A Microfluidic Chip for ICPMS Sample Introduction

Summary

We present a discrete droplet sample introduction system for inductively coupled plasma mass spectrometry (ICPMS). It is based on a cheap and disposable microfluidic chip that generates highly monodisperse droplets in a size range of 40−60 µm at frequencies from 90 to 7,000 Hz.

Abstract

This protocol discusses the fabrication and usage of a disposable low cost microfluidic chip as sample introduction system for inductively coupled plasma mass spectrometry (ICPMS). The chip produces monodisperse aqueous sample droplets in perfluorohexane (PFH). Size and frequency of the aqueous droplets can be varied in the range of 40 to 60 µm and from 90 to 7,000 Hz, respectively. The droplets are ejected from the chip with a second flow of PFH and remain intact during the ejection. A custom-built desolvation system removes the PFH and transports the droplets into the ICPMS. Here, very stable signals with a narrow intensity distribution can be measured, showing the monodispersity of the droplets. We show that the introduction system can be used to quantitatively determine iron in single bovine red blood cells. In the future, the capabilities of the introduction device can easily be extended by the integration of additional microfluidic modules.

Introduction

Elemental analysis of liquid samples by inductively coupled plasma mass spectrometry (ICPMS) is commonly carried out using nebulizers in combination with spray chambers as introduction system¹. In this sample introduction system the sample is sprayed by a nebulizer to generate a polydisperse aerosol. A downstream spray chamber is used to filter out large droplets. This method is associated with high sample consumption (>0.3 ml min^-1)² and an incomplete sample transport. Thus, it becomes impractical for applications where only microliter sample volumes are available, as in biological, forensic, toxicological and clinical studies³. To reduce the sample consumption, nebulizers with smaller nozzle dimensions were developed³. However, the reduced nozzle size increases the risk of clogging when samples of undigested biological fluids or concentrated salt solutions have to be analyzed³.

A different approach for sample introduction was proposed by Olesik et al.⁴. The authors injected a liquid into ICPMS in the form of monodisperse discrete microdroplets, which were produced by a piezo-electrically driven micropump. Even though this very system did not find wide application, it initiated the further development of the concept of discrete droplet introduction in ICPMS. Today, piezo-electrically driven dispensing systems, which can generate droplets in size of 30, 50, 70 and 100 µm and at frequencies of 100-2,000 Hz, can be purchased. The droplets can be transported into ICPMS with close to 100% efficiency⁵. These microdroplet dispensers have been applied for quantitatively measuring single nanoparticles^5,6 as well as characterizing individual biological cells⁷. A similar system based on thermal inkjet technology⁸ was tested for analysis of biological samples⁹. Although the available single droplet introduction systems are very efficient, can be used for small sample volumes and are promising for the analysis of nanoparticles and cells, they have several limitations. For a fixed nozzle size, the droplet size can be varied only slightly (unless custom settings are used¹⁰). Changes of the physical properties of the liquid (pH, salt content) can alter the droplet characteristics (size, injection speed). Also, these devices are rather expensive, prone to clogging and are difficult to clean.

Another method to generate droplets is known in the field of droplet microfluidics¹¹. In recent years droplet microfluidics has gained interest for (bio-)chemical reactions^12-15 and for single cell studies^16,17. Additionally, this technique was applied for introducing samples in electrospray ionization mass spectrometry^18,19 and for preparing samples in matrix-assisted laser desorption/ionization mass spectrometry^20,21.

