Difference between revisions of "Team:UMaryland/HokSok"
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<p align = "center"><img src = "https://static.igem.org/mediawiki/2015/4/4a/UMDHappyCell.jpeg"></p> | <p align = "center"><img src = "https://static.igem.org/mediawiki/2015/4/4a/UMDHappyCell.jpeg"></p> | ||
<p style = "font-size:18px" align = "center"><b>4. Can this cell living with Hok-Sok stay happy?</b></p> | <p style = "font-size:18px" align = "center"><b>4. Can this cell living with Hok-Sok stay happy?</b></p> | ||
− | <p style="font-size:24px">The ability to use plasmids as vectors to introduce genes of interest in E. coli is one of the most essential bioengineering tools. However, one of the limitations of transforming a bacterium with a plasmid, is that the organism will eventually eject the plasmid over time. To counter this, scientists add a positive selective pressure on E. coli to retain plasmids carrying resistance genes through the use of antibiotics. While this technique has proven to be reliable and effective, there are many limitations. The prevalent use of antibiotics both for medical and agricultural purposes has rapidly increased the number of pathogens that harbor antibiotic resistant genes. As a result, there is a pressing need to find an alternative to antibiotic use for plasmid maintenance to prevent the spread of antibiotic resistant genes. Many synthetic biology projects which focus of solving health or environmental issues are confined to the lab because of these limitations. The University of Maryland iGEM team seeks to solve this problem by developing an alternative plasmid maintenance system that should liberate other iGEM teams from the dependance on antibiotic usage. We hypothesized that Hok-Sok could maintain recombinant plasmids, as it does natural ones. We also hypothesized that Hok-Sok would have a slight negative effect on bacterial growth rate, in line with other alternative maintenance systems such as sRNBC (<a href = "http://parts.igem.org/Part:BBa_K817015">K817015</a>), as well as the amount of protein expression due to competing parallel promoters. In order to answer these questions, we set up a variety of testing procedures, as shown below.</p> | + | <p style="font-size:24px">The ability to use plasmids as vectors to introduce genes of interest in E. coli is one of the most essential bioengineering tools. However, one of the limitations of transforming a bacterium with a plasmid, is that the organism will eventually eject the plasmid over time. To counter this, scientists add a positive selective pressure on E. coli to retain plasmids carrying resistance genes through the use of antibiotics. While this technique has proven to be reliable and effective, there are many limitations. The prevalent use of antibiotics both for medical and agricultural purposes has rapidly increased the number of pathogens that harbor antibiotic resistant genes. As a result, there is a pressing need to find an alternative to antibiotic use for plasmid maintenance to prevent the spread of antibiotic resistant genes. Many synthetic biology projects which focus of solving health or environmental issues are confined to the lab because of these limitations. The University of Maryland iGEM team seeks to solve this problem by developing an alternative plasmid maintenance system that should liberate other iGEM teams from the dependance on antibiotic usage. We hypothesized that Hok-Sok, our plasmid maintenance system, could maintain recombinant plasmids, as it does natural ones. We also hypothesized that Hok-Sok would have a slight negative effect on bacterial growth rate, in line with other alternative maintenance systems such as sRNBC (<a href = "http://parts.igem.org/Part:BBa_K817015">K817015</a>), as well as the amount of protein expression due to competing parallel promoters. In order to answer these questions, we set up a variety of testing procedures, as shown below.</p> |
<p style="font-size:24px;text-align:center;font-family:Verdana, Geneva, sans-serif;">Section Summary</p> | <p style="font-size:24px;text-align:center;font-family:Verdana, Geneva, sans-serif;">Section Summary</p> | ||
<ul> | <ul> |
Revision as of 02:16, 19 September 2015