Difference between revisions of "Part:BBa K1958004"
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[[File:Nanjing-China Hydrogenase Operon.png|800px|thumb|center|Figure 1. The Hya operon on the genome of E.coli.]] | [[File:Nanjing-China Hydrogenase Operon.png|800px|thumb|center|Figure 1. The Hya operon on the genome of E.coli.]] | ||
− | <h1>Characterisation of | + | <h1>Characterisation of HyaD</h1> |
− | <p>First the recombinant plasmid with genes encoding E.coli hydrogenase 1 was constructed. This enzyme is encoded by hya operon | + | <p>First the recombinant plasmid with genes encoding E.coli hydrogenase 1 was constructed. This enzyme is encoded by hya operon consisting of six genes named hyaABCDEF (BBa_K1958001, BBa_K1958002, BBa_K1958003, BBa_K1958004, BBa_K1958000, BBa_K1958006) on the genome of E.coli. The sequence was PCR amplified according to the sequence from our vessel E.coli strain BL21(DE3). We have completed the plasmid pET28a with hya cluster promoted by a T7 promoter. The following figure shows the result of enzyme digestion assay of recombinant plasmid in which our target gene cluster displayed a band around 5.5kb, which indicated successful hydrogenase expression.</p> |
[[File:Nanjing-China Subclone.png|800px|thumb|center|Figure 2. Enzyme digestion assay of recombinant plasmid, showing the band hyaA-F. (B) SDS-PAGE analysis of recombinant E.coli, showing the band of purified HyaA and overexpressed hydrogenase in recombinant strain.]] | [[File:Nanjing-China Subclone.png|800px|thumb|center|Figure 2. Enzyme digestion assay of recombinant plasmid, showing the band hyaA-F. (B) SDS-PAGE analysis of recombinant E.coli, showing the band of purified HyaA and overexpressed hydrogenase in recombinant strain.]] | ||
− | <p>To detect induced expression of Ec-Hyd1 we performed SDS-PAGE assay. Note that only the small subunit HyaA had a His-tag for purification on this plasmid. The purified subunit ran as the reference for hydrogenase. The assay showed that recombinant strain overexpressed hydrogenase compared to E.coli with empty pET28a plasmids.</p> | + | <p>To detect induced expression of Ec-Hyd1 we performed an SDS-PAGE assay. Note that only the small subunit HyaA had a His-tag for purification on this plasmid. The purified subunit ran as the reference for hydrogenase. The assay showed that recombinant strain overexpressed hydrogenase compared to E.coli with empty pET28a plasmids.</p> |
[[File:Nanjing-China Qualitative.png|800px|thumb|center|Figure 3. Qualitative test of hydrogenase under anaerobic conditions.]] | [[File:Nanjing-China Qualitative.png|800px|thumb|center|Figure 3. Qualitative test of hydrogenase under anaerobic conditions.]] | ||
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[[File:Nanjing-China Quantitative.png|800px|thumb|center|Figure 4. Gas chromatography quantitative test of hydrogenase under anaerobic conditions.]] | [[File:Nanjing-China Quantitative.png|800px|thumb|center|Figure 4. Gas chromatography quantitative test of hydrogenase under anaerobic conditions.]] | ||
− | <p>To measure the exact quantity of hydrogen produced in 20h of anaerobic culture, a gas chromatography (GC) test on samples taken from reaction flask headspace was done accordingly later. Nitrogen was the gas carrier and bulk H2 | + | <p>To measure the exact quantity of hydrogen produced in 20h of anaerobic culture, a gas chromatography (GC) test on samples taken from reaction flask headspace was done accordingly later. Nitrogen was the gas carrier and bulk H2 ran as the reference, which showed a peak at approximately 1.4 minute. According to our result, the control group produced 0.58% hydrogen in headspace under 1.96% oxygen proportion which marked the level of native fermentation of E.coli. The recombinant group obviously produced more hydrogen which made up 1.25% in the headspace under 2.06% oxygen level. This doubles the production of native fermentation, indicating that our enzyme is effective under anaerobic conditions.</p> |
== Usage and Biology == | == Usage and Biology == |
Revision as of 15:56, 22 October 2016
HyaD -> E. coli
HyaD is a subunit of hydrogenase 1 (Hyd-1) from Escherichia coli genome. The hya operon, which contains gene for the two HYD1 structual subunits and four additional genes (HyaA-F) was mapped at 22min on the E.coli chromosome. And hyaD is the fourth gene of hya operon, sharing the first few base pairs with hyaC and the last few base pairs with hyaE. HyaD is the specific protease required for large subunit maturation-terminal processing. HyaD is a hydrogenase maturase.
Contribution
- Group: Nanjing-China
- Author: Members of Nanjing-China
- Summary: We cloned and characterised HyaD, the fourth exon of Hya1 operon in E.coli and sent it to the registry as a biobrick. Our biobrick can be found here Part:BBa_K1958004.
Usage and Biology
This part HyaD encodes for the fourth exon of hydrogenase 1 operon in E.coli.
Characterisation of HyaD
First the recombinant plasmid with genes encoding E.coli hydrogenase 1 was constructed. This enzyme is encoded by hya operon consisting of six genes named hyaABCDEF (BBa_K1958001, BBa_K1958002, BBa_K1958003, BBa_K1958004, BBa_K1958000, BBa_K1958006) on the genome of E.coli. The sequence was PCR amplified according to the sequence from our vessel E.coli strain BL21(DE3). We have completed the plasmid pET28a with hya cluster promoted by a T7 promoter. The following figure shows the result of enzyme digestion assay of recombinant plasmid in which our target gene cluster displayed a band around 5.5kb, which indicated successful hydrogenase expression.
To detect induced expression of Ec-Hyd1 we performed an SDS-PAGE assay. Note that only the small subunit HyaA had a His-tag for purification on this plasmid. The purified subunit ran as the reference for hydrogenase. The assay showed that recombinant strain overexpressed hydrogenase compared to E.coli with empty pET28a plasmids.
We determined that our enzyme is effective using both qualitative and quantitative tests under anaerobic condition. Solutions for reaction were flushed with nitrogen and then reaction cells were vacuumed and sealed tight. The qualitative test was done after 20h of anaerobic culture (Figure 3A). We found that the recombinant strain overexpresses hydrogenase produces more bubbles than control group. We assumed that this was because more hydrogen evolves in experiment group. WO3 is a redox dye which determines the existence of reduction force in the environment with a color change to blue, compared to its original green. Again in 20h of anaerobic culture (Figure 3B), the WO3 powders displayed a darker color in the recombinant strain than that of native E.coli strain. We assumed that recombinant strain has created more reduction force than native E.coli strain.
To measure the exact quantity of hydrogen produced in 20h of anaerobic culture, a gas chromatography (GC) test on samples taken from reaction flask headspace was done accordingly later. Nitrogen was the gas carrier and bulk H2 ran as the reference, which showed a peak at approximately 1.4 minute. According to our result, the control group produced 0.58% hydrogen in headspace under 1.96% oxygen proportion which marked the level of native fermentation of E.coli. The recombinant group obviously produced more hydrogen which made up 1.25% in the headspace under 2.06% oxygen level. This doubles the production of native fermentation, indicating that our enzyme is effective under anaerobic conditions.
Usage and Biology
Sequence and Features
- 10COMPATIBLE WITH RFC[10]
- 12COMPATIBLE WITH RFC[12]
- 21COMPATIBLE WITH RFC[21]
- 23COMPATIBLE WITH RFC[23]
- 25COMPATIBLE WITH RFC[25]
- 1000COMPATIBLE WITH RFC[1000]