key: cord-0901776-jlf7xamw
authors: Oh, Hyun-Kyung; Kim, Kihyeun; Park, Jinhee; Jang, Hyungjun; Kim, Min-Gon
title: Advanced trap lateral flow immunoassay sensor for the detection of cortisol in human bodily fluids
date: 2021-11-19
journal: Sci Rep
DOI: 10.1038/s41598-021-02084-7
sha: 347badf530fbd6c8ceb8203d572dfede2a6b8380
doc_id: 901776
cord_uid: jlf7xamw

Paper-based biosensors based on lateral flow immunoassay (LFI) are promising candidates for POC diagnosis because of their ease of use and rapid target detection. However, the low sensitivity of LFI limits its application, and signal amplification has been used in numerous studies to increase its sensitivity. We developed an advanced trap LFI (α-trapLFI), a simple-to-use sensor, with an additional step for signal amplification. Here, signal amplification is automatically implemented following delayed release of enhancement solution induced by water-soluble polyvinyl alcohol tape. As the polyvinyl alcohol tape is exposed to water, its polymer structure is perturbed (within 5 min), allowing ions to pass through. This new sensor was designed to have a short time delay between the flow of solutions used for the immunoassay and signal amplification. The α-trapLFI was subsequently used to detect cortisol with high sensitivity (9.1 pg∙mL(−1)) over a broad detection range (0.01–1000 ng∙mL(−1)) in bodily fluids. Furthermore, an excellent correlation was obtained by analyzing 20 human real saliva samples using this sensor and a conventional ELISA (R(2) = 0.90). The new sensor will be helpful in detecting various small molecules for simple, rapid, and portable POC diagnosis of stress disorders.

The stress hormone cortisol has emerged as a biomarker for the rapid diagnosis and treatment of post-traumatic stress disorders 1, 2 . Excessive and persistent cortisol secretion is known to cause serious side effects, such as increased blood pressure, decreased immune response, chronic fatigue, and insomnia 3 . A recent study showed that high cortisol concentrations in patients with coronavirus disease-2019 are associated with increased mortality and a decreased average survival rate 4 . Moreover, 24-h monitoring of cortisol secretion could be useful for diagnosis and treatment psychotic and nonpsychotic major depressive disorders associated with distinct patterns of HPA axis dysregulation 5 . Thus, quantification of cortisol levels is essential for evaluating and managing mental, physical, and physiological stresses. Among the various methods of monitoring cortisol secretion, point-ofcare (POC) testing is desirable because cortisol levels change depending on the surrounding environment and behavior of individuals during the day.

Biosensors based on a lateral flow immunoassay (LFI) are promising candidates for POC diagnosis, as they are easy to use by non-specialized individuals and enable rapid target detection without specialized equipment [6] [7] [8] . However, most LFI-based biosensors show low sensitivity and cannot provide quantitative results 9 . To overcome these limitations, several signal amplification methods have been evaluated for use with LFI, including the application of enzymes for additional color-developing reactions [10] [11] [12] [13] and application of nanoparticles for fluorescent signal enhancement [14] [15] [16] [17] . Although these methods can improve the detection limit of the assay, several limitations prevent operational POC diagnosis, including stability issues and the requirement for extra equipment to detect fluorescent signals.

In 2011, Wei et al. suggested using metal ions to enhance the sensitivity of LFI 18 . After performing a general immunoassay using metal nanoparticles, Wei et al. amplified the signal by inducing metal nanoparticle growth through addition of a metal ion and reducing agent. Specifically, detection antibody-gold nanoparticle (AuNP) conjugates bound to the analyte were immobilized on a detection antibody-loaded membrane and then reacted with gold ions and a reducing agent in the reaction buffer to enlarge the metal nanoparticle, leading to a superior signal amplification effect. Since then, several LFIs with gold ion signal amplification have been developed [19] [20] [21] [22] [23] [24] . www.nature.com/scientificreports/ However, these systems exhibit several disadvantages. For example, the reagents used for signal amplification must be added manually, and there is a long lag-time (≥10 min) after the immunoassay, rendering the system unsuitable for POC diagnosis (time lag-related complexity is not easily managed by nonexperts while performing an immunoassay). To make the LFI more user-friendly, various fluid flow control methods (also known as delayed-release of reagent-contained solution for enhancement methods) have been employed, including the use of wax filler 25 , dissolvable bridge 26 , sugar barrier 27 , delayed-release membrane 28 , valving system 29 , pressedphysical barrier 30,31 , pullulan film 32 , water-soluble nanofibers 33 , wax barrier 34 , and wax-printed channels 35 . Nevertheless, the complexity of these methods limits their application, reproducibility, and large-scale production. Thus, a highly sensitive LFI method based on a simple structure to delay the release of the signal-amplification solution, without long lag-time procedures, is warranted.

