key: cord-1015283-xg8i6gvu authors: Zhang, Jian; Lv, Hailong; Li, Linxian; Chen, Minjie; Gu, Dayong; Wang, Jin; Xu, Yong title: Recent Improvements in CRISPR-Based Amplification-Free Pathogen Detection date: 2021-09-30 journal: Front Microbiol DOI: 10.3389/fmicb.2021.751408 sha: 9c8026abf6488ac14d3ac3fa832dbfac20c935d3 doc_id: 1015283 cord_uid: xg8i6gvu Molecular diagnostic (MDx) methods directly detect target nucleic acid sequences and are therefore an important approach for precise diagnosis of pathogen infection. In comparison with traditional MDx techniques such as PCR, the recently developed CRISPR-based diagnostic technologies, which employ the single-stranded nucleic acid trans-cleavage activities of either Cas12 or Cas13, show merits in both sensitivity and specificity and therefore have great potential in both pathogen detection and beyond. With more and more efforts in improving both the CRISPR trans-cleavage efficiencies and the signal detection sensitivities, CRISPR-based direct detection of target nucleic acids without preamplification can be a possibility. Here in this mini-review, we summarize recent research progresses of amplification-free CRISPR-Dx systems and explore the potential changes they will lead to pathogen diagnosis. In addition, discussion of the challenges for both detection sensitivity and cost of the amplification-free systems will also be covered. Infectious diseases caused deaths account for about a quarter of the global human death, and the rate is higher in the mid-term-income countries (Lozano et al., 2012) . Since the beginning of the century, several epidemics have caused great loss of both life and property all over the world (Fournier et al., 2013) . Particularly, the outbreak of COVID-19, which is caused by the pathogenic agent SARS-CoV-2 virus, has caused more than 196 million infection and 4 million death (World Health Organization, 2021) and is right now challenging the public health safety, economic development, and social stability. To effectively stop the transmission and spread of the COVID-19 epidemic, dozens of rapid diagnostic methods, including both the nucleic-acidbased molecular diagnostic (MDx) and immunological methods, have been successfully developed soon after the report of the SARS-CoV-2 genomic sequence. Because of the high accuracy and the ability to distinguish the virus mutants, MDx methods are playing a more and more important role in COVID-19 diagnosis and screening. Frontiers in Microbiology | www.frontiersin.org 2 September 2021 | Volume 12 | Article 751408 Commonly used MDx technologies may include the quantitative polymerase chain reaction technology (qPCR), the isothermal nucleic acid amplification technologies, and the next-generation gene sequencing technology (NGS) . Although qPCR is the goldstandard technology for most nucleic-acid-based diagnosis and is well known for its sensitivity, accuracy, and robustness, it requires both expensive instruments and sophisticated technicians to handle the samples and accomplish the reactions (Mahony et al., 2009) . Isothermal methods such as LAMP (Loop-mediated isothermal AMPlification) and RPA (Recombinase Polymerase Amplification) have minimal requirements for the equipment and amplify target nucleic acids exponentially at constant temperature; however, these methods usually generate nonspecific amplification products and therefore lead to lower diagnostic specificity (Wang et al., 2015; Phillips et al., 2018) . The NGS is good at generating massive data but is limited by its cost, inconvenience, and low speed, which may prevent it from wide application in rapid pathogen diagnosis (Yozwiak et al., 2012; Wilson et al., 2014; Langelier et al., 2018) . By contrast, the recently developed CRISPR (Clustered Regularly Interspaced Short Palindromic Repeat) diagnostic technologies (CRISPR-Dx) have shown merits of high sensitivity, specificity, rapidness, convenience, and low cost and have been well recognized as the next-generation diagnostic technology (Chertow, 2018) . Moreover, a CRISPR-Dx product was issued with an Emergency Use Authorization (EUA) in COVID-19 diagnosis by the Food and Drug Administration (FDA) in the United States last year, which further demonstrates the great