Patent Grant
8124028
The present invention generally relates to devices for analyzing biological samples or for preparing biological samples for analysis.
The fields of life science research and pharmaceutical development are critically dependent upon highly selective and sensitive quantitative assays for a wide range of different biomolecules (such as proteins, antibodies, cytokines, receptors, enzymes, peptides, nucleic acids, hormones, and the like) in complex clinical or biological samples (such as blood, urine, tissue or cellular extracts, cell culture supernatants, bioprocess feedstreams, and the like). In typical samples (which may contain thousands of different molecular species) the analytes of interest may be present at extremely low concentrations (micrograms to nanograms per milliliter or less), but the samples may be available only in very small quantities (hundreds of microliters or less). The rapid growth in the field of biotechnology and the introduction of many potential new drug targets from genomic research have created an increasing demand for more rapid and efficient analytical methods, without any sacrifice in performance.
In order to simultaneously obtain high selectivity (the ability to measure one very specific molecule in a complex mixture) and high sensitivity (the ability to accurately quantify very small concentrations or amounts), a number of analytical methods have been developed which couple powerful molecular separations with extremely responsive detection methods.
One of the most widely used of these separation-based methods is the Enzyme-Linked Immuno-Sorbent Assay or ELISA. In ELISA, an antibody is immobilized on a solid phase support and exposed to a liquid sample, enabling any antigen (analytical target) to bind specifically to the antibody. Non-binding molecules in the sample are washed away. The solid phase with bound target can then be exposed to either antigen or a second antibody specific to the target that are labeled with a linked enzyme. After the non-binding labeled molecules are washed away, the solid phase is then exposed to enzyme substrate under controlled conditions so that the amount of colored or fluorescent enzyme product formed is proportional to the amount of label present, which can be used in turn to quantify the amount of target present in the original sample.
Currently in the fields of life science research and pharmaceutical development, ELISAs are done almost entirely using plastic (typically polystyrene) multi-well plates called microtiter plates or microplates. The wall of each well serves as both the solid phase for binding the antibody and antigen as well as the container for the sample and reagents that are added. Liquid addition is done by pipetting, and washing is done by rapidly pipetting a wash solution in and out of the well. Readout of the enzyme product is done through the transparent plastic wells with an optical plate reader that measures absorbance, fluorescence, or luminescence. This technique is quite simple, requires minimal specialized equipment and is very flexible in terms of the reagent systems and assay formats that can be used.
However, the microplate ELISA method suffers from a number of serious drawbacks. The most important is that the antibody is bound to the wall of the well, and thus the only way sample and reagent molecules can reach the surface to interact is by molecular diffusion. Diffusion is a relatively slow process over the potential path length of several millimeters found in a typical microplate well, and so after liquids are added for each step, the user should allow the plate to incubate for at least overnight to allow the binding reaction to approach equilibrium. Since the assay includes multiple steps, this is impractical, so incubations are typically shortened to an hour or two, meaning the binding reaction does not reach complete equilibrium. Even so, the total assay turnaround time is quite long, typically on the order of 4 to 24 hours.
In addition, microplate ELISAs are subject to a high degree of variability due to the critical techniques required. The pipetting must be done very accurately and consistently into each well. Because the binding reactions do not usually reach equilibrium, timing of pipetting between wells is critical. For the same reason, temperature variation between the inner and outer wells in a plate can lead to variability, as can jarring or vibration of the plates during incubation. Most operators are not as careful as required due to the tedium of the work, and assay coefficients of variation of 10 to 30% or more are not uncommon. Automation of microplate ELISAs using conventional liquid handling robotic equipment is possible but is quite complex and often does not improve reproducibility. Users often find that such automated assays must be constantly monitored by a human operator to prevent problems.