We previously reported the development of a trap LFI sensor (trapLFI) for sensitively and quantitatively detecting cortisol in saliva 36 . The trapLFI sensor has deletion and detection zones loaded with target-protein conjugate and an anti-mouse IgG antibody, respectively. By lowering the amount of AuNP-antibody conjugate, conjugates that do not react with the free analytes are completely "trapped" in the detection zone, whereas only the AuNP-antibody conjugate associated with the free analyte can escape from the deletion zone and react with immobilized secondary antibody on the detection zone, leading to a signal display. Although the platform showed high sensitivity and selectivity for detecting cortisol via ratio calculation of the quantified deletion and detection zones, an enhancement step with a long lag-time procedure was employed to amplify the signal. Thus, a new platform that can perform an immunoassay and a signal amplification in one-step could be highly advantageous for POC cortisol detection.

Herein, we report the development of an advanced trapLFI sensor, the "α-trapLFI" sensor. In this sensor, automatic signal amplification is achieved using water-soluble tape, and long lag-time procedures are not required for signal amplification. Polyvinyl alcohol (PVA) tape, which is commercially available, has excellent adhesive properties and is water-soluble. This tape is placed between the signal amplification pad and membrane where the immune reaction occurs. When the PVA tape is exposed to water, it dissolves and the structure collapses, allowing ions to pass through. This process takes approximately 5 min, facilitating the time delay between the immune reaction and signal amplification reaction. These properties enabled signal amplification in our sensor system. Although the sample solution and signal amplification solution were applied consecutively, the PVA tape between the conjugate pad and membrane for the immune reaction delayed the flow of signal-amplification solution through the membrane of the LFI. As a consequence, signal amplification only occurred after the immunoassay had proceeded for a set amount of time. This method can "simultaneously and automatically" induce signal amplification, which allows for target detection with high sensitivity in a user-friendly manner. The PVA tape-insulated LFI was successfully applied to detect cortisol in bodily fluids, such as saliva, serum, and urine, with high sensitivities. Our novel α-trapLFI provides a new benchmark for simple, rapid, and portable POC diagnosis of stress disorders.

Principle of α-trapLFI sensor. The proposed α-trapLFI sensor for cortisol analysis is shown schematically in Scheme 1. The sensor consists of a sample pad, conjugate pad, signal amplification pad, PVA tape, absorbent pad, and detection/deletion zones on the membrane (Scheme 1a). As the devised method involves the enlargement of AuNPs for signal amplification (Scheme S1), a signal amplification pad loaded with gold ions for signal amplification is placed on the PVA tape to induce a delayed-release effect. To investigate that the signal intensity is promoted by the enlargement of AuNPs growth, different concentration of AuNP conjugate applied strips were observed before and after introducing signal amplification solution. Before introducing the signal amplification solution, the signal can be detected from only 0.1X and 1X AuNP conjugate applied strips; however, after introducing the signal amplification solution, the signal can be detected from all strips ( Fig. S1a and Fig. S1b ).

