Difference between revisions of "Team:LMU-TUM Munich/Design"

 
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<div class="imagelink float-right">[[Media:Muc16_Sticker_Design_001.png]][[Image:Muc16_Sticker_Design_001.png|350px|link=]]
[[File:Muc16_Sticker_Design_001.png |right|350px]]
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=Design of synthetic receptors for pseudo-covalent cross-linking of cells for bioprinting=
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=Receptor design highlights=
 
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In the following, we are going to explore the thought processes that went into the design of the receptors that allow us to embed eukaryotic cells into a stable, three-dimensional protein matrix immediately upon printing.  
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''Think before you ink'' may be a popular slogan wielded by tattoo adversaries, but it has also been perfectly applicable to creating our synthetic biology approach of bioprinting. In the following, we explore the contemplations that contributed to the design of the membrane proteins (also referred to as 'receptors') that allow us to embed eukaryotic and bacterial cells into a [https://2016.igem.org/Team:LMU-TUM_Munich/Proof stable, three-dimensional and user-definable matrix] immediately upon printing.  
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</div>
  
For this purpose, we built '''two kinds of receptor constructs''' that both on their own, when being expressed in mammalian cells, are able to cross-link cells in streptavidin solution in our very own approach of bioprinting.
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=Human cell surface receptors=
  
1) '''A receptor containing an extracellular biotin acceptor peptide''' that is endogenously biotinylated by a coexpressed biotin ligase (BirA) and thus presents biotin groups at the cell surface.
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<div class="imagelink float-right">[[Media:Muc16 receptor schematic_002.png]][[Image:Muc16 receptor schematic_002.png|300px|link=]]
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<div class="caption">'''Figure 1''': A) Receptor constructs in a schematic representation of functional genetic elements. B) Schematic representation of a receptor presenting an extracellular single-chain avidin that is endogenously biotinylated by a coexpressed biotin ligase (BirA) and thus presents biotin groups at the cell surface.</div></div>
  
[[File:Muc16 receptor schematic_002.png|thumb|right|360px|'''A)''' Schematic depiction of the modular structure of the created genetic receptor constructs.
 
'''B)''' Schematic depiction of the modular structure of the membrane receptors for cross-linking of cells via biotin-streptavidin interactions.]]
 
The biotin acceptor peptide (BAP) is a 15 amino acid peptide sequence originating from <i>E. coli</i>. <ref>Chen, I., Howarth, M., Lin, W., & Ting, A. Y. (2005). Site-specific labeling of cell surface proteins with biophysical probes using biotin ligase. Nature methods, 2(2), 99-104.</ref> Being biotinylated by the biotin ligase BirA at a lysine residue within the recognition sequence, it mediates the functionality of the receptor by presenting biotin, allowing the interaction of the cell surface with streptavidin in the reservoir solution.
 
The biotin ligase BirA is therefore encoded by the same vector as the receptor, with an internal ribosome entry site (IRES) allowing translation of two open reading frames (ORFs) from a single polycistronic plasmid. BirA is targeted to the ER via an Ig&kappa; signal peptide as well as an ER retention signal, allowing it to biotinylate translocating proteins possessing the recognition sequence.
 
  
2) '''Receptors presenting an extracellular, monomeric or single-chain avidin variant'''.
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For this purpose, we built '''two kinds of receptor constructs''', both on their own able – when expressed in mammalian cells – to cross-link cells for our approach of bioprinting:
  
These avidin derivates, by design, allow the functional fusion of the otherwise tetrameric avidin molecule with our receptor. Two different variants were hereby used: The so-called ''enhanced monomeric avidin'', a single subunit avidin that is able to bind biotin as a monomer, and single-chain avidin, which resembles the naturally occuring avidin tetramer, but has the subunits being connected via polypeptide linkers.
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1) '''A receptor presenting an extracellular biotin acceptor peptide''' that is endogenously biotinylated by a coexpressed biotin ligase (BirA), thus presenting biotin molecules on the cellular surface and allowing it to interact with streptavidin in the printing solution.
  
Both receptors generally mediate the same purpose: By interacting with streptavidin in the printing reservoir - either directly by presenting biotin (biotin acceptor-peptide) or indirectly via binding to a biotinylated linker (single chain-avidin variants), cells are being cross-linked due to the polyvalent binding of single streptavidin molecules in the printing solution to several cellular biotin groups at once.
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2) '''Receptors presenting an extracellular monomeric or single-chain avidin variant'''.
</div>
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==The incredible journey: signal peptides and protein targeting==
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Essential to a protein's function is not only its activity or binding properties, but also its presence at the right time, at the right place - in our case, the right place being the cell surface. One of the most ubiquitous elements for protein targeting is the signal peptide, which enables the translocation of proteins to the ER, from where their journey may continue to their place of function. Proteins containing a signal peptide include transmembrane proteins, secreted proteins, proteins of the ER itself, proteins of the Golgi apparatus and several more.<ref>Rapoport, T. A. (2007). Protein translocation across the eukaryotic endoplasmic reticulum and bacterial plasma membranes. Nature, 450(7170), 663-669.</ref>  For our project, signal peptides constitute a crucial part for many constructs, being used for targeting of transmembrane proteins to the cell surface (receptors), targeting proteins to the ER (BirA) and the secretion of proteins into the surrounding medium (luciferase assays for the quantification of expression levels).
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[[File:Muc16 SP schematic.jpeg|thumb|right|420px|Schematic depiction of the co-translational translocation of a membrane protein into the ER. Shown are the nascent, unfolded peptide chain containing the signal peptide ('start-transfer sequence') as well as the stop-transfer sequence, and the ER membrane.<ref>Taken from Alberts, B., Bray, D., Hopkin, K., Johnson, A., Lewis, J., Raff, M., ... & Walter, P. (2010). Essential cell biology. Garland Science.</ref>]]
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The hydrophobic signal peptide (also called ''start-transfer sequence'') usually consists of less than 30 amino acids <ref>Walter, P., Ibrahimi, I., & Blobel, G. U. N. T. E. R. (1981). Translocation of proteins across the endoplasmic reticulum. I. Signal recognition protein (SRP) binds to in-vitro-assembled polysomes synthesizing secretory protein. The Journal of Cell Biology, 91(2), 545-550.</ref> and is recognized by the signal recognition particle upon translation at the rough ER, mediating the co-translational translocation of the nascent peptide chain into the ER.<ref>Keenan, Robert J., et al. "The signal recognition particle." Annual review of biochemistry 70.1 (2001): 755-775.</ref> During this project, three different signal peptide constructs are being tested in order to determine the one resulting in the highest expression levels:
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* The EGFR signal peptide was taken from the iGEM parts registry ([http://parts.igem.org/Part:BBa_K157001:Design BBa_K157001]) and combined with a BioBrick containing the CMV promoter sequence ([http://parts.igem.org/Part:BBa_K747096 BBa_K747096]) via the RFC10 cloning standard.
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In presenting avidin on the cell surface, cells are able to interact with a co-injected biotinylated linker peptide. With this linker connected to several cell surface avidins as well as streptavidin in the printing solution, a protein matrix is created that embeds cells and allows precise positioning of cells in a three-dimensional manner.
  