Recently, we introduced a microfluidic based system for sample introduction in ICPMS²². The key component of our introduction system is the liquid assisted droplet ejection (LADE) chip. This chip consists completely of poly(dimethylsiloxane) (PDMS). In the first channel junction flow focusing is used to generate monodisperse droplets of an aqueous sample solution (Figure 1). For this purpose the highly volatile (boiling point of 58-60 °C²³) and immiscible carrier phase perfluorohexane (PFH) is used (Figure 1). These PFH properties enable a stable droplet generation and fast removal of the carrier phase. Changes in the properties of the sample liquid influence this generation method less, compared to other droplet generators. The droplet size is adjustable over a wide range by changing the flow rates of the aqueous phase and the PFH. In a downstream secondary junction, more PFH is added to increase the flow speed to at least 1 m sec^-1. At this speed the liquid can be ejected from the chip in stable and straight jet (Figure 1) without droplet destruction (Figure 1 inset). This double-junction design allows controlling the jet stability independent of droplet generation. The droplets are transported to the ICPMS with a customized transport system. This system comprises a falling tube and a membrane desolvator to remove the PFH. The dried residues of the aqueous droplets are subsequently ionized in the plasma of the ICPMS and a mass detector measures the ions. The front part of the chip is barrel-shaped to ensure a tight connection with the droplet transport system. The ejection of the aqueous sample as droplets in PFH is beneficial, because contact with the nozzle is avoided. This considerably lowers the risk of nozzle clogging, which can be a problem when working with cell suspensions or concentrated salt solutions. The LADE chips, fabricated by PDMS soft lithography, are cheap (material cost approximately $2 per chip), disposable and easy to modify. In combination with the fabrication that requires only a small amount of manual work each experiment can be performed with a new chip. Therefore, a laborious cleaning is not needed and cross contamination is minimized.

Here, the fabrication of the LADE chip by soft lithography and its application for ICPMS are described. Examples of measurements with an aqueous solution and a cell suspension are presented.

Protocol

1. SU-8 Master Fabrication (Figure 2)

NOTE: Perform the fabrication of the SU-8 master molds in a clean room to prevent defects caused by dust particles. Two wafers are needed for the fabrication, one wafer with microfluidic features and one without.

1. Prepare the master molds for the microfluidic chip. First apply an adhesion layer to the silicon wafer.
   1. Dehydrate a silicon wafer for 10 min at 200 °C. Cool the wafer down to RT and load it on to a spin coater and spin coat it with SU-8 2002 with the following protocol.
   2. Dispense about 3 ml resist onto the wafer.
   3. Spin the wafer at 500 rpm for 10 sec to spread the resist over the whole wafer.
   4. Spin the wafer at 2,000 rpm for 30 sec to achieve a resist height of approximately 2 µm.
2. Remove excess resist from the edge of the wafer with an acetone soaked swab, to prevent sticking of the wafer to the hot plate in the next step. Bake the wafer for 60 sec at 95 °C on a hot plate.
3. Expose the whole wafer with ultraviolet light (80 mJ/cm² at 365 nm). Post-bake the wafer for 120 sec to 95 °C.
4. Cool the wafer down and immediately spin coat the wafer again using the following protocol for SU-8 2050:
   1. Spin the wafer at 100 rpm for 20 sec (dispense about 3 ml SU-8 resist during this step).
   2. Spin the wafer at 500 rpm for 10 sec to spread the resist over the whole wafer.
   3. Spin the wafer at 3,250 rpm for 30 sec resulting in a resist thickness of approximately 40 µm.
5. Again, remove excess resist from the edge of the wafer with an acetone soaked swab and soft bake the wafer on a hot plate for 180 sec at 65 °C and for 360 sec at 95 °C.
6. Prepare the photomask by sticking it to a soda-lime glass. See Figure 3 for the mask design. Use a mask aligner to expose the resist with ultraviolet light (160 mJ/cm², measured at 365 nm) through the prepared mask. Bake the exposed wafer again on a hot plate for 60 sec at 65 °C and for 360 sec at 95 °C.
7. After cooling down the wafer to RT, immerse it in a glass Petri dish filled with developer for 5 min to develop the resist. Gently agitate the petri dish to remove unexposed SU-8. Rinse the wafer with isopropanol and blow it dry with a nitrogen gun.
8. Examine the wafer under a microscope. In case undeveloped resist remains on the features, develop the wafer again for a few minutes, as described in step 1.7.
9. Remove any residual solvent by baking the wafers for 2 hr at 200 °C. Check the height of the features with a step profiler. In case the measured height differs from the desired height begin with this protocol again and adapt the spin speed in step 1.1.4.
10. To prevent sticking of the PDMS to the wafer silanize it by placing it in desiccator together with 50 µl of 1H,1H,2H,2H-perfluorodecyltrichlorosilane in a small porcelain dish. Reduce the pressure in the desiccator to 100 mbar and incubate the wafer for 12 hr.
    1. For the blank PDMS parts silanize another silicon wafer using the method of step 1.10. To save time silanize both wafers at the same time in a single desiccator.

