User:Jennifer Taylor/Sandbox 4

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[[Image:4Q7Q_D193A_mutation.png|thumb|left|250px|Figure 13: D193A mutation, transformed in DH5α.]][[Image:4Q7Q_H196A_mutation.png|thumb|right|250px|Figure 14. H196A mutation, transformed in DH5α.]][[Image:4Q7Q_S164A_mutation.png|thumb|left|250px|Figure 15. S164A mutation, transformed in DH5α.]][[Image:4Q7Q_D193A_H196A_mutations.png|thumb|right|250px|Figure 16. D193A and H196A mutations, transformed in DH5α.]]
[[Image:4Q7Q_D193A_mutation.png|thumb|left|250px|Figure 13: D193A mutation, transformed in DH5α.]][[Image:4Q7Q_H196A_mutation.png|thumb|right|250px|Figure 14. H196A mutation, transformed in DH5α.]][[Image:4Q7Q_S164A_mutation.png|thumb|left|250px|Figure 15. S164A mutation, transformed in DH5α.]][[Image:4Q7Q_D193A_H196A_mutations.png|thumb|right|250px|Figure 16. D193A and H196A mutations, transformed in DH5α.]]
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==Future Directions==
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Due to time constraints, we were unable to perform another pNPB assay using the mutated catalytic triad to confirm that our putative catalytic triad was accurate.
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Future directions include testing substrate specificity through using different types of lipids. Furthermore, we can attempt to optimize our enzymatic activity through varying pH, temperature, and other conditions. More assays using different concentrations of lipids are necessary to calculate We can also attempt to optimize our protein expression altogether, through varying concentrations of IPTG, since our concentration of protein was low.
</StructureSection>
</StructureSection>
== References ==
== References ==
<references/>
<references/>

Revision as of 14:53, 23 May 2018

4Q7Q

Structure of 4Q7Q

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References

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Jennifer Taylor

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