AU2002345465B2 - Flow cell method - Google Patents

Flow cell method Download PDF

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AU2002345465B2
AU2002345465B2 AU2002345465A AU2002345465A AU2002345465B2 AU 2002345465 B2 AU2002345465 B2 AU 2002345465B2 AU 2002345465 A AU2002345465 A AU 2002345465A AU 2002345465 A AU2002345465 A AU 2002345465A AU 2002345465 B2 AU2002345465 B2 AU 2002345465B2
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fluid
flow
flow cell
laminar
interface
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AU2002345465A1 (en
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Kjell Magnusson
Hakan Roos
Mattias Tidare
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Cytiva Sweden AB
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GE Healthcare Bio Sciences AB
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    • GPHYSICS
    • G01MEASURING; TESTING
    • G01NINVESTIGATING OR ANALYSING MATERIALS BY DETERMINING THEIR CHEMICAL OR PHYSICAL PROPERTIES
    • G01N21/00Investigating or analysing materials by the use of optical means, i.e. using sub-millimetre waves, infrared, visible or ultraviolet light
    • G01N21/01Arrangements or apparatus for facilitating the optical investigation
    • G01N21/03Cuvette constructions
    • G01N21/05Flow-through cuvettes
    • GPHYSICS
    • G01MEASURING; TESTING
    • G01NINVESTIGATING OR ANALYSING MATERIALS BY DETERMINING THEIR CHEMICAL OR PHYSICAL PROPERTIES
    • G01N21/00Investigating or analysing materials by the use of optical means, i.e. using sub-millimetre waves, infrared, visible or ultraviolet light
    • G01N21/17Systems in which incident light is modified in accordance with the properties of the material investigated
    • G01N21/55Specular reflectivity
    • G01N21/552Attenuated total reflection
    • G01N21/553Attenuated total reflection and using surface plasmons

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  • Physics & Mathematics (AREA)
  • Health & Medical Sciences (AREA)
  • Life Sciences & Earth Sciences (AREA)
  • Chemical & Material Sciences (AREA)
  • Analytical Chemistry (AREA)
  • Biochemistry (AREA)
  • General Health & Medical Sciences (AREA)
  • General Physics & Mathematics (AREA)
  • Immunology (AREA)
  • Pathology (AREA)
  • Optical Measuring Cells (AREA)
  • Automatic Analysis And Handling Materials Therefor (AREA)
  • Investigating Or Analysing Materials By Optical Means (AREA)

Description

WO 03/002985 PCT/SE02/01224 1 FLOW CELL METHOD Field of the invention The present invention generally relates to the control of a fluid flow over a surface, especially a sensing surface, within a flow cell of an analytical device and, more specifically, to the use of laminar flow cell techniques to position a fluid flow over desired surface areas within a flow cell.
Background of the invention Flow cells are used extensively nowadays in a variety of analytical systems.
Typically, the flow cell has an inlet opening, a flow channel and an outlet opening. A sample fluid to be investigated is introduced through the inlet opening, passes through the flow channel and leaves the flow cell through the outlet opening. In the flow channel, the sample fluid can be analysed. The flow cell may have more than one inlet opening and optionally more than one outlet opening to permit desired manipulations of the flow pattern within the flow cell.
In one type of flow cell, the flow channel or channels contain a sensing surface, usually a substance layer to which a recognition element for an analyte in the sample is immobilised, typically a biochemical affinity partner to the analyte. When the analyte interacts with the recognition element, a physical or chemical change is produced on the sensing surface that can be detected by a detector, e.g. an optical, electrochemical or calorimetric detector. A flow channel may contain two or more sensing surfaces with different recognition elements.
The sensing surface or surfaces in the flow cell may be functionalized, or sensitized, in situ, i.e. within the flow cell. WO 90/05305 discloses a method for functionalising a sensing surface having functional groups thereon by passing a reagent solution containing a bi- or polyfunctional ligand over the surface, the ligand having a function which immobilises the ligand on the sensing surface and at least one more function which is exposed on the sensing surface for interaction with the analyte.
WO 99/36766 discloses methods and systems using hydrodynamic addressing techniques to allow immobilisation of different ligands to discrete sensing areas within a single flow cell channel as well as to permit controlled sample delivery to such sensitised areas. In one embodiment, a so-called Y-cell having two inlet ports and one outlet port is used, wherein a laminar flow of a sample fluid (or sensitising fluid in case of sensitisation of the sensing surface) is provided adjacent to a laminar flow of a nonsensitising fluid a reference fluid) such that the fluids flow together over the sensing surface with an interface to each other. By adjustment of the relative flow rates of the two fluids the interface may be positioned laterally such that the sample fluid (or sensitising fluid) contacts a desired discrete area of the sensing surface. In a variant, a so-called -cell having three inlet ports is used to sandwich the sample fluid (or sensitising fluid) between two non-sensitising fluid flows. A shortcoming of the methods and systems described in WO 99/36766 is, however, that selective contacting of a desired fluid with different areas of the sensing surface is only possible laterally, i.e. transversely to the flow path extension between the flow cell ends.
WO 97/01087 discloses a flow cell having an inlet opening for sample and an outlet opening. A further inlet opening for a reference fluid is provided which is positioned such that the reference fluid flows counter to the sample in the flow channel.
In this way, the sample fluid may be kept away from the blocked volume occupied by the flowing reference fluid without the use of structural partitions in the flow channel.
Typically, a detection layer containing sensitive recognition elements for an analyte extends the whole length of the flow cell channel, and the sample-free region of the flow channel can be used to generate a reference signal. However, the flow cell of WO 97/01087 has a fixed lengthwise extension of the sample region and the sample-free region, and requires that an outlet opening be located between the inlet openings for sample and reference fluid, respectively.
It would be desirable to be able to selectively and variably control the extension of a fluid flow in the longitudinal or normal direction of the flow cell. It would also be desirable to be able to use in this context a conventional type flow cell, such as the Ycell or vy-cell mentioned above.
