Team:SJTU-BioX-Shanghai/Project/project2.2
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__NOTOC__ | __NOTOC__ | ||
- | =Membrane Accelerator - Fatty Acid and Alkane Biosynthesis= | + | =Membrane Accelerator<br><br> - Fatty Acid and Alkane Biosynthesis= |
{{Template:12SJTU_part_summary_head}} | {{Template:12SJTU_part_summary_head}} | ||
*'''State of the art''' | *'''State of the art''' | ||
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*'''Achievements''' | *'''Achievements''' | ||
- | + | ''4 enzyme-bearing fusion proteins'' constructed that localize on membrane and assemble orderly. | |
- | + | ''50% yield increase'' of fatty acids sinply through localizing single TesA onto ''E.coli'''s inner membrane. | |
- | + | ''24 fold of yield increase'' of fatty acids by localizing TesA, FabG, FabZ, and FabI onto ''E.coli'''s inner membrane. | |
- | + | ''fatty-acid-producing Membrane Accelerator upgrades'' by introducing additional two enzymes that convert fatty acids into alkane. | |
{{Template:12SJTU_part_summary_foot}} | {{Template:12SJTU_part_summary_foot}} | ||
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'''Alkane biosynthetic pathway''' | '''Alkane biosynthetic pathway''' | ||
- | 2011 iGEM team of [https://2011.igem.org/Team:Washington/Alkanes/Background Washington University] has introduced two enzymes that could convert ACP-Fatty Acid into alkane. The first enzyme is Acyl-ACP Reductase (AAR) which reduces long chain length acyl-ACPs into the corresponding fatty aldehydes. Long chain fatty aldehyde acts as a substrate for Aldehyde Decarbonylase (ADC), the second enzyme. The enzyme removes the carbonyl group (C=O) from the fatty aldehyde, yielding an alkane molecule one carbon shorter than the original Acyl-ACP and a molecule of formate. Note that FabA, FabB, FabD, FabF, FabG, FabH, FabI, FabZ, and ACP in ''E.coli could'' together synthesize long chain fatty | + | 2011 iGEM team of [https://2011.igem.org/Team:Washington/Alkanes/Background Washington University] has introduced two enzymes that could convert ACP-Fatty Acid into alkane. The first enzyme is Acyl-ACP Reductase (AAR) which reduces long chain length acyl-ACPs into the corresponding fatty aldehydes. Long chain fatty aldehyde acts as a substrate for Aldehyde Decarbonylase (ADC), the second enzyme. The enzyme removes the carbonyl group (C=O) from the fatty aldehyde, yielding an alkane molecule one carbon shorter than the original Acyl-ACP and a molecule of formate. Note that FabA, FabB, FabD, FabF, FabG, FabH, FabI, FabZ, and ACP in ''E.coli could'' together synthesize long chain fatty acyl ACP that could be readily processed by AAR and ADC to produce alkane. |
[[File:12SJTU Alkane Biosynthetic Pathway.png|thumb|center|600px|''Fig.2'' shows alkane synthetic pathway that originates from ''cyanobacteria'' species. Alkane Biosynthetic pathway is combined with Fatty Acid carbon-chain elongation pathway in ''E.coli'']] | [[File:12SJTU Alkane Biosynthetic Pathway.png|thumb|center|600px|''Fig.2'' shows alkane synthetic pathway that originates from ''cyanobacteria'' species. Alkane Biosynthetic pathway is combined with Fatty Acid carbon-chain elongation pathway in ''E.coli'']] | ||
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'''The Priority to Exportation''' | '''The Priority to Exportation''' | ||
- | [[File:12SJTU Fatty acid-wy-1.jpg|350px|right|thumb|''Fig. | + | [[File:12SJTU Fatty acid-wy-1.jpg|350px|right|thumb|''Fig.3'' shows how one solo enzyme anchored onto membrane could serve to facilitate the reaction in term of the priority to exportation.]] |
The fatty acid synthesis is terminated by the hydrolysis of fatty acyl-ACP and the release of free fatty acids into cytoplasm. We suppose TesA anchored on membrane could effectively increase the concentration of fatty acids near membrane, which in turn, facilitates the transmembrane transportation of fatty acids. Higher level of fatty acids in the culture media makes it easier to obtain and purify product and more suitable for industrialized production. On the other hand, TesA removes fatty acyl-ACP from the reaction and thus, according to Le Châtlier principle, shifts the chemical equilibrium to accelerate and to accumulate more fatty acids. | The fatty acid synthesis is terminated by the hydrolysis of fatty acyl-ACP and the release of free fatty acids into cytoplasm. We suppose TesA anchored on membrane could effectively increase the concentration of fatty acids near membrane, which in turn, facilitates the transmembrane transportation of fatty acids. Higher level of fatty acids in the culture media makes it easier to obtain and purify product and more suitable for industrialized production. On the other hand, TesA removes fatty acyl-ACP from the reaction and thus, according to Le Châtlier principle, shifts the chemical equilibrium to accelerate and to accumulate more fatty acids. | ||
