Team:Cornell/project/wetlab/fungal toolkit/characterization
From 2013.igem.org
(Difference between revisions)
Line 21: | Line 21: | ||
In our studies, GFP and monomeric red fluorescent protein (mRFP) were utilized as markers for gene expression. In developing our <a href = "https://2013.igem.org/Team:Cornell/project/wetlab/fungal_toolkit" > fungal toolkit </a>, we placed GFP and mRFP downstream of numerous promoters including the T7 promoter and fungal promoters PtrpC and <i>A. nidulans</i> PgpdA. The level of fluorescent activity would be indicative of promoter strength. <br /><br /> | In our studies, GFP and monomeric red fluorescent protein (mRFP) were utilized as markers for gene expression. In developing our <a href = "https://2013.igem.org/Team:Cornell/project/wetlab/fungal_toolkit" > fungal toolkit </a>, we placed GFP and mRFP downstream of numerous promoters including the T7 promoter and fungal promoters PtrpC and <i>A. nidulans</i> PgpdA. The level of fluorescent activity would be indicative of promoter strength. <br /><br /> | ||
- | Experimentation was done on the BL21 bacterial strain, which is the most common bacterial gene expression host and ideal for protein expression. BL21 utilizes the T7 promoter expression system, which is more effective at expressing proteins than any other system because it lacks two proteases, Ion and ompT, that degrade proteins before and after cell lysis [1]. DH5Alpha <i>E. coli</i> was used as a control. In addition, a ribosome binding site (RBS) was added to genetic constructs of the promoter and the fluorescent protein in order to control translation initiation and rate of translation. RBS was designed to optimize the genetic circuit and expression of the protein [4]. Hygromycin-resistance gene (hph) and kanamycin resistance gene (nptII) were added to form genetic constructs of promoter, fluorescent protein, and resistance gene. | + | Experimentation was done on the BL21 bacterial strain, which is the most common bacterial gene expression host and ideal for protein expression. BL21 utilizes the T7 promoter expression system, which is more effective at expressing proteins than any other system because it lacks two proteases, Ion and ompT, that degrade proteins before and after cell lysis [1]. DH5Alpha <i>E. coli</i> was used as a control. In addition, a ribosome binding site (RBS) was added to genetic constructs of the promoter and the fluorescent protein in order to control translation initiation and rate of translation. RBS was designed to optimize the genetic circuit and expression of the protein [4]. Hygromycin-resistance gene (hph) and kanamycin resistance gene (nptII) were added to form genetic constructs of promoter, fluorescent protein, and resistance gene. |
<br> | <br> |
Revision as of 03:12, 28 September 2013
Characterization
Flourescence
The green fluorescent protein (GFP) from the jellyfish Aequorea victoria has long been used as a molecular marker and reporter for eukaryotes and prokaryotes. Purified GFP absorbs blue light at a peak of 395 nm and emits green light at 509 nm, producing a stable fluorescence with little to no photobleaching [2]. GFP proved to be a valuable alternative to previous markers used in fungal research such as beta-glucuronidase, which was plagued with problems due to substrate uptake and leakiness [3]. Leaky gene expression is a result of initiation of transcription without the proper activator proteins. GFP was ideal because it does not require an exogenous substrate and does not negatively affect fungal tissue [3].In our studies, GFP and monomeric red fluorescent protein (mRFP) were utilized as markers for gene expression. In developing our fungal toolkit , we placed GFP and mRFP downstream of numerous promoters including the T7 promoter and fungal promoters PtrpC and A. nidulans PgpdA. The level of fluorescent activity would be indicative of promoter strength.
Experimentation was done on the BL21 bacterial strain, which is the most common bacterial gene expression host and ideal for protein expression. BL21 utilizes the T7 promoter expression system, which is more effective at expressing proteins than any other system because it lacks two proteases, Ion and ompT, that degrade proteins before and after cell lysis [1]. DH5Alpha E. coli was used as a control. In addition, a ribosome binding site (RBS) was added to genetic constructs of the promoter and the fluorescent protein in order to control translation initiation and rate of translation. RBS was designed to optimize the genetic circuit and expression of the protein [4]. Hygromycin-resistance gene (hph) and kanamycin resistance gene (nptII) were added to form genetic constructs of promoter, fluorescent protein, and resistance gene.