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| + | <tr><td> |
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| + | <table width="700px" align=center> |
| + | <tr><td width="340px"> |
| + | <span id="agar">'''アガロースゲル電気泳動'''</span></td><td width="20px"> </td><td width="340px"> |
| + | <span id="agareng">'''Agarose gel electrophoresis'''</span></td></tr> |
| + | <tr><td><table border=1 width="300px"><tr><td align=center rowspan=4 width="100px">50 x TAE</td><td width="200px">Tris base 242 g</td></tr><tr><td>無水酢酸 57.1 ml</td></tr> |
| + | <tr><td>0.5 M EDTA (pH 8.0) 100ml</td></tr><tr><td>ddH2Oを加えて1 Lにする</td></tr></table></td><td> </td><td><table border=1 width="300px"><tr><td align=center rowspan=4 width="100px">50 x TAE</td><td width="200px">242g Tris base</td></tr><td>57.1 ml of glacial Acetic acid</td></tr> |
| + | <tr><td>100ml of 0.5 M EDTA (pH 8.0)</td></tr><tr><td>Make up to 1 L with ddH2O</td></tr></table></td></tr> |
| + | <tr><td>1 x TAEを作るには、20 mlの50 x TAEに980 mlのH2Oを加える</td><td> </td><td>To make 1 x TAE from 50 x TAE stock, dilute 20 ml of stock into 980 ml of ddH2O.</td></tr> |
| + | <tr><td>↓ ゲルに使用するアガロースの量は扱うDNAによって変わるので下記の表に従えばよい</td><td> </td><td>↓ The amount of agarose to use in your gel depends on the DNA in question. Use the following table as a rough guide.</td></tr> |
| + | <tr><td><table border=1 width="300px"><tr><td width="150px" align=center>アガロース濃度 (g/100 ml)</td><td width="150px" align=center>最適なDNAの長さ(kb)</td></tr> |
| + | <tr><td align=center>0.5</td><td align=center>1 - 30</td></tr> |
| + | <tr><td align=center>0.7</td><td align=center>0.8 - 12</td></tr> |
| + | <tr><td align=center>1.0</td><td align=center>0.5 - 10</td></tr> |
| + | <tr><td align=center>1.2</td><td align=center>0.4 - 7</td></tr> |
| + | <tr><td align=center>1.5</td><td align=center>0.2 - 3</td></tr></table></td><td> </td><td><table border=1 width="300px"><tr><td width="150px" align=center>Agarose Concentration (g/100 ml)</td><td width="150px" align=center>Optimal DNA Length (kb)</td></tr> |
| + | <tr><td align=center>0.5</td><td align=center>1 - 30</td></tr> |
| + | <tr><td align=center>0.7</td><td align=center>0.8 - 12</td></tr> |
| + | <tr><td align=center>1.0</td><td align=center>0.5 - 10</td></tr> |
| + | <tr><td align=center>1.2</td><td align=center>0.4 - 7</td></tr> |
| + | <tr><td align=center>1.5</td><td align=center>0.2 - 3</td></tr></table></td></tr> |
| + | <tr><td>例えば、1%ゲルを作るには、1 gのアガロースをフラスコに量りとり、100 mlの1 x TAEを加え |
| + | る</td><td> </td><td>For example,to make a 1%agarose gel,weigh out 1 g of agarose into a flask and add 100 ml of 1 x TAE.</td></tr> |
| + | <tr><td>↓ 電子レンジでアガロースが完全に溶けるまで加熱する</td><td> </td><td>↓ Heat solution in a microwave until agarose is completely dissolved.</td></tr> |
| + | <tr><td>↓ 素手でフラスコの底が触れるまで冷ます</td><td> </td><td>↓ Let the agarose cool until touching the bottom of a flask with your bare hand.</td></tr> |
