal or oropharyngeal swabs could produce up to 30% FNR in the clinical diagnosis of COVID-19 [126, 127, 128] . On the standpoint of the clinical stage of the disease and different anatomic sites in the virus-carriers, sampling strategy has a close relationship with the inconsistency of viral load which resulted in the high FNR [39] . In a traditional sampling process, regular swabs can only provide limited physical interactions with mucosal tissues. As a result, only superficial tissues could be collected, which are also readily contaminated by food and drink, resulting in a low sampling efficacy [128] . Chen et al. reported a microneedle-based oropharyngeal swab for effective and precise viral sampling. Based on the soft-tissue penetration capability of these microneedles (MNs), there would be a significant increase in sample depth (Figure 3a ). In addition, the MNs are modified with antibodies, which will further assist in SARS-CoV-2 collection through chemical bonding [128] . Once the preparation process can be simplified, the proposed novel swab will act as a promising candidate for diverse oral or respiratory diseases sampling in the future. However, it is also worth noting that medical staffs will be in close contact with the suspected COVID-19 patients during sampling, leading to a high risk of cross-infection. In addition, the swabs themselves are potential source of infection [129] . To solve this problem, a miniature robot consisted of an active 2-degree of freedom (DOF) end-effector was proposed to assist nasopharyngeal swab collection remotely. The successful working of the miniature robot has already been verified on a pig nose. Subsequent works will focus on pursuing ethical approval for in-vivo tests. The captured nasal or oropharyngeal swabs will then be subjected to a series of standard procedures for the subsequent lysis and enrichment. Effective DNA extraction and enrichment is the premise of accurate detection [130] . However, this process not only relies on enhanced-biosafety lab, but also requires skilled personnel and mandatory instruments. Manual operation procedures may raise issues, such as artificial variants or biased data. Followed with sample preparation, a variety of nucleic-acid based methods, ranging from PCR-based methods to some isothermal amplification methods, are available to the diagnosis of infectious diseases. From sample preparation to the assay protocol, it usually requires a few hours [131] . To meet the diagnostic demands of the infectious pathogens, especially in those resource-limited settings, there is an urgent need for portable and integrated microfluidic platforms or micro/nano devices that can provide fast, accurate and even multiplex diagnosis at the point-of-care [132] .

