Team:NTNU Trondheim/Protocols
From 2012.igem.org
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- | + | <h1>Protocols <small> A list of recipes and laboratory procedures used by the team</small></h1> | |
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__TOC__ | __TOC__ | ||
- | ==Transformation== | + | ==Laboratory procedures== |
+ | ---- | ||
+ | ===Transformation=== | ||
Official iGEM transformation protocol: http://partsregistry.org/Help:Protocols/Transformation | Official iGEM transformation protocol: http://partsregistry.org/Help:Protocols/Transformation | ||
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The cells used are [http://products.invitrogen.com/ivgn/product/18265017 Subcloning Efficiency™ DH5α™ Competent Cells] from Life Technologies/Invitrogen | The cells used are [http://products.invitrogen.com/ivgn/product/18265017 Subcloning Efficiency™ DH5α™ Competent Cells] from Life Technologies/Invitrogen | ||
- | ==Inoculation after transformation== | + | ===Inoculation after transformation=== |
Using a sterile toothpick, pick/scratch a single colony from the transformants. Drop the toothpick into a plastic tube with 3 mL sterile liquid medium with the appropriate antibiotic(s). Close the tube but leave the cap slightly open to allow oxygen to enter, and incuate at 37 C with shaking. | Using a sterile toothpick, pick/scratch a single colony from the transformants. Drop the toothpick into a plastic tube with 3 mL sterile liquid medium with the appropriate antibiotic(s). Close the tube but leave the cap slightly open to allow oxygen to enter, and incuate at 37 C with shaking. | ||
- | ==DNA Isolation== | + | ===DNA Isolation=== |
We use the Promega Wizard Plus SV Minipreps DNA Purification System A1460 with the sentrifugation version of the [http://www.promega.com/~/media/files/resources/protocols/technical%20bulletins/0/wizard%20plus%20sv%20minipreps%20dna%20purification%20system%20protocol.pdf?la=en protocol] supplied by the vendor. | We use the Promega Wizard Plus SV Minipreps DNA Purification System A1460 with the sentrifugation version of the [http://www.promega.com/~/media/files/resources/protocols/technical%20bulletins/0/wizard%20plus%20sv%20minipreps%20dna%20purification%20system%20protocol.pdf?la=en protocol] supplied by the vendor. | ||
- | ==DNA Concentration measurements== | + | ===DNA Concentration measurements=== |
Concentrations of DNA after isolation was measured with the [http://www.nanodrop.com/library/nd-1000-v3.7-users-manual-8.5x11.pdf NanoDrop ND-1000 Spectrophotometer]. | Concentrations of DNA after isolation was measured with the [http://www.nanodrop.com/library/nd-1000-v3.7-users-manual-8.5x11.pdf NanoDrop ND-1000 Spectrophotometer]. | ||
- | ==Restriction digest== | + | ===Restriction digest=== |
We are using the single reaction protocol from partsregistry.org : [http://partsregistry.org/Help:Protocols/Restriction_Digest] | We are using the single reaction protocol from partsregistry.org : [http://partsregistry.org/Help:Protocols/Restriction_Digest] | ||
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*Run a portion of the digest on a gel (8ul, 100ng), to check that both plasmid backbone and part length are accurate. | *Run a portion of the digest on a gel (8ul, 100ng), to check that both plasmid backbone and part length are accurate. | ||
- | ==Ligation== | + | ===Ligation=== |
Ligation protocol from partsregistry.org [http://partsregistry.org/Help:Protocols/Ligation]: | Ligation protocol from partsregistry.org [http://partsregistry.org/Help:Protocols/Ligation]: | ||
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Remember to do religation of backbone!!!!!!!! | Remember to do religation of backbone!!!!!!!! | ||
- | ==Linearized plasmids== | + | ===Linearized plasmids=== |
[http://partsregistry.org/Help:Protocols/Linearized_Plasmid_Backbones Official iGEM protocol] | [http://partsregistry.org/Help:Protocols/Linearized_Plasmid_Backbones Official iGEM protocol] | ||
- | ==Gel electrophoresis== | + | ===Gel electrophoresis=== |
