WO2011023949A2 - Fluidics apparatus and fluipics substrate - Google Patents
Fluidics apparatus and fluipics substrate Download PDFInfo
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- WO2011023949A2 WO2011023949A2 PCT/GB2010/001600 GB2010001600W WO2011023949A2 WO 2011023949 A2 WO2011023949 A2 WO 2011023949A2 GB 2010001600 W GB2010001600 W GB 2010001600W WO 2011023949 A2 WO2011023949 A2 WO 2011023949A2
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- substrate
- droplet
- sample
- surface acoustic
- fluid sample
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- B—PERFORMING OPERATIONS; TRANSPORTING
- B01—PHYSICAL OR CHEMICAL PROCESSES OR APPARATUS IN GENERAL
- B01F—MIXING, e.g. DISSOLVING, EMULSIFYING OR DISPERSING
- B01F31/00—Mixers with shaking, oscillating, or vibrating mechanisms
- B01F31/80—Mixing by means of high-frequency vibrations above one kHz, e.g. ultrasonic vibrations
- B01F31/86—Mixing by means of high-frequency vibrations above one kHz, e.g. ultrasonic vibrations with vibration of the receptacle or part of it
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- B—PERFORMING OPERATIONS; TRANSPORTING
- B01—PHYSICAL OR CHEMICAL PROCESSES OR APPARATUS IN GENERAL
- B01F—MIXING, e.g. DISSOLVING, EMULSIFYING OR DISPERSING
- B01F33/00—Other mixers; Mixing plants; Combinations of mixers
- B01F33/30—Micromixers
- B01F33/302—Micromixers the materials to be mixed flowing in the form of droplets
- B01F33/3021—Micromixers the materials to be mixed flowing in the form of droplets the components to be mixed being combined in a single independent droplet, e.g. these droplets being divided by a non-miscible fluid or consisting of independent droplets
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- B—PERFORMING OPERATIONS; TRANSPORTING
- B01—PHYSICAL OR CHEMICAL PROCESSES OR APPARATUS IN GENERAL
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- B01J19/00—Chemical, physical or physico-chemical processes in general; Their relevant apparatus
- B01J19/0093—Microreactors, e.g. miniaturised or microfabricated reactors
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- B—PERFORMING OPERATIONS; TRANSPORTING
- B01—PHYSICAL OR CHEMICAL PROCESSES OR APPARATUS IN GENERAL
- B01L—CHEMICAL OR PHYSICAL LABORATORY APPARATUS FOR GENERAL USE
- B01L3/00—Containers or dishes for laboratory use, e.g. laboratory glassware; Droppers
- B01L3/50—Containers for the purpose of retaining a material to be analysed, e.g. test tubes
- B01L3/502—Containers for the purpose of retaining a material to be analysed, e.g. test tubes with fluid transport, e.g. in multi-compartment structures
- B01L3/5027—Containers for the purpose of retaining a material to be analysed, e.g. test tubes with fluid transport, e.g. in multi-compartment structures by integrated microfluidic structures, i.e. dimensions of channels and chambers are such that surface tension forces are important, e.g. lab-on-a-chip
- B01L3/502769—Containers for the purpose of retaining a material to be analysed, e.g. test tubes with fluid transport, e.g. in multi-compartment structures by integrated microfluidic structures, i.e. dimensions of channels and chambers are such that surface tension forces are important, e.g. lab-on-a-chip characterised by multiphase flow arrangements
- B01L3/502784—Containers for the purpose of retaining a material to be analysed, e.g. test tubes with fluid transport, e.g. in multi-compartment structures by integrated microfluidic structures, i.e. dimensions of channels and chambers are such that surface tension forces are important, e.g. lab-on-a-chip characterised by multiphase flow arrangements specially adapted for droplet or plug flow, e.g. digital microfluidics
- B01L3/502792—Containers for the purpose of retaining a material to be analysed, e.g. test tubes with fluid transport, e.g. in multi-compartment structures by integrated microfluidic structures, i.e. dimensions of channels and chambers are such that surface tension forces are important, e.g. lab-on-a-chip characterised by multiphase flow arrangements specially adapted for droplet or plug flow, e.g. digital microfluidics for moving individual droplets on a plate, e.g. by locally altering surface tension
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- C—CHEMISTRY; METALLURGY
- C12—BIOCHEMISTRY; BEER; SPIRITS; WINE; VINEGAR; MICROBIOLOGY; ENZYMOLOGY; MUTATION OR GENETIC ENGINEERING
- C12N—MICROORGANISMS OR ENZYMES; COMPOSITIONS THEREOF; PROPAGATING, PRESERVING, OR MAINTAINING MICROORGANISMS; MUTATION OR GENETIC ENGINEERING; CULTURE MEDIA
- C12N13/00—Treatment of microorganisms or enzymes with electrical or wave energy, e.g. magnetism, sonic waves
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- B—PERFORMING OPERATIONS; TRANSPORTING
- B01—PHYSICAL OR CHEMICAL PROCESSES OR APPARATUS IN GENERAL
- B01F—MIXING, e.g. DISSOLVING, EMULSIFYING OR DISPERSING
- B01F2101/00—Mixing characterised by the nature of the mixed materials or by the application field
- B01F2101/44—Mixing of ingredients for microbiology, enzymology, in vitro culture or genetic manipulation
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- B—PERFORMING OPERATIONS; TRANSPORTING
- B01—PHYSICAL OR CHEMICAL PROCESSES OR APPARATUS IN GENERAL
- B01J—CHEMICAL OR PHYSICAL PROCESSES, e.g. CATALYSIS OR COLLOID CHEMISTRY; THEIR RELEVANT APPARATUS
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- B01J2219/00828—Silicon wafers or plates
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- B01J2219/00837—Materials of construction comprising coatings other than catalytically active coatings
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- B—PERFORMING OPERATIONS; TRANSPORTING
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- B—PERFORMING OPERATIONS; TRANSPORTING
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- B01L2200/00—Solutions for specific problems relating to chemical or physical laboratory apparatus
- B01L2200/10—Integrating sample preparation and analysis in single entity, e.g. lab-on-a-chip concept
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- B—PERFORMING OPERATIONS; TRANSPORTING
- B01—PHYSICAL OR CHEMICAL PROCESSES OR APPARATUS IN GENERAL
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- B01L2300/0809—Geometry, shape and general structure rectangular shaped
- B01L2300/0816—Cards, e.g. flat sample carriers usually with flow in two horizontal directions
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- B—PERFORMING OPERATIONS; TRANSPORTING
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- B01L2300/0864—Configuration of multiple channels and/or chambers in a single devices comprising only one inlet and multiple receiving wells, e.g. for separation, splitting
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- B—PERFORMING OPERATIONS; TRANSPORTING
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- B01L2300/08—Geometry, shape and general structure
- B01L2300/0861—Configuration of multiple channels and/or chambers in a single devices
- B01L2300/0867—Multiple inlets and one sample wells, e.g. mixing, dilution
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- B—PERFORMING OPERATIONS; TRANSPORTING
- B01—PHYSICAL OR CHEMICAL PROCESSES OR APPARATUS IN GENERAL
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- B01L2300/08—Geometry, shape and general structure
- B01L2300/089—Virtual walls for guiding liquids
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- B—PERFORMING OPERATIONS; TRANSPORTING
- B01—PHYSICAL OR CHEMICAL PROCESSES OR APPARATUS IN GENERAL
- B01L—CHEMICAL OR PHYSICAL LABORATORY APPARATUS FOR GENERAL USE
- B01L2400/00—Moving or stopping fluids
- B01L2400/04—Moving fluids with specific forces or mechanical means
- B01L2400/0403—Moving fluids with specific forces or mechanical means specific forces
- B01L2400/0433—Moving fluids with specific forces or mechanical means specific forces vibrational forces
- B01L2400/0436—Moving fluids with specific forces or mechanical means specific forces vibrational forces acoustic forces, e.g. surface acoustic waves [SAW]
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- B—PERFORMING OPERATIONS; TRANSPORTING
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- B01L2400/00—Moving or stopping fluids
- B01L2400/04—Moving fluids with specific forces or mechanical means
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- B01L2400/0433—Moving fluids with specific forces or mechanical means specific forces vibrational forces
- B01L2400/0439—Moving fluids with specific forces or mechanical means specific forces vibrational forces ultrasonic vibrations, vibrating piezo elements
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- B—PERFORMING OPERATIONS; TRANSPORTING
- B01—PHYSICAL OR CHEMICAL PROCESSES OR APPARATUS IN GENERAL
- B01L—CHEMICAL OR PHYSICAL LABORATORY APPARATUS FOR GENERAL USE
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- B01L2400/0493—Specific techniques used
- B01L2400/0496—Travelling waves, e.g. in combination with electrical or acoustic forces
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- G—PHYSICS
- G01—MEASURING; TESTING
- G01N—INVESTIGATING OR ANALYSING MATERIALS BY DETERMINING THEIR CHEMICAL OR PHYSICAL PROPERTIES
- G01N33/00—Investigating or analysing materials by specific methods not covered by groups G01N1/00 - G01N31/00
- G01N33/48—Biological material, e.g. blood, urine; Haemocytometers
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- Y—GENERAL TAGGING OF NEW TECHNOLOGICAL DEVELOPMENTS; GENERAL TAGGING OF CROSS-SECTIONAL TECHNOLOGIES SPANNING OVER SEVERAL SECTIONS OF THE IPC; TECHNICAL SUBJECTS COVERED BY FORMER USPC CROSS-REFERENCE ART COLLECTIONS [XRACs] AND DIGESTS
- Y10—TECHNICAL SUBJECTS COVERED BY FORMER USPC
- Y10T—TECHNICAL SUBJECTS COVERED BY FORMER US CLASSIFICATION
- Y10T436/00—Chemistry: analytical and immunological testing
- Y10T436/25—Chemistry: analytical and immunological testing including sample preparation
- Y10T436/25125—Digestion or removing interfering materials
Definitions
- the present invention relates to fluidics apparatus and substrates for fluidics apparatus, and uses of such apparatus and substrates.
- interest is fluid sample manipulation in a microfluidics context.
- the invention has particular, but not exclusive, application to the manipulation of liquid droplets, for example in biological, biochemical, medical, veterinary and chemical assays, analysis, diagnosis, and synthesis and production of reagents and chemicals.
- the present invention further relates to methods for lysing cells and to the use of a fluidics apparatus for lysing cells in a fluid sample.
- WO 2005/100953 discloses a system for measuring viscosity of fluids. Fluids are moved along microfluidic passageways using a thermal pump.
- SAWs Surface acoustic waves
- Rayleigh waves are acoustic waves that can be caused to travel along the surface of a material.
- Surface acoustic waves can be conveniently formed at the surface of a piezoelectric material by the application of a suitable electrical signal to an electrode arrangement at the surface of the piezoelectric material.
- a suitable electrode arrangement utilizes interdigitated electrodes, where a first electrode has an arrangement of parallel electrode fingers having a regular spacing between the fingers.
- a corresponding second electrode of similar shape has fingers which protrude into the gaps between the fingers of the first electrode. The combination of the electrode arrangement and the piezoelectric material forms a transducer.
- SAW transducers are known particularly for use in frequency filters in telecommunications devices such as mobile telephones.
- a filter there is an input transducer and an output transducer.
- the input signal is applied to the input transducer, to form a series of SAWs which propagate to the output transducer.
- the SAWs are converted back into an electrical signal.
- Dogheche et al E. Dogheche, V. Sadaune, X. Lansiaux, D. Remiens, and T. Gryba "Thick LiNbO 3 layers on diamond- coated silicon for surface acoustic wave filters" Applied Physics Letters Vol. 81, No. 7 (12 August 2002) p. 1329] disclose the fabrication of piezoelectric films for SAW filters.
- Such filters are formed using known piezoelectric substrates such as quartz, LiTaO 3 or LiNbO 3 .
- quartz, LiTaO 3 or LiNbO 3 the formation of suitable interdigitated electrode patterns on the surface of such substrates by conventional photolithography whilst providing a filter operable up to suitable telecommunications frequencies is difficult. Accordingly,
- Dogheche et al formed thick (around 1 ⁇ m thick) piezoelectric LiNbO 3 layers on diamond- coated silicon and demonstrated their operation as SAW filters at 293 MHz.
- the transducer was formed with interdigitated electrodes having parallel fingers. Furthermore, Wu et al [Wu, T.T., L. C. Wu, and Z.G. Huang, "Frequency band-gap measurement of two-dimensional air/silicon phononic crystals using layered slanted finger interdigital transducers" Journal of Applied Physics, 2005. 97(9): p. 7] disclose the results of investigations using a similar phononic crystal using electrodes with interdigitated non-parallel fingers in the form of a fan shape.
- phononic crystal is used as an analogy to a "photonic crystal".
- a periodic structure causes reflections due to scattering of incident light, thereby allowing interference between the reflected light and the incident light as it propagates through the "crystal” (which typically is formed of an arrangement of dielectric materials based on a regular array, such as a Bragg reflector), at one or more wavelengths and angles of incidence.
- This interference manifests itself as a prevention of propagation of the light through the crystal at a certain wavelength (or range of wavelengths) and direction.
- a phononic crystal by analogy, has a periodic arrangement of discontinuities or variations in the mechanical properties of the material or materials making up the phononic crystal. Such a phononic crystal can prevent acoustic or mechanical waves of specific wavelength from propagating through the crystal. Since SAWs can be formed at tightly defined frequencies, the effect of phononic crystals on the propagation of SAWs has been studied by several groups.
- Mohammadi et al [Mohammadi, S., et al., "Complete phononic bandgaps and bandgap maps in two-dimensional silicon phononic crystal plates” Electronics Letters, 2007.