* The BM40 and Ig&kappa; signal peptides were designed by us and synthesized under the aspect of adding additional spacing and functional elements to the 5'-UTR of the constructs, and combined with a BioBrick containing the CMV promoter sequence ([http://parts.igem.org/Part:BBa_K747096 BBa_K747096]) via the RFC10 cloning standard.  
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Our chosen avidin derivates by design allow functional fusion of the otherwise tetrameric avidin molecule with our receptor. Two different variants were used: ''enhanced monomeric avidin'', a single-subunit avidin that is nevertheless able to bind biotin, and ''single-chain avidin'', which resembles the naturally occurring avidin tetramer but consisting of a single polypeptide chain.
  
As shown below, the EGFR signal peptide taken from the parts registry is constructed in a way that the signal peptide ORF immediately follows the RFC10 cloning scar after the CMV promoter, thus resulting in a very short 5’ untranslated region (UTR) of the transcribed mRNA. The combination of the CMV promoter with the synthesized BM40 and Ig&kappa; signal peptides allows for a considerably longer 5’ UTR of the resulting mRNA - additionally allowing them to contain a full Kozak consensus sequence by design. The Kozak sequence is recognized by the ribosome as a translational start site; this element missing or deviating from the consensus sequence may considerably decrease translation efficiency.<ref>Kozak, M. (1989). The scanning model for translation: an update. The Journal of cell biology, 108(2), 229-241.</ref> For the EGFR signal peptide construct, a Kozak sequence is not present, as it would have to preceed the start codon ATG - a position which is occupied by the RFC10 cloning scar.
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All receptors mediate the same function: By interacting with streptavidin in the printing reservoir – either directly by presenting biotin (biotin acceptor peptide) or indirectly via binding to a biotinylated linker (single-chain avidin variants), cells are cross-linked due to polyvalent binding of streptavidin molecules in the printing solution to several cellular biotin groups at once.
Since both the distance from the promoter to the open reading frame as well as the Kozak consensus sequence are considered crucial parameters for expression levels<ref>Kozak, M. (1987). An analysis of 5'-noncoding sequences from 699 vertebrate messenger RNAs. Nucleic acids research, 15(20), 8125-8148.</ref>, BM40 and Ig&kappa; signal peptide constructs are likely to resut in increased expression levels compared to proteins containing the EGFR signal peptide from the parts registry.
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</div>
 
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===Prediction of signal peptide functionality===
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==The incredible journey: signal peptides and protein targeting==
 
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As the quantitative functionality of signal peptides had to be determined before including one of these into the final receptor constructs, the three options (Ig&kappa;, BM40, EGFR) were tested via bioinformatic tools as well as a secretion assay of luciferase constructs.
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Essential to a protein's function are not only its activity or binding properties, but also its presence at the right time in the right place – the latter in our case being the cell surface. One ubiquitous element for protein targeting is the signal peptide, which enables translocation of proteins to the ER, from where their journey continues to their place of function. Proteins containing a signal peptide include transmembrane proteins, secreted proteins, proteins of the ER itself, proteins of the Golgi apparatus and several more.<ref>Rapoport, T. A. (2007). Protein translocation across the eukaryotic endoplasmic reticulum and bacterial plasma membranes. Nature, 450(7170), 663-669.</ref> For our project, signal peptides constituted a crucial part of many constructs, used to target transmembrane proteins to the cell surface (receptors) and proteins to the ER (BirA), and to secrete proteins into the surrounding medium (luciferase assays to quantify expression levels).
</div>
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===Bioinformatic signal peptide analysis via the SignalP server===
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<div class="imagelink float-right">[[Media:Muc16 SP schematic.jpeg]][[Image:Muc16 SP schematic.jpeg|420px|link=]]
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<div class="caption">'''Figure 2:''' Cotranslational translocation of a membrane protein into the ER in a schematic depiction showing the nascent, unfolded peptide chain containing signal peptide (''start-transfer sequence'') and ''stop-transfer sequence'' as well as the ER membrane.<ref>Taken from Alberts, B., Bray, D., Hopkin, K., Johnson, A., Lewis, J., Raff, M., ... & Walter, P. (2010). Essential cell biology. Garland Science.</ref></div></div>
  
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The hydrophobic signal peptide (also called ''start-transfer sequence'') usually consists of less than 30 amino acids <ref>Walter, P., Ibrahimi, I., & Blobel, G. U. N. T. E. R. (1981). Translocation of proteins across the endoplasmic reticulum. I. Signal recognition protein (SRP) binds to in-vitro-assembled polysomes synthesizing secretory protein. The Journal of Cell Biology, 91(2), 545-550.</ref> and is recognized by the signal recognition particle upon translation at the rough ER, mediating cotranslational translocation of the nascent peptide chain into the ER.<ref>Keenan, Robert J., et al. "The signal recognition particle." Annual review of biochemistry 70.1 (2001): 755-775.</ref>
The [http://www.cbs.dtu.dk/services/SignalP SignalP] server, being able to discriminate between the hydrophobic signal peptide sequence and the hydrophobic transmembrane domain<ref>Petersen, T. N., Brunak, S., von Heijne, G., & Nielsen, H. (2011). SignalP 4.0: discriminating signal peptides from transmembrane regions. Nature methods, 8(10), 785-786.</ref>, can determine whether a sequence possesses the biophysical requirements for functioning as a signal peptide. Furthermore, it is able to predict the probable cleavage site of the signal peptide after its translocation into the ER. For all constructs, signal peptide functionality is predicted, as well as a potential cleavage site. The complete translated amino acid sequences of the respective receptor constructs were used as input. The algorithm for eukaryotes with default D-cutoff value was chosen.  
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[[File:Muc16 SignalPeptideprediction_002.png|thumb|center|850px|
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During this project, three different signal peptide constructs were tested in order to determine that resulting in the highest expression levels:
  
