Integration of a Thermoelectric Heating Unit with Ionic Wind-Induced Droplet Centrifugation Chip to Develop Miniaturized Concentration Device for Rapid Determination of Salmonella on Food Samples Using Antibody-Functionalized SERS Tags

When a centrifugation-enriched sample of 100 μL containing the surface-enhanced Raman scattering (SERS) tag-bound bacteria (Salmonella in this study) is siphoned onto a glass slide next to an embedded thermoelectric heating chip, such a sessile droplet is quickly evaporated. As the size of the sample droplet is significantly reduced during the heating process, ionic wind streams from a corona discharge needle, stationed above the sample, sweep across the liquid surface to produce centrifugal vortex flow. Tag-bound Salmonella in the sample are then dragged and trapped at the center of droplet bottom. Finally, when the sample is dried, unlike the “coffee ring” effect, the SERS tag-bound Salmonella is concentrated in one small spot to allow sensitive detection of a Raman signal. Compared with our previous electrohydrodynamic concentration device containing only a corona discharge needle, this thermoelectric evaporation-assisted device is more time-effective, with the time of concentrating and drying about 100 μL sample reduced from 2 h to 30 min. Hence, sample throughput can be accelerated with this device for practical use. It is also more sensitive, with SERS detection of a few cells of Salmonella in neat samples achievable. We also evaluated the feasibility of using this device to detect Salmonella in food samples without performing the culturing procedures. Having spiked a few Salmonella cells into ice cubes and lettuce leaves, we use filtration and ultracentrifugation steps to obtain enriched tag-bound Salmonella samples of 200 μL. After loading an aliquot of 100 μL of sample onto this concentration device, the SERS tag signals from samples of 100 g ice cubes containing two Salmonella cells and 20 g lettuce leaf containing 5 Salmonella cells can be successfully detected.


Introduction
Conventional pathogenic bacteria tests require tedious cultivation procedures because microorganism counts are below 10 3 colony forming units (CFU) per mL in typical biological samples Sensors 2020, 20, 7177 3 of 14 to quantify pathogen cell numbers even down to the single bacterium level [18,24,25,27,28]. When a sample droplet of 30 µL was evaporated in half an hour using ionic wind to concentrate the collected bacteria, detection of a few cells of Salmonella was successfully accomplished [25].
However, because the evaporation rate of using ionic wind is not efficient enough to dry down typical concentrated food samples of sub-milliliter volume, there remains a need to develop a rapid evaporation and concentration device to identify food pathogens such as Salmonella. In particular, the concentrated NAEBs-bound pathogen cells allow simultaneous multiplex detection by Raman spectroscopy, which is expected to have a higher throughput in multiplex detection as compared to our previous multiplex detection approach using DEP to individually count pathogen cells [18]. This report presents our preliminary results on the detection of only one pathogen. We expect the analysis time will be similar for simultaneous multiplex detection of several pathogens using the corresponding number of NAEBs tagged by different Raman reporter molecules.
Having an embedded thermoelectric heating module on a metalized glass slide, we siphoned 100 µL aliquot of SERS tag-bound Salmonella sample on the slide next to the heater. As the size of the sample droplet was rapidly reduced during the accelerated heating process, tag-bound bacterial cells were then dragged and trapped at the center of droplet bottom by ionic wind-induced centrifugal flow. Because the cells were stationed at the stagnant point on the droplet bottom when the droplet was evaporated, typical "coffee ring"-like stains of particle sediments observed in ambient and heat-assisted drying of a droplet can be avoided. When the sample is finally dried, the SERS tag-bound cells can be concentrated in one small spot to allow sensitive detection of the Raman signal. Compared with our previous electrohydrodynamic concentration device containing only a corona discharge needle, this thermoelectric evaporation-assisted device is more time-effective, with the concentrating and drying time of a 100 µL sample significantly reduced. The capability of detecting a SERS signal from a few Salmonella cells should still maintain.
We used spiked food samples including ice cubes and lettuce leaves containing a few Salmonella cells to evaluate the method feasibility of using our rapid evaporation and concentration device. Without performing cell culturing procedures to amplify Salmonella cell numbers, we filtered these samples and subsequently used ultracentrifugation steps to obtain concentrated tag-bound Salmonella samples of 200 µL. The enriched turbid sample of 100 µL was loaded onto this concentration device to dry. Finally, SERS signals from the evaporated sample in the concentration spot were detected. With the single cell detection capability [18,27,28] provided by our SERS tags, our method is expected to provide the competence to comply with the food safety regulation requirement in a timely manner without tedious bacteria cultivation procedures.