A related set of highly selective separations are used in a micro-preparative mode to isolate a target from a complex sample in preparation for mass spectroscopy (MS), using either an ElectroSpray Interface (ESI) or Matrix Assisted Laser Desorption Interface (MALDI) to ionize the sample upon entry into the instrument. MS is unique in its ability to very rapidly provide comprehensive identity and structural information on analyte molecules with high sensitivity from very small volumes of sample. Because of the rich structural information MS gives about individual molecular species (especially proteins), complex samples must be fractionated or at least significantly simplified to enable a meaningful MS analysis to be performed. Purification methods are also needed when the target of interest is present in very small concentrations relative to other components in the sample, as is often the case in clinical or biological samples. Once the samples are separated into individual fractions or peaks, additional processing (such as concentration, desalting, enzymatic digestion, and/or matrix addition) often must be performed to prepare the sample for analysis by the MS instrument.
In sample prep for MS, the target molecules are selectively bound to a surface by immobilized antibodies or other selective surface groups (such as ion exchange, reversed phase, hydrophobic interaction, affinity, and the like), and non-binding contaminants are washed away. Then the bound target is eluted (using for example salt, acid or organic solvent) for collection into a tube or well, or on a surface for further analytical processing. It is also possible to immobilize an enzyme (such as a protease or glycosidase) to a packed bed to enable very rapid processing of the target molecule prior to further analysis. The amounts of target analyte required for MS are very similar to those required for detection using an ELISA.
Currently two separation methods most often used in front-end preparation for MS are two-dimensional gel electrophoresis and gradient high performance liquid chromatography (HPLC). Both of these techniques are powerful and work reasonably well for comprehensively searching through all the components in complex samples. However, these methods are not without problems. Two-dimensional gels, for example, are labor-intensive, have many steps, and require many hours or even days to complete (compared to the analysis time of MS, which is usually a matter of seconds). HPLC is sometimes not compatible with large proteins, and instrumentation systems with comparable throughput can be almost as expensive and complex as the mass spectrometer itself Sample carryover can also be an issue in high-throughput applications.
Many different types of small-scale adsorption-based separation devices have been developed, and some are offered for use in MS sample preparation. Most have been adapted from devices designed for solid phase extraction (SPE) used in general analytical chemistry. SPE-type columns are often driven by a vacuum manifold, using atmospheric pressure to drive samples and eluents through the column. Another popular approach is the “spin column,” in which a small packed bed is suspended in a microcentrifuge tube, with liquids driven through using a laboratory centrifuge. SPE-type columns are offered by a number of vendors in a range of common surface chemistries (normal phase, reversed phase, ion exchange, metal chelate affinity, etc.). Although they are simple, SPE columns suffer from the need to collect the final product in a test tube then transfer it by pipet to the next step in the process or to the MS interface. These sample transfer steps can lead to significant losses, especially with dilute samples. Also, most of the available spin columns are too large (typical bed volumes of 50 to 250 μL) for handling sample volumes in the low microliter range or below. It is also virtually impossible to control the flow rate through an SPE column (whether driven by vacuum or centrifugation), which can reduce capture efficiency and reproducibility.
Perhaps the most popular approach to simplifying sample preparation for MS is the use of modified pipet tips containing adsorbent materials. In the Millipore “ZIPTIP” product (Millipore Corporation, Billerica, Mass.), a standard chromatographic adsorbent is embedded in a sponge-like polymer matrix in the end of the tip. The matrix enables flow by aspiration in a standard pipettor with little pressure drop. Millipore has also made this technology available in a 96-well plate format (“ZIPPLATE”) driven by a vacuum manifold, primarily for use in in-gel digestion and purification of 2D gel spots. Glygen Corp. (Columbia, Md.) has developed a tip with a flattened area at the end with the adsorbent particles embedded thermally on the inner surface. The tip can handle sample volumes as low as 1 to 10 μL. PhyNexus, Inc. (San Jose, Calif.) produces pipet tips containing affinity chromatography resins sandwiched between sealed-on screens in standard 200 and 1000 μL pipet tips. The tips produce final product in an elution volume of 10 to 15 μL.
Packed bed pipet tip devices suffer from a number of serious drawbacks. These devices move liquids through the bed by air displacement—i.e. by pulling or pushing a fixed volume of air into the tip above the bed to provide a pressure drop across the bed to induce flow. As liquid flows into or out of the tip, the air volume (and thus the pressure) changes, causing a change in the flow rate. The actual flow rate achieved can also vary because of variations in the flow resistance of the packed bed or bed support means from device to device, because of variations in the viscosity of the liquid being pumped, or because of partial plugging of the packed bed from particles in the sample.
