TREA

Level sense and control system for biofluid drop ejection devices

Follow

Information

  • Patent Grant
  • 6623700
  • Patent Number
    6,623,700
  • Date Filed
    Wednesday, November 22, 2000
    24 years ago
  • Date Issued
    Tuesday, September 23, 2003
    21 years ago
Information
Abstract
A level control mechanism is provided for a biofluid drop ejection device which ejects biofluid drops in small volumes. The biofluid drop device includes a drop ejection mechanism having a transducer which generates energy used to emit the biofluid drops. A reagent cartridge or biofluid holding area holds a biofluid, isolated from the drop ejection mechanism to avoid contamination between the biofluid drop ejection mechanism and the reagent cartridge. The reagent cartridge is connected to the drop ejection mechanism such that upon operation of the mechanism, the biofluid is emitted in controlled biofluid drops. A level sensor is positioned to sense a height of the biofluid within the cartridge. Upon sensing the height of the biofluid below a certain level, an adjustment is made to the height by providing at least one of additional biofluid to the cartridge, and raising the level of the entire reagent cartridge.
Description




BACKGROUND OF THE INVENTION




The present invention is directed to sensing and controlling the level of fluids, and more particularly to sensing and controlling the level of biofluid within drop ejection devices.




Various designs have been proposed for the ejection of biofluids which permit the high-speed printing of sequences and arrays of drops of biofluids to be used in various tests and experiments. In the present discussion, a biofluid, also called a reagent, may be any substance used in a chemical reaction to detect, measure, examine or produce other substances, or is the substance which is to be detected, measured, or examined.




Biofluid ejection devices find particular utility in the depositing of drops on to a substrate in the form of a biological assay. For example, in current biological testing for genetic defects and other biochemical aberrations, thousands of the individual biofluids are placed on a glass substrate at different well-defined locations. Thereafter, additional depositing fluids may be deposited on the same locations. This printed biological assay is then scanned with a laser in order to observe changes in an optical property, such as fluorescence.




It is critical in these situations that the drop ejection device not be a source of contamination or permit unintended cross-contamination between different biofluids.




As these biofluids have a high cost, it is desirable to use only small volumes in the testing operations and to ensure the ejected drops are, in addition to being non-contaminated, fully formed. This requirement raises an issue as to proper level control of the biofluid and priming of ejection devices in order to generate a most efficient and useful drop output.




In view of the foregoing, it has been considered desirable to provide mechanism which ensure the proper delivery of biofluids to an ejector device in a timely, useful manner.




SUMMARY OF THE INVENTION




A level control mechanism is provided for a biofluid drop ejection device which ejects biofluid drops in small volumes. The biofluid drop ejection device includes a drop ejection mechanism having a transducer which generates energy used to emit the biofluid drops. A reagent cartridge or biofluid holding area holds a biofluid, isolated from the drop ejection mechanism to avoid contamination between the biofluid drop ejection mechanism and the reagent cartridge. The reagent cartridge is connected to the drop ejection mechanism such that upon operation of the mechanism, the biofluid is emitted in controlled biofluid drops. A level sensor is positioned to sense a height of the biofluid within the cartridge. Upon sensing the height of the biofluid below a certain level, an adjustment is made to the height by providing at least one of additional biofluid to the cartridge, and raising the level of the entire reagent cartridge.











BRIEF DESCRIPTION OF THE DRAWINGS





FIG. 1

illustrates an acoustic drop ejection unit with which the present invention may be implemented;





FIGS. 2A and 2B

depict fluid levels in a reagent cartridge;





FIG. 3

sets forth a laser biofluid level detection mechanism;





FIGS. 4A and 4B

depict an acoustic beam biofluid level detector configuration;





FIG. 5

illustrates a drop-counting detection mechanism;





FIG. 6

sets forth a first embodiment for movement of a reagent cartridge in a two-piece acoustic drop ejection unit;





FIG. 7

shows a second embodiment of a supplemental supply for a two-piece acoustic drop ejection mechanism;





FIG. 8

sets forth a single piece acoustic drop ejection mechanism within which the concepts of the present invention may be implemented;





FIG. 9

depicts a first embodiment for supplying additional biofluid in a single-piece system;





FIG. 10

sets forth a second embodiment for a one-piece acoustic drop ejection mechanism;





FIG. 11

depicts a second embodiment for a single-piece acoustic drop ejection mechanism;





FIG. 12

illustrates a single piece piezo-electric drop ejection mechanism having a secondary biofluid holding region;





FIG. 13

depicts a two-piece piezo-electric drop ejection mechanism having a secondary biofluid holding region;





FIG. 14

sets forth a priming configuration for a piezo-electric drop ejection mechanism; and





FIG. 15

illustrates a modified single piece piezoelectric drop ejection mechanism incorporating a priming reservoir.