| + | <tr><td>↓ ゲルトレーにゲルを注ぎ、コームを挿す</td><td> </td><td>↓ Pour into gel tray and insert comb(s).</td></tr> |
| + | <tr><td>↓ 室温で15分から30分間冷ます</td><td> </td><td>↓ Allow to cool for 15-30 minutes at room temperature.</td></tr> |
| + | <tr><td>↓ コームを外し、電気泳動槽にうつして、1 x TAEに浸す</td><td> </td><td>↓ Remove comb(s),place in electrophoresis chamber and cover with 1 x TAE.</td></tr> |
| + | <tr><td>↓ サンプルに6 x ローディングダイを加える</td><td> </td><td>↓ Add 6 x loading dye to samples.</td></tr> |
| + | <tr><td>↓ DNAとマーカー(100 bp DNA ladder,1 kb DNA ladder)をゲルにのせる</td><td> </td><td>↓ Load DNA and standard (100 bp DNA ladder,1 kb DNA ladder) onto gel.</td></tr> |
| + | <tr><td>↓ 100 Vで20分間電気泳動する</td><td> </td><td>↓ Electrophorese at 100 V for 20 minutes.</td></tr> |
| + | <tr><td>↓ EtBrでゲルを30分間染色する</td><td> </td><td>↓ Dye gel with EtBr for 30 minutes.</td></tr> |
| + | <tr><td>↓ UVを照射してDNAのバンドを可視化する</td><td> </td><td>↓ Visualize DNA bands using UV lightbox.</td></tr> |
| + | </table> |
| + | </td></tr> |
| + | <tr><td> |
| + | |
| + | <div align="right"><span style="font- |
| + | |
| + | size:10pt;">[[#Contents|>>back to Contents]] |
| + | |
| + | </span></div> |
| + | |
| + | </td></tr> |
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About protocol
As it is of common knowledge, iGEM is carried out within the framework of a protocol common to all teams. Whereas most of the teams are registered on this page, we have uploaded not only the English protocol but also the Japanese one, e.g., our mother tongue version. This is the common protocol with some improvements after we translated it into Japanese.Publishing the Japanese protocol in will be of help to other new Japanese teams in the future. Furthermore, this will be linked to an improvement of iGEM’s name identification in Japan and will enhance the public recognition of synthetic biology. It will also promote Science and Communication among people within not only the scientific but with the non-scientific communities as well. We believe that these improvements will constitute a contribution to the illustration of the public in general.
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Contents
Protocol
トランスフォーメーション | |
Bacterial transformation |
↓ 氷上でコンピテント細胞(DH5 Alpha:大腸菌株)を解凍する | | ↓ Thaw competent cells(DH5 Alpha:E.coli strain) on ice. |
↓ 前もって冷やしておいた1.5 mlチューブに100 μlのコンピテント細胞を分注する余ったコンピテント細胞は-80 °Cの冷凍庫に戻す | | ↓ Aliquot 100 μl cells into pre-chilled 1.5 ml tube.Put excess competent cells back into the -80 °C freezer. |
↓ DNAをチューブに1~5 μl加えて、氷上で30分間冷やす | | ↓ Add DNA (1 to 5 μl) to tube, incubate on ice for 30 minutes. |
↓ 42 °Cで45秒間熱ショックを与える | | ↓ Heat shock the cells at 42 °C for 45 seconds. |
↓ 0.9 mlのSOC培地を加える | | ↓ Add 0.9 ml SOC medium. |
↓ 37 °Cで1時間、振りながら回復培養する | | ↓ Rescue at 37 °C for 1 hour, shaking. |
↓ 1 mlをLBプレート(+amp,+kan,+camのいずれか)にまく | | ↓ Spread 1 ml on LB plates(Either +amp,+kan or +cam) |