- Olsson et al [Olsson, R. H., et al., "Microfabricated VHF acoustic crystals and waveguides" Sensors and Actuators a-Physical, 2008. 145: p. 87-93] disclose the formation of acoustic bandgaps in a structure formed by including periodic arrays of tungsten scatterers in a silica matrix. Waveguides for the acoustic waves are provided by removing selected scatterers along a desired path. Vasseur et al [Vasseur, J. O. et al., 2008. Absolute forbidden bands and waveguiding in two-dimensional phononic crystal plates.
- US 2008/0211602 discloses an acoustic wave device with a piezoelectric layer with transducer electrodes formed over a substrate, there being an omnidirectional acoustic mirror formed between the piezoelectric layer and the substrate.
- Renaudin et al [A. Renaudin, P. Tabourier, V. Zhang, J. C. Camart and C. Druon "SAW nanopump for handling droplets in view of biological applications" Sensors and Actuators B, 113, 2006, p. 389] report on the fabrication and development of a SAW device for microfluidics for biological applications. SAWs at about 20MHz are generated by interdigitated electrode transducers laid on a LiNbO 3 piezoelectric substrate. Droplets are transported along the surface of the transducer where hydrophilic micro tracks are provided between hydrophobic areas. Furthermore, the same research group [Renaudin, A. et al., 2009. Monitoring SAW-actuated microdroplets in view of biological applications. Sensors and Actuators B: Chemical, 138(1), 374-382] set out a method for determining the position of the droplet using echo signals detected by interdigitated transducers.
- concentration via a miniature surface acoustic wave device Lab on a Chip, 2007. 7(5): p. 618-625] disclose the use of SAWs to collect microparticles such as pollen particles in a droplet of water. A water droplet is conveyed along a SAW transducer via a fluidic track.
- Concentration of microparticles in droplets by asymmetric application of surface acoustic waves has also been described.
- Techniques described for breaking the symmetry of a surface acoustic wave involve aligning a drop on the edge of a parallel electrode interdigital transducer [A. Zhang, W. Liu, Z. Jiang and J. Fei, Appl. Acoust., 2009, 70, 1137-1142.], positioning a gel to partially absorb the surface acoustic wave reflection (so that only part of the drop lies in the transmission pathway) [H. Li, J. R. Friend and L. Y. Yeo, Biomed.
- Bennes et al [J. Bennes, S Alzuage, F. Cherioux, S. Ballandras, P. Vairac, J-F Manceau and F. Bastien, "Detection and high-precision positioning of liquid droplets using SAW systems" IEEE Transactions on Ultrasonics Ferroelectrics and Frequency Control, 2007, 54(10): p. 2146-2151] disclose droplet detection and positioning using SAWs.
- the SAW devices used are formed from lithium niobate substrates (LiNbO 3 cut (XY1)/128°).
- Bennes et al explain that the droplets are moved due to the refraction of incoming SAWs along the substrate surface at the air/liquid interface, producing a resultant force which can have a component directed along the substrate surface.
- the LiNbO 3 substrate is treated to make it hydrophobic - this increases the contact angle with an aqueous droplet and decreases the force required to move the droplet by interaction with SAWs.
- WO 02071051 discloses acoustic ejection of biomolecular samples for mass spectrometry.
- WO 2007/128045 discloses the use of a SAW transducer to atomize a liquid droplet from a substrate coupled to a piezoelectric transducer by a fluid coupling layer, thereby forming zeolite nanocrystals.
- Fluidics systems may be useful in the analysis of biological samples, for example in point- of-care diagnostic applications and portable biosensors.
- biological samples present a particular challenge for sample manipulation and analysis in fluidics, particularly microfluidics.
- Preparation of biological samples is often complex, involving multiple steps.
- the molecule of interest may be an intracellular molecule, such that sample preparation requires a cell disruption step in order to render intracellular molecules accessible for analysis and applications such as immunodiagnostics and pathogen detection.
- cell lysis There are a variety of ways to disrupt cells in order to release intracellular molecules for analysis.
- Cells are enclosed by a lipid bilayer called the plasma membrane (also known as the cell membrane, or cytoplasmic membrane), which defines the boundaries of the cell.
- Cell disruption by rupture of the plasma membrane is termed cell lysis, and this can be achieved by a variety of chemical and physical methods.
- a typical chemical lysis procedure involves numerous steps, including the addition of lytic agents (e.g. enzymes, detergents), washing (usually using centrifugation steps), and elution of the processed samples for further analysis.
- Physical lysis procedures include heating and mechanical methods such as agitation with small particles (e.g. glass beads) and sonication (or ultrasonication). Sonication typically involves transmitting mechanical energy, via an immersed probe that oscillates with high frequency, to a solution containing cells in suspension, and resultant cavitation (the creation and collapse of microscopic bubbles) ruptures cells in the sample.
- the present inventors have realised that it is possible to manipulate fluid samples using surface acoustic waves in combination with structures that affect the transmission, distribution and/or behaviour of the surface acoustic waves. This represents one general aspect of the present invention.
- the present invention provides a fluidics apparatus for manipulation of at least one fluid sample, the apparatus including a substrate having a substrate surface with a sample manipulation zone for location of the fluid sample and a transducer arrangement arranged to provide surface acoustic waves at the substrate surface for manipulation of the fluid sample, wherein the substrate surface has an arrangement of surface acoustic wave scattering elements for affecting the transmission, distribution and/or behaviour of surface acoustic waves at the substrate surface.
- the present invention provides a use of a fluidics apparatus to manipulate at least one fluid sample, the apparatus including a substrate having a substrate surface with a sample manipulation zone in which the fluid sample is located and further including a transducer arrangement providing surface acoustic waves at the substrate surface for manipulation of the fluid sample, wherein the substrate surface has an arrangement of surface acoustic wave scattering elements affecting the transmission, distribution and/or behaviour of surface acoustic waves at the substrate surface.
- the present invention provides a fluidics substrate for manipulation of at least one fluid sample, the substrate being couplable with a transducer arrangement for providing surface acoustic waves at a surface of the substrate for manipulation of the fluid sample, wherein the substrate surface has a sample
- the substrate surface further has an arrangement of surface acoustic wave scattering elements for affecting the transmission, distribution and/or behaviour of surface acoustic waves at the substrate surface.
- the fluid sample is in the form of a drop, e.g. a droplet such as a microfluidic droplet.
- a droplet such as a microfluidic droplet.
- other arrangements are possible for the fluid sample, e.g. a channel of fluid, or a fluid held in a chamber.
- the term "droplet" is used, but as discussed above, it is intended that the invention is not necessarily limited to the manipulation of droplets.
- the fluid may comprise a liquid.
- the fluid may comprise one or more particles.
- the fluid may be a liquid containing solid (or substantially solid) particles.
- fluids comprising a suspension of solid particles in a carrier liquid.
- the volume of the fluid sample depends on the application of the apparatus.
- the volume of the fluid sample may be at least 1 picolitre. More preferably, the volume of the fluid sample is at least 10 picolitre, at least 100 picolitre or at least 500 picolitre.
- volume of the fluid sample is about 5 millilitre, more preferably about 1 millilitre, still more preferably about 0.1 millilitre.
- the surface acoustic wave scattering elements have an arrangement based on a periodic arrangement.
- the periodic arrangement may be a one dimensional
- the periodic nature may be, for example, translational symmetry and/or rotational symmetry.
- the term "based on” is used here because it is considered that the arrangement need not be precisely periodic.
- the arrangement may be deliberately displaced from a true periodic arrangement in order to provide a specific effect on the surface acoustic waves.
- the arrangement may be progressively displaced from a true periodic arrangement with distance from a certain starting point in the arrangement.
- the arrangement may include one or more areas or lines of defective periodicity in the periodic arrangement.
- the periodicity can be varied amid a single crystal by use of gradients, over which the pitch and or the size of the elements is varied. This variation in periodicity can have applications in waveguiding or lenses (focusing the acoustic power).
- the periodic arrangement is a two-dimensional pattern, in that the periodicity extends in two dimensions.
- Suitable periodic patterns include translationally symmetrical lattice patterns such as tetragonal, square, trigonal, hexagonal, etc.
- Other suitable periodic patterns include rotationally symmetrical patterns, e.g. having a rotational symmetry of less than 360 degrees.
- the surface acoustic wave scattering elements may be arranged in a scattering zone at the substrate surface.
- the scattering zone may overlap with the sample manipulation zone. However, preferably the scattering zone does not overlap with the sample manipulation zone. It is possible for the scattering zone to be adjacent the sample manipulation zone, in order to affect the surface acoustic wave distribution in the sample manipulation zone.
- the scattering zone may be formed at one or more borders of the substrate surface. In this case, there may be one or more scattering elements located in the sample manipulation zone.
- the scattering zone provides in use a different transmission, distribution and/or behaviour of surface acoustic waves compared with the sample manipulation zone.
- the arrangement of the surface acoustic wave scattering elements preferably provides, in effect, a phononic crystal structure that interacts with or affects the acoustic field, e.g. in the sample manipulation zone.
- the manipulation of the droplet includes movement of the droplet along the sample manipulation zone.
- the sample manipulation zone may define a track for droplet movement.
- the manipulation of the droplet includes atomisation of the droplet from the sample manipulation zone.
- the manipulation of the droplets may include mixing of the droplets.
- Mixing may be achieved by moving the droplets along corresponding tracks to a mixing zone, where the droplets meet and are mixed to form one or more mixed droplets.
- the mixed droplet may then be moved onwardly from the mixing zone along a further track.
- the operation of the apparatus may allow splitting of a droplet into two or more daughter droplets.
- Each daughter droplet may be conveyed onwardly along respective tracks or along the same track.
- the operation of the apparatus may furthermore allow concentration of a species in one or more droplets. This can be achieved, for example, by allowing the SAWs to interact with the droplet to heat the droplet, thereby accelerating the evaporation of solvent.
- the acoustic field may be controlled by an appropriate arrangement of scattering elements and suitable control of the driving signal to the transducers to drive the species preferentially towards one part of the droplet.
- an acoustic cavity can be set up in order to provide a standing wave arrangement, which has been shown to provide particle concentration [Shi, J. et al., 2008. Focusing microparticles in a
- microfluidic channel with standing surface acoustic waves (SSAW). Lab on a Chip, 8(2), 221-223]. Heating without deliberately promoting evaporation is of interest in its own right, e.g. for PCR (polymerase chain reaction) applications for DNA or RNA.
- the operation of the apparatus may also allow concentration of a species in one or more droplets by inducing streaming within the droplet, which streaming concentrates species at a location within the droplet. In the context of the present invention, this type of concentration may be referred to as “centrifugation" (even though it may not represent true centrifugation) since it produces a "pellet"-like deposit of species within the
- the substrate surface includes an
- the droplet may be positioned on the substrate surface at a position relative to the surface acoustic wave scattering elements such that surface acoustic waves are partially scattered by the scattering elements and the droplet receives SAWs distributed asymmetrically with respect to the centre of the droplet footprint.
- the sample manipulation zone may include at least one droplet sensor.
- the droplet sensor may be operable to detect the presence of a droplet.
- One or more droplet sensors may be arranged sequentially in order to detect the presence of a droplet along a track. In this way, the apparatus may be operable to detect the movement of a droplet along a track.
- Droplet sensing can be carried out, for example, using echo location as discussed by Renaudin et al [Renaudin, A. et al., 2009. Monitoring SAW-actuated microdroplets in view of biological applications. Sensors and Actuators B: Chemical, 138(1), 374-382].
- droplet sensing can be carried out using imaging means such as a camera.
- the substrate may have more than one sample manipulation zone.
- a series of sample manipulation zones may be provided, in communication with each other, the droplet being transferred from one sample manipulation zone to the next.
- a first sample manipulation zone may provide droplet movement from a first location to a second location.
- a second sample manipulation zone may provide a mixing stage where the droplet, received from the first sample manipulation zone, is mixed (e.g. with another droplet or simply mixed to mix its own contents), and may provide onwards movement of the mixed droplet.
- a third sample manipulation zone may provide an atomisation stage where the mixed droplet, received from the second sample manipulation zone, is atomised. This atomisation stage may be for analysis of the droplet, e.g. using a mass spectrometer.
- suitable arrangements of scattering elements are provided for each zone, to affect the acoustic field in each zone in a suitable way to promote the required functionality of each zone.
- the transducer can be provided by any means which allows the formation of surface acoustic waves.
- suitable arrangements of optical, electrical or electromagnetic means are contemplated.
- a laser can be controlled to provide fast, localised heating of the substrate, resulting in the formation of
- the transducer comprises a layer of piezoelectric material.
- the layer of piezoelectric material may be a sheet (e.g. a self-supporting sheet) of
- the layer of piezoelectric material may be a single crystal, such as a single crystal wafer.
- a suitable material is LiNbO 3 .
- a preferred orientation for the cut for this material is Y-cut rot. 128°. This has a higher electromechanical coupling coefficient than other orientations.
- Other ferroelectric materials may be used, e.g. PZT, BaTiO 3 , SbTiO 3 or ZnO. Of these, ZnO is attractive because it easily integrated with silicon.
- the piezoelectric layer may be formed by any suitable fabrication technique. For example, the piezoelectric layer may be deposited by printing.
- the transducer preferably further comprises at least one arrangement of electrodes.
- the electrodes may be interdigitated.
- the transducer comprises two or more arrangements of electrodes. These may be disposed in order to provide the specific manipulation desired for the microfluidics droplets, although the arrangement of scattering elements significantly affects the distribution of the acoustic field at the substrate surface. Suitable arrangements are discussed below.
- the transducer is tunable, such that the lateral position of the SAWs emission train is movable. For example, the slanted interdigitated
- the sample manipulation zone is formed at a surface of the transducer, i.e. that the droplet is manipulated on the surface of the, e.g., piezoelectric chip.
- the substrate is separable from the transducer, e.g. as a separate entity that is removably locatable at the transducer.