Preparation of Antibody-Conjugated NAEBs
The procedures in previous papers were followed to prepare antibody-conjugated NAEBs [18,[24][25][26][27][28]. Each NAEB, of which the size was typically from 115 to 150 nm, encapsulated 2 to 5 AuNPs to form a nanoaggregate. Raman reporter molecules such as Safranin O were adsorbed onto AuNPs to initiate a clustering process to assemble a small-sized nanoaggregate. The nanoaggregate of this size was found to possess one characteristic absorption peak at 520 nm. Safranin O-labelled NAEBs were conjugated with a monoclonal antibody mAb 4B2D, one type of IgG1 protein obtained from a mouse immunized with Salmonella Choleraesuis strain OU7085. This mAb 4B2D antibody is specific for binding with Salmonella when the phase 2 flagellin FljB is recognized, as demonstrated in our previous paper [18].

Preparation of Spiked Salmonella Samples in De-Ionized Water
The bacteria Salmonella used in this study were heat-inactivated (56 • C, 30 min) for safety purposes. For the quantification of the bacterial concentration, the optical density of Salmonella at 600 nm in PBS solution was measured by a spectrophotometer (ChromTech CT-2300) using PBS as the reference background. Salmonella stock solutions were stored in phosphate buffer before use. Spiked water samples of various Salmonella concentrations were prepared by adding Salmonella from 2 to 20 cells into vials containing 1 mL de-ionized water. When added with an aliquot containing an excess amount of antibody-functionalized NAEBs, spiked water samples were shaken for 1 h to ensure Salmonella were bound with antibody-conjugated NAEBs. The NAEB-bound cells of Salmonella were collected by centrifuging the solution in a sample tube at 553 rcf for 15 min. The supernatant containing free unbound NAEBs was discarded using a pipette. The remaining NAEB-bound cells of Salmonella in the sample tube were re-dispersed using 200 µL de-ionized water.

Preparation of Spiked Salmonella Samples of Ice Cubes
Ice cubes were obtained from a local convenience store. Various amounts of Salmonella from 2 to 20 cells were added to batches of 100 g ice cubes to prepare spiked samples of different Salmonella concentrations. When these ice cubes in the samples were melted, each sample solution was fed into a stainless steel filtration funnel to flow through a membrane filter of mixed cellulose esters clamped at the end of the funnel to accomplish filtration using gravity force. The filtration funnel (SS-0289) and the filter membrane (pore size 0.45 µm) were from Finetech Research and Innovation Co. (New Taipei City, Taiwan, www.finetech-filter.com). Salmonella cells remained on the membrane filter were then collected by washing with 1 mL de-ionized water. To the collected solution of 1 mL, an aliquot containing an excess amount of antibody-functionalized NAEBs was added and the resulting solution was shaken for 1 h to ensure Salmonella cells were bound with antibody-conjugated NAEBs. The aforementioned procedures in Section 2.2.2 using the ultra-centrifugation method were followed to obtain enriched samples (ca. 200 µL).