potential of CRISPR technologies in pathogen diagnosis. CRISPR-Dx mainly employs the trans-cleavage activities of certain Cas proteins against single-stranded nucleic acids, which include both DNA-targeting type V Cas12 (Chen et al., 2018; Li et al., 2018a) and RNA-targeting type VI Cas13 (Gootenberg et al., 2017) . Upon the recognition and binding of target nucleic acids, Cas12 and the guide RNA form a ternary complex with the target nucleic acids, which is then triggered to unleash the trans-cleavage activities and nonspecifically cleaves any singlestranded DNA (ssDNA) sequences in the system. With the employment of this activity, several CRISPR-Dx methods such as HOLMES (Li et al., 2018b) and HOLMESv2 have been created for target nucleic acids detection. Specifically, at the presence of target nucleic acids, Cas12 is activated to trans-cleave the fluorophore quencher (FQ)-labeled ssDNA reporter and illuminate detectable fluorescent signals. Similarly, Cas13 recognizes target RNA and trans-cleaves FQ-labeled RNA reporter, on the basis of which methods such as SHERLOCK have been successfully developed (Gootenberg et al., 2017) . To achieve attomolar or higher sensitivity, the CRISPR-Dx step needs to be combined with the target nucleic acid amplification step performed by either PCR or isothermal technologies. The two steps are normally separated but can also be integrated into one tube after careful optimization of the isothermal amplification and trans-cleavage conditions Wang et al., 2019; Joung et al., 2020) . However, the amplification procedure not only is a waste of time but also has the risk of aerosol contamination. To overcome this limitation, several research groups have made great efforts in developing amplification-free CRISPR-Dx systems and exploring their application in pathogen diagnosis and beyond ( Table 1) . In this mini-review, we not only summarize the recent progresses but also discuss about the challenges facing them. Prior to the Cas-mediated trans-cleavage step, the preamplification step increases not only the concentration but also the proportion of the target nucleic acids in the test samples. As the CRISPR technology is of high specificity and distinguishes one base mismatch, the preamplification mainly improves the detection sensitivity of CRISPR-Dx. Therefore, the key factor of developing amplification-free CRISPR-Dx systems lies in the improvement of the detection sensitivity with minimal target nucleic acids. In principle, solutions can be divided into three small categories, including reducing the reaction volume to increase the target concentration, improving the detection sensitivity by electrochemical biosensors, and magnifying the output signals by Cas-mediated cascade amplification or biochemical circuits (Figure 1 ). It has been known that the target concentration is a prerequisite to trigger the trans-cleavage activities, e.g., 100 pM DNA for Cas12 (Li et al., 2018b) and ~50 pM RNA for Cas13 (Gootenberg et al., 2017) . To develop amplification-free systems, one may simply reduce the reaction volume to increase the target concentration and improve the LOD (limit of detection) without preamplification. For example, a confinement effect is recently introduced to inspire the Cas13a diagnostic system for singlemolecule target RNA detection. The target RNA-triggered Cas13a complex is confined in cell-like-sized reactors to increase the local target concentration via droplet microfluidics. In comparison with the bulk reaction conditions in microliter volume, the created picoliter-sized Cas13a system demonstrates more than 10,000 times enhancement in detection sensitivity and enables absolute target RNA quantitation . Using the same strategy, the Cas12a-based amplification-free system is then developed to perform an ultralocalized droplet assay, obtaining single-molecule sensitivity for quantitative target DNA detection . In a similar way, another group develops a platform called CRISPR-based amplification-free digital RNA detection (SATORI) through combining Cas13 detection and microchamber-array technologies, enabling the detection of target RNA at concentrations as low as 5 fM in 5 min (Shinoda et al., 2021) . The sensitivity of CRIPSR-Dx methods depends on