The present invention relates to a cell observation device, an electrical stimulation device, and a cell observation method for observing a reaction of a sample including a cell to electrical stimulation.
In the field of drug discovery screening, influence of a drug administered to a sample of cells or the like is evaluated by measuring light emitted from the cells in certain cases. Patent Literature 1 discloses a measurement device that monitors a biological response of cells to electric-field stimulation by fluorescence detection. This measurement device employs a configuration in which an electrode pair of a coaxial cable shape or a parallel flat plate shape including a positive electrode and a negative electrode can be located in each of wells in which the cells are placed. Patent Literature 2 discloses a measurement device that treats a membrane potential of a cell through the use of electrical stimulation. This measurement device includes an electrode pair of two parallel electrodes for generating an electric field in an observation area of a well.
Patent Literature 1: Japanese Unexamined Patent Publication No. 2005-514909
Patent Literature 2: Japanese Unexamined Patent Publication No. 2012-110327
In general, a microplate in which cells to be observed are arranged has a shape in which the bottom of each well is flat, but a microplate having a shape in which the bottom of each well is concave such as U-shaped has been recently used. When the microplate having such a shape is used, the measurement device described in Patent Literature 1 or Patent Literature 2 employs the electrode pair of a coaxial cable shape or the parallel electrodes and thus is likely to have difficulty in appropriately applying electrical stimulation to cells placed in the wells.
Therefore, the present invention has been accomplished in view of the above-mentioned problem and it is an object of the present invention to provide a cell observation device, an electrical stimulation device, and a cell observation method that can appropriately apply electrical stimulation to a cell placed in a holding unit.
The inventors of the present application found that a positional relationship of electrode pairs was important when electrical stimulation was applied to cells held in a sample case having a holding unit, which holds a sample including the cells, using the electrode pairs and a reaction of the cells thereto was observed, and have proposed the following configurations of the present invention.
That is, in order to achieve the above-mentioned object, according to an aspect of the present invention, there is provided a cell observation device for observing cell held by a sample case including a holding unit holding a sample including the cell, the cell observation device including: a mounting unit for holding the sample case thereon; an electrical stimulation unit including an electrode pair having a first electrode and a second electrode; and a position control unit for controlling a position of the electrical stimulation unit in a state in which the first electrode is disposed closer to the center of the holding unit than the second electrode when the electrode pair is disposed in the holding unit of the sample case, wherein a tip of the first electrode extends more than a tip of the second electrode.
Alternatively, according to another aspect of the present invention, there is provided an electrical stimulation device for being inserted into a sample case having a holding unit holding a sample including a cell and applying electrical stimulation to the cells, the electrical stimulation device including an electrode pair including a first electrode and a second electrode, wherein a tip of the first electrode extends more than a tip of the second electrode, and the first electrode is disposed closer to the center of the holding unit than the second electrode when the electrode pair is disposed in the holding unit of the sample case.
According to the cell observation device or the electrical stimulation device, by disposing the electrode pair including the first electrode and the second electrode in the holding unit formed in the sample case, it is possible to apply electrical stimulation to a sample including a cell using the electrode pair. Here, the tip of the first electrode disposed close to the center of the holding unit extends more than the tip of the second electrode disposed close to the circumference of the holding unit. Accordingly, even when the holding unit has a concave bottom, it is possible to cause the tip of the first electrode to easily approach the sample including a cell which is held on the bottom. As a result, it is possible to appropriately apply electrical stimulation to the sample from the electrode pair using only a simple position control mechanism and to obtain an appropriate evaluation result of the sample.
According to still another aspect of the present invention, there is provided a cell observation device for observing a cell held by a sample case including a holding unit holding a sample including the cell, the cell observation device including: a mounting unit fir holding the sample case thereon; an electrical stimulation unit including an electrode pair having a first electrode and a second electrode; a position control unit for controlling a position of the electrical stimulation unit such that the electrode pair is disposed in the holding unit of the sample case; and a position adjusting unit for adjusting a relative position of a tip of the first electrode to a tip of the second electrode.