DETAILED DESCRIPTION OF PREFERRED EMBODIMENTS





FIG. 1

is a cross-sectional view of an acoustic drop ejection unit


10


, having a reagent cartridge


12


inserted within an acoustic drop ejection mechanism


14


. A transducer


16


is supplied with energy by a power supply source


18


. Transducer


16


is provided on a surface of substrate


20


, such as glass. Patterned or located on an opposite surface of glass substrate


20


is a focusing lens configuration


22


, such as a Fresnel lens. It is to be appreciated that other types of focusing configurations may also be used in place of Fresnel lens


22


.




A connecting layer


24


, such as an acoustic coupling fluid is located between Fresnel lens


22


and reagent cartridge


12


. The acoustic coupling fluid


24


is selected to have low acoustic attenuation. An example of an acoustic coupling fluid having beneficial acoustic characteristics for this application include water. In an alternative embodiment connecting layer


24


may be provided as a thin layer of grease. The grease connection will be useful when the joining surfaces are relatively flat in order to minimize the possibility of trapped bubbles.




On top of glass substrate


20


are walls


26


,


28


which define interior chamber


30


within which reagent cartridge


12


is located. Side wall


31


of cartridge


12


includes a seal


32


extending from its outer surface. Seal


32


secures cartridge


12


within chamber


30


and maintains acoustic coupling fluid


24


below seal


32


. A precision depth stop


34


holds cartridge


12


at a desired insertion location. A thin membrane


36


is formed on a lower surface


37


of cartridge


12


, positioned substantially above Fresnel lens


22


. Membrane


36


is an acoustically thin membrane, wherein acoustically thin is defined in this context to mean that the thickness of the membrane is small enough that it passes over 50% of its incident acoustic energy through to biofluid


38


within cartridge


12


.




In operation, energization of transducer


16


emits an acoustic wave which travels through glass substrate


20


to Fresnel lens


22


. The lens produces a focused acoustic energy wave


39


that passes through acoustic coupling fluid


24


and membrane


36


, reaching an apex at biofluid meniscus surface


40


of biofluid


38


. Supplying of the focused energy to surface


40


causes disruptions in the surface resulting in ejection of a biofluid drop


42


from cartridge


12


to substrate


43


, such as paper, glass, plastic or other appropriate material. The biofluid ejected can be as small as approximately 15 μm in diameter. However, this size limitation is based on the physical components used, and it is to be understood that drops ejected by an acoustic drop ejection unit can be made smaller or larger in accordance with design changes to the physical components.




The surface from which biofluid drops


42


are ejected can be either totally open or contained by an aperture plate or lid


44


. The lid


44


will have a suitably sized aperture


45


, which is larger than the ejected drop size in order to avoid any interference with drop ejection. Aperture


45


must be sized so that the surface tension of meniscus


40


across aperture


45


sufficiently exceeds the gravitational force on biofluid


38


. This design will prevent biofluid


38


from falling from regent cartridge


12


when cartridge


12


is turned with aperture


45


facing down. The aperture down configuration has a benefit of maintaining the biofluid


38


clean from material which may fall from substrate


43


.




Operation of transducer


16


, power supply


18


, glass substrate


20


, and lens


22


function in a manner similar to previously discussed drop ejection units used in the field of acoustic ink printing. Such operation is well known in the art.




The foregoing design isolates biofluid


38


within reagent cartridge


12


, preventing it from coming into contact with drop ejection mechanism


14


, or other potential sources of contamination, such as airborne contamination or contamination from biofluids previously used with the ejection mechanism. Reagent cartridge


12


is separated from acoustic coupling fluid


24


by membrane


36


. The entire cartridge may be injection molded from a biologically inert material, such as polyethylene or polypropylene. Cartridge


12


is operationally linked to the acoustic drop emitter mechanism


14


by a connection interface which includes membrane


36


and acoustic coupling fluid


24


.




In a specific design of the present invention, the width of reagent cartridge


12


may be approximately 300 microns, and membrane


36


may be 3 microns thick. In this particular embodiment, with a design constraint of a focal acoustic wave length being 300 microns and at an operating frequency of known acoustic drop ejection mechanisms, the meniscus location should be maintained within plus or minus five microns from an ideal surface level.




Power supply source


18


is a controllably variable. By altering the output of power supply source


18


, energy generated by transducer


16


is adjusted, which in turn may be used to alter the volume of an emitted biofluid drop


42


.




As previously discussed, for proper operation of the acoustic drop ejection device


10


, the location of the meniscus surface


40


must be maintained within tolerances defined by the device configuration. While in the previously discussed embodiment, due to the specific acoustic drop ejection mechanism being used, that tolerance is +/−5 microns. It is to be appreciated other ranges exist for differently configured devices.