- the substrate may be in the form of a sheet having a first major surface and a second major surface, preferably formed substantially parallel with each other.
- the first major surface may provide the sample manipulation zone and the border zone.
- the second major surface may provide a coupling surface, for coupling with the transducer in operation. Coupling may be achieved using a coupling medium, preferably a fluid or gel coupling medium.
- the coupling medium may be an aqueous coupling medium, e.g. water.
- the coupling medium may be an organic coupling medium, such as an oil-based coupling medium or glycerol.
- the coupling medium provides intimate contact between the substrate and the transducer and allows the efficient transfer of acoustic energy to the substrate from the transducer.
- Typical SAW transducers are complex to manufacture. For this reason, they are typically expensive. Suitable microfluidic manipulations to be carried out using the transducer may be of the type that will contaminate the transducer if carried out on the transducer surface. Such contamination may be difficult or impossible to remove.
- removal may not be cost-effective, or may damage the transducer.
- the transducer can be re-used. Accordingly, it is preferred that the microfluidic droplet does not contact the transducer but instead contacts the substrate coupled to the transducer.
- the substrate itself may be disposable (e.g. disposed of after a single use).
- One or more suitable sample manipulation zones and one or more border zones may be formed in a substrate by various methods, such as microfabrication, embossing, moulding, spraying, lithographic techniques (e.g.
- the inventors have found, surprisingly, that coupling of SAWs to the substrate from the transducer can be efficient and the SAWs can be controlled at the substrate surface using the interaction between the sample manipulation zones and the scattering zones.
- the first surface of the substrate is substantially planar, excluding the scattering elements.
- the second surface of the substrate need not be planar, and in some circumstances may be formed with a topography that provides additional engineering of the SAWs.
- the second surface may include curved, projecting or recessed regions in order to direct the SAWs.
- suitable droplets for manipulation using the present invention have a volume in the range 0.1-10 ⁇ l_. More preferably, suitable droplets of volume 1-5 ⁇ L are used.
- the sample manipulation zone is in the form of a track, defining the intended path for the droplet.
- the track may be straight, curved, bent, angled, forked, split or joined with another track. It is preferred that the scattering zone is immediately adjacent the track.
- the track may be provided with a hydrophilic surface, typically bordered by one or more hydrophobic areas. In the case of an aqueous sample, this can assist with confining the droplet to the track.
- the dimensions of the track and the relative location of the arrangement of scattering elements causes the track to support only the fundamental mode of the surface acoustic waves at a particular wavelength.
- the surface acoustic wave scattering elements may be elements that provide an interface capable of significant scattering of surface acoustic waves.
- one or more of the scattering elements may be formed by a void at the substrate surface.
- the void may be gas-filled, e.g. air-filled.
- the void may be filled with a different solid or liquid material compared with the material of the remainder of the substrate.
- Filling the void with a contrasting (e.g. mechanically, structurally or functionally contrasting) solid material is desirable, because it allows the substrate to be formed with a smooth surface, therefore allowing the droplet to move across the arrangement of scattering elements if required.
- the contrast in mechanical properties between the substrate and the scattering elements may be changed in use, e.g. by the application of an external stimulus such as heat.
- the scattering elements preferably intersect the surface of the substrate. This is preferred since they are for scattering surface acoustic waves, which are predominantly surface phenomena.
- the scattering elements may extend to a non-zero depth in the substrate. For example, they may extend at least 5% into the thickness of the substrate. They may extend further than this, e.g. at least 10%, at least 20% or more into the thickness of the substrate. In some circumstances, the scattering elements may extend through the entire thickness of the substrate, although a depth of about half of the thickness of the substrate is advantageous.
- the scattering elements may be pits in the substrate. Alternatively, the scattering elements may be pillars upstanding from the substrate surface.
- the scattering elements are cylindrical (e.g. circular or oval cylindrical) in shape, or they may be prismatic or polygonal in shape.
- the scattering elements may be ridges or grooves in the substrate.
- Such shapes may have a straight form, but may alternatively have a curved or angled form.
- the substrate is in monolithic form.
- the scattering elements are formed in the substrate by addition or (more preferably) removal of substrate material from the substrate at the locations of the scattering elements. This may be done, for example, by embossing or etching, powder processing techniques (known in the field of metallurgy), machining (e.g. drilling).
- the scattering elements may be formed at the time of formation of the substrate, e.g. by moulding the substrate to the desired shape, including the scattering elements.
- the scattering elements are placed with respect to the sample manipulation zone, and also with respect to the transducer, in order that there is a different transmission, distribution and/or behaviour of surface acoustic waves in the border region compared with the sample manipulation zone.
- the arrangement of scattering elements it is possible for the arrangement of scattering elements to be such that an incident surface acoustic wave having a predetermined wavelength at a predetermined angle of incidence, is transmitted through the border zone at a significantly lower amplitude than through the sample manipulation zone.
- the incident surface acoustic wave may be substantially prevented from being transmitted through the border zone.
- the border zone acts as a phononic band gap structure to the incident SAWs.
- the effect of this is to concentrate the SAWs in the sample manipulation zone. This can provide very useful effects on the droplet in the sample manipulation zone.
- the scattering elements may have an element-to-element nearest neighbour spacing of at least 10 ⁇ m. This is suitable for SAWs in the MHz region (e.g. of frequency of around 100 MHz). More preferably, this spacing is at least 20 ⁇ m, at least 40 ⁇ m, at least 60 ⁇ m, at least 80 ⁇ m, or at least 100 ⁇ m. This spacing may be at most 5 mm (corresponding to relatively low frequency SAWs), more preferably at most 4 mm, more preferably at most 3 mm, more preferably at most 2 mm, more preferably at most 1 mm, more preferably at most 0.9 mm, at most 0.8 mm, at most 0.7 mm, at most 0.6 mm.
- an element-to-element nearest neighbour spacing in the range 200-500 ⁇ m has been shown to be suitable.
- smaller spacings are contemplated, e.g. in the range down to at least 1 ⁇ m.
- the scattering elements may provide various effects on the SAWs.
- the scattering elements may reflect (or partially reflect) the SAWs, and/or may diffract (or partially diffract) the SAWs, and/or may refract (or partially refract) the SAWs.
- the apparatus includes a signal source for driving the transducer. The signal applied to the transducer affects the SAWs that are produced.
- the transducer may have more than one set of electrodes, being independently controllable.
- the signal applied to each set of electrodes may be varied, in order to provide different manipulation of the droplet. For example, locating sets of electrodes so that SAWs are provided along different directions at the substrate surface may allow vector control of the movement of the droplet.
- the substrate may be treated in order to provide it with a hydrophobic surface.
- a contact angle between a water droplet and a flat region of the substrate surface may be not less than 65 degrees.
- the present inventors have found that it is possible to lyse cells using surface acoustic waves. This represents another general aspect of the invention.
- a method for lysing a cell wherein the cell is comprised in a fluid sample contacting a substrate surface, the method comprising providing surface acoustic waves at the substrate surface, such that the cell lyses.
- a fluidics apparatus for lysing a cell in a fluid sample wherein the fluidics apparatus includes a substrate having a substrate surface for contacting a fluid sample and a transducer arrangement arranged to provide surface acoustic waves at the substrate surface, and wherein said use comprises providing a surface acoustic wave at the substrate surface, such that a cell in a fluid sample contacting the substrate surface lyses.
- SAWs surface acoustic waves tend to at least partially refract into the fluid sample. This refraction is due to the fluid sample having, in general, a different speed of propagation for the SAWs compared with the substrate. This produces streaming in the fluid sample. It is considered that applying SAWs to a substrate surface contacting a fluid sample can create a specific structure of pressure waves and shear stresses in the sample. These pressure waves and shear stresses can mechanically disrupt cells contained in the sample to effect cell lysis. It is considered that, in the preferred embodiments of the present invention, SAW-mediated cell lysis can achieve efficiencies above 95%, which is very favourable compared with known chemical and mechanical methods of cell lysis.
- the fluid sample is a liquid sample containing cells.
- the fluid sample is an aqueous liquid sample containing cells.
- the fluid sample consists of or comprises blood, and therefore contains blood cells.
- the fluid sample is in the form of a drop, e.g. a droplet such as a microfluidic droplet.
- the fluid sample e.g. a channel of fluid, or a fluid held in a chamber.
- the term "droplet" is used, but as discussed above, it is intended that the invention is not necessarily limited to the lysis of cells in droplets.
- the volume of the droplet may be at least 1 picolitre.
- the volume of the droplet may be at least 10 picolitre, at least 100 picolitre or at least 500 picolitre.
- the volume of the droplet may be higher, e.g. at least 1 nanolitre, at least 10 nanolitre, at least 100 nanolitre or at least 500 nanolitre.
- the droplet is larger, e.g. at least 1 microlitre, at least 2 microlitre, at 5 microlitre, at least 10 microlitre, at least 15 microlitre, at least 20 microlitre, at least 25 microlitre or at least 50 microlitre.
- the preferred upper limit for the volume of the droplet is about 5 millilitre, more preferably about 1 millilitre, still more preferably about 0.1 millilitre.
- suitable droplets for cell lysis using the present invention have a volume in the range 0.1-100 microlitre, or 1-50 microlitre. More preferably, suitable droplets of volume 5-25 microlitre are used.
- the volume of the droplet may be adjusted according to the area of contact between the droplet and the substrate surface.
- the volume of the droplet may be adjusted to vary the contact angle (e.g. in the case where the droplet is confined to a particular fluid sample area - see below).
- the contact angle i.e. the included angle between the substrate surface and the tangent to the droplet surface at the substrate, measured in a plane containing the normal to the substrate surface
- the contact angle is 65 - 115 degrees, or more preferably 95 -115 degrees.
- the substrate surface may be provided with a fluid sample area in the form of a fluid sample pinning zone.
- the fluid sample pinning zone is provided in the form of a spot, for pinning a fluid sample droplet to the substrate surface.
- the perimeter of the fluid sample pinning zone may delineate a fluid sample pinning line.
- the fluid sample pinning zone is a hydrophilic area, for pinning an aqueous fluid sample to the substrate surface. More preferably, the fluid sample pinning zone is a hydrophilic area in the form of a spot, for pinning an aqueous droplet to the substrate surface.
- the hydrophilic area may be formed from e.g.
- lithium niobate LiNbO 3
- silicon Si wafer
- zinc oxide ZnO
- silicon oxide Si oxide
- glass or plastics (polymers or copolymers, e.g. with a polyethylene glycol moiety, PEG).
- PEG polyethylene glycol moiety
- These may be further modified using a specific chemical process such as a silanisation (e.g. with aminopropyltriethoxysilane), poly-L- lysine, or PEG or a combination of processes.
- the hydrophilic area may be surrounded by a hydrophobic zone, which may be formed from e.g.
- the fluid sample pinning zone can also be formed by physical structures, for example the pinning zone may be formed as a well in the substrate surface.
- the pinning zone may be formed by a wall or walls that define the perimeter of the pinning zone, which wall or walls may be formed from pillars, or from scattering elements (i.e. elements that contribute to a phononic property of the substrate surface) for example pillars that act as scattering elements.
- the fluid sample pinning zone is not essential for cell lysis, but it may prevent the droplet from moving when surface acoustic waves hit it at high powers and may facilitate adjustment of the area of contact between the fluid sample and the substrate surface in order to vary the contact angle.
- the fluid sample pinning zone preferably has a width or diameter of (or has a width or diameter in the range of up to ) about 1 millimeter, about 2 millimeters, about 3 millimeters, about 4 millimeters, or about 5 millimeters.
- the size (e.g. width, maximum allowed width, or diameter) and/or shape of the fluid sample pinning zone may be varied in order to vary the contact angle and surface tension properties at the fluid sample pinning line for a particular fluid sample volume, and thereby influence the propagation of the pressure wave from the incident SAW through the sample, such that a cell in the fluid sample is lysed.
- the concentration of cells in the fluid sample may be adjusted in order to optimise cell lysis.
- the concentration is about 5 million cells/millilitre or less, about 3 million cells/millilitre or less, about 1 million cells/millilitre or less, about 500,000 cells/millilitre or less, or about 100,000 cells/millilitre or less.
- the fluid sample may consist of or comprise a biological sample such as blood, saliva or urine.
- the fluid sample may be whole blood.
- the fluid sample is diluted blood, for example whole blood diluted in PBS.
- the dilution of the sample expressed as sample:diluent may be about 1 :10 or greater (dilution factor 0.1 or lower), about 1 :25 or greater (dilution factor 0.05 or lower), 1:50 or greater (dilution factor 0.02 or lower), or 1 :100 or greater (dilution factor 0.01 or lower).
- the present inventors have shown that the necessary conditions for cell lysis can be achieved using a variety of different SAW platforms and configurations.
- the present invention thus provides multiple routes to integrate preparation of biological samples in a complete assay on a microchip.
- the present inventors believe that, e.g. by focussing the acoustic power of SAWs at a position within a fluid sample containing cells, it is possible to create acoustic pressure fields and streaming within the sample that lyse the cells.
- surface acoustic waves are provided to the substrate surface contacting a droplet such that rotational streaming is induced in the fluid sample droplet.
- rotational streaming results in the creation of one or more vortexes in the sample, and, under appropriate conditions, the pressures and shear stresses near the centre of a vortex are sufficient to lyse cells.
- Rotational streaming may be induced in the droplet by providing the SAWs to the droplet in an asymmetrical manner in relation to the droplet, that is, providing the SAWs such that it hits the droplet asymmetrically.
- asymmetrical here refers to the distribution of the SAWs with respect to the droplet.
- One example of a suitable asymmetric distribution is provided where the SAW path incompletely overlaps with the footprint of the droplet on the substrate surface, as described below.
- the term SAW "beam” is used herein to define the emission train, or path, of surface acoustic waves provided at a substrate surface.
