Microfluidic Pneumatic Cages: A Novel Approach for In-chip Crystal Trapping, Manipulation and Controlled Chemical Treatment

Note: Two layers of a double-layer microfluidic device are designed using a drawing software, e.g., AutoCAD and printed to form high-resolution film masks, with a feature precision limit of 5 µm. Master molds are created by SU-8 lithography on 4" silicon wafers, allowing the production of structures 50 µm in height.

1. Master Mold Fabrication Using SU-8 Photolithography

1. Place the silicon wafer on a hot plate set at 200 °C for 10 min to dehydrate.
   Note: Silicon wafer dehydration provides a better contact and ensures the spreading of the SU-8 photoresist during the spin coating step.
2. Cool the dehydrated wafer down to room temperature over a period of 3 min.
3. Load the wafer onto a spin coater and deposit 4 ml of SU-8 photoresist (approximately 1 ml of SU-8 per inch of substrate) at the center of the wafer.
   1. First, spread the deposited SU-8 slowly at 500 revolutions per minute (rpm) for 10 sec. Such a rotational speed ensures that SU-8 coverage is increased over the entire wafer surface.
   2. Second, control the thickness of the SU-8 by spinning the substrate at higher speeds. In the current experiments, use a spin speed of 3,000 rpm for 30 sec to generate SU-8 features 50 µm high.
4. Wipe the edge bead of the wafer carefully with a cotton wipe while spinning at a low rpm (typically 100 rpm).
5. Heat the spin-coated wafer on a hot plate at 95 °C for 15 min to remove residual solvent from the SU-8 (i.e., "soft bake").
   Note: The presence of patterns or "wrinkles" in the resist layer indicates the incomplete removal of solvent.
6. Cool the baked wafer back down to room temperature and contact the emulsion printed side of the photomask with the wafer prior to exposure.
7. Turn on the UV-lamp and exposure unit and let the system stabilize over a period of 10 min. Measure the lamp intensity at 365 nm using an UV-optometer, and estimate the required exposure time (according to time = exposure energy/intensity at 365 nm).
   Note: The exposure energy in the current experiments was calculated to be 250 mJ/cm².
8. Expose the photomask on the spin-coated wafer to UV light for the time estimated in the previous step. Here, expose for 79.6 sec.
9. Immediately after exposure, bake the exposed wafer on a hot plate at 65 °C for 1 min and subsequently at 95 °C for 5 min. In this step, the reaction is initiated by UV -light and completed after baking.
10. Leave the post-baked wafer to cool down to room temperature over a period of 3 min.
11. Develop the non-crosslinked SU-8 on the wafer by dissolving it in the SU-8 developer over 8 min. To ensure complete removal of non-crosslinked SU-8, split the process into two steps.
    1. In the first, immerse the wafer in the developer solution for 5 min, removing the majority of non-crosslinked SU-8.
    2. Then immerse the wafer in a fresh solution of developer for 3 min to dissolve the remaining non-crosslinked SU-8 (typically trapped between crosslinked structures).
12. Rinse the developed wafer with isopropanol and let the wafer having patterned structures (hereinafter referred to as "master mold") stand to dry out. Observation of a milky residue upon rinsing the master mold indicates that development is incomplete.
13. Heat the dried master mold on a hot plate at 200 °C for 2-5 min to "hard bake" the substrate and anneal potential cracks in the resist.
14. Allow the fabricated master mold to cool down to room temperature.
15. Place the master mold in a desiccator (connected to a vacuum pump) inside a fume hood.
16. Pour 100 µl of trimethylsilyl chloride (TMCS) into a glass beaker and place this inside the desiccator.
    CAUTION: TMCS is flammable, corrosive and toxic; thus, handling steps should be performed under a fume hood, with the user wearing protective gloves, goggles and a lab coat.
17. Put the desiccator under vacuum and wait at least 1 hr to allow the TMCS vapor to deposit onto the master mold surface.
18. After 1 hr, slowly equilibrate the pressure within desiccator and open to the atmosphere.
    CAUTION: Do not breathe directly above the open desiccator.
19. Remove the silanized master and close the desiccator.

2. Fabrication of Double-layer Microfluidic Devices

Note: The protocol is particularly sensitive to the time and temperature. Any failure to follow to the time frame and temperature may lead to fabrication of non-bonded, and therefore, non-functional devices.