the Cas trans-cleavage activities, which are triggered by target nucleic acid to nonspecifically trans-cleave single-stranded nucleic acid reporters (Gootenberg et al., 2017; Li et al., 2018a) . Usually, reporters are dual labeled with fluorescence and quencher units, and the trans-cleavage reactions are monitored by a fluorescence reader. Alternatively, reporters can be labeled with biotin and Frontiers in Microbiology | www.frontiersin.org carboxyfluorescein, and the cleavage is detected by a lateral flow assay (LFA; Kellner et al., 2019) . Although the above labeling and detection methods are robust and convenient, the output signals are relatively weak, which may result in limited detection sensitivity. Considering the fact that most target nucleic acids are of a low concentration and the amplification-free CRISPR-Dx systems may generate weak transcleavage activities, a much more sensitive signal detection approach is required to detect the weak output signal. Researchers compare various types of biosensing platforms and intelligently combine the CRISPR trans-cleavage activities with the electrochemical biosensors, which are highly sensitive, compact, and cheap. Take the E-CRIPSR (CRISPR Cas12a-based electrochemical biosensor), for example, the ssDNA reporter is linked with methylene blue (MB) on a three-electrode-based sensor to monitor the Cas12a trans-cleavage activities (Dai et al., 2019) . E-CRISPR successfully detects target nucleic acids such as human papillomavirus 16 (HPV-16) and parvovirus B19 (PB-19) at the picomolar level without preamplification of target DNA. The ssDNA reporter can also be optimized to the interfacial hairpin DNA that has an incompact morphological structure to facilitate highly efficient Cas12a cleavage, leading to higher detection sensitivity . Using the same electrochemical strategy, Cas12a has been used in direct detection of many other pathogens such as the dengue virus with the LOD of 100 fM (Lee et al., 2021) . Besides, the solid-state nanopore sensor has shown great potential in detecting single molecules and is an alternative approach to magnify the signal output. With the combination of Cas12a-mediated trans-cleavage and the glass nanopore sensor toward an electronic sensing platform, target nucleic acids such as the HIV-1 DNA can be specifically and sensitively detected without the requirement of preamplification (Nouri et al., 2020) . Cas13a detection can also be combined with electrochemical biosensor through linking the reporter RNA with the glucose oxidase, which produces H 2 O 2 that can be amperometrically detected, facilitating sensitive diagnosis of miRNAs (Bruch et al., 2019) . Through combining the electrochemical biosensor and a dual signal amplification strategy consisting of both Cas13a and a catalytic hairpin DNA circuit, the LOD for target RNAs can be further improved to 50 aM within a readout time of 6 min and an overall process time of 36 min, without the need of target RNA amplification (Sheng et al., 2021) . To detect multiplexed targets, the electrochemical biosensor can be integrated with microfluidic technology by dividing the channel into subsections, allowing for the amplification-free and simultaneous quantification of multiple target RNAs (Bruch et al., 2021) . The above CRISPR-Dx systems rely on both the target-specific binding and nonspecific trans-cleavage of single-stranded nucleic acids. Besides, there exist another group of CRISPR-Dx systems that merely employ the Cas-mediated specific binding and ciscleavage and detect the immobilized reporter through electrochemical principle. In the CRISPR-based enhanced electrochemical DNA system (E-DNA), the ssDNA signaling probe first anneals with target ssDNA, forming the double-stranded DNA for subsequent Cas9-or Cas12a-mediated cis-cleavage, which removes the electrochemical tag from the probe and induces apparent signal change to facilitate diagnosis (Xu et al., 2020) . Alternatively, through combining catalytically dead Cas9 (dCas9)based specific binding of target nucleic acids and the graphenebased field-effect transistor, the obtained platform, namely CRISPR-Chip, can rapidly (within 15 min) and sensitively (1.7fM) detect At the presence of target ssDNA or dsDNA, the