When the sample and signal amplification solutions were consecutively injected onto the sample and the signal amplification pads, respectively, at the strip (without a long lag-time between injections), the PVA tape delayed the release of the gold ions at the signal amplification pad, whereas the target molecule in the sample solution and AuNP-antibody conjugate were promptly started to move forward and reached the detection zone. After approximately 5 min of exposure to water (amplification solution), subsequent dissolution of the PVA tape allowed the gold ions to flow from the signal amplification pad to the membrane, resulting in automatic sequential signal amplification (Movie S1). It should be noted that, in terms of sensitivity, the α-trapLFI sensor takes not only advantages of simultaneous and automatic signal amplification, but also those of trapLFI which was previously reported by our group 36 . In the trapLFI, a test line of a conventional LFI was used as a deletion zone which could trap target-free conjugates, and thus, only target-bounded conjugates could escape from deletion zone and captured at detection zone. Such a detection strategy resulted in high sensitivity due to ratiometric calculation between deletion and detection zones, and enabled quantitative and signal-on detection towards the target molecules. Therefore, unlike conventional competitive LFI that is only detectable at a high concentration of target, α-trapLFI is detectable at both low and high concentrations of target due to automatic signal amplification and the trap strategy (Scheme 1c).

Characteristics of α-trapLFI sensor. Structure of PVA tape before and after exposure to solutions. To investigate the structures of dry and wetted PVA tape, field emission scanning electron microscopy and optical microscopy were used. The surface of the PVA tape before exposure to water was polished (Fig. 1a) . In contrast, the surface of the PVA tape was pitted after exposure to water (Fig. 1b) . In addition, before exposure to water, interpenetrated fiber structure without distinct holes were observed (Fig. 1c) ; whereas a few of hole were observed www.nature.com/scientificreports/ after exposure to water (Fig. 1d) . These results confirm that the PVA tape dissolved upon exposure to water, and that its rigid structure was collapsed and perturbed leading to a porous structure.

Delayed-release effect of PVA tape. To confirm the delayed-release effect, the effect of PVA tape was compared to that of conventional membranes, including NC membranes, plasma separation (Vivid) membranes, and asymmetric (MMM) membranes. Thus, the various types of membranes were applied to the LFI sensor for comparative testing. Bare AuNP solution was immobilized on each membrane (1 µL•cm −1 ), and a gold(III) ionloaded signal amplification pads (8.2 µL•3.8 mm −2 ) were applied onto each LFI. To initiate LFI, a sample solution although conventional LFI sensors can detect the target at high concentrations, the α-trapLFI sensor can detect the target at both low and high concentrations. This is due to two reasons: i) simultaneous and automatic signal amplification and ii) the ratiometric calculation with deletion and detection zones. www.nature.com/scientificreports/ (10% DMSO/PBS (v/v)) and signal amplification solution were consecutively loaded at the sample pad and he signal amplification pad, respectively. In the case of using a bare membrane, NC membrane, Vivid membrane, and MMM membrane, the signal amplification was occurred within 1 min. In contrast, a delayed-release effect was observed when PVA tape was used, and the signal amplification was started after approximately 5 min ( Fig. 2 and Fig. S2 ). These results confirm that the PVA tape induced a superior delayed-release effect compared to the other membranes, and thus could be appropriately used as a signal amplification platform based on its delayed-release property.

The PVA tape was also compared to a general double-sided tape to further investigate the observed ion diffusion effect. For the comparison, the double-sided tape was placed between the signal amplification pad and membrane, and the same structure using PVA tape instead of the double-sided tape was prepared. The sample and amplification solutions were applied to the sample and signal amplification pads, respectively. No signal appeared over time on the strip with the general double-sided tape, whereas the signal intensity increased on the strip with the PVA tape at approximately 5-7 min after loading the sample and amplification solutions (Fig. S3a) . A comparison of the resulting signal intensities (Fig. S3b) confirmed that only the PVA tape permitted ion diffusion.

The ion-diffusion permissible property of PVA tape may be attributed to its water-solubility. To confirm this, the general double-sided and PVA tapes (size 3.8 × 8.0 mm 2 ) were exposed to water, and the weight was measured at different time points. Each tape was completely dried in an oven to reduce deviation, and the weight was measured using an ultra-microbalance. The general double-sided tape showed no change in weight after exposure to water. Whereas the weight of the PVA tape decreased with the time of exposure to water, decreasing by 19.5% after 5 min (Fig. S3c) . Thus, the ion diffusion permissible property of PVA tape was attributed to water dissolution.

