Team:NYMU-Taipei/Project/Speedy reporter

From 2010.igem.org

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(EGFP/ERFP + split eIF4A)
(RNA reporter device)
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==RNA reporter device==
==RNA reporter device==
===[[Team:NYMU-Taipei/Project/Speedy reporter/Material and Methods#GFP| GFP ]]===
===[[Team:NYMU-Taipei/Project/Speedy reporter/Material and Methods#GFP| GFP ]]===
-
*Splitting the GFP({{:Team:NYMU-Taipei/BBa|E0040}}) on the split point between 157th and 158th amino acid which was generated by iGEM07_Davidson_Missouri's {{:Team:NYMU-Taipei/BBa|I715019}} and {{:Team:NYMU-Taipei/BBa|I715020}}.The A-part split is the same as {{:Team:NYMU-Taipei/BBa|I715019}} ,but the B-part is one base different from {{:Team:NYMU-Taipei/BBa|I715020}}.After the spliting,we both add linkers in back of A-part split and B-part split via PCR.By doing so,we can get well-prepared for the next step.
+
*Splitting the GFP({{:Team:NYMU-Taipei/BBa|E0040}}) between the 157th and 158th amino acid which was generated by iGEM07_Davidson_Missouri's {{:Team:NYMU-Taipei/BBa|I715019}} and {{:Team:NYMU-Taipei/BBa|I715020}}.The A-part split is the same as {{:Team:NYMU-Taipei/BBa|I715019}}, the B-part is one base different from {{:Team:NYMU-Taipei/BBa|I715020}}.After splitting, we added linkers in back of A-part split and in front of B-part split via PCR.
=== [[Team:NYMU-Taipei/Project/Speedy reporter/Material and Methods#RFP| RFP ]] ===
=== [[Team:NYMU-Taipei/Project/Speedy reporter/Material and Methods#RFP| RFP ]] ===
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*Splitting RFP ({{:Team:NYMU-Taipei/BBa|E1010}}) on the split point between 154th and 155th amino acid used by iGEM07_Davidson_Missouri's {{:Team:NYMU-Taipei/BBa|I715022}} and {{:Team:NYMU-Taipei/BBa|I715023}}.The A-part split is the same as {{:Team:NYMU-Taipei/BBa|I715022}}, but the B-part has one base difference from {{:Team:NYMU-Taipei/BBa|I715023}}.After the spliting,we both add linkers in back of A-part split and B-part split via PCR.By doing so,we can get well-prepared for the next step.
+
*Splitting RFP ({{:Team:NYMU-Taipei/BBa|E1010}}) between the 154th and 155th amino acid used by iGEM07_Davidson_Missouri's {{:Team:NYMU-Taipei/BBa|I715022}} and {{:Team:NYMU-Taipei/BBa|I715023}}.The A-part split is the same as {{:Team:NYMU-Taipei/BBa|I715022}}, the B-part has one base difference from {{:Team:NYMU-Taipei/BBa|I715023}}. After splitting, we added linkers in back of A-part split and in front of B-part split via PCR.
=== [[Team:NYMU-Taipei/Project/Speedy reporter/Material and Methods#eIF4A| eIF4A]] (need help)===
=== [[Team:NYMU-Taipei/Project/Speedy reporter/Material and Methods#eIF4A| eIF4A]] (need help)===
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*We take the protein coding region from the [http://www.ncbi.nlm.nih.gov/nuccore/NM_144958 eIF4A mRNA transcript sequence from Mouse (from NCBI)] and found it had 2 PstI cutting sites. For fear that our PstI cutting enzyme would cut the wrong place,we need to mutate the two PstI cutting sites.After mutation,we split eIF4A ({{:Team:NYMU-Taipei/BBa|K411100}}) at 215&216th amino acid.
+
*We take the protein coding region from the [http://www.ncbi.nlm.nih.gov/nuccore/NM_144958 eIF4A mRNA transcript sequence from Mouse (from NCBI)] and found that it had 2 PstI cutting sites. Fearing that PstI cutting enzyme would cut in the wrong place, we mutated the two PstI cutting sites. After mutation, we split eIF4A ({{:Team:NYMU-Taipei/BBa|K411100}}) between the  215th and 216th amino acid.
*The template of eIF4A on a [http://genome-www.stanford.edu/vectordb/vector_descrip/COMPLETE/PGEX4T1.SEQ.html pGEX-4TI vector] was kindly provided by Pro.C.Proud.
*The template of eIF4A on a [http://genome-www.stanford.edu/vectordb/vector_descrip/COMPLETE/PGEX4T1.SEQ.html pGEX-4TI vector] was kindly provided by Pro.C.Proud.