It is also very difficult in these devices to achieve the very low flows required for complete binding, especially when affinity or antibody separations are used. As a result, multiple aspirate/dispense cycles are needed. This, in turn, leads to non-quantitative and/or non-reproducible capture of the bound target. Like SPE columns, pipet tips can only perform one separation step at a time, with some type of transfer operation required between steps and likely concomitant sample loss. Flow through the pipet tip can only go in and out through the distal port, which greatly limits the efficiency of washing and elution operations, because each aliquot of wash or elution buffer is completely mixed by the multiple aspirate/dispense steps.
A number of academic labs and companies have worked to integrate the separation and other processing steps or improve MS sensitivity through modifications to the MALDI plate itself. One example is the SELDI (Surface-Enhanced Laser Desorption Ionization) “PROTEINCHIP” product from Bio-Rad Laboratories, Inc. (Hercules, Calif.). In this approach, various surface chemistries are incorporated into a spot on the plate to cause physical adsorption, ion exchange, or separations with affinity binding using antibodies or receptors, etc. A small volume of sample is incubated on the spot. The non-binding materials washed off, and then matrix is added prior to analysis. The MALDI plate approaches are, of course, not amenable for use in electrospray MS. They are also limited to use with single binding selectivity, so that other separation and preparation steps must be carried out elsewhere. The amount of sample that can be processed in this manner is also limited, so significant concentration is difficult to achieve.
A combined system approach has been developed by Intrinsic Bioprobes, Inc. (Tempe, Ariz.). The Mass Spectrometric ImmunoAssay (MSIA) technology developed by this company uses pipet tips incorporating a porous glass frit, onto which antibodies are immobilized. The bound antigens isolated from samples are eluted onto a MALDI plate for analysis. In other products, a pipet tip antibody-based separation device (using a porous glass monolith solid phase) is used in combination with enzymes (such as trypsin) immobilized on the MALDI plate. Gyros AB (Uppsala, Sweden) has developed a microfluidic system in the form of a compact disk (CD)—shaped device that incorporates several separation steps (including antibody affinity) driven by centrifugal force. The major applications for this system are ELISA and sample preparation for MALDI MS. Bruker Daltonics, Inc. (Billerica, Mass.) has introduced the “CLINPROT” system for sample purification for MALDI MS based upon robotic liquid handling and magnetic beads.
Thus, the field of biomolecule separation is one in which there is still room for improvement to overcome some of the limitations in prior art approaches and standard equipment. In particular, the use of the microtiter plate is less appropriate today given the sensitivity and speed desired by modern analytical biochemistry.
The present invention addresses the above-mentioned limitations in the prior art by providing a novel system for efficiently and accurately analyzing targets in samples through a variety of assays, including ELISAs, and for preparing samples for analysis with analytical methods, such as MS.
One aspect of the invention provides an assay assembly including a flow-through assay unit which interfaces with a syringe pump through a probe.
In another aspect, the invention provides a flow-through assay unit having a packed particle bed; a pair of bed supports; a frustum-shaped inlet sealing surface immediately above the packed bed; and a vented, frustum-shaped opening above the inlet sealing surface.
In another aspect, the flow-through unit of the invention is releasably attached to a probe on a liquid handling device, forming a fluid-tight connection between the probe and the packed bed.
In another aspect, the invention provides a probe on a liquid handling device having a needle or tube designed both for directly aspirating or dispensing small volumes of liquids and for connecting to the inlet sealing surface of the assay unit. It also provides a hub designed both to seal to a standard disposable pipet tip and to provide a friction fit on the vented opening of the flow-through assay unit.
In another aspect, the probe is connected either directly or via tubing to a syringe pump to aspirate or dispense fluids through the probe and/or flow-through assay unit at a precisely controlled flow rate.
In yet another aspect, the invention also provides a method of using the flow-through assay assembly and liquid handling device to identify an analytical target by loading a sample solution and a reagent onto a packed bed of the flow-through unit, aspirating unbound antigen and reagents such as enzyme conjugates through the unit, and identifying the analytical target of interest.