Preparation of Spiked Salmonella Samples of Lettuce Leaves
Lettuce leaves in a ready-to-eat salad box were obtained from a local convenience store. Various amounts of Salmonella from 4 to 20 cells were added to batches of 50 g lettuce leaves to prepare spiked samples of different Salmonella concentrations. Each lettuce leaf sample was placed in a plastic bag filled with 450 mL de-ionized water. The bags were shaken vigorously to wash Salmonella cells out from the lettuce leaves. Each washing solution was loaded into a syringe filtration device (A1-1 PureTech™) equipped with a membrane filter (pore size 5.0 µm) from Finetech Research and Innovation Co. (New Taipei City, Taiwan, www.finetech-filter.com). When the syringe piston was pressed by hands, the solution was pushed through the filter membrane to accomplish the initial filtration step to remove small leaf debris. Next, the filtrate solution containing Salmonella cells was filtered using a stainless steel filtration funnel (SS-0289) equipped with a membrane filter of mixed cellulose esters (pore size 0.45 µm), also from Finetech Research and Innovation Co., with the assistance of vacuum suction. The Salmonella cells stayed on the filter membrane were collected by washing with 10 mL de-ionized water. The collected washing solution was again filtered using the same filtration apparatus and the filter membrane was washed with just 1 mL de-ionized water to reduce sample volume. To the final collected solution of 1 mL, an aliquot containing excess amount of antibody-functionalized NAEBs was added and the resulting solution was shaken for 1 h to ensure Salmonella cells were bound with antibody-conjugated NAEBs. The aforementioned procedures in Section 2.2.2 using ultra-centrifugation method were followed to obtain enriched samples (ca. 200 µL).

Equipmental Set-Up
As shown in Figure 1, except the evaporation and concentration device embedded with a thermoelectric heating unit, this study used the same set of apparatus as that in our previous paper. [25] Briefly, a function generator from Agilent Technologies (www.agilent.com) provided the ac output waveform of 50 kHz (0.5-1.0 V), pumped to ∼1000 V rms via a two-stage amplification system containing one broadband voltage amplifier and a transformer, which was obtained from Industrial Testing Equipment Co. (Port Washington, NY, USA, www.industrialtest.com). The final output cord of the amplification system providing ∼1000 V rms was connected to the corona needle of platinum wire (0.5 cm) to produce ionic wind. Similar to the conditions used in previous works [24,25], the optimized corona parameters were as follows. A platinum needle wire was inclined at 30-degree angle from the slide surface level and off the droplet center, pointing tangentially near the edge of the droplet. Besides, this wire was stationed 3 mm above the loaded droplet on the device slide.
Sensors 2020, 20, x FOR PEER REVIEW 6 of 15 droplets was accelerated. The droplet soon became a liquid film and further contracted inwards. Finally, this droplet was dried as a spot-like deposit containing the concentrated bacterial cells. The typical time span to complete the whole concentration process was 30 min. The photo-microscopic images of dried Salmonella spots were acquired. When necessary, the dried spot was colored with using Gram coloring method to enhance visualization effects. As described in Section 2.3, this evaporation and concentration device was stationed on the stage of one inverted-view microscope.
One CCD camera was used to videotape the process of drying the sample droplet. When the sample was finally dried to concentrate the bacterial cells, the SERS spectra of Safranin O in NAEBs were acquired from the deposited area using a micro-Raman spectroscope (XploRA, Horiba Scientific, Kyoto, Japan, www.horiba.com). These SERS spectra were obtained using a 10X objective when the laser light beam at 638 nm stroke on the sample spot.

Droplet Shrinking and Drying Processes
The whole evaporation and concentration process using our thermoelectric heater-embedded The evaporation and concentration device in this study comprised one ITO coated conducting glass slide. One small piece of copper ribbon electrode was attached on one end of this slide as an electrical contact with the ground line of power source. In addition, one thermoelectric heating chip (TEC1-049.03), from Tande Energy and Temperature Associates Co. (New Taipei City, Taiwan, www.tande.com.tw), was adhered on the other end of the same conducting slide using thermal pad (TG-A6200) from T-Global Technology Co. (Taoyuan, Taiwan, www.tglobalcorp.com) to accelerate the evaporation rate of the sample droplet. The area and thickness of this heating chip were 25 × 25 mm and 4.7 mm, respectively. This device to evaporate and concentrate Salmonella sample was clamped at the stage of one inverted-view microscope (IX51, Olympus Corp., Tokyo, Japan, www.olympus-global.com). One CCD camera (ProgRes ® , Jenoptik, Germany, www.jenoptik.com) was used to acquire microscopic images, which were then stored in a personal computer.