The concept of maintaining biofluid levels of a reagent cartridge


12


within a set level of parameters is illustrated by

FIGS. 2A and 2B

. For example,

FIG. 2A

shows reagent cartridge


12


when it is full of biofluid


38


. In

FIG. 2B

the same cartridge


12


is shown in an empty state. It is to be appreciated that empty in this embodiment refers to there being less biofluid


38


than the predetermined parameter height


46


, in this instance


10


microns. Thus, there is still biofluid within cartridge


12


. However, due to the operational characteristics of acoustic drop ejection unit


10


, once biofluid


38


is outside of the predetermined level


46


biofluid drops cannot be reliably ejected. This situation exists since the apex of acoustic wave


39


is not occurring at surface


40


of biofluid


38


, and sufficient energy is not transferred to disturb the surface to the degree that a drop will be ejected at this lower level.




Thus, for useful operation of biofluid drop ejection unit


10


, it is desirable to provide a configuration which detects the biofluid level while the cartridge


12


is within acoustic drop mechanism


14


.




Turning to

FIG. 3

, illustrated is a first embodiment of a biofluid level detection mechanism


50


which is capable of measuring the level of biofluid


38


within cartridge


12


, when cartridge is within ejector mechanism


14


.




As biofluid drops are ejected from cartridge


12


, the level of biofluid


38


will change. Biofluid level detection mechanism


50


includes a laser


52


positioned such that laser beam


54


emitted therefrom is reflected off of the upper surface


56


of biofluid


38


. A laser detection configuration


58


includes a first laser beam detector


60


and a second laser beam detector


62


. First laser beam detector


60


is positioned at an angle relative to the acoustic drop ejection unit


10


such that when cartridge


12


has biofluid within the predetermined parameters, the angle of reflected laser beam


64


will impinge upon sensor


60


. Laser beam detector


62


is positioned at an angle relative to acoustic drop ejection unit


10


such that it will sense reflected laser beam


66


which is at an angle corresponding to the biofluid


38


being out of the acceptable range for proper operation.




The outputs of sensor detector


60


and sensor detector


62


are provided to a controller


68


. This information, along with preprogrammed information as to location of the laser


52


and detectors


60


,


62


, is used to calculate the biofluid level. The information obtained by controller


68


may then be used in further control of the biofluid level, as will be discussed in greater detail below.




Turning to

FIGS. 4A and 4B

, set forth is a second embodiment for level sensing in accordance with the present invention. Particularly, controller


70


controls the output of power supply


72


to initiate a short pulse acoustic wave


76


to be transmitted from Fresnel lens


78


to the upper surface


80


of biofluid


38


. Controller


70


controls the output from power supply


72


such that short pulse acoustic wave


76


is not sufficient to cause the emission or ejection of a biofluid drop. Rather, short pulse acoustic wave


76


is emitted, and sensed by lens


22


. This outbound acoustic wave


76


, as shown in

FIG. 4A

reaches surface


80


and is then reflected back


84


towards lens


22


, generating an rf signal provided to controller


70


with an indication of the emission and return of acoustic wave


76


.




The time taken for acoustic wave


76


to travel to surface


80


and back to lens


22


is used to determine whether the biofluid is at an appropriate level. This information will be used to adjust the fluid level, as will be discussed in further detail below. In an alternative embodiment, it is possible to vary the supplied frequency to shift the focus, in order to maintain the acoustic wave at the meniscus surface.




Controller


70


is designed to determine the time from emission of the outbound acoustic wave


76


until receipt of the reflected wave


84


having been preprogrammed with parameters as to the speed of the acoustic wave, the depth of the biofluid in cartridge


12


when full, the viscosity of the biofluid as well as other required parameters. Using this information controller


70


calculates the biofluid level within cartridge


12


. This information is then used in later level control designs which will be discussed in greater detail below.




In an alternative embodiment controller


70


may be designed to sense an amplitude of the returned wave. The sensed amplitude is correlated to the biofluid level. Particularly, the returned signal of acoustic wave


76


will carry with it amplitude information. If the fluid height is not at an appropriate level, either too high or too low, the amplitude will be lower than expected. The returned amplitude will be at a peak when the fluid is at a correct level for ejector operation. Therefore, to determine the proper level the volume of biofluid is altered and a measurement is made to determine if the returned amplitude is closer or further from maximum amplitude. Dependent upon whether fluid was added or removed and the reaction of the amplitude, it can be determined whether more or less biofluid is needed.