Automatic signal amplification using PVA tape. To verify an automatic signal amplification using PVA tape, the signal intensities of a conventional LFI and PVA tape-applied LFI were compared. Regarding the conventional www.nature.com/scientificreports/ LFI, anti-mouse IgG antibody were immobilized on a membrane (1 µL•cm −1 ), and an AuNP-antibody conjugate (onefold) loaded pad was applied to the membrane. Regarding the PVA tape-applied LFI, a PVA tape (3.8 × 8.0 mm 2 ) and a gold(III)-ion loaded pad (8.2 µL•3.8 mm −2 ) were additionally applied to the membrane. The sample solution was loaded for conventional LFI, and the sample solution and signal amplification solution were consecutively loaded for PVA tape-applied LFI.

Comparison of the signal intensities obtained from conventional LFI and PVA tape-applied LFI is shown in Fig. 3 . In PVA tape-applied LFI, the signal was amplified approximately 5-6 min after sample and amplification solution injection, and a higher signal (compared with conventional LFI) was achieved (Fig. 3 ). As shown in Fig. 3b , the signal achieved from PVA tape-applied LFI was approximately 6.9-fold higher than that achieved from conventional LFI.

α-trapLFI sensor for detecting small molecules. In the previous report on the trapLFI sensor developed by our group 36 , we found that detection of cortisol with high sensitivity could be achieved by applying deletion and detection zones, rather than the test and control zones used in typical LFI. Moreover, because we used a small amount of AuNP-antibody conjugate, the conjugate not reacting with antigen could be effectively "trapped" at the deletion zone, minimizing the false-positive signal in the detection zone. However, the amount of conjugate could not be reduced further for the trapLFI sensor, as the signal needed to be detectable to measure its intensity. Herein, our previous trapLFI sensor was adopted as a platform to which the PVA tape-mediated delayed release method could be appended. In our modified sensor, the advanced trap-LFI (α-trapLFI), the advantages of the trapLFI sensor are combined with signal amplification by delayed release of gold ions to further increase sensitivity. As shown in Figure S4 , although weak signal was detected in a conventional LFI using the lowest amount of AuNP-antibody conjugate (Fig. S4 left) , a strong signal was detected when the α-trapLFI sensor was used due to signal amplification by delayed-release gold ions and a reducing agent (Fig. S4 right) . In the α-trapLFI platform, the delayed-release effect induced by PVA tape was essential as shown in Fig. 2 . The absence of PVA tape causes no signal because the gold ions were released before immunoreaction was occurred (Fig. S4 middle) . Notably, the PVA tape was confirmed to have a negligible effect on the immunoreaction (Fig. S5) .

Comparison of the conventional LFI sensor and α-trapLFI sensor for cortisol analysis was also conducted to evaluate sensitivity (Fig. 4) . The target-BSA conjugate and anti-mouse IgG antibody was immobilized on a www.nature.com/scientificreports/ membrane (1 µL•cm −1 ), and then a conjugate pad loaded with the AuNP-antibody conjugate (onefold for conventional LFI; 0.001-fold for α-trapLFI) was applied to the membrane. For the α-trapLFI sensor, a signal amplification pad, PVA tape, and signal amplification solution were additionally applied, and the assay was carried out as described above. The results demonstrate that the conventional LFI shows the signal changes from about 1 ng/ mL, whereas the α-trapLFI shows a different signal even at a lower concentration of cortisol. Thus, cortisol was detected with high sensitivity over a broad-detection range with the α-trapLFI sensor.