Evaporation and Concentration of Salmonella Samples
Firstly, we loaded 100 µL water samples containing polystyrene microspheres (5 µm in diameter) to observe the evaporation and concentration processes when the droplet location was heated to 35 • C, 40 • C, and 55 • C. As shown in the Appendix A section, unlike the image showing coffee ring stains of microsphere sediments obtained using direct heating device ( Figure A1), each image in Figure A2a-c obtained using our device at the aforementioned heating temperatures, respectively, shows one spot of concentrated microspheres. The evaporation time reduced from 28 to 20 min when the heating temperature increased from 35 to 40 • C. Although the evaporation time could be further marginally reduced at higher temperature, overheating caused charred marks as appeared in Figure A2c. Therefore, we chose 40 • C as the optimum heating temperature to concentrate Salmonella samples.
In an air conditioning laboratory at 25 • C and 50% relative humidity, when one aliquot of 100-µL enriched sample containing NAEB-bound Salmonella cells was dropped onto an ITO slide next to the thermoelectric heating unit with a pipette, it formed a hemispheric sessile droplet. As the slide was pre-heated to 40 • C, this sample droplet immediately started to be evaporated and began to shrink. At the same time, the corona needle with ac voltage produced ionic wind streams from the wire tip. Similar to our previous observations, when the evaporating droplet decreased to a size that was significantly smaller than its original size, the observed centrifugal vortex flows dragged tag-bound Salmonella cells downwards, which gradually accumulated near the center of droplet bottom [25]. With the assistance of thermoelectric heating, the evaporation rate of ionic wind-impinged droplets was accelerated. The droplet soon became a liquid film and further contracted inwards. Finally, this droplet was dried as a spot-like deposit containing the concentrated bacterial cells. The typical time span to complete the whole concentration process was 30 min. The photo-microscopic images of dried Salmonella spots were acquired. When necessary, the dried spot was colored with using Gram coloring method to enhance visualization effects. As described in Section 2.3, this evaporation and concentration device was stationed on the stage of one inverted-view microscope. One CCD camera was used to videotape the process of drying the sample droplet. When the sample was finally dried to concentrate the bacterial cells, the SERS spectra of Safranin O in NAEBs were acquired from the deposited area using a micro-Raman spectroscope (XploRA, Horiba Scientific, Kyoto, Japan, www.horiba.com). These SERS spectra were obtained using a 10X objective when the laser light beam at 638 nm stroke on the sample spot.

Droplet Shrinking and Drying Processes
The whole evaporation and concentration process using our thermoelectric heater-embedded micro centrifugation device takes about 30 min to obtain the dried spot containing concentrated bacterial cells. The images in Figure 2 show the shape evolution of a sample droplet during the drying processes. The loaded sessile droplet of 100 µL containing 1000 CFU/mL Salmonella shrank from dia.
Sensors 2020, 20, 7177 7 of 14 6 mm (Image A) to dia.~4.6 mm (Image B) in 13 min because of sufficient thermoelectric heating. The side of the droplet closer to the heater evaporated more rapidly than the other side because it received heat more efficiently. Therefore, similar to our previous observations of only using ionic wind to dry down a sample droplet, the evaporation rate along the droplet surface varied, resulting in the collapse of the droplet as a film (dia.~2 mm) in 23 min after the evaporation process. At the same time, the ionic wind-induced micro-centrifugal flow transported the NAEB-bound Salmonella cells to the center of droplet bottom (Image C) and finally, a spot-like dried deposit was obtained (Image D). When one side of droplet evaporates more rapidly than the other side, the resulted internal flow circulation can drive the NAEB microparticles to self-assemble at the surface. [29] Remaining free unbound NAEB particles accumulated at the surface alter the surface tension. The droplet is, therefore, stretched to collapse. The side of the droplet closer to the heater evaporated more rapidly than the other side because it received heat more efficiently. Therefore, similar to our previous observations of only using ionic wind to dry down a sample droplet, the evaporation rate along the droplet surface varied, resulting in the collapse of the droplet as a film (dia. ~2 mm) in 23 min after the evaporation process. At the same time, the ionic wind-induced micro-centrifugal flow transported the NAEB-bound Salmonella cells to the center of droplet bottom (Image C) and finally, a spot-like dried deposit was obtained (Image D). When one side of droplet evaporates more rapidly than the other side, the resulted internal flow circulation can drive the NAEB microparticles to self-assemble at the surface. [29] Remaining free unbound NAEB particles accumulated at the surface alter the surface tension. The droplet is, therefore, stretched to collapse.

