Patent Grant
7811521
This application is based on Japanese Patent Applications No. 2005-086682 filed on Mar. 24, 2005 in Japanese Patent Office, the entire contents of which are hereby incorporated by reference.
This invention relates to a testing microchip that can be used as a microreactor in genetic screening for example, and to a testing apparatuses this microchip.
In recent years, using micro-machine technology and microscopic processing technology, systems are developed in which devices and means, for example, pumps, valves, flow channels, sensors and the like for performing conventional sample preparation, chemical analysis, chemical synthesis and the like are miniaturized and integrated on a single chip.
These systems are called μ-TAS (Micro Total Analysis System), bioreactor, lab-on-chips, and biochips, and much is expected of their application in the fields of medical testing and diagnosis, environmental measurement and agricultural manufacturing.
As seen in genetic screening in particular, in the case where complicated steps, skilful operations, and machinery operations are necessary, a microanalysis system, which is automatic, has high speed and is simple, is very beneficial not only in terms of reduction in cost, required amount of sample and required time, but also in terms of the fact that it makes analysis possible in cases where time and place cannot be selected.
At a site where various testing such as clinical testing is carried out, even in a case of measuring with a microreactor of a chip type which can quickly output results regardless of place, quantitation and accuracy in analysis are deemed to be important.
However, it is required to establish a reliable liquid feeding system with a simple structure, since there are severe limitation with respect to size and shape for an analysis chip such as a chip type microreactor. A micro liquid control device that has high accuracy and excellent reliability is needed. The inventors of the present invention have already proposed a suitable micropump system as a micro liquid control device which satisfies this requirement (Patent Document 1: Japanese Patent Application Laid-Open No. 2001-322099 Publication and Patent Document No. 2: Japanese Patent Application Laid-Open No. 2004-108285 Publication).
Furthermore, the inventors of the present invention have already proposed, in Patent Document 3 (Japanese Patent Application 2004-138959), a testing microchip (microreactor) including: a specimen storage section in which specimen is stored; a reagent storage in which reagent is stored; a reaction section which has a reaction flow channel in which the specimen stored in the specimen storage section and the reagent stored in the reagent storage section are merged to perform a predetermined reaction processing; and a testing section which has a testing channel for performing a predetermined test on the reaction-processed substance obtained from the reaction in the reaction section, wherein the specimen storage section, the reagent storage section, the reaction section, and the testing section are connected continuously by a series of flow channels from the upstream side to the downstream side on a single flow channel.
In the microreactor of Patent Document 3 (Japanese Patent Application No. 2004-138959), the flow channels have a number of liquid feed control sections 113 as shown in
That is to say, each liquid feed control section 113 includes a liquid feed control path (with a smaller flow channel diameter) 151 having a smaller cross-sectional flow area than the flow channels 115, through which the flow channel 115 on the upstream side (hereinafter, also referred to as “the upstream flow channel”) and the flow channel 115 on the downstream side (hereinafter, also referred to as “the downstream flow channel”) communicate with each other. Thus, liquid having reached the liquid feed control channel 151 is restricted from passing from the flow channel 115 on the upstream side to the other side.
Due to surface tension, a predetermined feed pressure is needed in order to expel liquid from the liquid feed control path end 151a which has a small cross-sectional area (small diameter) to the downstream flow channel which has a large cross-sectional area (large diameter). Thus, liquid feed control sections 113 are disposed at predetermined locations on the flow channels of the testing microchip, and by controlling the pump pressure from the micropump that is not shown, passing and stopping of the liquid is controlled.
Thus, it is possible for example to temporarily stop the movement of liquid at a predetermined location on a flow channel, and then resume feeding of the liquid to the downstream flow channel at a predetermined timing. Herein, if the inner surface of the liquid feed control path 151 is formed of a hydrophilic material, it is preferable that the inner surface of the liquid feed control path 151 is coated with a water repellent coating such as a fluorine based coating.
By providing a liquid feed control path 151 which allows an upstream flow channel 115 and a downstream flow channel 115 to communicate with each other and has a smaller cross-sectional flow area than the flow channels, feed timing can be controlled.