More specifically, the invention provides an apparatus comprising an assay unit and a multi-function hub. The assay unit comprises a packed bed, porous bed supports mounted in the assay unit at opposite ends of the packed bed, solid phase support beads located in the packed bed and having a selective-binding or reaction reagent mounted on their surface, an outlet from the assay unit having an outer perimeter and located below the packed bed, an inlet sealing surface adjacent to the packed bed, wherein the outer perimeter of the outlet from the assay unit is dimensioned to form a fluid-tight, friction seal with the inlet sealing surface when two assay units are nested, and an upper section dimensioned to form a friction contact with a probe or a second assay unit when two assay units are nested. The multi-function probe comprises a hub and a needle with a lumen disposed within the hub and extending from the hub, wherein the needle is dimensioned and configured to aspirate and dispense liquid directly and to form a fluid-tight liquid seal with the inlet sealing surface of the assay unit.
In some versions, the upper section of the assay unit and the hub are frusto-conical in shape.
In other versions, the upper section of the assay unit further comprises a raised set of ribs, the hub is dimensioned and configured to form a friction fit with the ribs of the assay unit, and the ribs of the assay unit define a channel between the upper section of the assay unit and the hub when the probe is inserted in the assay unit.
In other versions, the inlet sealing surface is dimensioned to form a fluid-tight, friction seal with a device selected from the group consisting of tubing having an outer diameter of from about 0.75 to about 1 mm and hypodermic needles having a gauge of from about 19 to about 21.
In other versions, the assay unit further comprises a chamber having a frusto-conical shape and positioned between the upper section and the inlet sealing surface.
In other versions, the hub forms a fluid-tight, friction seal with a proximal end of a pipet tip, wherein the multi-function probe is dimensioned and configured to aspirate and dispense liquid through the needle when the pipet tip is not attached to the hub and to aspirate and dispense liquid through the pipet tip when the pipet tip is attached to the hub.
In other versions, the apparatus further comprises a tubular probe shaft, a syringe pump, and a Cartesian robot, wherein the multi-function probe is mounted on the tubular probe shaft and is in fluid connection with the tubular probe shaft, the Cartesian robot controls movement of the tubular probe shaft and the attached multi-function probe in X, Y, and Z axes, and the syringe pump is configured to aspirate and dispense liquids through the multi-function probe.
In other versions, the apparatus further comprises a syringe barrel and a syringe plunger, wherein the multi-function probe is mounted on the syringe barrel and is in fluid connection with the syringe barrel, and the syringe plunger is configured to aspirate and dispense liquids through the multi-function probe.
In other versions, the apparatus further comprises a cylindrical extension mounted on the syringe plunger, wherein the cylindrical extension moveably fits into the lumen of the needle.
In other versions, the apparatus further comprises a support plate, an upper retaining plate, and a seal, wherein the support plate is disposed below the syringe barrel, the upper retaining plate is disposed above the syringe barrel, and the support plate and the upper retaining plate are configured to prevent movement of the syringe barrel in a vertical axis, and wherein the seal is connected to the needle within the syringe barrel, and the seal and the plunger are configured to prevent movement of the syringe barrel in a horizontal axis.
In other versions, the apparatus further comprises a wash manifold. The wash manifold itself may comprise a chimney, a suction chamber, and a plenum, wherein the chimney is dimensioned and configured to hold liquid and to fit the needle or the pipet tip within it, the suction chamber is configured to remove liquid from the chimney, and the plenum is configured to pump liquid into the chimney.
In other versions, the apparatus further comprises a stripper plate, used to strip assay units or pipet tips off probes.
In yet other versions, the invention comprises an automated liquid handling array. The automated liquid handling array may comprise two or more apparatuses. The apparatuses may be assembled in a one- or two-dimensional array and the syringe plungers may be coupled to a common drive plate. In some versions, the two-dimensional array may comprise an 8×12 array of 96 syringe barrels, which may be constructed to correspond to a standard 96-well microplate layout
Unless otherwise defined, all technical and scientific terms used herein have the same meaning as commonly understood by one of ordinary skill in the art to which this invention belongs. Although suitable methods and materials for the practice or testing of the present invention are described below, other methods and materials similar or equivalent to those described herein, which are well known in the art, can also be used.