'''A)''' Schematic depiction of a protein-coding mRNA containing a 5'- and 3'-UTR, the first of which being an important factor in translation efficiency. '''B)''' Identification of signal peptides within the receptor construct containing the EGFR, Ig&kappa; and BM40 signal peptide via the SignalP 4.1 server. Plotted probabilities represent the raw cleavage site “C-score”, the signal peptide “S-score” and the combined cleavage site “Y-score”. '''C)''' ClustalW multiple  sequence alignment of the BM40, EGFR and Ig&kappa; signal peptide construct, depicting a gap for the EGFR-signal peptide construct compared to the newly designed ones, indicating smaller length of the 5'-UTR . For the Ig&kappa; and BM40 signal peptide constructs, a T7 promoter spacer as well as a Kozak sequence increase the distance between TATA-box and protein-coding region.]]
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* The '''EGFR signal peptide''' was taken from the iGEM parts registry ([http://parts.igem.org/Part:BBa_K157001:Design BBa_K157001]) and combined with a BioBrick containing the CMV promoter sequence ([http://parts.igem.org/Part:BBa_K747096 BBa_K747096]) via the RFC10 cloning standard.
  
For all three signal peptides, the high S-score indicates high signal peptide functionality. For the Ig&kappa; signal peptide, a cleavage site between amino acid 20 and 21 within the signal peptide is predicted. For the BM40 signal peptide, a cleavage site between amino acid 17 and 18 is predicted, and for the EGFR signal peptide, a cleavage site between amino acid 24 and 25 is predicted.
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* The '''BM40 and Ig&kappa; signal peptides''' were designed by us and synthesized with regard to adding additional spacing and functional elements to the 5'-UTR of the constructs, and combined with a BioBrick containing the CMV promoter sequence ([http://parts.igem.org/Part:BBa_K747096 BBa_K747096]) via the RFC10 cloning standard.
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===Quantification of signal-peptide mediated translocation via a secretion luciferase assay===
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The EGFR signal peptide taken from the parts registry is constructed such that the signal peptide ORF immediately follows the RFC10 cloning scar after the CMV promoter, thus resulting in a very short 5’ untranslated region (UTR) of transcribed mRNA. The combination of the CMV promoter with the synthesized BM40 and Ig&kappa; signal peptides allows for a considerably longer 5’-UTR – and can thus be made to contain a full Kozak consensus sequence by design. The Kozak sequence is recognized by the ribosome as a translational start site; if this element is missing or deviates from the consensus sequence, this may considerably decrease translation efficiency.<ref>Kozak, M. (1989). The scanning model for translation: an update. The Journal of cell biology, 108(2), 229-241.</ref> For the EGFR signal peptide construct, a Kozak sequence is not present, as it would have to precede the start codon ATG, i.e. the position occupied by the RFC10 cloning scar.
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Since both the distance from the promoter to the open reading frame and the Kozak consensus sequence are considered crucial parameters for expression levels<ref>Kozak, M. (1987). An analysis of 5'-noncoding sequences from 699 vertebrate messenger RNAs. Nucleic acids research, 15(20), 8125-8148.</ref>, BM40 and Ig&kappa; signal peptide constructs are likely to result in increased expression levels compared to proteins containing the EGFR signal peptide from the parts registry.
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</div>
  
 
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For the quantification of signal peptide functionality via a luciferase assay, three constructs were created and tested - each containing one of three signal peptides (the EGFR signal peptide, the Ig&kappa; signal peptide or the BM40 signal peptide) and a nanoluciferase as well as a CMV promoter, a ''Strep''-tag II for immunochemical detection and the hGH polyadenylation signal sequence. Not containing a transmembrane domain, the nanoluciferase fusion protein is being translocated into the ER and then secreted into the medium. Using a luciferase assay, one can quantifiy the amount of luminescence - and thus, proportionally, the amount of secreted luciferase - by measuring the conversion of luciferin into visible light and integrating it over a timespan of 5 s. Therefore, medium samples were taken every 12 h after transfection of cells and measured via the Promega NanoGlo luciferase assay system according to the manufacturer's instructions.  
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In order to predict whether our designed signal peptides would be functional, we used the [http://www.cbs.dtu.dk/services/SignalP SignalP] server, which allows to make theoretical predictions about signal peptide functionality and cleavage.<ref>Petersen, T. N., Brunak, S., von Heijne, G., & Nielsen, H. (2011). SignalP 4.0: discriminating signal peptides from transmembrane regions. Nature methods, 8(10), 785-786.</ref>
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<div class="imagelink float-right">[[Media:Muc16 SignalPeptideprediction_002.png]][[Image:Muc16 SignalPeptideprediction_002.png|820px|link=]]
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<div class="caption">'''Figure 3:''' A) Schematic depiction of a protein-coding mRNA containing a 5'- and 3'-UTR, the first of which is an important factor in translation efficiency. B) Theoretical prediction of signal peptides within the receptor construct containing the EGFR, Ig&kappa; and BM40 signal peptide via the SignalP 4.1 server. Plotted probabilities represent the raw cleavage site “C-score”, the signal peptide “S-score” and the combined cleavage site “Y-score”. C) ClustalW multiple sequence alignment of the BM40, EGFR and Ig&kappa; signal peptide construct, depicting a gap for the EGFR signal peptide construct compared to the newly designed ones and thus indicating a shorter length of the 5'-UTR . For Ig&kappa; and BM40 signal peptide constructs, a T7 promoter spacer as well as a Kozak sequence increase the distance between TATA box and protein-coding region.</div></div>
  
[[File:Rsz receptor signalpeptideresults 003.png|thumb|center|850px|'''A)''' Schematic depiction of the genetic constructs used for signal peptide testing via a secretion luciferase assay. '''B)''' Results of the luciferase assay, showing luminescence in relative luminescence units (RLU) as a function of time for the previously described three different signal peptide constructs as well as a control construct containing no signal peptide. '''C)''' Detection of secreted luciferases in the medium via a Western Blot, using an anti-<i>Strep</i>-tag II antibody as well as a horse raddish peroxidase-coupled secondary antibody for detection.]]
 
