Team:NRP-UEA-Norwich/Week2
From 2012.igem.org
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As we are looking at producing a potential cancer therapeutic as part of our project we focused on looking at how that particular application could be used. Our main idea is to attach a nitric oxide-sensing promoter to an enzyme producing more nitric oxide (NO) in order to bring NO levels to a toxic threshold. We have found two key classes of NO-producing enzyme that may be applicable to our project: the first is nitric oxide synthase (NOS), most commonly from ''Nocardia'' species (known as NOSNoc) as it is a bacterial form of NOS, however so far we found little information on the intricacies of the enzyme and therefore feel it may not be the best enzyme to use; the other enzyme we have looked at is nitrite reductase (NiR), specifically copper-based NiR as it has a much cleaner reaction mechanism (producing just NO and H+) compared with other species of NiR. | As we are looking at producing a potential cancer therapeutic as part of our project we focused on looking at how that particular application could be used. Our main idea is to attach a nitric oxide-sensing promoter to an enzyme producing more nitric oxide (NO) in order to bring NO levels to a toxic threshold. We have found two key classes of NO-producing enzyme that may be applicable to our project: the first is nitric oxide synthase (NOS), most commonly from ''Nocardia'' species (known as NOSNoc) as it is a bacterial form of NOS, however so far we found little information on the intricacies of the enzyme and therefore feel it may not be the best enzyme to use; the other enzyme we have looked at is nitrite reductase (NiR), specifically copper-based NiR as it has a much cleaner reaction mechanism (producing just NO and H+) compared with other species of NiR. | ||
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===Labs=== | ===Labs=== | ||
Rebecca and Lukas went back into the labs today in order to try and transform the ''E. coli'' once again. Using the knowledge we had gained through research into why the previous transformations had been unsuccessful agar was used that had a reduced amount of chloramphenicol in order to try and grow more cells. | Rebecca and Lukas went back into the labs today in order to try and transform the ''E. coli'' once again. Using the knowledge we had gained through research into why the previous transformations had been unsuccessful agar was used that had a reduced amount of chloramphenicol in order to try and grow more cells. | ||
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We were also visited by Josh Wright from Bioline who very kindly donated a large amount of plasmid isolation kits and PCR gel clean-up kits, as well as giving us a discount on Bioline products. This kind of support from Bioline is extremely important to our project and we are very thankful! | We were also visited by Josh Wright from Bioline who very kindly donated a large amount of plasmid isolation kits and PCR gel clean-up kits, as well as giving us a discount on Bioline products. This kind of support from Bioline is extremely important to our project and we are very thankful! | ||
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Following Josh's visit Lukas, Russell and Khadija decided to try out the plasmid isolation kits for the first time as they tried to extract the chloramphenicol-resistance plasmid from some culutured ''E. coli''. The kits were extremely easy to use, however in keeping with our previous problems with growing ''E. coli'' we were unable to extract the plasmid, which was proven to us by a blank agarose gel picture. | Following Josh's visit Lukas, Russell and Khadija decided to try out the plasmid isolation kits for the first time as they tried to extract the chloramphenicol-resistance plasmid from some culutured ''E. coli''. The kits were extremely easy to use, however in keeping with our previous problems with growing ''E. coli'' we were unable to extract the plasmid, which was proven to us by a blank agarose gel picture. | ||
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The protocol for all lab work can be found [https://2012.igem.org/Team:NRP-UEA-Norwich/Protocol Here] | The protocol for all lab work can be found [https://2012.igem.org/Team:NRP-UEA-Norwich/Protocol Here] |
Revision as of 09:48, 25 July 2012