Development of gold nanoparticle-based biosensors for COVID-19 diagnosis

Abstract The outbreak of the novel coronavirus disease (COVID‐19) quickly spread all over China and to more than 20 other countries. Although the virus (severe acute respiratory syndrome coronavirus [SARS‐Cov‐2]) nucleic acid real‐time polymerase chain reaction (PCR) test has become the standard method for diagnosis of SARS‐CoV‐2 infection, these real‐time PCR test kits have many limitations. In addition, high false‐negative rates were reported. There is an urgent need for an accurate and rapid test method to quickly identify a large number of infected patients and asymptomatic carriers to prevent virus transmission and assure timely treatment of patients. We have developed a rapid and simple point‐of‐care lateral flow immunoassay that can detect immunoglobulin M (IgM) and IgG antibodies simultaneously against SARS‐CoV‐2 virus in human blood within 15 minutes which can detect patients at different infection stages. With this test kit, we carried out clinical studies to validate its clinical efficacy uses. The clinical detection sensitivity and specificity of this test were measured using blood samples collected from 397 PCR confirmed COVID‐19 patients and 128 negative patients at eight different clinical sites. The overall testing sensitivity was 88.66% and specificity was 90.63%. In addition, we evaluated clinical diagnosis results obtained from different types of venous and fingerstick blood samples. The results indicated great detection consistency among samples from fingerstick blood, serum and plasma of venous blood. The IgM‐IgG combined assay has better utility and sensitivity compared with a single IgM or IgG test. It can be used for the rapid screening of SARS‐CoV‐2 carriers, symptomatic or asymptomatic, in hospitals, clinics, and test laboratories.

Rapid detection of nucleic acids is integral for clinical diagnostics and biotechnological applications. We recently developed a platform termed SHERLOCK (Specific High Sensitivity Enzymatic Reporter UnLOCKing) that combines isothermal pre-amplification with Cas13 to detect single molecules of RNA or DNA. Through characterization of CRISPR enzymology and application development, we report here four advances integrated into SHERLOCKv2: 1) 4-channel single reaction multiplexing using orthogonal CRISPR enzymes; 2) quantitative measurement of input down to 2 aM; 3) 3.5-fold increase in signal sensitivity by combining Cas13 with Csm6, an auxilary CRISPR-associated enzyme; and 4) lateral flow read-out. SHERLOCKv2 can detect Dengue or Zika virus ssRNA as well as mutations in patient liquid biopsy samples via lateral flow, highlighting its potential as a multiplexable, portable, rapid, and quantitative detection platform of nucleic acids.

To the Editor: CRISPR (clustered regularly interspaced short palindromic repeats)–based diagnostic tests 1,2 collectively provide a nascent platform for the detection of viral and bacterial pathogens. Methods such as SHERLOCK (specific high-sensitivity enzymatic reporter unlocking), which typically use a two-step process (target amplification followed by CRISPR-mediated nucleic acid detection), 1,2 have been used to detect SARS-CoV-2. 3 These approaches, however, are more complex than those used in point-of-care testing because they depend on an RNA extraction step and multiple liquid-handling steps that increase the risk of cross-contamination of samples. Here, we describe a simple test for detection of SARS-CoV-2. The sensitivity of this test is similar to that of reverse-transcription–quantitative polymerase-chain-reaction (RT-qPCR) assays. STOP (SHERLOCK testing in one pot) is a streamlined assay that combines simplified extraction of viral RNA with isothermal amplification and CRISPR-mediated detection. This test can be performed at a single temperature in less than an hour and with minimal equipment. The integration of isothermal amplification with CRISPR-mediated detection required the development of a common reaction buffer that could accommodate both steps. To amplify viral RNA, we chose reverse transcription followed by loop-mediated isothermal amplification (LAMP) 4 because LAMP reagents are widely available and use defined buffers that are amenable to Cas enzymes. LAMP operates at 55 to 70°C and requires a thermostable Cas enzyme such as Cas12b from Alicyclobacillus acidiphilus (AapCas12b). 5 We systematically evaluated multiple LAMP primer sets and AapCas12b guide RNAs (a guide RNA helps AapCas12b recognize and cut target DNA) to identify the best combination to target gene N, encoding the SARS-CoV-2 nucleocapsid protein, in a one-pot reaction mixture (see Figs. S1 through S3 in the Supplementary Appendix, available with the full text of this letter at NEJM.org). We termed this assay STOPCovid, version 1 (STOPCovid.v1). As expected, STOPCovid.v1 detection produced a signal only when the target was present, whereas LAMP alone can produce a nonspecific signal (Fig. S3E). STOPCovid.v1 is compatible with lateral-flow and fluorescence readouts and can detect an internal control with the use of a fluorescence readout (Figs. S4 through S6). To simplify RNA extraction and to boost sensitivity, we adapted a magnetic bead purification method (Fig. S9). The magnetic beads concentrated SARS-CoV-2 RNA genomes from an entire nasopharyngeal or anterior nasal swab into one STOPCovid reaction mixture. We streamlined the test by combining the lysis and magnetic bead–binding steps and eliminating the ethanol wash and elution steps to reduce the duration of sample extraction to 15 minutes with minimal hands-on time. We refer to this streamlined test as STOPCovid, version 2 (STOPCovid.v2) (Figure 1A). We compared STOPCovid.v2 with the Centers for Disease Control and Prevention (CDC) standard two-step test (i.e., RNA extraction followed by RT-qPCR) (Fig. S10C). The concentration of substrate by magnetic beads in STOPCovid.v2 allowed detection of viral RNA from the entire swab sample, yielding an input (in terms of quantity of viral RNA) that was 600 times that afforded by the CDC test. As a result, STOPCovid.v2 reliably detected a viral load that was one thirtieth that detected by the CDC RT-qPCR test (100 copies per sample, or 33 copies per milliliter, as compared with 1000 copies per milliliter). Analysis of two independent dilution series from nasopharyngeal swab samples revealed that STOPCovid.v2 had a limit of detection that was similar to an RT-qPCR cycle-threshold (Ct) value of 40.3 (Fig. S10D and S10E). In blinded testing at an external laboratory at the University of Washington, we tested 202 SARS-CoV-2–positive and 200 SARS-CoV-2–negative nasopharyngeal swab samples obtained from patients. These samples were prepared by adding 50 μl of swab specimens obtained from patients with Covid-19 to a clean swab, in accordance with the recommendation of the Food and Drug Administration for simulating whole swabs for regulatory applications (see the Methods section in the Supplementary Appendix). This testing showed that STOPCovid.v2 had a sensitivity of 93.1% and a specificity of 98.5% (Figure 1B and 1C, Fig. S11A, and Table 1). STOPCovid.v2 false negative samples had RT-qPCR Ct values greater than 37. Positive samples were detected in 15 to 45 minutes. Finally, we used fresh, dry, anterior nasal swabs (collected according to the recommendations of the CDC) to validate STOPCovid.v2, and we correctly identified 5 positive samples (Ct values, 19 to 36) and 10 negative samples (Fig. S11B through S11E). A detailed protocol for STOPCovid.v2 is provided in the Supplementary Appendix. The simplified format of STOPCovid.V2 is suited for use in low-complexity clinical laboratories.