Our α-trapLFI sensor with simultaneous signal amplification accomplished by using the delayed release effect of PVA tape was successfully optimized. Next, cortisol was detected in buffer, human saliva, human serum, and human urine, to evaluate the performance of the α-trapLFI sensor. The sensitivity of the α-trapLFI sensor was tested by using cortisol standard solutions at various concentrations in DMSO, saliva, serum, and urine/buffer (10:90, v/v). The colorimetric signal intensities were determined at 15 min after consecutively adding the loading sample and signal amplification solutions, and the results were obtained by calculating the ratios of signals observed in the deletion and detection zones (ΔI (Delta I) = sum (deletion zones)/detection zone). As shown in Fig. 5 and Figure S6a , the α-trapLFI sensor was highly sensitive to cortisol in various human bodily fluids. The limit of detection (LOD) for the α-trapLFI was calculated as the sum of the blank signal plus 3 × the standard deviation of a control cortisol sample. LOD values for cortisol in DMSO, saliva, serum, and urine were 6.9, 9.1, 14.9, and 15 pg•mL −1 , respectively, and the signal intensity was linear from 0.01 to 100 ng•mL −1 for all bodily fluids with an R 2 of 0.9704, 0.9777, 0.9672, 0.9785 for buffer, saliva, serum and urine sample (Fig. S6b) . Table 1 shows a comparison of the characteristics of the α-trapLFI sensor with previously reported LFI. The α-trapLFI sensor demonstrated a better LOD with a broader detection range compared to the other sensors, and it could successfully detect cortisol in various human bodily fluids. www.nature.com/scientificreports/ Cross-reactivity of the α-trapLFI sensor was evaluated by exposure to other steroid hormones (Fig. 6a) , including cortisone, corticosterone (CORT), progesterone (P4), and 17α-hydroxyprogesterone (17-OHP4), at 10 ng•mL -1 . The results of these assays are shown in Fig. 6b and Figure S7 . The cortisol specificity of the α-trapLFI sensor was high, and no cross-reactivity with the other steroid hormones was observed. Thus, the α-trapLFI sensor can be used as a rapid and simple detection method for cortisol diagnosis.

Twenty human saliva samples were tested using the α-trapLFI sensor. The values obtained from the saliva test samples analyzed on the α-trapLFI sensor were compared with those analyzed by ELISA which is widely used as a gold standard method (Fig. 7) , revealing the following correlation: y = − 0.0661x + 0.5114 (R 2 = 0.90). The above correlation indicated reliable agreement with the ELISA results. Hence, the α-trapLFI sensor can be used as a highly reliable sensor platform for detecting cortisol in real saliva samples. Together, our results support that our α-trapLFI sensor is a simple and practical platform for cortisol detection in human bodily fluids with high sensitivity.

In this study, we developed an α-trapLFI sensor for simultaneous signal amplification without long lag-time procedures, which takes advantages of the trapLFI sensor previously reported by our group. The application of PVA tape, which exhibits delayed release effect, enable to amplify the signal without additional long lag-time steps. In addition, the performance of the α-trapLFI sensor was superior because the conjugates that did not react with the target were 'trapped' , resulting in no signal in the detection zones when there was no target.; this is an inherent advantage of a trapLFI sensor. The performance of proposed sensor was verified using human bodily fluids including saliva, serum, and urine, and the correlation of the assay with the ELISA results was R 2 = 0.90 in Table 1 . Comparison of the specificities of αlpha-trapLFI with previously developed lateral flow immunoassay (LFI). Selectivity results comparing cortisol and other steroid hormones. All images were obtained using a ChemiDoc XPS + imaging system (Bio-Rad), and the band intensities were measured using Image Lab software (version 6.1, https:// www. bio-rad. com/ en-uk/ produ ct/ image-lab-softw are? source_ wt= image labso ftware_ surl& ID= KRE6P 5E8Z). Error bars indicate the standard deviation from three independent experiments. www.nature.com/scientificreports/ the real saliva samples. Particularly, the PVA tape used for simultaneous signal amplification is inexpensive and easy to procure and apply to signal amplification sensors; it also has a simple structure. Therefore, it can be easily applied to all LFI platforms to detect not only small molecules, but also various other targets. Characterization of PVA tape. The structure of PVA tape was characterized by field emission scanning electron microscopy and light microscopy. The PVA tape characteristics were also compared to a general doublesided tape to determine its delayed-release effect. AuNP colloid (15 nm in diameter, 1 × AuNP, λ max O.D. = 1.0) was immobilized on an NC membrane (1 μL·cm -1 ), and then gold(III) chloride trihydrate (0.1 M) was applied on the signal amplification pad. The general double-sided and PVA tapes were attached beneath the signal amplification pad. The sample solution, 10% (v/v) DMSO/PBS, and the signal amplification solution, 10 mM hydroxylamine in 10 mM citrate (pH 3.8), were applied onto the sample and signal amplification pads, respectively. The weight of the PVA tape was measured at five time points after loading the buffer. The PVA and general double-sided tapes (size, 3.8 × 8.0 mm 2 ) were placed in an e-tube containing citrate buffer (10 mM, pH 3.8) and vigorously vortexed. After 15 min, the tapes were dried completely, and their weights were measured using an ultra-microbalance. Effective delayed release from the PVA tape was confirmed as described above with different membranes. To determine whether the PVA tape impacts the immunoassay, anti-mouse IgG antibodies (1 mg·mL -1 ) were immobilized on an NC membrane (1 μL·cm -1 ), and then AuNP-antibody conjugate (three-fold) was applied Figure 7 . Human salivary cortisol level measured using conventional ELISA and α-trapLFI sensor. All images were obtained using a ChemiDoc XPS + imaging system (Bio-Rad), and the band intensities were measured using Image Lab software (version 6.1, https:// www. bio-rad. com/ en-uk/ produ ct/ image-lab-softw are? source_ wt= image labso ftware_ surl& ID= KRE6P 5E8Z). www.nature.com/scientificreports/ on a conjugate pad. The PVA tape was attached beneath the signal amplification pad, and the sample and signal amplification solutions were applied to the sample and signal amplification pads, respectively.