[Patent Document 1] Japanese Patent Application Laid-Open No. 2001-322099 Publication
[Patent Document No. 2] Japanese Patent Application Laid-Open No. 2004-108285 Publication
[Patent Document 3] Japanese Patent Application No. 2004-138959
[Non-Patent Document 1] “DNA Chip Technology and Applications” “Proteins, Nucleic Acids and Enzymes” Volume 43 Issue 13 (1998) Published by Fusao Kimizuka and Ikunoshin Kato, Kyoritsu Publishing Corp.
In such a known testing microchip, if gas bubbles are present in the liquid, as shown in
Accordingly, a micropump pressure not lower than a set pressure is needed in order to pass liquid from the upstream flow channel 115 with a large diameter, via the liquid feed control path 151 with a small diameter, to the downstream flow channel 115 with a large diameter, and accurate liquid feed control becomes impossible.
Thus, it is possible, for example, that a predetermined testing may not be performed accurately because the specimen and the reagent are not mixed at a suitable time or they are not mixed in a predetermined mixing ratio, resulting in no reaction.
Furthermore, a gas bubble K that blocks the flow path entrance 115a may flow all at once from the upstream channel 115 with a large diameter to the downstream flow channel 115 with a large diameter via the liquid feed control path 151 with a small diameter, and bonding of the reagent, such as a biotin modified chimera primer for specific hybridization of the gene to be an object of detection, and a specimen is inhibited due to the effect of the gas bubbles and the appropriate testing cannot be performed at the testing section.
The present invention was conceived in view of this situation, and the object thereof is to provide a testing microchip and a testing apparatus in which this testing microchip is used. At a liquid feed control section disposed in a flow channel of the testing microchip, gas bubbles which come from an upstream liquid flow channel do not collect at a flow path entrance which leads to a liquid feed control path with a small diameter nor block the flow path entrance; the passage of liquid can be temporarily stopped and then resumed at a predetermined pressure at an appropriate time. It is possible to stop the liquid flow once and pass the liquid at a predetermined pressure and at a suitable timing, while preventing the gas bubbles from passing downstream. Thus, the accuracy of the liquid feed control section is high and accurate testing can be performed with the reliable testing microchip and the testing apparatus using the microchip.
In an aspect in accordance with the invention, there is provided a testing microchip including: a specimen storage section that stores a specimen; a reagent storage section that stores a reagent; a reaction section having a reaction flow channel for mixing the specimen stored in the specimen storage section and the reagent stored in the reagent storage section and performing a predetermined reaction processing; a testing section having a testing flow channel for performing a predetermined test of a reaction product obtained from the reaction in the reaction section; a liquid feed control section; and a gas bubble trapping structure. Herein, the specimen storage section, the reagent storage section, the reaction section, and the testing section are connected continuously by a series of flow channels from an upstream side to a downstream side; the liquid feed control section is provided for the series of the flow channels, stops passing liquid until a liquid feeding pressure in a normal direction from the upstream side to the downstream side reaches a predetermined pressure, and passes the liquid when the liquid feeding pressure becomes higher than the predetermined pressure; and the gas bubble trapping structure is provided at the liquid feed control section and traps a gas bubble in the liquid that flows in the flow channel so that the gas bubble does not flow to the downstream side and only the liquid passes to the downstream side.
In another aspect in accordance with the invention, there is provided a testing apparatus that performs a test in the testing section of the testing microchip, described above, wherein the testing microchip is attachably and detachably mounted to the apparatus.
The invention includes the following structures.
Item 1
A testing microchip, including: a specimen storage section that stores a specimen; a reagent storage section that stores a reagent; a reaction section having a reaction flow channel for mixing the specimen stored in the specimen storage section and the reagent stored in the reagent storage section and performing a predetermined reaction processing; a testing section having a testing flow channel for performing a predetermined test of a reaction product obtained from the reaction in the reaction section; a liquid feed control section; and a gas bubble trapping structure.
Herein, the specimen storage section, the reagent storage section, the reaction section, and the testing section are connected continuously by a series of flow channels from an upstream side to a downstream side; the liquid feed control section is provided for the series of the flow channels, stops passing liquid until a liquid feeding pressure in a normal direction from the upstream side to the downstream side reaches a predetermined pressure, and passes the liquid when the liquid feeding pressure becomes higher than the predetermined pressure; and the gas bubble trapping structure is provided at the liquid feed control section and traps a gas bubble in the liquid that flows in the flow channel so that the gas bubble does not flow to the downstream side and only the liquid passes to the downstream side.