Determination of Salmonella in Spiked Water Samples
The traces in Figure 3 show the SERS spectra of Safranin O-labelled NAEBs acquired from the dried spots of tag-bound Salmonella cells. The amount of Salmonella spiked in these samples prepared using 1 mL de-ionized water are from 2 to 20 cells. Each spiked sample is added with antibody-conjugated NAEBs and enriched to ca. 200 μL from 1 mL solution using ultra-centrifugation where the supernatant liquid is removed. One aliquot of 100 μL enriched sample is pipetted on the concentration device to be dried. The embedded micro-photographic image in Figure 3

Determination of Salmonella in Spiked Water Samples
The traces in Figure 3 show the SERS spectra of Safranin O-labelled NAEBs acquired from the dried spots of tag-bound Salmonella cells. The amount of Salmonella spiked in these samples prepared using 1 mL de-ionized water are from 2 to 20 cells. Each spiked sample is added with antibody-conjugated NAEBs and enriched to ca. 200 µL from 1 mL solution using ultra-centrifugation where the supernatant liquid is removed. One aliquot of 100 µL enriched sample is pipetted on the concentration device to be dried. The embedded micro-photographic image in Figure 3 shows bottom trace in green color using a blank aliquot containing only antibody-conjugated NAEBs labelled with Safranin O in the absence of Salmonella cells. Ideally, the green trace of the blank should be close to the background Raman intensity. Although quite reproducible in intensity, the non-negligible characteristic peaks of Safranin O in the green trace of the blank suggest that some free unbound NAEBs remain in the sediment after centrifugation. The causes for this are still under investigation and one possibility is that some NAEBs aggregated, resulting in heavier particles not being removed by centrifugation. Our preliminary results using dextran-coated NAEBs show smaller blank signals, indicating that an anti-nonspecific adsorption coating on NAEBs minimizes aggregation of NAEBs. The spectral traces in Figure 3 also show that the peak intensity increased when the spiked amount of Salmonella cells increases. These findings are consistent with the results of our previous study of detecting Salmonella using SERS tags with an ionic wind-based micro-centrifugal concentration device [25].
reproducible in intensity, the non-negligible characteristic peaks of Safranin O in the green trace of the blank suggest that some free unbound NAEBs remain in the sediment after centrifugation. The causes for this are still under investigation and one possibility is that some NAEBs aggregated, resulting in heavier particles not being removed by centrifugation. Our preliminary results using dextran-coated NAEBs show smaller blank signals, indicating that an anti-nonspecific adsorption coating on NAEBs minimizes aggregation of NAEBs. The spectral traces in Figure 3 also show that the peak intensity increased when the spiked amount of Salmonella cells increases. These findings are consistent with the results of our previous study of detecting Salmonella using SERS tags with an ionic wind-based micro-centrifugal concentration device [25].
Each sample was firstly enriched to ca. 200 μL and one aliquot of 100 μL was siphoned to pipette onto the concentration device. Therefore, in Figure 3, the pink traces are from just two NAEB-bound Salmonella cells. This finding is consistent with the results in our previous study of using NAEB Raman tags to detect a single cell of Salmonella. [25] Therefore, there should be no considerable sample loss during the aforementioned enrichment procedures.