Generally, traditional PCR instruments are practical obstacles for wide use in POCT scenarios due to the reason that they are more expensive and bigger in size [28] . They rely heavily on external electric powers to realize quick increase or decrease of the temperature. Owing to their greatly reduced size, micro/nano devices possess many unique properties compared to macro-scale devices, which opens a new perspective for field testing based on PCR. They require less reagents during amplification and have higher heat transfer efficiency. Moreover, the improved portability makes them an ideal choice for point-of-care diagnosis of COVID-19 [133, 134] . Shi et al. reported a miniaturized, portable and battery-powered heater with functions of thermo-cycled control and passive continuous-flow control as the platform for PCR reactions (Figure 3b ). Integrated with a 3D microreactor, the system can be used for multiplexed detection of clinical-level DNA targets with more convenience [28] . Microfluidic systems are also well suited for highly automated processes. Recently, a microfluidic device integrated with functions of sample treatment, one step RT-PCR and direct fluorescence detection was developed and verified with influenza-A viruses (Figure 3c ). The device enabled automatic sample lysis and enrichment by using glycan-coated magnetic beads, whose capture rates could be 50% [135] . The sealed microfluidic device, with all reagents preloaded, could be adapted to detect SARS-CoV-2 easily. Another factor that limits the widespread use of PCR is the detection time. Under normal conditions, a standard PCR procedure takes at least 45 min. Based on microfluidic devices, a compact, high-speed reciprocal flow RT-qPCR system, GeneSoC ® , has become available for specific gene amplification and detection within 15 min [136] ( Figure 3d) . The system has one heater for the RT reaction and two heaters for thermal cycling, with two micro-blowers at each flow ends for the high-speed shuttle of the PCR solution. It can achieve a limit of detection (LOD) of 1.0 × 10 1 copies/reaction with the use of a single disposable tip per analysis. Although it has some disadvantages, such as requiring the simplification and refinement of the RNA extraction procedure, it has been demonstrated with some clinical samples that it could In addition to PCR-based methods, micro/nano biomedical devices that utilize isothermal nucleic acid amplification methods have also been investigated. Due to the isothermal amplification does not need a thermal cycling, it's much easier to be engineered with micro and nano device, e.g. coupling with microfluidics technology [137, 138] . Recent researchers have developed a range of microfluidic devices with different structures for detection of bacterial and viral pathogens, which enable multiplexed detection of different targets with corresponding primer sets deposited in each channel (Figure 4a, Figure 4b) [139, 140, 141] . In general, compared to thermal cycling-based amplification methods, the isothermal amplification methods can usually provide lower cost, faster reaction speed, less specialized equipment and easy readout [79] . They can be combined with the application of various fully enclosed micro-structured devices, with less energy consumption to maintain a constant temperature [142] . These features greatly simplify isothermal amplification implementation in POCT platforms. Compared with those microfluidic chips based on PCR, these devices enhance their applicability for rapid detection with less requirements for instruments during amplification. The isothermal amplification can be triggered on a thermostatic heating plate or even within a thermos [143] , which is very promising to provide a sample-in-result-out solution for the in-filed testing of SARS-CoV-2. By using a smartphone, the fluorescence emission generated by the dyes based on the device during amplification can be monitored in real-time [144] . The image analysis could also provide quantitative results on the time at which amplification occurred ( Figure  4c ). Yang et al. reported a simple yet efficient isothermal amplification platform containing a custom-fabricated detector and a multiplexed microwell array chip to perform the RT-LAMP assay within 25 min (Figure 4d ). The platform integrated functions of sample preparation, isothermal amplification. The results could be read with naked eyes directly [145] . The system has been successfully used to detect 130 real clinical samples.

In resource-limited settings, the lack of the required infrastructure and facilities for pathogens detection will lead to infected people either not being detected or, if identified, being diagnosed at a sufficiently late stage. With developments in paper-based microfluidic devices, some paper-based platforms based on isothermal amplification methods have been proposed for their low cost [146] . An additional feature of paper-based devices, especially for detection of infectious pathogens is that they are readily disposable, which prevents the potentials of cross-infection. Xu et al. reported a microfluidic origami-paper-based device for multiplexed detection of malaria from whole blood by using LAMP (Figure 4e ) [147] . All the required steps, including nucleic acid extraction, isothermal amplification and visual detection were integrated into the device for POCT application. Tang et al. proposed another fully functioned paper-based device (Figure 4f ). The device allowed on-chip dried reagent storage and equipment-free isothermal amplification, which further promoted their potential applications in remote settings [148] . Nguyen et al. created a sliding-paper device that combines LAMP with dopamine to detect SARS-COV-2 DNA in 25 minutes with a detection limit of 10 4 ng/μl [81] .

ID NOW was launched initially in 2014 as an advanced molecular diagnostic platform for the detection of influenza A&B, streptococcus A and respiratory syncytial viruses. As to the detection of SARS-CoV-2, two primers targeting at the RdRp gene are used to trigger the amplification. Combined with fluorescence detection, it allows you to make effective clinical decisions sooner. It can enable detection of positive samples within 5 min and negative ones in 13 min (Figure 4g) [93, 149, 150] . Due to the characteristics of smaller size and faster reaction speed, it has already been distributed to numerous medical centers and non-traditional places where the testee can get detection results in several minutes. However, the sensitive and specificity of the system are highly reliable on the nicking enzyme and modified primers. The disintegration difference of the enzyme will lead to different amplification efficiency, which will affect the accuracy and repeatability of the results ultimately.