Cas12/ crRNA binary complex specifically binds target DNA and forms a ternary complex, which then both cis-cleaves the target DNA and trans-cleaves non-target ssDNAs in the reaction system. Similarly, Cas13 recognizes target ssRNA and then forms a ternary complex, which cis-cleaves target ssRNA and trans-cleaves non-target ssRNAs into small pieces. (B) Categories of amplification-free CRISPR-Dx systems. Samples are first treated to release the target DNA or RNA, which is then detected by CRISPR-based diagnostic methods in an amplification-free way. Briefly, the amplification-free CRISPR-Dx methods can be divided into three categories, including (1) increasing the target concentration via reducing the reaction volumes, (2) improving the detection sensitivity via electrochemical biosensor, and (3) magnifying the output signals via either CRISPR cascade amplification (3a) or Cas-mediated positive feedback (3b). Frontiers in Microbiology | www.frontiersin.org 5 September 2021 | Volume 12 | Article 751408 unamplified genomic DNA (Hajian et al., 2019) , and its improved version termed CRISPR-SNP-Chip demonstrates the ability in detecting single-nucleotide mutations (Balderston et al., 2021) . Learning from the principle of the fluorescence in situ hybridization (FISH) technology, target nucleic acids were first specifically bound by the complex of dCas9 and sgRNA and then viewed by SYBR Green I (SG I) dyeing, and the obtained dCas9/sgRNA-SG I-based DNA-FISH system has shown advantages in simplicity, precision, and rapidness in detecting pathogens such as the methicillinresistant Staphylococcus aureus (Guk et al., 2017) . Without target amplification, the weak trans-cleavage signal can be magnified by Cas-based cascade amplification to facilitate amplification-free diagnosis. Following this principle, Cas13a and Cas12f (previously known as Cas14a) are combined together to develop the casCRISPR system, where the Cas13a transcleaved products serve as the activators for Cas12f and further trigger the Cas12f-mediated trans-cleavage of reporters, illuminating magnified output signals. Noticeably, the casCRISPR system achieves a detection limit of 1.33 fM, i.e., 1,000 times more sensitive than that of Cas13a alone (Sha et al., 2021) . Similarly, the Csm6 RNA endonuclease can also be employed for signal amplification, which was previously employed in the SHERLOCKv2 system to improve the CRISPR detection sensitivity (Gootenberg et al., 2018) and was recently further optimized in the FIND-IT system by using a chemically stabilized activator, facilitating direct diagnosis of target SARS-CoV-2 RNA by Cas13 without preamplification . Specifically, at the presence of target RNA, Cas13a is triggered to trans-cleave a preactivator sequence, generating mature activators for Csm6, which then cleaves the RNA reporter to illuminate fluorescent signals. Moreover, the FIND-IT system can be used for rapid diagnosis of clinical samples, i.e., with a diagnostic sensitivity of RT-qPCR-derived cycle threshold (C t ) values up to 33 and within 40 min of detection time. The Cas-mediated positive feedback circuit is another excellent idea to amplify the trans-cleavage signals. In the CRISPR-Caspowered catalytic nucleic acid circuit, namely CONAN, there exist two crRNA sequences, pairing to the target nucleic acids and an assistant probe, respectively. The assistant crRNA is blocked by ssDNA FQ-reporter and can be released once the ssDNA blocker is trans-cleaved by Cas12a at the presence of target nucleic acids, further guiding Cas12a to target the assistant probe and trans-cleave more FQ-reporters in a positive feedback circuit (Shi et al., 2021) . Noticeably, the amplification-free CONAN requires only Cas12a for the one-step and real-time detection of genomic DNA with attomolar sensitivity and is so far the most minimalistic of Cas-based signal amplification system. Under the guidance of CRISPR RNAs, Cas proteins as well as their engineered variants show high specificity in target nucleic acids recognition and binding, which property favors the development of diagnostic methods such as the CRISPR-Chip (Hajian et al., 2019; Balderston et al., 2021) and the paired dCas9 reporter system (Zhang et al., 2017) . The subsequent