P \OPERD I 2395970 21 M spl I do-.2 1/0]'267 -3- Summary of the Invention In accordance with the invention, there is provided a method of operating an analytical flow cell device comprising an elongate flow cell having a first end and a second end, at least two ports at the first end, at least one port at the second end, and at least one sensing surface on a wall surface located between the first end and the second end of the flow cell, which method comprises introducing a laminar flow of a first fluid at the first end of the flow cell, introducing a laminar counter flow of a second fluid at the second end of the flow cell, discharging each laminar fluid flow at the first end or the second end of the flow cell, and adjusting the position of the interface between the first fluid and the second fluid in the longitudinal direction of the flow cell by controlling the relative flow rates of the first fluid and the second fluid, and wherein further either: A. the at least one sensing surface comprises at least one detection area at a first distance from the first end of the flow cell and at least one detection area at a second, greater distance from the first end of the flow cell, and the interface between the flow of the first fluid and the flow of the second fluid is adjusted to be at a position between the first distance and the second distance from the first end of the flow cell, such that the first fluid contacts the detection area or areas at the first distance and the second fluid contacts the detection area or areas at the second distance from the first end of the flow cell; or B. the first fluid is capable of reacting with the sensing surface or surfaces, and the second fluid does not react with the sensing surface or surfaces, the at least one sensing surface comprises at least one detection area between the first end and the second end of the flow cell, and the interface between the flow of the first fluid and the flow of the second fluid is adjusted to be at a position between the first end and the at least one detection area, such that the first fluid contacts a sensing surface region extending from the first end substantially up to the at least one detection area; or C. the flow cell comprises at least one detection area between the first end and the second end of the flow cell, and, in a first state, the interface is adjusted to be at a position between the first end and the at least one detection area, and, in a second state, the interface between the first fluid and the second fluid is moved to a position between the at least one detection area and the second end of the flow cell, such that the first fluid is brought in contact with the at least one detection area; or P 'OPER\D~I239597l 21 Mw 07 spal dmr-210)J32(K J -4- D. the flow cell has two openings at the second end and at least one detection area between the first end and the second end, and, in a first state, the first fluid is introduced through a first opening at the first end, the second fluid is introduced through a first opening at the second end, and each fluid flow is discharged at a second opening at the first end of the flow cell, such that the interface between the two fluid flows is at a position between the first end and the at least one detection area, and in a second state, the first fluid is introduced through the first opening at the first end of the flow cell, the second fluid is introduced through the first opening at the second end, and each fluid flow is discharged through a second opening at the second end, such that the interface between the two fluids is at a position between the at least one detection area and the second end of the flow cell.
In another aspect, there is provided a method of sensitising a sensing surface arranged to be passed by a fluid flow within a flow cell, comprising the steps of: passing a laminar flow of an activating fluid through the flow cell to chemically activate the sensing surface, passing a laminar flow of a deactivating fluid and a laminar counter flow of a blocking fluid over the sensing surface with an interface to each other, and adjusting the flow rates of the two fluids such that the deactivating fluid selectively contacts and deactivates a predetermined region of the activated sensing surface extending from one end of the flow cell, and selectively sensitising the activated part of the sensing surface by passing a laminar flow ofa sensitising fluid over the sensing surface.
In another aspect, there is provided a method of analysing a fluid sample for an analyte, comprising sensitising a detection area on a sensing surface by the method, as described above, contacting the sensitised area with the fluid sample, and detecting interaction between the analyte and the detection area In another aspect, there is provided a method of analysing a fluid sample for an analyte, comprising the steps of: providing a flow cell having a first end and a second end, and a sensing surface on a wall surface within the flow cell, introducing a laminar flow of a sensitising fluid at the first end of the flow cell, P \OPER\DH1239Y7ll 21 Me 7 sl~p I d c2ml1inW7 introducing a laminar counter flow of a blocking fluid at the second end of the flow cell, discharging each laminar fluid flow at the first end or at the second end of the flow cell, and adjusting the position of the interface between the sensitising fluid and the blocking fluid such that the sensitising fluid contacts a first portion of the sensing surface and the blocking fluid contacts a second portion of the sensing surface to selectively sensitise the first portion of the sensing surface, introducing a laminar flow of the fluid sample at the first end of the flow cell and discharging the flow of fluid sample at the second end of the flow cell, such that the sample flow sequentially passes the sensitised portion of the sensing surface and the nonsensitised portion of the sensing surface, and detecting interaction of the analyte with the sensitised and non-sensitised portions of the sensing surface.
In another aspect, there is provided a method of analysis, comprising the steps of: providing a flow cell having a first end and a second end, and at least one sensing area on a wall surface within the flow cell spaced from the first end of the flow cell, introducing a laminar flow of a test fluid at the first end of the flow cell, introducing a laminar counter flow of a second fluid at the second end of the flow cell, and discharging each fluid flow at the first end or at the second end of the flow cell, such that an interface is formed between the two fluids which extends substantially transversely to the extension of the flow cell between the ends thereof, in a first state, setting the relative flow rates of the test fluid and the second fluid to position the interface such that the test fluid is at a position between the first end and the at least one sensing area, in a second state, changing the relative flow rates of the laminar fluid flows such that the interface is at a position between the at least one sensing area and the second end of the flow cell, and determining the influence of the test fluid on the at least one sensing area.