J o u r n a l P r e -p r o o f In addition to nucleic-acid tests, micro/nano technologies have also been extensively investigated for developing immunoassay-based POCT platforms. Presently, commercial products of IgM only and IgM-IgG combined LFI tests have been developed by a couple of In Vitro Diagnostic (IVD) companies [51] . These simple yet robust point-of-care LFI can simultaneously detect IgM and IgG antibodies of the test at different infection stages [151, 152, 153] . However, traditional colloidal gold-based LFI is usually limited to relatively low sensitivity and incapable of quantification measurement [154] . With the aid of nano technologies, the LFI assays enable more sensitive and rapid detection. Wang et al. reported a LFI assay based on a selenium nanoparticlemodified SARS-CoV-2 nucleoprotein to be with high sensitivity and detection speed (Figure 5a ) [155] . The assay enabled simultaneous detection of IgG and IgM in human serum with a limit of detection of 5 ng/mL and 20 ng/mL, respectively, within 10 min. To get more quantitative results, Chen et al. reported another LFI assay for detection of IgG in human serum based on a recombinant nucleocapsid phosphoprotein and lanthanide-doped polystyrene nanoparticles (LNPs) as a fluorescent reporter [156] . Once the functionalized LNPs were captured at the control or test zone, they would produce a bright fluorescence whose excitation and emission wavelengths are 365 nm and 615 nm, respectively. The proposed assay can improve from semiquantitative to accurate quantification by using official IgG standard. Based on microfluidic devices, a novel smartphone-based POCT analyzer with microchannel capillary flow assay platform was developed for quantitation analysis of malaria biomarker (Figure 5b ) [157] . The novel analyzer integrated the ultra-high sensitivity of chemiluminescent detection, the high reaction kinetics of the microfluidic spiral chambers design and the data processing capabilities of smartphone, reaching a limit of detection (LOD) of 8 ng/mL for malaria. The terminal results derived from the positive and negative controls to decrease the risk of false diagnosis. Furthermore, the quantitative platform could easily be adapted for the detection of IgM and IgG. Essentially, the test results from this category of methods cannot confirm the existence of the target virus. Instead, it provides a piece of immunological evidence for physicians to make the correct diagnosis along with other tests, as well as establish a treatment strategy.

Rapid and early identification of infectious pathogens allows for effective implementation of disease prevention and treatment measures. Based on micro/nano technologies and the principle of immunoassay, some POCT platforms are constructed directly for detection of infectious pathogens waiving nucleic acid amplifications. Integrating the detection devices into wearables can expand opportunities for long-term and noninvasive monitoring of infections [158, 159] . Xue et al. reported an intelligent wearable face mask integrated with a flexible immunosensor for highly sensitive screening of exhaled coronavirus aerosols. In addition, some other kinds of on-site detection devices, such as the electrochemical biosensors, allow detection of multiple kinds of molecules, including antigens and antibodies with high sensitivity and specificity [160, 161, 162, 163] . Yakoh et al. reported a paper-based electrochemical biosensor for label-free detection of SARS-CoV-2 antibodies without the specific requirements of antibodies [164] . With optical assistance, Mohammad et al. designed an electro-optofluidic chip that detected target SARS-CoV-2 RNAs without amplification, the detection limits up to 10 4 -10 9 copies/ml for swab samples [165] . A custom-made fidget spinner that rapidly concentrated pathogens in 1 ml samples of undiluted urine by more than 100-fold for the on-device colorimetric detection of bacterial load and pathogen identification was designed and fabricated ( Figure 5c ) [166] . The device enabled on-site detection of infection with naked eyes within 50 min in urine samples from 39 patients suspected of having a urinary tract infection. Although the device is aimed to detect urinary tract infection (UTI) in their original report, we believe it will be a good, inexpensive handheld point-of-care device for the rapid concentration and detection of SARS-CoV-2 in low-resource, undeveloped countries. The use of nanomaterials or nanostructures could efficiently increase the sensitivity to meet the detection requirements. By using graphene sheets to modify the field-effect transistor (FET), Park et al. reported an ultra-sensitive sensor for detection of SARS-CoV-2 in clinical samples [167] . The limit of detection of the graphene modified FET sensor could be up to 1 fg/mL. Yu et al. reported an immunofluorescence microdevice integrated with ZnO nanorods for highly sensitive detection of avian influenza virus (AIV) [168] . The unique properties of ZnO nanorods boost the LOD of the device to an ultra-low level, which can be approximate 22 times more sensitive than conventional ELISA (Figure 5d ).