characterization of the trans-cleavage activities of Cas12 and Cas13 further improves the detection sensitivity, which has undoubtedly accelerated the development of CRISPR-Dx systems for rapid diagnosis of both pathogens and other target nucleic acids. Besides, the CRISPR-Dx methods can also be employed as a signal amplifier and combined with approaches such as aptamers and allosteric transcription factors (aTFs) for detection of non-nucleic acid (NNA) targets, which may include metabolic small molecules and metal ion (Liang et al., 2019; Xiong et al., 2020) . Usually, the presence of NNA leads to the specific binding of aptamers or aTFs, which then produces specific nucleic acid sequences to trigger the trans-cleavage activities of Cas12 or Cas13 to cleaving reporters, illuminating detection signals. Similarly, using an antibody-DNA conjugate, the Cas12abased Dx was integrated with the enzyme-linked immunosorbent assay (ELISA) to ultra-sensitively detect the pathogen Cryptosporidium parvum in a recent study (Li et al., 2021) . Although the above CRISPR-based approaches in NNA detection have shown advantages in both detection sensitivities and are amplification-free, we here mainly focused on the most recent progresses of trans-cleavage-based MDx technologies, which directly detect target nucleic acids and are of both sensitivity and specificity. At first, the CRISPR-Dx systems such as SHERLOCK (Gootenberg et al., 2017) , HOLMES (Li et al., 2018b) , and DETECTR (Chen et al., 2018) consist of two physically separated procedures, i.e., amplification of the target nucleic acids and detection of the amplicons by Cas-mediated trans-cleavage. To reduce the possibility of aerosol contamination during transferring the amplified products, scientists subsequently developed one-tube HOLMESv2 CRISPR-Dx system , which combines isothermal LAMP amplification and Cas12b trans-cleavage and therefore avoids transferring the amplicons. Albeit one-tube CRISPR-Dx systems may integrate the advantages of both sensitivity and convenience from isothermal amplification technology and specificity from CRISPR technology, the complexity remarkably increases in the optimization of the sequences of amplification primers and guide RNAs as well as the reaction conditions. Moreover, as long as there exists the amplification step, one may still worry about the possibility of aerosol contamination, and more efforts will be required to design complex chips to prevent the contamination event. Therefore, considering both the diagnostic convenience and the cost, it is necessary to develop amplification-free methods, and CRISPR-Dx technologies are so far the most likely to achieve the goal. Up to now, variant types of amplification-free CRISPR-Dx systems have been successfully developed, and there will be more in the future. Moreover, besides the above-mentioned methods, there exist many other efforts to improve the detection sensitivity. For example, using the principle of metal-enhanced fluorescence, the output fluorescent signals are remarkably magnified by the Frontiers in Microbiology | www.frontiersin.org 6 September 2021 | Volume 12 | Article 751408 DNA-functionalized Au nanoparticle gold nanoparticles, which has been demonstrated to support amplification-free detection of target DNA with the Cas12a-mediated trans-cleavage activities . In addition, through optimizing the reaction conditions and designing more than one crRNAs for a target nucleic acid sequence, the detection sensitivity can also be enhanced (Fozouni et al., 2021; Nguyen et al., 2021) . Taken together, the present amplification-free methods may use different diagnostic principles and have varied LOD and operational convenience. Albeit some amplification-free CRISPR-Dx methods have demonstrated high detection sensitivity within an acceptable detection time (Hajian et al., 2019; Zhou et al., 2020; Balderston et al., 2021; Sheng et al., 2021; Tian et al., 2021; Yue et al., 2021) , the requirement of special chips and instruments as well as the detection cost will limit their wide application and need to be further solved. In a recent study, Cas13a-based trans-cleavage is employed to trigger the exponential amplification of reporter DNAs by both a nicking enzyme