With this structure, the gas bubbles in the liquid flowing in the flow channel are trapped, so as not to flow downstream, by the gas bubble trapping structure of the liquid feed control section that is arranged in the flow channel. Thus, the gas bubbles never flow in the large diameter downstream flow channel, and reaction of the reagent and the specimen, for example, is not inhibited by the effect of gas bubbles, and thus the desired testing can be accurately performed in the testing section.
Since it is allowed to pass liquid only, by applying a feed pressure which is not less than a predetermined value using the gas bubble trapping structure of the liquid feed control section formed in the flow channel, the movement of liquid may be temporarily stopped and then fed to the downstream flow channel at a predetermined timing, and thus stoppage and passage of the liquid can be accurately controlled.
Thus, the specimen and the reagent, for example, are mixed at appropriate times and at a predetermined mixing ratio to react with each other, and a testing microchip is provided in which the accuracy of the liquid feed control section is high, accurate testing is performed and excellent reliability is obtained.
Item 2
The testing microchip of Item 1, wherein the liquid feed control section includes a liquid feed control path through which a flow channel on the upstream side and a flow channel on the downstream side communicate with each other, and the liquid feed control path has a smaller cross-sectional flow area than these flow channels.
With this structure, because of surface tension, a predetermined feed pressure is needed in order to expel liquid from the liquid feed control path which has a small cross-sectional area (small diameter) to the flow channel with a large cross-sectional flow area (large diameter) on the downstream side. Thus, each liquid feed control section is disposed at a predetermined location on a flow channel of the testing microchip, and by controlling the pump pressure from a micropump, passage and stoppage of liquid is controlled, and feeding timing is controlled.
Thus, a specimen and a reagent, for example, are mixed at an appropriate time and at a predetermined mixing ratio to react with each other, and a predetermined testing can be accurately performed.
Item 3
The testing microchip of Item 2, wherein the gas bubble trapping structure is disposed between the liquid feed control path and the flow channel on the upstream side, and includes a buffer path having a larger cross-sectional area than the cross-sectional area of the liquid feed control path.
With this structure, since a buffer path which has a larger cross-sectional area than the cross-sectional area of the liquid feed control path is provided between the liquid feed control path and the upstream flow channel, even if gas bubbles that are in the liquid flowing in the upstream flow channel collect at the downstream end of it, the gas bubbles are trapped at the entrance of the buffer path, and furthermore, since the buffer path has a large cross-sectional area, a flow channel for the liquid around the gas bubbles is secured.
Thus, the liquid in the upstream flow channel can flow into the downstream flow channel via the feed control path at a predetermined pressure, and by controlling the pump pressure from the micropump, stopping and passing of the liquid is controlled to control the timing of feeding the liquid.
Thus, the specimen and the reagent, for example, are mixed at an appropriate time and at a predetermined mixing ratio to react with each other, and a predetermined testing can be accurately performed.
Furthermore, even if the gas bubbles included in the liquid that flows in the upstream flow channel collect at the downstream end of it, since the gas bubbles are trapped at the entrance of the buffer path, the gas bubbles never flow into the large diameter flow channel all at once. As a result, reaction of the reagent and the specimen is not inhibited by the effect of gas bubbles, and thus the desired testing can be accurately performed in the testing section.
Item 4
The testing microchip of Item 3, wherein the buffer path has a width that is approximately the same as a width of the flow channel on the upstream side.
With this a structure, since the buffer path that is provided between the liquid feed control path and the upstream flow channel has substantially the same width as that of the upstream flow channel, a liquid flow channel is secured at the periphery of the bubbles having been trapped at the entrance of the buffer path, in other words, secured at both end portions, in the lateral direction, of the buffer path.
Thus, the liquid in the upstream flow channel can flow to the downstream flow channel via the liquid feed control path at a predetermined pressure, and by controlling the pump pressure from the micropump, stopping and passing of liquid is controlled to thereby control feed timing.
Accordingly, for example, the specimen and the reagent are mixed at an appropriate time and at a predetermined mixing ratio to react with each other, and predetermined testing can be accurately performed.
Item 5
The testing microchip of Item 3, wherein the buffer path has a depth smaller than a depth of the flow channel on the upstream side.