2. LADE Chip Fabrication

NOTE: The LADE chip is made out of two PDMS pieces that are bonded together by adhesive bonding²⁴. The first part contains the microfluidic features. The other part is flat and used to seal the channels. Bonded together, they form the round shape necessary to interface the chip with the droplet transport system. Here, the fabrication of the two parts and their bonding is described. All process steps are shown in Figure 4.

1. Prepare 44 g of PDMS by mixing 40 g of prepolymer with 4 g of the PDMS curing agent (this will result in up to 6 chips). Degas the PDMS in a desiccator until it is bubble free (this will take about 20 min).
2. Replica molding of the structured halves.
   1. Place the casting form on top of the wafer and snap it into place using the guiding structures around the design (see Figure 5). Skip the snapping into place for the flat PDMS halve.
   2. Pour approximately 3 to 4 g of the degased PDMS in the casting form and place it for 6 min on a hot plate at 150 °C. Cool down the cured PDMS in the casting form and carefully lift the casting form wafer using a spatula.
   3. In order to prevent any contamination of the microfluidic channels cover the side of the chip that was previously in contact with the wafer with tape. Carefully cut the tape along the edge of the PDMS part to remove excess PDMS.
3. To fabricate the flat PDMS halves repeat the above-mentioned steps 2.2.1 to 2.2.3 with the blank silanized wafer.
4. Peel of the tape and punch fluid connection holes into the structured halves with a biopsy puncher. Protect the structures with tape during storage.
5. Bond the PDMS parts together by adhesive bonding using the PDMS curing agent²⁴.
   1. Take an untreated silicon wafer and spin coat it with PDMS curing agent for 30 sec at 6,000 rpm. Take the wafer out of the spin coater.
   2. Remove the tape from the structured halves and place them with the structures facing downwards onto the wafer. Gently push on top of the PDMS to remove air bubbles.
   3. Remove the tape from the blank PDMS halves. Take a structured halve from the wafer and manually align it on top of the flat PDMS halve. Gently squeeze the part together to remove air bubbles and let the assembled chip cure for 24 hr at RT. Do not push the parts together with force as this can cause the channels to collapse.
6. Cut the tip of the chip along the indicator line orthogonal to the nozzle channel with a utility knife to open the outlet nozzle. Use an alignment device to ensure a straight cut, which is necessary for a straight liquid ejection. Inspect the chip under a microscope for defects in the microfluidic channels and dust particles. Put a tape over the inlet holes to protect the chips during storage.
7. Connect a Woulff bottle with tubing to a dry nitrogen source and to all inlets of the LADE chip. Deposit 50 µl of 1H,1H,2H,2H-perfluorodecyltrichlorosilane at the bottom of the Woulff bottle and close it.
8. Silanize the microfluidic channels by flushing all channels for 20 min with the nitrogen stream carrying 1H,1H,2H,2H-perfluorodecyltrichlorosilane at a flow rate of approximately 1 ml/sec. The chips are ready for experiments and can be stored for at least several weeks at RT.

3. Preparations for Measurement / Droplet Transport System

NOTE: Build the whole droplet transport system on top of an optical table, since it is necessary to construct a stable supporting structure for the setup. A scheme of the whole droplet transportation system is depicted in Figure 6.