and a DNA polymerase. Through further combination of the Cas13a and the electrochemiluminescence technologies, target miRNA can be directly detected at a high sensitivity, e.g., at the LOD of fM level (Zhou et al., 2020) . In the future, one can expect that more approaches of distinct principles are integrated to develop an amplification-free CRISPR-Dx method, which is of high sensitivity, high specificity, low cost, rapidness, and good portability. Without the need of preamplification of target nucleic acids, there will be remarkable reduction of both the detection time and the requirements of the machines and other consumables. Therefore, it is worth expecting that the whole detection can be performed more conveniently with lower cost. Moreover, the application scenarios of CRISPR-Dx can be further explored, e.g., from clinical uses to in-home uses. During the COVID-19 pandemic, there has been a trend toward using home tests for diagnosis of SARS-CoV-2 and several MDx-based products using technologies such as RT-LAMP have been approved by the FDA for more sensitive diagnosis. Compared to the isothermal amplification methods, the CRISPR-Dx results are more specific and there will be no worry about potential risks of aerosol contamination if diagnosed in an amplification-free procedure. Besides, some modified immunological technologies have also shown their advantages in sensitivity. For example, with the employment of the antibody sandwich protocol for target antigen capture and an ultrabright fluorescence-labeled antibody for signal readout, the obtained method could sensitively detect SARS-CoV-2 and influenza A antigens from clinical samples (Stambaugh et al., 2021) . Moreover, some on-chip sample preparation systems could also remarkably promote the hybridization between the capture probes and target virus RNA and enhance the capture efficiency, e.g., through using metered air bubbles to stir up the magnetic beads, which will certainly improve the following detection sensitivity (Du et al., 2017) . Therefore, one can expect that different sample preparation and signal detection methods can be integrated with the amplification-free CRISPR-Dx methods to further improve the detection sensitivity in the future. Till then, the amplificationfree CRISPR-Dx technologies will find their applications not only in diagnosis of pathogens and genetic diseases but may also in agriculture and beyond. JZ and HL wrote the main manuscript. LL, MC, DG, JW, and YX revised the manuscript. YX and JW coordinated contributions and provided the final draft of the manuscript. All authors contributed to the article and approved the submitted version. GJHZ20200731095604013, and JCYJ20210317073338001). The sponsors have no involvement in the study design, collection, analysis, and interpretation of data, the writing of the manuscript, and the decision to submit the manuscript for publication. Discrimination of single-point mutations in unamplified genomic DNA via Cas9 immobilized on a graphene field-effect transistor CRISPR/Cas13a-powered electrochemical microfluidic biosensor for nucleic acid amplification-free mirna diagnostics CRISPR-powered electrochemical microfluidic multiplexed biosensor for target amplification-free miRNA diagnostics CRISPR-Cas12a target binding unleashes indiscriminate single-stranded DNase activity Next-generation diagnostics with CRISPR CRISPR-Cas12a-based nucleic acid amplification-free dna biosensor via au nanoparticleassisted metal-enhanced fluorescence and colorimetric analysis Exploring the trans-cleavage activity of CRISPR-Cas12a (cpf1) for the development of a universal electrochemical biosensor Multiplexed efficient on-chip sample preparation and sensitive amplificationfree detection of Ebola virus Modern clinical microbiology: new challenges and solutions Amplification-free detection of SARS-CoV-2 with CRISPR-Cas13a and mobile phone microscopy Multiplexed and portable nucleic acid detection platform with Cas13, Cas12a, and Csm6 Nucleic acid detection with CRISPR-Cas13a/C2c2 A facile, rapid and sensitive detection of MRSA using a CRISPRmediated DNA FISH method, antibody-like dCas9/sgRNA complex Detection of unamplified target genes via CRISPR-Cas9 immobilized on a graphene field-effect