US20100147682A1 - Probe for measuring electric potential of cell - Google Patents

Probe for measuring electric potential of cell Download PDF

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Publication number
US20100147682A1
US20100147682A1 US12/712,370 US71237010A US2010147682A1 US 20100147682 A1 US20100147682 A1 US 20100147682A1 US 71237010 A US71237010 A US 71237010A US 2010147682 A1 US2010147682 A1 US 2010147682A1
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probe
opening
flow passage
plate
well
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US12/712,370
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Masaya Nakatani
Nobuhiko Ozaki
Hiroaki Oka
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    • GPHYSICS
    • G01MEASURING; TESTING
    • G01NINVESTIGATING OR ANALYSING MATERIALS BY DETERMINING THEIR CHEMICAL OR PHYSICAL PROPERTIES
    • G01N33/00Investigating or analysing materials by specific methods not covered by groups G01N1/00 - G01N31/00
    • G01N33/48Biological material, e.g. blood, urine; Haemocytometers
    • G01N33/483Physical analysis of biological material
    • G01N33/487Physical analysis of biological material of liquid biological material
    • G01N33/48707Physical analysis of biological material of liquid biological material by electrical means
    • G01N33/48728Investigating individual cells, e.g. by patch clamp, voltage clamp

Definitions

  • the present invention relates to a probe for measuring an electric potential of a cell, such as an intracellular potential or an extracellular potential, used for measuring physicochemical change produced by activity of the cell.
  • a patch clamping method is known as a conventional method of screening candidate pharmaceuticals by monitoring electrical activity of a cell in order to select effective pharmaceutical.
  • a hollow glass tube having a microscopic tip is inserted directly into a cell, thereby measuring a difference between an inside and outside of the cell.
  • This method provides accurate measurement of the status of activities of an ion channel existing in a cell membrane.
  • WO02/055653 discloses a device and a method for measuring an extracellular electric potential.
  • This device includes a substrate having a holding section and electrodes to measure an extracellular electric potential.
  • This device provides data as accurate as data provided by the patch clamping method, and measures a large amount of samples easily and quickly.
  • FIG. 24 is a sectional view of the above-mentioned device for measuring an extracellular electric potential.
  • Culture solution 51 is put in container 50 .
  • Target cell 52 is caught and held with the holding section provided at substrate 53 .
  • This holding section is formed with cavity 54 , opening 55 , and through-hole 56 which are all formed in substrate 53 , and hole 56 communicating with cavity 54 .
  • Reference electrode 58 is provided in container 50 .
  • Measuring electrode 57 is provided near through-hole 56 .
  • Electrode 57 a sensing section, is coupled to an external signal detector via wiring.
  • Target cell 52 is sucked via through-hole 56 by a suction pump from the outside, contacts cavity 54 , thus being held at cavity 54 . Electrical signals produced by activity of target cell 52 is detected as an electric potential difference between measuring electrode 57 disposed near through-hole 56 and reference electrode 58 without leakage into culture solution 51 .
  • This conventional device includes substrate 53 having cavity 54 and through-hole 56 formed therein and container 50 provided on substrate 53 .
  • Container 50 is used for receiving and storing culture solution and chemicals. This structure, therefore, cannot measure electric potentials of cells floating in the solution in a large space as it is in this environmental condition.
  • the conventional device has two areas partitioned with substrate 53 , namely, one area having target cell 52 therein and the other area having measuring electrode 57 , and cannot introduce respective culture solutions or chemicals different from each other into the areas.
  • a probe for measuring an electric potential of a cell includes a plate having a surface having a first cavity provided therein, and a sensor element provided in the first cavity.
  • a second cavity is provided in the bottom surface of the first cavity.
  • the first flow passage having first and second openings is provided in the plate. The first and second openings of the first flow passage open to the second cavity and outside the plate, respectively.
  • the sensor element includes a thin plate, and a supporting substrate provided around the thin plate and in the first cavity of the plate.
  • the thin plate has a through-hole therein having a first opening and a second opening communicating with the second cavity of the plate.
  • the first flow passage allows fluid to flow therein.
  • a sucking device is coupled with the second opening of the first flow passage as to suck the fluid flowing in the first flow passage.
  • This probe can measure an electric potential of a cell floating in solution as it is in a current environment.
  • FIG. 1 is a perspective view of a probe for measuring an electric potential of a cell in accordance with Exemplary Embodiment 1 of the present invention.
  • FIG. 2 is an exploded perspective view of the probe in accordance with Embodiment 1.
  • FIG. 3 is a sectional perspective view of the probe in accordance with Embodiment 1.
  • FIG. 4 is an enlarged sectional perspective view of the probe in accordance with Embodiment 1.
  • FIG. 5 is a sectional view of the probe in accordance with Embodiment 1.
  • FIG. 6 is an enlarged sectional view of the probe in accordance with Embodiment 1.
  • FIG. 7 is a perspective view of the probe in accordance with Embodiment 1.
  • FIG. 8 is a perspective view of the probe for illustrating its usage in accordance with Embodiment 1.
  • FIG. 9 is a schematic diagram of the probe in accordance with Embodiment 1.
  • FIG. 10 is a sectional view of the probe in accordance with Embodiment 1.
  • FIG. 11 is a sectional view of the probe in accordance with Embodiment 1.
  • FIG. 12 is a sectional view of the probe in accordance with Embodiment 1.
  • FIG. 13 is a sectional view of the probe in accordance with Embodiment 1.
  • FIG. 14 is a sectional view of the probe in accordance with Embodiment 1.
  • FIG. 15 is a plan view of another probe for measuring an electric potential of a cell in accordance with Embodiment 1.
  • FIG. 16A is an enlarged sectional view of the probe shown in FIG. 15 .
  • FIG. 16B is an enlarged sectional view of still another probe for measuring an electric potential of a cell in accordance with Embodiment 1.
  • FIG. 17 is a sectional view of a probe for measuring an electric potential of a cell in accordance with Exemplary Embodiment 2 of the invention.
  • FIG. 18 is an enlarged sectional view of the probe in accordance with Embodiment 2.
  • FIG. 19A is a sectional view of the probe for illustrating its usage in accordance with Embodiment 2.
  • FIG. 19B is an enlarged sectional view of the probe shown in FIG. 19A .
  • FIG. 20 is an exploded perspective view of a probe for measuring an electric potential of a cell in accordance with Exemplary Embodiment 3 of the invention.
  • FIG. 21 is a sectional perspective view of the probe in accordance with Embodiment 3.
  • FIG. 22 is an enlarged sectional view of the probe in accordance with Embodiment 3.
  • FIG. 23 is a perspective view of a probe array for measuring an electric potential of a cell in accordance with Embodiment 3.
  • FIG. 24 is a sectional view of a conventional probe for measuring an electric potential of a cell.
  • FIG. 1 is a perspective view of probe 1 for measuring an electric potential of a cell in accordance with Exemplary Embodiment 1 of the present invention.
  • FIG. 2 is an exploded perspective view of probe 1 .
  • FIG. 3 is a sectional perspective view of probe 1 .
  • FIG. 4 is an enlarged sectional perspective view of probe 1 .
  • FIG. 5 is a sectional view of probe 1 .
  • FIG. 6 is an enlarged sectional view of an essential part of probe 1 .
  • Probe 1 includes sensor element 4 and plate 2 made of insulating material, such as resin or glass. Plate 2 has cavity 3 provided in upper surface 2 C thereof. Sensor element 4 is fit into cavity 3 .
  • Cavity 6 is provided under bottom surface 3 A of cavity 3 . Cavity 6 is positioned under sensor element 4 .
  • Plate 2 includes molded plate 2 A and molded plate 2 B attached onto plate 2 A, and can be shaped in a complicated shape easily.
  • Plate 2 B has flow passages 10 and 11 having groove shapes.
  • Plate 2 A has openings 12 and 22 shaped like through-holes.
  • Cavity 3 shaped like a through-hole and cavity 6 communicate with each other.
  • Cavity 6 communicates with openings 10 A and 11 A of flow passages 10 and 11 communicating with the outside of plate 2 , respectively.
  • Other openings 12 and 22 of flow passages 10 and 11 open to upper surface 2 C of plate 2 , respectively.
  • the sectional area of each of flow passages 10 and 11 is not smaller than 0.01 mm 2 to so as preventing flow passages 10 and 11 from being clogged and so as to enable the passages to be cleaned easily.
  • Lower surface 6 A of cavity 6 has bump 17 thereon projecting toward sensor element 4 , i.e. projecting upward towards cavity 6 .
  • This structure enables the adjusting of the sectional areas of flow passages 10 and 11 and the sectional areas of the vicinity of openings 10 A and 11 A at cavity 6 , so that solution to be used for measuring can move smoothly through flow passage 10 , cavity 6 , and flow passage 11 .
  • Sensor element 4 includes supporting substrate 7 made of a silicon substrate or a laminated body including a silicon substrate and a silicon-dioxide film on the silicon substrate.
  • Upper surface 7 A of supporting substrate 7 faces towards a direction identical to a direction towards which upper surface 2 C of plate 2 faces, and has cavity 5 provided therein.
  • Thin plate 8 provides bottom surface 5 A of cavity 5 .
  • Thin plate 8 has through-holes 9 having small diameters allowing upper surface 8 A (bottom surface 5 A of cavity 5 ) to communicate with lower surface 8 B of thin plate 8 .
  • One opening 9 A of each of through-holes 9 opens to cavity 5
  • another opening 9 B of each of through-holes 9 communicates with cavity 6 provided in plate 2 .
  • Measuring electrode 19 made of platinum, gold, silver, or silver chloride is provided on lower surface 8 B of thin plate 8 , i.e., on lower surface 7 B of supporting substrate 7 of sensor element 4 .
  • Measuring electrode 19 is connected with a lead electrode made of a wire or a thin-film electrode for which connecting the measuring electrode with a measuring instrument outside probe 1 for detecting a signal.
  • Sensor element 4 is bonded so securely into cavity 3 with an adhesive so that the solution (measurement solution) to be used for measurement filling passages 10 and 11 and cavity 6 can be prevented completely from leakage.
  • Sensor element 4 may be bonded into cavity 3 by fusion bonding or ultrasonic bonding.
  • FIG. 7 is a perspective view of probe 1 for measuring an electric potential of a cell.
  • Tube 24 A is connected with opening 12 of flow passage 10 .
  • Tube 24 B is connected with flow passage 11 .
  • Tube 24 B is connected with sucking device 13 , and tube 24 A is connected with container 15 .
  • Valve 23 is provided between container 15 and opening 12 to stop the flow of fluid, such as the measurement solution, upon necessary.
  • Sucking device 13 provides cavity 6 with decompressed atmosphere therein having a pressure lower than that in cavity 5 .