 
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===Other receptor elements: stability and detection===
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==Elements for stability and detection==
  
 
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For anchoring in the membrane, we decided to use a type I membrane protein, which possesses a single membrane span with defined localization of N- and C-terminus out- and inside of the cell, respectively. The N-terminal transmembrane &alpha;-helix of human EGFR (UniProt P00533, amino acids 622-653) was herefore chosen (see below the topology prediction of EGFR via the [http://www.cbs.dtu.dk/services/TMHMM/ TMHMM 2.0 server for the prediction of transmembrane helices]<ref>Sonnhammer, E. L., Von Heijne, G., & Krogh, A. (1998, July). A hidden Markov model for predicting transmembrane helices in protein sequences. In Ismb (Vol. 6, pp. 175-182).</ref>). A stop-transfer sequence consisting of charged amino acids - being characteristic for type I membrane proteins - was added at the C-terminus, and the sequence was furthermore flanked by a (GGGGC)<sub>2</sub>-linker at the N- and C-terminus, respectively. The addition of a stop-transfer sequence as in the naturally occuring EGFR sequence, as well as the addition of flexible linkers, makes our EGFR-TMD an improvement over the BioBrick [http://partsregistry.org/wiki/index.php?title=Part:BBa_K157002 BBa_K157002], which does not possess either of these elements.
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For anchoring in the membrane, a type I membrane protein with defined localization of N- and C-terminus out- and inside of the cell was used. The N-terminal transmembrane &alpha;-helix of human EGFR (UniProt P00533, amino acids 622-653) was herefore chosen (see below the topology prediction of EGFR via the [http://www.cbs.dtu.dk/services/TMHMM/ TMHMM 2.0 server for the prediction of transmembrane helices]<ref>Sonnhammer, E. L., Von Heijne, G., & Krogh, A. (1998, July). A hidden Markov model for predicting transmembrane helices in protein sequences. In Ismb (Vol. 6, pp. 175-182).</ref>). A stop-transfer sequence consisting of charged amino acids - being characteristic for type I membrane proteins - was added at the C-terminus, and the sequence was furthermore flanked by a (GGGGC)<sub>2</sub>-linker at the N- and C-terminus, respectively. The addition of a stop-transfer sequence as in the naturally occurring EGFR sequence, as well as the addition of flexible linkers, makes our EGFR-TMD an improvement over the BioBrick [http://partsregistry.org/wiki/index.php?title=Part:BBa_K157002 BBa_K157002], which does not possess either of these elements.
  
  
[[File:Receptor TMD 002.png|thumb|center|850px|'''A)''' Multiple sequence alignment of human EGFR (see [http://www.uniprot.org/uniprot/P00533 UniProt P00533]), the EGFR transmembrane domain BioBrick from the registry ([http://partsregistry.org/wiki/index.php?title=Part:BBa_K157002 BBa_K157002] and the extended EGFR transmembrane designed by us, containing a charged stop-transfer domain as well as linker elements at the C- and N-termini. '''B)''' Transmembrane domain prediction by the [http://www.cbs.dtu.dk/services/TMHMM/ TMHMM 2.0 server], indicating positioning of N- and C-termini out- and inside of the cell, respectively, as well as predicting functionality of transmembrane regions. '''C)''' Schematic depiction of the C-terminal stop-transfer sequence of the receptor.]]
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<div class="imagelink float-right">[[Media:Receptor TMD 002.png]][[Image:Receptor TMD 002.png|820px|link=]]
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<div class="caption"></div>'''Figure 4:''' A) Multiple sequence alignment of human EGFR (see [http://www.uniprot.org/uniprot/P00533 UniProt P00533]), the EGFR transmembrane domain BioBrick from the registry ([http://partsregistry.org/wiki/index.php?title=Part:BBa_K157002 BBa_K157002] and the extended EGFR transmembrane designed by us, containing a charged stop-transfer domain as well as linker elements at the C- and N-termini. B) Transmembrane domain prediction by the [http://www.cbs.dtu.dk/services/TMHMM/ TMHMM 2.0 server], indicating positioning of N- and C-termini out- and inside of the cell, respectively, as well as predicting functionality of transmembrane regions. C) Schematic depiction of the C-terminal stop-transfer sequence of the receptor.</div>
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==Elements for detection==
  
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In order to confirm the correct expression and localization of the receptor, the receptor contains '''three functional elements for its detection''' for both the N- and the C-terminal receptor domains:
  
Moreover, the receptor contains '''three functional elements for its detection''': The intracellularly located red fluorescent protein mRuby 3 for detection of the receptor via fluorescence microscopy, an extracellular epitope domain for immunochemical detection via A3C5-antibody fragments and an intracellular <i>Strep</i>-tag II for the detection and purification via immunochemical methods.
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* The intracellularly located C-terminal '''red fluorescent protein mRuby 3''' for detection of the receptor via fluorescence microscopy while also providing a stable, folded domain at the C-terminus,
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* an '''extracellular epitope domain''' near the N-terminus for immunochemical detection via A3C5-antibody fragments as well as FACS, and  
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* an '''intracellular <i>Strep</i>-tag II''' at the N-terminus for the detection and purification via immunochemical methods.
  
The vector furthermore contains the poly-adenylation signal of human growth hormone (hGH) for functional polyadenylation of the transcribed mRNA. A description for the respective functional elements is given in the following sections.
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Further elements that were included into the expression construct are the CMV promoter for overall high expression levels of the receptor, resulting in a high-avidity-interaction. At the 3'-end, the construct contains the polyadenylation signal of human growth hormone (hGH) for functional polyadenylation of the transcribed mRNA.  
 
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===A3C5 epitope tag===
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=Design of an autotransporter construct for bacterial surface display=
 