Revision as of 17:01, 27 October 2010


Contents

Overview design by figure

Abstract

  • Our Speedy RNA+protein reporter effectively skips protein folding when reporting, thus reducing the time for a fluorescent response.

More specific insights into molecular mechanisms and gene regulation are essential for improvement in synthetic biology. Understanding these mechanisms requires time. Our speedy reporter for reporting RNA and protein expression in a cell effectively skips protein folding when reporting -- the longest part of gene expression -- thus reducing the time needed to get a fluorescence. By speeding up the reporter, in both RNA and protein, we have also speed up the exploration for rules in the biological system. We can not only generate more novel circuits but also explore gene regulations in synthetic biology.

Introduction

Recent studies of mRNA localization show that a great part of mRNA localize in specific cytoplasm position (Martin, 2009). For examples, ASH1 mRNA localize at bud tip of budding yeast to allow asymmetric segregation from mother to daughter cell (Paquin, 2007). In the Drosophila the localization of mRNA at anterior and posterior of oocyte play an important role in the developing embryo (Johnstone, 2001). Local translation of mRNAs in axonal growth cones helps axon navigate to it synaptic partners (Lin, 2007). β-actins mRNA localize at sites of active actins polymerization, cytoskeletal-mediate motility need mRNA translation (Huttelmaier, 2005). All the examples above is studies on eukaryotic system. there are a few studies of mRNA location in prokaryotic system. And most of synthetic biology designs on prokaryotic bacteria. The more basic rule of prokaryotic system we know, the more successful and speedy experiments we will have.

The common way to detect mRNA is RT-PCR, which can only be done in vitro but can’t in a real living cell. The common way to detect the protein is fusion a reporter protein such as GFP to report it, and the folding of GFP takes about four hours. In order to do both assay speedy and in vivo, we apply a novel technique Bimolecular Fluorescence Complementation, BiFC. In our design, we need not to wait four hours for folding of GFP to detect our protein fusion GFP. We can get our signal in few minute using this method. And it also can detect the mRNA both location and quantity (Demidov, 2006). We can use this method save about fours for protein assay and two hours for mRNA assay (Fig.1).

Figure.1 compare to the traditional method of detecting mRNA and protein. our speedy reporter only need 3 min to obtain signal (Demidov, 2006).
BiFC is developed base on the technique Protein-fragment Complement Assay, PCA (Demidov, 2006; Barnard, 2008). Protein-protein interactions coupled to refolding of a pair of split enzymes in the PCA technique. The enzyme used in PCA has it activity only when two split parts reconstruct together. The activities of enzyme act as a detector of protein-protein interaction (Remy, 2007). While the BiFC technique use split fluorescent protein instead of split enzyme in the PCA. The split form of fluorescent protein alone has no fluorescence. Fluorescence appears when two split parts reassembly together immediately in few minutes. For mRNA detection, we design a system differ from BiFC’s protein-protein interaction to RNA-protein interaction. Where a GFP is split into two inactive parts and fused with two parts of the split-eIF4A protein, a kind of RNA binding protein. On the other hand, we designed an mRNA aptamer that the eIF4A protein can bind to. EGFP will fluoresce through the interaction of split eIF4A and its corresponding aptamer. Using this method, we can immediately detect mRNA quantity and location in vivo. For protein detection, we design another system of BiFC which RFP is splits into two inactive parts and fused with two parts of antibody light chain and heavy chain. And then we fused the antigen to target protein. When target protein fusion antigen appears, the light chain and heavy chain combine with antigen. And then split RFPs reconstruct and fluoresce.