transistor Detection of SARS-CoV-2 with SHERLOCK one-pot testing SHERLOCK: nucleic acid detection with CRISPR nucleases Metagenomic sequencing detects respiratory pathogens in hematopoietic cellular transplant patients Fabrication of ultrasensitive electrochemical biosensor for dengue fever viral RNA based on CRISPR/Cpf1 reaction CRISPR-Cas12a has both cis-and trans-cleavage activities on single-stranded DNA CRISPR-Cas12a-assisted nucleic acid detection CRISPR/Cas12a-powered immunosensor suitable for ultra-sensitive whole cryptosporidium oocyst detection from water samples using a plate reader HOLMESv2: a CRISPR-Cas12b-assisted platform for nucleic acid detection and DNA methylation quantitation A CRISPR-Cas12a-derived biosensing platform for the highly sensitive detection of diverse small molecules Accelerated RNA detection using tandem CRISPR nucleases Global and regional mortality from 235 causes of death for 20 age groups in 1990 and 2010: a systematic analysis for the Global Burden of Disease Study Cost analysis of multiplex PCR testing for diagnosing respiratory virus infections CRISPR-ENHANCE: an enhanced nucleic acid detection platform using Cas12a Sequence-specific recognition of HIV-1 DNA with solid-state CRISPR-Cas12a-assisted nanopores (SCAN) Strand displacement probes combined with isothermal nucleic acid amplification for instrument-free detection from complex samples Cascade CRISPR/cas enables amplification-free microRNA sensing with fM-sensitivity and single-base-specificity A CRISPR/Cas13a-powered catalytic electrochemical biosensor for successive and highly sensitive RNA diagnostics A CRISPR-Cas autocatalysis-driven feedback amplification network for supersensitive DNA diagnostics Amplification-free RNA detection with CRISPR-Cas13 Optofluidic multiplex detection of single SARS-CoV-2 and influenza A antigens using a novel bright fluorescent probe assay An ultralocalized Cas13a assay enables universal and nucleic acid amplification-free singlemolecule RNA diagnostics Two methods for increased specificity and sensitivity in loop-mediated isothermal amplification Cas12aVDet: a CRISPR/Cas12a-based platform for rapid and visual nucleic acid detection Actionable diagnosis of neuroleptospirosis by next-generation sequencing Coronavirus disease (COVID-19) Functional DNA regulated CRISPR-Cas12a sensors for point-of-care diagnostics of non-nucleic-acid targets Surpassing the detection limit and accuracy of the electrochemical DNA sensor through the application of CRISPR Cas systems Virus identification in unknown tropical febrile illness cases using deep sequencing Droplet Cas12a assay enables DNA quantification from unamplified samples at the single-molecule level Paired design of dCas9 as a systematic platform for the detection of featured nucleic acid sequences in pathogenic strains CRISPR/Cas12a-mediated interfacial cleaving of hairpin DNA reporter for electrochemical nucleic acid sensing CRISPR/Cas13a powered portable electrochemiluminescence chip for ultrasensitive and specific MiRNA detection We are grateful to the First Affiliated Hospital of Shenzhen University and Shenzhen Institute of Advanced Technology for their support and assistance to our work. The authors declare that the research was conducted in the absence of any commercial or financial relationships that could be construed as a potential conflict of interest.Publisher's Note: All claims expressed in this article are solely those of the authors and do not necessarily represent those of their affiliated organizations, or those of the publisher, the editors and the reviewers. Any product that may be evaluated in this article, or claim that may be made by its manufacturer, is not guaranteed or endorsed by the publisher.Copyright © 2021 Zhang, Lv, Li, Chen, Gu, Wang and Xu. This is an open-access article distributed under the terms of the Creative Commons Attribution License (CC BY). The use, distribution or reproduction in other forums is permitted, provided the original author(s) and the copyright owner(s) are credited and that the original publication in this journal is cited, in accordance with accepted academic practice. No use, distribution or reproduction is permitted which does not comply with these terms.