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Antibodies have various areas of application in life science, including protein detection, pulldown experiments and even immunotherapy. Having originally been discovered in 1995 during an ''in vitro'' screening for antibodies against cytomegaloviral proteins<ref>Alexander, H., Harpprecht, J., Podzuweit, H. G., Rautenberg, P., & Müller-Ruchholtz, W. (1994). Human monoclonal antibodies recognize early and late viral proteins of human cytomegalovirus. Human Antibodies, 5(1-2), 81-90.</ref>, the A3C5 antibody is an established molecular tool for specific recognition of proteins. By tagging cell surface proteins with an epitope specifically recognized by A3C5 (being a peptide sequence of 11 amino acids), one is easily able to detect tagged proteins via immunofluorescence microscopy, FACS or one may purify them via pulldown experiments. Through the latter, one may also screen for in vivo interaction partners of the tagged protein.
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Besides the design of biotinylated and biotin-binding receptors for eukaryotic cells, we also wanted to apply our <span style="color:#009440">biot</span><span style="color:#3070b3">INK</span> approach for prokaryotic cells. For this purpose, we designed an autotransporter device that is able to present biotinylated or biotin-binding protein domains on the surface of ''E. coli''. Constructs for bacterial surface display are hereby already well known in the field of protein engineering of therapeutic proteins, such as antibodies. There, they are used to screen libraries of different antibodies concerning their affinity towards a given therapeutic target.  
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===mRuby 3===
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We based our design on the autotransporter EspP<ref>Binder, U., Matschiner, G., Theobald, I., & Skerra, A. (2010). High-throughput sorting of an Anticalin library via EspP-mediated functional display on the Escherichia coli cell surface. Journal of molecular biology, 400(4), 783-802.</ref>.
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<div class="imagelink float-right">[[Media:Muc16 Autotransporterdesign_001.png]][[Image:Muc16 Autotransporterdesign_001.png|820px|link=]]
Having originally been engineered as a monomeric form of the red fluorescent protein eqFP611, mRuby variants are sine of the brightest red fluorescent proteins available. <ref>Kredel, S., Oswald, F., Nienhaus, K., Deuschle, K., Röcker, C., Wolff, M., ... & Wiedenmann, J. (2009). mRuby, a bright monomeric red fluorescent protein for labeling of subcellular structures. PloS one, 4(2), e4391.</ref> With an excitation maximum at a wavelength of 558 nm and an emission wavelength maximum of 605 nm, the resulting stokes shift of 57 nm makes mRuby a good choice for fluorescent microscopy imaging and, thus, allows the visualization of the receptor in its cellular environment by being fused to the C-terminus of the transmembrane domain. mRuby is especially powerful for the fusion with receptors - not only due to its small size and high stability, but also due to the fact that, in comparison with eGFP, it appears up to 10 times brighter in membrane enviroments. The mRuby variant used here is mRuby 3, having been engineered for even more improved brightness and photostability.<ref>Bajar, B. T., Wang, E. S., Lam, A. J., Kim, B. B., Jacobs, C. L., Howe, E. S., ... & Chu, J. (2016). Improving brightness and photostability of green and red fluorescent proteins for live cell imaging and FRET reporting. Scientific reports, 6.</ref>
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<div class="caption"></div>'''Figure 5'''</div>
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===<i>Strep</i>-tag II===
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The autotransporter system itself is established and functional (see Fig. A<ref>Binder, U., Matschiner, G., Theobald, I., & Skerra, A. (2010). High-throughput sorting of an Anticalin library via EspP-mediated functional display on the Escherichia coli cell surface. Journal of molecular biology, 400(4), 783-802.</ref>), and here we "bricked" it down into RFC[10] and RFC[25] BioBricks. At first, we tested different inducible bacterial promoter systems (e.g. "TetR repressed GFP"; [http://parts.igem.org/Part:BBa_K577893 BBa_K577893]) that are available in the parts registry, but when we saw that two of the available systems did not work in our own hands, we decided to built the system on our own. We used the Tet-Repressor generator that was available on the distribution plates ([http://parts.igem.org/Part:BBa_I739001 BBa_I739001]) as we believe that it is very important for the standardization in SynBio to use available parts. Downstream of this repressor generator we designed and fused a BioBrick ([http://parts.igem.org/Part:BBa_K2170141 BBa_K2170141]) that encodes a double Tet-Operator (Tet-Repressor binding site together with a bacterial promoter and an signal peptide of the outer membrane protein A (OmpA<ref>Ghrayeb, J., Kimura, H., Takahara, M., Hsiung, H., Masui, Y., & Inouye, M. (1984). Secretion cloning vectors in Escherichia coli. The EMBO journal, 3(10), 2437.</ref>) from ''E. coli'' that has a 3' RFC[25] restriction site, allowing the protein fusion of proteins that are secreted into the bacterial periplasm when expressed with this BioBrick. As a protein fusion, we then assembled a protein cargo domain that is generally exchangeable for any protein that is so small in size that it can be transported through the outer membrane by the EspP autotransporter. In our project we used the same extracellular domains as for the eukaryotic receptors: enhanced monomeric Avidin (eMA; [http://parts.igem.org/Part:BBa_K2170204 BBa_K2170204]), single-chain Avidin (scAvidin; [http://parts.igem.org/Part:BBa_K2170205 BBa_K2170205]) and a composite part composed of a N-terminal Biotinylation acceptor peptide (BAP) and a C-terminal NanoLuciferase (together shown as BAP; ; [http://parts.igem.org/Part:BBa_K2170118 BBa_K2170118], see Fig. B). Our design features an A3C5-epitope tag further downstream that can be recognized by a high-affinity Fab-fragment and is generally used to detect and quantify the surface display of the cargo domain<ref>Costa, J., Grabenhorst, E., Nimtz, M., & Conradt, H. S. (1997). Stable expression of the Golgi form and secretory variants of human fucosyltransferase III from BHK-21 cells Purification and characterization of an engineered truncated form from the culture medium. Journal of Biological Chemistry, 272(17), 11613-11621.</ref>. Further downstream of this affinity tag we fused the BioBrick for the EspP autotransporter from ''E. coli''<ref>Barnard, T. J., Dautin, N., Lukacik, P., Bernstein, H. D., & Buchanan, S. K. (2007). Autotransporter structure reveals intra-barrel cleavage followed by conformational changes. Nature structural & molecular biology, 14(12), 1214-1220.</ref><ref>Skillman, K. M., Barnard, T. J., Peterson, J. H., Ghirlando, R., & Bernstein, H. D. (2005). Efficient secretion of a folded protein domain by a monomeric bacterial autotransporter. Molecular microbiology, 58(4), 945-958.</ref> which is then followed by a bacterial terminator. For the termination we chose again  a well-working terminator from the distribution plate ("double terminator"; [http://parts.igem.org/Part:BBa_B0010 BBa_B0010]-[http://parts.igem.org/Part:BBa_B0012 BBa_B0012]).<br> But this was just the DNA-part. What is expected to happen on a protein level? The construct constantly produces Tet-repressor that binds to the Tet-Operator and repressed the promoter activity of the autotransporter gene. As soon as the inducer anhydrotetracycline (aTc) is added to the culture, it binds to the Tet-repressor that can't bind anymore to the Tet-operator and thus the expression of the autotransporter can be regulated. Although the TetR-system is known to be a tight promoter system there is always a certain background expression with most promoters. If the protein expression of the autotransporter is induced using aTc the autotransporter is transcribed and translated. Due to the bacterial signal peptide, the protein is secreted into the bacterial periplasm (the space between the two bacterial membranes of gram-negative bacteria such as ''E. coli''). When present in the bacteria periplasm the autotransporter diffused to the outer membrane and inserts into the membrane. After the integration into the outer membrane, the protein cargo is transported through the beta-barrel of the autotransporter and is presented on the bacterial surface. We are sure that this BioBrick will be a valuable contribution to the Parts Registry as it allows future teams to display small protein domains on the surface of gram-negative bacteria, such as ''E. coli''.
<div class="white-box">
+
The <i>Strep</i>-tag II is an eight amino acid peptide sequence that specifically interacts with Streptavidin and can thus be used for easy one-step purification of the receptor via immunochemical methods.<ref>Schmidt, T. G., & Skerra, A. (2007). The Strep-tag system for one-step purification and high-affinity detection or capturing of proteins. Nature protocols, 2(6), 1528-1535.</ref>
+
 