Design

  • Our circuit design:
    • EGFP-eIF4A system / RNA aptamer on plasmid pSB1C3.

EGFP-eIF4A system on plasmid pSB1C3. RNA aptamer on plasmid pSB1C3.

EGFP/ERFP + split eIF4A

  • split GFP/RFP

We split the EGFP/ERFP into two parts, the larger N-terminal part and the smaller C-terminal part. The N-terminal part contains performed chromophore and has a very weak fluorescence that is hard to detect. Only when it combines with the small C-terminal fragment, does the fluorescence becomes very bright. When both parts combine, we can detect the location of the mRNA and protein. The probability that these two split parts of EGFP/ERFP can fit together without an outside force is very low, thus ther are few false-positive signal (Demidov, 2006).

  • eIF4A

eIF4A is an abbreviation for eukaryotic initiation factor 4A. It is a member of the DEAD-box RNA helicase protein family eIF4F (Zunakamu, 2002), and the DEAD-box is one of the largest subgroups of the RNA helicase protein family (Story, 2000). Eukaryotic translation initiation factor 4F (eIF4F) is a protein consist of eIF4A, eIF4E, and eIF4G. eIF4A is a helicase need ATP to unwind the secondary structure of mRNA untranslated region and make ribosome binds easier. eIF4E can binds to the cap structure of mRNA. eIF4G is like a scaffold of eIF4A and eIF4E helping them coordinate their functions. Without eIF4E and eIF4G the eIF4A alone exist much lower RNA helicase activity than complete eIF4F (Imataka et al., 1997).

eIF4A aptamer

  • What is eIF4A aptamer? (Zunakamu, 2002)

The eIF4A aptamer that we used has a high affinity for complete eIF4A protein. Its affinity is strong enough that it will combine the split eIF4A(described above) into a complete eIF4A protein. In the presence of eIF4A aptamer, ATP hydrolysis is inhibited and the RNA substrate which binds onto the eIF4A cannot unwind. It is proposed that the eIF4A structure is in a equilibrium between dumbbell-shaped structure and compact struction in solution. In the presence of ATP and absence of RNA aptamer, the equilibrium will be shifted into the dumbbell-shaped eIF4A (Fig.2). In the opposite condition, the equilibrium will be shifted into the compact one (Valencia-Burton, 2007).

Figure.2 Two domains and the structure equilibrium of eIF4A (Zunakamu, 2002)
  • eIF4A aptamer Secondary structure:
    • Structure predicted by RNAfold:
      Figure.3 Aptamer Structure predicted by RNAfold
    • Structure of eIF4A aptamer:
      Figure.4 Aptamer Structure (Oguro, 2002)

Material and Methods

We constructed two devices by the parts below:

  • RNA reporter consists of :
    • EGFP
    • ERFP
    • eIF4A
    • fusion parts
    • aptamer
  • protein reporter consists of :
    • split RFP
    • split peptide adaptor

RNA reporter device

GFP

  • Splitting the GFP([http://partsregistry.org/Part:BBa_E0040 BBa_E0040]) between the 157th and 158th amino acid which was generated by iGEM07_Davidson_Missouri's [http://partsregistry.org/Part:BBa_I715019 BBa_I715019] and [http://partsregistry.org/Part:BBa_I715020 BBa_I715020].The A-part split is the same as [http://partsregistry.org/Part:BBa_I715019 BBa_I715019], the B-part is one base different from [http://partsregistry.org/Part:BBa_I715020 BBa_I715020].After splitting, we added linkers in back of A-part split and in front of B-part split via PCR.

