JP2006197872A - Method of electroporation and cuvette for electroporation - Google Patents
Method of electroporation and cuvette for electroporation Download PDFInfo
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- JP2006197872A JP2006197872A JP2005014044A JP2005014044A JP2006197872A JP 2006197872 A JP2006197872 A JP 2006197872A JP 2005014044 A JP2005014044 A JP 2005014044A JP 2005014044 A JP2005014044 A JP 2005014044A JP 2006197872 A JP2006197872 A JP 2006197872A
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- C—CHEMISTRY; METALLURGY
- C12—BIOCHEMISTRY; BEER; SPIRITS; WINE; VINEGAR; MICROBIOLOGY; ENZYMOLOGY; MUTATION OR GENETIC ENGINEERING
- C12M—APPARATUS FOR ENZYMOLOGY OR MICROBIOLOGY; APPARATUS FOR CULTURING MICROORGANISMS FOR PRODUCING BIOMASS, FOR GROWING CELLS OR FOR OBTAINING FERMENTATION OR METABOLIC PRODUCTS, i.e. BIOREACTORS OR FERMENTERS
- C12M35/00—Means for application of stress for stimulating the growth of microorganisms or the generation of fermentation or metabolic products; Means for electroporation or cell fusion
- C12M35/02—Electrical or electromagnetic means, e.g. for electroporation or for cell fusion
Abstract
Description
本発明は、生体細胞を足場に接着状態のまま電気穿孔を行う細胞電気穿孔装置に関する。 The present invention relates to a cell electroporation apparatus that performs electroporation while living cells are adhered to a scaffold.
従来、細胞の遺伝子操作において細胞内部に外的物質を導入する際には細胞膜に一時的に透過性を持たせる事が必要であり、リポフェクション法や電気穿孔法などが用いられてきた。このうち、リポフェクション法はリポフェクションに用いる薬剤に毒性があり、細胞種によっては使用できないという欠点がある。 Conventionally, when introducing an external substance into a cell during genetic manipulation of the cell, it is necessary to make the cell membrane temporarily permeable, and a lipofection method or an electroporation method has been used. Among these, the lipofection method is toxic to the drug used for lipofection and has a drawback that it cannot be used depending on the cell type.
電気穿孔法は例えば非特許文献1記載の方法であり、細胞を足場から剥がし、浮遊状態で細胞に比較的強力な電場を与える事によって細胞に微小開口を形成し、外的物質を導入する方法であるが、細胞を浮遊状態にする必要があるため、十分に分化した細胞や組織を形成している細胞には適用できない場合があるという欠点がある。また、未分化細胞に電気穿孔を行った場合も再び足場に接着させ、分化を誘導しなければならないが、電気穿孔法で導入した遺伝子の効果は48時間程度で消えてしまい、細胞が十分に分化した状態で導入遺伝子の効果を見る事は難しかった。 The electroporation method is, for example, a method described in Non-Patent Document 1, wherein a cell is peeled off from a scaffold, a microscopic opening is formed in the cell by applying a relatively strong electric field to the cell in a floating state, and an external substance is introduced. However, since the cells need to be in a floating state, there is a drawback that they may not be applicable to cells that are sufficiently differentiated cells or cells forming tissues. In addition, even when electroporation is performed on undifferentiated cells, it must adhere to the scaffold again to induce differentiation, but the effect of the gene introduced by electroporation disappears in about 48 hours, and the cells are sufficiently It was difficult to see the effect of the transgene in a differentiated state.
電気穿孔法における上記の問題を解決するため、特許文献1にあるような生体に直接接触させる形の電極や特許文献2にあるような針状の電極が公開されている。しかし、これらの方法は組織への遺伝子導入を目的として考案されており、外的物質導入後に細胞を生きたまま観察する事はできないという問題があった。 In order to solve the above problems in the electroporation method, an electrode in the form of direct contact with a living body as in Patent Document 1 and a needle-shaped electrode as in Patent Document 2 are disclosed. However, these methods have been devised for the purpose of gene introduction into tissues, and there is a problem that cells cannot be observed alive after introduction of an external substance.