The pandemic of COVID-19 has caused wide-scope outcomes to most low-and middle-income countries where the infrastructure and core-facilities for early detection are insufficient. This review provides a comprehensive summary of micro/nano biomedical devices, as well as two main categories of technologies for the rapid diagnosis of COVID-19 (including nucleic acid-based methods and immunoassays) and their working principles and targets of the virus. Among these is an immunochromatographic assay that is more applicable to primary screening in these areas. Immunoassay offers advantages such as direct detection of the serum/plasma and whole blood specimens without additional processing steps and expensive equipment. In comparison, nucleic acid-based methods are more accurate for diagnosis of COVID-19. A series of isothermal amplification techniques based on LAMP, RPA and NEAR, which do not rely on expensive thermalcycling instruments, have shown their advantages in low-cost and simple-operations. However, after more than 20 years' development, there are still few instruments or devices based on these isothermal amplification methos that have been widely used on the market. A lot of optimization works need to be done to avoid problems such as false-positive results. Moreover, CRISPR-based techniques enable promising sensitivity and ultralow detection limit down to a few viral RNA copies, showing an emerging methodology for diagnosis. Clinicians may make a choice of selections in terms of their local circumstances. However, it's necessary to take into account of both the advantages and disadvantages of each method may be more effective and affordable in most area.

Meanwhile, it is worth noting that the false negative rate from single testing by even gold standard assay (RT-PCR) is relatively high in the clinical diagnosis of COVID-19, according to previous statistics. Further researches are still needed under the current circumstances. Till now, clinicalrecognized high-throughput testing is unavailable with the infections continue to emerge, there is an urgent call for the development of multiplexed, high-throughput POCT platforms for on-site detection. The capability of early and rapid diagnosis will facilitate the chance of patients obtaining proper medical treatment, decrease the risk of medical staff infection, support therapeutic drug delivery systems. In addition, the instruments that can be used for screening a variety of viruses simultaneously should be further developed and prepared for the future contingencies. 

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J o u r n a l P r e -p r o o f

COVID-19: towards understanding of pathogenesis

WHO International Health Regulations Emergency Committee for the COVID-19 outbreak

COVID-19: Transmission, prevention, and potential therapeutic opportunities

A Public Health Laboratory Response to the COVID-19 Pandemic

An overview of coronaviruses including the SARS-2 coronavirus-Molecular biology, epidemiology and clinical implications

Diagnosing COVID-19: The Disease and Tools for Detection

Recent advances and perspectives of nucleic acid detection for coronavirus

Strategies shift as coronavirus pandemic looms

A review of the 2019 Novel Coronavirus (COVID-19) based on current evidence

Detection and quantification of Covid-19 antiviral drugs in biological fluids and tissues

Evaluation of performance of two SARS-CoV-2 Rapid whole-blood finger-stick IgM-IgG Combined Antibody Tests

An updated estimation of the risk of transmission of the novel coronavirus (2019-nCov)

Diagnostic Techniques for COVID-19: A Mini-review of Early Diagnostic Methods

Genome Detective Coronavirus Typing Tool for rapid identification and characterization of novel coronavirus genomes

COVID-19 Pandemic and Role of Human Saliva as a Testing Biofluid in Point-of-Care Technology