</div>
 
</div>
  
===Nanoluciferase===
+
=References=
 
<div class="white-box">
 
<div class="white-box">
The concept of bioluminescence has a great meaning for several invertebrate species, allowing communication with other individuals, signaling receptiveness or deterring predators.<ref>Case, J. F. (2004). Flight studies on photic communication by the firefly Photinus pyralis. Integrative and comparative biology, 44(3), 250-258.</ref> The most common enzyme responsible for the creation of bioluminescence are the luciferases (from the latin words ’lux’ and ’ferre’, meaning ’light-carrier’).
+
<references />
These enzymes, among others found in fireflies and deep-sea shrimp, commonly consume a substrate called luciferin as well as energy in the form of ATP or reduction equivalents in order to create light-emission through oxidation. The underlying mechanism hereby relies on the creation of an instable, highly excited intermediate under the consumption of energy. This high-energy intermediate then spontaneously falls back into a state of lower energy, emitting the energetical difference as visible light. While mainly being used as a folded, stabilizing element at the N-terminus for the construct containing the biotin acceptor peptide, the nanoluciferase could also be used for advanced binding studies via luciferase assays.<ref>Zhang, L., Song, G., Xu, T., Wu, Q. P., Shao, X. X., Liu, Y. L., ... & Guo, Z. Y. (2013). A novel ultrasensitive bioluminescent receptor-binding assay of INSL3 through chemical conjugation with nanoluciferase. Biochimie, 95(12), 2454-2459.</ref>
+
[[File:Muc16 Nanoluc Mech.png|thumb|right|400px| Reaction scheme of the reaction catalyzed by the NanoLuc nanoluciferase. Taken from the [https://www.promega.com/-/media/files/resources/protocols/technical-manuals/101/nanoglo-luciferase-assay-system-protocol.pdf NanoGlo Assay Kit manual.]]]
+
Luciferases have also found their way into biotechnological applications.<ref>Gould, S. J., & Subramani, S. (1988). Firefly luciferase as a tool in molecular and cell biology. Analytical biochemistry, 175(1), 5-13.</ref> The simplistic concept of creating visible (and thus easily measurable) light makes luciferases ideal reporters for the expression of secretable proteins via a corresponding assay. This project also made use of a luciferase for the determination of expression levels of the BAP surface receptor while providing a stable and folded domain at the N-terminus, as well as having been used for the choice of signal peptide. The monomeric luciferase used in this project, the so-called ’NanoLuc&trade;'<ref>Hall, M. P., Unch, J., Binkowski, B. F., Valley, M. P., Butler, B. L., Wood, M. G., ... & Robers, M. B. (2012). Engineered luciferase reporter from a deep sea shrimp utilizing a novel imidazopyrazinone substrate. ACS chemical biology, 7(11), 1848-1857.</ref> (due to terms of simplicity referred to as ’nanoluciferase’ in the following), can be fused to other proteins in order to make their expression visible and quantifiable. This engineered luciferase emits a steady, easily detectable glow when exposed to its substrate, while being only 19 kDa large and being brighter, more specific and steadier than other luciferases commonly found in nature. Using luciferases for the quantification of expression levels offers several advantages over fluorescent proteins, including higher sensitivity and smaller size.
+
 
</div>
 
</div>
 
===CMV promoter===
 
<div class="white-box">
 
Last but not least, high expression levels of the receptor, so that a high avidity for the interaction may be reached. The CMV promoter (taken from the parts registry, [http://parts.igem.org/Part:BBa_K74709 BBa_K74709]) therefore enables constitutively high expression of the receptor - and, in the case of the BAP-construct, the biotin ligase BirA.
 
</div>
 
 
==The final construct==
 
 
<div class="white-box">
 
The final expression construct for the eukaryotic cell receptor is shown belown for the receptor with the biotin acceptor peptide (BAP). Other constructs differ from this one by not encoding the eIF4G1-IRES as well as not encoding the biotin ligase BirA. Instead of the biotin acceptor peptide, those constructs encode a monomeric or single-chain avidin variant.
 
 
[[File:Muc16 BAP vecto.jpeg |thumb|center|800px| Schematic depiction of the complete expression vector for the BAP-based receptor as well as the corresponding biotin ligase. Shown are the CMV promoter element, the signal peptide (depending on the construct being the EGFR signal peptide, the Ig&kappa; signal peptide or the BM40 signal peptide, the latter two furthermore possessing an elongated 5’ UTR), the biotin acceptor peptide, a nanoluciferase, an epitope tag for A3C5 antibodies, the EGFR N-terminal transmembrane &alpha;-helix, mRuby, a ''Strep''-tag II, an IRES from eIF4G1 for polycistronic transcription, BirA including a Ig&kappa; signal peptide as well as an ER retention signal sequence, and the hGH polyadenylation signal sequence.]].
 
 
=References=
 
 
 
 
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{{LMU-TUM_Munich_html_end}}

Latest revision as of 14:10, 3 December 2016

Receptor design highlights

Think before you ink may be a popular slogan wielded by tattoo adversaries, but it has also been perfectly applicable to creating our synthetic biology approach of bioprinting. In the following, we explore the contemplations that contributed to the design of the membrane proteins (also referred to as 'receptors') that allow us to embed eukaryotic and bacterial cells into a stable, three-dimensional and user-definable matrix immediately upon printing.

Human cell surface receptors


For this purpose, we built two kinds of receptor constructs, both on their own able – when expressed in mammalian cells – to cross-link cells for our approach of bioprinting:

1) A receptor presenting an extracellular biotin acceptor peptide that is endogenously biotinylated by a coexpressed biotin ligase (BirA), thus presenting biotin molecules on the cellular surface and allowing it to interact with streptavidin in the printing solution.