  • Sucking device 13 may be an ordinary pump, such as a diaphragm pump, a syringe pump, or sucking with a human mouth, and is not limited to these.
  • FIG. 8 is a perspective view of probe 1 for illustrating its usage.
  • Probe 1 is mounted to measuring stick 25 .
  • Probe 1 is fixed to end 25 A of measuring stick 25 .
  • Tube 24 A coupled with flow passage 10 , tube 24 B coupled with flow passage 11 , and electrode wire 19 A electrically coupled with measuring electrode 19 are arranged inside stick 25 , and are drawn out from another end 25 B of stick 25 .
  • Electrode wire 19 A is connected with an external measuring instrument for supplying measured signals to the instrument.
  • FIG. 9 is a schematic diagram of probe 1 which being used.
  • Measuring stick 25 having probe 1 mounted thereto is dipped into culture solution 21 stored in container 14 .
  • Target cells 20 float in solution 21 .
  • Reference electrode 18 contacts solution 21 in container 14 , thus sensing an electric potential of solution 21 in container 14 .
  • Probe 1 is positioned so that sensor element 4 can be dipped in solution 21 .
  • FIGS. 10 to 14 are sectional views of probe 1 for illustrating a method for measuring an electric potential of a cell with the probe.
  • target cells 20 float above sensor element 4 in solution 21 .
  • valve 23 is closed so that flow passages 10 and 11 and cavity 6 are shut off from container 15 .
  • cavity 6 is decompressed by sucking device 13 to have a pressure therein lower than that in cavity 5 .
  • This operation causes solution 21 and cells 20 filling cavity 5 to be sucked towards through-holes 9 , and then, causes solution 21 to flow into cavity 6 .
  • Each of cells 20 has a size larger than the sectional area of through-hole 9 , and hence, does not pass through through-holes 9 , thus being held at openings 9 A of holes 9 .
  • Solution 21 flowing into cavity 6 contacts measuring electrode 19 , thereby allowing an electric potential in cavity 6 to be detected. In this situation, a difference between respective electric potential of reference electrode 18 and measuring electrode 19 , an electrical resistance between the electrodes, and a capacitance between the electrodes can be measured.
  • sensor element 4 separates culture solution 21 into portion 21 A in cavity 5 and portion 21 B in cavity 6 , thereby increases the resistance between reference electrode 18 and measuring electrode 19 .
  • cavity 6 is further decompressed by sucking device 13 , and accordingly, as shown in FIG. 12 , the surface of target cell 20 is urged more strongly onto opening 9 A of hole 9 , accordingly providing the resistance between electrodes 18 and 19 larger than that of the case that cell 20 is merely held at opening 9 A.
  • the resistance exceeds 100M ⁇ and may exceed 1GSZ, which is called “Giga-Seal”.
  • Giga-Seal an ion-channel activity of cells 20 causes ion exchange between culture solution 21 and cells 20 , thereby changing an inner electric potential of each of cells 20 . This change can be detected as the difference between respective electric potentials of reference electrode 18 and measuring electrode 19 .
  • the ion channel activity changes according to pharmaceutical contained in culture solution 21 , and is detected as the difference of respective electrical potentials of electrodes 18 and 19 so as to detect an influence to target cells 20 , thus allowing a pharmaceutical chemically effect to cells 20 to be determined.
  • Reference electrode 18 and measuring electrode 19 are arranged near openings 9 A and 9 B of through-holes 9 , respectively, to measure the electric potential difference around cell 20 accurately.
  • Probe 1 can catch cells 20 floating in solution 21 easily to provide the Giga-Seal.
  • Upper surface 2 A of plate 2 is flush with upper surface 7 A of supporting substrate 7 , and hence, solution 21 including cells 20 can be directly supplied onto upper surface 7 A of supporting substrate 7 or into cavity 5 with a plate pipette, as shown in FIG. 13 .
  • This arrangement allows cells 20 to be observed easily with a microscope from above upper surface 2 C of plate 2 . Further, this arrangement allows bubbles produced around cells 20 to be removed easily, accordingly enabling the pharmaceutical to be applied to cells 20 without fail.
  • measurement solution 16 in container 15 is sucked into flow passage 10 and cavity 6 , as shown in FIG. 14 .
  • container 15 functions as a pouring device for introducing measurement solution 16 into flow passage 10 .
  • Flow passage 11 is decompressed by sucking device 13 , and accordingly, portion 21 B of solution 21 in cavity 6 is replaced by measurement solution 16 .
  • Measurement solution 16 including a large concentration of K + , allows the change in the electrical potential of cells 20 to be measured more accurately.
  • Reference electrode 18 and measuring electrode 19 may be formed near openings 9 A and 9 B of through-holes 9 by a thin-film technique to detect the change in the electric potential of target cell 20 .
  • FIG. 15 is a plan view of another probe 1 A for measuring an electric potential of a cell in accordance with Embodiment 1.
  • Each of flow passages 110 and 111 has a curved portion. This structure provides a large resistance to the flow of the fluid passing through passages 110 and 111 , accordingly preventing culture solution 21 and measurement solution 16 flowing into cavity 6 from leaking to outside, and from having bubbles in the solutions from outside.
  • FIG. 16A is an enlarged sectional view of probe 1 A at line 16 - 16 shown in FIG. 15 .
  • Pocket 37 A having a diameter larger than that of through-hole 9 is provided at opening 9 A of through-hole 9 facing cavity 5 as to catch the target cell more securely.
  • FIG. 16B is an enlarged sectional view of still another probe 1 B in accordance with Embodiment 1 .
  • pocket 37 B having a diameter larger than that of through-hole 9 is provided at openings 9 B of through-holes 9 facing cavity 6 .
  • This structure stabilizes the fluidity of culture solution 21 in cavity 6 and the fluidity of measurement solution 16 near openings 9 B of through-holes 9 .
  • edge 117 A of bump 117 and edge 6 B of cavity 6 are chamfered to have rounded shapes, thereby allowing measurement solution 16 to flow smoothly.
  • the insulating material, resin or glass, of plate 2 may be transparent to transmit visible light through the material. This structure allows the user to observe openings 9 A of through-holes 9 easily from cavity 6 with a microscope. Hence, monitoring culture solution 21 and measurement solution 16 flowing into cavity 6 as well as presence of bubbles, a user can measure the electric potential of target cell 20 .
  • Thin plate 8 of sensor element 4 may be made of transparent material, such as resin or glass, transmitting visible light therein. This structure allows a user to observe target cell 20 from below the lower surface of plate 2 with a microscope.
  • FIG. 17 is a sectional view of probe 27 for measuring an electric potential of a cell in accordance with Exemplary Embodiment 2 of the present invention.
  • FIG. 18 is an enlarged sectional view of sensor element 29 of probe 27 .
  • Components identical to those of Embodiment 1 are denoted by the same reference numerals, and their descriptions will be omitted.
  • Probe 27 includes plate 28 and sensor element 29 .
  • Upper surface 28 C of plate 28 has cavity 83 provided therein.
  • Cavity 6 is provided in bottom surface 83 A of cavity 83 .
  • Sensor element 29 is fit into cavity 83 .
  • Sensor element 29 includes supporting substrate 26 .
  • Supporting substrate 26 has lower surface 26 B having cavity 32 provided therein.
  • Thin plate 30 is provided at bottom surface 32 A of cavity 32 .
  • Thin plate 30 has through-holes 31 allowing upper surface 30 A of plate 30 to communicate with lower surface 30 B (bottom surface 32 A of cavity 32 ) of plate 30 . Opening 31 A of each of through-holes 31 opens at upper surface 30 A of thin plate 30 (upper surface 26 A of supporting substrate 26 ) and communicates with the outside.
  • Opening 31 B of each of through-holes 31 opens at lower surface 30 B of thin plate 30 and communicates with cavity 32 and cavity 6 .
  • through-holes 31 communicate with flow passages 10 and 11 via cavity 6 provided in plate 28 .
  • Measuring electrode 19 is provided on lower surface 30 B of thin plate 30 upon necessary.
  • FIG. 19A is a sectional view of probe 27 for illustrating its usage.
  • FIG. 19B is an enlarged sectional view of probe 27 shown in FIG. 19A .
  • upper surface 26 A of supporting substrate 26 of sensor element 29 is flush with upper surface 28 C of plate 28 , so that no bump or dip is provided thereon.
  • This structure allows target cell 35 to be observed more closely to the cell with microscope 33 .
  • Observing cells 35 with microscope 33 a user can attach patch probe 34 to cell 35 . This operation allows the user to measure ion-channel activity at plural portions of cell 35 .
  • the probe when pharmaceutical is put into culture solution 36 , the probe can detect simultaneously two electric potentials: an electric potential of patch probe 34 attached to portion 35 A near an applying position where cell 35 is supplied; and an electric potential of measuring electrode 19 near portion 35 B of cell 35 caught at through-holes 31 . Portion 35 A is farther from the applying position than portion 35 A. This simultaneous detection of those two electric potentials allows a transferring state from portion 35 A to portion 35 B of ion-channel activity in cell 35 to be detected.
  • plate 28 and thin plate 30 of probe 27 may be made of transparent material transmitting visible light therethrough, providing effects similar to those of Embodiment 1.
  • FIG. 20 is an exploded perspective view of probe 501 for measuring an electric potential of a cell in accordance with Exemplary Embodiment 3 of the present invention.
  • FIG. 21 is a sectional perspective view of probe 501 .
  • FIG. 22 is an enlarged sectional view of an essential part of probe 501 .
  • Probe 501 includes plate 502 , sensor element 504 , and well array 520 .
  • Plate 502 is made of insulating material, such as resin or glass.
  • Upper surface 502 C of plate 502 has cavity 503 provided therein.
  • Bottom surface 503 A of cavity 503 has cavity 506 provided therein.
  • Sensor element 504 is fit into cavity 503 .
  • Cavity 506 is positioned below sensor element 504 .
  • Cavity 506 is connected with flow passages 509 and 510 communicating with the outside.
  • Flow passage 509 has opening 511 thereof provided in upper surface 502 C of plate 502 .
  • Flow passage 510 has opening 518 thereof provided at upper surface 502 C.
  • Flow passages 509 and 510 communicate with the outside of plate 502 .
  • Molded plate 502 A previously molded is stuck on molded plate 502 B previously molded, thus providing plate 502 .
  • Flow passages 509 and 510 having groove shapes are provided in molded plate 502 B. Openings 511 and 518 shaped like through-holes are provided in molded plate 502 A.
  • Cavities 503 and 506 provided in molded plate 502 A are shaped like a through-hole and communicate with each other.
  • Sensor element 504 includes supporting substrate 512 and thin plate 507 .
  • cavity 505 is provided below thin plate 507 (at the side of lower surface 512 B of plate 502 opposite to upper surface 502 C about plate 502 ).
  • thin plate 507 provides bottom surface 505 A of cavity 505 .