また、第3の遺伝子導入方法としてマイクロインジェクション方法がある。これは中空のガラスマイクロニードルを細胞に挿入し、外来物質を直接導入する方法だが、細胞一つ一つに手作業で導入することになるため、高い技術を持った人間が行っても導入できる細胞の数はごくわずかという欠点があった。 There is a microinjection method as a third gene introduction method. This is a method in which a hollow glass microneedle is inserted into a cell and a foreign substance is directly introduced. However, since it is introduced manually into each cell, it can be introduced even by a highly skilled person. The number of cells was very small.
上記のように、従来の技術では培養細胞を足場に接着状態のまま遺伝子などの外的物質を導入し、細胞が生きたまま観察する事が難しいという問題があった。 As described above, the conventional technique has a problem that it is difficult to observe a cell while it is alive by introducing an external substance such as a gene while the cultured cell is adhered to the scaffold.
本発明は、細胞を足場に接着状態のまま電気穿孔を行い、かつ、生きたままの状態で観察する事ができる装置の提供を目的としている。 An object of the present invention is to provide an apparatus capable of performing electroporation while adhering a cell to a scaffold and observing the cell while alive.
本発明によれば、透明電極上に生体細胞を培養し、透明電極と対向電極の間に電気パルスを与えることにより透明電極上の生体細胞に遺伝子などの外的物質を導入する事ができる。 According to the present invention, an external substance such as a gene can be introduced into a living cell on the transparent electrode by culturing the living cell on the transparent electrode and applying an electric pulse between the transparent electrode and the counter electrode.
また、本発明は、底部に光学的に透明な電極を設置してなる所定の容積を有する容器と前記容器の上方から被せて前記容器を密封し、かつ前記透明電極に対向して配設した対向電極を備え、前記容器と上下方向に対向して設置される蓋体とを備えたことを特徴とする電気穿孔用キュベットを提供する。 Further, the present invention provides a container having a predetermined volume formed by placing an optically transparent electrode on the bottom, and the container is sealed from above the container, and disposed opposite to the transparent electrode. There is provided an electroporation cuvette comprising a counter electrode, and comprising a lid body disposed opposite to the container in the vertical direction.
以上説明したように本発明によれば、透明電極上に培養した生体細胞を足場に接着した状態のまま電気穿孔により遺伝子などの外的物質を導入する事が可能となる。また、細胞接着面は透明板であるため、生体細胞の形態を光学的に観察することが可能である。細胞生物学の分野では導入した外的物質が分化した細胞内でどのように振る舞い、どのような場所に局在しているのかを調べることがその主たる手法であり、細胞が生きた状態のまま光学的な観察が可能という点は大きな利点である。以上のような特徴から、この電気穿孔装置は細胞を分化誘導した後など足場から剥がす事によって細胞が死んでしまうような状況での外的物質の導入に有用である。また、本発明によって得られる装置を用いた外的物質の導入手法は特別な技術を必要とせず、誰にでも簡便に再現性が高い実験が行えるという利点もある。 As described above, according to the present invention, an external substance such as a gene can be introduced by electroporation while the living cells cultured on the transparent electrode are adhered to the scaffold. Further, since the cell adhesion surface is a transparent plate, it is possible to optically observe the morphology of the living cells. In the field of cell biology, the main method is to investigate how the introduced external substance behaves in the differentiated cells and where it is localized, and the cells remain alive. The fact that optical observation is possible is a great advantage. Due to the above characteristics, this electroporation apparatus is useful for introducing an external substance in a situation where the cells die by being peeled off from the scaffold such as after differentiation induction of the cells. In addition, the method of introducing an external substance using the apparatus obtained by the present invention does not require any special technique and has an advantage that anyone can easily perform experiments with high reproducibility.
