Difference between revisions of "Part:BBa K1985005"
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The his-tagged proteins were purified by nickle affinity chromatography. An absorbance spectra was produced of all three proteins as well as the control. MamX has a significant increase in absorbance to the control both at 280nm displaying an increase in protein and at 407nm showing the heme group of mamX. | The his-tagged proteins were purified by nickle affinity chromatography. An absorbance spectra was produced of all three proteins as well as the control. MamX has a significant increase in absorbance to the control both at 280nm displaying an increase in protein and at 407nm showing the heme group of mamX. | ||
− | [[File: | + | [[File:Allprotein graph.jpeg||400px|thumb|centre|Figure 5. UV spectra of nickle affinity chromatography protein fractions from E.coli expressing mamX, P and T as well as the control. For mamX (Red) a significant peak was seen compared to the control (grey) at 407nm.]] |
Latest revision as of 17:31, 27 October 2016
mamX his-tagged, signal sequence cleaved
This part is an differentiation on Part:BBa_K1985002. The wild type sequence was altered to remove the membrane anchor so that the part is soluble and a SecS sequence was added to target the protein to the periplasm. A his-tag was added for easier protein purification.
Sequence and Features
- 10COMPATIBLE WITH RFC[10]
- 12COMPATIBLE WITH RFC[12]
- 21COMPATIBLE WITH RFC[21]
- 23COMPATIBLE WITH RFC[23]
- 25INCOMPATIBLE WITH RFC[25]Illegal AgeI site found at 216
- 1000INCOMPATIBLE WITH RFC[1000]Illegal SapI.rc site found at 783
Usage and Biology
This part has a his-tag included so was used to purify the expressed mamX protein. MamX is usually targeted to the membrane, however in this part the targeting sequence has been cleaved and it should instead be targeted to the periplasm. It was expressed, purified and then exposed to iron. For more information on its biology and usage, see part BBa_K1985002.
Validation
The part was first validated with a diagnostic restriction digest using EcoRI and PstI and agarose gel electrophoresis. The expected band sizes from the digest were: 2029 base pairs for the plasmid backbone and 838 for the insert. A 1kB plus DNA marker was used to verify the sizes of the bands and it was confirmed that the correct plasmid had been produced.
SDS-PAGE images revealed bands in all gels that were not present in the before induction samples and the control. For MamX the band indicated by the arrow equates to the, 24 kDa, soluble MamX protein with his-tag.
The his-tagged proteins were purified by nickle affinity chromatography. An absorbance spectra was produced of all three proteins as well as the control. MamX has a significant increase in absorbance to the control both at 280nm displaying an increase in protein and at 407nm showing the heme group of mamX.