- the terms SAW beam, SAW emission train and SAW path are used herein interchangeably.
- the width of the SAW beam is notionally defined by the aperture of the transducer that emits the SAW beam.
- the aperture of a transducer is the part of the transducer that resonates to emit a SAW beam.
- the lateral width of an aperture of a transducer is taken to define the lateral width of the SAW beam.
- the aperture is typically the lateral expanse of the region of overlap between the electrode fingers (see w, Fig. 6).
- the edge of the SAW beam is laterally aligned with the edge of the IDT aperture along the direction of propagation of the SAWs. Whilst it is understood that in reality the edge of a SAW beam is not necessarily sharp, as explained below, for the purposes of the present invention, an edge of a SAW beam is defined as a notional longitudinal edge in lateral alignment with an edge of a transducer aperture. It is understood that the amplitude of the SAWs decreases with lateral distance from the edge of the SAW beam.
- rotational streaming may be induced in the droplet by providing a surface acoustic wave at the substrate surface such that the surface acoustic wave path only partially overlaps with the droplet footprint (at least in terms of the position of the notional edge of the SAW path with respect to the droplet).
- a droplet may have an approximately circular footprint, for example, and the surface acoustic wave path may overlap with a segment of the footprint.
- a surface acoustic wave path may overlap with about 10 - 90% of the droplet footprint.
- a surface acoustic wave may be provided at the substrate surface such that the surface acoustic wave path overlaps with about 50% of the droplet footprint, wherein the edge of the surface acoustic wave path passes near the centre of the droplet.
- a surface acoustic wave is provided at the substrate surface by a transducer arrangement (e.g. a parallel electrode interdigital transducer) and the droplet is positioned on the substrate surface at a position relative to the transducer arrangement such that the droplet receives SAWs distributed asymmetrically with respect to the centre of the droplet.
- the droplet may be longitudinally displaced from but laterally aligned with respect to an edge of an aperture of an interdigital transducer (IDT) arrangement, wherein said edge of the aperture defines an edge of a SAWs emission train, such that the droplet is only partly located on the SAWs emission train provided by the IDT arrangement.
- IDT interdigital transducer
- a surface acoustic wave is provided at the substrate surface by a transducer arrangement for which it is possible to control the lateral position of the SAWs emission train with respect to the transducer arrangement, for example by tuning the input frequency.
- the droplet is placed on the substrate surface and the lateral position of the SAWs emission train is tuned to a position on the substrate surface such that the droplet receives SAWs distributed asymmetrically with respect to the centre of the droplet.
- the transducer arrangement may be a slanted IDT (also known as a slanted finger IDT) for which the lateral position of the SAWs emission train can be adjusted by varying the input frequency.
- An advantage of this embodiment is that it does not require precise positioning of the droplet on the substrate surface, since the lateral position of the SAWs emission train on the substrate surface can be adjusted relative to that of the droplet.
- it is more difficult to define a notional edge of the SAWs emission train since the amplitude of the SAWs across the emission train may decrease relatively gradually laterally from a central maximum of the emission train.
- the notional edge of the SAWs emission train can be considered to be the lateral position at full width half maximum of the SAWs amplitude distribution in the lateral direction.
- the substrate surface includes an arrangement of surface acoustic wave scattering elements arranged to scatter surface acoustic waves provided at the substrate surface into a configuration for inducing rotational streaming in the fluid sample.
- the scattering elements may affect the transmission, distribution or behaviour of surface acoustic waves at the substrate surface.
- the droplet may be positioned on the substrate surface at a position relative to the surface acoustic wave scattering elements such that surface acoustic waves are partially scattered by the scattering elements and the droplet receives SAWs distributed asymmetrically with respect to the centre of the droplet.
- the surface acoustic wave induces rotational streaming in order for cell lysis to be achieved.
- the pressure fields necessary for cell lysis may be induced using a wide range of surface acoustic wave geometries, encompassing standing waves as well.
- the inventors believe that it is possible to use surface acoustic waves to lyse cells within a droplet, without necessarily creating rotational streaming or a vortex within the droplet, by focusing acoustic power at a position within the droplet.
- the surface acoustic wave is provided to the droplet asymmetrically in order for rotational streaming to be achieved.
- Cell lysis can be achieved when multiple vortexes are formed in configurations where the SAW hits the droplet in a more symmetrical manner.
- a fluidics apparatus it is possible to design a fluidics apparatus to achieve reproducible multiple vortexes in fluid sample droplets, for example by including arrangements of scattering elements or phononic structures (also known as phononic lattices or phononic crystals) on the substrate surface
- the substrate may be provided with a transducer arrangement
- the transducer can be provided by any means which allows the formation of surface acoustic waves
- suitable arrangements of optical, electrical or electromagnetic means are contemplated
- a laser can be controlled to provide fast, localised heating of the substrate, resulting in the formation of corresponding mechanical waves
- the transducer comprises a layer of piezoelectric material
- the layer of piezoelectric material may be a sheet (e g a self-supporting sheet) of piezoelectric material
- the layer of piezoelectric material may be a single crystal, such as a single crystal wafer
- a suitable material is LiNbO 3
- a preferred orientation for the cut for this material is Y-cut rot 128° This has a higher electromechanical coupling coefficient than other orientations
- Other ferroelectric materials may be used, e g PZT, BaTiO 3 , SbTiO 3 or ZnO Of these, ZnO is attractive because it easily integrated with silicon
- the piezoelectric layer may be formed by any suitable fabrication technique For example, the piezoelectric layer may be deposited by printing
- the transducer preferably further comprises at least one arrangement of electrodes
- the electrodes may be interdigitated
- the transducer may comprise two or more arrangements of electrodes These may be disposed in order to provide specific manipulation desired of microfluidic droplets Suitable arrangements are discussed below
- the transducer is tunable, such that the lateral position of the SAWs emission train is movable
- the arrangement of electrodes is the slanted interdigitated arrangement of electrodes suggested by Wu and Chang [Wu, T & Chang, 1 , 2005 Actuating and detecting of microdroplet using slanted finger interdigital transducers Journal of Applied Physics, 98(2), 024903-7] Slanted interdigitated arrangements of electrodes for use in the present invention are described in more detail below It is possible for the substrate surface to be formed at a surface of the transducer, i.e.
- the droplet is manipulated on the surface of the, e.g., piezoelectric chip.
- the substrate is separable from the transducer, e.g. as a separate entity that is removably locatable at the transducer.
- the substrate may be in the form of a sheet having a first major surface and a second major surface, preferably formed substantially parallel with each other.
- the first major surface may provide a substrate surface for contacting the fluid sample.
- the second major surface may provide a coupling surface, for coupling with the transducer in operation. Coupling may be achieved using a coupling medium, preferably a fluid or gel coupling medium.
- the coupling medium may be an aqueous coupling medium, e.g. water.
- the coupling medium may be an organic coupling medium, such as an oil-based coupling medium or glycerol.
- the coupling medium provides intimate contact between the substrate and the transducer and allows the efficient transfer of acoustic energy to the substrate from the transducer.
- Typical SAW transducers are complex to manufacture. For this reason, they are typically expensive. Suitable microfluidic manipulations to be carried out using the transducer may be of the type that will contaminate the transducer if carried out on the transducer surface. Such contamination may be difficult or impossible to remove.
- removal may not be cost-effective, or may damage the transducer.
- the transducer can be re-used. Accordingly, it is preferred that the microfluidic droplet does not contact the transducer but instead contacts the substrate coupled to the transducer.
- the substrate itself may be disposable (e.g. disposed of after a single use).
- the inventors have found, surprisingly, that coupling of SAWs to the substrate from the transducer can be efficient and the SAWs can be controlled at the substrate surface, for example using scattering elements (e.g. phononic crystals, also known as phononic lattices) or by using a tunable electrode arrangement (.e.g. slanted finger IDT).
- scattering elements e.g. phononic crystals, also known as phononic lattices
- a tunable electrode arrangement e.g. slanted finger IDT
- Disposable substrates are especially useful for the analysis of biological samples.
- Disposable substrates may reduce sample cross contamination in point-of-care diagnostic applications, and may reduce contamination of samples with species that may compromise the molecule of interest (e.g. RNAse, where messenger RNA is the molecule of interest).
- the input power of the surface acoustic wave may between -19 dBm and 0 dBM, between around -14 dBm and around -6 dBmb around -14 dBm or higher, around -12 dBm or higher, around -10 dBm or higher, around - 9 dBm or higher, around -8 dBm, around -7 dBm, or around -6 dBm or higher.
- the related power arriving at the IDT can be obtained using the table below.
- the power arriving at the IDT is calculated by converting the input power value, expressed in dBM, to a value expressed in W and multiplying the W value by 5000 (the amplification by the amplifier).
- a method of lysing cells may comprise providing SAWs to a droplet containing cells, and progressively increasing the input power, and thereby progressively increasing the power of the SAWs, until cell lysis is achieved. This way, for a given set of conditions, cells can be lysed using the minimum power necessary to achieve cell lysis under those conditions. For example, cells of a particular type can be lysed using the minimum power necessary to achieve cell lysis for that cell type.
- the frequency of the surface acoustic wave may be in the range of about 1OkHz to about 1 GHz, preferably about 1 MHz to about 100MHz, more preferably about 5MHz to about 50MHz, more preferably about 5MHz to about 20MHz, more preferably about 15 MHz to about 5 MHz, more preferably between about 13 MHz and about 9 MHz.
- the frequency of the surface acoustic wave may be about 12 MHz, about 11 MHz, about 10 MHz, or about 9 MHz.
- the SAW may be provided at the substrate surface for about 0.1 seconds or longer.
- the SAW may be provided for about 0.1-60 seconds.
- the SAW is provided for about 1 second or less, about 2 seconds or less, or about 3, 4, 5, 6, 7, 8, 9, 10, 15, 20, 25, 30, or 35 seconds or less.
- cell lysis efficiency is affected by several factors, including the surface tension of the droplet, the contact angle of the droplet on the substrate surface, the concentration of cells in the droplet, power of the SAW and the amount of time for which the SAW is provided to the droplet.
- the optimum combination of values for each factor may depend on cell type. The skilled person, by adjusting these variables in combination or in isolation, based on the teaching provided herein, is able to provide conditions in which cell lysis can be achieved.
- a cell is preferably a eukaryotic cell.
- a cell may be an animal cell, for example a mammalian cell (e.g. a blood cell, such as an erythrocyte).
- a cell may be that of a unicellular organism, (e.g. a trypanosome), which may be a protozoan or a protist.
- the cell is a cell of a pathogen, for example a pathogenic protozoan, protist, or bacterium.
- a cell may have a cell wall, or may be wall-less (i.e. without a cell wall).
- a fluid sample may contain a mixture of cells or cell types.
- the present inventors have found that the minimum power sufficient to lyse cells may vary depending on cell type. For example, under particular conditions (e.g. cell concentration, droplet contact angle) a specific power may sufficient to lyse cells of a first type, but insufficient to lyse cells of a second type. Under such conditions, if a SAW of that specific power is applied to a droplet containing a mixture of cells of the first and second type, cell lysis will be achieved for the cells of the first type but not cells of the second type. Accordingly, SAWs may be applied to a fluid sample containing a mixture of cell types in order to differentially lyse cells of different types.
- Different cell “type” may mean different taxonomic groups, for example different domains (eukaryotic cell type is different to prokaryotic cell type), kingdoms (e.g. animal cell type is different from fungal cell type), different physical or physiological types (e.g. a leukocyte is a different cell type from an erythrocyte).
- different cell types are cells that are differentially lysable (e.g. a first cell type is more easily lysed than a second cell type, that is, under a given set of experimental conditions, the lowest power necessary to achieve cell lysis for the first cell type is lower than the lowest power necessary to achieve cell lysis for the second cell type).
- cell lysis is used herein to refer to any type of cell disruption.
- cell lysis is used to refer to cell disruption that results in release of intracellular molecules to the extracellular milieu, for example by rupture of the plasma membrane.
- Cell lysis encompasses rupture of the plasma membrane, and may encompass rupture of intracellular compartment (e.g. organelle) membranes such as the nuclear envelope and mitochondrial outer and inner membranes.
- Cell lysis is typically a complete and irreversible rupture of the plasma membrane, resulting in cell death. In the context of the present invention, however, cell lysis may encompass cell membrane poration, where the plasma membrane is incompletely ruptured (i.e. the plasma membrane temporarily and reversibly ruptures).
- Such poration may improve certain assays such as ELISA, in a similar way to that described in Borthwick et al [Kathryn A. J. Borthwick, Tracey E. Love, Martin B. McDonnell and W. Terence Coakley, Improvement of Immunodetection of Bacterial Spore Antigen by Ultrasonic Cavitation, Anal. Chem. 2005, 77, 7242-7245].
- the term intracellular molecule, or intracellular molecule of interest includes
- intracellular molecule encompasses any molecule having an intracellular moiety of interest (e.g. a transmembrane protein).
- a molecule of interest is compromised if the structure of the molecule becomes significantly different from its native structure or intracellular structure, for example such that the molecule less amenable to analysis (e.g. an epitope required for immunological analysis is no longer present or has become immunologically inaccessible).
- “compromised” as used herein encompasses denaturation (e.g of a protein of interest) and degradation (e.g. hydrolysis of a polynucleotide, polypeptide or polysaccharide of interest).
- Fig. 1 shows a schematic plan view of a substrate for use with the present invention, showing a "funnel" type sample manipulation zone.
- Fig. 2 shows a schematic plan view of another substrate for use with the present invention, showing a "waveguide” type sample manipulation zone.
- Fig. 3 shows a schematic plan view of another substrate for use with the present invention, showing a "combination" type sample manipulation zone
- Figs. 4 and 5 show micrographic images from a video sequence captured on a droplet, viewed from the side, on substrates coupled to a piezoelectric device in the manner described above.
