Difference between revisions of "Part:BBa K3503001"
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<h2>Sequencing and sequence alignment of K3503001</h2> | <h2>Sequencing and sequence alignment of K3503001</h2> | ||
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<div class="legend">Figure 1. Representative sequencing results of K3503001 | <div class="legend">Figure 1. Representative sequencing results of K3503001 | ||
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<h2>Fire retardant test of K3503001</h2> | <h2>Fire retardant test of K3503001</h2> | ||
<p>The test subject was in the size of bed sheet in 300*130mm and the average Moisture content% is 13.55%-14.37%. As demonstrated on Fig 3, all of our engineered flame retardant displayed a significant improvement compared with the water control.</p> | <p>The test subject was in the size of bed sheet in 300*130mm and the average Moisture content% is 13.55%-14.37%. As demonstrated on Fig 3, all of our engineered flame retardant displayed a significant improvement compared with the water control.</p> | ||
Revision as of 19:35, 26 October 2020
Alpha-s1-casein-His
The milk protein α-s1-casein from Bos taurus with his tag
Sequence and Features
- 10COMPATIBLE WITH RFC[10]
- 12COMPATIBLE WITH RFC[12]
- 21INCOMPATIBLE WITH RFC[21]Illegal BamHI site found at 643
- 23COMPATIBLE WITH RFC[23]
- 25COMPATIBLE WITH RFC[25]
- 1000COMPATIBLE WITH RFC[1000]
Sequencing and sequence alignment of K3503001
To future confirm that our constructs have the correct sequence, we send our clones (with positive PCR results) out to sequencing.
The sequencing results show that we have successfully assembled target genes K3503001 to the vector (pET-11a).
Successful expression of K3503001
In order to validate the protein expression of K3503001, K3503007 and K3503008, we performed SDS-PAGE (coomassie blue staining) and Western blot analysis. To make K3503001, K3503007 and K3503008 easily detectable via Western Blot, we designed our constructs to include a “His tag” which is targeted by a commercially available antibody. With the SDS-PAGE and western blot (anti-his for his-tagged protein), we found successful expression of K3503001, K3503007 and K3503008.
Before performing the SDS-PAGE, we grew up our engineered E. coli cells containing a plasmid with K3503001, K3503007 and K3503008 under control of the T7 promoter. Cells were induced with0.1mM IPTG until either OD0.4 (wavelength: 600nm) at 30°C. After expression, cells were then lysed according to our protein extraction protocol, and supernatant and pellet were collected for the SDS-PAGE.
(a)
- Lane1: Bio rad protein dual color ladder;
- Lane2: pet11a
- Lane3: K3503001
- Lane4:K3503001 with 0.1mM IPTG induction
- Lane5: K3503007
- Lane6: K3503007 with 0.1mM IPTG induction
- Lane7: K3503008
- Lane8:K3503008 with 0.1mM IPTG induction
Fire retardant test of K3503001
The test subject was in the size of bed sheet in 300*130mm and the average Moisture content% is 13.55%-14.37%. As demonstrated on Fig 3, all of our engineered flame retardant displayed a significant improvement compared with the water control.
As demonstrated in Fig 4, all of our engineered K3503001, K3503007 and K3507008 flame retardants displayed a significant improvement compared with the water control.