1. Pour a mixture of PDMS elastomer and curing agent (5:1 in weight) into a disposable weighing dish and completely mix with a plastic spatula. In the current experiments, use 50 g of elastomer and 10 g of curing agent to form a PDMS layer approximately 5 mm in height^19,26.
2. Place the well mixed PDMS in a desiccator under vacuum to degas and remove trapped bubbles for 15 min.
3. Mix PDMS elastomer and curing agent (20:1 in weight) in a disposable weighing dish (e.g., 10 g elastomer and 0.5 g curing agent)^19,26.
4. Fix the "control layer" master mold in a frame (in the current experiments, an 11 mm round polytetrafluoroethylene (PTFE) ring).
5. After 15 min, place the 20:1 PDMS mixture in the desiccator under vacuum for degassing.
6. At the same time as the previous step, take out the 5:1 PDMS mixture from the desiccator and pour this onto the "control layer" master mold that is located inside the round frame. Place the frame containing the PDMS and master mold into the desiccator under vacuum as well. Keep the surplus PDMS.
7. After 45 min (and 30 min after putting both PDMS mixtures into the desiccator), take both PDMS mixtures out of the desiccator and place the frame containing 5:1 PDMS and the "control layer" master mold in an oven at 80 °C.
8. At the same time, begin to spin coat the "fluidic layer" master mold with the 20:1 PDMS mixture. The rotational speed for spin coating is determined based on the desired height, and has been reported elsewhere²⁷. Aim to terminate spin coating at 60 min and keep the residual PDMS.
9. After 60 min, put the "fluidic layer" master mold spin coated with 20:1 PDMS into an oven at 80 °C.
10. At 75 min, take both master molds out of the oven.
11. Peel off only the 5:1 PDMS from the "control layer" master mold, dice the substrate with a blade and punch the holes for control layers with a 1 mm biopsy puncher at the inlets positions determined in the design. Here, the control layer is 24 mm in length and 24 mm in width.
12. Remove debris from diced chips using adhesive tape.
13. Manually assemble the diced and punched control layer chips on top of the 20:1 PDMS spin coated on the "fluidic layer" master mold using a stereomicroscope with the magnification of 500X (Figure 1).
14. Pour and draw the residual PDMS around the assembled chips to make a thicker PDMS layer and thereby facilitate removal of the bonded fluidic and control layers at the end.
15. Place the "fluidic layer" master mold containing the two layer devices in an oven at 80 °C and store overnight.
16. The following day, take the cured assembly out of the oven and allow it to cool down to room temperature.
17. Peel off the PDMS assembly from the "fluidic layer" master mold, dice the fabricated double-layer devices with a blade (24 mm in length and 24 mm in width) and punch fluidic inlets/outlets with a 1.5 mm biopsy puncher.
18. Treat the surface of chips with open channels and glass coverslips (24 mm × 40 mm) with a corona discharge and immediately bond them together. Treat by moving the corona discharge over the PDMS slab and glass coverslip over 1 min. Alternatively, use a benchtop plasma system to facilitate bonding.
19. Store the bonded double-layer chips in an oven at 70-80 °C for at least 4 hr.

3. Microfluidic System Assembly

1. After the microfluidic device has been assembled, connect the fluidic layer inlets of the chip to the fluidic reservoirs (syringes) using polytetrafluoroethylene (PTFE) tubing (0.8 mm id).
2. Connect the pressure supply source to the control layer inlets using silicone rubber tubing and metal connectors that have an external diameter of 1.6 mm.
3. Open and close the valves by applying pressurized air at 3 bar using a pressure source which is operated manually. Supply fluids to the channels using a series of computer controlled syringe pumps.
4. Visualize actuation of valves and device operation with a high resolution camera mounted on an inverted microscope. Use 5X to 63X magnification.

4. Manipulation of the Laminar Flow Regime by Pneumatic Cage Actuation

Note: The fluidic layer consists of two inlet converging channels, which are 150 µm in width, to a wider main channel 300 µm in width. And the control layer has a series of identical rectangular valves (250 µm × 200 µm) that are located on top of the main fluidic channel.

1. Once the set-up is connected to the syringe pump and pneumatic controller systems, introduce an aqueous dye flow via one of the inlet channels at the flow rate of 20 µl/min.
2. Close the valve by actuating it at 3 bar.
3. Be aware that the fluid can still flow around the valve. This feature is important in achieving controlled chemical treatment of trapped structures^18,25.
4. Open the valve by releasing the pressure.
5. While the dye solution flows through the first channel, inject another aqueous fluid into the second inlet channel at 20 µl/min. An interface between two aqueous flows is formed due to the laminar flow regime present in the microfluidic device.
6. Close the valve by actuating it at 3 bar. In this case, the actuation of the valve changes the interface of the two aqueous flows; a result that can be used to modify the synthetic pathway during the formation of a CP (vide infra)^18,28.
7. Change the fluid flow rates to 30 µl/min and 10 µl/min and observe the down- or up-shifted guiding of the interface generated between the two fluids.

5. Localization of Microparticles

1. Connect the fabricated double-layer chip to the syringe pump and pneumatic controller systems.
2. Prepare an aqueous solution containing 10 wt.% polystyrene fluorescent particles (5 µm in diameter, excitation and emission max at 468 nm and 508 nm, respectively).
3. Use laser excitation source operating at a wavelength of 488 nm.
4. Introduce the particle-laden fluid into the two inlet channels at a total flow rate of 20 µl/min.
5. Wait for 2 min until a stable flow is established.
6. Actuate the valve at 3 bar to close it. Several particles will be trapped underneath the valve and localized on the surface whilst the flow is maintained.

6. Generation and Controlled Reduction of a Coordination Polymer (CP)

1. Prepare a 2.5 mM aqueous solution of silver nitrate (AgNO₃).
2. Prepare a 2.5 mM aqueous solution of cysteine (Cys).
3. Prepare a saturated ascorbic acid solution in ethanol¹⁸.
4. Use the same double-layer chip and inject the two reagents into the two inlet channels (one reagent per inlet) each at a flow rate of 50 µl/min.
5. Observe the formation of silver and cysteine (Ag(I)Cys) CPs at the interface of two co-flowing steams.
6. Actuate the valve at 3 bar to trap the formed Ag(I)Cys CPs underneath the valve.
7. Flush distilled water into the inlet channels at a flow rate of 50 µl/min to wash away the surplus reagents used during the synthetic process.
8. Release the pressure and open the valve. The generated CPs remain underneath the valve under stopped-flow conditions.
9. In order to conduct a controlled chemical reduction of trapped Ag(I)Cys CPs, release the valve pressure at 1 bar and flush the saturated ascorbic acid solution in ethanol at a flow rate of 10 µl/min.
10. Observe a clear color change that is attributed to the reduction of Ag(I) to metallic silver (Ag(0)) by the ascorbic acid¹⁸.