- Fig. 4 shows a droplet on a plain silicon surface without a border zone.
- Fig. 5 shows a droplet on a substrate according to an embodiment of the invention.
- Fig. 6 shows a plan view of an electrode structure for use on a transducer for use with an embodiment of the invention.
- the electrode overlap w is 15 mm
- the finger width for each electrode is 170 ⁇ m
- the finger pitch p is 330 ⁇ m.
- Fig. 7 shows a schematic plan view of a disposable substrate for use with an embodiment of the invention, including typical (but non-limiting) dimensions.
- Fig. 8 provides a surface plot of the acoustic field intensity of a phononic cone structure illustrating the intensity at a first frequency of 11.36 MHz.
- the vertical and horizontal axes together denote position on the substrate surface.
- Fig. 9 provides a surface plot of the acoustic field intensity of a phononic cone structure illustrating the intensity at a first frequency of 11.56 MHz.
- the vertical and horizontal axes together denote position on the substrate surface.
- Figs. 10-13 show a series of consecutive frames from micrographic video footage of an embodiment of the device operating. These images clearly show that acoustic energy is being focused and reflected.
- Fig. 14 shows the dispersion curve for a free plate, with phase velocity as a function of excitation frequency.
- Fig. 15 shows a schematic view of a device according to an embodiment of the invention.
- a separable phononic substrate (or phononic superstrate) in the form of a phononic cone is shown coupled to a lithium niobate substrate which comprises an IDT.
- Fig. 16 shows a schematic view of a device according to an embodiment of the invention.
- a separable phononic substrate (or phononic superstrate) patterned with a phononic lattice in the form of a phononic cone is shown (a) separated from and (b) coupled to a lithium niobate substrate which comprises an IDT. In (c) a sample droplet is located near the apex of the phononic cone.
- Fig. 17 shows (a) a schematic diagram of an embodiment of the device in use; (b) and (c) a series of consecutive micrograph frames from video footage of an embodiment of the device operating; (d) a micrograph of a nebulised droplet; and (e) and (f) simulations of an embodiment of the device operating at two different frequencies, showing that input frequency can be used to excite specific cavities within a phononic cone.
- Fig. 18 shows the size of droplets ejected during nebulisation performed (a) on a phononic substrate coupled to a piezoelectric transducer arrangement, and (b) directly on the surface of the piezoelectric transducer arrangement.
- Fig. 19 shows movement of a droplet between cavities of a phononic cone.
- Fig. 20 shows (a) a schematic view of an embodiment of a device comprising a substrate that includes a phononic lattice in the form of a square, for use in centrifugation of a droplet; (b) a simulation of SAW intensity on the device showing that the phononic lattice interferes with the SAWs; (c) a series of micrographs showing concentration of particles in the centre of a droplet by centrifugation of the droplet on the device; (d) a graph showing that an in increase in power results in a higher local concentration of particles in the centrifuged droplet.
- Fig. 21 shows the band structure of the phononic lattice shown in Fig. 20.
- Fig. 22 shows a series of consecutive micrograph frames from video footage of an embodiment of the device operating to centrifuge blood cells in a droplet of diluted blood.
- Fig. 23 shows (a) a schematic representation of a device including a slanted IDT, for which the lateral position of the SAW emission train is dependent upon the input frequency; and (b) a graph showing the relationship between input frequency and SAW position as calculated theoretically (line) and as determined experimentally on a lithium niobate transducer (horizontally hatched area) and on a separable substrate coverslip (vertically hatched area).
- the inset in Fig. 23(b) shows the magnitude of the S-parameter.
- FIG. 24 shows (a) two micrographs of a droplet containing polystyrene beads before (left image) and after (right image) centrifugation using a slanted IDT device; (b) schematic representation of rotational streaming observed, including a magnified representation of the interaction of the SAWs train with the droplet in which counterclockwise rotational streaming takes place; (c) graph showing relationship between input frequency and time taken to concentrate beads in the centre of the droplet (squares) and estimated area of the interface between the wave and the fluid (curve). Fig.
- FIG. 25 shows, on the left, schematic representations of the interaction between liquid droplets, a substrate and a slanted IDT device and, on the right, micrographic images from a movie at the different stages during a series of fluid manipulations of droplets on the device.
- Three different input frequencies were used to navigate between each manipulation. /3 (11 MHz) moves the left hand droplet to the centre, /4 (9.2 MHz) moves the right hand droplet to merge it and /5 (9.6 MHz) mixes the droplet and concentrates reduced silver in the centre of the droplet.
- Figs. 26, 27 and 28 shows three preferred embodiments of the invention.
- a schematic view of each embodiment is shown at the top of each panel, followed by four consecutive micrographic frames from video recordings of cell lysis.
- a transducer arrangement Near the bottom of each schematic view is shown a transducer arrangement, which is a slanted finger IDT in the case of Fig. 26, and a parallel electrode IDT in the case of Figs. 27 and 28.
- the SAWs emission train is indicated emanating from the transducer arrangement in each case.
- a circular droplet of blood is shown a near the top of each schematic view, and the direction of rotational streaming induced in the droplet by the SAWs is indicated by an arrow.
- the droplet is shown as located on a substrate that is separable from the transducer arrangement.
- Fig. 29 shows cell lysis efficiency of the invention evaluated by (a) reporting the proportion of cells lysed for different cell types, droplet volumes, and sample dilutions (b) reporting the proportion of live (unlysed) cells remaining following treatment using different input powers.
- Fig. 30 shows efficiency of release of intracellular molecules, as determined
- microfluidic technologies can enable the precise control of the delivery of reagents, drugs and metabolites to single cells or to groups of cells. Such methods for can be used for new medicines discovery, or to deliver reagents and samples in diagnostic technologies.
- the present inventors have developed new techniques for droplet manipulation in the microfluidic regime. These techniques are based upon the use of surface acoustic waves (SAWs) generated on a piezoelectric device, such as a device based on lithium niobate, LiNbO 3 .
- SAWs surface acoustic waves
- a Raleigh wave is a coupled compressional-shear system where the longitudinal and the transverse motion are out of phase by 90°.
- the present inventors have demonstrated that it is possible to propagate such longitudinal Raleigh waves (an example of SAWs) from the piezoelectric device, through a coupling medium (which can, for example be water or an oil) into a thin disposable microfluidic chip substrate formed of plastic, glass or other suitable material.
- the waves carry sufficient energy to subsequently drive the fluids on the disposable substrate.
- the LiNbO 3 piezoelectric device is, itself, relatively expensive, in this format it is a re-usable platform, and it is only the substrate that is disposed of after a (typically single) use.
- the only physical contact for actuation of the droplet is through the medium between the LiNbO 3 and the disposable chip.
- a substrate e.g. a thin chip
- Raleigh waves and Lamb waves are types of surface acoustic waves.
- the term surface acoustic wave (SAW) is used herein to describe both Raleigh waves and Lamb waves unless indicated otherwise.
- the functionality of the platform can, however, also be readily extended beyond simple pumping of fluids or droplets.
- microfabricating multiple SAW transducers on the piezoelectric device, and through the subsequent differential actuation of these transducers it is possible to manipulate droplets in a variety of different directions (linear, orthogonal or at any angle between). If necessary, by combining different relative components of wave generation from orthogonal actuators, it is possible to enable splitting and recombination of droplets.
- Fig. 1 shows a schematic example of a substrate in plan view.
- the substrate typically has a length of 20 mm and a width of 14 mm.
- the example of Fig. 1 is a funnel design, in which the sample manipulation zone 10 is bounded by a boundary zone 12.
- the boundary zone includes a phononic bandgap structure of holes formed in the substrate surface.
- the holes are arranged in a two dimensional square lattice pattern.
- each hole has a radius of 176 ⁇ m.
- the spacing between the centres of adjacent holes is 374 ⁇ m.
- Fig. 2 is similar to Fig. 1 , except that the design is a waveguide design.
- Fig. 3 is similar to Fig. 1 , except that the design is a combination design.
- a 4 inch (9 cm) silicon wafer was coated in AZ4562 photoresist and a pattern transferred into the resist using photolithography.
- the pattern consisted of a square array of circular holes arranged to provide a funnel, a waveguide with split or combination of funnel and waveguide, as shown in Figs. 1-3, respectively.
- the photoresist pattern was used as a dry etched mask where the holes were etched to a depth of approximately 230 ⁇ m. This depth equated to half the thickness of the Si wafer.
- the wafer was then cleaned in acetone and then cleaved to provide individual test structures.
- the test structures were cleaned again given an oxygen plasma treatment and then immersed in a solution of heptane and a tri-chloro-tri-deca-fluoro-octylsilane in order to give a hydrophobic surface to the silicon test structures, contact angle >65°.
- the surface acoustic wave source consisted of a 3 inch (6.75 cm) LiNb ⁇ 3 with an interdigitated electrode structure. This is referred to as an interdigitated transducer (IDT).
- IDT interdigitated transducer
- the IDT was resonant at a frequency of 6.18MHz and SAWs at this frequency were used for the tests.
- a programmable signal generator was used to provide an input of 6.18MHz with amplitude of -1OdBm (1 ⁇ W) pulsed at 50Hz to an amplifier with 4OdB gain to present approximately 1OdBm (1W) to the IDT.
- De-ionised water was used as a coupling agent between the silicon test substrates and the lithium niobate wafer; approximately 10 ⁇ l_ was used for this purpose. In order to test mobility and atomisation, the droplet size was about 2 ⁇ l_.
- each of the structures shown in Figs. 1-3 influenced the movement of the water droplets on the silicon surface.
- the structure that appeared to function most efficiently was the funnel (Fig. 1) and this was primarily thought to be due to the relative size of the structure, although the inventors do not wish to be bound by theory in this regard.
- the funnel efficiently moved and focused the drops to the focal point of the funnel irrespective of the initial starting point of the droplet in the sample manipulation zone.
- the test structures were used multiple times their efficacy decreased with usage, as it was difficult to adequately clean dried droplet stains from the exposed silicon surface. This suggests that the substrate should, where possible, should be used only once and then disposed of.
- the waveguide structure (Fig. 2) provided guiding of the water droplets and reduced or eliminated wander of the droplet trajectory on the silicon surface that would be observed without the border zone. No splitting of droplets was observed although movement into either waveguide split was observed.
- the combination structure (Fig. 3) provided focusing of droplets to the waveguide structure and transit along the structure was also observed.
- FIGs. 4 and 5 show micrographic images from a video sequence captured on a droplet, viewed from the side, on substrates coupled to a piezoelectric device in the manner described above.
- Fig. 4 shows a droplet on a plain silicon surface without a border zone.
- Fig. 5 shows a droplet on a substrate according to an embodiment of the invention (i.e. having a border zone with a phononic band gap structure as described above). The image in each case is taken approximately 250 microsecs after the surface acoustic wave meets the droplet. As can be seen, more energy is transferred to the droplet in Fig. 5 than in Fig. 4.
- Each droplet has a volume of 1 ⁇ l_.
- the power used in these experiments was OdBm input which supplied 5W at the IDT.
- the excitation frequency was 9.56MHz.
- the dimensions of the substrates were 2cm by 1.5cm.
- the amount of coupling fluid was reduced to 4 ⁇ L - this provided a layer of approximately 13 ⁇ m thick.
- the substrates were placed in the same position and were of the same thickness (450 ⁇ m).
- a piezoelectric device was fabricated on a 128° Y-cut X-propagating 3 inch (6.75 cm) LiNbO 3 wafer. Transducers were formed on the wafer, each having 20 pairs of electrode “fingers” to form interdigitated transducers (IDT). The electrode "fingers” were located with approximately 330 ⁇ m pitch p, 180 ⁇ m finger width f, with 15 mm aperture w
- the direction of overlap of the fingers can be considered to be a transverse direction of the IDT.
- the electrodes were patterned using a lift off process where after photolithography, using acetate masks, a 20 nm adhesion layer of titanium was deposited prior to 100 nm of gold onto the wafer, lift off was then carried out in a beaker with acetone to produce the IDT electrodes for the SAW device.
- the amplifier was powered by a TTi EX354D Dual Power Supply 280W that could supply 3A and +24V DC. Approximately 1 W of power was applied to the IDT.
- the driving signal for the SAW device was pulsed for 20ms every 100ms, to avoid excess heating. Droplets were imaged at 62 frames per second using a high speed camera (Red Lake M3), which allowed the capture of atomisation from single pulses to be visualized, when the surface acoustic waves travelled through the droplet.
- Fig. 7 shows a schematic plan view of a disposable substrate for use with this embodiment.
- This substrate was constructed using a silicon wafer with a thickness of about 0.5mm.
- the 4 inch Si wafer was coated in AZ4562 photoresist and patterned using photolithography.
- the pattern consisted of a square array of circular holes arranged to provide a funnel or cone of unpatterned silicon (sample manipulation zone).
- the photoresist pattern was then transferred into the silicon using dry etch where the holes were etched to a depth of approximately 0.23 mm.
- the wafer was then cleaned in acetone and then cleaved to provide individual test structures.
- the dimension of the cone patterned substrate was approximately 15 mm by 30 mm.
- the aperture for the cone was 10 mm and the apex was approximately 0.57mm (corresponding to two holes missing).
- De-ionised water was used as a coupling agent between the silicon test structures and the lithium niobate wafer; approximately 10 ⁇ L was used for this purpose, providing a coupling medium layer of less than about 20 ⁇ m between wafer and test substrate.
- two 1 ⁇ l_ drops were used, one at the apex of the cone, the other approximately 10mm away from the apex.
- the phononic structure in the border zone consisted of a square array of holes etched into silicon, to a depth about half way through the wafer. This regular perturbation in the Young's modulus of the material provides the material with a frequency dependent acoustic transmission or reflection property.