Alternatively, according to still another aspect of the present invention, there is provided an electrical stimulation device for being inserted into a sample case having a holding unit holding a sample including a cell and applying electrical stimulation to the cells, the electrical stimulation device including: an electrode pair including a first electrode and a second electrode; and a position adjusting unit for adjusting a relative position of a tip of the first electrode to a tip of the second electrode.
Alternatively, according to still another aspect of the present invention, there is provided a cell observation method for observing a cell held by a sample case having a holding unit holding a sample including the cell, using an electrode pair including a first electrode and a second electrode, the cell observation method including: a step of adjusting a relative position of a tip of the first electrode to a tip of the second electrode; and a step of applying electrical stimulation to the sample using the electrode pair.
According to the cell observation device, the electrical stimulation device, or the cell observation method, by disposing the electrode pair including the first electrode and the second electrode in the holding unit formed in the sample case, it is possible to apply electrical stimulation to a sample including a cell using the electrode pair. Here, the relative position of the tip of the first electrode to the tip of the second electrode can be adjusted. Accordingly, even when the holding unit has a concave bottom, it is possible to cause the tip of the first electrode to easily approach the sample including a cell which is held on the bottom. As a result, it is possible to appropriately apply electrical stimulation to the sample from the electrode pair when the electrode pair is disposed in the holding unit and to obtain an appropriate evaluation result of the sample.
According to the present invention, it is possible to appropriately apply electrical stimulation to a cell disposed in a concave well.
Hereinafter, a cell observation device, an electrical stimulation device, and a cell observation method according to embodiments of the present invention will be described in detail with reference to the accompanying drawings. In the description of the drawings, the same elements will be referenced by the same reference signs and description thereof will not be repeated. It should be noted that each of the drawings was prepared for the purpose of description and made with special emphasis on objects of description. For this reason, dimensional ratios of members in the drawings do not always agree with actual ones.
The sample S includes predetermined cells. Examples of the predetermined cells include myocardial cells, muscle cells, which are differentiated from stem cells such as iPS (induced Pluripotent Stem) cells or ES (Embryonic Stem) cells, neurons, skin cells, photoreceptor cells, reproductive cells, and lever cells. The predetermined cells may be cells dyed with a membrane potential sensitive pigment, a calcium sensitive pigment, or a sodium ion sensitive pigment. The cell observation device, the electrical stimulation device, and the cell observation method according to this embodiment can be generally applied to optical measurement of measuring light such as phosphorescence and luminescence emitted from a sample as well as fluorescence measurement. The configuration of the cell observation device 1 will be described below.
The cell observation device 1 illustrated in
The microplate 20 which is used as a sample case in this embodiment is a plate-shaped member in which a plurality of wells (holding units) 21 are arranged in a two-dimensional array and has a configuration in which each of the plurality of wells 21 can hold a sample S, as illustrated in
The bottom face 22 of the microplate 20 is formed of a material (for example, glass, quartz glass, polyethylene, polypropylene, or polystyrene) which can transmit fluorescence-measuring excitation light applied to the sample S and fluorescent light emitted from the sample S. In general, in the cell observation device 1, the bottom face 22 of the microplate 20 only has to be formed of a material which can transmit light emitted from the sample S to be measured.
In the dark box 15, the microplate 20 is placed on a microplate holder (mounting unit) 11 having an opening for fluorescence observation. A microplate carrying mechanism 12 that carries the microplate 20 and the microplate holder 11 in a predetermined direction (a direction from right to left in
On one side of the dark box 15 which is an inlet side in the carrying direction of the microplate 20 in the carrying mechanism 12, an inlet-side microplate stacker 13 on which a predetermined number of (for example, 25) microplates 20 holding samples S before measurement are stacked is installed. On the other side of the dark box 15 which is an outlet side in the carrying direction of the microplate 20, an outlet-side microplate stacker 14 on which the microplate 20 after measurement is stacked is installed.
