Difference between revisions of "Part:BBa K4152008"

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~~__NOTOC__~~

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~~<partinfo>BBa_K4152008 short</partinfo>~~

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~~To improve the performance of Proteinase K, we designed many Proteinase K mutant genes. PK_MT8 is a complicated mutation of Proteinase K, which contains 2 mutation sites: P175F-S197W.~~

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~~<!-- Add more about the biology of this part here~~

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~~===Usage and Biology===~~

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~~~~

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~~Sequence and Features~~

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~~<partinfo>BBa_K4152008 SequenceAndFeatures</partinfo>~~

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~~<!-- Uncomment this to enable Functional Parameter display~~

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~~===Functional Parameters===~~

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~~<partinfo>BBa_K4152008 parameters</partinfo>~~

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~~~~

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~~===Origin(organism)===~~

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~~Tritirachium album limber~~

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~~===Structure Design===~~

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*1. Use PyMOL to mutate some residues of Proteinase K, analyse the possibility of the formation of new interaction forces like hydrogen bond, salt bond, disulfide bond and π-π interaction.

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*2. Use AlphaFold v2.1.0 to predict the structure of the mutated PK.

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~~~~

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~~[[File:mt8-alphafold.png|400px]] ~~

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~~'''Figure 1.''' The mutated PK structure compared to the Wild type PK. ~~

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~~~~

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*3. Use FoldX to calculate the Gibbs Free Energy compared to wild type PK with Ca2+. (PDB ID: 1ic6) The result of this mutated PK's ΔΔG is '''-13.81''' kcal/mol.

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~~===Molecular cloning===~~

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~~We used the wild type Proteinase K(Hereinafter referred to as PK) DNA gene to overlap our mutated PK gene.~~

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~~~~

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~~[[File:mt8-total of pcr'.png|600px]] ~~

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~~'''Figure 2.''' The process of PCR for our mutated PK gene. ~~

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*1. Use mutated PK primers to clone our small fragments.

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~~~~

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~~[[File:mt8-pcr1'.png|400px]] ~~

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~~'''Figure 3.''' Fragments of mutated PK gene are PCR-amplified independently. ~~

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*2. Fuse the segments together in a subsequent reaction by High-fidelity thermostable DNA polymerase.

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~~[[File:Mt8-pcr3'.png|500px]] ~~

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~~'''Figure 4.''' PCR Mutagenesis by Overlap Extension to obtain the mutated PK gene. ~~

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~~~~

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*4. Use Ligase to link our mutated PK and pPIC9 after double digestion.

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*5. Transform the constructed plasmid into competent DH5α cells to expand the plasmid largely

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*6. Extract the recombinant pPIC9-PK and verify it by double digestion (XhoⅠ and EcoRⅠ), and sequence it for verication of mutation sites.

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~~~~

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~~[[File:Mt8-dd3'.png|400px]] ~~

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~~'''Figure 5.''' Double digestion verification of Recombinant pPIC9-PK. ~~

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~~~~

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~~After verification, it was determined that the construction is successful. We transformed the constructed plasmid into competent DH5α cells to expand the plasmid largely ~~

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~~===Expression in Pichia Pastoris===~~

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~~'''Linearization of Recombinant pPIC9-PK:''' ~~

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~~We used restriction endonuclease SalⅠ to linearize our recombinant plasmid.~~

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~~~~

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~~[[File:Mt8-linearization.png|500px]] ~~

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~~'''Figure 6.''' Linearization of Recombinant pPIC9-PK. ~~

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~~~~

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~~'''Electrotransformation:''' ~~

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~~Add several μg linearized pPIC9-PK to GS115 competence cells, then use 1.5kV electric pulse to drill holes to let gene get in. ~~

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~~'''Screen positive colonies and culture preservation:''' ~~

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* 1. Use MD solid medium to screen positive GS115 cells which can grow without Histidine. (Because GS115 cannot grow at medium without Histidine except our gene was introduced in).

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* 2. Extract the genomic DNA of recombinant GS115 and verify the sequence of Recombinant pPIC9-PK (from AOX1 promoter to AOX1 Terminator, about 1500bp).

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~~~~

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~~===Conclusion===~~

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In conclusion,the thermostability of the Mutated PK has improved '''在这里填东西''' times with Ca2+, improved '''在这里填东西''' times without Ca2+ compared with wild type of PK.