In another aspect, there is provided a method of analysis, comprising the steps of: providing a flow cell having a first end and a second end, each end having two openings, and at least one sensing area on a wall surface within the flow cell spaced from the ends of the flow cell, P OPER\DfMr 29597O 21 M I doc2 I /)iir2()7 5a in a first state, introducing a laminar flow of a test fluid through a first opening at the first end of the flow cell, introducing a laminar counter flow of a second fluid through a first opening at the second end of the flow cell, and discharging each fluid flow through a second opening at the first end, such that an interface between the two laminar fluid flows is formed at a position between the first end of the flow cell and the at least one sensing area, in a second state, introducing a laminar flow of the test fluid through the first opening at the first end of the flow cell, introducing a laminar counter flow of the second fluid through the first opening at the second end of the flow cell, and discharging each fluid flow through a second opening at the second end, such that the interface between the two laminar fluid flows is at a position between the second end of the flow cell and the at least one sensing area, changing between at least one of(i) the first state and the second state, and (ii) the second state and the first state, and determining the influence of the change on the at least one sensing area.
In another aspect, there is provided a method of chemically treating a surface area within a flow cell, comprising the steps of: providing a flow cell having a first end and a second end, introducing a laminar flow of a treating fluid at the first end of the flow cel I, introducing a laminar counter flow of a blocking fluid at the second end of the flow cell, discharging each laminar fluid flow at the first end or at thc second end of the flow cell, such that two fluids pass the flow cell with an interface between them, and adjusting the relative flow rates of the two fluids such that the interface is positioned at a predetermined distance from the first end of the flow cell to selectively contact with the treating fluid a wall surface area within the flow cell extending the predetermined distance from the first end of the flow cell.
In the specification and the appended claims, the singular forms and "the" are meant to include plural reference unless it is stated otherwise. Also, unless defined otherwise, technical and scientific terms used herein have the same meanings as commonly understood to a person skilled in the related to the invention.
It is also to be noted that the terms "comprising", "including" and "having" can be used interchangeably.
Brief description of the drawings Figure 1 schematically illustrates an embodiment of the method according to the present invention where a flow cell having two openings at one end and one opening at the opposite end is used.
Figure 2 schematically illustrates the method embodiment in Fig. 1 applied to a flow cell having two detection areas arranged at different distances from an inlet end.
Figure 3 schematically illustrates another embodiment of the invention using a flow cell having two openings at each end and two detection areas arranged at different distances from the ends.
Figure 4 schematically illustrates a variant of the embodiment in Fig. 3.
Figures 5A to 5C schematically illustrate embodiments of the invention where a flow cell having three parallel detection areas is used.
Figures 6A and 6B schematically illustrate still another embodiment of the invention where a flow cell having two openings at each end is used.
Detailed description of the invention As mentioned above, this invention is generally directed to the control of the fluid flow in the flow channel or flow channels of an analytical flow cell device, which usually has at least one sensing surface, using laminar flow techniques to control the fluid flow such that it can be made to occupy a variable portion of the flow channel length between the flow cell ends. While WO 99/36766 mentioned above (the entire disclosure of which is incorporated by reference herein) describes the controlled lateral WO 03/002985 PCT/SE02/01224 7 movement of a fluid flow passing a flow cell from one end to the other using hydrodynamic addressing techniques, the present invention is directed to the control of the longitudinal spread of a fluid flow in the flow cell. Optionally, the present invention may be used in supplement to the methods and systems disclosed in WO 99/36766.
As in WO 99/36766, the configuration and dimensions of the flow cells to be used may vary widely depending upon the specific application and/or the specific detection method.
Representative detection methods include, but are not limited to, mass detection methods, such as piezoelectric, optical, thermo optical and surface acoustic wave (SAW) methods, and electrochemical methods, such as potentiometric, conductometric, amperometric and capacitance methods. With regard to optical detection methods, representative methods include those that detect mass surface concentration, such as reflection-optical methods, including both internal and external reflection methods, angle, wavelength or phase resolved, for example ellipsometry and evanescent wave spectroscopy (EWS), the latter including surface plasmon resonance (SPR) spectroscopy, Brewster angle refractometry, critical angle refractometry, frustrated total reflection (FTR), evanescent wave ellipsometry, scattered total internal reflection (STIR), optical wave guide sensors, evanescent wave-based imaging, such as critical angle resolved imaging, Brewster angle resolved imaging, SPR angle resolved imaging, and the like. Further, photometric methods based on, for example, evanescent fluorescence (TIRF) and phosphorescence may also be employed, as well as waveguide interferometers.
SPR spectroscopy may be mentioned as an exemplary commercially available analytical system to which the present invention may be applied. One type of SPRbased biosensors is sold by Biacore AB (Uppsala, Sweden) under the trade name BIACORE® (hereinafter referred to as "the BIACORE instrument"). These biosensors utilize a SPR based mass-sensing technique to provide a "real-time" binding interaction analysis between a surface bound ligand and an analyte of interest. An analytical system comprising a two-dimensional optical detector based on total internal or external reflection, e.g. an SPR detector, is disclosed in WO 98/34098 (the full disclosure of which is incorporated by reference herein).
WO 03/002985 PCT/SE02/01224 8 However, any instrumentation or technique wherein a sample is brought into contact with a sensing surface within a flow cell under laminar flow conditions may benefit from this invention.
With regard to suitable flow cells for use in the practice of this invention, such flow cells may assume a number of forms, the design of which may vary widely depending upon the intended application and/or use. While several representative flow cells are disclosed herein for purpose of illustration, it should be recognized that any type of flow cell which is capable of contacting a liquid sample to a sensing surface under laminar flow conditions may be employed in the practice of this invention.
The basic principle of the present invention is schematically illustrated in Fig. 1.
The flow cell 1 partially depicted in Fig. 1, referred to herein as an "Y-cell", has two openings 2, 3 (here shown as arms) at one end and one opening 4 at the opposite end of the flow cell. A sensing surface (not shown) is located between the two ends. A laminar flow of a desired fluid, indicated by arrow 5, is introduced through one of the two openings at the first end, here at 2, and a laminar counter flow of a (different) "blocking fluid", indicated by arrow 6, is introduced through the opening 4 at the opposite end of the flow cell. Both laminar fluid flows exit the flow cell through the second opening 3 at the first end. The discharge (typically suction) flow through the outlet opening 3, indicated by arrow 7, is considerably higher than the fluid flow 5 through inlet opening 2. As indicated by the hatched region 8 in Fig. 1, the desired fluid will only occupy the initial portion of the flow cell length (as seen from the first end). The remaining flow cell volume 9, including a small region extending through the outlet opening 3, is occupied by the blocking fluid which prevents the desired fluid from passing further into the flow cell. The spreading, or extension, of the pulse of the first fluid in the flow cell may be controlled by varying the ratio of the exit (suction) flow and the inlet flow of the second fluid. Thus, the higher the ratio, the larger part of the flow cell volume will be occupied by the second fluid.