RFP

  • Splitting RFP ([http://partsregistry.org/Part:BBa_E1010 BBa_E1010]) between the 154th and 155th amino acid used by iGEM07_Davidson_Missouri's [http://partsregistry.org/Part:BBa_I715022 BBa_I715022] and [http://partsregistry.org/Part:BBa_I715023 BBa_I715023].The A-part split is the same as [http://partsregistry.org/Part:BBa_I715022 BBa_I715022], the B-part has one base difference from [http://partsregistry.org/Part:BBa_I715023 BBa_I715023]. After splitting, we added linkers in back of A-part split and in front of B-part split via PCR.

eIF4A (need help)

  • We take the protein coding region from the [http://www.ncbi.nlm.nih.gov/nuccore/NM_144958 eIF4A mRNA transcript sequence from Mouse (from NCBI)] and found that it had 2 PstI cutting sites. Fearing that PstI cutting enzyme would cut in the wrong place, we mutated the two PstI cutting sites. After mutation, we split eIF4A ([http://partsregistry.org/Part:BBa_K411100 BBa_K411100]) between the 215th and 216th amino acid.
  • The template of eIF4A on a [http://genome-www.stanford.edu/vectordb/vector_descrip/COMPLETE/PGEX4T1.SEQ.html pGEX-4TI vector] was kindly provided by Pro.C.Proud.

Fusion parts

GFP fusion system

  • We fuse the split-GFP part with split-eIF4A part by PCR. So we get two sequences: split-GFP-A+linker+split-eIF4A-A([http://partsregistry.org/Part:BBa_K411101 BBa_K41111])and split-GFP-B+linker+split-eIF4A-B([http://partsregistry.org/Part:BBa_K411102 (BBa_K11102)])We add terminators in back of both sequences and insert them into one plasmid.
EGFP-eIF4A system on plasmid pSB1C3.





The picture shows the templates of PCR potocol. The split-GFP part and split-eIF4A parthave complementary linker sequences, which will be able to anneal during the PCR process.

RFP fusion system

  • We fuse the split-RFP part with split-eIF4A part by PCR. So we get two sequences:split-RFP-A+linker+split-eIF4A-A ([http://partsregistry.org/Part:BBa_K411103 BBa_K411103])and split-GFP-B+linker+split-eIF4A-B([http://partsregistry.org/Part:BBa_K411104 BBa_K411104])


aptamer

  • We performed PCR to get the needed aptamer by ourselves based on sequence showed on a paper of (Valencia-Burton07).

We first designed primers that adding prefix in the front of the aptamer sequence and suffix in the end of the aptamer sequence. We then digested the aptamer with Xbal&PstI cutting enzymes and the pLac with Spal&PstI cutting enzymes. Then we then used ligase to join them together.

protein reporter device

The basic principle of protein reporter device is the same as the RNA reporter. First, we fuse split RFP with anti-His tag antibody light chain and heavy chain. Second, we fuse His-tag sequence with our target protein sequence. Once our target protein sequence being tranlated the anti-His tag antibody will binding on the Histidine tag. And then with combining of the heavy chain and the light chain, The split ERFP reconstruct and make brightly fluorescence.

Figure.5 The structure of anti-His tag antibody. Green stand for the heavy chain and the red stand for the light chain (PDB ID: 1KTR).

Advantage

1.Test the promotor strength in a speedy way.

  • In tradition, the inducible promoter strength is tested by the reporter gene (e.g. GFP)behind the promoter. And need to wait for GFP folding for about four hours. In our design, we can test the promoter strength in the mRNA level and it only needs 3 min for the split GFP to reconstitute a functional protein.
  • If your promoter is strong, it will transcribe into more RNA apmaters. In presence of more RNA aptamer, more of our split GFP will bind on it and emit stronger fluorescence. If your promoter is not strong enough, it won't transcribe into amounts of RNA aptamer. The less the RNA aptamer will be produced, the less our split GFP will bind on to it. Therefore, the less the fluorescence will come out.

2.Locate a specific gene or chemicals which can be heavy metals or so.

  • Like the promoter testing, we can use the inducible promoter which inducers are heavy metal(e.g. As or Zn). When the heavy metal is present, the promoter will be induced and transcribed into mRNA aptamer. With our GFP reporter, it will bind to the RNA aptamer and emit fluorescence as usual. So, we can know that there must be heavy metal pollution in that environment.