↓ 37 °Cで一晩培養する | | ↓ Cultivate overnight in 37 °C. |
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アルカリミニプレップ | |
DNA miniprep |
Solution I | 50 mM グルコース (MW 180) | | 10 mM EDTA(pH 8.0) | | 25 mM Tris-HCl (pH 8.0) |
Solution II | 0.2 N NaOH | | 1% SDS | Solution III | 3 M 酢酸カリウム | | 1.8 M 酢酸 |
| | Solution I | 50 mM glucose (MW 180) |
| 10 mM EDTA(pH 8.0) | | 25 mM Tris-HCl (pH 8.0) |
Solution II | 0.2 N NaOH | | 1% SDS | Solution III | 3 M potassium acetate | | 1.8 M acetic acid |
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↓ LBプレート(+amp,+kan,+camのいずれか)に大腸菌をまき、37 °Cで一晩培養する | | ↓ Streak E.coli to LB plates(Either +amp,+kan or +cam) and cultivate overnight in 37 °C. |
↓ プレートからシングルコロニーを分離する | | ↓ Pick up a single colony from plate. |
↓ 2 mlのLB培地で37 °Cで一晩振とう培養する | | ↓ Cultivate in 2 ml LB medium overnight in 37 °C, shaking. |
↓ 1.5 mlの培養液を1.5 mlチューブにうつす | | ↓ Pipet 1.5 ml of overnight culture into a 1.5 ml tube. |
↓ 15,000 rpm、4 °Cで1分間遠心し、 上清を捨てる | | ↓ Centrifuge for 1 minute at 15,000 rpm in 4 °C and discard the supernatant. |
↓ 100 μlの氷冷したSolution Iを沈殿に加え、懸濁する | | ↓ Add 100 μl of refrigerated Solution I to the pellet and vortex to resuspend. |
↓ 200 μlのSolution IIを加え、混ぜる、ボルテックスは使用しない | | ↓ Add 200 μl of Solution II and invert gently to mix. Do not vortex. |
↓ 氷上で5分間冷やす | | ↓ Incubate on ice for 5 minutes. |
↓ 150 μlの氷冷したSolution IIIを加え、穏やかに反転し混ぜる、ボルテックスは使用しない | | ↓ Add 150 μl of refrigerated Solution III and invert gently to mix. Do not vortex. |
↓ 氷上で5分間冷やす | | ↓ Incubate on ice for 5 minutes. |
↓ 15,000 rpm、4 °Cで5分間遠心する | | ↓ Centrifuge for 5 minutes at 15,000 rpm in 4 °C. |
↓ 400 μlのきれいな上清を注意してピペットで新しいチューブにとる | | ↓ Carefully pipet 400 μl of the clean supernatant into a new tube. |
↓ 900 μlの2-プロパノールを加え、混ぜる | | ↓ Add 900 μl of 2-propanol and mix. |
↓ 2分間室温で放置する | | ↓ Incubate for 2 minutes in room temperature. |
↓ 15,000 rpm、4 °Cで10分間遠心し、上清を捨てる | | ↓ Centrifuge for 10 minutes at 15,000 rpm in 4 °C and discard supernatant. |
↓ 1 mlの70%エタノールを加える | | ↓ Add 1 ml 70% EtOH to the pellet. |
↓ 15,000 rpm、4 °Cで2分間遠心し、上清を捨てる | | ↓ Centrifuge for 2 minutes at 15,000 rpm in 4 °C and discard supernatant. |
↓ 沈殿を10分~15分乾かす | | ↓ Dry the pellet for 10-15 minutes. |
↓ プラスミドDNAを30 μlのRNaseのはいったTEに溶かす | | ↓ Resuspend the plasmid DNA in 30 μl of TE with RNase. |
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ポリメラーゼ連鎖反応(PCR) | |
Polymerase Chain Reaction(PCR) |
↓ ソフトウェアプログラムを使って、プライマーの設計をする | | ↓ Design primers with software programs. | [http://ginkgobioworks.com/cgi/primer.cgi>>Ginkgo BioWorks] | | [http://ginkgobioworks.com/cgi/primer.cgi>>Ginkgo BioWorks] |
↓ 下記の組成に従って試薬を混ぜる | | ↓ Mix the reagent according to the following components. |
Primer Mix | 1.5 μl |
鋳型 DNA | 0.5 μl | 10 x PCR Buffer for KOD-Plus- | 5 μl | 2 mM dNTPs | 5 μl |
2 mM MgSO4 | 4 μl | ddH2O | 33 μl | KOD-Plus- | 1 μl |
| 全量 50 µl |