In this configuration, the microplate 20 carried in the dark box 15 from the inlet-side microplate stacker 13 is held by the microplate holder 11 and is carried by the carrying mechanism 12. The microplate 20 is temporarily stopped at the measurement position P, and necessary optical measurement is performed on the sample S held by the microplate 20 in this state. After the measurement is completed, the microplate 20 is carried again by the carrying mechanism 12 and is carried out to the outlet-side microplate stacker 14. In
Above the measurement position P at which the microplate 20 and the sample S are disposed at the time of optical measurement, an electrical stimulation unit (electrical stimulation device) 16 that is inserted into the well 21 of the microplate 20 and applies an electric field (electrical stimulation) to the sample S is installed. Below the measurement position P, a moving image acquiring unit 40 that is used to detect fluorescence emitted from the sample S accommodated in the well 21 via the bottom face 22 of the microplate 20 is installed.
The moving image acquiring unit 40 is moving image acquiring means for detecting a two-dimensional optical image representing a two-dimensional optical intensity distribution of the microplate 20 including light emitted from the sample S held in the well 21 of the microplate 20 and acquiring moving image data of the two-dimensional optical image. The detected two-dimensional optical image may be a optical intensity distribution including light emitted from the sample S held in at least one well 21. The moving image acquiring unit 40 includes an imaging device 45, a light-guiding optical system 41, an optical filer unit 42, and an excitation light source 43. The imaging device 45 has a two-dimensional pixel structure in which a plurality of pixels are two-dimensionally arranged and detects a fluorescent image which is a two-dimensional detected optical image based on fluorescence emitted from the sample S. For example, a camera equipped with an area image sensor such as a CCD image sensor or a CMOS image sensor with high sensitivity can be used as the imaging device 45. If necessary, the moving image acquiring unit 40 may be configured by disposing an image intensifier such as a micro channel plate (MCP), a relay lens, and the like in the front of the camera. The moving image acquiring unit 40 may acquire a still image and has a function of an image acquiring unit that acquires a moving image and/or a still image.
The light-guiding optical system 41 is installed between the measurement position P at which the microplate 20 is disposed and the imaging device 45. The light-guiding optical system 41 is an optical system that guides a two-dimensional optical image, which is obtained when the microplate 20 holding the samples S of the plurality of wells 21 is viewed from the bottom face 22, to the imaging device 45. The light-guiding optical system 41 can be specifically appropriately configured using optical elements that can implement necessary functions (for example, a focusing function and a optical image reducing function) depending on the configurations of the microplate 20 and the imaging device 45. An example of such an optical element is a taper fiber (see Japanese Unexamined Patent Publication No. 2001-188044). The light-guiding optical system 41 may have a configuration using a light irradiation device with a light guide member having concavities and convexities (see Japanese Unexamined Patent Publication No. 2010-230397 and Japanese Unexamined Patent Publication No. 2010-230396).
In
The excitation light source 43 is excitation light supply means for supplying fluorescence-measuring excitation light to the sample S. The excitation light source 43 can be specifically appropriately configured depending on the type of the sample S to be subjected to fluorescence measurement, the wavelength of excitation light to be applied to the sample 5, and the like. For example, the excitation light source can be configured using an illumination light source that supplies light and an optical filter unit that selects and switches the wavelength of excitation light. When supply of excitation light is not necessary depending on the type of optical measurement which is performed on the sample S, the excitation light source 43 may not be installed.
In this embodiment, the light-guiding optical system 41 includes an optical system that can guide a two-dimensional optical image from the microplate 20 and the sample S to the imaging device 45 and guide excitation light from the excitation light source 43 to the sample S. Such an optical system can be configured, for example, using a dichroic mirror that transmits fluorescence from the microplate 20 and reflects excitation light from the excitation light source 43 or the like. In
The microplate 20 which is used in the cell observation device 1 can employ various shapes of a well 21. Parts (a)-(d) in
The configuration of the electrical stimulation unit 16 will be described below in detail.