1. Install a custom cyclonic poly(methyl methacrylate) (PMMA) adapter with an 50 cm attached stainless steel tube vertically. Attach the adapter to a helium source with a mass flow controller. Attach a (high-speed) camera and a lamp to the adapter on the opposite sites for droplet visualization.
2. Place a cartridge heater in the middle of the steel tube and use poly(vinyl chloride) (PVC) tubing and a Legris tube connector to connect the end of the steel tube with the inlet of the membrane desolvator.
3. Connect the outlet of the desolvator with another PVC tubing to a laminar flow adapter, which is directly connected to the ICPMS inlet. Connect the laminar flow adapter to an argon source with a mass flow controller and later on use it to admix Argon to achieve a stable operation condition.
4. Align the adapter as well as the steel tube vertical with a spirit level. If the alignment is not accurate, it may lead to significant losses of droplets. Insert a plug into the adapter to prevent gases leaking out during the system warm up time.
5. Start all above-mentioned gas flows and devices using the settings from Table 1. Allow the system to warm up for 15 min. The cartridge heater needs 2 hr to stabilize the temperature, switch it on in advance.
6. Place the syringe pumps on a rack at the height of cyclonic helium adapter. Keep the distance between the syringe pumps and the adapter as short as possible.

4. Measurements

NOTE: The following protocol is written in general terms because of the variety of solutions and suspensions that can be used. However, cell suspensions should be diluted to a concentration of < 1 x 10⁷ cells/ml, when single cell analysis is performed, to ensure that the majority of the droplets carry only one cell. For measurements with cells place the syringe pumps at an angle so that the outlet of the syringes point downwards and install the tubing in such a way that they point downwards.

1. Attach tubing to the syringes. Load two 5 ml syringes with perfluorohexane and one 1 ml syringe with a sample solution or suspension. Remove all bubbles trapped in the syringes and tubing.
2. Install the syringes in a syringe pump and connect them to the inlets of the chip. Start the syringe pumps using the start settings from Table 1 (or higher flow rates). Give the flows 3 to 5 min to stabilize.
   1. Remove excess liquid from the tip of the chip with a tissue. The liquids should now eject from the chip in a straight jet. If a straight ejection cannot be achieved by wiping with a tissue replace the chip and start over with this step. 
3. Remove the plug from the adapter and carefully insert the chip into the adapter. Lubricate the chip with FC-40 if necessary. A chip can be used for at least 2 hr of experiments.
4. Change the flow rate to be within the recommended measurement settings from Table 1. Lower flow rate of the PFH not only saves PFH but also reduces signal background, caused by isobaric interferences.
5. Give the system 2-5 min to stabilize (depending on the chosen flow rates). Optimize the ICPMS for the highest signal intensity of the analytes of interest.
   1. Successively adjust the flows of all the gases on the mass flow controllers (see the recommended ranges in Table 1) until the maximum signal intensity of the analytes of interest is achieved. Tune the plasma power and the focusing lens voltages (according to the manufacturer's recommended ranges) on the ICPMS in the same way.
6. Set the ICPMS to a dwell time of 10 msec (applied for the very ICPMS used but can be adjusted with other instruments to ensure a time-resolved acquisition). Start recording the signal of a particular m/z using manufacturer’s protocol.
7. After the measurement, transfer the raw data to data analysis program for evaluation. Bin the data, given in counts per 10 msec, with a built-in-function, and plot resulting bin center values against counts. Fit each peak in the plotted frequency distribution histogram with a Gauss function. The mean and sigma of the fit represent the mean signal intensity and its standard deviation, respectively.

5. Calibration Concept

1. Measure a single or multi-element standard solution containing the element or elements of interest at the same flow rates as the sample.
2. Place a LADE chip in a petri dish on a microscope. For a better image quality use a non-round chip. Fabricate this chip as described in step 2, but using a simple rectangular casting form instead of the partially round shaped one.
3. Follow the steps 4.1 to 4.2.1 to start the droplet generation. Set the flow rates to the flow rates used in step 5.1.
4. Record images of the aqueous droplets with a high-speed camera attached to a microscope (20X objective). Use an image analysis software like the droplet morphometry and velocimetry software by Basu²⁵ to obtain the average droplet diameter from the recordings.
5. Use average droplet diameter to calculate the droplet volume, assuming the droplet is a spherical object.
   1. From this volume and the known concentration of an analyte in the droplet calculate the number of corresponding atoms. Divide the number of measured ions per droplet by the number of atoms to obtain the detection efficiency. Use this detection efficiency to calculate the number of atoms in an unknown sample.
      NOTE: Since the variations between individual chips are small²², it is not necessary to repeat the measurement of the droplet size for every chip or solution if the flow rates remain the same. A list of the droplet sizes and frequencies according to the specific flow rates is published by Verboket et al.²².