Preparation of AuNP conjugate. The anti-cortisol antibody (5 μL, 2 mg·mL -1 ) was added to a mixture of 1 mL of AuNP colloid (15 nm in diameter, 1 × AuNP, λ max O.D. = 1.0) and 100 μL of 0.1 M borate buffer (pH 8.5).

After incubation for 30 min at 21 °C, 10 µL of protein saver (100 mg·mL -1 in PBS) was added to the mixture to block non-specific binding sites on the AuNP surface. After incubation for 1 h at 21 °C, the mixture was centrifuged at 15 602 × g for 15 min at 10 °C. The supernatant was discarded and the AuNP conjugate was resuspended in 1 mL of 10 mM borate buffer (pH 8.5), and the AuNP conjugate was concentrated by tenfold and stored in storage buffer composed of 5% (w/v) D-( +)-trehalose, 0.5% (w/v) Protein saver, 0.2% (v/v) Tween 20, and 1% (v/v) Triton™ X-100 in PBS, at 4 °C until use.

Preparation of α-trapLFI sensor using PVA tape. To prepare an α-trapLFI sensor, 250 μg·mL -1 cortisol-BSA and 1 mg·mL -1 anti-mouse IgG antibody were immobilized on an NC membrane (1 μL·cm -1 ) to create two deletion zones and one detection zone, respectively; the distance between each zone was approximately 2.5 mm. An absorbent pad was attached on top of the membrane with a 2-mm overlap. The AuNP conjugate was diluted by 1000-fold with a solution containing 1% (w/v) PVP 10 K and 0.5% (w/v) S10G in PBS, and 3.61 μL of diluted AuNP conjugate was applied to the conjugate pad. Next, 8.2 μL of solution containing 0.1 M gold(III) chloride trihydrate in 10 mM phosphate buffer (pH 7.4) was applied to the signal amplification pad. The AuNP conjugate-loaded conjugate pad was attached to the bottom of the prepared strip, and a sample pad was placed underneath it to load the sample. The PVA tape was attached to the membrane at 2-mm above the conjugate pad, and a gold(III) chloride trihydrate-loaded signal amplification pad was placed in the middle of the PVA tape. The assembled membrane was cut into 3.8-mm wide strips and stored in a humidity-controlled chamber (21 °C; 23% relative humidity) until use. Before use, the strip was placed in a plastic case provided by Infopia Co., Ltd. (Anyang, Gyeonggi, Korea).