Other objects, advantages and features of the present invention will become apparent from the following specification taken in conjunction with the accompanying drawings.
Flow-Through Assay Unit:
An important element of this invention is a disposable flow-through assay unit which includes a packed bed of solid-phase adsorbent or immobilized-enzyme particles contained within a cylindrical or frustum-shaped chamber by inlet and outlet screens or filters. This device may be used in at least two major application areas—immunoassays (ELISA) and analytical sample preparation through purification and/or enzymatic treatment. A packed bed, flow-through assay unit of the present invention provides highly sensitive, rapid, and reproducible results for immunoassay and microliter-scale sample-prep applications, as described above, but can also be adapted to run large numbers of samples per day using typical automated liquid handling technology. In order to meet these requirements, the design of the assay unit itself, the nature of the liquid handling/pumping, and the interface between the liquid handler and the assay unit all had to be integrated in a novel way.
The use of a packed bed of solid-phase, non-porous adsorbent beads in the assay unit of the present invention reduces the diffusion path for binding of molecules in the sample to molecules immobilized on the surface to the order of microns (the space between the beads). Because of this, complete binding equilibrium can be reached with a residence time as brief as 30 seconds. This dramatically reduces the overall assay time (15-30 minutes vs. 4-24 hours) by eliminating long incubations. It also eliminates most of the sources of variability mentioned above because the binding reactions in each step actually reach completion, so the timing of the steps and control of mixing is not critical. Reagent addition (performed at a controlled flow rate through a packed bed of adsorbent particles rather than by incubation in a well) can be very reproducible with proper design of the pumps used. The most critical parameters controlling reproducibility are the measurement of the sample volume (all other reagents are added in excess, so volume control for them is less critical) and the flow rate of substrate addition. These can be easily controlled to a precision of well under 5% using standard instrumentation.
The same assay unit of the present invention can also be used in a micro-preparative mode to purify particular molecules of interest for other micro-scale analytical techniques such as MS. In this mode, a packed bed contains any of a number of different particulate adsorbents (including but not limited to porous or non-porous particles, made of materials such as polystyrene-divinylbenzene, polyacrylamide, agarose, cellulose, silica, alumina, zirconia, composites thereof, and the like) with immobilized binding molecules (including but not limited to antibodies, antigens, nucleic acids, hormones, cytokines, receptors, enzymes, and the like) or other selective surface chemistries (including but not limited to ion exchange, normal phase, reversed phase, hydrophobic interaction, gel filtration, affinity chromatography, mimetic ligand chromatography, metal chelate chromatography, and the like). Any of the above-mentioned binding molecules or selective surface chemistries, or any other similar reagents, may be used as selective-binding reagents with the present invention. In use, samples containing the target molecules are passed through the packed bed. The target molecules bind to the selective adsorbent particles, and non-binding contaminants are washed away. The bound target is then eluted using, for example, acid or a salt solution and collected into a tube or on a surface spot for further analytical processing. It is also possible to immobilize a reaction reagent such as an enzyme (including but not limited to proteases, kinases or glycosidases) to the packed bed to enable very rapid selective digestion or other processing of the target molecule as it passes through the packed bed at a controlled flow rate prior to further analysis.
The applications for which the assay unit of the present invention may be used are typically in the fields of life science research and pharmaceutical development. Samples in these fields are normally from biological systems or clinical patients. The sample volumes can be quite small (in the range of tens to hundreds of microliters), and are quite precious. In addition, many of the antibodies and other reagents used in the tests are expensive, so there is a strong desire to minimize the consumption per test. These factors drive toward minimizing the scale of the tests as much as possible. It is also important, however, to utilize industry-standard microplates, pipet tips, and other labware as much as possible. Complete automation of the analytical procedure is also a critical need.
