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<li> After weeks of waiting we finally received a delivery of cytochrome c so there was a mad scramble to do an assay to demonstrate the activity of Fer.</li> | <li> After weeks of waiting we finally received a delivery of cytochrome c so there was a mad scramble to do an assay to demonstrate the activity of Fer.</li> | ||
<li> Hanging up the lab coat marked a brief moment of reflection then someone reminded us about the looming wiki deadline and everyone dived head first into their computers. </li> | <li> Hanging up the lab coat marked a brief moment of reflection then someone reminded us about the looming wiki deadline and everyone dived head first into their computers. </li> | ||
+ | <center><img src="https://static.igem.org/mediawiki/2017/e/ee/T--Macquarie_Australia--improvefig3.png" width="500px" height="447px"> </center> | ||
+ | <center> <p align="justify" style="width:500px;word-wrap:break-word"> | ||
+ | <b><i>Figure 4.</i></b> Spectrophotometer at 550 nm of purified ferredoxin reductase (FNR) fraction. The peaks (blue) correspond to the reduction of cytochrome C by the oxidisation of NADPH to NADP<sup>+</sup> by FNR. This validates the characterisation of the <i>fer</i> biobrick. | ||
+ | </p> | ||
<li> The End. </li> | <li> The End. </li> | ||
</ul> | </ul> |
Revision as of 09:18, 31 October 2017
Glossary
- FNR - Ferredoxin NADP+ reductase.
- Fer- Ferredoxin and Ferredoxin NADP+ reductase (FNR).
- Hyd- hyd 1 coding for the enzymatic part of the Hydrogenase molecular machine.
- Fer/Hyd- Fer and Hyd as described above in a new biobrick construct.
- HydEF- coding two of the three maturation enzymes.
- HydEFG- hyd EF and hyd G, coding all three maturation enzymes in a new biobrick construct.
- Fer/Hyd/EFG, Omega Ω or HGPCC - plasmid with all the necessary genes coding the total Hydrogenase molecular machine. Ferredoxin, Ferredoxin NADP+ reductase, Hyd 1, Hyd EF and Hyd G all in a new biobrick construct. This plasmid gained the official bio-brick name – Hydrogen Gas Producing Gene Cluster (HGPGC).
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Figure 1. Agarose gel (1%) electrophoresis. Lanes 1 and 10 contain a Neb 1kb marker. Lanes 2, and 6 were negative controls. Lane 4 shows no bands and indicates failed PCR of AMP in KOD. Lanes 7-9 show no bands and indicate unsuccessful PCR of respective antibiotics in Quick cells. Lanes 3 and 5 show successful band of CAM and AMP respectively at ~1600 bp. Lanes 11-14 show bands of ~3000 bp psbMZHWK (PS2) plasmid as expected cut with Eco-RI (E), XbaI (X), SpeI (S) and PstI (P). Lanes 15-18 show successful cut of PS2 plasmid at ~1000 bp and ~2000 bp, indicating all restriction enzymes are functional in cutsmart buffer. |
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Figure 7. Agarose gel (1%) electrophoresis of single and double digests using Eco-RI (E) and PstI (P) in fer/hyd1 gene in transformed colony samples A, B, C and D. Lane 1 contains a 1kb ladder. Samples A (lanes 3-4), B (lanes 4-5) and C (lanes 6-7) are from the same transformed plate. Samples A and B show expected band weights for the single digests (~5400bp) and double digests (~3400 bp and 2000 bp) respectively, and were submitted for sequencing confirmation. Band weights in sample C do not correspond with expected band weights and were unsuccessful. Sample D was spun down prior to loading and no band weights were detected. This gel validates the fer/hyd1 Biobrick to the designed constructs in samples A and B. |
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Figure 5. SDS-PAGE gel of induced and purified fer fractions. |
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Figure 4. Spectrophotometer at 550 nm of purified ferredoxin reductase (FNR) fraction. The peaks (blue) correspond to the reduction of cytochrome C by the oxidisation of NADPH to NADP+ by FNR. This validates the characterisation of the fer biobrick. |
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