| | Primer Mix | 1.5 μl | Template DNA | 0.5 μl | 10 x PCR Buffer for KOD-Plus- | 5 μl | 2 mM dNTPs | 5 μl | 2 mM MgSO4 | 4 μl | ddH2O | 33 μl | KOD-Plus- | 1 μl | | 50 μl system |
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↓ PCRのプログラム設定 | | ↓ PCR program |
Start | 94 °C、2分 | Cycle x 35 | 94 °C、15秒 (熱変性) | (Tm-10) °C、0.5分 (アニーリング) | 68 °C、1 kb/min (伸長) | End | 68 °C、2分 |
4 °Cで保存 |
| | Start | 94 °C for 2 minutes. | Cycle x 35 | 94 °C for 15 seconds. (denaturing) | (Tm-10) °C for 0.5 minutes. (annealing) | 68 °C for 1 kb/min. (extension) | End | 68 °C for 2 minutes. | Keep at 4 °C forever. |
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制限酵素処理 | |
DNA digestion by restriction enzymes |
↓ 下記の組成に従って試薬を混ぜる | | ↓ Mix the reagent according to the following components. |
10 x Buffer | 2 μl (全量の10分の1) |
- [http://www.bio.toyobo.co.jp/bio01/cgi-bin/catalog_shohin_index?item=H-BUFF&us_id=&us_pwd=&bun_id=020010020&iv_trademark=BUF-1&kskh_kbn=01&ksk_jkn=BUF-1 H Buffer]
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- [http://www.bio.toyobo.co.jp/bio01/cgi-bin/catalog_shohin_index?item=M-BUFF&us_id=&us_pwd=&bun_id=020010020&iv_trademark=BUF-1 M Buffer]
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DNA溶液 | DNA量が1 μgになるように調整する |
制限酵素 | 3ユニットになるように調整する |
- [http://www.bio.toyobo.co.jp/bio01/cgi-bin/catalog_shohin_index?item=ECO-111&us_id=&us_pwd=&bun_id=0200100100410&iv_trademark=ECO-1&kskh_kbn=01&ksk_jkn=ECO-1 EcoR I]
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- [http://www.bio.toyobo.co.jp/bio01/cgi-bin/catalog_shohin_index?item=XBA-101W&us_id=&us_pwd=&bun_id=0200100100970&iv_trademark=XBA-1&kskh_kbn=01&ksk_jkn=XBA-1Xba I]
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- [http://www.bio.toyobo.co.jp/bio01/cgi-bin/catalog_shohin_index?item=PST-111&us_id=&us_pwd=?us_id=&bun_id=0200100100760&iv_trademark=PST-1&kskh_kbn=01&ksk_jkn=PST-1 Pst I]
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- [http://www.bio.toyobo.co.jp/bio01/cgi-bin/catalog_shohin_index?item=SPE-101&us_id=&us_pwd=?us_id=&bun_id=0200100100900&iv_trademark=SPE-1&kskh_kbn=01&ksk_jkn=SPE-1 Spe I]
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ddH2O | 全量が20 μl になるように調整する |
| 全量 20 μl | | |
10 x Buffer | 2 µl (1/10 of total) |
- [http://www.bio.toyobo.co.jp/bio01/cgi-bin/catalog_shohin_index?item=H-BUFF&us_id=&us_pwd=&bun_id=020010020&iv_trademark=BUF-1&kskh_kbn=01&ksk_jkn=BUF-1 H Buffer]
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- [http://www.bio.toyobo.co.jp/bio01/cgi-bin/catalog_shohin_index?item=M-BUFF&us_id=&us_pwd=&bun_id=020010020&iv_trademark=BUF-1 M Buffer]
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DNA solution | Adjust for the amount of DNA to become 1 μg. |
Restriction enzyme | Adjust to become 3 units. |
- [http://www.bio.toyobo.co.jp/bio01/cgi-bin/catalog_shohin_index?item=ECO-111&us_id=&us_pwd=&bun_id=0200100100410&iv_trademark=ECO-1&kskh_kbn=01&ksk_jkn=ECO-1 EcoR I]