To identify and to evaluate the priority of products to exportation, controlled experiments were designed and conducted. Wild type ''E.coli'' and ''E.coli'' overexpressing diffusing cytoplasmic TesA were used as control groups. TesA fused with Lgt was expressed in experimental group. | To identify and to evaluate the priority of products to exportation, controlled experiments were designed and conducted. Wild type ''E.coli'' and ''E.coli'' overexpressing diffusing cytoplasmic TesA were used as control groups. TesA fused with Lgt was expressed in experimental group. | ||
- | [[File:12SJTU membraneTesA.jpg|200px|center|thumb|''Fig. | + | [[File:12SJTU membraneTesA.jpg|200px|center|thumb|''Fig.4'' shows the construction details of membrane anchored TestA]] |
'''The Refinement of Interaction''' | '''The Refinement of Interaction''' | ||
- | [[File:12SJTU Fatty acid-wy-2.jpg|350px|right|thumb|''Fig. | + | [[File:12SJTU Fatty acid-wy-2.jpg|350px|right|thumb|''Fig.5'' shows how membrane could serve to refine and stabilize the interaction upon which enzymes aggregate and cooperate.]] |
Enzymes fused with membrane anchors will be directed to the membrane as expected right after their translation. Thus, the distribution of enzymes is restricted to the 2D membrane rather than diffusing randomly throughout the cytoplasm. Due to spatial restriction, each membrane anchor is more easily to interact with each other. Moreover, the interaction could be stabilized by phospholipid around transmembrane domain. We believe a tandem of enzymes involved in sequential reactions could be organized on the membrane swiftly and orderly in ''Membrane Accelerator''. | Enzymes fused with membrane anchors will be directed to the membrane as expected right after their translation. Thus, the distribution of enzymes is restricted to the 2D membrane rather than diffusing randomly throughout the cytoplasm. Due to spatial restriction, each membrane anchor is more easily to interact with each other. Moreover, the interaction could be stabilized by phospholipid around transmembrane domain. We believe a tandem of enzymes involved in sequential reactions could be organized on the membrane swiftly and orderly in ''Membrane Accelerator''. | ||
To testify and to assess the refinement of interaction, controlled experiments were designed and conducted. Four enzymes are selected based on previous study. We express thioesterase(TesA) and full complement of reductive enzymes(FabG, FabZ and FabI) because previous studies showed moderate overexpression of TesA in ''E.coli'' gave rise to elevated fatty acid productivity and overexpression of reductive enzymes could lead to 50% increase in fatty acid turnover. Wild type ''E.coli'' and ''E.coli'' overexpressing diffusing TesA, FabG, FabZ and FabI were used as control groups. In experimental group, TesA, FabG, FabZ and FabI were linked to orderly organized Membrane Anchors, aligning with corresponding reactions occurring in sequence. All four fusion Membrane Anchors were co-expressed in one cell. | To testify and to assess the refinement of interaction, controlled experiments were designed and conducted. Four enzymes are selected based on previous study. We express thioesterase(TesA) and full complement of reductive enzymes(FabG, FabZ and FabI) because previous studies showed moderate overexpression of TesA in ''E.coli'' gave rise to elevated fatty acid productivity and overexpression of reductive enzymes could lead to 50% increase in fatty acid turnover. Wild type ''E.coli'' and ''E.coli'' overexpressing diffusing TesA, FabG, FabZ and FabI were used as control groups. In experimental group, TesA, FabG, FabZ and FabI were linked to orderly organized Membrane Anchors, aligning with corresponding reactions occurring in sequence. All four fusion Membrane Anchors were co-expressed in one cell. | ||
- | [[File:12SJTU Fatty acid accelerator.jpg|450px|center|thumb|''Fig. | + | [[File:12SJTU Fatty acid accelerator.jpg|450px|center|thumb|''Fig.6'' demonstrates the construction details of ''Membrane Accelerator'' for use of fatty acid synthesis.]] |