Turning to

FIG. 5

, illustrated is a further embodiment of biofluid level detection in accordance with the present invention. Sound pulses emitted by lens


22


are supplied to controller


88


. The controller


88


is configured to accumulate and count the pulses received, and to correlate that value to the known average volume of biofluid ejected in each drop. Controller


88


then inferentially calculates the level of biofluid


38


within cartridge


12


. This biofluid level information is then used to control the biofluid level.




It is to be appreciated that while alternative embodiments for biofluid level detection in cartridge


12


, have been disclosed in connection with

FIGS. 3

,


4


A,


4


B and


5


, other configurations may also be implemented.




As previously mentioned, by altering the frequency of operation it is possible, using a Fresnel lens design, to alter the amplitude of the emitted acoustic wave. Using this capability the peak of the emitted acoustic wave is controllable. Therefore, as biofluid is emitted, but still within an acceptable range, the amplitude may be adjusted to properly sense the new surface level. By this design additional biofluid does not need to be added until a lower surface level is sensed.




Turning to

FIG. 6

, illustrated is a first embodiment for altering the position of the reagent cartridge


12


located within the acoustic drop ejection mechanism


14


. The position change is made in response to the detection of biofluid levels by techniques shown, for example, in connection with

FIGS. 3

,


4


A,


4


B or


5


.




When the level of biofluid is determined to be out of a desired range, an adjustment to the level of the reagent cartridge


12


is undertaken. Particularly, provided is an auxiliary fluid chamber


90


placed in operational communication with chamber


30


via chamber connect


92


. When it is determined the biofluid level is out of an acceptable range, additional acoustic connection fluid


94


is supplied to chamber


30


by activation of plunger


96


. Plunger


96


may be a high-precision plunger controlled by a computer-driven actuator


98


. Computer-driven actuator


98


is provided with signals via any one of the controllers


68


,


70


or


88


previously discussed in connection with

FIGS. 3

,


4


A,


4


B and


5


. Plunger


96


is moved inward forcing supplementing acoustic connection fluid


94


into chamber


30


to raise reagent cartridge


12


to a sufficient amount to ensure that surface


80


is within the acceptable height range.





FIG. 7

is a side view of a two piece drop ejection unit


100


employing an alternative reagent cartridge


102


configuration. In addition to ejection reservoir


104


which holds biofluid


38


, a main reservoir


106


is also provided to feed ejection reservoir


104


. A connection path between the ejection reservoir


104


and main reservoir


106


is provided via reservoir connect


108


. In this design, as biofluid


38


is ejected from ejection reservoir


104


, additional biofluid


38


is supplied via the main reservoir


106


and reservoir connect


108


.




Reagent cartridge


102


is in operational arrangement with acoustic drop ejection mechanism


110


. Ejection reservoir


104


is located over lens


22


, glass substrate


20


, and transducer


16


in a manner which allows generated acoustic energy to be focused, and transferred to the ejection reservoir


104


with sufficient energy to emit biofluid drops. In implementing this two piece design connecting layer


24


, such as an acoustic coupling fluid is provided, and a bottom portion of cartridge


102


is formed with membrane


112


which allows sufficient acoustic energy to be transferred to ejection reservoir


104


.




Main reservoir


106


is filled through filling port


114


. The main reservoir


106


and reservoir connect


108


use capillary action to assist in an initial filling oft he ejection reservoir


104


when it is in an empty state. Thereafter, as drops are ejected from ejection reservoir


104


surface tension causes biofluid from the main reservoir to be drawn into the ejection reservoir. Particularly, aperture


45


of ejection reservoir


104


is sufficiently sized smaller than filling port


114


of main reservoir


106


and also small enough to overcome gravitational forces due to reservoir height, that biofluid in main reservoir


106


is drawn into the ejection reservoir


104


.




Turning to

FIG. 8

, set forth is a single piece biofluid acoustic ejection unit


120


. Distinctions between the two-piece biofluid drop ejection unit


10


and the single-piece unit


120


, include that seal


32


of reagent cartridge


12


is no longer used. Rather, reagent cartridge


122


has side wall


124


with a planar external surface


126


in direct contact with walls


26


,


28


of mechanism


14


. Therefore, a permanent connection is made between walls


26


,


28


and reagent cartridge


122


. Such connection may be made during the manufacture of the device via lithographic techniques and/or by use of known adhesion technology.




In a further embodiment, lower surface


128


, including membrane


130


, may be removed allowing biofluid


38


to come into direct contact with lens


22


. Still a further embodiment is to remove cartridge


112


and supply the biofluid directly into chamber


30


, where chamber


30


acts as a non-contaminated biofluid containment area. Under this design chamber


30


is filled with biofluid in a contamination-free environment.