The electrical stimulation unit 16 has a structure in which a plurality of electrode pairs 17 extending vertically to the microplate 20 are fixed to a base 18 so as to be two-dimensionally arranged. Specifically, the electrode pairs 17 are arranged in a two-dimensional shape corresponding to the two-dimensional array of the plurality of wells 21 of the microplate 20 so as to extend to face the wells 21 of the microplate 20.
The first electrode 17a of the electrode pair 17 may have various shapes other than the columnar shape.
The first electrode 17a of the electrode pair 17 may be coated with an insulator except for the tip which is used to apply electrical stimulation to the sample S.
Here, the electrode pair 17 is not limited to the configuration in which each of the first electrode 17a and the second electrode 17b is formed of a single member, but one or both may be formed of plural members.
Referring to
The position controller (position control unit) 30, the imaging controller 32, and the electrical stimulation controller 34 are connected to the data acquiring device 10 having the above-mentioned configuration. The position controller 30 is electrically connected to the moving mechanism 19 and controls the moving mechanism 19 to dispose the electrode pairs 17 in the wells 21 of the microplate 20 when the optical measurement of the samples S is started. Specifically, the position controller 30 controls the position of each electrode pair 17 such that the electrode pair 17 is inserted into and removed from the well 21 in a state in which the first electrode 17a is disposed closer to the center of the well 21 than the second electrode 17b when the electrode pair 17 is disposed in the well 21, as illustrated in
The position controller 30, the imaging controller 32, and the electrical stimulation controller 34 are connected to the computer 50. The computer 50 includes a data analyzing unit 51 that acquires moving image data including a detected optical image acquired by the moving image acquiring unit 40 and performs an analysis process on the moving image data. The computer 50 includes a control unit 52 that controls operations of the units of the data acquiring device 10 via the position controller 30, the imaging controller 32, and the electrical stimulation controller 34 and controls fluorescence measurement of the sample S in the cell observation device 1 (details of which will be described later). In
The operation of the cell observation device 1 at the time of optical measurement of a sample S and the cell observation method according to this embodiment will be described below with reference to
First, when an instruction to start optical measurement of cells is input via the input device 62, the microplate 20 holding a sample S to be measured in the microplate stacker 13 is carried to the measurement position P in the dark box 15 by the microplate carrying mechanism 12 in a state in which the microplate is placed on the microplate holder 11 (step S01). Then, by causing the computer 50 to control the position of the electrical stimulation unit 16 using the moving mechanism 19, the tips of a plurality of electrode pairs 17 are inserted into the corresponding wells 21 of the microplate 20 (step S02). At this time, the computer 50 controls the positions of the electrode pairs 17 such that the tip of the second electrode 17b of each electrode pair 17 comes in contact with the outside of the center of the bottom face 22 of the microplate 20. Accordingly, the first electrode 17a is disposed in a state in which the tip thereof is separated by a predetermined distance from the center of the bottom face 22 of the well 21.
Thereafter, by causing the computer 50 to control the electrical stimulation controller 34, an electrical signal is supplied to the electrode pairs 17 and electrical stimulation is applied to the samples S in the wells 21 of the microplate 20 (step S03). The irradiation of electrical stimulation is repeatedly performed with a predetermined cycle (for example, 1 to 10 Hz). In the state in which the application of electrical stimulation is started, application of excitation light from the excitation light source 43 is started by causing the computer 50 to control the imaging controller 32 (step S04). Then, a two-dimensional optical image of the microplate 20 including fluorescence emitted from the sample S held in the well 21 is detected by the moving image acquiring unit 40, and moving image data representing the two-dimensional optical image is acquired by the computer 50. The frame rate of the moving image acquiring unit 40 is set to be higher than the frequency of the electrical signal. By causing the computer 50 to perform optical intensity analysis in the analysis area set as an area of the microplate 20 on the microplate holder 11 facing the electrode pair 17 on the two-dimensional optical image included in the acquired moving image data, analysis information (monitoring result) of the sample S is acquired and is output to the display device 61 (step S05).