  • Thin plate 507 has small through-holes 508 allowing upper surface 507 A (upper surface 512 A of supporting substrate 512 ) to communicate with lower surface 507 B. Openings 508 A of through-holes 507 provided at upper surface 507 A (upper surface 512 A of supporting substrate 512 ) hold target cells, respectively. Through-holes 508 necessarily have diameters smaller than the sizes of the target cells. Similarly to the probe shown in FIG.
  • a pocket having a diameter larger than that of through-hole 508 may be provided at each of openings 508 A to hold the target cell securely and stably.
  • Each of through-hole 508 has opening 508 B which opens to cavity 505 at lower surface 507 B (lower surface 505 A of cavity 505 ) of thin plate 507 .
  • Opening 508 A of through-hole 508 communicates with upper surface 512 A of substrate 512 of sensor element 504 .
  • Opening 508 B of through-hole 508 communicates with cavity 506 via cavity 505 . This structure allows liquid, such as culture solution and chemicals, to flow in through-holes 508 and cavities 505 and 506 .
  • thin pate 507 is placed at the upper part, that is, upper surface 512 A of supporting substrate 512 and upper surface 502 C of plate 502 are positioned in a single, common plane.
  • cavity 505 may be provided in upper surface 512 A of supporting substrate 512 .
  • Well array 520 is placed on upper surface 502 A of plate 502 .
  • Well array 520 has a predetermined capacity for receiving, storing, or circulating liquid, such as culture solution and chemicals, therein.
  • Well array 520 has wells 522 , 523 , and 524 provided therein.
  • Lower surface 522 A of well 522 has through-hole 521 A provided therein and communicates with opening 511 of flow passage 509 .
  • Lower surface 523 A of well 523 has through-hole 521 B provided therein and communicates with through-hole 508 provided in thin plate 507 of sensor element 504 .
  • Lower surface 524 A of well 524 has through-hole 521 C provided therein and communicates with opening 518 of flow passage 510 .
  • Wells 522 , 523 , and 524 have openings 522 B, 523 B, and 524 B at their tops, respectively, for receiving culture solution or chemicals.
  • Reference electrode 514 is provided in well 523 .
  • Measuring electrode 515 is provided in flow passage 510 and is drawn out to the outside of plate 502 .
  • Culture solution containing the target cells is introduced into well 523 from opening 523 B, and is sucked from opening 524 B of well 524 with a sucking device, such as a suction pump.
  • the culture solution accordingly flows in through-holes 508 and is sucked into well 524 via cavities 505 and 506 , flow passage 510 , and opening 518 .
  • measurement solution or culture solution is introduced into well 522 , and is sucked from well 524 . Then, the solution sufficiently fills flow passages 509 and 510 and cavities 505 and 506 , and is prevented from producing bubbles therein, thereby providing accurate measurement.
  • the measurement solution may be introduced preferably before the target cells are input in well 523 so as to sufficiently fill flow passages 509 and 510 . Then, opening 522 of well 522 is closed, and after that, the cells are input into well 523 while the measurement solution is sucked from well 524 .
  • through-holes 508 of sensor element 504 have the diameters small enough to preventing the target cells from passing through the holes, the cells can be held at openings 508 A of holes 508 , thereby having electric potentials measured while held at through-holes 508 .
  • thin plate 507 has plural through-holes 508 provided therein, thus measuring the electric potentials of the cells at once. After the target cells clogs all of through-holes 508 , the other cells remain in well 523 . Then, the amount of the culture solution flowing into cavity 505 accordingly decreases, and it is accordingly detected that the cells are held at openings 508 A of through-holes 508 .
  • This operation can be performed by controlling a suctioning force at well 524 while measuring a flow rate of the culture solution. The suctioning may be performed from well 522 , providing the same effects.
  • Opening 523 B of well 523 is closed. Then, chemicals is introduced into well 522 and is sucked from well 524 with the sucking device, accordingly flowing in through-hole 521 A, through opening 511 , flow passage 509 , cavities 506 and 505 , flow passage 510 , and opening 518 , and then being sucked into well 524 . At this moment, the chemicals contact, through openings 508 B of holes 508 , the target cells trapped at openings 508 A of through-holes 508 , causing the cells to react with the chemicals. The electric potentials of the cells produced due to the reaction can be measured through reference electrode 514 contacting the culture solution in well 523 and through measuring electrode 515 contacting the chemicals in flow passage 510 .
  • Probe 501 allows liquids, such as culture solution and chemicals, different from each other to be introduced into well 523 having the target cells therein and flow passage 510 having measuring electrode 515 therein, respectively. Sucking the solution between well 522 and well 524 allows one solution to be replaced easily by the other solution.
  • Well array 520 having three wells 522 , 523 , and 524 and its usage have been described. There is a case that chemicals, instead of the culture solution, are introduced into well 523 to measure just the electric potential of the cells after the target cells are held at small through-holes 508 .
  • the well array may have only two wells (for example, wells 523 and 524 ) therein as to perform the measurement.
  • Upper surface 502 C of plate 502 is attached securely onto bottom surface 520 A of well array 520 to enable well array 520 to seal plate 502 securely, thereby preventing the solution securely from leakage.
  • Well array 520 may be made of material identical to that of plate 502 , hence preventing their deformation due to a difference between respective expansion coefficients of the materials, and thereby sealing plate 502 securely.
  • Well array 520 and plate 502 may be made of thermoplastic resin, such as polystyrene, cycloolefin polymer, or cycloolefin copolymer, hence providing a secure sealing by ultrasonic fusion or laser welding, and allowing probe 501 to be manufactured at a high productivity.
  • thermoplastic resin such as polystyrene, cycloolefin polymer, or cycloolefin copolymer
  • Well array 520 and plate 502 may be made of glass material or quartz material. These materials can have surfaces directly bonded onto each other without an adhesive if the surfaces are polished to be finished in mirror-like. Each of these materials has a large resistance to heat, thus being bonded to each other with non-organic adhesive, such as glass adhesive or ceramic adhesive. Well array 520 and plate 502 made of these materials have large heat resistance, hence providing probe 501 re-usable by heat-washing.
  • At least through-hole 521 B out of through-holes 521 A, 521 B, and 521 C provided in lower surfaces 522 A, 523 A, and 524 A of wells 522 , 523 , and 524 , respectively, may flare toward opening 523 B of well 523 , that is, may taper towards through-hole 508 of sensor element 504 .
  • This structure introduces the culture solution or chemicals, which are put into well 523 , into through-holes 508 of sensor element 504 quickly.
  • through-hole 521 B has a size larger than that of thin plate 507 having through-holes 508 provided therein, allowing the target cells to be introduced efficiently into through-holes 508 .
  • Well array 520 has well 523 having the culture solution containing the target cells input thereinto, well 522 having the chemicals input thereinto, and well 524 coupled with the sucking device. This structure allows upper surface 502 C of plate 502 to hold the target cells easily, and allows operations, such as the inputting of the chemicals, to be performed independently from above well array 520 , thus allowing probe 501 to be manipulated easily for measuring the electric potential.
  • Through-hole 521 A of well 522 has a size larger that of opening 511 of flow passage 509
  • through-hole 521 C of well 524 has a size larger than that of opening 518 of flow passage 510 .
  • This structure can introduce liquid, such as the chemicals, quickly into the flow passages, allowing probe 501 to measure the electric potential of the cells accurately with little variation.
  • Reference electrode 514 is provided in well 523 at a predetermined position contacting the culture solution.
  • Measuring electrode 515 is provided in flow passage 510 and contacts the liquid, such as the culture solution or the chemicals, in flow passage 510 . This structure can measure an electric potential of the target cell in the culture solution and an electric potential of the cell after the liquid, such as the chemicals is input from well 522 or well 523 , thus measuring the change between the above potentials.
  • Measuring electrode 515 may be provided near cavity 505 or cavity 506 .
  • Reference electrode 514 and measuring electrode 515 are made of wires or thin-film electrodes, and are coupled to a measuring instrument outside probe 501 for detecting signals from those electrodes.
  • the culture solution containing the target cells is introduced into well 523 , and is sucked with by the sucking device from well 522 or well 524 for holding the cells at through-holes 508 of sensor element 504 .
  • An electric resistance between reference electrode 514 which contacts the culture solution and is provided in well 523 , and measuring electrode 515 provided in flow passage 510 is measured.
  • a suctioning pressure of the suction device is controlled so that the resistance between electrodes 514 and 515 , that is, the resistance between the culture solution stored in well 523 and the culture solution stored in flow passage 510 exceeds 100 M ⁇ .
  • Reference electrode 514 and measuring electrode 515 are made of conductive material, such as Au, Ag, or AgCl, and contact the culture solution to be connected electrically with the solution. Therefore, the positions of electrodes 514 and 515 are not limited to the positions described in above.
  • the measurement solution such as chemicals
  • the measurement solution are stored in well 522 and is sucked from well 524 , thereby causing the culture solution in flow passage 509 , cavities 505 and 506 , and flow passage 510 to be replaced by the measurement solution.
  • solutions, such as the culture solution and the measurement solution different from each other can be introduced easily into well 523 having the cells therein and cavity 506 having measuring electrode 515 therein, respectively. This operation allows the electric potential of the cells to be measured quickly.
  • Wells 522 , 523 , and 524 may have valves or lids, allowing the measurement of the electric potentials with probe 5 to be controlled easily.
  • FIG. 23 is an exploded perspective view of probe 519 (probe array 519 ) for measuring an electric potential of a cell.
  • Probes 501 are arranged in a matrix having four rows and eight columns.
  • Plural well arrays 520 each having wells 522 , 523 , and 524 can be manufactured at once as well array unit 520 A.
  • Probe array 519 including plural probes 501 arranged in a predetermined arrangement allows a robot to pour the chemicals, to input cells, and to suck the cells. Thus, probe 519 can measure respective electric potentials of a lot of cells in a short time for determining pharmacological effect, thus screening candidate pharmaceuticals quickly.
  • a probe for measuring an electric potential of a cell according to the present invention can measure electric potentials of cells floating in solution as they are in environment, hence being used for determining pharmacological effects to the cells and for screening pharmaceuticals.