Using the height intensity of the 1556 cm −1 peak of each sample, one standard curve was established, as shown in the inset of Figure 3. This curve indicates a highly linear relationship (R = 0.99) between the Raman intensity and number of Salmonella cells in the spiked samples, where two replicates were determined for each sample.  Each sample was firstly enriched to ca. 200 µL and one aliquot of 100 µL was siphoned to pipette onto the concentration device. Therefore, in Figure 3, the pink traces are from just two NAEB-bound Salmonella cells. This finding is consistent with the results in our previous study of using NAEB Raman tags to detect a single cell of Salmonella [25]. Therefore, there should be no considerable sample loss during the aforementioned enrichment procedures.
Using the height intensity of the 1556 cm −1 peak of each sample, one standard curve was established, as shown in the inset of Figure 3. This curve indicates a highly linear relationship (R = 0.99) Sensors 2020, 20, 7177 9 of 14 between the Raman intensity and number of Salmonella cells in the spiked samples, where two replicates were determined for each sample. Figure 4 contains the SERS traces of Safranin O-labelled NAEB tags acquired from the tag-bound Salmonella cells in the dried spots of ice cube samples of 100 g, in which various amounts of Salmonella from 2 to 20 cells were spiked. After a spiked ice cube sample was melted and filtered, the Salmonella cells remaining on the filter were collected by washing with 1 mL de-ionized water. Then, each sample of the collected solution was added with antibody-conjugated NAEBs and enriched to ca. 200 µL from 1 mL using ultra-centrifugation where the supernatant liquid was removed. One aliquot of 100 µL enriched sample was pipetted onto the concentration device to be dried. The embedded photographic image in Figure 4 shows the dried spot of the concentrated ice cube sample, spiked with six cells of Salmonella. Similar to the spectra in Figure 3, the green trace of the spiked sample containing only two cells of Salmonella can also be distinguished from the bottom trace in indigo, using an aliquot containing only antibody-conjugated NAEBs labelled with Safranin O in the absence of Salmonella cells. In addition to clear characteristic peaks of Safranin O in these spectra in Figure 4, the height intensities of each trace at 1556 cm −1 are comparable with that of 1 mL de-ionized water samples spiked with the same amount of Salmonella cells in Figure 3. Using the peak intensities at 1556 cm −1 corresponding to 2, 6, 12, 16, and 20 cells in Figure 4, we also obtained a linear relationship (R = 0.985) between Raman intensity and number of Salmonella cells in the spiked samples, as shown in the inset of Figure 4, where two replicates were determined for each sample. The Raman intensity of the blanks was reproducible with a value of 860 ± 35. To avoid a false-positive signal due to the background signal, we define the background level (shown as a dashed line in Figure 3) as the mean plus 3-times the standard deviation of the Raman intensity from the blanks. It can be seen that the signal from the sample with only two Salmonella cells is well above the background level.