Cortisol analysis in buffer, saliva, serum, and urine samples. Cortisol solutions at various concentrations in DMSO, human saliva, serum, and urine were diluted tenfold in 1 × PBS buffer (10% concentration). The signal amplification solutions were prepared at 10 mM in citrate buffer (pH 3.8). Subsequently, 100 μL of the prepared sample solution (10% (v/v) DMSO/PBS) and 20 μL of the signal amplification solution (10 mM hydroxylamine in 10 mM citrate (pH 3.8)) were applied to the sample and signal amplification pads of the strip, respectively. The strip was then incubated at 21 °C for 20 min. In addition, several other steroid hormones were also analyzed with same methods described above. All images were obtained using a ChemiDoc XPS + imaging system (Bio-Rad, Hercules, CA, USA), and the band intensities were measured using Image Lab software (version 6.1, https:// www. bio-rad. com/ en-uk/ produ ct/ image-lab-softw are? source_ wt= image labso ftware_ surl& ID= KRE6P 5E8Z). After measuring the intensities of each strip, the value of ΔI (delta I) is introduced to increase sensitivity and quantitative results. The limit of detection was calculated with the mean value and the standard deviation (mean + 3SD).

Collection of saliva samples. Human saliva samples were obtained from 20 volunteers from the Gwangju Institute of Science and Technology (GIST) in Gwangju, Korea. We collected samples of saliva from healthy individuals between 08:00 and 09:00 using a saliva collecting kit. The participants were asked to refrain from eating, drinking, and performing oral hygiene procedures until the morning of saliva collection. All participants provided informed consent to participate in the study. The study was approved by GIST (Approval number: 20190510-BR-45-08-02). The collected saliva samples were centrifuged at 1274×g for 5 min to remove cell debris and other proteins, and the collected saliva samples were immediately used for testing. All experiments were performed in accordance with relevant guidelines and regulations.

Analysis of cortisol in human saliva samples. The results obtained using the sensor platform were compared to those obtained with an enzyme-linked immunosorbent assay (ELISA). Briefly, ELISA was performed in 96-well microplates. The anti-cortisol antibody (100 μL, 4 μg·mL -1 ) was added to each well, and the plates were incubated at 4 °C overnight. After removing unbound antibodies by washing the wells with PBS-Tween (137 mM NaCl, 0.05% (v/v) Tween 20, pH 7.4), the wells were blocked with 200 μL of BSA solution (0.5 mg·mL -1 in PBS) at 21 °C for 2 h. Next, individual wells were incubated with 100 μL of the diluted saliva samples and cortisol-HRP conjugate (1 μg·mL -1 ) mixture at 21 °C for 5 h. After removing all unbound proteins, the samples were incubated with TMB substrate solution (50 μL) in the dark at 21 °C for 10 min. Finally, sulfuric acid (50 μL, 2 N) was added to immediately stop the enzyme reaction. The absorbance of the solution was determined at 450 nm using a spectrometry system (Cytation 5; BioTek Instruments, Winooski, VT, USA).

A microcentrifuge (smart R17 plus; Hanil Scientific Inc., Gimpo, Korea) was used to separate the AuNP conjugate, and a multi-purpose centrifuge (1580R; LABOGENE Co., Ltd., Lillerød, Denmark) was used to collect saliva samples. A drying oven (KO-100; LK Lab Co., Namyangju, Korea) was used to dry the membranes and all pads following antibody and sample loading. A dispenser (DCI100; Zeta Co., Gunpo, Korea) was used to immobilize samples on a membrane, and a cutting device (TBC-50Ts; Taewoo Co., Namyangju, Korea) was used to cut the membranes. A field emission scanning electron microscope (Hitachi S-4700, Tokyo, Japan) and a light microscope (Olympus BX43, Tokyo, Japan) were used to characterize the structure of PVA tape. An XPR ultra-microbalance (XPR6UD5; Mettler Toledo, Masstron, OH, USA) was used to weigh tapes. www.nature.com/scientificreports/ All signals from the strips were measured and analyzed with a ChemiDoc XPS + imaging system and Image lab software (6.1; Bio-Rad Laboratories), respectively. The ELISA results were evaluated using a cell imaging multimode reader (Cytation 5).

All data generated or analyzed during this study are included in this published article (and its Supplementary Information files).

Received: 30 April 2021; Accepted: 9 November 2021

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The authors declare no competing interests.

The online version contains supplementary material available at https:// doi. org/ 10. 1038/ s41598-021-02084-7.Correspondence and requests for materials should be addressed to M.-G.K.

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