Abstract

A probe for measuring an electric potential of a cell includes a plate having a surface having a first cavity provided therein, and a sensor element provided in the first cavity. A second cavity is provided in the bottom surface of the first cavity. The first flow passage having first and second openings is provided in the plate. The first and second openings of the first flow passage open to the second cavity and outside the plate, respectively. The sensor element includes a thin plate, and a supporting substrate provided around the thin plate and in the first cavity of the plate. The thin plate has a through-hole therein having a first opening and a second opening communicating with the second cavity of the plate. The first flow passage allows fluid to flow therein. A sucking device is coupled with the second opening of the first flow passage as to suck the fluid flowing in the first flow passage. This probe can measure an electric potential of a cell floating in solution as it is in this environment.

Description

    TECHNICAL FIELD
  • The present invention relates to a probe for measuring an electric potential of a cell, such as an intracellular potential or an extracellular potential, used for measuring physicochemical change produced by activity of the cell.
    • BACKGROUND OF THE INVENTION
  • A patch clamping method is known as a conventional method of screening candidate pharmaceuticals by monitoring electrical activity of a cell in order to select effective pharmaceutical. In the patch clamping method, a hollow glass tube having a microscopic tip is inserted directly into a cell, thereby measuring a difference between an inside and outside of the cell. (For instance, “Single Channel Currents Recorded From Membrane of Denervated Frog Muscle Fibers”, Nature 260: 799-802, Neher E & Sakmann B, 1976) This method provides accurate measurement of the status of activities of an ion channel existing in a cell membrane.
  • International Publication No. WO02/055653 discloses a device and a method for measuring an extracellular electric potential. This device includes a substrate having a holding section and electrodes to measure an extracellular electric potential. This device provides data as accurate as data provided by the patch clamping method, and measures a large amount of samples easily and quickly.
  • FIG. 24 is a sectional view of the above-mentioned device for measuring an extracellular electric potential. Culture solution 51 is put in container 50. Target cell 52 is caught and held with the holding section provided at substrate 53. This holding section is formed with cavity 54, opening 55, and through-hole 56 which are all formed in substrate 53, and hole 56 communicating with cavity 54. Reference electrode 58 is provided in container 50. Measuring electrode 57 is provided near through-hole 56. Electrode 57, a sensing section, is coupled to an external signal detector via wiring.
  • Target cell 52 is sucked via through-hole 56 by a suction pump from the outside, contacts cavity 54, thus being held at cavity 54. Electrical signals produced by activity of target cell 52 is detected as an electric potential difference between measuring electrode 57 disposed near through-hole 56 and reference electrode 58 without leakage into culture solution 51.
  • This conventional device includes substrate 53 having cavity 54 and through-hole 56 formed therein and container 50 provided on substrate 53. Container 50 is used for receiving and storing culture solution and chemicals. This structure, therefore, cannot measure electric potentials of cells floating in the solution in a large space as it is in this environmental condition.
  • The conventional device has two areas partitioned with substrate 53, namely, one area having target cell 52 therein and the other area having measuring electrode 57, and cannot introduce respective culture solutions or chemicals different from each other into the areas.
    • SUMMARY OF THE INVENTION
  • A probe for measuring an electric potential of a cell includes a plate having a surface having a first cavity provided therein, and a sensor element provided in the first cavity. A second cavity is provided in the bottom surface of the first cavity. The first flow passage having first and second openings is provided in the plate. The first and second openings of the first flow passage open to the second cavity and outside the plate, respectively. The sensor element includes a thin plate, and a supporting substrate provided around the thin plate and in the first cavity of the plate. The thin plate has a through-hole therein having a first opening and a second opening communicating with the second cavity of the plate. The first flow passage allows fluid to flow therein. A sucking device is coupled with the second opening of the first flow passage as to suck the fluid flowing in the first flow passage.
  • This probe can measure an electric potential of a cell floating in solution as it is in a current environment.
    • BRIEF DESCRIPTION OF THE DRAWINGS
  • FIG. 1 is a perspective view of a probe for measuring an electric potential of a cell in accordance with Exemplary Embodiment 1 of the present invention.
  • FIG. 2 is an exploded perspective view of the probe in accordance with Embodiment 1.
  • FIG. 3 is a sectional perspective view of the probe in accordance with Embodiment 1.
  • FIG. 4 is an enlarged sectional perspective view of the probe in accordance with Embodiment 1.
  • FIG. 5 is a sectional view of the probe in accordance with Embodiment 1.
  • FIG. 6 is an enlarged sectional view of the probe in accordance with Embodiment 1.
  • FIG. 7 is a perspective view of the probe in accordance with Embodiment 1.
  • FIG. 8 is a perspective view of the probe for illustrating its usage in accordance with Embodiment 1.
  • FIG. 9 is a schematic diagram of the probe in accordance with Embodiment 1.
  • FIG. 10 is a sectional view of the probe in accordance with Embodiment 1.
  • FIG. 11 is a sectional view of the probe in accordance with Embodiment 1.
  • FIG. 12 is a sectional view of the probe in accordance with Embodiment 1.
  • FIG. 13 is a sectional view of the probe in accordance with Embodiment 1.
  • FIG. 14 is a sectional view of the probe in accordance with Embodiment 1.
  • FIG. 15 is a plan view of another probe for measuring an electric potential of a cell in accordance with Embodiment 1.
  • FIG. 16A is an enlarged sectional view of the probe shown in FIG. 15.
  • FIG. 16B is an enlarged sectional view of still another probe for measuring an electric potential of a cell in accordance with Embodiment 1.
  • FIG. 17 is a sectional view of a probe for measuring an electric potential of a cell in accordance with Exemplary Embodiment 2 of the invention.
  • FIG. 18 is an enlarged sectional view of the probe in accordance with Embodiment 2.
  • FIG. 19A is a sectional view of the probe for illustrating its usage in accordance with Embodiment 2.
  • FIG. 19B is an enlarged sectional view of the probe shown in FIG. 19A.
  • FIG. 20 is an exploded perspective view of a probe for measuring an electric potential of a cell in accordance with Exemplary Embodiment 3 of the invention.
  • FIG. 21 is a sectional perspective view of the probe in accordance with Embodiment 3.
  • FIG. 22 is an enlarged sectional view of the probe in accordance with Embodiment 3.
  • FIG. 23 is a perspective view of a probe array for measuring an electric potential of a cell in accordance with Embodiment 3.
  • FIG. 24 is a sectional view of a conventional probe for measuring an electric potential of a cell.
    •  REFERENCE NUMERALS
    • 1 Probe for Measuring Electric Potential of Cell
    • 2 Plate
    • 2A Molded Plate
    • 2B Molded Plate
    • 3 Cavity (First Cavity)
    • 4 Sensor Element
    • 5 Cavity (Third Cavity)
    • 6 Cavity (Second Cavity)
    • 7 Supporting Substrate
    • 8 Thin Plate
    • 9 Through-Hole
    • 10 Flow Passage (Second Flow Passage)
    • 10A Opening (First Opening)
    • 11 Flow Passage (First Flow Passage)
    • 11A Opening (First Opening)
    • 12 Opening (Second Opening)
    • 13 Sucking Device
    • 15 Container (Pouring Device)
    • 16 Measurement Solution
    • 17 Bump
    • 18 Reference Electrode (First Electrode)
    • 19 Measuring Electrode (Second Electrode)
    • 20 Target Cell
    • 21 Culture Solution
    • 22 Opening (Second Opening)
    • 23 Valve
    • 26 Supporting Substrate
    • 27 Probe for Measuring Electric Potential of Cell
    • 28 Plate
    • 29 Sensor Element
    • 30 Thin Plate
    • 31 Through-Hole
    • 32 Cavity
    • 33 Microscope
    • 34 Patch Probe
    • 35 Target Cell
    • 36 Culture Solution
    • 37A, 37B Recess
    • 117 Bump
    • 501 Probe for Measuring Electric Potential of Cell
    • 502 Plate
    • 503 Cavity (First Cavity)
    • 504 Sensor Element
    • 505 Cavity (Third Cavity)
    • 506 Cavity (Second Cavity)
    • 507 Thin Plate
    • 508 Through-Hole
    • 509 Flow Passage (Second Flow Passage)
    • 510 Flow Passage (First Flow Passage)
    • 511 Opening (Second Opening)
    • 512 Supporting Substrate
    • 514 Reference Electrode (First Electrode)
    • 515 Measuring Electrode (Second Electrode)
    • 518 Opening (Second Opening)
    • 519 Probe Array for Measuring Electric Potential of Cell
    • 520 Well Array
    • 521A Through-Hole
    • 521B Through-Hole
    • 521C Through-Hole
    • 522 Well
    • 523 Well
    • 524 Well
    DETAIL DESCRIPTION OF THE PREFERRED EMBODIMENTS
  • Exemplary Embodiment 1
  • FIG. 1 is a perspective view of probe 1 for measuring an electric potential of a cell in accordance with Exemplary Embodiment 1 of the present invention. FIG. 2 is an exploded perspective view of probe 1. FIG. 3 is a sectional perspective view of probe 1. FIG. 4 is an enlarged sectional perspective view of probe 1. FIG. 5 is a sectional view of probe 1. FIG. 6 is an enlarged sectional view of an essential part of probe 1. Probe 1 includes sensor element 4 and plate 2 made of insulating material, such as resin or glass. Plate 2 has cavity 3 provided in upper surface 2C thereof. Sensor element 4 is fit into cavity 3. Cavity 6 is provided under bottom surface 3A of cavity 3. Cavity 6 is positioned under sensor element 4.
  • Plate 2 includes molded plate 2A and molded plate 2B attached onto plate 2A, and can be shaped in a complicated shape easily. Plate 2B has flow passages 10 and 11 having groove shapes. Plate 2A has openings 12 and 22 shaped like through-holes. Cavity 3 shaped like a through-hole and cavity 6 communicate with each other.
  • Cavity 6 communicates with openings 10A and 11A of flow passages 10 and 11 communicating with the outside of plate 2, respectively. Other openings 12 and 22 of flow passages 10 and 11 open to upper surface 2C of plate 2, respectively. The sectional area of each of flow passages 10 and 11 is not smaller than 0.01 mm2 to so as preventing flow passages 10 and 11 from being clogged and so as to enable the passages to be cleaned easily. Lower surface 6A of cavity 6 has bump 17 thereon projecting toward sensor element 4, i.e. projecting upward towards cavity 6. This structure enables the adjusting of the sectional areas of flow passages 10 and 11 and the sectional areas of the vicinity of openings 10A and 11A at cavity 6, so that solution to be used for measuring can move smoothly through flow passage 10, cavity 6, and flow passage 11.
  • Sensor element 4 includes supporting substrate 7 made of a silicon substrate or a laminated body including a silicon substrate and a silicon-dioxide film on the silicon substrate. Upper surface 7A of supporting substrate 7 faces towards a direction identical to a direction towards which upper surface 2C of plate 2 faces, and has cavity 5 provided therein. Thin plate 8 provides bottom surface 5A of cavity 5. Thin plate 8 has through-holes 9 having small diameters allowing upper surface 8A (bottom surface 5A of cavity 5) to communicate with lower surface 8B of thin plate 8. One opening 9A of each of through-holes 9 opens to cavity 5, and another opening 9B of each of through-holes 9 communicates with cavity 6 provided in plate 2.
  • Measuring electrode 19 made of platinum, gold, silver, or silver chloride is provided on lower surface 8B of thin plate 8, i.e., on lower surface 7B of supporting substrate 7 of sensor element 4. Measuring electrode 19 is connected with a lead electrode made of a wire or a thin-film electrode for which connecting the measuring electrode with a measuring instrument outside probe 1 for detecting a signal.