Determination of Salmonella in Spiked Ice Cube Samples
Sensors 2020, 20, x FOR PEER REVIEW 9 of 14 the Salmonella cells remaining on the filter were collected by washing with 1 mL de-ionized water. Then, each sample of the collected solution was added with antibody-conjugated NAEBs and enriched to ca. 200 μL from 1 mL using ultra-centrifugation where the supernatant liquid was removed. One aliquot of 100 μL enriched sample was pipetted onto the concentration device to be dried. The embedded photographic image in Figure 4 shows the dried spot of the concentrated ice cube sample, spiked with six cells of Salmonella. Similar to the spectra in Figure 3, the green trace of the spiked sample containing only two cells of Salmonella can also be distinguished from the bottom trace in indigo, using an aliquot containing only antibody-conjugated NAEBs labelled with Safranin O in the absence of Salmonella cells. In addition to clear characteristic peaks of Safranin O in these spectra in Figure 4, the height intensities of each trace at 1556 cm -1 are comparable with that of 1 mL de-ionized water samples spiked with the same amount of Salmonella cells in Figure 3. Using the peak intensities at 1556 cm -1 corresponding to 2, 6, 12, 16, and 20 cells in Figure 4, we also obtained a linear relationship (R = 0.985) between Raman intensity and number of Salmonella cells in the spiked samples, as shown in the inset of Figure 4, where two replicates were determined for each sample. The Raman intensity of the blanks was reproducible with a value of 860 ± 35. To avoid a false-positive signal due to the background signal, we define the background level (shown as a dashed line in Figure 3) as the mean plus 3-times the standard deviation of the Raman intensity from the blanks. It can be seen that the signal from the sample with only two Salmonella cells is well above the background level.
If sample loss possibly occurs in the filtration and collection procedures for the ice cube samples spiked with only two Salmonella cells, the signal intensity should vary significantly with some samples exhibiting a SERS intensity below the background level because some sample aliquots may contain no Salmonella cells. The reasonable reproducibility at the point of two cells in the aforementioned standard curve suggests that the sample loss is negligible while the method achieves the capability of detecting a SERS signal from a single cell. The safety requirement of drinking water is that no Salmonella should be found in the 100 mL cultured sample. When an ice cube sample in street drinks or beverages was determined, the detection limit of our method nearly reached the regulation compliance standard without cultivation procedures. If sample loss possibly occurs in the filtration and collection procedures for the ice cube samples spiked with only two Salmonella cells, the signal intensity should vary significantly with some samples exhibiting a SERS intensity below the background level because some sample aliquots may contain no Salmonella cells. The reasonable reproducibility at the point of two cells in the aforementioned standard curve suggests that the sample loss is negligible while the method achieves the capability of detecting a SERS signal from a single cell. The safety requirement of drinking water is that no Salmonella should be found in the 100 mL cultured sample. When an ice cube sample in street drinks or beverages was determined, the detection limit of our method nearly reached the regulation compliance standard without cultivation procedures. Figure 5 shows the clear SERS traces of Safranin O-labelled NAEBs from the tag-bound Salmonella cells in the dried spots of spiked lettuce leaf samples. The spiked amounts in these samples of 50 g lettuce leaves were 6, 12, 16, and 20 cells. In Figure 5, the second to bottom and bottom traces in green and indigo, respectively, used a negative control sample containing Safranin O-labelled NAEBs but no Salmonella cells and a blank containing only lettuce leaves but without Safranin O-labelled NAEBs and Salmonella cells. When a sample solution of 450 mL de-ionized water containing spiked lettuce leaves was filtered, the bacterial cells that remained on the filter membrane were collected by washing with 1 mL de-ionized water. Then, each sample of collected solution was enriched to ca. 200 µL from 1 mL using ultra-centrifugation where the supernatant liquid was removed. One aliquot of 100 µL enriched sample was pipetted onto the concentration device to be dried. The upper embedded micro-photographic image in Figure 5 next to the main frame shows the dried concentrated sample of lettuce leaf washing solution, spiked with 6 Salmonella cells. Using the peak intensities at 1556 cm −1 corresponding to 6, 12, 16, and 20 cells in Figure 5, one standard calibration curve was obtained, as shown in the inset of Figure 5. The intensity values of these samples are somewhat higher than that with the same number of cells in Figure 3 or Figure 4. However, the linearity of the standard curve between Raman intensity and number of Salmonella cells in the spiked samples deteriorated to a fairly acceptable level (R = 0.97), when two replicates were determined for each sample.

