Difference between revisions of "Part:BBa K1412014:Experience"
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=='''Protocol'''== | =='''Protocol'''== | ||
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| − | [[File: | + | [[File:.verification_2jpg.jpg |700px|thumb|center|<b>Figure 1</b> Verification of plasmid BBa_K1412000.]] |
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==='''Activiation'''=== | ==='''Activiation'''=== | ||
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| − | 1. Transfer 50 μL bacterium solution (pLac-RBS (1.0)- | + | 1. Transfer 50 μL bacterium solution (pLac-RBS (1.0)-cheZ-TT, pLac-RBS (0.01)-cheZ-TT, pLac-RBS (0.3)-cheZ-TT) into 5 ml new LB liquid medium whose chloromycetin concentration is 50ug/ml to culture for 12 hours in 37℃ horizontal rotators at 200 rpm. |
| − | medium whose chloromycetin concentration is 50ug/ml to culture | + | 2. Then transfer another 50μL bacterium solution from the LB above to another new 5ml LB liquid medium whose chloromycetin concentration is 50ug/ml to culture in 37℃ horizontal rotators at 200rpm for 3 hours. |
| − | + | ==='''Culture & Measurement'''=== | |
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| − | ==='''Culture'''=== | + | |
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| − | + | ===='''Culture'''==== | |
| − | 1. Firstly, draw three dots on a plate before using | + | 1. Firstly, draw three dots on a plate before using oily pen from the bottom of culture dish. |
2. Secondly, stab 3μl bacterium medium into the M63 semisolid medium at the dots. | 2. Secondly, stab 3μl bacterium medium into the M63 semisolid medium at the dots. | ||
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3. Finally, culture the bacteria in constant temperature and humidity incubator at 37℃ and observe the condition of bacterium growth. | 3. Finally, culture the bacteria in constant temperature and humidity incubator at 37℃ and observe the condition of bacterium growth. | ||
| + | [[File:Xmu_project_application_RBSpromoter02.png |810px|thumb|center|<b>Figure 2</b>. The schematic diagram of how we measure the diameter of colonies.]] | ||
| − | ==='''Measurement'''=== | + | ===='''Measurement'''==== |
| − | + | 1. Observe the the condition of bacterium growth,and prepare a ruler. | |
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2. When we can see a visible difference of the diameter of semi-solid medium with time pass by, begin to measure the diameter of bacterium | 2. When we can see a visible difference of the diameter of semi-solid medium with time pass by, begin to measure the diameter of bacterium | ||
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colonies from the bottom of the semi-solid medium to avoiding the collapse of semi-solid medium. | colonies from the bottom of the semi-solid medium to avoiding the collapse of semi-solid medium. | ||
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| + | 3. Recording data: The diameter of initial colonies(0h) is recorded as R1. And the diameter of the colonies at 12h, 24h, 30h, 36h, 42h... as | ||
| + | R2, R3, R4, R5, R6, R7…. | ||
==='''Results'''=== | ==='''Results'''=== | ||
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| − | [[File:Xmu_project_application_RBSpromoter03.png | | + | [[File:Xmu_project_application_RBSpromoter03.png |800px|thumb|center|<b>Figure 2A.</b>Culturing with 0.02 L-arabione for 48 hours, distinguish difference of chemotaxis diameters between each colonies is shown. <b>Figure 2B.</b> The relative activity of different promoters to pLac.]] |
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| − | between each colony diameters was fixed after 36 hours. If we set the fixed ratio as relative promoter activities, from our | + | Firstly, set the diameter of the colony with promoter Lac as '''1.0''', and plot the data in excel, We got the following table (Figure 3). As we can see, the ratio between each colony diameters was fixed after 36 hours. If we set the fixed ratio as relative promoter activities, from |
| + | our characterization, promoter TetR (BBa_R0040) activity is '''1.86''' relative to promoter Lac (BBa_R0010). | ||
| − | + | Refer to published papers [1] [2], promoter activity between pTetR and pLac has already been measured, and their ratio (pTetR/pLac) is '''1.58'''. So our system is reliable as it could tell the difference between different promoter activities. | |
| − | + | ===Applications of BBa_K1412614=== | |
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| − | ===Applications of | + | |
===User Reviews=== | ===User Reviews=== | ||
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Latest revision as of 00:21, 18 October 2014
Protocol
Verification
Activiation
1. Transfer 50 μL bacterium solution (pLac-RBS (1.0)-cheZ-TT, pLac-RBS (0.01)-cheZ-TT, pLac-RBS (0.3)-cheZ-TT) into 5 ml new LB liquid medium whose chloromycetin concentration is 50ug/ml to culture for 12 hours in 37℃ horizontal rotators at 200 rpm.
2. Then transfer another 50μL bacterium solution from the LB above to another new 5ml LB liquid medium whose chloromycetin concentration is 50ug/ml to culture in 37℃ horizontal rotators at 200rpm for 3 hours.
Culture & Measurement
Culture
1. Firstly, draw three dots on a plate before using oily pen from the bottom of culture dish.
2. Secondly, stab 3μl bacterium medium into the M63 semisolid medium at the dots.
3. Finally, culture the bacteria in constant temperature and humidity incubator at 37℃ and observe the condition of bacterium growth.
Measurement
1. Observe the the condition of bacterium growth,and prepare a ruler.
2. When we can see a visible difference of the diameter of semi-solid medium with time pass by, begin to measure the diameter of bacterium colonies from the bottom of the semi-solid medium to avoiding the collapse of semi-solid medium.
3. Recording data: The diameter of initial colonies(0h) is recorded as R1. And the diameter of the colonies at 12h, 24h, 30h, 36h, 42h... as R2, R3, R4, R5, R6, R7….
Results
Firstly, set the diameter of the colony with promoter Lac as 1.0, and plot the data in excel, We got the following table (Figure 3). As we can see, the ratio between each colony diameters was fixed after 36 hours. If we set the fixed ratio as relative promoter activities, from
our characterization, promoter TetR (BBa_R0040) activity is 1.86 relative to promoter Lac (BBa_R0010).
Refer to published papers [1] [2], promoter activity between pTetR and pLac has already been measured, and their ratio (pTetR/pLac) is 1.58. So our system is reliable as it could tell the difference between different promoter activities.
Applications of BBa_K1412614
User Reviews
UNIQ7f689ae1374e8386-partinfo-00000000-QINU UNIQ7f689ae1374e8386-partinfo-00000001-QINU