Agarose with Gel Green is used when molding the gel. Choose an appropriate ladder as a referance to size of the fragments and put 2 µl of ladder in wells on either side of the samples. When applying the samples, add 20% loading dye to the sample. For instance, if the initial sample is 10 µl, add 2 µl loading dye. Apply the samples to individual wells in the gel. | Agarose with Gel Green is used when molding the gel. Choose an appropriate ladder as a referance to size of the fragments and put 2 µl of ladder in wells on either side of the samples. When applying the samples, add 20% loading dye to the sample. For instance, if the initial sample is 10 µl, add 2 µl loading dye. Apply the samples to individual wells in the gel. | ||
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Let the gel run for 45 min at 90 V, and if the bands are poorly separated, run a little longer. Beware that if the gel runs for a very long time, the smaller bands may move out of the gel. | Let the gel run for 45 min at 90 V, and if the bands are poorly separated, run a little longer. Beware that if the gel runs for a very long time, the smaller bands may move out of the gel. | ||
- | ==Gel purification== | + | ===Gel purification=== |
We are using the QIAquick Gel Extraction kit, following the protocol from www.qiagen.com. | We are using the QIAquick Gel Extraction kit, following the protocol from www.qiagen.com. | ||
[http://www.qiagen.com/literature/render.aspx?id=201083] | [http://www.qiagen.com/literature/render.aspx?id=201083] | ||
- | ==Preparation of samples for RNA isolation== | + | ===Preparation of samples for RNA isolation=== |
* Grow overnight cultures | * Grow overnight cultures | ||
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* Spin down at 6000 g for 10 minutes in 4 °C | * Spin down at 6000 g for 10 minutes in 4 °C | ||
- | ==RNA isolation== | + | ===RNA isolation=== |
(RNAquenous kit from Ambion) | (RNAquenous kit from Ambion) | ||
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* Measure concentrations on NanoDrop | * Measure concentrations on NanoDrop | ||
- | ==DNAse reaction== | + | ===DNAse reaction=== |
* Calculate the volume of RNA solution necessary to obtain a total of 3000 ng RNA | * Calculate the volume of RNA solution necessary to obtain a total of 3000 ng RNA | ||
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* Incubate for 10 minutes at 65 °C | * Incubate for 10 minutes at 65 °C | ||
- | ==cDNA reaction== | + | ===cDNA reaction=== |
* Prepare bulk mixture: | * Prepare bulk mixture: | ||
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* If qPCR is not to be performed immediately, the cDNA samples should be frozen down at -80 °C | * If qPCR is not to be performed immediately, the cDNA samples should be frozen down at -80 °C | ||
- | == | + | <!--===Master mix for real time PCR=== |
- | Coming soon... | + | Coming soon...--> |
- | ==OD measurements== | + | ===OD measurements=== |
Unless otherwise noted, all OD measurements are made at 600 nm with a PerkinElmer Lambda 35 spectrometer, with un-inoculated medium as reference. | Unless otherwise noted, all OD measurements are made at 600 nm with a PerkinElmer Lambda 35 spectrometer, with un-inoculated medium as reference. | ||
- | ==Fluorescence measurements== | + | ===Fluorescence measurements=== |
Fluorescence were measured with a Tecan Infinite M200 Pro microplate reader using Nunclon flat bottom black polystyrol 96 well plates. | Fluorescence were measured with a Tecan Infinite M200 Pro microplate reader using Nunclon flat bottom black polystyrol 96 well plates. | ||
==Recipes== | ==Recipes== | ||
- | + | ---- | |
===Growth media=== | ===Growth media=== | ||
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===Cake=== | ===Cake=== | ||
Batter is prepared following the protocol by Kakemonsen ([http://www.kakemonsen.no/sider/vis.asp?id=1186 1]). Sliced pieces of ''Malus domestica'' is inserted into the batter, while sucrose and ground ''Cinnamomum verum'' bark is mixed 2:1 by volume and distributed evenly on top of the batter, which is placed in a 26 cm diameter open-top vessel. The mixture is incubated in a dry air oven at ~180 C for 45 min. | Batter is prepared following the protocol by Kakemonsen ([http://www.kakemonsen.no/sider/vis.asp?id=1186 1]). Sliced pieces of ''Malus domestica'' is inserted into the batter, while sucrose and ground ''Cinnamomum verum'' bark is mixed 2:1 by volume and distributed evenly on top of the batter, which is placed in a 26 cm diameter open-top vessel. The mixture is incubated in a dry air oven at ~180 C for 45 min. | ||
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Latest revision as of 17:40, 25 September 2012