2) Receptors presenting an extracellular monomeric or single-chain avidin variant.

In presenting avidin on the cell surface, cells are able to interact with a co-injected biotinylated linker peptide. With this linker connected to several cell surface avidins as well as streptavidin in the printing solution, a protein matrix is created that embeds cells and allows precise positioning of cells in a three-dimensional manner.

Our chosen avidin derivates by design allow functional fusion of the otherwise tetrameric avidin molecule with our receptor. Two different variants were used: enhanced monomeric avidin, a single-subunit avidin that is nevertheless able to bind biotin, and single-chain avidin, which resembles the naturally occurring avidin tetramer but consisting of a single polypeptide chain.

All receptors mediate the same function: By interacting with streptavidin in the printing reservoir – either directly by presenting biotin (biotin acceptor peptide) or indirectly via binding to a biotinylated linker (single-chain avidin variants), cells are cross-linked due to polyvalent binding of streptavidin molecules in the printing solution to several cellular biotin groups at once.

The incredible journey: signal peptides and protein targeting

Essential to a protein's function are not only its activity or binding properties, but also its presence at the right time in the right place – the latter in our case being the cell surface. One ubiquitous element for protein targeting is the signal peptide, which enables translocation of proteins to the ER, from where their journey continues to their place of function. Proteins containing a signal peptide include transmembrane proteins, secreted proteins, proteins of the ER itself, proteins of the Golgi apparatus and several more.[1] For our project, signal peptides constituted a crucial part of many constructs, used to target transmembrane proteins to the cell surface (receptors) and proteins to the ER (BirA), and to secrete proteins into the surrounding medium (luciferase assays to quantify expression levels).

The hydrophobic signal peptide (also called start-transfer sequence) usually consists of less than 30 amino acids [3] and is recognized by the signal recognition particle upon translation at the rough ER, mediating cotranslational translocation of the nascent peptide chain into the ER.[4]

During this project, three different signal peptide constructs were tested in order to determine that resulting in the highest expression levels:

  • The EGFR signal peptide was taken from the iGEM parts registry ([http://parts.igem.org/Part:BBa_K157001:Design BBa_K157001]) and combined with a BioBrick containing the CMV promoter sequence ([http://parts.igem.org/Part:BBa_K747096 BBa_K747096]) via the RFC10 cloning standard.
  • The BM40 and Igκ signal peptides were designed by us and synthesized with regard to adding additional spacing and functional elements to the 5'-UTR of the constructs, and combined with a BioBrick containing the CMV promoter sequence ([http://parts.igem.org/Part:BBa_K747096 BBa_K747096]) via the RFC10 cloning standard.


The EGFR signal peptide taken from the parts registry is constructed such that the signal peptide ORF immediately follows the RFC10 cloning scar after the CMV promoter, thus resulting in a very short 5’ untranslated region (UTR) of transcribed mRNA. The combination of the CMV promoter with the synthesized BM40 and Igκ signal peptides allows for a considerably longer 5’-UTR – and can thus be made to contain a full Kozak consensus sequence by design. The Kozak sequence is recognized by the ribosome as a translational start site; if this element is missing or deviates from the consensus sequence, this may considerably decrease translation efficiency.[5] For the EGFR signal peptide construct, a Kozak sequence is not present, as it would have to precede the start codon ATG, i.e. the position occupied by the RFC10 cloning scar. Since both the distance from the promoter to the open reading frame and the Kozak consensus sequence are considered crucial parameters for expression levels[6], BM40 and Igκ signal peptide constructs are likely to result in increased expression levels compared to proteins containing the EGFR signal peptide from the parts registry.

In order to predict whether our designed signal peptides would be functional, we used the [http://www.cbs.dtu.dk/services/SignalP SignalP] server, which allows to make theoretical predictions about signal peptide functionality and cleavage.[7]

Elements for stability and detection

Apart from the functional parts that mediate the (strept)avidin-biotin interaction, other elements in the receptor were designed to make sure it is optimally translocated to the membrane, as stable as possible, and easily detectable.

EGFR transmembrane domain

For anchoring in the membrane, a type I membrane protein with defined localization of N- and C-terminus out- and inside of the cell was used. The N-terminal transmembrane α-helix of human EGFR (UniProt P00533, amino acids 622-653) was herefore chosen (see below the topology prediction of EGFR via the [http://www.cbs.dtu.dk/services/TMHMM/ TMHMM 2.0 server for the prediction of transmembrane helices][8]). A stop-transfer sequence consisting of charged amino acids - being characteristic for type I membrane proteins - was added at the C-terminus, and the sequence was furthermore flanked by a (GGGGC)2-linker at the N- and C-terminus, respectively. The addition of a stop-transfer sequence as in the naturally occurring EGFR sequence, as well as the addition of flexible linkers, makes our EGFR-TMD an improvement over the BioBrick [http://partsregistry.org/wiki/index.php?title=Part:BBa_K157002 BBa_K157002], which does not possess either of these elements.


Elements for detection

In order to confirm the correct expression and localization of the receptor, the receptor contains three functional elements for its detection for both the N- and the C-terminal receptor domains:

  • The intracellularly located C-terminal red fluorescent protein mRuby 3 for detection of the receptor via fluorescence microscopy while also providing a stable, folded domain at the C-terminus,
  • an extracellular epitope domain near the N-terminus for immunochemical detection via A3C5-antibody fragments as well as FACS, and
  • an intracellular Strep-tag II at the N-terminus for the detection and purification via immunochemical methods.

Further elements that were included into the expression construct are the CMV promoter for overall high expression levels of the receptor, resulting in a high-avidity-interaction. At the 3'-end, the construct contains the polyadenylation signal of human growth hormone (hGH) for functional polyadenylation of the transcribed mRNA.

Design of an autotransporter construct for bacterial surface display

Besides the design of biotinylated and biotin-binding receptors for eukaryotic cells, we also wanted to apply our biotINK approach for prokaryotic cells. For this purpose, we designed an autotransporter device that is able to present biotinylated or biotin-binding protein domains on the surface of E. coli. Constructs for bacterial surface display are hereby already well known in the field of protein engineering of therapeutic proteins, such as antibodies. There, they are used to screen libraries of different antibodies concerning their affinity towards a given therapeutic target.

We based our design on the autotransporter EspP[9].

