Team:Washington/Alkanes/Future/DecarbDesign
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<big>'''DECARBONYLASE REDESIGN'''</big> | <big>'''DECARBONYLASE REDESIGN'''</big> |
Revision as of 04:07, 13 September 2011
Contents |
Background
The objective of this subproject was to modify the ADC protein so that we can synthesize a wider variety of alkanes; in other words, mutate the protein so that it works better on a range of saturated fatty aldehydes. The protein was originally surmised to work best on C18 aldehydes, as the crystal structure derived Pymol model of the protein revealed a C18 carboxylic acid bounded to the metal center (though the vector with AAR and ADC proved to work best on C16 aldehydes while less on C14 and C18 aldehydes). Consequently, we decided to strive to modify ADC to work on shorter chain aldehydes, specifically tetradecanal. The substrate on the original Pymol file was modified to model C14 aldehyde, and then the file was converted to a Fold-it puzzle for human interaction. We decided to avoid changing amino acids near the active site, which binds to the aldehyde group, as we wanted to maintain the basic chemistry, decarbonylation (or perhaps deformylation). There was also the issue of the Fold-it modeling 122-Tyrosine hydrogen bonded to the substrate and another side chain, and according to Fold-it's notifications, serine, threonine, and tyrosine cannot "have more than 1 donor and 2 acceptors." As the amino acid we will change will be around the alkyl chain, there are no hydrogen bonds to be made(hydrogen bonds show up on the interface). If we are to make changes so that the protein binds more favorably to C14 aldehydes, we must improve dispersion intermolecular interactions by increasing the surface interaction between protein and substrate. Comparison with the original Pymol file showed that the removal of the four carbon atoms created a spatial “void area.” Targeting the void area with minimal interference or clashes between atoms, the most promising mutation sites are on adjacent sections of two helices positioned opposite of the substrate’s carbon end. The adjacent sections take up amino acids 21 to 25 and 67 to 71, the former of which, being closer, shows promise as a site to mutate to fill in the void area and avoid interferences.
Methods
After creating several aldehyde decarbonylase (ADC) mutants using Fold-It, a computational design program, three different types of reactions were developed and these reactions were later analyzed using using GC-MS to see if our mutants can produce C13 alkanes. These three types of reactins that were set up are cell lysis assay, protein purification assay, and in vivo assay.
In Vitro Assays
Cell Lysis Assay
First, ADC cells were grown overnights in TB and an antibiotic, Kanamycin.
Protein Purification Assay
Use higher concentrations of protein: 1. grow up 10X more protein and purifying
In Vivo Assay
In vivo (in the cell, start from glucose) : cells’ membrane will keep proteins in smaller volume, but the main point is that we can compare with native ADC cell results from other groups (the cells probably will make more alcohol anyway
Current Status
- Discuss mutations made and construct submitted
- Show protein gel of expression
- Discuss in vitro assay and how it hasn't worked yet (even for WT)
- Discuss plan for future testing
Parts Submitted
- Plasmids with mutations
- ADC_AB4
- 1C2
- 7A5
- 8BE
- 9A1
- 10B5