Determination of Salmonella in Spiked Lettuce Leaf Samples
Using a lettuce leaf sample as a blank containing no Salmonella cells and Safranin O-labelled NAEBs, the Raman spectrum as shown in the bottom indigo trace of Figure 5 does not contain spectral peak features of Safranin O. In addition, the intensities around the characteristic peaks of Safranin O are much lower than that of the negative control sample, as shown in the second bottom green trace. For the negative control sample, as shown in the lower micro-photographic image of Figure 5 next to the main frame, some fibrous tiny residues of lettuce leaves were also found to sediment on the slide, although not in the same location of trapped bacterial cells. The peak intensity at 1556 cm −1 in the second to bottom green trace in Figure 5 was about 5000 counts, higher than the intensities (≤2000 counts) of other negative control samples without the fibrous residues, as shown in Figures 3  and 4, indicating the possibility of nonspecific adsorption of NAEBs onto the fibrous residues. Hence, it is important to minimize the anti-nonspecific adsorption property of the NAEBs by an antifouling coating in order to lower the detection limit. Because the Raman intensity of the negative control samples (2985 ± 1766) varies highly, we defined the background level (shown as a dashed line in Figure 5) as the mean plus 3-times the standard deviation of the Raman intensity from the negative control samples and accepted only the results above the background level as positive results. By this definition, we estimated that the detection limit of determining spiked lettuce leaf sample was 12 Salmonella cells per 50 g.
The safety requirement of ready-to-eat lettuce is that no Salmonella should be found in the cultured sample of 20 g leaves. Because of the problem of residue absorption of NAEBs onto lettuce leaves, our detection limit of 5 Salmonella cells per 20 g lettuce leaves is slightly higher than the regulation compliance standard. When our method was employed to determine real samples, in addition to increasing the sampling weight of lettuce leaves to 50 g, it was important to further improve the anti-nonspecific adsorption property of the NAEB surface. the negative control samples and accepted only the results above the background level as positive results. By this definition, we estimated that the detection limit of determining spiked lettuce leaf sample was 12 Salmonella cells per 50 g.
The safety requirement of ready-to-eat lettuce is that no Salmonella should be found in the cultured sample of 20 g leaves. Because of the problem of residue absorption of NAEBs onto lettuce leaves, our detection limit of 5 Salmonella cells per 20 g lettuce leaves is slightly higher than the regulation compliance standard. When our method was employed to determine real samples, in addition to increasing the sampling weight of lettuce leaves to 50 g, it was important to further improve the anti-nonspecific adsorption property of the NAEB surface.

Conclusions
We have successfully developed a miniaturized rapid evaporation and concentration device via integrating a thermoelectric heating unit with ionic wind-induced droplet centrifugation chip to determine spiked Salmonella in food samples without bacteria cultivation steps. The loaded sample aliquot of~100 µL containing Raman tag-bound Salmonella cells can be dried in 30 min because of the efficient evaporation provided by thermoelectric heater. At the same time, Salmonella cells were dragged toward to the center of sample droplet bottom by ionic wind-induced centrifugal flows to concentrate in a dried spot. Single cell detection capability is provided by the sensitive scattering signals acquired from concentrated Raman tag-bound Salmonella deposits. Using SERS detection, we demonstrated that this device can detect 2 and 12 Salmonella cells spiked in a 100 g ice cube sample and 50 g lettuce leaf sample, respectively. With this high sensitivity, the detection limit of our method is close to the food safety regulation compliance standard, while tedious bacteria cultivation is not required.
Using this simple device, rapid sample concentration can be accomplished by a nontechnical person simply by loading a sample droplet using a pipette. The evaporation and concentration efficiency of this device should be further improved through combining a Marangoni effect-based technique such as a superhydrophobic surface coating with surfactant or viscosity modifier addition. The contact line pinning of the sample droplet will be controlled more precisely during the evaporation process to avoid overheating at high temperature. Tag-bound Salmonella cells could precipitate in a more concentrated manner at the bottom of a conical well when the droplet drying is completed. We will investigate the aforementioned ideas in the future.

Conflicts of Interest:
The authors declare no conflict of interest.

Appendix A
person simply by loading a sample droplet using a pipette. The evaporation and concentration efficiency of this device should be further improved through combining a Marangoni effect-based technique such as a superhydrophobic surface coating with surfactant or viscosity modifier addition. The contact line pinning of the sample droplet will be controlled more precisely during the evaporation process to avoid overheating at high temperature. Tag-bound Salmonella cells could precipitate in a more concentrated manner at the bottom of a conical well when the droplet drying is completed. We will investigate the aforementioned ideas in the future. δ, in plane bending; γ, out of plane bending; ω, wagging; υ, stretching.