3.Help to test other teams' biobricks.

4.mRNA positioning in a sigle cell.

  • By understanding the RNA localization in a cell, we can know more about how gene regulation works in a cell. And by understanding more about the precise gene regulations, we can explore more about the design rules in synthetic biology.

5.Can measure the quantities of the mRNA.

6.View the temporal dynamics in a cell

7.Speed up the reporting progress.

  • We can do a protein assay or mRNA assay in our speedy reporter system and get our signals within about 3 mins. It is faster than RT-PCR for mRNA which needs about two hours and western blot for protein quantitative analysis which needs a bout 4.5 hours.
  • The split GFP is constitutive in the cell. Once the RNA aptamer is transcribed, the split GFP linked with eIF4A will bind to the RNA aptamer due to its high affinity. We skip the translation process due to the well-generated GFP.

References

  • Maria Valencia-Burton, Ron M McCullough, Charles R Cantor & Natalia E Broude. 2007. RNA visualization in live bacterial cells using fluorescent protein complementation. Nature method 4 (5), 421-427.
  • Akihiro Oguro, Takahashi Ohtsu, Yuri V. Svitkin, Nahum Sonenberg, and
  • Yoshika Zunakamu RA1 .2002. RNA aptamers to initiation factor 4A helicase hinder cap-dependent translation by blocking ATP hydrolysis.
  • Hiroaki Imataka, and Nahum Sonenberg. 1997. Human Eukaryotic Translation Initiation Factor 4G (eIF4G) Possesses Two Separate and Independent Binding Sites for eIF4A. Mol. Cell. Biol. 17:6940-6947
  • Randall M. Story, Hong Li*, and John N. Abelson. 2000. Crystal structure of a DEAD box protein from the hyperthermophile Methanococcus jannaschii.
  • Oliver Rackham and Chris M Brown. 2004. Visualization of RNA–protein interactions in living cells: FMRP and IMP1 interact on mRNAs.
  • Vadim V Demidov & Natalia E Broude,2006. Profluorescent protein fragments for fast bimolecular fluorescence complementation in vitro.
  • Paula Montero Llopis, Audrey F. Jackson, Oleksii Sliusarenko, Ivan Surovtsev, Jennifer Heinritz, Thierry Emonet, Christine Jacobs-Wagner.,2010. Spatial organization of the flow of genetic information in bacteria.
  • Dale Muzzey, Alexander van Oudenaarden.,2009. Quantitative Time-Lapse Fluorescence Microscopy in Single Cells.
  • Andrew C Lin and Christine E Holt,2007. Local translation and directional steering in axons. The EMBO journal 26:3729-3736
  • Stefan Hüttelmaier, Daniel Zenklusen, Marcell Lederer, Jason Dictenberg, Mike Lorenz, XiuHua Meng, Gary J. Bassell, John Condeelis & Robert H. Singer., 2005. Spatial regulation of β-actin translation by Src-dependent phosphorylation of ZBP1. Nature 438:512-515
  • Kelsey C. Martin, and Anne Ephrussi, 2009. mRNA Localization: Gene Expression in the Spatial Dimension. Cell 136:719-730
  • Nicolas Paquin and Pascal Chartrand,2007. Local regulation of mRNA translation: new insights from the bud. Trends in Cell Biology 18 , v3:105-111
  • Oona Johnstone and Paul Lasko, 2001. TRANSLATIONAL REGULATION AND RNA LOCALIZATION IN DROSOPHILA OOCYTES AND EMBRYOS. Annu. Rev. Genet. 35, 365-406
  • Ingrid Remy and Stephen W. Michnick, 2007. Application of protein-fragment complementation assays in cell biology. BioTechniques 42 (2),137-145
  • Emma Barnard, Neil V. McFerran, Alan Trudgett, John Nelson and David J. Timson. 2008. Development and implementation of split-GFP-based bimolecular fluorescence complementation (BiFC) assays in yeast. Biochem. Soc. Trans. 36, 479-482.