Severe acute respiratory syndrome coronavirus 2 (SARS-CoV-2) and corona virus disease-2019 (COVID-19): the epidemic and the challenges

Genomic characterisation and epidemiology of 2019 novel coronavirus: implications for virus origins and receptor binding

Molecular Targets for the Testing of COVID-19

A pneumonia outbreak associated with a new coronavirus of probable bat origin

Return of the Coronavirus: 2019-nCoV

The reproductive number of COVID-19 is higher compared to SARS coronavirus

Laboratory diagnosis of COVID-19: current issues and challenges

Laboratory testing of SARS-CoV, MERS-CoV, and SARS-CoV-2 (2019-nCoV): Current status, challenges, and countermeasures

SARS and other coronaviruses as causes of pneumonia

Detection of 2019 novel coronavirus (2019-nCoV) by real-time RT-PCR

Roomtemperature-storable PCR mixes for SARS-CoV-2 detection

Diagnostics for SARS-CoV-2 infections

A PCR microreactor machinery with passive micropump and battery-powered heater for thermo-cycled amplifications of clinical-level and multiplexed DNA targets

Rapid and sensitive detection of SARS-CoV-2 RNA using the SimplexaTM COVID-19 direct assay

Comparison of the Elecsys® Anti-SARS-CoV-2 immunoassay with the EDITM enzyme linked immunosorbent assays for the detection of SARS-CoV-2 antibodies in human plasma

Performance Characteristics of Four High-Throughput Immunoassays for Detection of IgG Antibodies against SARS-CoV-2

Comparison of commercial RT-PCR diagnostic kits for COVID-19

A Rolling Circle-Amplified G-Quadruplex/Hemin DNAzyme for Chemiluminescence Immunoassay of the SARS-CoV-2 Protein

Detection of IgM and IgG antibodies in patients with coronavirus disease 2019

A method to prevent SARS-CoV-2 IgM false positives in gold immunochromatography and enzyme-linked immunosorbent assays

Evolution of the novel coronavirus from the ongoing Wuhan outbreak and modeling of its spike protein for risk of human transmission

Point of Care Diagnostics in the Age of COVID-19

Development of a Laboratorysafe and Low-cost Detection Protocol for SARS-CoV-2 of the Coronavirus Disease 2019 (COVID-19)

Quantitative Detection and Viral Load Analysis of SARS-CoV-2 in Infected Patients

Point-of-care nucleic acid testing for infectious diseases

Novel approaches for rapid detection of COVID-19 during the pandemic: A review

All-in-One dual CRISPR-cas12a (AIOD-CRISPR) assay: a case for rapid, ultrasensitive and visual detection of novel coronavirus SARS-CoV-2 and HIV virus

Highly sensitive detection of SARS-CoV-2 RNA by multiplex rRT-PCR for molecular diagnosis of COVID-19 by clinical laboratories

Rapid pathogen-specific phenotypic antibiotic susceptibility testing using digital LAMP quantification in clinical samples

Evaluation of a COVID-19 IgM and IgG rapid test; an efficient tool for assessment of past exposure to SARS-CoV-2

Detection of serum IgM and IgG for COVID-19 diagnosis

Detection of antibodies against SARS-CoV-2 in patients with COVID-19

Profile of IgG and IgM antibodies against severe acute respiratory syndrome coronavirus 2 (SARS-CoV-2)

Serological Approaches for COVID-19: Epidemiologic Perspective on Surveillance and Control

A Peptide-based Magnetic Chemiluminescence Enzyme Immunoassay for Serological Diagnosis of Corona Virus Disease 2019 (COVID-19)

Evaluation of two automated and three rapid lateral flow immunoassays for the detection of anti-SARS-CoV-2 antibodies

Portable chest X-ray in coronavirus disease-19 (COVID-19): A pictorial review

CT chest findings in coronavirus disease-19 (COVID-19)

Transmission electron microscopy imaging of SARS-CoV-2

Profiling early humoral response to diagnose novel coronavirus disease (COVID-19)