- Fig. 8 provides a surface plot of the acoustic field intensity of a phononic cone structure illustrating the intensity at a first frequency of 11.36 MHz.
- Fig. 9 provides a surface plot of the acoustic field intensity of a phononic cone structure illustrating the intensity at a first frequency of 11.56 MHz. These plots together show the effectiveness of the phononic structure to confine the acoustic field depending on the frequency used: a change of 200 KHz from 11.36 MHz to 11.56 MHz can provide a 3dB change in intensity.
- the present inventors aimed to find the resonant frequency of the IDT to obtain the most efficient frequency to atomise the drops from the lithium niobate.
- 12.85MHz was found to be the resonant frequency for the IDT and droplet atomisation from the lithium niobate surface.
- this frequency of operation did not provide suitable operation of the phononic structures in the border zone. It was observed that by reducing the excitation frequency for the IDT down to 12.64MHz a dramatic increase in atomisation was observed on the substrates with phononic structures. The increase in substrate activity was more than enough to compensate for any decrease in IDT acoustic conductance (the amount of electrical power that can be transformed into mechanical power).
- the wavelength of the SAW depends on the pitch of an IDT.
- the observed change in acoustic response of the phononic structure would indicate a change in the wavelength of the SAW and hence variation in the pitch of the intedigitated electrodes.
- This variation was a consequence of using acetate masks for prototyping.
- the masks did posses a variation in the electrode thickness but these variations were thought to be insignificant, which appears not to be the case. So in effect the inventors were using an IDT with a range of pitches allowing a number of possible wavelengths to be radiated.
- the transducer uses a slanted interdigitated electrode structure. This is then used as a tunable source of SAWs. By slanting the electrodes the inter-electrode distance changes with lateral position across the electrode structure. This arrangement can be modelled by an array of IDT's with differing inter electrode spacing. The position of the SAW depends on the excitation frequency used.
- the device of the present embodiment was designed for a certain operating wavelength (frequency) but typically there are always some deviations from the design parameters due to manufacturing tolerances during fabrication. As shown in Figs. 8 and 9, the phononic structures are highly frequency/wavelength dependent. Therefore, by varying the excitation frequency slightly away from the predicted operating frequency, it is possible to tune in to a useful operating regime where the SAW wavelength is shifted enough to allow the device to function substantially as designed.
- Figs. 10-13 show a series of consecutive frames from video footage of an embodiment of the device operating. These images clearly show that acoustic energy is being focused and reflected.
- Figs. 10 -13 two 1 ⁇ l_ droplets have been placed onto the surface of the silicon phononic substrate.
- the first droplet is directly in the path of the second droplet, about 10 mm behind the first droplet.
- the second droplet should in effect "steal" some of the acoustic energy before the acoustic energy can reach the other first droplet. This would be observed, for example, if the droplets were located on the surface of the piezoelectric transducer (and without a border zone). Despite this, atomisation was observed only for the first droplet, at the apex of the phononic cone.
- the length of the substrate in this case was 30mm. The power used in this case was five times lower than in the experiments reported above.
- FIG. 10 shows the first of a series of frames taken from a movie captured at 62 frames per second. This first image is just prior to an ultrasonic SAW pulse arriving at the droplets at about 4000 m/s. Approximately 1 W of power was applied to the IDT.
- Fig. 11 shows the droplets irradiated by the SAWs with the second droplet clearly agitated but not atomising, whereas the first drop near the apex of the cone is atomising (or more correctly nebulising).
- Fig. 12 shows a frame in which the 20ms pulse has stopped but some free oscillation in the drops can be observed. It is interesting to note that the drop that was atomising was in the shadow of the second drop and would normally experience much less acoustic radiation as the second drop would absorb a significant amount of the Rayleigh wave energy. In Fig. 13 the oscillations have stopped and only the plume expelled from the first drop can be seen. This illustrates the efficacy of the device.
- the surface acoustic waves were generated on the piezoelectric LiNb ⁇ 3 wafer by an interdigitated transducer (IDT) and propagated as Rayleigh waves, in a non dispersive manner with a single velocity.
- the resonant frequency, fo is directly related to the Rayleigh wave velocity in the material, c R , (3996 m/s), the SAW wavelength ⁇ and the pitch of the interdigitated electrodes, D 1 as per equation (1): f (1)
- the Rayleigh waves were coupled into a substrate in the form of a sheet, or plate (which substrate sheet or plate may be referred to as a chip), via an intermediate thin film of water.
- the substrate supports a number of propagation modes, termed Lamb waves (named after Lamb, the first to carry out the analysis).
- Lamb waves names of propagation modes, symmetric and antisymmetric, that can be resolved using the Rayleigh-Lamb frequency equations (2) and (3).
- J Va 2 J) 4k PV , symmetric modes (2)
- Fig. 14 shows the dispersion curve for a free plate, with phase velocity as a function of excitation frequency.
- two asymmetric and three symmetric modes can be excited.
- the phase velocities of the lowest order modes A 0 and So are the closest to that of the propagating Rayleigh wave in the substrate sheet (C phase, 3996 m/s), which the inventors worked with, and thus these modes are excited in preference to higher order ones.
- V.(-VP) - 0
- the inventors developed simple phononic structures, where the lattice comprises an array of holes, and where all cases were treated with Neumann boundary conditions. Using these design criteria the inventors produced a series of square lattice 2D phononic crystals, which amplified or shaped the acoustic field, within the substrate sheet. The phononic crystal was used to create acoustic cavities, which were excited at different wavelengths, resulting either in scattering or reflection of the energy. This can focus the energy into specific regions of the chip. As a consequence, the interaction between the Lamb wave and the phononic lattice generates spatial variations of the acoustic field intensity, associated with the different propagation regimes within the chip.
- the Lamb waves propagated in the chip interact with the droplet of liquid placed on its surface in a similar fashion as Rayleigh waves in a piezoelectric material would.
- the interaction with the liquid dampens the surface-propagating wave, which decays as it propagates along the surface. It is then termed a leaky Rayleigh wave and radiates a compressional wave into the liquid, which cannot support shear waves.
- the SAW device was fabricated on a 128° Y-cut X-propagating 3 inch LiNbO 3 wafer, each device consisted of 20 pairs of electrodes to form an inter-digitated transducer (IDT) with pitch of 160 ⁇ m, 80 ⁇ m width, and a 10mm aperture.
- IDT inter-digitated transducer
- the SAW IDTs were patterned using a lift off process where, after pattern transfer into an S 1818 resist, a 20 nm titanium adhesion layer was evaporated prior to deposition of 100nm of gold. Lift-off was then performed in acetone, in order to realise the pattern.
- An Agilent Technologies MXG Analog Signal Generator N5181A was used in conjunction with a Mini Circuits ZHL-5W-1 , 5-500MHz amplifier and a 3A, ⁇ 24V DC power supply to power the SAW device.
- the driving signal for the SAW device was pulsed for 20ms every 100ms, to avoid heating.
- Droplets were imaged at 62 fps using a Red Lake M3 high-speed camera mounted on a Leica upright microscope, which allowed the capture of nebulisation from the droplets to be visualized, when the surface acoustic waves travelled through the droplet.
- the IDT's were characterised using an Agilent Technologies E5071C ENA series network analyser.
- the substrate was fabricated using silicon wafer with an approximate thickness of 470 micrometre.
- the 4 inch Si wafer was coated in AZ4562 photoresist and patterned using standard photolithography.
- the pattern comprised a square array (pitch 203 micrometre) of circular holes (radius 82 micrometre) and was transferred into resist layer.
- the photoresist pattern was then transferred into the silicon using dry etch (STS ICP) where the holes were etched.
- STS ICP dry etch
- the wafer was cleaned in acetone and cleaved to provide the substrates.
- the dimension of the patterned substrate was approximately 20 mm by 30 mm.
- the aperture for the cone was made to be 10mm to coincide with the IDT aperture and the apex of the cone was approximately 1.22 mm wide.
- the same square array of circular holes was used and actuation of the fluid was observed with 10 micrometre polystyrene beads (Duke Scientific G1000)).
- a 5 microlitre volume of de-ionised water was placed between the substrate and the transducer surface to provide a coupling layer approximately 50 micrometre thick to promote SAW coupling.
- a schematic of the device is shown in Fig.
- the phononic crystal comprised holes of 82 micrometre radius with a pitch of 203 micrometre, to provide a fill factor of 0.8, etched into [100] silicon (where structure was aligned to the [011] direction of the silicon wafer, the propagation direction of the Lamb waves was parallel to the [011] direction).
- Fig. 16 provides schematic perspective views of the device.
- Fig. 16a illustrates the transducer arrangement, comprising a lithium niobate wafer and an IDT, on to which a substrate including a phononic lattice (a phononic substrate) is to be placed.
- Fig. 16b shows the phononic substrate on the transducer arrangement.
- Fig. 16c shows the droplet to be manipulated placed onto the phononic substrate.
- the phononic substrate was designed in the form of a phononic cone in order to focus the acoustic energy, as a series of steps (or cavities), with each feature being resonant at a particular frequency, and acting as a Fabry Perot cavity [Qiu C, Liu Z, Mei J, Shi J (2005) Mode-selecting acoustic filter by using resonant tunneling of two-dimensional double phononic crystals. Appl. Phys. Lett. 87:104101-104103; Wu TT 1 Hsu CH 1 Sun JH (2006) Design of a highly magnified directional acoustic source based on the resonant cavity of two-dimensional phononic crystals. Appl. Phys. Lett.
- Fig. 17a shows a schematic drawing of the device, similar to Fig. 16c.
- the droplet is shown placed on the phononic substrate (phononic cone), and the phononic substrate is coupled to the transducer arrangement.
- Six steps, or cavities, of the phononic cone are numbered 1 to 6 in Figs 17 b and c.
- 17d presents a side view captured with a fast camera and shows a picture of the flattened droplet during nebulisation captured at 4 000 frames per second (using a Phantom 7.1 camera, Research Vision, Inc.). The nebulised mist can be seen above the drop.
- Figs 17 e and f show simulations of the phononic cone structure when excited at 12.6 MHz and 13.2 MHz respectively.
- Standing waves develop as a consequence of the sidewalls acting as a series of Fabry Perot etalons.
- the standing waves in the cavities are of up to an order of magnitude larger than the acoustic field on an unmodified substrate (a substrate with no phononic lattice), depending on the frequency.
- Each cavity could be excited at different frequencies, where there was about 300 KHz spacing between each cavity (i.e. between cavities 1 and 2; between cavities 2 and 3, etc).
- the second cavity showed the highest enhancement factor of about 10 at 13.2 MHz whereas the fourth cavity showed an enhancement of about 6 at 12.60 MHz excitation.
- the phononic cone was modelled as a simple 2-D diffraction problem using COMSOL Multiphysics v3.5a.
- the data presented in Figs 17 e and f show that different cavities of the device can be excited at different frequencies.
- the device has been designed so that the phononic structure acts as an efficient reflector and little energy is dissipated into the lattice.
- the simulations also show that the spatial variation in acoustic intensities, as well as the generation of standing waves, were perpendicular to the direction of propagation of the Lamb waves. Changes in frequency of 0.6 MHz can provide significant variations in acoustic field intensity, a fact corroborated experimentally.
- Fig. 17d shows the nebulisation of a 1 microlitre droplet proceeding on the phononic substrate.
- FIG. 18 shows the size of droplets ejected during nebulisation. Nebuisation of water droplets (1-2 microlitres) was performed on the cone phononic substrate coupled to the piezoelectric transducer arrangement (Fig. 18a) or directly on the surface of the piezoelectric transducer arrangement (Fig. 18b) with excitation frequencies around 12 MHz (+/- 1.2 MHz). The size of the droplets ejected was measured with a Phase Doppler Particle Analyser.
- the spatial control of the acoustic energy also enabled the reproducible placement of the drop on the phononic substrate as it aligned itself to the excited cavity when deposited around it, as described further below. Droplet movement and splitting was observed using the device shown in Fig. 17, as described below.
- R is the radius of the drop
- y is the surface tension
- ⁇ a and ⁇ r are the advancing and receding contact angles of the drop when no acoustic wave is applied.
- the spatial variation of the acoustic energy densities results in acoustic forces on the droplet which splits and / or moves of the droplet as it moves towards the cavity with the higher energy.
- droplets will either divide symmetrically or asymmetrically.
- the process of droplet movement or division is driven by refracted waves (one directed) and reflected waves in the opposite direction (back from the phononic cone).
- the mobility of the drop can be improved by reducing the contact angle hysteresis, by making the surface hydrophobic.
- a 5 microlitre water droplet was observed to move back and forth between 3 cavities of a phononic cone treated with a hydrophobic silane.
- Fig. 19 shows the movement of a 5 microlitre water droplet between three cavities of a phononic cone, at different times (a. 0 seconds; b. 0.2 seconds; c.
- transducer arrangement used for droplet nebulisation, splitting or movement, can be used to create an on-chip "centrifuge” (more correctly “separator”, as discussed above, but others in the art use the term “centrifuge”), by using a different substrate, coupled to the transducer arrangement, as described below.
- Fig. 20a The device used for centrifugation of particles within fluid droplets is shown schematically in Fig. 20a.
- the transducer arrangement and substrate were made as described above with reference to Figs 10 - 19, except the phononic lattice was formed as a square, rather than as a cone.
- Fig 20b shows simulation results (Comsol multiphysics 3.5a) where a pressure wave was propagated in the superstrate at 12.6 MHz and has its symmetry broken by the phononic lattice.
- Fig. 21 shows the band gap of the square phononic array.
- the wave propagation was investigated using the two-dimensional plane wave expansion method [Hsu J and Wu T, (2006) Efficient formulation for band-structure calculations of two-dimensional phononic- crystal plates. Phys Rev. B 1 74, 144303].