Such variable length extension of a flow pulse may be used for different purposes. In one embodiment, a bottom) wall of the flow cell supports a substance layer capable of reaction with a reagent solution, and the inventive procedure is used to react only a part of the substance layer with the reagent. One application of such a procedure is to provide a sensing area and a reference area arranged sequentially in the normal flow direction in a flow cell as will be described below with reference to Fig. 2.
WO 03/002985 PCT/SE02/01224 9 In Fig. 2, where corresponding parts have the same reference numerals as in Fig.
1, the bottom wall of the flow cell supports a substance layer containing a recognition element, such as a receptor, for an analyte-specific ligand. Two detection areas 10, 11 are defined along the flow cell by the detection system used, for example an optical detection system. First, a flow of an inert fluid one that does not react with the substance layer) is passed through the flow cell, being introduced through the opening 4 and discharged through at least one of the openings 2, 3. Then, a ligand-containing fluid is introduced via opening 2 and discharged via opening 3, such that the ligandcontaining fluid volume 8 extends past the first detection area 10 but not up to the second detection area 11, the interface 12 between the two fluids thus being positioned between the detection areas 10 and 11. Thereby, the detection area 10 will support the ligand, whereas the detection area 11 will not. When subsequently using the flow cell for analysing a sample flow for an analyte introduced through, for example, one (or both) of the openings 2, 3 and discharged via the opening 4, the detection area 10 will form a sensing area, and the detection area 11 will form a reference area.
Another embodiment of providing sequentially arranged sensing and reference areas in a flow cell is shown in Fig. 3. A flow cell 20, which may be characterised as a "double Y-cell", has two inlet arms 21, 22, and two outlet arms 23, 24. In the same way as in Fig. 2, the bottom wall of the flow cell supports a substance layer containing a recognition element for a ligand, and two detection areas are defined by the detection system used. One detection area 25 is located centrally in the flow cell, and the other detection area 26 is located in one of the outlet arms, here 24. A laminar flow of buffer fluid is first passed through the flow cell, entering via the inlets 21, 22 and the outlet 24, and exiting via the outlet 23. Then, the buffer flow through inlets 21, 22 (but not through outlet 24) is replaced by a laminar flow of ligand-containing fluid. This will result in the ligand-containing fluid occupying the hatched region 27 including the detection area 25, while the buffer fluid entering via outlet 24 will occupy the "blocked" region 28. The detection area 25 will thus react with and support the ligand, whereas the detection area 26 will not be contacted with ligand. When subsequently using the flow cell for analysis of an analyte-containing sample fluid, the sample fluid may be introduced through one (or both) of the inlet arms 21, 22, and discharged through outlet 24 (and optionally also through outlet 23). The detection area 25 will then serve as a sensing area and the detection area 26 as a reference area.
WO 03/002985 PCT/SE02/01224 Fig. 4 illustrates a variant design of the embodiment in Fig. 3. Corresponding parts are indicated by the same reference numerals as in Fig. 3. In Fig. 4, the inlet arms are replaced by ports 21, 22 opening within the flow cell 20, and the outlet arms are replaced by ports 23, 24, also within the flow cell. By controlling the ratio between the laminar flows of the ligand-containing fluid entering via ports 21, 22 and the buffer fluid entering via port 24, the blocked region occupied by the buffer fluid may be made to include the detection area 26.
It is readily appreciated by the skilled person that the procedures of the invention outlined above may be carried out with many other types of flow cells, such as, the so-called "Mr-cell" (described in the above-mentioned WO 99/36766) which has three inlets and one outlet.
The present invention may advantageously be used in conjunction with the hydrodynamic addressing techniques disclosed in the above-mentioned WO 99/36766, as will be described below.
Figs. 5A to 5C illustrate a flow cell 30 of the "Y-cell" type having two inlet ports 31 and 32 (at the ends of respective inlet arms 31a and 32a), and one outlet port 33 (at the end of an outlet arm 33a). Centrally in the flow cell are located three detection areas 34, 35, 36. The whole bottom wall of the flow cell 30 (the whole flow cell surface shown in the figure) supports a material layer containing a functional group capable of being activated by an activating agent. This material layer may, for example, be a carboxymethyl-modified dextran gel, wherein the carboxyl groups may be activated by, for instance, N-hydroxysuccinimide (NHS) and N-ethyl-N-dimethylaminopropyl carbodiimide (EDC) to form reactive N-hydroxysuccinimide ester groups.
With reference to Fig. 5A, according to the hydrodynamic addressing techniques described in the above-mentioned WO 99/36766, a laminar flow of buffer is introduced through inlet port 31 and a laminar flow of a fluid containing activating agent is introduced through inlet port 32. The laminar flow rates of the two fluids are adjusted such that the interface 37 between the two fluids is between the detection areas 35 and 36, the activating fluid covering the hatched region in Fig. 5A. This means that only detection area 36 will be contacted by activating agent and activated whereas detection areas 34 and 35 will not.
The detection area 36 is then to be reacted with a ligand-containing solution such that it may be used as a sensing area when an analyte-containing sample is passed WO 03/002985 PCT/SE02/01224 11 through the flow cell. However, before reacting the detection area 36 with the ligandsolution, the present invention concept is used to deactivate the inlet portion of the flow cell 30 up to the vicinity of the detection area 36. In this way, the material on the flow cell bottom upstream of the detection area 36 will not contain activated reactive groups and will therefore not bind ligand. This means in turn that the depletion of analyte on its way to the detection area 36 will be minimised when subsequently passing a sample flow through the flow cell from the inlet end to the outlet end.