Results

The presented system can be employed to measure small volumes of solutions or suspensions containing cells or nanoparticles. Examples of a measurement of a standard solution and characterization of single cells are shown here. More examples can be found in Verboket et al.²².

Typically the signal of a single droplet of a solution is a very short event. It usually lasts for a few 100 µsec²⁶. With the ICPMS used here (dwell time 10 msec) short signals like thes...

Discussion

Although the fabrication of the chips is very reliable there are some critical points during the fabrication that require special attention. First, cleanliness during the assembly is highly important to prevent contamination of the chip by dust. The dust can block the channels and prevent a stable droplet generation. Second, it is especially important that the tip is cut orthogonal to the nozzle channel. The angle of the cut strongly influences the ejection angle. If the liquid is ejected at an angle it can cause a loss ...

Materials

Name	Company	Catalog Number	Comments
Silicon wafer 100 mm	Si-Mat (Kaufering, Germany)
SU-8 2002	Microchem Corp. (Massachusetts, U.S.A.)
SU-8 2050	Microchem Corp. (Massachusetts, U.S.A.)
Acetone	Merk VWR (Darmstadt, Germany)	100014
MR-developer 600	Microresist Technology GmbH (Berlin, Germany)
Isopropanol	Merk VWR (Darmstadt, Germany)	109634
1H,1H,2H,2H-perfluorodecyltrichlorosilane	ABCR-Chemicals (Karlsruhe, Germany)	AB111155
Sylgard 184 silicone elastomer kit (PDMS)	Dow Corning (Michigan, U.S.A.)	39100000
Perfluorohexane 99%	Sigma-Aldrich (Missouri, U.S.A.)	281042
FC-40	ABCR-Chemicals (Karlsruhe, Germany)	AB103511
Phosphate-buffered saline	Life Technologies (Paisley, U.K.)	10010-015
Red blood cells in phosphate-buffered saline	Rockland Immunochemicals Inc. (Pennsylvania, U.S.A.)	R400-0100
Single-element standard solutions Na, Fe	Inorganic Ventures (Virginia, U.S.A.)
Multielement standard solution	Merck Millipore (Massachusetts, U.S.A.)	IV
Nitric acid	Sub-boiled
Ultrahigh-purity water	Merck Millipore (Massachusetts, U.S.A.)
Hot plate HP 160 III BM	Sawatec (Sax, Switzerland)		used for wafer preparation
Spin modules SM 180 BM	Sawatec (Sax, Switzerland)		used for wafer preparation
High resolution film photomask	Microlitho (Essex, U.K.)
Step profiler Dektak XT advanced	Bruker  (Massachusetts, U.S.A.)
Hot plate MR 3002	Heidolph (Schwabach, Germany)		used for replica molding
1.5 mm biopsy puncher	Miltex (Pennsylvania, U.S.A.)	33-31AA/33-31A
Spin coater  WS-400 BZ-6NPP/LITE	Laurell (Pennsylvania, U.S.A.)		used for adhesive bonding
Syringe pump neMESYS	Cetoni (Korbussen, Germany)
1 ml syringe	Codan (Lensahn, Germany)	62.1002
5 ml syringe	B. Braun (Melsungen, Germany)	4606051V
PTFE tubing	PKM SA (Lyss, Switzerland)	PTFE-AWG-TFT20.N
Quadrupole-based ICPMS ELAN6000	PerkinElmer (Massachusetts, U.S.A.)
Membrane desolvator CETAC6000AT+	CETAC Technologies (Nebraska, U.S.A.)		only the desolvator unit is used
High speed camera Miro M110	Vision Research (New Jersey, U.S.A.)
Data analysis program Origin pro	OriginLab Corp. (Massachusetts, U.S.A.)	version 8.6
Microscope	Olympus (Tokyo, Japan)	IX71