For example, when the sample S includes myocardial cells exposed to a reagent, the analysis information is obtained by monitoring the fluorescence intensity from the myocardial cells dyed with a calcium ion sensitive pigment in time series. At this time, since a strength or cycle of a heartbeat can be aligned by applying electrical stimulation to the myocardial cells, it is possible to quantitatively evaluate the reagent. Accordingly, it is possible to evaluate a side effect of the reagent on the myocardial cells. When the cells in the sample S are dyed with a membrane potential sensitive fluorescent pigment and electrical stimulation is applied thereto, a variation in membrane potential with opening and closing of an ion channel of the cells is observed as a variation in fluorescence intensity. When the sample S include cells dyed with a membrane potential sensitive pigment or a sodium ion sensitive pigment, the membrane potential may be controlled by applying electrical stimulation to the sample S. As a technique of analyzing optical intensity in the analysis area, a technique of calculating the amplitude, the changing rate, the peak cycle, the number of peaks, the peak time, the rising time, the falling time, and the peak fluctuation width, and the like of the change of the pixel values in the analysis area as evaluation values can be considered.
According to the above-mentioned cell observation device 1 and the cell observation method using the cell observation device 1, by disposing the electrode pair 17 including the first electrode 17a and the second electrode 17b in the well 21 installed in the microplate 20, it is possible to apply electrical stimulation to a sample S including cells using the electrode pair 17. Here, since the tip of the first electrode 17a disposed close to the center of the well 21 extends more than the tip of the second electrode 17b disposed close to the circumference of the well 21, it is possible to cause the tip of the first electrode 17a to approach the sample S including cells held on the bottom of the well even when the well 21 has a concave bottom. Accordingly, it is possible to apply electrical stimulation to the sample S from the electrode pair 17 by only using a simple position control mechanism and to obtain an appropriate evaluation result for the sample S.
With the above-mentioned structure of the electrode pair 17, it is possible to easily fit the shape of the electrode pair 17 to the concave internal shape of the well 21 and to reduce the distance between the sample S held on the bottom of the well 21 and the first electrode 17a when the electrode pair 17 is disposed in the well 21 of the microplate 20. As a result, it is possible to efficiently apply electrical stimulation to the sample S. When the first electrode 17a as a pillar shape, it is possible to easily reduce the distance between the sample S held on the bottom of the well 21 and the first electrode 17a. As a result, it is possible to efficiently apply electrical stimulation to the sample S.
A second embodiment of the present invention will be described below.
The cell observation device 1A illustrated in the drawing is different from the cell observation device 1 according to the first embodiment, in that an electrical stimulation unit 16A includes a position adjusting mechanism 71. The other configuration of the cell observation device 1A is the same as in the first embodiment. The position adjusting mechanism 71 is fixed to the base 18 of the electrical stimulation unit 16A and supports the electrode pairs 17 so as to independently move the first electrode 17a and the second electrode 17b.
According to the position adjusting mechanism 71 having the above-mentioned configuration, it is possible to independently move the first electrodes 17a of the plurality of electrode pairs 17 and the second electrodes 17b of the plurality of electrode pairs 17 in the direction parallel to the axis of the second electrodes 17b (the length direction of the first electrodes 17a). As a result, it is possible to simultaneously adjust the relative positions of the tip of the first electrode 17a to the tip of the second electrode 17b in the plurality of electrode pairs 17. Particularly, according to the configuration in which the plurality of first electrodes 17a and the plurality of second electrodes 17b are attached to the first and second supports 72a and 72b, respectively, it is possible to simultaneously and easily adjust the positions of the tips of the plurality of electrode pairs 17.