To achieve the desired deactivation, now referring to Fig. 5B, a laminar flow of a buffer fluid is introduced through outlet port 33 to exit the flow cell via inlet port 31.
A laminar flow of deactivating agent is then introduced through port 32 and discharged through inlet port 31, such that a laminar flow of buffer fluid introduced through outlet port 33 is maintained. The ratio of the laminar inlet flow through inlet port 32 and the laminar outlet flow through port 31 is adjusted such that the interface 37 between the flows of deactivating fluid and buffer fluid is positioned close to the detection areas 34 to 36, such that the deactivating fluid passes near but does not spread into the detection areas. The flow cell region occupied by of the deactivating fluid in the flow cell 30 is illustrated by the hatched region 38 in Fig. 5B. The flow cell volume blocked by the buffer fluid flow is indicated by reference numeral 39.
The same procedure as just described above with reference to Figs. 5A and may then be applied to the detection area 34 to immobilise a different ligand thereto after deactivation of the flow cell inlet region upstream of the detection area 34. The detection areas 34 and 36 will thereby form sensing areas while the intermediate detection area 35 will form a reference area. It is appreciated that such formation of a number of parallel detection areas by a hydrodynamic addressing technique in the present type of flow cell (such as Y-cell, ji-cell etc.) permits effective use of the sensing surface area of the flow cell.
To analyse a sample solution for ligand-specific analytes, a laminar fluid flow of the sample solution may be introduced through one (or both) of the inlet ports 31, 32 and discharged via outlet port 33, addressing all three detection areas 34 to 36 in the flow cell simultaneously.
Alternatively, the sample solution may be analysed using the hydrodynanmic addressing technique described in WO 99136766. With reference to Fig. 5C, buffer fluid is first passed through the flow cell 30. A laminar flow of the sample solution is then WO 03/002985 PCT/SE02/01224 12 introduced through inlet port 32, and a laminar flow of buffer is introduced through inlet port 31. The laminar flow rates of the two fluids are adjusted to bring the sample flow (the hatched region in Fig. 5C) into contact with the detection areas 35 and 36 by placing the fluid interface 37 between the reference area 35 and the sensing area 34.
Thereby the sample fluid will contact the sensing area 36 and the reference area 35 and analyte specific to the ligand immobilised on sensing area 36 will bind to the analyte.
To address the detection areas 34 and 35, the same (or another) sample fluid is introduced via inlet port 31 and buffer fluid via inlet port 32, and the interface 37 is moved to a location between the detection areas 35 and 36.
It is readily appreciated that the hydrodynamic addressing techniques described in WO 99/36766 may also be used together with the present invention to provide a sensing surface having two or three parallel sensing areas as in Figs. 5A to 5C) and one or more reference areas located downstream as in Figs. 2 to 4).
In a particular type of flow cells, one or more flow cells are formed by pressing a plate or chip with one or more sensing surfaces, below referred to as a sensor unit, in contact with an element or block having one or more open channels therein. Such a flow cell device is described in, for instance, WO 90/05245 (the disclosure of which is incorporated by reference herein) and is also used in the commercial BIACORE instrument mentioned above. Using a detachable sensor unit like that will permit e.g.
sensitisation (including optional activation and deactivation) according to the invention in one or more flow cells and after removal of the sensor unit, analysis with the sensor unit in another analytical device (which could, of course, also be another flow cell device).
The present invention may also be used to cause a rapid change or shift of a fluid contacting one or more sensing areas in a flow cell. While WO 99/36766 discloses a rapid shift of a contacting fluid by lateral movement of the interface between two different fluids flowing through the flow cell, the present invention permits such a shift by movement of the interface between the fluids in the longitudinal direction of the flow cell. This may be illustrated by reference to Fig. 5B. Assume that the sensing areas 34 and 36 support ligands capable of specifically reacting with an analyte in a sample. A laminar flow of the sample is introduced through the port 32 and a laminar buffer flow is introduced through the port 33. Both the sample flow and the buffer flow are discharged through the port 31, the ratio between the sample flow and the buffer flow WO 03/002985 PCT/SE02/01224 13 being adjusted to position the interface 37 near but not within the detection areas 34 to 36, such that the sample flow 38 (the hatched region in Fig. 5B) is not in contact therewith. The sample and buffer flow rates are then adjusted to move the interface 37 to a position (not shown in Fig. 5B) on the other (upstream) side of the detection areas 34 to 36, thus bringing the sample flow into contact with the detection areas.
Alternatively, rather than moving the interface 37 as above, the interface may be removed by filling the whole flow cell with sample by closing the port 31, stopping the buffer flow and discharging the sample flow through the port 33.
It is appreciated that the rise and fall times are limited only by the movement of the interface from a first position not in contact with the detection areas to a second position such that the sample flow is in contact with the detection areas. The volume of sample required to move the interface from the first to the second position is a fraction of the volume of the flow cell itself. Thus, instead of shifting from buffer flow to sample flow with valves at some distance from the sensing area, the interface can be moved with only a fraction of the volume of the flow cell. Since the rise time is proportional to the volume that has to be displaced, a tenfold decrease in volume reduces the rise time by about 10 fold. Similar advantages are achieved with shorter fall times.
Such fast rise and fall times are of necessity when measuring fast reaction kinetics, for example, when studying association and dissociation. In one embodiment, an analyte may be passed over a sensitised sensing area(s). The sample flow may then be displaced from contact with the sensitised sensing area(s), and the dissociation rate can be detected. Alternatively, a sample flow may be rapidly displaced onto a sensitised sensing area(s), thereby allowing for the detection and analysis of association kinetics.