以下、本発明の実施の形態を、図面を参照しながら説明する。 Hereinafter, embodiments of the present invention will be described with reference to the drawings.
図1は本発明の実施の形態による電気穿孔装置の概略構成を示す図である。図1を参照すると、容器(1)の下部に透明電極(2)が電気伝導面が上向きになるように設置されており、この透明電極上に生体細胞(4)を培養する。 FIG. 1 is a diagram showing a schematic configuration of an electroporation apparatus according to an embodiment of the present invention. Referring to FIG. 1, a transparent electrode (2) is installed at the lower part of the container (1) so that the electrically conductive surface faces upward, and living cells (4) are cultured on the transparent electrode.
透明電極外周部は、容器の下部に設置された金属電極板(3)と上面を接するよう配置される。このような形態により、容器内部の培養液が金属電極と接する事なく、電気パルス発生装置と接続された下部電極(6)から通電可能となる。 A transparent electrode outer peripheral part is arrange | positioned so that a metal electrode plate (3) installed in the lower part of a container may contact | connect an upper surface. With such a configuration, the culture solution inside the container can be energized from the lower electrode (6) connected to the electric pulse generator without contacting the metal electrode.
対向電極(5)は蓋体(7)に設置され、生体細胞に電気穿孔を与える時に用いられ、通常培養時には電極がない蓋体で培養する事ができる。電気穿孔時には透明電極(2)と対向電極(5)の間を生体細胞に導入しようとする外的物質を含む溶液を満たし、電気パルスを与えることによって透明電極上の生体細胞に一時的に透過性を与え、外的物質を生体細胞に導入する。 The counter electrode (5) is placed on the lid (7) and is used when electroporation is given to living cells, and can be cultured in a lid without electrodes during normal culture. During electroporation, the space between the transparent electrode (2) and the counter electrode (5) is filled with a solution containing an external substance to be introduced into the living cell, and is temporarily transmitted to the living cell on the transparent electrode by applying an electric pulse. Gives sex and introduces external substances into living cells.
本実施例では低栄養培地で筋肉様組織へと分化誘導されるC2C12筋芽細胞を用いた。この細胞はリポフェクションでは遺伝子を導入することが難しく、また、分化誘導後に基板から剥がすと死んでしまうため、電気穿孔法を用いることもできないため本発明による方法が最適な遺伝子導入法である。C2C12筋芽細胞をZnOでコートしたガラス基板上にてダルベッコ改変イーゲル培地+10% 牛胎児血清において培養した(図3)。3日間上記条件で培養後、ダルベッコ改変イーゲル培地+2%ウシ血清に置換し、1週間培養することによって分化したC2C12筋管細胞を得た(図4)。細胞どうしが融合し、チューブ上の構造を示していることから分化していることがわかる。 In this example, C2C12 myoblasts induced to differentiate into muscle-like tissues in a low nutrient medium were used. This cell is difficult to introduce a gene by lipofection, and if it is peeled off from the substrate after differentiation induction, the method according to the present invention is the optimum gene introduction method because the electroporation method cannot be used. C2C12 myoblasts were cultured in Dulbecco's modified Egel medium + 10% fetal bovine serum on a glass substrate coated with ZnO (Fig. 3). After culturing under the above conditions for 3 days, the C2C12 myotube cells differentiated were obtained by substituting Dulbecco's modified Egel medium + 2% bovine serum and culturing for 1 week (FIG. 4). It can be seen that the cells are differentiated from each other because the cells are fused and show the structure on the tube.