Specifically, as illustrated in
The position adjusting mechanism 71 may fix the position of the second support 72b and adjust the distance of the first support 72a from the base 18, or may fix the position of the first support 72a and adjust the distance of the second support 72b from the base 18, or may adjust the distances of the first and second supports 72a and 72b from the base 18. In any case, it is possible to adjust the relative position of the tip of the first electrode 17a and the tip of the second electrode 17b. The position adjusting mechanism 71 may be constituted by an electrical driving unit using a piezoelectric actuator or a stepping motor, may be constituted by a manual mechanism that can manually adjust a position, or may have a structure employing a screw structure. When the position adjusting mechanism 71 is constituted by the electrical driving unit, the adjustment unit 73 is electrically connected to the position controller 30 and the positions of the first and second supports 72a and 72b can be electronically controlled using a control signal from the position controller 30.
When the position adjusting mechanism 71 is configured to be electrically controllable, the position of the electrode pair 17 may be controlled as follows. First, shape information of the wells 21 (for example, information indicating that the bottom has a flat shape or a U shape or depth information of a U-shaped bottom) of the microplate 20 which is used for observation or information on the tip position (width or height information) of the first electrode 17a relative to the tip position of the second electrode 17b is input by the input device 62. Then, the relative position of the tip of the first electrode 17a to the tip of the second electrode 17b is determined and the gap between the first support 72a and the second support 72b is automatically adjusted to achieve the relative position, by the position controller 30. In this way, the position adjusting mechanism 71 can adjust the relative position of the tip of the first electrode 17a to the tip of the second electrode 17b.
The operation of the cell observation device 1A at the time of optical measurement of a sample S and the cell observation method according to this embodiment will be described below in detail with reference to
First, when an instruction to start the optical measurement of cells and shape information of the wells 21 are input via the input device 62, the positional relationship between the tip of the first electrode 17a and the tip of the second electrode 17b in the plurality of electrode pairs 17 is automatically adjusted under the control of the position controller 30 (step S21). Thereafter, the microplate 20 holding a sample S to be measured in the microplate stacker 13 is carried to the measurement position P in the dark box 15 by the microplate carrying mechanism 12 in a state in which the microplate is placed on the microplate holder 11 (step S22). Then, by causing the computer 50 to control the position of the electrical stimulation unit 16 using the moving mechanism 19, the tips of the plurality of electrode pairs 17 are inserted into the corresponding wells 21 of the microplate 20 (step S23). At this time, the computer 50 controls the positions of the electrode pairs 17 such that the tip of the second electrode 17b of each electrode pair 17 comes in contact with the outside of the center of the bottom face 22 of the microplate 20. Accordingly, the first electrode 17a is disposed in a state in which the tip thereof is separated by a predetermined distance from the center of the bottom face 22 of the well 21.
Thereafter, by causing the computer 50 to control the electrical stimulation controller 34, an electrical signal is supplied to the electrode pairs 17 and electrical stimulation is applied to the samples S in the wells 21 of the microplate 20 (step S24). The application of electrical stimulation is repeatedly performed with a predetermined cycle (for example, 1 to 10 Hz). In the state in which the application of electrical stimulation is started, irradiation of excitation light from the excitation light source 43 is started by causing the computer 50 to control the imaging controller 32 (step S25). Then, a two-dimensional optical image of the microplate 20 including fluorescence emitted from the sample S held in the well 21 is detected by the moving image acquiring unit 40, and moving image data representing the two-dimensional optical image is acquired by the computer 50. The frame rate of the moving image acquiring unit 40 is set to be higher than the frequency of the electrical signal. By causing the computer 50 to perform optical intensity analysis in the analysis area set as an area of the microplate 20 on the microplate holder 11 facing the electrode pair 17 on the two-dimensional optical image included in the acquired moving image data, analysis information (monitoring result) of the sample S is acquired and is output to the display device 61 (step S26).