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- [http://www.bio.toyobo.co.jp/bio01/cgi-bin/catalog_shohin_index?item=XBA-101W&us_id=&us_pwd=&bun_id=0200100100970&iv_trademark=XBA-1&kskh_kbn=01&ksk_jkn=XBA-1Xba I]
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- [http://www.bio.toyobo.co.jp/bio01/cgi-bin/catalog_shohin_index?item=PST-111&us_id=&us_pwd=?us_id=&bun_id=0200100100760&iv_trademark=PST-1&kskh_kbn=01&ksk_jkn=PST-1 Pst I]
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- [http://www.bio.toyobo.co.jp/bio01/cgi-bin/catalog_shohin_index?item=SPE-101&us_id=&us_pwd=?us_id=&bun_id=0200100100900&iv_trademark=SPE-1&kskh_kbn=01&ksk_jkn=SPE-1 Spe I]
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ddH2O | Adjust to become total 20 μl. |
| 20 μl system | |
↓ 37 °Cで1時間放置する | | ↓ Incubate for 1 hour in 37 °C. |
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アガロースゲル電気泳動 | |
Agarose gel electrophoresis |
50 x TAE | Tris base 242 g | 無水酢酸 57.1 ml |
0.5 M EDTA (pH 8.0) 100ml | ddH2Oを加えて1 Lにする |
| | 50 x TAE | 242g Tris base | 57.1 ml of glacial Acetic acid | </tr>
100ml of 0.5 M EDTA (pH 8.0) | Make up to 1 L with ddH2O |
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1 x TAEを作るには、20 mlの50 x TAEに980 mlのH2Oを加える | | To make 1 x TAE from 50 x TAE stock, dilute 20 ml of stock into 980 ml of ddH2O. |
↓ ゲルに使用するアガロースの量は扱うDNAによって変わるので下記の表に従えばよい | | ↓ The amount of agarose to use in your gel depends on the DNA in question. Use the following table as a rough guide. |
アガロース濃度 (g/100 ml) | 最適なDNAの長さ(kb) |
0.5 | 1 - 30 |
0.7 | 0.8 - 12 |
1.0 | 0.5 - 10 |
1.2 | 0.4 - 7 |
1.5 | 0.2 - 3 |
| | Agarose Concentration (g/100 ml) | Optimal DNA Length (kb) |
0.5 | 1 - 30 |
0.7 | 0.8 - 12 |
1.0 | 0.5 - 10 |
1.2 | 0.4 - 7 |
1.5 | 0.2 - 3 |
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例えば、1%ゲルを作るには、1 gのアガロースをフラスコに量りとり、100 mlの1 x TAEを加え
る | | For example,to make a 1%agarose gel,weigh out 1 g of agarose into a flask and add 100 ml of 1 x TAE. |
↓ 電子レンジでアガロースが完全に溶けるまで加熱する | | ↓ Heat solution in a microwave until agarose is completely dissolved. |
↓ 素手でフラスコの底が触れるまで冷ます | | ↓ Let the agarose cool until touching the bottom of a flask with your bare hand. |
↓ ゲルトレーにゲルを注ぎ、コームを挿す | | ↓ Pour into gel tray and insert comb(s). |
↓ 室温で15分から30分間冷ます | | ↓ Allow to cool for 15-30 minutes at room temperature. |
↓ コームを外し、電気泳動槽にうつして、1 x TAEに浸す | | ↓ Remove comb(s),place in electrophoresis chamber and cover with 1 x TAE. |
↓ サンプルに6 x ローディングダイを加える | | ↓ Add 6 x loading dye to samples. |
↓ DNAとマーカー(100 bp DNA ladder,1 kb DNA ladder)をゲルにのせる | | ↓ Load DNA and standard (100 bp DNA ladder,1 kb DNA ladder) onto gel. |
↓ 100 Vで20分間電気泳動する | | ↓ Electrophorese at 100 V for 20 minutes. |
↓ EtBrでゲルを30分間染色する | | ↓ Dye gel with EtBr for 30 minutes. |
↓ UVを照射してDNAのバンドを可視化する | | ↓ Visualize DNA bands using UV lightbox. |
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