ZnOでコートしたガラス基板上にて培養した分化誘導後のC2C12細胞に本発明による装置によってCFP遺伝子を導入した。電気パルス発生装置としてBio-Rad社のGenePulsar Xcellを用い、電圧150V、静電容量1000mFの指数減衰パルスを電極間隔3mmでDNA濃度100mg/mlのPBS中で与えた。その後、ダルベッコ改変イーゲル培地+2%ウシ血清にて24時間培養し、蛍光顕微鏡によってCFPの蛍光を観察した(図5)。蛍光を発している細胞(図5で白く見える細胞)が観察された事から、本発明による装置によって細胞が足場に接着した状態のままCFP遺伝子が導入され、その遺伝子が細胞中で発現していることがわかる。 The CFP gene was introduced into the differentiated C2C12 cells cultured on a glass substrate coated with ZnO by the apparatus according to the present invention. GenePulsar Xcell of Bio-Rad was used as an electrical pulse generator, and an exponential decay pulse with a voltage of 150 V and a capacitance of 1000 mF was applied in PBS with a DNA concentration of 100 mg / ml at an electrode interval of 3 mm. Thereafter, the cells were cultured in Dulbecco's modified Egel medium + 2% bovine serum for 24 hours, and the fluorescence of CFP was observed with a fluorescence microscope (FIG. 5). Since fluorescent cells (cells that look white in FIG. 5) were observed, the device according to the present invention introduced the CFP gene with the cells adhered to the scaffold, and the gene was expressed in the cells. I understand that.
本発明に係わる電気穿孔装置は、分子生物学、細胞生物学、遺伝子工学、再生医療など様々な分野に適用できる。 The electroporation apparatus according to the present invention can be applied to various fields such as molecular biology, cell biology, genetic engineering, and regenerative medicine.
1 容器
2 透明電極
3 金属電極板
4 生体細胞
5 対向電極
6 下部電極
7 蓋体
DESCRIPTION OF SYMBOLS 1 Container 2 Transparent electrode 3 Metal electrode plate 4 Living cell 5 Counter electrode 6 Lower electrode 7 Lid
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Cited By (4)
| Publication number | Priority date | Publication date | Assignee | Title |
|---|---|---|---|---|
| JP2012120452A (en) * | 2010-12-06 | 2012-06-28 | Dainippon Printing Co Ltd | Container for cell test, and cell test method using the same |
| JP2016506751A (en) * | 2013-02-20 | 2016-03-07 | チン,ジェン | Electroporation method and electroporation apparatus |
| JP2021514705A (en) * | 2018-02-26 | 2021-06-17 | ゼネラル・エレクトリック・カンパニイ | Systems and methods for electrical pulse-based activation of biological samples |
| US11225638B2 (en) * | 2016-04-04 | 2022-01-18 | CyteQuest, Inc. | System, device and method for electroporation of cells |
Citations (1)
| Publication number | Priority date | Publication date | Assignee | Title |
|---|---|---|---|---|
| WO2005035755A1 (en) * | 2003-10-08 | 2005-04-21 | Kyoto University | Method of introducing nucleic acid |
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| Publication number | Priority date | Publication date | Assignee | Title |
|---|---|---|---|---|
| WO2005035755A1 (en) * | 2003-10-08 | 2005-04-21 | Kyoto University | Method of introducing nucleic acid |
Cited By (5)
| Publication number | Priority date | Publication date | Assignee | Title |
|---|---|---|---|---|
| JP2012120452A (en) * | 2010-12-06 | 2012-06-28 | Dainippon Printing Co Ltd | Container for cell test, and cell test method using the same |
| JP2016506751A (en) * | 2013-02-20 | 2016-03-07 | チン,ジェン | Electroporation method and electroporation apparatus |
| US11225638B2 (en) * | 2016-04-04 | 2022-01-18 | CyteQuest, Inc. | System, device and method for electroporation of cells |
| JP2021514705A (en) * | 2018-02-26 | 2021-06-17 | ゼネラル・エレクトリック・カンパニイ | Systems and methods for electrical pulse-based activation of biological samples |
| JP7382945B2 (en) | 2018-02-26 | 2023-11-17 | ゼネラル・エレクトリック・カンパニイ | Systems and methods for electrical pulse-based activation of biological samples |
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