With this structure, because the buffer path has a smaller depth than that of the upstream flow channel, even if the gas bubbles included in the liquid that flows in the upstream flow channel collect at the downstream end of the upstream flow channel, trapping of the bubbles at the buffer path entrance is further secured, and so the gas bubbles never flow into the large diameter flow channel all at once. Accordingly, reaction of the reagent and the specimen is not inhibited by the effect of gas bubbles, and thus the desired testing can be accurately performed at the testing section.
Item 6
The testing microchip of Item 1, wherein the specimen storage section includes a specimen pre-processing section that mixes specimen and a specimen pre-processing liquid and performs a specimen pre-processing.
With this structure, pre-processing appropriate for the amplification reaction of the specimen, such as separation and condensation of the object of analysis (analyte) or protein removal, can be carried out, and a testing microchip can be provided in which predetermined testing can be performed efficiently and quickly.
Item 7
A testing apparatus that performs a test in the testing section of the testing microchip of Item 1, wherein the testing microchip is attachably and detachably mounted to the apparatus.
With this structure, a predetermined testing can be performed accurately and quickly by simply mounting a testing microchip which is portable and has excellent handling properties, to a testing apparatus, without the need to use special techniques or performing difficult and complex operations.
In accordance with the invention, the gas bubbles in the liquid that flows in the flow channel are trapped, so as not to flow downstream, by the gas bubble trapping structure of the liquid feed control section that is arranged in the flow channel. Thus, gas bubbles never enter the large diameter downstream flow channel, and accordingly, for example, reaction of the reagent and the specimen is not inhibited by the effect of gas bubbles, and thus a desired testing can be performed accurately at the testing section.
Also, because of the gas bubble trapping structure of the liquid feed control section that is arranged in the flow channel, only liquid is permitted to pass by applying a feed pressure that is not lower than a predetermined value, and thus movement of liquid can be temporarily stopped, and then feeding to the downstream flow channel can be resumed at a predetermined timing thus to control stopping and passing of the liquid accurately.
In this way, the specimen and the reagent, for example, are mixed at an appropriate time and at a predetermined mixing ratio to react with each other, and a testing microchip is provided, by which the accuracy of the liquid feed control section is high, accurate testing is performed and reliability is excellent.
In accordance with the invention, predetermined testing can be performed accurately and quickly by simply mounting a testing microchip which is portable and has excellent handling properties to a testing apparatus, without the need to use special techniques or performing difficult and complex operations.
The following is detailed description of a preferred embodiment in accordance with the invention with reference to the drawings.
As shown in
A series of flow channels are formed in the testing microchip 2, as shown in
In the following description, the testing microchip 2 is one for genetic screening. However, the testing microchip 2 is not limited to this example, and may be used for screening various specimens. In addition, the arrangement, shape, dimensions, size and the like of the flow channel structure described in the following, may be subjected to various modifications, depending on the type and item of testing.
That is to say, the testing microchip 2 in the present embodiment is one in which an amplification reaction is carried out using ICAN (isothermal chimera primer initiated nucleic acid amplification) method, and a gene amplification reaction is carried out in the testing microchip 2 using a specimen extracted from blood or sputum, a reagent including biotin modified chimera primer for specific hybridization of the gene to be detected, a DNA polymerase having chain substitution activity and an endonuclease. (See Japanese Patent No. 3433929)
The reaction solution is fed into a flow channel in which streptavidin is adsorbed after the modification process, and the amplified gene is fixed in the flow channel.
Next, the probe DNA whose end has been modified by fluorescein isothiocyanate (FITC) and the fixed gene are hybridized. The gold colloid whose surface has been modified with a FITC antibody is adsorbed to the probe that has been hybridized with the fixed gene and the amplified gene is detected by optically measuring the concentration of the gold colloid.
The testing microchip 2, shown in
For example, by just dropping about 2-3 μl of blood specimen in a chip having a length and width of a few centimeters and by mounting the testing microchip 2 on the testing apparatus main body 3 of
As shown in
That is to say, as shown in
In this case, it is preferable that the reagents are stored in advance in these reagent storage sections 18a, 18b and 18c such that testing can be done quickly regardless time and place. The surfaces of the reagent storage sections 18a, 18b and 18c are sealed in order to prevent evaporation, leakage, mixing of gas bubbles, contamination, and denaturing of the reagents which are stored in the testing microchip 2.
Furthermore, when the testing microchip 2 is stored, the reagent storage sections 18a, 18b, and 18c are preferably sealed by a sealing member to prevent the reagents from leaking therefrom into the micro flow channels and causing reaction. Preferably, the sealing member is in a solid or gel state in refrigeration conditions, and dissolves into a liquid state when the microchip 2 is brought to room temperature conditions. For example; the sealing member can be oil.