The Parts Registered as Membrane Anchor 2 without MS2-TesA, Membrane Anchor 3-FabG, Membrane Anchor 4-FabZ, Membrane Anchor 5 without VVD-FabI are [http://partsregistry.org/Part:BBa_K771305 Part:BBa_K771305], [http://partsregistry.org/Part:BBa_K771306 Part:BBa_K771306], [http://partsregistry.org/Part:BBa_K771307 Part:BBa_K771307], [http://partsregistry.org/Part:BBa_K771308 Part:BBa_K771308], respectively. | The Parts Registered as Membrane Anchor 2 without MS2-TesA, Membrane Anchor 3-FabG, Membrane Anchor 4-FabZ, Membrane Anchor 5 without VVD-FabI are [http://partsregistry.org/Part:BBa_K771305 Part:BBa_K771305], [http://partsregistry.org/Part:BBa_K771306 Part:BBa_K771306], [http://partsregistry.org/Part:BBa_K771307 Part:BBa_K771307], [http://partsregistry.org/Part:BBa_K771308 Part:BBa_K771308], respectively. | ||
===Membrane Accelerator in Alkane Biosynthesis=== | ===Membrane Accelerator in Alkane Biosynthesis=== | ||
+ | |||
+ | '''Flexibility of Reaction Space''' | ||
+ | |||
+ | [[File:12SJTU alkanereactionspace-1.jpg|350px|right|thumb|''Fig.7'' shows we can easily change the reaction space from cytoplasm to periplasm with ''Membrane Accelerator''.]] | ||
As mentioned above, fatty acyl-ACP is produced in ''E.coli'' by a nine-component enzyme system, in which FabG, FabZ, FabI play crucial part. AAR and ADC could then convert fatty acyl-ACP into alkane, the main constituents of diesel fuel. At first, we planned to link FabG, FabZ, FabI, AAR and ADC with constitutively assembling membrane anchors to create a new ''Membrane Accelerator''. In this case, all enzymes face cytoplasm. However, a problem would occur because alkane is very hard to be exported to periplasm. To much alkane would pose stress on ''E.coli''. | As mentioned above, fatty acyl-ACP is produced in ''E.coli'' by a nine-component enzyme system, in which FabG, FabZ, FabI play crucial part. AAR and ADC could then convert fatty acyl-ACP into alkane, the main constituents of diesel fuel. At first, we planned to link FabG, FabZ, FabI, AAR and ADC with constitutively assembling membrane anchors to create a new ''Membrane Accelerator''. In this case, all enzymes face cytoplasm. However, a problem would occur because alkane is very hard to be exported to periplasm. To much alkane would pose stress on ''E.coli''. | ||
- | As we know, aldehyde is more easily to be exported through cell membrane than | + | As we know, aldehyde is more easily to be exported through cell membrane than alkane. Considering the uniqueness and adaptability of Membrane Scaffold system, we decided to place ADC in the periplasmic function domain of Membrane Anchor, as shown in ''Fig.7''. Thus, after the production of fatty aldehyde by AAR in cytoplasm near inner membrane, the long chain aldehyde molecule is readily exported to periplasm. In periplasm, fatty aldehyde is processed by ADC to be converted into free alkane. The upgraded ''Membrane Accelerator'' is expected to facilitate alkane production in ''E.coli'' not only by aggregating enzymes but also by improving alkane exportation. |
- | [[File:12SJTU Alkane accelerator.jpg|450px|center|thumb|''Fig. | + | We have constructed corresponding fusion proteins shown in ''Fig.8''. Full result and data analysis will be out soon. |
+ | |||
+ | [[File:12SJTU Alkane accelerator.jpg|450px|center|thumb|''Fig.8'' demonstrates the construction details of ''Membrane Accelerator'' for use of alkane synthesis.]] | ||
==Result and Discussion== | ==Result and Discussion== | ||
- | === | + | ===Membrane Accelerator in Fatty Acid Biosynthesis=== |
+ | |||
+ | '''Overview''' | ||
+ | |||
Excitingly, the fatty acid biosynthesis was accelerated sharply by recruiting ''membrane accelerator''. The introduction of TesA on membrane alone results in '''50% increase in fatty acids yield'''. By gathering FabG, FabI, FabZ and TesA on the membrane, the production of fatty acid was '''enhanced significantly by 9 fold '''compared with ''E.coli'' overexpressing the same amount of corresponding cytoplasmic enzymes. The statistical data strongly support the superiority of ''Membrane Accelerator''. | Excitingly, the fatty acid biosynthesis was accelerated sharply by recruiting ''membrane accelerator''. The introduction of TesA on membrane alone results in '''50% increase in fatty acids yield'''. By gathering FabG, FabI, FabZ and TesA on the membrane, the production of fatty acid was '''enhanced significantly by 9 fold '''compared with ''E.coli'' overexpressing the same amount of corresponding cytoplasmic enzymes. The statistical data strongly support the superiority of ''Membrane Accelerator''. | ||
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Statistical data are shown as below and GC-MS data are attached to https://2012.igem.org/Team:SJTU-BioX-Shanghai/Parts | Statistical data are shown as below and GC-MS data are attached to https://2012.igem.org/Team:SJTU-BioX-Shanghai/Parts | ||
- | + | ||