A variant embodiment of the invention to achieve rapid fluid shifts will be described below with reference to Figs. 6A and 6B. This embodiment utilizes a flow cell 40 which like the flow cell in Figs. 3 and 4 has two openings 41, 42 at one end and two openings 43, 44 at the other end. Each opening 41 to 44 is associated with a respective valve (not shown) which opens or closes the opening. A number of detection areas (here three) 45a to 45c are located centrally in the flow cell In Fig. 6A, a laminar flow of e.g. a sample fluid, indicated by arrow 46, is introduced through the opening 41, and laminar flow of e.g. buffer, indicated by arrow 47, is introduced through the opening 43. Both fluid flows are discharged through the WO 03/002985 PCT/SE02/01224 14 opening 42, indicated by arrow 50. The sample flow 48 (the hatched region in Fig. and the buffer flow 49 together form a combined flow with an interface 51 between them. In this state of the flow cell 40, the detection areas 45a-c are in contact only with the buffer flow.
The state of the flow cell 40 is then changed to that shown in Fig. 6B by closing the valve associated with the opening 42 and opening the valve associated with the opening 44. This causes the sample flow and the buffer flow to exit the flow cell through the opening 44 in a combined flow, indicated by arrow 52, the interface 51 being displaced towards the opposite end of the flow cell 40, such that only the sample flow (the hatched region in Fig. 6B) contacts the detection areas 45a-c. Thus, by opening the valve associated with the opening 44 and closing the valve associated with the opening 42, or vice versa, a rapid shift of the fluid contacting the detection areas may be obtained. Depending on the detailed design of the flow cell 40, it will usually be necessary to also regulate the individual flow rates of the buffer and sample flows, respectively.
In order to achieve the desired fluid shift as rapidly as possible, the interface 51 between the two laminar fluid flows is preferably positioned close to the row of detection areas 45a-c in Fig. 6A but not in contact therewith when a subsequent rapid contact with sample is desired for studying the association of an analyte in the sample to a surface-bound ligand), and close to the row of detection areas 45a-c but on the opposite side thereof when a subsequent rapid contact with buffer is desired for studying the dissociation of analyte from surface-bound ligand).
It is appreciated that with the procedure described above, the "dead volume" of the flow cell 40 will be very low and be reduced to only a part of the flow cell volume.
In the non-limiting Example following further below in order to illustrate the present invention further, a BIACORE instrument is used. As mentioned above, the BIACORE insLrument is based on surface plasmon resonance (SPR). The analytical data is provided in the form of a sensorgram which plots the signal in resonance units (RU) as a function of time. A signal of 1,000 RU corresponds to the binding of about 1 ng of analyte per mm 2 A detailed discussion of the technical aspects of the BIACORE instruments and the phenomenon of SPR may be found in U.S. Patent No. 5,313,264.
More detailed information on matrix coatings for biosensor sensing surfaces is given in, for example, U.S. Patents Nos. 5,242,828 and 5,436,161. In addition, a detailed WO 03/002985 PCT/SE02/01224 discussion of the technical aspects of the biosensor chips used in connection with the BIACORE instruments may be found in U.S. Patent No. 5,492,840. The full disclosures of the above-mentioned U.S. patents are incorporated by reference herein.
EXAMPLE 1 Deactivation of an activated inlet area of a flow cell to increase the mass transport to a sensing area A BIACORE S51® instrument (Biacore AB, Uppsala, Sweden) was used. The instrument includes a Y-channel flow cell of the type illustrated in Figs. 5A to 5C. As sensor chip was used Sensor Chip CM5 (Biacore AB), which supports a gold surface with a covalently linked carboxymethyl-modified dextran polymer hydrogel. The optical system measures three detection spots located centrally on the sensing surface forming one channel wall of the flow cell.
Materials Ligand: Biotin-jeffamine conjugate, Mw 374.5 (made in-house), 2 mM, 1.75 mg.in 2386 gl of 10 mM borate, pH Analyte: Biotin-antibody (from Biotin Kit, Biacore AB) Coupling reagent: Aminc coupling kit (Biacore AB), EDC/NHS (N-ethyl-Ndimethylaminopropylcarbodiimide and N-hydroxysuccinimide) Drive buffer: PBS pH 7.2 Deactivating reagent: Ethanolamine A. Sensitisation of sensor chip CM5 Method 1 (prior art) The sensor chip was first activated by injection of EDC/NHS for 420 s at a flow rate of 30 [l/min. Ligand, diluted 1:2 in borate buffer, was then injected for 140 s at a flow rate of 10 pl/min. After the immobilisation of the ligand, ethanolamine was injected for 7 min at 30 pl/min to deactivate all activated sites that had not bound to ligand. Analyte, diluted 1:10 in PBS, was then injected for 120 s at 20 Il/min and the uptake of analyte at the detection spots was measured.
B. Sensitisation of sensor chip CM5 Method 2 (method of the invention) The sensor chip was first activated by injection of EDC/NHS for 420 s at a flow rate of 30 tl/min. The flow cell area preceding the detection spots was then selectively WO 03/002985 PCT/SE02/01224 16 deactivated according to the procedure of the present invention as described above with reference to Fig. 5B, by injecting for 60 s ethanolamine at 21 pl/min and a counter flow of buffer at 40 tl/min. Ligand, diluted 1:2 in borate buffer, was then injected for 140 s at a flow rate of 10 pl/min, and activated sites that had not bound to ligand were deactivated by ethanolamine injection for 7 min at 30 pl/min. Analyte, diluted 1:10 in PBS, was then injected for 120 s at 20 tl/min and the uptake of analyte at the detection spots was measured.
Results Sensitisation method Uptake Normal (Method 1) 262 RU Deactivated inlet part of flow cell (Method 2) 447 RU Ratio (deact./normal) 1.71 From the above results it is seen that deactivation of the activated inlet area (up to the detection spots) in the flow cell, which prevents immobilisation of ligand, increases the mass transport by approximately 70% in the present example. It may therefore be concluded that deactivation of all active area/volume before the detection spots (detection areas/detection volumes) minimises the depletion of analyte. It is further apparent that use of this deactivation technique will permit the positioning of inlet channels having an "active surface" at an arbitrary distance from detection spots or detection areas or detection volumes.