A micropump 11 is connected at the upstream side of each of the reagent storage sections 18a, 18b and 18c by a pump connection portion 12. Reagent is fed to the downstream flow channel 15a from the reagent storage sections 18a, 18b and 18c by the micropump 11.
Micropumps 11 are incorporated into the testing apparatus main body 3 which is separate from the testing microchip 2, and by mounting the testing microchip 2 to the testing apparatus main body 3, the micropumps 11 are connected through the pump connection portions 12 to the testing microchip 2. However, the micropumps 11 may be incorporated in advance into the testing microchip 2.
A piezo pump is preferably used as a micropump 11.
A micropump 11 includes: a first liquid chamber 48, a first flow channel 46, a pressure chamber 45, a second flow channel 47, and a substrate 42 formed with a second liquid chamber 49. Further, there are provided an upper substrate 41 which is laminated on the substrate 42, a vibration plate 43 which is laminated on the upper substrate 41, a pressure chamber 45 of the vibration plate 43, a piezoelectric element 44 which is laminated on the opposite side; of the vibration plate 43, to the pressure chamber 45, and a drive section (not shown) for driving the piezoelectric element 44.
In a micropump 11 configured as described above, by changing the drive voltage and frequency of the pump, the feed direction and feeding speed of the liquid can be controlled.
As shown in
That is to say, the flow channel 15b communicates with a specimen reaction and detection system including the channel on the left side, shown in
The following mainly describes the flow channel 15b with reference to
The reagent mixture liquid that is fed into the flow channel 15b is then loaded into a reservoir section 17a, as shown in
That is to say, as shown in
Feeding of fixed quantities of reagent is performed as follows. First, a reagent 31 is loaded by being supplied to the reagent loading flow channel 15a at a feed pressure that does not allow the reagent 31 to pass further than the liquid feed control section 13 immediately downstream of reservoir section 17a, from the side of the reverse flow protection section 16.
Next, by feeding a drive liquid 25 in the direction of the reagent loading flow channel 15a from the branched flow channel 15b using the micropump 11 at a feed pressure that allows the reagent 31 to pass further than the liquid feed control section 13 immediately downstream of reservoir section 17a, the reagent 31 that has been loaded in the reagent loading flow channel 15a is pushed further than the liquid feed control section 13 immediately downstream of reservoir section 17a, and thus-a fixed quantity of the reagent 31 is fed. Herein, by providing a large capacity reservoir section 17a in the reagent loading flow channel 15a, variation in the quantitation is reduced.
On the other hand, as shown in
Also, the specimen storage section 20 has substantially the same mechanism as the reagent quantitation section mentioned above and a fixed quantity of specimen is loaded by the micropump 11, and a fixed quantity is fed to the successive flow channel 15e.
That is to say, the specimen loaded in the reservoir section 17b, and the reagent mixture liquid loaded in the reservoir section 17a are fed to the flow channel 15e via a Y-shaped flow channel, and mixing and the ICAN reaction are performed in the flow channel 15e.
Herein, the specimen and the reagents are fed, for example, by alternately driving each micropump 11 and alternately introducing the specimen and reagent mixed liquid in slices to the flow channel 15e and, preferably, the specimen and the reagents are quickly dispersed and mixed.
As shown in
Next, as shown in
Rinsing solution stored in rinsing solution storage sections 21d is fed to the detection sections 22a and 22b and rinsing is performed. Then, buffer stored in hybridization buffer storage sections 21c and probe DNAs, which are stored in a probe DNA storage section 21f (internal control probe DNA storage section 21g for internal control) and whose end have been subjected to fluorescent marking with FITC, are fed to detection sections 22a and 22b, and the probe DNAs are hybridized with the single gene strands that are fixed in the detection sections 22a and 22b. Herein, in the step prior to fixing the single strands of the amplified genes in the detection sections 22a and 22b, the probe DNAs may be hybridized to the single strands of the amplified genes.
Next, after the detection sections 22a and 22b are rinsed with rinsing solution, the gold colloid solution marked with a FITC antibody is fed from the gold colloid storage section 21e to the detection sections 22a and 22b, and thus gold colloid is bound to the fixed amplified genes via the FITC. The bound gold colloid is irradiated with a measuring beam from a LED, for example, and a determination is made as to whether there was amplification, or the efficiency of amplification is measured by detecting transmitted beams or reflected beams using an optical detection means such as photodiode or a photomultiplier.