  • Sensor element 4 is bonded so securely into cavity 3 with an adhesive so that the solution (measurement solution) to be used for measurement filling passages 10 and 11 and cavity 6 can be prevented completely from leakage. Sensor element 4 may be bonded into cavity 3 by fusion bonding or ultrasonic bonding.
  • FIG. 7 is a perspective view of probe 1 for measuring an electric potential of a cell. Tube 24A is connected with opening 12 of flow passage 10. Tube 24B is connected with flow passage 11. Tube 24B is connected with sucking device 13, and tube 24A is connected with container 15. Valve 23 is provided between container 15 and opening 12 to stop the flow of fluid, such as the measurement solution, upon necessary. Sucking device 13 provides cavity 6 with decompressed atmosphere therein having a pressure lower than that in cavity 5. Sucking device 13 may be an ordinary pump, such as a diaphragm pump, a syringe pump, or sucking with a human mouth, and is not limited to these.
  • A method of measuring an electric potential of a cell with probe 1 will be described below.
  • FIG. 8 is a perspective view of probe 1 for illustrating its usage. Probe 1 is mounted to measuring stick 25. Probe 1 is fixed to end 25A of measuring stick 25. Tube 24A coupled with flow passage 10, tube 24B coupled with flow passage 11, and electrode wire 19A electrically coupled with measuring electrode 19 are arranged inside stick 25, and are drawn out from another end 25B of stick 25. Electrode wire 19A is connected with an external measuring instrument for supplying measured signals to the instrument.
  • FIG. 9 is a schematic diagram of probe 1 which being used. Measuring stick 25 having probe 1 mounted thereto is dipped into culture solution 21 stored in container 14. Target cells 20 float in solution 21. Reference electrode 18 contacts solution 21 in container 14, thus sensing an electric potential of solution 21 in container 14. Probe 1 is positioned so that sensor element 4 can be dipped in solution 21.
  • FIGS. 10 to 14 are sectional views of probe 1 for illustrating a method for measuring an electric potential of a cell with the probe.
  • As shown in FIG. 10, target cells 20 float above sensor element 4 in solution 21.
  • Next, as shown in FIG. 11, valve 23 is closed so that flow passages 10 and 11 and cavity 6 are shut off from container 15. Then, cavity 6 is decompressed by sucking device 13 to have a pressure therein lower than that in cavity 5. This operation causes solution 21 and cells 20 filling cavity 5 to be sucked towards through-holes 9, and then, causes solution 21 to flow into cavity 6. Each of cells 20 has a size larger than the sectional area of through-hole 9, and hence, does not pass through through-holes 9, thus being held at openings 9A of holes 9. Solution 21 flowing into cavity 6 contacts measuring electrode 19, thereby allowing an electric potential in cavity 6 to be detected. In this situation, a difference between respective electric potential of reference electrode 18 and measuring electrode 19, an electrical resistance between the electrodes, and a capacitance between the electrodes can be measured.
  • When target cells 20 are held at openings 9A of through-holes 9, sensor element 4 separates culture solution 21 into portion 21A in cavity 5 and portion 21B in cavity 6, thereby increases the resistance between reference electrode 18 and measuring electrode 19.
  • Then, cavity 6 is further decompressed by sucking device 13, and accordingly, as shown in FIG. 12, the surface of target cell 20 is urged more strongly onto opening 9A of hole 9, accordingly providing the resistance between electrodes 18 and 19 larger than that of the case that cell 20 is merely held at opening 9A. At this moment, the resistance exceeds 100MΩ and may exceed 1GSZ, which is called “Giga-Seal”. In the Giga-Seal, an ion-channel activity of cells 20 causes ion exchange between culture solution 21 and cells 20, thereby changing an inner electric potential of each of cells 20. This change can be detected as the difference between respective electric potentials of reference electrode 18 and measuring electrode 19.
  • The ion channel activity changes according to pharmaceutical contained in culture solution 21, and is detected as the difference of respective electrical potentials of electrodes 18 and 19 so as to detect an influence to target cells 20, thus allowing a pharmaceutical chemically effect to cells 20 to be determined.
  • Reference electrode 18 and measuring electrode 19 are arranged near openings 9A and 9B of through-holes 9, respectively, to measure the electric potential difference around cell 20 accurately. Probe 1 can catch cells 20 floating in solution 21 easily to provide the Giga-Seal.
  • Upper surface 2A of plate 2 is flush with upper surface 7A of supporting substrate 7, and hence, solution 21 including cells 20 can be directly supplied onto upper surface 7A of supporting substrate 7 or into cavity 5 with a plate pipette, as shown in FIG. 13. This arrangement allows cells 20 to be observed easily with a microscope from above upper surface 2C of plate 2. Further, this arrangement allows bubbles produced around cells 20 to be removed easily, accordingly enabling the pharmaceutical to be applied to cells 20 without fail.
  • When valve 23 is opened in the Giga-Seal shown in FIG. 12, measurement solution 16 in container 15 is sucked into flow passage 10 and cavity 6, as shown in FIG. 14. Thus, container 15 functions as a pouring device for introducing measurement solution 16 into flow passage 10. Flow passage 11 is decompressed by sucking device 13, and accordingly, portion 21B of solution 21 in cavity 6 is replaced by measurement solution 16. Measurement solution 16, including a large concentration of K+, allows the change in the electrical potential of cells 20 to be measured more accurately.
  • Reference electrode 18 and measuring electrode 19 may be formed near openings 9A and 9B of through-holes 9 by a thin-film technique to detect the change in the electric potential of target cell 20.
  • FIG. 15 is a plan view of another probe 1A for measuring an electric potential of a cell in accordance with Embodiment 1. Each of flow passages 110 and 111 has a curved portion. This structure provides a large resistance to the flow of the fluid passing through passages 110 and 111, accordingly preventing culture solution 21 and measurement solution 16 flowing into cavity 6 from leaking to outside, and from having bubbles in the solutions from outside.
  • FIG. 16A is an enlarged sectional view of probe 1A at line 16-16 shown in FIG. 15. Pocket 37A having a diameter larger than that of through-hole 9 is provided at opening 9A of through-hole 9 facing cavity 5 as to catch the target cell more securely.
  • FIG. 16B is an enlarged sectional view of still another probe 1B in accordance with Embodiment 1. In probe 1B, pocket 37B having a diameter larger than that of through-hole 9 is provided at openings 9B of through-holes 9 facing cavity 6. This structure stabilizes the fluidity of culture solution 21 in cavity 6 and the fluidity of measurement solution 16 near openings 9B of through-holes 9.
  • As shown in FIGS. 16A and 16B, edge 117A of bump 117 and edge 6B of cavity 6 are chamfered to have rounded shapes, thereby allowing measurement solution 16 to flow smoothly.
  • The insulating material, resin or glass, of plate 2 may be transparent to transmit visible light through the material. This structure allows the user to observe openings 9A of through-holes 9 easily from cavity 6 with a microscope. Hence, monitoring culture solution 21 and measurement solution 16 flowing into cavity 6 as well as presence of bubbles, a user can measure the electric potential of target cell 20.
  • Thin plate 8 of sensor element 4 may be made of transparent material, such as resin or glass, transmitting visible light therein. This structure allows a user to observe target cell 20 from below the lower surface of plate 2 with a microscope.
    • Exemplary Embodiment 2
  • FIG. 17 is a sectional view of probe 27 for measuring an electric potential of a cell in accordance with Exemplary Embodiment 2 of the present invention. FIG. 18 is an enlarged sectional view of sensor element 29 of probe 27. Components identical to those of Embodiment 1 are denoted by the same reference numerals, and their descriptions will be omitted.
  • Probe 27 includes plate 28 and sensor element 29. Upper surface 28C of plate 28 has cavity 83 provided therein. Cavity 6 is provided in bottom surface 83A of cavity 83. Sensor element 29 is fit into cavity 83. Sensor element 29 includes supporting substrate 26. Supporting substrate 26 has lower surface 26 B having cavity 32 provided therein. Thin plate 30 is provided at bottom surface 32A of cavity 32. Thin plate 30 has through-holes 31 allowing upper surface 30A of plate 30 to communicate with lower surface 30B (bottom surface 32A of cavity 32) of plate 30. Opening 31A of each of through-holes 31 opens at upper surface 30A of thin plate 30 (upper surface 26A of supporting substrate 26) and communicates with the outside. Opening 31B of each of through-holes 31 opens at lower surface 30B of thin plate 30 and communicates with cavity 32 and cavity 6. Thus, through-holes 31 communicate with flow passages 10 and 11 via cavity 6 provided in plate 28. Measuring electrode 19 is provided on lower surface 30B of thin plate 30 upon necessary.
  • FIG. 19A is a sectional view of probe 27 for illustrating its usage. FIG. 19B is an enlarged sectional view of probe 27 shown in FIG. 19A. Similarly to probe 1 of Embodiment 1, upper surface 26A of supporting substrate 26 of sensor element 29 is flush with upper surface 28C of plate 28, so that no bump or dip is provided thereon. This structure allows target cell 35 to be observed more closely to the cell with microscope 33. Observing cells 35 with microscope 33, a user can attach patch probe 34 to cell 35. This operation allows the user to measure ion-channel activity at plural portions of cell 35. For instance, when pharmaceutical is put into culture solution 36, the probe can detect simultaneously two electric potentials: an electric potential of patch probe 34 attached to portion 35A near an applying position where cell 35 is supplied; and an electric potential of measuring electrode 19 near portion 35B of cell 35 caught at through-holes 31. Portion 35A is farther from the applying position than portion 35A. This simultaneous detection of those two electric potentials allows a transferring state from portion 35A to portion 35B of ion-channel activity in cell 35 to be detected.
  • As well as probe 1, plate 2, and supporting substrate 7 of Embodiment 1, plate 28 and thin plate 30 of probe 27 may be made of transparent material transmitting visible light therethrough, providing effects similar to those of Embodiment 1.
    • Exemplary Embodiment 3
  • FIG. 20 is an exploded perspective view of probe 501 for measuring an electric potential of a cell in accordance with Exemplary Embodiment 3 of the present invention. FIG. 21 is a sectional perspective view of probe 501. FIG. 22 is an enlarged sectional view of an essential part of probe 501. Probe 501 includes plate 502, sensor element 504, and well array 520. Plate 502 is made of insulating material, such as resin or glass. Upper surface 502C of plate 502 has cavity 503 provided therein. Bottom surface 503A of cavity 503 has cavity 506 provided therein. Sensor element 504 is fit into cavity 503. Cavity 506 is positioned below sensor element 504.
