Template:KIT-Kyoto/Parts1
From 2010.igem.org
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(→We use these parts for making original biobrick parts) |
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- | == | + | == オリジナルのbiobrickパーツ作成の為に用いたパーツ == |
- | === 1. | + | === 1.2010 iGEM kitからのパーツ === |
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- | === 2. | + | === 2. iGEM HQから直接送ってもらったパーツ === |
We characterize this BioBrick Part and enter the new information back on the Registry. This parts don’t include detailed information on pSB6 and the reasons leading to its usage in our work to produce GFP. In general, pSB6 is a low copy plasmid which makes it more suitable for protein production than the high copy vector. However this information cannot be found in any sites related to iGEM. Consequently, we tried to compare the performances of the low copy vector pSB1 and pSB6. We have confirmed in this way that pSB6 is more efficient at producing GFP protein than PSB1. We have thus proved that this part is very useful to evaluate the capabilities of a promoter, in this case by observing the degree of fluorescence of GFP protein. We are very thankful to the 08’Tokyo-Tech group who has supplied us with this part. | We characterize this BioBrick Part and enter the new information back on the Registry. This parts don’t include detailed information on pSB6 and the reasons leading to its usage in our work to produce GFP. In general, pSB6 is a low copy plasmid which makes it more suitable for protein production than the high copy vector. However this information cannot be found in any sites related to iGEM. Consequently, we tried to compare the performances of the low copy vector pSB1 and pSB6. We have confirmed in this way that pSB6 is more efficient at producing GFP protein than PSB1. We have thus proved that this part is very useful to evaluate the capabilities of a promoter, in this case by observing the degree of fluorescence of GFP protein. We are very thankful to the 08’Tokyo-Tech group who has supplied us with this part. | ||
Revision as of 16:01, 20 October 2010
オリジナルのbiobrickパーツ作成の為に用いたパーツ
1.2010 iGEM kitからのパーツ
Name | Part type | Resistance | Insert | Vector | Contents |
---|---|---|---|---|---|
<partinfo>pSB3k3</partinfo>(<partinfo>BBa_J04450</partinfo>) | Plasmid backbone | Kanamycin | 738bp | 2750bp | promoter(LacI) +RBS+mRFP+T+T |
<partinfo>pSB6A1</partinfo>(<partinfo>BBa_J04450</partinfo>) | Plasmid backbone | Ampicillin | 738bp | 4032bp | promoter(LacI) +RBS+mRFP+T+T |
<partinfo>pSB1C3</partinfo>(<partinfo>BBa_J04450</partinfo>) | Plasmid backbone | Chloramphenicol | 1069bp | 2072bp | promoter(LacI) +RBS+mRFP+T+T |
<partinfo>pSB1A2</partinfo>(<partinfo>BBa_I3522</partinfo>) | Composite | Ampicillin | 937bp | 2079bp | promoter(TetR)+RBS+GFP+T+T |
<partinfo>pSB1A2</partinfo>(<partinfo>BBa_R0040</partinfo>) | Regulatory | Ampicillin | 54bp | 2079bp | promoter(TetR) |
<partinfo>pSB1A2</partinfo>(<partinfo>BBa_I732019</partinfo>) | Regulatory | Ampicillin | 3230bp | 2079bp | RBS+LacZ+T+T |
<partinfo>pSB1AK3</partinfo>(<partinfo>BBa_I732950</partinfo>) | Protein domain | Kanamycin | 3230bp | 2079bp | RBS+LacZ+T+T |
<partinfo>pSB4A5</partinfo>(<partinfo>BBa_K193602</partinfo>) | Composite | Ampicillin | 1896bp | 3395bp | |
<partinfo>pSB1A2</partinfo>(<partinfo>BBa_E0240</partinfo>) | Protein domain | Ampicillin | 883bp | 2079bp | RBS+GFP+T+T |
<partinfo>pSB1A2</partinfo>(<partinfo>BBa_I13507</partinfo>) | Protein domain | Ampicillin | 937bp | 2079bp | RBS+RFP+T+T |
<partinfo>pSB1A2</partinfo>(<partinfo>BBa_E0420</partinfo>) | Protein domain | Ampicillin | 878bp | 2079bp | RBS+CFP+T+T |
<partinfo>pSB1A2</partinfo>(<partinfo>BBa_E0430</partinfo>) | Protein domain | Ampicillin | 878bp | 2079bp | RBS+YFP+T+T |
<partinfo>pSB1A2</partinfo>(<partinfo>BBa_I13600</partinfo>) | Composite | Ampicillin | 940bp | 2079bp | promoter(TetR)+RBS+CFP+T+T |
<partinfo>pSB1A2</partinfo>(<partinfo>BBa_J22005</partinfo>) | Composite | Ampicillin | 2079bp | 2623bp | promoter(TetR)+RBS+YFP+T+T |
2. iGEM HQから直接送ってもらったパーツ
We characterize this BioBrick Part and enter the new information back on the Registry. This parts don’t include detailed information on pSB6 and the reasons leading to its usage in our work to produce GFP. In general, pSB6 is a low copy plasmid which makes it more suitable for protein production than the high copy vector. However this information cannot be found in any sites related to iGEM. Consequently, we tried to compare the performances of the low copy vector pSB1 and pSB6. We have confirmed in this way that pSB6 is more efficient at producing GFP protein than PSB1. We have thus proved that this part is very useful to evaluate the capabilities of a promoter, in this case by observing the degree of fluorescence of GFP protein. We are very thankful to the 08’Tokyo-Tech group who has supplied us with this part.
Name | Part Type | Resistance | Insert | Vector | |
---|---|---|---|---|---|
<partinfo>pSB6A1</partinfo>(<partinfo>BBa_K121013</partinfo>) | Protein domain | Ampicillin | 883bp | 4022bp | RBS+GFP+T+T |