Herein, as shown in
As shown in
For this reason, in this invention, a liquid feed control section 13 is structured as shown in
With such a liquid feed control section 13 in the structure as described in Patent Document 3 (Japanese Patent Application No. 2004-138959), if there are gas bubbles present in the liquid, as shown in
Accordingly, in order to pass liquid from the upstream flow channel 115 with a large diameter to the downstream flow channel 115 with a large diameter via the small diameter liquid feed control path 151, a micropump pressure that is greater than or equal to a predetermined pressure is needed, and thus accurate feed control cannot be performed.
Thus, there is a possibility that a predetermined testing may not be accurately carried out because the reagent and the specimen, for example, are not be mixed at a suitable time, or they are not mixed in a predetermined mixing ratio and thus do not react with each other.
Also, the gas bubbles K that close the flow path entrance 115a sometimes flow all at once from the upstream flow channel 115 with a large diameter to the downstream flow channel 115 with a large diameter via the small diameter feed control path 151, and bonding of the reagent, such as a biotin modified chimera primer for specific hybridization with the gene to be an object of detection, and the specimen is inhibited due to the effect of the gas bubbles and a predetermined testing cannot be performed in the testing section.
For this reason, in this invention, a liquid feed control section 13 is structured as shown in
That is, the upstream flow channel 15 and the down stream flow channel 15 communicate with each other through the liquid feed control section 13, and the liquid feed control section 13 has a liquid feed control path (a portion with a smaller flow channel diameter) 51 whose flow channel cross-sectional diameter is smaller than that of the flow channels 15, and thus, passing of liquid reaching the feed control path (with the smaller flow channel diameter) 51 from one end side to the other end side is restricted.
As shown in
The gas bubble trapping structure 50 includes a buffer path 52 that has a larger cross-sectional area than that of the liquid feed control path 51.
As shown in
With such a structure for the gas bubble trapping structure, liquid can flow in liquid flow channel 52(b) and 52(c) (arrow A) at the periphery of the gas bubble K, at both ends in the lateral direction, even when gas bubble K has a large diameter and is present in the liquid in upstream flow channel 15 at the flow path entrance 52(a) of the buffer path 52 as shown by the guided lines in
Thus, the liquid in the upstream flow channel 15 is flows to the downstream flow channel 15 via the feed control path 51 at a predetermined pressure, and by controlling the pump pressure from the micropump, passing and stopping of the liquid is controlled and feed timing is thereby controlled.
In such a manner, the specimen and the reagent, for example, are mixed at an appropriate time and at a predetermined mixing ratio to react with each other, and predetermined testing can be accurately performed.
Furthermore, because the buffer path 52 has a smaller depth d than the depth D of the upstream flow channel 15, as shown in
Accordingly, reaction of the reagent such as the biotin modified chimera primer for specific hybridization with the gene to be an object of detection, and the specimen is not inhibited by the effect of gas bubbles, and thus a predetermined testing can be accurately performed at the testing section.
Herein, considering the gas bubble trapping function described above, the depth d of the buffer path 52 is 0.75D or smaller with respect to the depth D of the upstream flow channel 15, and is preferably smaller than 0.5 D. It is preferable that the depth d of the buffer path 52 is approximately the same as the depth of the downstream feed control path 51.
Further considering the gas trapping function described above, the width w of the buffer path 52 is preferably 0.5 W or larger, and more preferably approximately the same as the width W of the upstream flow channel 15.
Still further considering the gas bubble trapping function described above, the length L of the buffer path 52 should be 1 μm to 5 mm and preferably 10-500 μm.
A preferred embodiment in accordance with the invention has been described above, however, the invention is not limited thereto. For example, although in the above embodiment, an ICAN method is used for the testing microchip for gene screening, various modifications may be made to disposition, shape, dimensions, size and the like, in accordance with the kind of specimen and the testing items provided that they do not depart form the scope of the invention.
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| 2005-086682 | Mar 2005 | JP | national |
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| WO 2004061418 | Jul 2004 | WO |
| Number | Date | Country | |
|---|---|---|---|
| 20060216201 A1 | Sep 2006 | US |