Here, the process of adjusting the position of the electrode pair 17 in step S21 may be performed when the electrode pair 17 is inserted into the well 21 in step S22. The process of step S21 may be performed after the process of inserting the electrode pair 17 into the well 21 in step S23 and before the process of starting application of electrical stimulation in step S24, or a cycle of evaluating a reaction of the sample S on the basis of a monitoring result of light from the sample in step S26, performing the process of adjusting the position of the electrode pair 17 in step S21, performing the process of applying electrical stimulation in step S24, performing the process of irradiating excitation light in step S25, and performing the process of monitoring light in step S26 may be carried out. This cycle may be repeated plural times. As a result, it is possible to adjust the intensity of electrical stimulation (a voltage value or a current value) to be applied depending on the reaction of the sample S.
According to the above-mentioned cell observation device 1A and the cell observation method using the cell observation device 1A, by disposing the electrode pair 17 including the first electrode 17a and the second electrode 17b in the well 21 installed in the microplate 20, it is possible to apply electrical stimulation to a sample S including cells using the electrode pair 17. Here, since the relative position of the tip of the first electrode 17a to the tip of the second electrode 17b can be adjusted, it is possible to cause the tip of the first electrode 17a to approach the sample S including cells held on the bottom of the well even when the well 21 has a concave bottom. Even when the well 21 has another shape such as a flat bottom, the tip of the first electrode 17a can be made to appropriately approach the sample S to correspond to the shape. Accordingly, it is possible to apply electrical stimulation to the sample S from the electrode pair 17 when the electrode pair 17 is disposed in the well 21, and to obtain an appropriate evaluation result for the sample S.
The present invention is not limited to the above-mentioned embodiments.
For example, the structure of the electrode pair 17 of the electrical stimulation unit 16 in the cell observation devices 1 and 1A is not limited to the tubular shape, but may employ various shapes.
Here, the electrode pairs 17A to 17E which are employed by the cell observation device 1 have a structure in which the tip of the first electrode 17a extends more than the tip of the second electrode 17b. In the electrode pairs 17 and 17A to 17E, when the first electrode 17a is formed of a plate-shaped electrode, it is preferable that the width of the tip of the first electrode 17a be set to be smaller than the width of the tip of the second electrode 17b.
Here, in the above-mentioned cell observation device or the above-mentioned electrical stimulation device, the second electrode may have a tubular shape and the first electrode may be disposed in the second electrode. According to this configuration, when the electrode pair is disposed in the holding unit of the sample case, it is possible to easily fit the shape of the electrode pair to the concave internal shape of the holding unit and to easily reduce the distance between the sample held on the bottom of the holding unit and the first electrode. As a result, it is possible to efficiently apply electrical stimulation to the sample.
The second electrode may include a plurality of electrode members and the first electrode may be disposed between the plurality of electrode members. According to this configuration, it is possible to easily decrease the size of the electrode pair and to appropriately apply electrical stimulation to the sample in the holding unit.
The first electrode may have a pillar shape. In this case, it is possible to easily reduce the distance between the sample held on the bottom of the holding unit and the first electrode. As a result, it is possible to efficiently apply electrical stimulation to the sample.
The width of the tip of the first electrode may be set to be smaller than the width of the tip of the second electrode. According to this configuration, it is possible to easily reduce the distance between the sample held on the concave bottom of the holding unit and the first electrode. As a result, it is possible to efficiently apply electrical stimulation to the sample.
The present invention is used for the cell observation device, the electrical stimulation device, and the cell observation method that can observe a reaction of a simple including cell to electrical stimulation and has enabled electrical stimulation to be appropriately applied to a cell disposed in the holding unit.
17, 17A-17G electrode pair; 1, 1A cell observation device; 10 data acquiring device; 11 microplate holder (mounting unit); 12 microplate carrying mechanism; 16, 16A electrical stimulation unit (electrical stimulation device); 17a first electrode; 17b second electrode; 19 moving mechanism; 20 microplate (sample case); 21 well (holding unit); 22 bottom face; 30 position controller (position control unit); 32 imaging controller; 34 electrical stimulation controller; 40 moving image acquiring unit; 50 computer; 51 data analyzing unit; 52 control unit; 71 position adjusting mechanism (position adjusting unit); 72a, 72b support; 73 adjustment unit; S sample
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Child | 16527423 | US |