Part:BBa_K4229034
XiaI with SpyCatcher N-terminal and TnaB under the T7promotor and lacoperator
We had this BioBrick together with BBa_K4229033 on our Plasmid, which was transformed into BL21(DE3) E.Coli. We successfully produced Indigo and Indirubin with our transformed bacteria. The production of the compounds was shown visibly by the colour change of the culture[Fig.1]. After sample preparation, we could also measure the absorbance/fluorescence of both compounds at their respective absorption peaks (see [Fig.2] ) in all our production assays.
NMR and HPLC-followed mass spectrometry measurements of our samples additionally underlined that our synthesised products are Indigo and Indirubin.
The NMR proton-measurement of Indirubin from our bioproduction shows peaks at a shift of 7 – 7.6 ppm (see [Fig.3]), which roughly fits the expected spectrum of Indirubin from the literature [Ref.1]. However, the peaks are too weak to detect any further information. This might be due to too high contamination with other cell substances, as we did not have the equipment to purify them further. The most prominent peak at ~4 ppm is most likely from water, and the peak at ~2.5 ppm from DMSO. To prevent the massive water contamination, we freeze-dried the sample for Indigo before measuring. Another reason for the low signal of Indirubin could be that we had too little Indirubin in our sample.
After the HLPC separation of our Indirubin from our bioproduction, which fell out after ~16 min, the molecular mass could be detected via mass spectrometry ([Fig.4]). The result is as follows: ESI-MS, positive mode: m/z 263.1 (calculated mass for C16H10N2O2 [M + H]+ 263.2). It is likely to be Indirubin, with a literature value for its molecular weight of 262.26 [Ref.1].
Through this western blots [Fig.5 and 6] we could successfully prove, that our target enzymes of the Indigo pathway are caught to the T1 protein of the wiffleball. We can see that the band for the T1 protein runs significantly lower if our indigo producing enzymes are not expressed. If mentioned enzymes are present however, they form a complex with the T1 proteins, as a result the band runs higher.
[Ref.1] PubChem, https://pubchem.ncbi.nlm.nih.gov/compound/10177,Computed by PubChem
Sequence and Features
- 10COMPATIBLE WITH RFC[10]
- 12COMPATIBLE WITH RFC[12]
- 21COMPATIBLE WITH RFC[21]
- 23COMPATIBLE WITH RFC[23]
- 25INCOMPATIBLE WITH RFC[25]Illegal NgoMIV site found at 965
Illegal AgeI site found at 855 - 1000COMPATIBLE WITH RFC[1000]
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