- this type of reduced wave vector diagram is a convenient way to describe band gaps in symmetrical structures.
- a phononic crystal has a particular symmetry, it is not necessary to consider all the possible propagation directions of a wave in the crystal.
- the reciprocal lattice is the Fourier map of the crystal (or its diffraction pattern), where the wave vector of a wave is the direction of propagation with respect to the reciprocal lattice.
- the hatched area corresponds to the absolute band gap from 7.67 MHz to 14.48 MHz.
- Fig. 20c shows micrographic stills at different time points from a 7 second experiment with 10 micrometre polystyrene beads in a 10 microlitre water droplet, using a power of -8 dBm, ending with the concentration of the beads in the centre of the droplet.
- Fig. 2Od shows the relationship between the increase in concentration (measured as the area covered by the beads at the end of the experiment using pixel counting image software) of
- the inventors observed anti-clockwise streaming with the configuration shown in Fig. 20a (with the phononic filter toward the left of the IDT and the left side of the droplet). However, if the microfluidic chip was turned through 90 degrees relative to the IDT (such that the phononic filter was positioned towards the right of the IDT and the right side of the droplet), then the observed fluid streaming was clockwise in direction.
- Fig. 22 shows stills from an experiment with blood (diluted 1: 50 in PBS) using a power of -7 dBm, at different time points over a 5 second experiment, at the end of which the blood cells can be seen to concentrate in the middle of the 10 microlitre droplet.
- the inventors have demonstrated a new concept in microfluidics showing that complex microfluidic manipulations, including for example the centrifugation of blood, can be performed on a disposable phononic chip.
- the SAW excitation frequency was chosen to couple across the transducer-substrate interface, where droplet manipulation was achieved.
- the phononic structures interact with the acoustic field, providing excellent reflectivity or scattering to the incoming acoustic waves.
- the experiments described herein show how droplet actuation is dependent upon the geometric design and elastic contrast within the phononic crystal, as well as the frequency of the acoustic wave, and how a variety of different fluid motions on a disposable chip can be produced on-chip, including droplet movement, splitting, nebulisation and centrifugation (without the need for electrodes, channels or pumps, for example).
- This flexible and powerful method does not require complex interconnect technologies, nor high voltages (as is the case in many electrokinetic techniques).
- the substrates made according to the preferred embodiments of the invention are very frequency and/or wavelength selective.
- the phononic structures do interact with the acoustic field if working in the correct operating regime providing good reflectivity to the incoming acoustic waves. It has been shown that such structures can be used to engineer the acoustic field to provide enhanced manipulation (such as atomisation) of liquid droplets from the substrate surface.
- Manipulation processes applied to the fluid sample can be one or more of:
- embodiments of the present invention allow sensing of fluid samples (e.g. sensing the location of one or more fluid samples) by considering attenuation of mechanical waves picked up by one or more transducers at the piezoelectric layer.
- the transducer includes a slanted interdigitated arrangement of electrodes, known as a slanted IDT or slanted finger IDT.
- Slanted finger IDTs are used in data terminals as mid-band and wide-band filters.
- the theory of using slanted electrodes in microfluidics has been described [Wu, T. & Chang, I., 2005. Actuating and detecting of microdroplet using slanted finger interdigital transducers.
- slanted IDTs in microfluidics, in particular the use of a slanted IDT in combination with a separable substrate (a substrate sheet, or "superstrate"), as described herein in accordance with certain aspects of the present invention.
- the SAW amplitude excited by a slanted IDT is not uniform and different profiles can be obtained by tuning the input frequency.
- Equation 1 The resonant frequency, f, is dependent upon the pitch of the fingers D, and the sound velocity on the piezoelectric wafer, c (Equation 1 , above, reproduced in slightly different form as Equation 1* below). Consequently, for a given input frequency, the SAW output is only generated when the gap (D/2) between the IDT satisfies the ability of the electrodes to support the resonance.
- Figure 23a shows a schematic representation of the slanted IDT with the propagation of the SAW on a lithium niobate wafer for a selected input frequency of 13 MHz. Only that part of the IDT that supports the resonance condition is excited, resulting in the propagation of a SAW with a smaller aperture, when compared with a parallel electrode IDT. Thus, by tuning the frequency, it was possible to control the lateral position of the excitation wave, as shown theoretically and experimentally in Fig. 23b.
- Fig. 23b shows the experimental input frequency needed to actuate a droplet on the surface of the LiNbO 3 wafer, as well as on a coverslip coupled to the LiNbO 3 wafer, as a function of the position, and the theoretical calculation of the centre of the SAW pathway.
- Results for the lithium niobate wafer are shown using horizontal hatching and results for the coverslip are shown using vertical hatching.
- the theoretical response is shown using a line.
- the inset in Fig. 23b shows the magnitude of the S-parameter obtained with an Agilent Technologies E5071C ENA series network analyzer.
- An Agilent Technologies MXG Analog Signal Generator N5181A was used in conjunction with a Mini Circuits ZHL- 5W-1 , 5-500MHz amplifier and a 3A, 24V DC power supply to power the SAW device.
- the wafer was fixed with thermal paste on a heat sink to avoid overheating.
- the aperture was characterized for each input frequency at a power of -12 dBm, by observing the agitation of an array of 1 microlitre droplets arranged in front of the IDT. The inventors then showed that the same spatial control of the SAW, using the excitation frequency, can be extended to applications involving the use of a separable substrate coupled to the LiNbO 3 wafer.
- the movable lateral position of the SAW beam using the slanted IDT was then used to actuate a microfluidic droplet.
- the inventors demonstrated that a tunable IDT can provide SAWs to a droplet to induce rotational streaming in the droplet, and thereby centrifuge particles in the droplet to concentrate them in the centre of the droplet.
- the concentration of 10 micrometre polystyrene beads was achieved in 10 microlitre water droplets, by locating a droplet a substrate and providing SAWs to the droplet using a slanted IDT and tuning the frequency as shown in Figs 24(a) and 24(b).
- the slanted IDT was fabricated as described above.
- the droplet was placed directly on the lithium niobate wafer, and contained 3 million beads (Duke Scientific G 1000) per millilitre.
- the droplet was positioned 9 mm from the left of the IDT (i.e. 9 mm from the left edge of the IDT as represented schematically in Fig. 24b).
- the input frequency was chosen using the results presented in Fig 23(b) as guide, so that only part of the drop lay in the SAW transmission pathway, thus breaking the symmetry of the acoustic wave.
- Fig 24a is a micrograph of the droplet before (left image) and after (right image) actuation with the SAW. Due to actuation with the SAW (right image) the beads concentrated in the centre of the droplet.
- the direction of the streaming was controlled by tuning the input frequency.
- the SAW excited with a frequency, f ⁇ of 9.6 MHz interacted with the right side of the droplet inducing an angular momentum and created an anti-clockwise streaming.
- a SAW excitation frequency of /2 of 11 MHz the SAW interacted with the left side of the droplet inducing an angular momentum and created a clockwise flow.
- Fig. 24(b) shows schematically the observed anticlockwise and clockwise streaming induced by SAW for f1 approximately 9.6 MHz and f ⁇ approximately 11 MHz, respectively.
- the corresponding streaming direction observed in the droplet 40 is indicated by an arrow.
- the SAW interacts with the right side of the droplet and creates an anti-clockwise streaming
- the SAW interacts with the left side of the droplet and creates a clockwise streaming.
- the overlap area represents the surface of the drop interacting with the SAW
- the inventors investigated the time taken to concentrate a population of polystyrene beads of diameter 10 micrometre in the centre of a 10 microlitre droplet positioned at 9 mm from the left of the IDT directly on the lithium niobate wafer as a function of the input frequency (or the equivalent lateral position of the SAW emission train).
- the range of frequencies over which excitation occurs depends upon the size of the droplet. For example, using the data presented in Fig. 23b for the device described above, it is estimated that for a droplet having a diameter of 3 mm the SAW will interact with the fluid over a range of frequencies between 9 and 11 MHz. This prediction was confirmed by the experimental results presented in Fig. 24c, which show that centrifugation was only observed at frequencies between 9.2 and 11.0 MHz (the shaded/hatched areas represent frequencies at which no centrifugation was observed).
- Fig. 24c is a graph showing the time taken to concentrate 10 micrometre beads in the centre of a 10 microlitre droplet positioned at 9 mm from the left of the IDT as a function of the input frequency (equivalent to the position of the SAW) at - 18 dBm.
- the areas shaded/hatched on the graph represent frequencies for which no concentration of beads was observed.
- the points on the graph show averaged data from three sets of measurements for frequencies between 9.2 MHz to 11.0 MHz with a step of 0.2 MHz, (bars represent the standard deviation from the mean).
- the data were obtained from videos (25 images per second ) analyzed with Time Series Analyzer plug-in in ImageJ software.
- the curve represents the calculated area of the interface between the wave and the fluid, estimated geometrically.
- slanted IDT give the opportunity to programme multiple functions with a single electrode.
- the inventors demonstrated that it is possible to move, merge, mix and centrifuge a droplet on a glass substrate by tuning the frequency of the input signal.
- a system comprising a slanted IDT transducer arrangement coupled to a glass substrate was used.
- the hydrophilic glass substrate 42 coverslip
- hydrophobic dots are not necessarily scattering elements within the meaning of the present invention - they are not used to influence the SAW, but to influence the interaction between the droplet and the substrate surface.
- a droplet 40 of 2 microlitres of hydroxylamine hydrochloride (1.67 mM) and sodium hydroxide (3.33 mM) (pH 9.0) and a droplet of 2 microlitres of silver nitrate (10 mM) were pipetted onto the substrate as shown in Fig. 25a.
- the frequency f3 11 MHz
- -2 dBm the left hand droplet (of silver nitrate) was moved towards the centre of the substrate.
- the right hand droplet (sodium hydroxide and hydroxylamine hydrochloride) was moved towards the centre of the substrate (Fig. 25b), where it merged with the first droplet (starting the reduction of the silver salt to form colloidal silver).
- the frequency /5 (9.6 MHz) was used to apply a SAW asymmetrically to the merged droplet to induce streaming in the droplet, resulting in the mixing of reagents and concentration of the silver colloid in the centre of the droplet. It is possible to integrate the on-chip formation of colloids with both surface enhanced Raman scattering (SERS) and surface enhanced resonance Raman scattering (SERRS) for sensitive bioanalyte detection.
- SERS surface enhanced Raman scattering
- SERRS surface enhanced resonance Raman scattering
- a slanted IDT in which the lateral position of the SAW emission train is dependent upon the input frequency, can be used to design complex fluidic functions directly into a chip.
- the inventors have demonstrated the potential of this powerful tool to manipulate droplets and particles within droplets.
- a clear advantage of this flexible method lies in the ability to induce streaming in a droplet in a chosen direction and at any position.
- known techniques are also restricted to varying the input power to control the concentration of particles, the inventors have demonstrated that it is possible to control the concentration of particles in a droplet by shifting the position of the SAW (i.e. moving the lateral position of the SAW emission train), and hence its region of interaction with the droplet.
- the inventors also demonstrated that complex tasks can be programmed sequentially into a single IDT device, by demonstration that two droplets cab be moved, merged, mixed and centrifuged on a substrate (in this case a disposable glass substrate).
- a substrate in this case a disposable glass substrate.
- the SAW Rayleigh wave which normally propagates in the piezoelectric wafer, can be coupled into a disposable superstrate as a Lamb wave, providing a clear route by which 'lab-on-chip' technology can be applied to low cost, point of care diagnostics.
- the surface acoustic excitation in the piezoelectric wafer is usually coupled into the
- the inventors have now demonstrated a new concept in SAW microfluidics, which combines the use of a separable substrate that is coupled to a transducer arrangement that includes, for example, a slanted finger IDT.
- a disposable glass coverslip was used as the separable substrate.
- the inventors have provided a powerful method by which it is possible to handle droplets and particles in a programmable fashion, and have demonstrated, for example, droplet movement, merging and centrifugation, on the same substrate, with only the need to change the SAW excitation frequency to achieve a high degree of functional integration.
- sample preparation is a key component of "lab-on-chip” systems (LOC). More particularly, cell lysis and blood handling are usually required for a wide range of biological assays in diagnostic applications.
- LOC label-on-chip
- chemical-free mechanical methodologies overcame the limitations of translating traditional procedures, involving lytic agents and subsequent washes, on microfluidic platforms, that arose from the detrimental effects of the chemicals on the molecules to be analysed.
- these new techniques often require external pressure-driven systems that constrain their integration into standalone LOC systems, or the use of high energies (heat, electricity or ultrasonication) that may compromise the molecules.
- the present invention makes use of the acoustic pressure-fields and liquid streaming induced in a droplet by SAW.
- Methods according to the present invention carried out on biological samples resulted in the lysis of above 99.8 % of all cells in the samples.
- the availability of intracellular material in the resulting suspension was studied with optical absorbance measurements and was comparable to a lab-based chemical procedure.
- the present inventors also demonstrated that the necessary conditions for lysis can be achieved using different SAW platforms, providing multiple routes to integrate sample preparation in a complete assay on a microchip.
- the present inventors show for the first time that cells in diluted whole blood can be lysed mechanically in a small droplet in a matter of seconds, using surface acoustic waves as the actuation mechanism.
- Cell lysis using acoustic energy was developed previously using ultrasonication (sometimes called 'sonication') either through harsh cavitation at high energies, or by using beads as crushing support. Proceeding differently here, the present inventors created a specific structure of pressure waves and shear stresses, both red blood cells and white blood cells can be lysed, without cavitation and without the addition of materials to the sample.
- the lysis efficiency of method of the invention was compared to chemical means by measuring the free haemoglobin in suspension, while the number of cells remaining after treatment showed a 95% lysis, comparable to other mechanical solutions.