  • Cavity 506 is connected with flow passages 509 and 510 communicating with the outside. Flow passage 509 has opening 511 thereof provided in upper surface 502C of plate 502. Flow passage 510 has opening 518 thereof provided at upper surface 502C. Flow passages 509 and 510 communicate with the outside of plate 502. Molded plate 502A previously molded is stuck on molded plate 502B previously molded, thus providing plate 502. Flow passages 509 and 510 having groove shapes are provided in molded plate 502B. Openings 511 and 518 shaped like through-holes are provided in molded plate 502A. Cavities 503 and 506 provided in molded plate 502A are shaped like a through-hole and communicate with each other. Sensor element 504 includes supporting substrate 512 and thin plate 507. As shown in FIG. 22, cavity 505 is provided below thin plate 507 (at the side of lower surface 512B of plate 502 opposite to upper surface 502C about plate 502). In other words, thin plate 507 provides bottom surface 505A of cavity 505. Thin plate 507 has small through-holes 508 allowing upper surface 507A (upper surface 512A of supporting substrate 512) to communicate with lower surface 507B. Openings 508A of through-holes 507 provided at upper surface 507A (upper surface 512A of supporting substrate 512) hold target cells, respectively. Through-holes 508 necessarily have diameters smaller than the sizes of the target cells. Similarly to the probe shown in FIG. 16A, a pocket having a diameter larger than that of through-hole 508 may be provided at each of openings 508A to hold the target cell securely and stably. Each of through-hole 508 has opening 508B which opens to cavity 505 at lower surface 507B (lower surface 505A of cavity 505) of thin plate 507. Opening 508A of through-hole 508 communicates with upper surface 512A of substrate 512 of sensor element 504. Opening 508B of through-hole 508 communicates with cavity 506 via cavity 505. This structure allows liquid, such as culture solution and chemicals, to flow in through-holes 508 and cavities 505 and 506.
  • In sensor element 504, thin pate 507 is placed at the upper part, that is, upper surface 512A of supporting substrate 512 and upper surface 502C of plate 502 are positioned in a single, common plane. However, similarly to the probe shown in FIG. 6 in accordance with Embodiment 1, cavity 505 may be provided in upper surface 512A of supporting substrate 512.
  • Well array 520 is placed on upper surface 502A of plate 502. Well array 520 has a predetermined capacity for receiving, storing, or circulating liquid, such as culture solution and chemicals, therein. Well array 520 has wells 522, 523, and 524 provided therein. Lower surface 522A of well 522 has through-hole 521A provided therein and communicates with opening 511 of flow passage 509. Lower surface 523A of well 523 has through-hole 521B provided therein and communicates with through-hole 508 provided in thin plate 507 of sensor element 504. Lower surface 524A of well 524 has through-hole 521C provided therein and communicates with opening 518 of flow passage 510. Wells 522, 523, and 524 have openings 522B, 523B, and 524B at their tops, respectively, for receiving culture solution or chemicals. Reference electrode 514 is provided in well 523. Measuring electrode 515 is provided in flow passage 510 and is drawn out to the outside of plate 502.
  • Culture solution containing the target cells is introduced into well 523 from opening 523B, and is sucked from opening 524B of well 524 with a sucking device, such as a suction pump. The culture solution accordingly flows in through-holes 508 and is sucked into well 524 via cavities 505 and 506, flow passage 510, and opening 518. Alternately, measurement solution or culture solution is introduced into well 522, and is sucked from well 524. Then, the solution sufficiently fills flow passages 509 and 510 and cavities 505 and 506, and is prevented from producing bubbles therein, thereby providing accurate measurement. In this case, the measurement solution may be introduced preferably before the target cells are input in well 523 so as to sufficiently fill flow passages 509 and 510. Then, opening 522 of well 522 is closed, and after that, the cells are input into well 523 while the measurement solution is sucked from well 524.
  • Since through-holes 508 of sensor element 504 have the diameters small enough to preventing the target cells from passing through the holes, the cells can be held at openings 508A of holes 508, thereby having electric potentials measured while held at through-holes 508. According to Embodiment 3, thin plate 507 has plural through-holes 508 provided therein, thus measuring the electric potentials of the cells at once. After the target cells clogs all of through-holes 508, the other cells remain in well 523. Then, the amount of the culture solution flowing into cavity 505 accordingly decreases, and it is accordingly detected that the cells are held at openings 508A of through-holes 508. This operation can be performed by controlling a suctioning force at well 524 while measuring a flow rate of the culture solution. The suctioning may be performed from well 522, providing the same effects.
  • Opening 523B of well 523 is closed. Then, chemicals is introduced into well 522 and is sucked from well 524 with the sucking device, accordingly flowing in through-hole 521A, through opening 511, flow passage 509, cavities 506 and 505, flow passage 510, and opening 518, and then being sucked into well 524. At this moment, the chemicals contact, through openings 508B of holes 508, the target cells trapped at openings 508A of through-holes 508, causing the cells to react with the chemicals. The electric potentials of the cells produced due to the reaction can be measured through reference electrode 514 contacting the culture solution in well 523 and through measuring electrode 515 contacting the chemicals in flow passage 510.
  • Probe 501 allows liquids, such as culture solution and chemicals, different from each other to be introduced into well 523 having the target cells therein and flow passage 510 having measuring electrode 515 therein, respectively. Sucking the solution between well 522 and well 524 allows one solution to be replaced easily by the other solution.
  • Well array 520 having three wells 522, 523, and 524 and its usage have been described. There is a case that chemicals, instead of the culture solution, are introduced into well 523 to measure just the electric potential of the cells after the target cells are held at small through-holes 508. In this case, the well array may have only two wells (for example, wells 523 and 524) therein as to perform the measurement.
  • Upper surface 502C of plate 502 is attached securely onto bottom surface 520A of well array 520 to enable well array 520 to seal plate 502 securely, thereby preventing the solution securely from leakage.
  • Well array 520 may be made of material identical to that of plate 502, hence preventing their deformation due to a difference between respective expansion coefficients of the materials, and thereby sealing plate 502 securely.
  • Well array 520 and plate 502 may be made of thermoplastic resin, such as polystyrene, cycloolefin polymer, or cycloolefin copolymer, hence providing a secure sealing by ultrasonic fusion or laser welding, and allowing probe 501 to be manufactured at a high productivity.
  • Well array 520 and plate 502 may be made of glass material or quartz material. These materials can have surfaces directly bonded onto each other without an adhesive if the surfaces are polished to be finished in mirror-like. Each of these materials has a large resistance to heat, thus being bonded to each other with non-organic adhesive, such as glass adhesive or ceramic adhesive. Well array 520 and plate 502 made of these materials have large heat resistance, hence providing probe 501 re-usable by heat-washing.
  • As shown in FIG. 21, at least through-hole 521B out of through- holes 521A, 521B, and 521C provided in lower surfaces 522A, 523A, and 524A of wells 522, 523, and 524, respectively, may flare toward opening 523B of well 523, that is, may taper towards through-hole 508 of sensor element 504. This structure introduces the culture solution or chemicals, which are put into well 523, into through-holes 508 of sensor element 504 quickly.
  • As shown in FIG. 21, through-hole 521B has a size larger than that of thin plate 507 having through-holes 508 provided therein, allowing the target cells to be introduced efficiently into through-holes 508. Well array 520 has well 523 having the culture solution containing the target cells input thereinto, well 522 having the chemicals input thereinto, and well 524 coupled with the sucking device. This structure allows upper surface 502C of plate 502 to hold the target cells easily, and allows operations, such as the inputting of the chemicals, to be performed independently from above well array 520, thus allowing probe 501 to be manipulated easily for measuring the electric potential.
  • Through-hole 521A of well 522 has a size larger that of opening 511 of flow passage 509, and through-hole 521C of well 524 has a size larger than that of opening 518 of flow passage 510. This structure can introduce liquid, such as the chemicals, quickly into the flow passages, allowing probe 501 to measure the electric potential of the cells accurately with little variation.
  • Reference electrode 514 is provided in well 523 at a predetermined position contacting the culture solution. Measuring electrode 515 is provided in flow passage 510 and contacts the liquid, such as the culture solution or the chemicals, in flow passage 510. This structure can measure an electric potential of the target cell in the culture solution and an electric potential of the cell after the liquid, such as the chemicals is input from well 522 or well 523, thus measuring the change between the above potentials. Measuring electrode 515 may be provided near cavity 505 or cavity 506.
  • Reference electrode 514 and measuring electrode 515 are made of wires or thin-film electrodes, and are coupled to a measuring instrument outside probe 501 for detecting signals from those electrodes.
  • A method of measuring an electric potential of the cells with probe 501 will be described below.
  • First, the culture solution containing the target cells is introduced into well 523, and is sucked with by the sucking device from well 522 or well 524 for holding the cells at through-holes 508 of sensor element 504. An electric resistance between reference electrode 514 which contacts the culture solution and is provided in well 523, and measuring electrode 515 provided in flow passage 510 is measured. A suctioning pressure of the suction device is controlled so that the resistance between electrodes 514 and 515, that is, the resistance between the culture solution stored in well 523 and the culture solution stored in flow passage 510 exceeds 100 MΩ. Reference electrode 514 and measuring electrode 515 are made of conductive material, such as Au, Ag, or AgCl, and contact the culture solution to be connected electrically with the solution. Therefore, the positions of electrodes 514 and 515 are not limited to the positions described in above.
  • Next, the measurement solution, such as chemicals, are stored in well 522 and is sucked from well 524, thereby causing the culture solution in flow passage 509, cavities 505 and 506, and flow passage 510 to be replaced by the measurement solution. Thus, solutions, such as the culture solution and the measurement solution, different from each other can be introduced easily into well 523 having the cells therein and cavity 506 having measuring electrode 515 therein, respectively. This operation allows the electric potential of the cells to be measured quickly.
  • Even if respective functions of well 522 and well 524 are replaced by each other, the electric potential of the cells can be measured.
  • Wells 522, 523, and 524 may have valves or lids, allowing the measurement of the electric potentials with probe 5 to be controlled easily.
  • Another probe 519, probe array 519, including plural probes 501 in accordance with Embodiment 3 will be described below. FIG. 23 is an exploded perspective view of probe 519 (probe array 519) for measuring an electric potential of a cell. Probes 501 are arranged in a matrix having four rows and eight columns. Plural well arrays 520 each having wells 522, 523, and 524 can be manufactured at once as well array unit 520A.
  • Probe array 519 including plural probes 501 arranged in a predetermined arrangement allows a robot to pour the chemicals, to input cells, and to suck the cells. Thus, probe 519 can measure respective electric potentials of a lot of cells in a short time for determining pharmacological effect, thus screening candidate pharmaceuticals quickly.
    • INDUSTRIAL APPLICABILITY
  • A probe for measuring an electric potential of a cell according to the present invention can measure electric potentials of cells floating in solution as they are in environment, hence being used for determining pharmacological effects to the cells and for screening pharmaceuticals.