@@ Line 1: / Line 1: @@
-__NOTOC__
-<partinfo>BBa_K4152008 short</partinfo>
-To improve the performance of Proteinase K, we designed many Proteinase K mutant genes. PK_MT8 is a complicated mutation of Proteinase K, which contains 2 mutation sites: P175F-S197W.
-<!-- Add more about the biology of this part here
-===Usage and Biology===
-<!-- -->
-<span class='h3bb'>Sequence and Features</span>
-<partinfo>BBa_K4152008 SequenceAndFeatures</partinfo>
-<!-- Uncomment this to enable Functional Parameter display
-===Functional Parameters===
-<partinfo>BBa_K4152008 parameters</partinfo>
-<!-- -->
-===Origin(organism)===
-Tritirachium album limber
-===Structure Design===
-*1. Use PyMOL to mutate some residues of Proteinase K, analyse the possibility of the formation of new interaction forces like hydrogen bond, salt bond, disulfide bond and π-π interaction.
-*2. Use AlphaFold v2.1.0 to predict the structure of the mutated PK.
-<p style="text-align: center;">
-[[File:mt8-alphafold.png|400px]]<br>
-'''Figure 1.'''   The mutated PK structure compared to the Wild type PK.<br>
-</p>
-*3. Use FoldX to calculate the Gibbs Free Energy compared to wild type PK with Ca<sup>2+</sup>. (PDB ID: 1ic6) The result of this mutated PK's ΔΔG is '''-13.81''' kcal/mol.
-===Molecular cloning===
-We used the wild type Proteinase K(Hereinafter referred to as PK) DNA gene to overlap our mutated PK gene.
-<p style="text-align: center;">
-[[File:mt8-total of pcr'.png|600px]]<br>
-'''Figure 2.'''   The process of PCR for our mutated PK gene.<br>
-</p>
-*1. Use mutated PK primers to clone our small fragments.
-<p style="text-align: center;">
-[[File:mt8-pcr1'.png|400px]]<br>
-'''Figure 3.'''   Fragments of mutated PK gene are PCR-amplified independently.<br>
-</p>
-*2. Fuse the segments together in a subsequent reaction by High-fidelity thermostable DNA polymerase.
-<p style="text-align: center;">
-[[File:Mt8-pcr3'.png|500px]]<br>
-'''Figure 4.'''   PCR Mutagenesis by Overlap Extension to obtain the mutated PK gene.<br>
-</p>
-*4. Use Ligase to link our mutated PK and pPIC9 after double digestion. <br>
-*5. Transform the constructed plasmid into competent DH5α cells to expand the plasmid largely <br>
-*6. Extract the recombinant pPIC9-PK and verify it by double digestion (XhoⅠ and EcoRⅠ), and sequence it for verication of mutation sites.
-<p style="text-align: center;">
-[[File:Mt8-dd3'.png|400px]]<br>
-'''Figure 5.'''   Double digestion verification of Recombinant pPIC9-PK.<br>
-</p>
-After verification, it was determined that the construction is successful. We transformed the constructed plasmid into competent DH5α cells to expand the plasmid largely<br>
-===Expression in <i>Pichia Pastoris</i>===
-'''Linearization of Recombinant pPIC9-PK:'''<br>
-We used restriction endonuclease SalⅠ to linearize our recombinant plasmid.
-<p style="text-align: center;">
-[[File:Mt8-linearization.png|500px]]<br>
-'''Figure 6.'''   Linearization of Recombinant pPIC9-PK.<br>
-</p>
-'''Electrotransformation:'''<br>
-Add several μg linearized pPIC9-PK to GS115 competence cells, then use 1.5kV electric pulse to drill holes to let gene get in.<br>
-'''Screen positive colonies and culture preservation:'''<br>
-* 1. Use MD solid medium to screen positive GS115 cells which can grow without Histidine. (Because GS115 cannot grow at medium without Histidine except our gene was introduced in).<br>
-* 2. Extract the genomic DNA of recombinant GS115 and verify the sequence of Recombinant pPIC9-PK (from AOX1 promoter to AOX1 Terminator, about 1500bp).
-</p>
-===Conclusion===
-In conclusion,the thermostability of the Mutated PK has improved '''在这里填东西''' times with Ca<sup>2+</sup>, improved '''在这里填东西''' times without Ca<sup>2+</sup> compared with wild type of PK.