- lysis was achieved in many configurations of SAW microfluidics (Figs. 26, 27 and 28). Namely, directly on the piezoelectric transducer (Fig. 26), on an unstructured substrate coupled to the piezoelectric transducer and placed strategically to interact with the SAW (Fig. 27), and on a substrate comprising a phononic crystal and coupled to the piezoelectric transducer (Fig. 27).
- the cell lysis method of the invention can be easily integrated with other functionalities in a single SAW system.
- Figs. 26, 27 and 28 show the arrangement of apparatus for use according to three respective preferred embodiments of the invention.
- the top of each figure shows a schematic view of the apparatus arrangement.
- the remainder of each figure includes four images, which are micrographs extracted from video recordings of blood cells being lysed according to an embodiment of the present invention.
- Each image shows a 10 microlitre droplet of diluted blood (whole blood dilulted 50 times in PBS).
- a rotational movement was incurred to the fluid inside the droplet as follows: in the embodiment shown in Fig. 26, using a slanted IDT exited at 11.6 MHz with a power of -9 dBm; in the embodiment shown in Fig.
- the substrates were coupled to the SAW on the piezoelectric transducer by a thin film of deionised water.
- the timescales give an idea of the speed of the lysis, but are not suitable for direct comparison between different apparatus configurations because lysis conditions were not optimised.
- the droplet at the beginning of the experiment (0 s) is about 4 mm in diameter.
- the vortexes used in this study were induced by a concentration streaming in the droplet, achieved when the propagating SAW symmetry was broken. Although it is not shown in the figures, lysis was also obtained when multiple vortexes were formed in other configurations where the SAW hit the droplet in a more symmetrical manner.
- rotational streaming was induced in sample droplets by providing a SAW beam, or SAW emission train, to the droplet asymmetrically.
- the SAW beam provided to the droplet only partially overlapped with the droplet footprint, as shown schematically in Figs 26-28.
- the notional lateral width of the SAW beam, or SAW emission train, emitted by the transducer is determined by the lateral width of the aperture of the transducer (that part of the transducer which resonates and produces SAWs). Whist it is understood that the edge of a SAW beam is not sharp (i.e.
- SAWs may propagate at lateral locations beyond the lateral width of the transducer aperture), as explained below, in the context of the present invention a SAW beam, or SAW emission train, is defined has having a lateral width that corresponds to the lateral width of the transducer aperture.
- this width corresponds to the lateral extent of overlap between electrode fingers (w, Fig. 6).
- this width corresponds to the lateral with of the resonating part of the transducer, considered above in relation to the full width at half maximum of the amplitude distribution laterally across the SAW beam.
- a SAW beam can be understood as overlapping with a droplet footprint when the centre of the beam overlaps with the droplet foot print.
- a SAW beam that partially overlaps with a droplet footprint encompasses the use of a phononic lattice to scatter a SAW beam such that the droplet receives a distribution of SAWs that is asymmetrical with respect to the centre of the droplet.
- the interdigitated transducers were designed to emit SAWs in Y cut Lithium Niobate propagating in the Z direction and therefore the emitted SAW beam should be diffractionless.
- the wavelength of the surface acoustic waves emitted from the IDT's were of the order 400 micrometres where the length of propagation of the SAW prior to irradiating a droplet was never more than 75 wavelengths (near field), implying that diffraction and beam steering losses are not significant even for anisotropic mediums, where the direction of propagation is not along a principle axis. Assuming that the beam amplitude maxima of the emitted SAWs are commensurate with the IDT aperture then a -3dB drop off in power would be observed less than 5
- Fig. 29(a) shows the lysis efficiencies achieved for diluted whole blood sample droplets processed on a slanted IDT, using a range of droplet volumes and dilution factors. Error bars represent the standard deviation over three samples. Results shown in Fig. 29(a) attest the very high rate of cell lysis for most of the conditions tested, above 98 %, and above 99.8 % ( ⁇ 0.4%) for the optimised condition (20 microlitre sample at a power of -9 dBm). This compares well with other non-chemical methods [M. T. Taylor,
- Fig. 29(a) shows that when the blood sample droplet volume was 5 microlitres, if the dilution factor was 1 :50 or 1 :25 then the lysis efficiency was relatively low.
- the lysis efficiency achieved using a 5 microlitre droplet of blood diluted 1 :25 was 45 % (this is not visible in Fig. 29(a) due to the vertical axis scale used).
- the droplet was confined to the hydrophilic spot, its edges pinned to the outline of the spot. It is believed by the inventors that the observed relationship between droplet volume and cell lysis efficiency can be explained by vortex creation in the droplet having a
- HL60 cells a model for chronic myeloid leukaemia
- Trypanosoma cyclops a model for parasite-born infectious diseases such as sleeping sickness
- Fig. 29(b) shows the lysis achieved for a 15 microlitre droplet of a solution containing either 1 million HL60 cells per millilitre in PBS, or 3 million trypanosomes per millilitre in PBS, processed on a slanted IDT for 10 seconds. Results are expressed as a proportion of live cells after processing, expressed relative to an unprocessed control sample (e.g. 100% live cells after processing corresponds to 0% lysis efficiency). The trypanosomes were lysed at lower powers than the mammalian cells. At a power of -14 dBm, cells were concentrated in the centre of the droplet, but there was no significant lysis of HL60 cells and the majority of trypanosomes did not lyse.
- haemoglobin 414 nm and 540 nm
- total DNA 260 nm
- protein contents 280 nm
- Haemoglobin is contained in red blood cells and is the most widely used marker of red blood cell lysis.
- Spectroscopy is used routinely to evaluate haemoglobin levels in plasma as a diagnostic tool for haemolysis.
- Fig. 30(a) shows the levels of haemoglobin in 20 microlitre samples of blood diluted to various ratios with PBS and lysed using SAW on a slanted IDT at -8 dBm (0.8W), relative to samples in which cells were lysed chemically with the detergent Triton X-100.
- PBS blood:PBS + Triton X-100
- the samples lysed with SAW are indistinguishable from chemically lysed samples.
- the lysis efficiency was considerably lower.
- Fig. 30(a) show micrographic images captured during the lysis experiments, where the right insert shows higher blood concentration and cell aggregation (highlighted by ring). By varying the power of the SAW, it is possible to find conditions where the samples are only centrifuged and not lysed.
- Fig. 30(c) shows the levels of haemoglobin in
- the cell lysis method of the present invention can be integrated in to a complex sequence of fluidic manipulation in a biological assay.
- the cell lysis method of the invention can be integrated into a sequence of fluid manipulation steps including steps of moving, mixing, centrifuging, selectively concentrating, fractionating (i.e. selective concentration of species according to their size or mass) and nebulising (atomising) a droplet comprising live intact (unlysed) cells and/or lysed cells.
- a method comprising a series of steps comprising one or more droplet manipulation steps and one or more cell lysis steps may be conveniently performed on a microfluidics apparatus.
- One or more analysis steps may also be included, such as microscopic or spectroscopic analyses.
- a droplet comprising lysed cells, or downstream e.g.
- Analysis steps may include microarray-based analysis, for example of intracellular proteins or nucleic acids released from cells lysed according to the present invention. Analysis steps may include immunological detection steps (e.g. ELISA), gel electrophoresis, electrochemical detection, PCR or other amplification-based techniques. Such analysis may be of particular use in point-of-case diagnostic applications (e.g. to detect an intracellular molecule indicative of a pathogenic cell in the sample) and portable biosensors (e.g. to detect an intracellular molecule indicative of the presence of a biological contaminant or weapon in a sample)
- diagnostic applications e.g. to detect an intracellular molecule indicative of a pathogenic cell in the sample
- portable biosensors e.g. to detect an intracellular molecule indicative of the presence of a biological contaminant or weapon in a sample
- the SAW was propagated on piezoelectric 128° Y-cut X-propagating 3 inch LiNbO 3 wafers. For transmission microscopy, 4 inch double-sided polished wafers were used.
- the devices consisted of 20 pairs of electrodes to form an inter-digitated transducer (IDT) with a pitch of 200 micrometres, 100 micrometres width, and a 10 millimetre aperture, yielding a frequency of ⁇ 10 MHz for the propagating SAW (measured as 9.61 MHz).
- IDT inter-digitated transducer
- the transparent slanted electrode IDT contained 20 pairs of electrodes, with a pitch from 150 micrometres at the highest frequency (about 13 MHz) and 222.5 micrometres at the highest frequency (about 9 MHz) at the lowest, with an aperture of 3 cm.
- the fingers width varied accordingly from 75 micrometres to 111 micrometres.
- the phononic crystal superstrate comprised a square array (pitch 203 micrometres) of circular holes (radius 82 micrometres) in a 470 micrometre-thick silicon wafer that scattered the SAW to obtain an asymmetry in the propagating waves.
- the specific mechanical forces acting on the cells arose from a rotational streaming in the droplet.
- the surface holding the sample droplet was patterned with a hydrophilic spot of 4 mm in diameter, surrounded by a silane (FOTS, Sigma), obtained by immersing the photoresist- patterned (AZ4562) wafer in a 1.6 mM silane solution in heptane (Sigma, H9629) for 10 min and dissolving the resist in acetone.
- This treatment resulted in a contact angle of 107° ⁇ 0.2° (standard deviation) on silicon and 98° ⁇ 1.4° on LiNbO 3 .
- the hydrophilic spot prevents the droplet from moving at higher powers, but is not essential for lysis.
- the temperature of a droplet excited by a SAW can increase drastically, depending on the viscosity of the liquid [J.
- an infrared camera FLIR i60, FLIR Systems
- FLIR i60 FLIR Systems
- lysis was achieved in different configurations, illustrated in Figs. 26-28.
- the IDT was connected to an Agilent Technologies MXG Analog Signal Generator N5181A in conjunction with a Mini Circuits ZHL-5W-1 , 5-500MHz amplifier and a 3A, ⁇ 24V DC power supply.
- the lysis was observed under a stereomicroscope (Leica MZ 12).
- a substrate either unpatterned or with a phononic lattice, that is separable from the piezoelectric wafer was used, it was placed on top of the piezoelectric wafer and coupled with 2-5 microlitres of water in between, yielding water film approximately 50 micrometres thick.
- the wafer was placed in a transparent container for safety concern EDTA-chelated human whole blood (O + ) was obtained from the Glasgow and West of Scotland Blood Transfusion Service and stored at 4 0 C until needed. Samples were discarded after a week.
- HL60 cells ATCC CCL-240, acute promyelocyte leukemia
- Dulbecco's RPMI media supplemented with 10% heat-inactivated fetal calf serum (FCS) and 5% penicillin- streptomycin, at 37°C (5% CO 2 ). Trypanosomes were maintained at 27 0 C in
- Haemoglobin released from the red blood cells was quantified by measuring direct light absorption at 414 nm and 540 nm [E. Eschbach, J. P. Scharsack, U. John, L. K. Medlin, Improved Erythrocyte Lysis Assay in Microtitre Plates for Sensitive Detection and Efficient Measurement of Haemolytic Compounds from lchthyotoxic Algae, J. Appl. Toxicol., 2001 , 21, 513-519].
- a range of blood dilutions was processed on the SAW system.
- Six samples of 20 microlitres of each dilution were lysed at the power specified in the text at -8 dBm (0.8 W) collected (pooled) in an Eppendorf tube and diluted 5 times to fit in the spectrophotometer cuvette (500 microlitres). The extent of lysis was compared to a chemical method.
- the diluted blood samples were mixed (1 :1 v/v) with a solution of 6% (w/w) Triton X-100 (Sigma, T-9284) in PBS and agitated for 5 min. Finally a plasma sample was prepared by centrifuging the blood at 1000 g for 10 min.
- the extent of lysis was also studied by counting the cells remaining intact after the SAW treatment.
- Fig. 29a different volumes of diluted blood were processed on the SAW system with a slanted IDT (11.6 MHz, -9 dBm). After resuspension of the contents of the droplet, 10 microlitres of the solution was harnessed and inserted into a heamocytometer (Neubauer improved). The remaining cells were counted and the extent of lysis reported as a percentage with regards to the cell contents of the original solution. Other types of cells were also lysed and the lysis efficiency studied in a similar fashion (Fig. 29b). HL60 cells at a concentration of 1 million cells/ml in PBS, trypanosomes (cyclops) at a concentration of 3 million/ml. In these experiments, the extent of lysis was evaluated by determining the number of live
- non-lysed cells present at the end of the process and expressing it as a percentage of the number of live cells in an control sample that had not been treated with SAWs.
- the values higher than 100 % live cells for HL60 cells treated using low powers may be explained by sampling variability and/or evaporation of the sample on the chip during treatment concentrating the contents of the SAW-treated droplets.
- Live (unlysed) cells were distinguished from dead (lysed) cells using Trypan blue.
- IDT lnterdigitated transducer also known as an interdigital transducer
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AU2010288268A AU2010288268B2 (en) | 2009-08-24 | 2010-08-24 | Fluidics apparatus and fluidics substrate for surface acoustic wave manipulation of fluid samples |
CN201080048009.XA CN102612405B (en) | 2009-08-24 | 2010-08-24 | For fluidics equipment and the fluidics substrate of the surface acoustic wave process of fluid sample |
CA2771961A CA2771961C (en) | 2009-08-24 | 2010-08-24 | Fluidics apparatus and fluidics substrate |
EP10752900.0A EP2470297B1 (en) | 2009-08-24 | 2010-08-24 | Fluidics apparatus for surface acoustic wave manipulation of fluid samples |
IN2455DEN2012 IN2012DN02455A (en) | 2009-08-24 | 2010-08-24 | |
US13/391,762 US9375690B2 (en) | 2009-08-24 | 2010-08-24 | Fluidics apparatus and fluidics substrate |
US15/167,712 US9751057B2 (en) | 2009-08-24 | 2016-05-27 | Fluidics apparatus and fluidics substrate |
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