The assay unit 1 is shaped so as to have three distinct frustum-shaped surfaces. The first, closest to the packed bed 2, is the inlet sealing surface 5. The inlet sealing surface 5 is frusto-conical in shape and has an inlet diameter 6, an outlet diameter 7, and a length 8 defined to enable either a tip or needle shaped similarly to a standard pipet tip or the outlet tip of another assay unit to form an air-tight and fluid-tight seal when inserted in the assay unit 1. The second surface, above the inlet sealing surface 5, is a chamber 9 serving as a spacer between the first and third surfaces. The chamber 9 has a volume designed to hold typical required amounts of samples or reagents, typically ranging from 5 to 100 μL so that the assay unit may be used as a spin column or in a vacuum manifold like a conventional SPE device. The third frusto-conical surface, adjacent to the proximal end of the assay unit 1, is the upper section 10. The upper section 10 is sized to fit on the distal end of a standard 200 μL laboratory pipet (i.e. is shaped identically to the proximal end of a standard 200 μL, pipet tip) but has venting means to prevent the formation of a liquid- or gas-tight seal on the pipet.
The dimensions of the inlet sealing surface 5 are critical for enabling the inlet of the packed bed 2 to be in fluid-tight connection to tips, probes, or needles used for accurately aspirating or dispensing microliter liquid volumes.
The inlet diameter 6 of the assay unit inlet sealing surface 5 is selected so that tips, probes, needles, or tubing having the sizes mentioned above will just fit into the upper portion of the inlet sealing surface 5 to form a fluid-tight seal. The inlet diameter 6 may be approximately at least 1 mm and is preferably in the range of 1.2 to 1.5 mm. The outlet diameter 7 is selected so that when the tip is inserted into the inlet sealing surface 5, it will form an interference seal before touching the inlet porous bed support 3, as shown in
This type of sealing mechanism is highly reliable, despite only gentle force (1-3 lb) along the axis of the assay unit 1 being required to make or break the seal. Seals can easily be made by automated robotic systems, which aid in automating the entire assay process. Because of the very small diameters involved, the seals are capable of pressures in excess of 5 bar, even with just the friction of the interfering taper fit.
Prior Art Devices:
Many of the prior art devices designed to provide a small-volume packed bed for extraction of specific molecules from microliter-scale samples are based on the standard disposable pipet tip 22 (
When a packed bed 2 is placed in the end of the pipet tip, as seen in
One major problem with this approach is that liquids are moved through the packed bed by pressure changes caused by air displacement. Because air is compressible, the system is not “hydraulically hard,” and small differences between the flow resistance of the packed bed or bed supports between individual devices or between the viscosities of different liquids will cause differences in the liquid flow rate. In addition, as the liquid flows into or out of the tip, the volume of air changes, causing changes in the pressure and thus the flow rate. Thus, with this type of device it is impossible to control the flow rate with any precision. This leads to wide potential variability in binding or recovery, even in simple binding/elution procedures. For immunoassays in a packed bed device, the degree of colored or fluorescent product formation for a given amount of bound enzyme is inversely proportional to the substrate flow rate, so changes in the flow rate will change the final result significantly. Air displacement-type pipet tip devices are thus not suitable at all for immunoassay applications.
Solid phase extraction (SPE) devices are another approach. Many SPE devices are based on syringe barrels with frits inserted to retain the packed bed. These are typically used with vacuum manifolds to drive liquids through and so have no direct flow rate control. They are also relatively large volume and are poorly suited for microliter scale samples. Some SPE devices are designed to interface with smaller probe tips or needles. The SPE device of Gamble et al. (U.S. Pat. No. 7,001,774, incorporated herein by reference), uses a septum to provide a seal with a hypodermic needle of a syringe or probe and thus can provide good flow control. However, this device does not provide any means for the automated liquid handler to utilize pipet tips for general liquid handling. The SPE device 26 of Cook et al. (U.S. Pat. No. 6,761,855, incorporated herein by reference) (
Multi-Function Liquid Handling Probe for Use with Assay Unit:
Another key element of the current invention is a multi-function probe for use in an automated liquid handling system dimensioned and configured to perform three distinct functions: 1) directly aspirate or dispense microliter fluid volumes; 2) operate with standard disposable pipet tips; and 3) interface with the flow-through assay units of the current invention, also described in U.S. patent application Ser. No. 11/188,535. These three functions can be performed while providing high precision control of the flow rate and volume. The ability of the multi-function probe to directly handle small volumes by itself is very useful for directly dispensing or diluting samples and reagents, and for picking up liquids for directly dispensing them into the assay unit. In cases where carry-over between samples is less critical (such as for dispensing buffers for dilution), direct liquid handling also eliminates the need to use pipet tips and the consequent generation of solid waste. In cases where prevention of carry-over between samples is highly critical (such as with very sensitive immunoassays) the use of standard pipet tips enables the liquid handling system to perform general functions such as aliquotting and diluting in addition to operating the assay units.
