Difference between revisions of "Part:BBa K4162118"
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===Characterization===
 
===Characterization===
  
====定性1标题 ====
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====Agarose gel electrophoresis====
  
定性1文字
+
[[File:T--Fudan--Agarose gel electrophoresis--crtEBIY.png|400px|thumb|none|'''Figure 1. T--Fudan--Agarose gel electrophoresis--crtEBIY.png.''' The first lane was loaded with D2000 DNA ladder whose sizes were marked on the image. We chose Taq DNA polymerase for its low cost and high reliability, and we designed forward and reverse primers for each carotene synthesis enzyme (crt for short). The PCR reaction was composed of 2 μL 10x Taq polymerase buffer, 16 μL H2O, 0.5 μL Taq polymerase, 0.5 μL dNTP (10 mM each), 0.5 μL forward primer (10 mM), 0.5 μL reverse primer (10 mM), and 1 μL bacterial culture or 1μL colony. Using the same forward primer, and different reverse primers, we were able to detect the composition of various crt genes. After PCR, the correct bacterial clones were sent for Sanger sequencing. Once verified, these clones would be used for further experiments. The sequences of primers are: > 5-crtE 5-ATGACGGTCTGCGCAAAAAAAC-3; > rev320crtB 5-CCTTCCAGATGATCAAACGCGTAAG-3; > rev320crtE 5-ATGAGAATGAATGGTAGGGCGTC-3; > rev320crtI 5-GGATTAAACTGCTGAATCTGCGCTTC-3; > rev320crtY 5-CCGCGGTATCCATCCACAAG-3.]]
  
[[File:T--Fudan--定性1图片不要用中文做文件名.png|400px|thumb|none|'''Figure 1. 图标题.''' 图注 引用的不要忘了写某某人某某年的出处]]
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====Successful product expression====
  
定性1小结
 
  
====定性2标题 ====
 
  
定性2文字
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[[File:T--Fudan--EBI--96.png|400px|thumb|none|'''Figure 5. 96-well plate of module crtEBI [https://parts.igem.org/Part:BBa_K4162108 BBa_K4162108].''' All wells had similar lycopene content in the bacterial pellets.]]
  
[[File:T--Fudan--定性2图片不要用中文做文件名.png|400px|thumb|none|'''Figure 2. 图标题.''' 图注 引用的不要忘了写某某人某某年的出处]]
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[[File:T--Fudan--118.png|400px|thumb|none|'''Figure 3. ''']]
  
定性2小结
 
  
 
====定性3标题 ====
 
 
定性3文字 <ref>T7 phage factor required for managing RpoS in Escherichia coli. Tabib-Salazar A,  Liu B,  Barker D,  Burchell L,  Qimron U,  Matthews SJ,  Wigneshweraraj S. Proc Natl Acad Sci U S A, 2018 Jun 5;115(23):E5353-E5362.  PMID:29789383</ref>. 又一个参考文献在一对尖括号内,例子里的参考文献格式是pubmed直接copy的
 
 
[[File:T--Fudan--定性3图片不要用中文做文件名.png|400px|thumb|none|'''Figure 3. 图标题.''' 图注 引用的不要忘了写某某人某某年的出处]]
 
 
定性3小结
 
  
 
<!-- Add more about the biology of this part here
 
<!-- Add more about the biology of this part here

Revision as of 16:17, 11 October 2022


ribozyme+RBS+CDS module: crtEBIY

Introduction

2021 Fudan

This biobrick was created through overlapping PCR of BBa_K4162009(ribozyme+B0_RBS+crtE), BBa_K4162013(ribozyme+T7_RBS+crtB), BBa_K4162016(ribozyme+T7_RBS+crtI) and BBa_K4162019(ribozyme+T7_RBS+crtY). These genes are a part of the carotenoid biosynthesis pathway and together, this biobrick converts farnesyl pyrophosphate to beta-carotene. In this part, the RNA sequences of hammerhead ribozyme conduct self-cleaving, and the polycistronic mRNA transcript is thus co-transcriptionally converted into individual mono-cistrons in vivo. Self-interaction of the polycistron can be nullified and each cistron can initiate translation with comparable efficiency.

Usage and Biology

We transfected this biobrick into E. coli to build single-cell factory for beta-carotene production. Coding sequences of crtEBIY are separated by ribozyme sequences. In this part, the RBS of crtBIY has equal intensity while the RBS of crtE is significantly stronger than the others. Since crtE catalyzes the first step of the carotenoid reaction chain, the concentration of substrate for the reaction catalyzed by this enzyme is significantly higher than for the next three steps of the reaction. To avoid more serious flux imbalance problems, we boosted the RBS intensity of crtE only in this biobrick and explored whether the carotenoid production of the strain could be significantly enhanced.

Characterization

Agarose gel electrophoresis

Figure 1. T--Fudan--Agarose gel electrophoresis--crtEBIY.png. The first lane was loaded with D2000 DNA ladder whose sizes were marked on the image. We chose Taq DNA polymerase for its low cost and high reliability, and we designed forward and reverse primers for each carotene synthesis enzyme (crt for short). The PCR reaction was composed of 2 μL 10x Taq polymerase buffer, 16 μL H2O, 0.5 μL Taq polymerase, 0.5 μL dNTP (10 mM each), 0.5 μL forward primer (10 mM), 0.5 μL reverse primer (10 mM), and 1 μL bacterial culture or 1μL colony. Using the same forward primer, and different reverse primers, we were able to detect the composition of various crt genes. After PCR, the correct bacterial clones were sent for Sanger sequencing. Once verified, these clones would be used for further experiments. The sequences of primers are: > 5-crtE 5-ATGACGGTCTGCGCAAAAAAAC-3; > rev320crtB 5-CCTTCCAGATGATCAAACGCGTAAG-3; > rev320crtE 5-ATGAGAATGAATGGTAGGGCGTC-3; > rev320crtI 5-GGATTAAACTGCTGAATCTGCGCTTC-3; > rev320crtY 5-CCGCGGTATCCATCCACAAG-3.

Successful product expression

Figure 5. 96-well plate of module crtEBI BBa_K4162108. All wells had similar lycopene content in the bacterial pellets.
Figure 3.


Sequence and Features


Assembly Compatibility:
  • 10
    COMPATIBLE WITH RFC[10]
  • 12
    COMPATIBLE WITH RFC[12]
  • 21
    INCOMPATIBLE WITH RFC[21]
    Illegal BamHI site found at 2202
  • 23
    COMPATIBLE WITH RFC[23]
  • 25
    INCOMPATIBLE WITH RFC[25]
    Illegal NgoMIV site found at 1681
    Illegal NgoMIV site found at 1811
    Illegal AgeI site found at 839
  • 1000
    COMPATIBLE WITH RFC[1000]