'''Assay of the Priority to Exportation''' | '''Assay of the Priority to Exportation''' | ||
- | + | The construction detail of experimental group is shown in ''Fig.4''. Control group is ''E.coli'' expressing the same amount of diffusing cytoplasmic TesA. | |
- | + | TesA is responsible for the hydrolysis of fatty acyl-ACP, with special affinity to C16- and C18- precursor. As ''Fig.9 A'' indicates, 20 hours after induction, ''E.coli'' with membrane anchored TesA experienced a 50% increase in C-16, C-18 fatty acids content and total fatty acids (''Fig.9 B'') in supernatant, compared with ''E.coli'' with free TesA. | |
- | + | [[File:12SJTU-TesA-supernatant.png|thumb|center|750px|''Fig.9'' shows fatty acid content in supernatant of three groups to evaluate the advantages of membrane anchored TesA. A indicates C16/C18 fatty acids content among three groups. B stands for the total amount of fatty acids among three groups.]] | |
- | + | Fatty acids yielded in supernatant went up to 0.71mg/(L·OD). The result supports that membrane anchored TesA could efficiently transfer fatty acyl-ACP into desirable fatty acids right beneath inner membrane, thus making it much easier for the final products to diffuse into periplasmic space. | |
- | ''Fig. | + | [[File:12SJTU-TesA-sediment.png|thumb|center|750px|''Fig.10'' shows fatty acid content in the sediment of three groups to evaluate the advantages of membrane anchored TesA. A indicates C16/C18 fatty acids content among three groups. B stands for the total amount of fatty acids among three groups.]] |
+ | |||
+ | ''Fig.10'', on the other hand, showed fatty acids content in sedimentation also went up by 40%, up to 5.02mg/(L·OD). The result is still within our expectation since fatty acyl-ACP has been removed from the reaction system to form free fatty acids. As a result, the chemical equilibrium shifts and more fatty acids would be accumulated. | ||
We also witnessed a slight decrease in ''E.coli expressing'' free TesA compared with the wildtype, which testifies the statement in a previous study that high levels of TesA inhibits fatty acids synthesis activity but could enhance the activity at low concentrations. | We also witnessed a slight decrease in ''E.coli expressing'' free TesA compared with the wildtype, which testifies the statement in a previous study that high levels of TesA inhibits fatty acids synthesis activity but could enhance the activity at low concentrations. | ||
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'''Assay of the Refinement of Interaction''' | '''Assay of the Refinement of Interaction''' | ||
- | We tried to facilitate exportation of fatty acids by linking TesA to membrane protein. In this way, we accelerated the reaction and increased the turnover per unit time and finally make it possible to efficiently produce fatty acids with longer carbon chains which are much more preferable biofuel precursors. The result verifies one privilege of Membrane Scaffold. Actually another privilege that Membrane Scaffold | + | We have tried to facilitate exportation of fatty acids by linking TesA to membrane protein. In this way, we accelerated the reaction and increased the turnover per unit time and finally make it possible to efficiently produce fatty acids with longer carbon chains which are much more preferable biofuel precursors. The result verifies one privilege of Membrane Scaffold: Priority to Exportation. Actually another privilege that Membrane Scaffold enjoys is that protein interaction is improved and stabilized due to the spatial restriction. Thus we could more easily assemble different enzymes together to decrease the distance that intermediates need to travel between each enzyme. In this way biochemical reaction should be accelerated sharply. |
- | FabG, FabI, FabZ play significant roles in the elongation of carbon chain of fatty acyl-ACP. To optimize the productivity of the system we established, we tried to combine these two privileges (Priority to Exportation and Refinement of Interaction) together, gathering TesA, FabG, FabI and FabZ through protein interaction | + | FabG, FabI, FabZ play significant roles in the elongation of carbon chain of fatty acyl-ACP. To optimize the productivity of the system we established, we tried to combine these two privileges (Priority to Exportation and Refinement of Interaction) together, gathering TesA, FabG, FabI and FabZ on membrane through protein interaction. Notable increase in both diversity and amount of fatty acids was detected compared to control group, which lends strong support to our hypothesis. |
- | + | The construction detail of experimental group is shown in ''Fig.5''. Control group is ''E.coli'' expressing the same amount of diffusing cytoplasmic TesA, FabG, FabI and FabZ. | |