Having a firm friction fit between the assay unit upper section 10 and the probe hub 32 is critical for holding the assay unit securely on the probe during operation. However, if the assay unit upper section 10 were to form an air-tight seal on the probe similar to the seal formed between a conventional automated probe 25 and a pipet tip 22 (as shown in
Because the ribs 34 are on the assay unit 1 and not the probe 30, the probe 30 creates a seal when connected to a pipet tip. The seal is established through connections with the pipet tip 22 and the hub 32 of the probe 30, as shown in
Another important feature of both the assay unit and corresponding multi-function system probe is that the devices are dimensioned so that two assay units 1 may be connected in tandem (i.e., nested) as shown in
Liquid Handling Systems for the Multi-Function Probe and Assay Unit:
One embodiment of an automated liquid handling system using a multi-function system probe and assay unit of the current invention is shown in
A potential limitation for some applications with the type of system shown in
Another potential limitation with the type of system shown in
In order to overcome this limitation, the multi-function probe 30 can be directly mounted on a syringe barrel 50, as shown in
Because the probe syringe in the device shown in
As shown in
The design in
Method of Operating the Assay Unit:
In cases where carryover is a critical concern, a pipet tip 22 may be used to transfer liquids in the system, as shown in
After some steps, it may be necessary to remove the assay unit or pipet tip from the probe. This is done as shown in
In virtually all analytical procedures, a critical operation is to wash away unbound molecules and excess liquid (sample or reagent) from both the outside of the assay unit and from the packed bed itself. Complete washing is vital to insure that only molecules that are specifically bound to the adsorbent beads are carried through to the next step of the procedure.
As shown in
The final step in virtually all assay procedures is to dispense liquid from the syringe through the packed bed of the assay unit 1 into a well or tube 70, as shown in
In some cases, additional separation or treatment steps are needed that can be performed on an assay unit packed with different adsorbent beads. This can be done by stacking the assay units 1 in tandem as shown in
A second type of application for the tandem stacked mode of operation is the use of an immobilized protease, such as trypsin, in the lower assay unit. During passage of a sample aliquot aspirated in the upward direction through the lower assay unit, the proteins present would be digested by the immobilized enzyme into defined peptides. By using immobilized enzyme, a much higher amount of enzyme can be used than is normally employed in the solution phase, giving rise to a faster digestion with no chance of autolysis products from the enzyme contaminating the analysis. If a reversed phase packing is used in the upper unit, the digested peptides would be captured and concentrated, and any salt required in the digestion buffer would be removed by washing after the units are decoupled. The peptides could then be eluted in an organic solvent solution that is compatible with the mass spectrometer.
This application is a continuation-in-part of U.S. patent application Ser. No. 11/188,535, filed Jul. 25, 2005 now U.S. Pat. No. 7,799,279 and claims priority to U.S. provisional patent application Ser. No. 61/014,967, filed Dec. 19, 2007, both of which incorporated herein by reference in their entirety.
| Filing Document | Filing Date | Country | Kind | 371c Date |
|---|---|---|---|---|
| PCT/US2008/087744 | 12/19/2008 | WO | 00 | 7/21/2010 |
| Publishing Document | Publishing Date | Country | Kind |
|---|---|---|---|
| WO2009/079661 | 6/25/2009 | WO | A |
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| WO 2004007081 | Jan 2004 | WO |
| Number | Date | Country | |
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| 20110020919 A1 | Jan 2011 | US |
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| 61014967 | Dec 2007 | US |
| Number | Date | Country | |
|---|---|---|---|
| Parent | 11188535 | Jul 2005 | US |
| Child | 12808833 | US |