P \OPER\DHI239070 l Ma 07 pl I doc I/031r2O7 17- The reference in this specification to any prior publication (or information derived from it), or to any matter which is known, is not, and should not be taken as an acknowledgment or admission or any form of suggestion that that prior publication (or information derived from it) or known matter forms part of the common general knowledge in the field of endeavour to which this specification relates.
Throughout this specification and the claims which follow, unless the context requires otherwise, the word "comprise", and variations such as "comprises" and "comprising", will be understood to imply the inclusion of a stated integer or step or group of integers or steps but not the exclusion of any other integer or step or group of integers or steps.

Claims (26)

1. A method of operating an analytical flow cell device comprising an elongate flow cell having a first end and a second end, at least two ports at the first end, at least one port at the second end, and at least one sensing surface on a wall surface located between the first end and the second end of the flow cell, which method comprises introducing a laminar flow of a first fluid at the first end of the flow cell, introducing a laminar counter flow of a second fluid at the second end of the flow cell, discharging each laminar fluid flow at the first end or the second end of the flow cell, and adjusting the position of the interface between the first fluid and the second fluid in the longitudinal direction of the flow cell by controlling the relative flow rates of the first fluid and the second fluid, and wherein further either: A. the at least one sensing surface comprises at least one detection area at a first distance from the first end of the flow cell and at least one detection area at a second, greater distance from the first end of the flow cell, and the interface between the flow of the first fluid and the flow of the second fluid is adjusted to be at a position between the first distance and the second distance from the first end of the flow cell, such that the first fluid contacts the detection area or areas at the first distance and the second fluid contacts the detection area or areas at the second distance from the first end of the flow cell; or B. the first fluid is capable of reacting with the sensing surface or surfaces, and the second fluid does not react with the sensing surface or surfaces, the at least one sensing surface comprises at least one detection area between the first end and the second end of the flow cell, and the interface between the flow of the first fluid and the flow of the second fluid is adjusted to be at a position between the first end and the at least one detection area, such that the first fluid contacts a sensing surface region extending from the first end substantially up to the at least one detection area; or C. the flow cell comprises at least one detection area between the first end and the second end of the flow cell, and, in a first state, the interface is adjusted to be at a position between the first end and the at least one detection area, and, in a second state, the interface between the first fluid and the second fluid is moved to a position between the at least one detection area and the second end of the flow cell, such that the first fluid is P \OPEP\r)(HI21597U II 0(7 sp, I do2 1) l01707 -19- brought in contact with the at least one detection area; or D. the flow cell has two openings at the second end and at least one detection area between the first end and the second end, and, in a first state, the first fluid is introduced through a first opening at the first end, the second fluid is introduced through a first opening at the second end, and each fluid flow is discharged at a second opening at the first end of the flow cell, such that the interface between the two fluid flows is at a position between the first end and the at least one detection area, and in a second state, the first fluid is introduced through the first opening at the first end of the flow cell, the second fluid is introduced through the first opening at the second end, and each fluid flow is discharged through a second opening at the second end, such that the interface between the two fluids is at a position between the at least one detection area and the second end of the flow cell.
2. The method according to claim 1, wherein in variant A the at least one detection area at the first distance is an analyte-binding sensing area and the at least one detection area at the second distance is a reference area.
3. The method according to claim 1, wherein in variant B the at least one sensing surface has been chemically activated by an activating agent, and the first fluid contains a deactivating agent, such that the sensing surface region contacted by the first fluid is deactivated.
4. The method according to claim 1, wherein in variant C, in the first state, the interface is adjusted such that the first fluid contacts a sensing surface region extending from the first end substantially up to the at least one detection area.
The method according to claim 1, wherein in variant D a change from the first state to the second state comprises stopping the fluid flow through the second opening at the first end and discharging the two fluid flows through the second opening at the second end.
6. The method according to claim 5, wherein a change from the second state to the P 'OPER\DMI12395970 21 M (2O spI CM.l o 10l3/07 first state comprises stopping the fluid flow through the second opening at the second end and discharging the two fluid flows through the second opening at the first end.
7. The method according to any one of claims 1 to 6, wherein the flow cell is a Y-type flow cell or a y-type flow cell.
8. A method of sensitising a sensing surface arranged to be passed by a fluid flow within a flow cell, comprising the steps of: passing a laminar flow of an activating fluid through the flow cell to chemically activate the sensing surface, passing a laminar flow of a deactivating fluid and a laminar counter flow of a blocking fluid over the sensing surface with an interface to each other, and adjusting the flow rates of the two fluids such that the deactivating fluid selectively contacts and deactivates a predetermined region of the activated sensing surface extending from one end of the flow cell, and selectively sensitising the activated part of the sensing surface by passing a laminar flow of a sensitising fluid over the sensing surface.
9. The method according to claim 8, wherein the flow cell has a first end and a second end and the interface between the deactivating fluid and the blocking fluid extends substantially transversely to the extension of the flow cell between the two ends thereof. The method according to claim 8 or 9, wherein the sensitising step comprises: providing a laminar flow of a first, sensitising fluid and a laminar flow of a second fluid adjacent to the flow of the sensitising fluid such that the two fluids flow together over the sensing surface with an interface to each other, at least the sensitising fluid being capable of sensitising the sensing surface, and adjusting the relative flow rates of the sensitising fluid and the second fluid to position the interface such that the sensitising fluid contacts a discrete sensing area of the sensing surface for selective sensitisation thereof.
P \OPER\DFi 2 1YS90)( 21 M, 0 Sllpa dX.2,i/A)/2n -21
11. The method according to claim 10, wherein the flow cell has a first end and a second end and the interface between the sensitising fluid and the second fluid extends substantially in parallel to the extension of the flow cell between the first end and the second end thereof.