- | + | [[File:12SJTU-fattyAGZI.png|thumb|center|750px|''Fig.11'' shows fatty acid content in supernatant of three groups to evaluate the advantages of membrane anchored TesA,FabG,FabZ and FabI. A indicates C16/C18 fatty acids content. B stands for the total amount of fatty acids. C shows the changes in products diversity.]] | |
- | + | Cluster of FabG, FabI and FabZ provides C16- and C18 specific TesA with sufficient amount of fatty acyl-ACP to hydrolyze and release. Therefore, we witnessed a tremendous growth in the turnover of fatty acids with C16 and C18 skeleton in the supernatant.(Fig.11 A) | |
- | + | Moreover, fatty acid with C14 skeleton was first detected in ''E.coli'' expressing membrane anchored enzymes compared with ones with free enzymes. It is probably because the high productivity of membrane anchored TesA quickly released free fatty acid. Monounsaturated fatty acids also emerge in considerable amount for the first time since TesA is located so closely to the cluster of FabG, FabI and FabZ that it catches intermediate with C16 and C18 skeleton even before they are reduced.(Fig.11 C) | |
- | [[File:12SJTU-123.png|thumb|center|750px|''Fig. | + | Augment in both diversity and amount of fatty acids led to 24 fold increase in total fatty acid yield compared with wild type and 9 fold compared with ''E.coli'' expressing diffusing cytoplasmic enzymes. (Fig.11 B) The exciting result convincingly proves that membrane scaffold enhances protein interaction and cluster of enzymes makes reaction faster to a surprising extent. Products accumulated near inner membrane can traval a shorter distance to be exported to membrane. |
+ | |||
+ | [[File:12SJTU-123.png|thumb|center|750px|''Fig.12'' shows fatty acid content in sediment of three groups to evaluate the advantages of ''Membrane Accelerator''. A indicates C16/C18 fatty acids content. B stands for the total amount of fatty acids.]] | ||
The fatty acids yields increase in sediment is relevantly moderate. The reason might be that membrane anchored enzymes facilitate exportation of large quantity of fatty acids so the amount of fatty acid remaining in cytoplasm is limited. It is notable that C19 fatty acids only exist in cytoplasm because large molecular weight of C19 fatty acid prevents it from exportation and finally they are trapped in the cell. C19 fatty acids yield in ''Membrane Accelerator'' Group is even less than Group with diffusing cytoplasmic enzymes. We suppose it is caused by the high efficiency of TesA which leads to quick release of free fatty acid. | The fatty acids yields increase in sediment is relevantly moderate. The reason might be that membrane anchored enzymes facilitate exportation of large quantity of fatty acids so the amount of fatty acid remaining in cytoplasm is limited. It is notable that C19 fatty acids only exist in cytoplasm because large molecular weight of C19 fatty acid prevents it from exportation and finally they are trapped in the cell. C19 fatty acids yield in ''Membrane Accelerator'' Group is even less than Group with diffusing cytoplasmic enzymes. We suppose it is caused by the high efficiency of TesA which leads to quick release of free fatty acid. | ||
==Future Direction== | ==Future Direction== | ||
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- | + | [[File:12SJTU_Cyano.jpg|350px|right|thumb|Fig.13 ''Cyanobacteria'' under light microscope]] | |
+ | We haven't optimized experiment conditions with respect to strains, growth media, temperature etc., but the result has proved that ''Membrane Accelerator'' could accelerate biosynthetic pathway in ''E.coli'' marvelously. Moreover, changing the proportion of different enzymes in each enzyme assembly on membrane would promisingly enhance biosynthesis rate even more. In the near future, we expected to optimize those conditions to further improve the efficiency of ''Membrane Accelerator''. | ||
- | + | To produce economic biofuel which could be put into mass production, we wanted to transform alkane-producing ''Membrane Accelerator'' into ''Cyanobacteria''. ''Cyanobacteria'' is an autotrophic species which could utilize carbon dioxide and light to produce varieties of organics. Someday we might engineered a new strain of ''Cyanobacteria'' carrying alkane-producing ''Membrane Accelerator'', which could produce and export alkane effectively just by utilizing carbon dioxide and light. Thus the energy crisis would no longer be a problem. | |
==Reference== | ==Reference== |
Latest revision as of 03:54, 27 October 2012
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