Claims (29)

1-33. (canceled)
34. A probe for measuring an electric potential of a cell, said probe being arranged to be used with a sucking device, said probe comprising:
a plate made of resin and having a surface, the plate having a first cavity provided in the surface of the plate, a second cavity, and a first flow passage provided in the plate, the first cavity having a bottom surface, the second cavity being provided in the bottom surface of the first cavity, the first flow passage having a first opening and a second opening, the first opening of the first flow passage opening to the second cavity, the second opening of the first flow passage opening outside the plate; and
a sensor element made of silicon and provided in the first cavity, the sensor element including
a thin plate having a first surface and a second surface opposite to the first surface of the thin plate, the thin plate having a through-hole provided therein, the through-hole having a first opening and a second opening, the first opening of the through-hole opening to the first surface of the thin plate, the second opening of the through-hole opening to the second surface of the thin plate and connected with the second cavity of the plate, and a supporting substrate provided around the thin plate and in the first cavity of the plate,
wherein the first flow passage allows fluid to flow therein, and the sucking device is arranged to be coupled with the second opening of the first flow passage so as to suck the fluid flowing in the first flow passage, and
wherein the second opening of the second flow passage is arranged to be coupled to a pouring device, and the pouring device is operable to put fluid into the second opening of the second flow passage.
35. The probe of claim 34, wherein the bottom surface of the first cavity and the second surface of the thin plate of the sensor element are flush with each other.
36. The probe of claim 35, wherein
the supporting substrate of the sensor element have a first surface and a second surface, the first surface of the supporting substrate facing towards a direction identical to a direction towards which the surface of the plate faces, the second surface of the supporting substrate is provided on the bottom surface of the first cavity of the plate, and
a third cavity is provided on the first surface of the thin plate.
37. The probe of claim 34, wherein the supporting substrate of the sensor element is bonded to the plate.
38. The probe of claim 34, wherein the plate further have a second flow passage provided therein, the second flow passage having a first opening and a second opening, the first opening of the second flow passage opening to the second cavity, the second opening of the second flow passage opening outside the plate.
39. The probe of claim 38, wherein the second opening of the second flow passage is arranged to be coupled to a pouring device, and the pouring device is operable to put fluid into the second opening of the second flow passage.
40. The probe of claim 34, wherein a valve is arranged to be connected between the pouring device and the second flow passage.
41. The probe of claim 38, wherein at least one of the first flow passage and the second flow passage has a curved portion.
42. The probe of claim 38, wherein the plate includes a bump which is provided between the first flow passage and the second flow passage and 10 which projects toward the second cavity.
43. The probe of claim 34, further comprising electrodes provided on the sensor element around the first opening of the through-hole and the second opening of the through-hole, respectively.
44. The probe of claim 34, wherein the thin plate of the sensor element has a pocket provided therein at at least one of the first opening of the through-hole and the second opening of the through-hole of the thin plate, the pocket having a diameter larger than a diameter of the through-hole of the thin plate.
45. The probe of claim 34, wherein the surface of the plate and the first surface of the thin-plate of the sensor element are flush with each other.
46. The probe of claim 45, wherein
the supporting substrate of the sensor element have a first surface and a second surface, the first surface of the supporting substrate facing towards a direction identical to a direction towards which the surface of the plate faces, the second surface of the supporting substrate is provided on the bottom surface of the first cavity of the plate, and
a third cavity is provided on the first surface of the thin plate.
47. The probe of claim 34, further comprising a well array having a first well, a second well, and a third well provided therein, the first well, the second well, and the third well having openings and bottom surfaces, respectively, wherein
the bottom surface of the first well has a through-hole which is provided therein and which communicates with the second opening of the first flow passage,
the bottom surface of the second well has a through-hole which is provided therein and which communicates with the through-hole of the thin plate of the sensor element, and
the bottom surface of the third well has a through-hole which is provided therein and which communicates with the second opening of the second flow passage.
48. The probe of claim 47, wherein the through-hole of the second well tapers toward the through-hole of the thin-plate of the sensor element.
49. The probe of claim 47, further comprising:
a first electrode provided in the second well; and
a second electrode provided in one of the third well and the first flow passage.
50. The probe of claim 47, wherein
fluid including a target cell is input in the second well,
fluid for detecting reaction with the target cell is input into the third well, and
the first well is coupled to the sucking device.
51. The probe of claim 47, wherein the second well is provided above the first surface of the thin plate of the sensor element.
52. The probe of claim 51, wherein the through-hole of the second well has a size larger than a size of the thin plate.
53. The probe of claim 47, wherein the through-hole of the first well is larger than the second opening of the first flow passage.
54. The probe of claim 47, wherein the through-hole of the third well is larger than the second opening of the second flow passage.
55. The probe of claim 47, wherein the well array has a bottom surface, the bottom surface of the well array having the through-hole of the first well, the through-hole of the second well, and the through-hole of the third well open thereto, the bottom surface of the well array and the surface of the plate is positioned in a plane.
56. The probe of claim 47, wherein the well array comprises material identical to material of the plate.
57. The probe of claim 47, wherein the plate and the well array comprise thermoplastic resin.
58. The probe of claim 47, further comprising:
another plate having a plurality of openings provided therein; and another sensor element including another thin plate, the another thin plate having a plurality of through-holes opening in a direction identical to a direction in which the plurality of openings of the another plate open,
wherein the well array further has a plurality of other wells, each of the other wells having bottom surfaces, the bottom surfaces of the other wells having a plurality of through-holes provided therein, respectively, and the plurality of through-holes of the other wells communicate with the plural openings of the another plate and the plurality of through-holes of the another sensor element, respectively.
59. The probe of claim 34, the resin is exposed to the first flow passage entirely from the first opening of the first flow passage to the second opening of the first flow passage.
60. The probe of claim 38, the resin is exposed to the second flow passage entirely from the first opening of the second flow passage to the second opening of the second flow passage.
61. The probe of claim 34, further comprising:
a first tube connected to the second opening of the first flow passage to suck the fluid through the first tube; and
a second tube connected to the second opening of the second flow passage to put the fluid into the second flow passage through the second tube.
US12/712,370 2004-08-25 2010-02-25 Probe for measuring electric potential of cell Abandoned US20100147682A1 (en)

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Cited By (3)

* Cited by examiner, † Cited by third party
Publication number Priority date Publication date Assignee Title
US20110006303A1 (en) * 2008-03-18 2011-01-13 Canon Kabushiki Kaisha Semiconductor apparatus manufacturing method and semiconductor apparatus
US9932239B2 (en) 2010-04-27 2018-04-03 Panasonic Intellectual Property Management Co., Ltd. Sheet-like fiber structure, and battery, heat insulation material, waterproof sheet, scaffold for cell culture, and holding material each using the sheet-like fiber structure
CN109473614A (en) * 2017-09-08 2019-03-15 莫仕连接器(成都)有限公司 Battery connection module

Families Citing this family (12)

* Cited by examiner, † Cited by third party
Publication number Priority date Publication date Assignee Title
US8202439B2 (en) 2002-06-05 2012-06-19 Panasonic Corporation Diaphragm and device for measuring cellular potential using the same, manufacturing method of the diaphragm
US20100019756A1 (en) * 2006-05-17 2010-01-28 Matsushita Electric Industrial Co., Ltd. Device for measuring cellular potential, substrate used for the same and method of manufacturing substrate for device for measuring cellular potential
US8445263B2 (en) * 2006-07-06 2013-05-21 Panasonic Corporation Device for cellular electrophysiology sensor, cellular electrophysiology sensor using the device, and method for manufacturing the cellular electrophysiology sensor device
JP4811251B2 (en) * 2006-11-30 2011-11-09 パナソニック株式会社 Cell electrophysiological sensor
JP5011984B2 (en) * 2006-12-01 2012-08-29 パナソニック株式会社 Cell electrophysiological sensor
KR20080060661A (en) * 2006-12-27 2008-07-02 삼성전자주식회사 Device for providing hybridization chambers whose structure prevents air bubbles and hybridization device comprising the same device
KR101414232B1 (en) * 2007-08-02 2014-08-06 삼성전자 주식회사 Biochip package and biochip packaging substrate
US8643383B2 (en) * 2011-01-28 2014-02-04 Rockwell Automation Technologies, Inc. Drive failure protection
WO2015115448A1 (en) * 2014-01-30 2015-08-06 並木精密宝石株式会社 Cell membrane observation and analysis device and cell membrane observation and analysis method
JP6472664B2 (en) * 2014-04-14 2019-02-20 日置電機株式会社 Measuring apparatus and measuring method
JP6806787B2 (en) * 2016-03-21 2021-01-06 オンテラ インコーポレイテッド Wafer-scale assembly of insulator-membrane-insulator devices for nanopore sensing
US11458467B2 (en) * 2019-08-06 2022-10-04 Bio-Rad Laboratories Inc. Structures to define flow confinement shape and confinement stability with uniform aspiration