12. A method of analysing a fluid sample for an analyte, comprising sensitising a detection area on a sensing surface by the method according to any one of claims 8 to 11, contacting the sensitised area with the fluid sample, and detecting interaction between the analyte and the detection area.
13. A method of analysing a fluid sample for an analyte, comprising the steps of: providing a flow cell having a first end and a second end, and a sensing surface on a wall surface within the flow cell, introducing a laminar flow of a sensitising fluid at the first end of the flow cell, introducing a laminar counter flow of a blocking fluid at the second end of the flow cell, discharging each laminar fluid flow at the first end or at the second end of the flow cell, and adjusting the position of the interface between the sensitising fluid and the blocking fluid such that the sensitising fluid contacts a first portion of the sensing surface and the blocking fluid contacts a second portion of the sensing surface to selectively sensitise the first portion of the sensing surface, introducing a laminar flow of the fluid sample at the first end of the flow cell and discharging the flow of fluid sample at the second end of the flow cell, such that the sample flow sequentially passes the sensitised portion of the sensing surface and the non- sensitised portion of the sensing surface, and detecting interaction of the analyte with the sensitised and non-sensitised portions of the sensing surface.
14. A method of analysis, comprising the steps of: providing a flow cell having a first end and a second end, and at least one sensing area on a wall surface within the flow cell spaced from the first end of the flow cell, introducing a laminar flow of a test fluid at the first end of the flow cell, P %OPERH)MI23Y5970 21 Ma 07 spat d0 .2 I 3/0312 -22- introducing a laminar counter flow of a second fluid at the second end of the flow cell, and discharging each fluid flow at the first end or at the second end of the flow cell, such that an interface is formed between the two fluids which extends substantially transversely to the extension of the flow cell between the ends thereof, in a first state, setting the relative flow rates of the test fluid and the second fluid to position the interface such that the test fluid is at a position between the first end and the at least one sensing area, in a second state, changing the relative flow rates of the laminar fluid flows such that the interface is at a position between the at least one sensing area and the second end of the flow cell, and determining the influence of the test fluid on the at least one sensing area.
The method according to claim 14, wherein, in the first state, the interface is positioned such that the test fluid extends from the first end substantially up to but not into contact with the at least one sensing area.
16. The method according to claim 14 or 15, wherein, in the second state, the interface is positioned such that the second fluid extends from the second end substantially up to but not into contact with the at least one sensing area.
17. A method of analysis, comprising the steps of: providing a flow cell having a first end and a second end, each end having two openings, and at least one sensing area on a wall surface within the flow cell spaced from the ends of the flow cell, in a first state, introducing a laminar flow of a test fluid through a first opening at the first end of the flow cell, introducing a laminar counter flow of a second fluid through a first opening at the second end of the flow cell, and discharging each fluid flow through a second opening at the first end, such that an interface between the two laminar fluid flows is formed at a position between the first end of the flow cell and the at least one sensing area, in a second state, introducing a laminar flow of the test fluid through the first P OVERD) 2395970) 21 M, 07 spa I am 4)1/20037N -23- opening at the first end of the flow cell, introducing a laminar counter flow of the second fluid through the first opening at the second end of the flow cell, and discharging each fluid flow through a second opening at the second end, such that the interface between the two laminar fluid flows is at a position between the second end of the flow cell and the at least one sensing area, changing between at least one of(i) the first state and the second state, and (ii) the second state and the first state, and determining the influence of the change on the at least one sensing area.
18. The method according to claim 17, wherein, in the first state, the interface is positioned such that the test fluid extends from the first end substantially up to but not into contact with the at least one sensing area, and, in the second state, the interface is positioned such that the second fluid extends from the second end substantially up to but not into contact with the at least one sensing area.
19. The method according to any one of claims 17 to 18, wherein the change firom the first state to the second state comprises closing the second opening at the first end and opening the second opening at the second end, and wherein the change from the second state to the first state comprises closing the second opening at the second end and opening the second opening at the first end.
The method according to any one of claims 14 to 19, wherein the test fluid contains an analyte and the association of an analyte to a sensing area is determined, or wherein the test fluid is analyte-free and the dissociation of the analyte from a sensing area is determined.
21. The method according to any one of claims 1 to 20, wherein the flow cell device comprises a fluid channel element having at least one channel in a flat surface thereof, and a plate member having at least one sensing surface on a face thereof, which plate member is adapted to be detachably pressed against the fluid channel element to form with each channel a sensing surface-containing flow cell. P \OPERID)1 2195970 :1 km(l 7 ,p I dm 2 1 I(V2(X7 -24-
22. The method according to claim 21, comprising the steps of: treating at least one sensing surface by the method according to any one of claims 1 to 11, and moving the plate membcr from the flow cell device to an analytical device and subjecting the treated sensing surface or surfaces to an analytical procedure.
23. The method according to any one of claims 12 to 23, which comprises detecting interaction events at one or more detection areas by an optical sensor, wherein the optical sensor preferably is based on evanescent sensing, especially surface plasmon resonance.
24. A method of chemically treating a surface area within a flow cell, comprising the steps of: providing a flow cell having a first end and a second end, introducing a laminar flow of a treating fluid at the first end of the flow cell, introducing a laminar counter flow of a blocking fluid at the second end of the flow cell, discharging each laminar fluid flow at the first end or at the second end of the flow cell, such that two fluids pass the flow cell with an interface between them, and adjusting the relative flow rates of the two fluids such that the interface is positioned at a predetermined distance from the first end of the flow cell to selectively contact with the treating fluid a wall surface area within the flow cell extending the predetermined distance from the first end of the flow cell.
25. A method of operating an analytical flow cell device, substantially as described with reference to the drawings and/or examples.
26. A method of analysing a fluid sample, substantially as described with reference to the drawings and/or examples.
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