COVID-19 infection: Origin, transmission, and characteristics of human coronaviruses

Clinical characteristics and intrauterine vertical transmission potential of COVID-19 infection in nine pregnant women: a retrospective review of medical records

The epidemiology and pathogenesis of coronavirus disease (COVID-19) outbreak

Review of the clinical characteristics of coronavirus disease 2019 (COVID-19)

Clinical, laboratory and imaging features of COVID-19: A systematic review and meta-analysis

Combination of RT-qPCR testing and clinical features for diagnosis of COVID-19 facilitates management of SARS-CoV-2 outbreak

A systematic review on the efficacy and safety of chloroquine for the treatment of COVID-19

Baricitinib as potential treatment for 2019-nCoV acute respiratory disease

Pharmacologic treatments for coronavirus disease 2019 (COVID-19): a review

Point-of-care diagnostics for infectious diseases: From methods to devices

Next-generation DNA sequencing

Identification and validation of reference genes for quantitative RT-PCR normalization in wheat

Fast SARS-CoV-2 detection by RT-qPCR in preheated nasopharyngeal swab samples

A Real-Time PCR Assay for Bat SARS-Like Coronavirus Detection and Its Application to Italian Greater Horseshoe Bat Faecal Sample Surveys

Ante mortem diagnosis of human rabies using saliva samples: Comparison of real time and conventional RT-PCR techniques

RT-qPCR Testing of SARS-CoV-2: A Primer

Digital polymerase chain reaction technology -recent advances and future perspectives

Polymerase chain reaction: basic protocol plus troubleshooting and optimization strategies

Limitations of Different PCR Protocols Used in Diagnostic Laboratories: A Short Review

A new self-containing lyophilized PCR Mix for RNA amplification

Rapid detection of SARS-CoV-2 by low volume real-time single tube reverse transcription recombinase polymerase amplification using an exo probe with an internally linked quencher (exo-IQ)

Comparison of Cepheid Xpert Xpress and Abbott ID Now to Roche cobas for the Rapid Detection of SARS-CoV-2

Homogeneous circle-to-circle amplification for real-time optomagnetic detection of SARS-CoV-2 RdRp coding sequence

Isothermal amplification of nucleic acids

Loop mediated isothermal amplification (LAMP) assays as a rapid diagnostic for COVID-19

Polydopamine aggregation: A novel strategy for power-free readout of loop-mediated isothermal amplification integrated into a paper device for multiplex pathogens detection

Loop-mediated isothermal amplification of DNA

Accelerated reaction by loop-mediated isothermal amplification using loop primers

Development of one-step reverse transcription loop-mediated isothermal amplification for norovirus detection in oysters

A colorimetric RT-LAMP assay and LAMP-sequencing for detecting SARS-CoV-2 RNA in clinical samples

A paper-based colorimetric molecular test for SARS-CoV-2 in saliva

Recombinase polymerase amplification for diagnostic applications

Microfluidic lab-on-a-foil for nucleic acid analysis based on isothermal recombinase polymerase amplification (RPA)

Recombinase polymerase amplification: basics, applications and recent advances

Point-of-care RNA-based diagnostic device for COVID-19

Isothermal recombinase polymerase amplification-lateral flow detection of SARS-CoV-2, the etiological agent of COVID-19

TwistAmp® Liquid: a versatile amplification method to replace PCR

Evaluation of Alere i Influenza A&B for rapid detection of influenza viruses A and B

COVID-19 Infection Diagnosis: Potential Impact of Isothermal Amplification Technology to Reduce Community Transmission of SARS-CoV-2

Rolling circle amplification: a versatile tool for chemical biology, materials science and medicine

Research progress on rolling circle amplification (RCA)-based biomedical sensing

Detection of nucleic acids with a novel stem-loop primer rolling circle amplification technique