FIG. 9

shows an embodiment for supplying additional biofluid to reagent cartridge


140


in order to maintain the biofluid


38


at a desired level. In this embodiment auxiliary fluid holding area


142


has a bellows-shaped configuration with an interior


144


filled with biofluid


38


.




Upon receipt of a signal from a level-sensing device (e.g.

FIGS. 3

,


4


A,


4


B and


5


) indicating biofluid within ejection reservoir


146


is below a desired level, precision plunger


148


, controlled by computer operated actuator


150


, is moved inward compressing auxiliary biofluid holding chamber


142


. This action forces a predetermined amount of biofluid


38


into main chamber


146


such that biofluid meniscus surface


152


is moved to an acceptable, usable level.





FIG. 10

depicts a second embodiment for supplying additional biofluid


38


to reagent chamber


160


. In this instance, collapsible auxiliary area or chamber


162


is in fluid communication with ejection reservoir


164


. Upon receiving a level signal indicating the level of biofluid


38


is required to be replenished, squeezing mechanism


166


is activated by a computer-controlled actuator


168


to provide inward force on collapsible chamber


162


. Pressure is applied in a sufficient amount to resupply ejection reservoir


164


with biofluid, to an acceptable usable level.




Turning to

FIG. 11

, illustrated is an alternative embodiment for a single piece acoustic drop ejection unit


170


. In this figure, ejection reservoir


172


and main reservoir


174


are placed in fluid communication by reservoir connect


176


. Biofluid


38


is supplied from main reservoir


174


to ejection reservoir


172


due to surface tension at the meniscus, as discussed in connection with FIG.


7


. Transducer


16


is in operational connection to substrate


178


on a first surface


180


, and lens


22


is on a second surface


182


whereby these components are formed as part of the single unit


170


. In this embodiment, connecting layer


24


of

FIG. 7

is not required due to the single component disposable nature of the present embodiment. In ejection reservoir


172


, biofluid comes into direct contact with lens


22


. Therefore, there is no need for the acoustic coupling fluid provided in FIG.


7


. Main reservoir


174


is filled through filling port


183


.





FIG. 12

is a side view of a single piece piezoelectric drop ejection unit


190


. Ejection reservoir


192


is connected to main reservoir


194


via reservoir connect


196


. Biofluid is supplied to main reservoir


194


via filling port


198


. A piezo actuator


200


is in operational attachment to a lower surface


202


of ejection reservoir


192


. An upper surface defining the ejection reservoir


192


has formed therein an ejection nozzle


204


.




In operation piezo actuator


200


is actuated by power supply


210


, which in combination with lower surface


202


, define a unimorph, and deflects in response to an applied voltage. In this instance a force is imposed such that the unimorph configuration moves into ejection reservoir


192


, thereby altering the volume of ejection reservoir


192


, which in turn forces biofluid from the ejection reservoir


202


through nozzle


204


as an ejected biodrop. The size of nozzle


204


is a controlling factor as to the size of. the ejected drops.




As biofluid drops are emitted from ejection reservoir


192


, surface tension in the ejection reservoir causes biofluid located in main reservoir


194


to be drawn through reservoir connect


196


into ejection reservoir


192


, thereby replenishing the biofluid level. In the present embodiment, main reservoir


194


has an internal dimension of 1 cm in length and 2.5 mm in height. The width of the overall piezoelectric drop ejection unit is 5 mm. In one embodiment the volume of biofluid in a full main reservoir may be from 50 to 150 microliters and the biofluid in the ejection reservoir may be between 5 and 25 microliters. The ratio of biofluid in the reservoirs may range from 2 to 1 up to 10 to 1. In other situations the ratio may be greater. The volume of biofluid drops may be in the picoliter range.




As can be seen in

FIG. 12

, lower surface


202


connected to piezo actuator


200


is integrated into the overall piezoelectric drop ejector unit


190


. Under this construction, when biofluid of unit


190


is depleted, the entire unit


190


may be disposed.




Turning to

FIG. 13

, illustrated is a side view of a two piece piezoelectric biofluid drop ejection unit


220


having a disposable portion and a reusable portion. The disposable portion includes a main reservoir


222


and an ejection reservoir


224


which has integrated therein an ejection nozzle


226


. The ejection reservoir


224


, being connected to main reservoir


222


via reservoir connect


230


. Transmission of biofluid from main reservoir


222


to ejection reservoir


224


, via reservoir connect


230


occurs due to surface tension existing in ejection reservoir


224


. Also included is a filling port


232


.




The reusable portion of unit


220


includes piezo actuator


240


powered by a power supply source


242


. The piezo actuator


240


is carried on a reusable frame


244


.