Citations (22)

* Cited by examiner, † Cited by third party
Publication number Priority date Publication date Assignee Title
US2366654A (en) * 1942-05-04 1945-01-02 Lincoln Eng Co Pump
US4704255A (en) * 1983-07-15 1987-11-03 Pandex Laboratories, Inc. Assay cartridge
US5183744A (en) * 1988-10-26 1993-02-02 Hitachi, Ltd. Cell handling method for cell fusion processor
US6046056A (en) * 1996-06-28 2000-04-04 Caliper Technologies Corporation High throughput screening assay systems in microscale fluidic devices
US20010046706A1 (en) * 1999-07-21 2001-11-29 Boris Rubinsky Controlled electroporation and mass transfer across cell membranes
US20010052460A1 (en) * 2000-02-23 2001-12-20 Ring-Ling Chien Multi-reservoir pressure control system
US20020063067A1 (en) * 2000-10-02 2002-05-30 Morten Bech System for electrophysiological measurements
WO2002055653A1 (en) * 2001-01-09 2002-07-18 Matsushita Electric Industrial Co., Ltd. Device for measuring extracellular potential, method of measuring extracellular potential by using the same and apparatus for quickly screening drug provided therewith
US20030032946A1 (en) * 2001-06-29 2003-02-13 Fishman Harvey A. Artificial synapse chip interface for electronic prosthetic retina
US20030107386A1 (en) * 1999-12-24 2003-06-12 John Dodgson Apparatus for and method of making electrical measurements of objects
US20030121778A1 (en) * 1999-12-24 2003-07-03 John Dodgson Apparatus for and method of making electrical measurements on an object
US20030132109A1 (en) * 2001-11-30 2003-07-17 Andrew Bullen Pipette configurations and arrays thereof for measuring cellular electrical properties
US6682649B1 (en) * 1999-10-01 2004-01-27 Sophion Bioscience A/S Substrate and a method for determining and/or monitoring electrophysiological properties of ion channels
US20040033483A1 (en) * 2001-08-09 2004-02-19 Hiroaki Oka Cell diagnosing method, and device and apparatus use for it
US6776896B1 (en) * 2000-10-11 2004-08-17 Axon Instruments, Inc. Method of positioning cells for electrophysiological testing
US20050058990A1 (en) * 2001-03-24 2005-03-17 Antonio Guia Biochip devices for ion transport measurement, methods of manufacture, and methods of use
US20050221469A1 (en) * 2003-03-07 2005-10-06 Matsushita Electric Industrial Co., Ltd. Extracellular potential measuring device and its manufacturing method
US6984297B2 (en) * 1999-10-08 2006-01-10 NMI Naturwissenschaftliches und Medizinisches Institut an der Universität Tübingen Device for taking measurements of cells which are contained in a liquid environment
US7006929B2 (en) * 2001-06-05 2006-02-28 Matsushita Electric Industrial Co., Ltd. Signal detecting sensor provided with multi-electrode
US20060163063A1 (en) * 2002-08-28 2006-07-27 Commissariat A L'energie Atomique Device for measuring the electrical activity of biological elements and its applications
US7501278B2 (en) * 2002-06-05 2009-03-10 Panasonic Corporation Extracellular potential measuring device and method for fabricating the same
US20090263648A1 (en) * 2005-10-19 2009-10-22 Mitsuo Saitoh Method of forming metal oxide film, metal oxide film and optical electronic device

Family Cites Families (13)

* Cited by examiner, † Cited by third party
Publication number Priority date Publication date Assignee Title
JP2829005B2 (en) 1988-11-11 1998-11-25 株式会社日立製作所 Micro-chamber plate, cell detection method, treatment method and apparatus using the same, and cell
FR2754716B1 (en) * 1996-10-18 1998-11-13 Synthelabo HANDPIECE FOR SURGICAL WASHING DEVICE
EP0938674B1 (en) * 1996-11-16 2005-06-01 NMI Naturwissenschaftliches und Medizinisches Institut an der Universität Tübingen in Reutlingen Stiftung Bürgerlichen Rechts Array of microelements, method of contacting cells in a liquid environment and method for the production of an array of microelements
AU746580B2 (en) * 1997-12-17 2002-05-02 Ecole Polytechnique Federale De Lausanne Positioning and electrophysiological characterization of individual cells and reconstituted membrane systems on microstructured carriers
DK1221046T3 (en) 1999-10-01 2006-06-12 Sophion Bioscience As Assembly and method for determining and / or monitoring electrophysiological properties of ion channels
JP2004000163A (en) * 2002-03-29 2004-01-08 Shimadzu Corp Cell used for treating cell
JP3945317B2 (en) 2002-06-05 2007-07-18 松下電器産業株式会社 Extracellular potential measuring device and manufacturing method thereof
JP3925439B2 (en) 2003-03-07 2007-06-06 松下電器産業株式会社 Extracellular potential measuring device and manufacturing method thereof
JP3861831B2 (en) 2003-03-07 2006-12-27 松下電器産業株式会社 Extracellular potential measuring device and manufacturing method thereof
JP3945338B2 (en) 2002-08-01 2007-07-18 松下電器産業株式会社 Extracellular potential measuring device and manufacturing method thereof
KR100471747B1 (en) * 2002-08-23 2005-03-16 재단법인서울대학교산학협력재단 Micro Channel
WO2004038410A1 (en) * 2002-10-24 2004-05-06 Sophion Bioscience A/S Apparatus and method for determining &/or monitoring electrophysiological properties of ion channels
WO2005116242A1 (en) * 2004-05-31 2005-12-08 Matsushita Electric Industrial Co., Ltd. Medicine safety testing method and medicine safety testing system

Patent Citations (23)

* Cited by examiner, † Cited by third party
Publication number Priority date Publication date Assignee Title
US2366654A (en) * 1942-05-04 1945-01-02 Lincoln Eng Co Pump
US4704255A (en) * 1983-07-15 1987-11-03 Pandex Laboratories, Inc. Assay cartridge
US5183744A (en) * 1988-10-26 1993-02-02 Hitachi, Ltd. Cell handling method for cell fusion processor
US6046056A (en) * 1996-06-28 2000-04-04 Caliper Technologies Corporation High throughput screening assay systems in microscale fluidic devices
US20010046706A1 (en) * 1999-07-21 2001-11-29 Boris Rubinsky Controlled electroporation and mass transfer across cell membranes
US6682649B1 (en) * 1999-10-01 2004-01-27 Sophion Bioscience A/S Substrate and a method for determining and/or monitoring electrophysiological properties of ion channels
US6984297B2 (en) * 1999-10-08 2006-01-10 NMI Naturwissenschaftliches und Medizinisches Institut an der Universität Tübingen Device for taking measurements of cells which are contained in a liquid environment
US20030121778A1 (en) * 1999-12-24 2003-07-03 John Dodgson Apparatus for and method of making electrical measurements on an object
US20030107386A1 (en) * 1999-12-24 2003-06-12 John Dodgson Apparatus for and method of making electrical measurements of objects
US20010052460A1 (en) * 2000-02-23 2001-12-20 Ring-Ling Chien Multi-reservoir pressure control system
US20020063067A1 (en) * 2000-10-02 2002-05-30 Morten Bech System for electrophysiological measurements
US6776896B1 (en) * 2000-10-11 2004-08-17 Axon Instruments, Inc. Method of positioning cells for electrophysiological testing
US20030113833A1 (en) * 2001-01-09 2003-06-19 Hiroaki Oka Device for measuring extracellular potential, method of measuring extracellular potential by using the same and apparatus for quickly screening drug provided therewith
WO2002055653A1 (en) * 2001-01-09 2002-07-18 Matsushita Electric Industrial Co., Ltd. Device for measuring extracellular potential, method of measuring extracellular potential by using the same and apparatus for quickly screening drug provided therewith
US20050058990A1 (en) * 2001-03-24 2005-03-17 Antonio Guia Biochip devices for ion transport measurement, methods of manufacture, and methods of use
US7006929B2 (en) * 2001-06-05 2006-02-28 Matsushita Electric Industrial Co., Ltd. Signal detecting sensor provided with multi-electrode
US20030032946A1 (en) * 2001-06-29 2003-02-13 Fishman Harvey A. Artificial synapse chip interface for electronic prosthetic retina
US20040033483A1 (en) * 2001-08-09 2004-02-19 Hiroaki Oka Cell diagnosing method, and device and apparatus use for it
US20030132109A1 (en) * 2001-11-30 2003-07-17 Andrew Bullen Pipette configurations and arrays thereof for measuring cellular electrical properties
US7501278B2 (en) * 2002-06-05 2009-03-10 Panasonic Corporation Extracellular potential measuring device and method for fabricating the same
US20060163063A1 (en) * 2002-08-28 2006-07-27 Commissariat A L'energie Atomique Device for measuring the electrical activity of biological elements and its applications
US20050221469A1 (en) * 2003-03-07 2005-10-06 Matsushita Electric Industrial Co., Ltd. Extracellular potential measuring device and its manufacturing method
US20090263648A1 (en) * 2005-10-19 2009-10-22 Mitsuo Saitoh Method of forming metal oxide film, metal oxide film and optical electronic device

Cited By (4)

* Cited by examiner, † Cited by third party
Publication number Priority date Publication date Assignee Title
US20110006303A1 (en) * 2008-03-18 2011-01-13 Canon Kabushiki Kaisha Semiconductor apparatus manufacturing method and semiconductor apparatus
US8546801B2 (en) * 2008-03-18 2013-10-01 Canon Kabushiki Kaisha Semiconductor apparatus manufacturing method and semiconductor apparatus
US9932239B2 (en) 2010-04-27 2018-04-03 Panasonic Intellectual Property Management Co., Ltd. Sheet-like fiber structure, and battery, heat insulation material, waterproof sheet, scaffold for cell culture, and holding material each using the sheet-like fiber structure
CN109473614A (en) * 2017-09-08 2019-03-15 莫仕连接器(成都)有限公司 Battery connection module

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US20070105183A1 (en) 2007-05-10
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