Target-triggered three-way junction structure and polymerase/nicking enzyme synergetic isothermal quadratic DNA machine for highly specific, one-step, and rapid microRNA detection at attomolar level

CRISPR/Cas systems towards next-generation biosensing

An ultrasensitive and specific point-of-care CRISPR/Cas12 based lateral flow biosensor for the rapid detection of nucleic acids

Next-generation pathogen diagnosis with CRISPR/Cas-based detection methods

CRISPR-Cas12-based detection of SARS-CoV-2

Rapid and sensitive detection of COVID-19 using CRISPR/Cas12a-based detection with naked eye readout, CRISPR/Cas12a-NER

RNA targeting with CRISPR-Cas13

The molecular architecture for RNAguided RNA cleavage by Cas13a

Point-of-care testing for COVID-19 using SHERLOCK diagnostics

Integrated sample inactivation, amplification, and Cas13-based detection of SARS-CoV-2

Recent progress on rapid SARS-CoV-2/COVID-19 detection by CRISPR-Cas13-based platforms

Understanding antibody testing for covid-19

Diagnostic value and dynamic variance of serum antibody in coronavirus disease 2019

Clinical significance of IgM and IgG test for diagnosis of highly suspected COVID-19 infection

Development and clinical application of a rapid IgM-IgG combined antibody test for SARS-CoV-2 infection diagnosis

Quantification of antibody avidities and accurate detection of SARS-CoV-2 antibodies in serum and saliva on plasmonic substrates

Application of nano-ELISA in food analysis: recent advances and challenges

Analytical performances of a chemiluminescence immunoassay for SARS-CoV-2 IgM/IgG and antibody kinetics

An automated chemiluminescent immunoassay (CLIA) detects SARS-CoV-2 Neutralizing antibody levels in COVID-19 patients and vaccinees

Automatic label-free immunoassay with high sensitivity for rapid detection of SARS-CoV-2 nucleocapsid protein based on chemiluminescent magnetic beads

Dynamic profile for the detection of anti-SARS-CoV-2 antibodies using four immunochromatographic assays

Lateral flow assays

SERS-based lateral flow immunoassay for sensitive and simultaneous detection of anti-SARS-CoV-2 IgM and IgG antibodies by using gap-enhanced Raman nanotags

Development of a molecular-beacon-based multi-allelic real-time RT-PCR assay for the detection of human coronavirus causing severe acute respiratory syndrome (SARS-CoV): a general methodology for detecting rapidly mutating viruses

Preparation of Armored RNA as a Control for Multiplex Real-Time Reverse Transcription-PCR Detection of Influenza Virus and Severe Acute Respiratory Syndrome Coronavirus

Unique epidemiological and clinical features of the emerging 2019 novel coronavirus pneumonia (COVID-19) implicate special control measures

Early and consecutive RT-PCR tests with both oropharyngeal swabs and sputum could improve testing yield for patients with COVID-19: An Observation Cohort Study in China

Reducing false negatives in COVID-19 testing by using microneedle-based oropharyngeal swabs

DNA enrichment and tagmentation method for species-level identification and strain-level differentiation using ON-rep-seq

A review of the current isothermal amplification techniques: applications, advantages and disadvantages

Rapid PCR powered by microfluidics: A quick review under the background of COVID-19 pandemic

Sequence-specific and multiplex detection of COVID-19 virus (SARS-CoV-2) using proofreading enzyme-mediated probe cleavage coupled with isothermal amplification

Point-of-care testing detection methods for COVID-19

An integrated microfluidic system for rapid detection and multiple subtyping of influenza A viruses by using glycan-coated magnetic beads and RT-PCR

Evaluation of a high-speed but low-throughput RT-qPCR system for SARS-CoV-2 detection

Rapid molecular diagnostics of COVID-19 by RT-LAMP in a centrifugal polystyrene-toner based microdevice with end-point visual detection

Ultraviolet-induced in situ gold nanoparticles for point-of-care testing of infectious diseases in loop-mediated isothermal amplification