A lower surface of ejection reservoir


224


is formed as a membrane


246


and is connected to an upper surface or diaphragm


248


of reusable frame


244


. Diaphragm


248


is bonded or otherwise connected to piezo actuator


240


such that diaphragm


248


acts as part of a unimorph structure to create a necessary volume change within ejection reservoir


224


in order to eject a biofluid drop from ejection nozzle


226


. Membrane


246


of cartridge


222


acts to transfer the volume change in the reusable portion


244


into the disposable portion.




In a further embodiment, the reusable portion has a flexible membrane with a piezo actuator on one surface to generate the volume displacement necessary to expel a biofluid drop. A container may be fabricated to place a connecting liquid in contact with the transducer/membrane. This liquid assists in transmitting the transducer-induced volume changes to a second membrane on a different container surface. The container edges are constructed to make a hermetic seal between the reusable and the disposable parts. The container has a provision for removing (bleeding) air bubbles from the connecting liquid. The opposite surface is open before assembling with the disposable part.




A hermetic seal is provided between the disposable and reusable portions, and the reusable portion is filled with a connecting liquid to transmit the volume changes from the transducer to the disposable portion. To minimize compliance and absorption of volume changes, all air bubbles in this fluid are removed before operation by bleeding them through a bleeding mechanism in the reusable portion.




One skilled in the art would understand that other piezo actuator configurations, such as bulk or shear mode designs, may also be used in conjunction with the present invention.




In the foregoing discussion, configurations are disclosed which function to ensure that the necessary biofluid levels are maintained in a system. In an alternative embodiment, the concepts discussed in connection with

FIGS. 4A and 4B

may be used in systems where additional biofluid is not added.




In one embodiment an adjustment of the generated acoustic wave is used to extend the operational capabilities of the system. This embodiment is applicable to both a Fresnel lens and a spherical lens.




With attention to

FIGS. 4A and 4B

, rather than using controller


70


to selectively activate an actuator, controller


70


supplies signal generator


12


with an indication to increase or decrease amplitude output when it is determined that the fluid height is not at the desired level. By this action, the focal point of the acoustic wave is adjusted to occur at the actual meniscus height.




A further embodiment would be to again use the concepts of

FIGS. 4A and 4B

to detect that the fluid height is not at a desired level. Thereafter, when using a Fresnel lens, it is possible to change operational frequency in order to tune the focal point to the exact fluid height existing at a particular time within the device. For a Fresnel lens the focal position is substantially a linear function of frequency. Therefore, in

FIGS. 4A and 4B

, the initial step is measurement of the actual biofluid level. Then, controller


70


tunes the frequency of operation such that the focal point is moved to where the meniscus surface actually exists.




Using the foregoing design, it is possible to present a system which forgoes the use of an actuator. Rather, use of frequency control and/or amplitude control expands the range of the appropriate biofluid level for operation of the device. For example, without amplitude or frequency control described above, the range for appropriate use would be +/−5 microns from an ideal level. However, by implementing amplitude control this can be expanded to potentially +/−10 microns, and through frequency control to +/−30 microns.




The frequency and acoustic control concepts may be used alone, without the use of an actuator, or in connection with actuator concepts to provide a more refined control.




In piezoelectric drop ejection units, initial operation may not produce desired drop output. Particularly, when air bubbles exist within the ejection reservoir, non-spherical drops, or drops which are not of a proper consistency or size may be ejected, and more likely no drops will be produced. Therefore, a priming of the ejection unit is desirable.





FIG. 14

illustrates a primer connection or mechanism


250


which may be used in accordance with the present invention. As shown in

FIG. 14

, the primer connection


250


is located over a nozzle (


204


,


226


) which is configured to emit biofluid from an ejection reservoir (


192


,


224


). In operation, disposable primer connection


250


may be a robotically actuated device, which moves over an ejection nozzle (


204


,


226


). The primer connection


250


includes a permanent vacuum nozzle


252


connected to a vacuum unit


254


. Placed around permanent vacuum nozzle


252


is a disposable tubing


256


made of an elastomaric or other suitable material. Once located over ejection nozzle (


204


,


224


), the vacuum nozzle


252


is moved downward, placing the disposable tubing


256


into a loose contact with nozzle (


204


,


226


). Vacuuming action vacuums air out of the ejection reservoir (


204


,


226


).




A robotically controlled liquid height detection sensor


258


determines when the biofluid has reached a level out of the nozzle, such that it is ensured air within the ejection reservoir has been removed. This priming operation permits for proper initial drop ejection operation.




Turning to

FIG. 15

, illustrated is a modified single piece piezoelectric drop ejection unit


260


designed in a manner similar to the ejection unit


190


illustrated in FIG.