The autotransporter system itself is established and functional (see Fig. A[10]), and here we "bricked" it down into RFC[10] and RFC[25] BioBricks. At first, we tested different inducible bacterial promoter systems (e.g. "TetR repressed GFP"; [http://parts.igem.org/Part:BBa_K577893 BBa_K577893]) that are available in the parts registry, but when we saw that two of the available systems did not work in our own hands, we decided to built the system on our own. We used the Tet-Repressor generator that was available on the distribution plates ([http://parts.igem.org/Part:BBa_I739001 BBa_I739001]) as we believe that it is very important for the standardization in SynBio to use available parts. Downstream of this repressor generator we designed and fused a BioBrick ([http://parts.igem.org/Part:BBa_K2170141 BBa_K2170141]) that encodes a double Tet-Operator (Tet-Repressor binding site together with a bacterial promoter and an signal peptide of the outer membrane protein A (OmpA[11]) from E. coli that has a 3' RFC[25] restriction site, allowing the protein fusion of proteins that are secreted into the bacterial periplasm when expressed with this BioBrick. As a protein fusion, we then assembled a protein cargo domain that is generally exchangeable for any protein that is so small in size that it can be transported through the outer membrane by the EspP autotransporter. In our project we used the same extracellular domains as for the eukaryotic receptors: enhanced monomeric Avidin (eMA; [http://parts.igem.org/Part:BBa_K2170204 BBa_K2170204]), single-chain Avidin (scAvidin; [http://parts.igem.org/Part:BBa_K2170205 BBa_K2170205]) and a composite part composed of a N-terminal Biotinylation acceptor peptide (BAP) and a C-terminal NanoLuciferase (together shown as BAP; ; [http://parts.igem.org/Part:BBa_K2170118 BBa_K2170118], see Fig. B). Our design features an A3C5-epitope tag further downstream that can be recognized by a high-affinity Fab-fragment and is generally used to detect and quantify the surface display of the cargo domain[12]. Further downstream of this affinity tag we fused the BioBrick for the EspP autotransporter from E. coli[13][14] which is then followed by a bacterial terminator. For the termination we chose again a well-working terminator from the distribution plate ("double terminator"; [http://parts.igem.org/Part:BBa_B0010 BBa_B0010]-[http://parts.igem.org/Part:BBa_B0012 BBa_B0012]).
But this was just the DNA-part. What is expected to happen on a protein level? The construct constantly produces Tet-repressor that binds to the Tet-Operator and repressed the promoter activity of the autotransporter gene. As soon as the inducer anhydrotetracycline (aTc) is added to the culture, it binds to the Tet-repressor that can't bind anymore to the Tet-operator and thus the expression of the autotransporter can be regulated. Although the TetR-system is known to be a tight promoter system there is always a certain background expression with most promoters. If the protein expression of the autotransporter is induced using aTc the autotransporter is transcribed and translated. Due to the bacterial signal peptide, the protein is secreted into the bacterial periplasm (the space between the two bacterial membranes of gram-negative bacteria such as E. coli). When present in the bacteria periplasm the autotransporter diffused to the outer membrane and inserts into the membrane. After the integration into the outer membrane, the protein cargo is transported through the beta-barrel of the autotransporter and is presented on the bacterial surface. We are sure that this BioBrick will be a valuable contribution to the Parts Registry as it allows future teams to display small protein domains on the surface of gram-negative bacteria, such as E. coli.

References

  1. Rapoport, T. A. (2007). Protein translocation across the eukaryotic endoplasmic reticulum and bacterial plasma membranes. Nature, 450(7170), 663-669.
  2. Taken from Alberts, B., Bray, D., Hopkin, K., Johnson, A., Lewis, J., Raff, M., ... & Walter, P. (2010). Essential cell biology. Garland Science.
  3. Walter, P., Ibrahimi, I., & Blobel, G. U. N. T. E. R. (1981). Translocation of proteins across the endoplasmic reticulum. I. Signal recognition protein (SRP) binds to in-vitro-assembled polysomes synthesizing secretory protein. The Journal of Cell Biology, 91(2), 545-550.
  4. Keenan, Robert J., et al. "The signal recognition particle." Annual review of biochemistry 70.1 (2001): 755-775.
  5. Kozak, M. (1989). The scanning model for translation: an update. The Journal of cell biology, 108(2), 229-241.
  6. Kozak, M. (1987). An analysis of 5'-noncoding sequences from 699 vertebrate messenger RNAs. Nucleic acids research, 15(20), 8125-8148.
  7. Petersen, T. N., Brunak, S., von Heijne, G., & Nielsen, H. (2011). SignalP 4.0: discriminating signal peptides from transmembrane regions. Nature methods, 8(10), 785-786.
  8. Sonnhammer, E. L., Von Heijne, G., & Krogh, A. (1998, July). A hidden Markov model for predicting transmembrane helices in protein sequences. In Ismb (Vol. 6, pp. 175-182).
  9. Binder, U., Matschiner, G., Theobald, I., & Skerra, A. (2010). High-throughput sorting of an Anticalin library via EspP-mediated functional display on the Escherichia coli cell surface. Journal of molecular biology, 400(4), 783-802.
  10. Binder, U., Matschiner, G., Theobald, I., & Skerra, A. (2010). High-throughput sorting of an Anticalin library via EspP-mediated functional display on the Escherichia coli cell surface. Journal of molecular biology, 400(4), 783-802.
  11. Ghrayeb, J., Kimura, H., Takahara, M., Hsiung, H., Masui, Y., & Inouye, M. (1984). Secretion cloning vectors in Escherichia coli. The EMBO journal, 3(10), 2437.
  12. Costa, J., Grabenhorst, E., Nimtz, M., & Conradt, H. S. (1997). Stable expression of the Golgi form and secretory variants of human fucosyltransferase III from BHK-21 cells Purification and characterization of an engineered truncated form from the culture medium. Journal of Biological Chemistry, 272(17), 11613-11621.
  13. Barnard, T. J., Dautin, N., Lukacik, P., Bernstein, H. D., & Buchanan, S. K. (2007). Autotransporter structure reveals intra-barrel cleavage followed by conformational changes. Nature structural & molecular biology, 14(12), 1214-1220.
  14. Skillman, K. M., Barnard, T. J., Peterson, J. H., Ghirlando, R., & Bernstein, H. D. (2005). Efficient secretion of a folded protein domain by a monomeric bacterial autotransporter. Molecular microbiology, 58(4), 945-958.

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LMU & TUM Munich

Technische Universität MünchenLudwig-Maximilians-Universität München

United team from Munich's universities

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Address

iGEM Team TU-Munich
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