A centrifugal direct recombinase polymerase amplification (direct-RPA) microdevice for multiplex and real-time identification of food poisoning bacteria

Sample-to-answer on molecular diagnosis of bacterial infection using integrated lab-on-a-disc

A lab-on-chip device for the sample-in-result-out detection of viable Salmonella using loop-mediated isothermal amplification and real-time turbidity monitoring

A "sample-in-multiplex-digital-answer-out" chip for fast detection of pathogens

Monitoring Genetic Population Biomarkers for Wastewater-Based Epidemiology

Smartphone-based multiplex 30-minute nucleic acid test of live virus from nasal swab extract

Low-Cost and Scalable Platform with Multiplexed Microwell Array Biochip for Rapid Diagnosis of COVID-19

Rapid veterinary diagnosis of bovine reproductive infectious diseases from semen using paper-origami DNA microfluidics

Paper-Origami-Based Multiplexed Malaria Diagnostics from Whole Blood

A fully disposable and integrated paper-based device for nucleic acid extraction, amplification and detection

Multicenter clinical evaluation of the Alere i respiratory syncytial virus isothermal nucleic acid amplification assay

Sensitive onsite detection of SARS-CoV-2 by ID NOW COVID-19

Cross-validation of ELISA and a portable surface plasmon resonance instrument for IgG antibody serology with SARS-CoV-2 positive individuals

Ultrasensitive, high-throughput, and rapid simultaneous detection of SARS-CoV-2 antigens and IgG/IgM antibodies within 10 min through an immunoassay biochip

Rapid, label-free, and sensitive point-of-care testing of anti-SARS-CoV-2 IgM/IgG using all-fiber Fresnel reflection microfluidic biosensor

Diagnostic performance of immunochromatography assay for rapid detection of IgM and IgG in coronavirus disease 2019

A point-of-care selenium nanoparticlebased test for the combined detection of anti-SARS-CoV-2 IgM and IgG in human serum and blood

Rapid and Sensitive Detection of anti-SARS-CoV-2 IgG, Using Lanthanide-Doped Nanoparticles-Based Lateral Flow Immunoassay

A new microchannel capillary flow assay (MCFA) platform with lyophilized chemiluminescence reagents for a smartphone-based POCT detecting malaria

An intelligent face mask integrated with high density conductive nanowire array for directly exhaled coronavirus aerosols screening

Wearable materials with embedded synthetic biology sensors for biomolecule detection

Electrochemical Biosensor with Enhanced Antifouling Capability for COVID-19 Nucleic Acid Detection in Complex Biological Media

Rapid single-molecule detection of COVID-19 and MERS antigens via nanobody-functionalized organic electrochemical transistors

Ultrafast, sensitive, and portable detection of COVID-19 IgG using flexible organic electrochemical transistors

Rapid, Ultrasensitive, and Quantitative Detection of SARS-CoV-2 Using Antisense Oligonucleotides Directed Electrochemical Biosensor Chip

Paper-based electrochemical biosensor for diagnosing COVID-19: Detection of SARS-CoV-2 antibodies and antigen

Optical trapping assisted label-free and amplification-free detection of SARS-CoV-2 RNAs with an optofluidic nanopore sensor

A fidget spinner for the point-of-care diagnosis of urinary tract infection

Rapid Detection of COVID-19 Causative Virus (SARS-CoV-2) in Human Nasopharyngeal Swab Specimens Using Field-Effect Transistor-Based Biosensor

A nanostructured microfluidic immunoassay platform for highly sensitive infectious pathogen detection

Signature: Yang Wang: Writing -original draft; Writing -review & editing; Investigation; Methodology; Huiren Xu: Writing -original draft; Zaizai Dong: Writing -original draft; Writing -review & editing; Zhiying Wang: Investigation; Zhugen Yang: Funding acquisition

Writing -review & editing; Lingqian Chang: Funding acquisition; Investigation; Methodology

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