12


. Therefore common elements are numbered similarly. However, the presently configured unit


260


also includes a priming reservoir


262


having a priming opening


264


. Priming is accomplished by movement of priming system


250


to a position over priming opening


264


. Once sleeve


256


is engaged with opening


264


, a vacuum pressure is applied to draw the biofluid for priming purposes. During this operation, power supply


210


generates pulses for activation of piezo actuator


200


in order to move biofluid within ejection reservoir


192


up to nozzle


204


.




It is to be understood that the reagent cartridges discussed in the foregoing embodiments are simply representative designs of such a device, and that there are many possible variations to the cartridge configuration.




While the forgoing description sets forth embodiments for acoustic drop ejection units and piezoelectric drop ejection units, the concepts of the present invention may be extended to other drop ejection mechanisms and for fluid other than biofluids for which avoidance of contamination is beneficial.




It is to be further understood that while the figures in the above description illustrate the present invention, they are exemplary only. Others will recognize numerous modifications and adaptations of the illustrated embodiments which are in accord with the principles of the present invention. Therefore, the scope of the present invention is to be defined by the appended claims.



Claims
  • 1. A biofluid drop ejection device which ejects biofluid drops, comprising:a biofluid drop ejection mechanism having a transducer which generates energy and a focusing lens used to emit the biofluid drops; a reagent cartridge holding a biofluid, isolated and removable from the drop ejection mechanism to avoid contamination between the biofluid drop ejection mechanism and the reagent cartridge, the reagent cartridge in operative connection with the drop ejection mechanism such that upon operation of the drop ejection mechanism, the biofluid is emitted as the biofluid drops; and a level sensor positioned to sense a height of the biofluid within the cartridge, wherein upon sensing the height of the biofluid below a defined level, an adjustment is made to at least one of the biofluid, the reagent cartridge, and the transducer.
  • 2. The invention according to claim 1 further including a biofluid adjustment mechanism, configured to alter the level of at least one of the biofluid within the reagent cartridge and the level of the reagent cartridge in relationship to the biofluid drop ejection mechanism, when the level sensor senses the height of the biofluid below the predetermined level.
  • 3. The invention according to claim 1 wherein the level sensor includes:at least one acoustic pulse generator/detector capable of emitting an acoustic pulse, the acoustic pulse generator/detector positioned in relationship to the biofluid such that the acoustic pulse emitted from the acoustic pulse generator/detector travels through the biofluid to a surface of the biofluid, where the acoustic pulse is then reflected back through the biofluid and further configured to sense emission of the acoustic pulse and to sense arrival of the reflected acoustic pulse; a timer to determine the time from acoustic pulse emission to acoustic pulse arrival; and a biofluid height calculator, configured to receive the determined time and to calculate the height of the biofluid.
  • 4. The invention according to claim 1 wherein the level sensor includes:at least one laser capable of emitting a laser beam, the laser positioned in relationship to the biofluid such that the laser beam emitted from the laser is reflected from the surface of the biofluid; an optical sensor configuration positioned to sense the laser beam reflected from the biofluid surface; and a biofluid height calculator configured to receive data from at least the optical sensor, wherein the received data represents the biofluid height level.
  • 5. The invention according to claim 1 wherein the level sensor includes:a drop detector designed to detect a number of drops emitted from the reagent cartridge; and a biofluid height calculator configured to determine the height of the biofluid based on the number of drops emitted.
  • 6. The invention according to claim 2 wherein the adjustment mechanism includes:a chamber having an amount of biofluid contained therein, the chamber in fluid communication with an interior of the reagent cartridge; and an actuator in operational connection with the chamber, to selectively regulate movement of biofluid between the reagent cartridge and the chamber.
  • 7. The invention according to claim 2 wherein the adjustment mechanism includes:a reagent cartridge holding chamber within which is located the reagent cartridge; a reagent cartridge control fluid reservoir in fluid communication with outer surfaces of the reagent cartridge holding chamber; and an actuator in operational connection with the fluid reservoir, to selectively regulate movement of reagent cartridge control fluid between the reagent cartridge holding chamber and the reagent cartridge control fluid reservoir.
  • 8. The invention according to claim 1 wherein the biofluid ejection mechanism and the reagent cartridge are configured as a single unit.
  • 9. The invention according to claim 1 wherein the biofluid ejection mechanism and reagent cartridge are separate components, with the biofluid ejection mechanism configured to be reusable with a plurality of reagent cartridges holding biofluid distinct from each other.
  • 10. The invention according to claim 1 wherein the biofluid drop ejection mechanism is an acoustic drop ejection mechanism.
  • 11. The invention according to claim 1 wherein the biofluid drop ejection mechanism is a piezoelectric drop ejection mechanism.
  • 12. The invention according to claim 1, wherein the drop ejection mechanism further includes a substrate.
  • 13. The invention according to claim 1 further including an adjustment mechanism, configured to alter the level of the reagent cartridge in relationship to the biofluid drop ejection mechanism, wherein adjustment occurs when the level sensor senses the height of the biofluid below the predetermined level.
  • 14. The invention according to claim 4, wherein the level sensor is separate from the reagent cartridge.
  • 15. A biofluid drop ejection system which ejects biofluid drops, comprising:a biofluid drop ejection mechanism having a transducer which generates energy and a focusing lens used to emit the biofluid drops; and a reagent cartridge holding a biofluid, isolated and removable from the drop ejection mechanism to avoid contamination between the biofluid drop ejection mechanism and the reagent cartridge, the reagent cartridge connected to the drop ejection mechanism such that upon operation of the drop ejection mechanism the biofluid is emitted as the biofluid drops.
  • 16. The invention according to claim 15 wherein the reagent cartridge includes:an ejection reservoir holding biofluid to be ejected; a main reservoir holding biofluid to be supplied to the ejection reservoir; and a reservoir connect which places the ejection reservoir and main reservoir in fluid communication.
  • 17. The invention according to claim 16 wherein the main reservoir supplies biofluid to the ejection reservoir by capillary action.
  • 18. The invention according to claim 15 wherein the biofluid ejection mechanism and the reagent cartridge are configured as a single unit.
  • 19. The invention according to claim 15 wherein the biofluid ejection mechanism and reagent cartridge are separate components, with the biofluid ejection mechanism configured to be reusable with a plurality of reagent cartridges holding biofluid distinct from each other.
  • 20. The invention according to claim 15 wherein the biofluid drop ejection mechanism is an acoustic drop ejection mechanism.
  • 21. The invention according to claim 15 wherein the biofluid drop ejection mechanism is a piezoelectric drop ejection mechanism.
  • 22. A biofluid drop ejection device which ejects biofluid drops, comprising:a biofluid drop ejection mechanism having a transducer which generates energy and a focusing lens used to emit the biofluid drops; a removable biofluid containment area holding the biofluid in a contamination-free state, the biofluid containment area configured within the drop ejection mechanism such that upon operation of the drop ejection mechanism, the biofluid is emitted as the biofluid drops; a controller configured to sense a height of the biofluid within the biofluid containment area; and a power source connected to the transducer, and to the controller, wherein the controller adjusts at least one of an output power from the power source and a frequency of the power source, to alter a generated acoustic wave to a level substantially equal to the sensed height of the biofluid.
US Referenced Citations (38)
Number Name Date Kind
4520374 Koto May 1985 A
5023625 Bares et al. Jun 1991 A
5477249 Hotomi Dec 1995 A
5521140 Matsuda et al. May 1996 A
5565113 Hadimioglu et al. Oct 1996 A
5618337 Shinozaki et al. Apr 1997 A
5631678 Hadimioglu et al. May 1997 A
5713673 Nemoto et al. Feb 1998 A
5781210 Hirano et al. Jul 1998 A
5798779 Nakayasu et al. Aug 1998 A
5828391 Shinozaki et al. Oct 1998 A
5847732 Shinozaki et al. Dec 1998 A
5877789 Reinten Mar 1999 A
5898446 Moriyama Apr 1999 A
5903291 Yoshimura et al. May 1999 A
5943075 Lee et al. Aug 1999 A
6114122 Besemer et al. Sep 2000 A
6221653 Caren et al. Apr 2001 B1
6242266 Schleifer et al. Jun 2001 B1
6284113 Bjornson et al. Sep 2001 B1
6364459 Sharma et al. Apr 2002 B1
6365378 Hirota et al. Apr 2002 B1
6384210 Blanchard May 2002 B1
6399396 Bass Jun 2002 B1
6420180 Bass Jul 2002 B1
6435396 Eldridge Aug 2002 B1
6439694 Silverbrook Aug 2002 B1
6439695 Silverbrook Aug 2002 B2
6440725 Pourahmadi et al. Aug 2002 B1
6447723 Schermer et al. Sep 2002 B1
6450616 Kubota et al. Sep 2002 B1
20010043243 Tachihara et al. Nov 2001 A1
20020008732 Moon et al. Jan 2002 A1
20020061598 Mutz et al. May 2002 A1
20020063752 Clark May 2002 A1
20020093547 Dante et al. Jul 2002 A1
20030012892 Lee et al. Jan 2003 A1
20030048341 Mutz et al. Mar 2003 A1
Non-Patent Literature Citations (1)
Entry
Experts in Microdispensing & Precision Printing (MicroFab Technologies, Inc.) http://www.microfab.com—last updated Jun. 12, 2000.