RedStar2 expression cassette (BBa_K2983077) in YL-pOdd1
This part is a RedStar2 (BBa_K2983060) expression cassette under the control of pTef1e promoter (BBa_K2983052) and Lip2 terminator (BBa_K2983055) inserted by Golden Gate with BsaI in YL-pOdd1 (BBa_K2983030).
It belongs to a series of 5 similar parts (BBa_K2983174, BBa_K2983175, BBa_K2983176, BBa_K2983177 and BBa_K2983178) that differ one from the other with respect to the pTef1 promoter that drives the expression of the reporter gene RedStar2 (BBa_K2983060).
Usage and Biology
In the context of iGEM 2019 competition, we developed a metabolic engineering projet for the production of medically-relevant Conjugated Linolenic Acids (CLnAs) and used as a chassis the oleaginous yeast Yarrowia lipolytica, an organism whose metabolism is naturally poised for lipid production. For the expression of our enzymes, we choose the pTef1 promoter, a constitutive promoter native for Y. lipolytica. It is a strong promoter that controls the expression of the translation elongation factor-1 alpha , a protein that is one of the most expressed in most cells (between 3-10% of the soluble proteins ).
Our bibliographic research led us to designing and characterisation of several versions of the pTef1 promoter (Figure 1 and Table 1).
We started our research from iGEM’s part registry and we quickly found in the database the pTef1 promoter (BBa_K2117000), that we’ll refer to as pTef1a.
This promoter has been used to drive the expression of hrGFP (BBa_K2117001) in the composite part BBa_K2117005 which was built by standard 3A assembly which leaves TACTAG (BBa_G0000) as a scar between the promoter and the ATG of the downstream gene. We will refer to BBa_K2117000+scar as pTef1b.
pTef1 (BBa_K2117000) seemed suitable for our project, but had a major disadvantage: the presence of a BsaI site that makes it incompatible with the Type IIS RFC-compatible Loop assembly system that we designed for Y. lipolytica. To circumvent this incompatibility with the RFC standard, we mutated the BsaI site (GGTCTC) to GGTCTg and thus created a new compatible part,BBa_K2983050, that we’ll refer to as pTef1c.
A quick sequence analysis of BBa_K2117000 revealed several differences compared to wild-type pTef1 promoter (nucleotides 1227374 to 1226969) of Y. lipolytica W29 chromosome C (GenBank Acc. n° CP028450.1). Three of the four mutations were introduced by the iGEM16_DTU-Denmark in order to remove two illegal restriction sites for BioBrick RFC-compatibility (SpeI, PstI). As these sites are accepted in the Type IIS RFC standard, we created a closer to wild-type version of pTef1 promoter, BBa_K2983051, that has also a mutated BsaI site (GGTCTC to GGTCTg) which makes this part compatible with the iGEM Type IIS RFC standard. We will refer to BBa_K2983051 as pTef1d.
Continuing our research, we discovered another version of the pTef1 promoter, which is shorter and Type IIS RFC compatible [3,4]: BBa_K2983052, that we’ll refer to as pTef1e.
Unpublished observations of our PI, Jean-Marc Nicaud, suggest that the presence of a 4 nucleotide sequence CACA just upstream the ATG of the gene may lead to increased gene expression. Thus, we added BBa_K2983053 to the list of pTef1 variants to test. We will refer to BBa_K2983053 as pTef1f.
A sequence comparison of all pTef1 variants is presented in figure 1.
One of the main questions related to the modification of a promoter sequence is related to the impact it may have on its activity. To estimate if the pTef1 promoter activity is impaired by the modifications highlighted in Figure 1, we used a fluorescent reporter gene.
For this, we decided to use RedStar2 (BBa_K2983060), as it is the “brightest and most yeast-optimized version of the red fluorescent protein” .
We placed RedStar2 under the control of a pTef1 promoter variant and of the Lip2 terminator (BBa_K2983055). The resulting transcriptional units (BBa_K2983075, BBa_K2983076, BBa_K2983077 and BBa_K2983078) were assembled into our YL-pOdd1 plasmid (BBa_K2983030) which is part of our Loop assembly system dedicated to our chassis, the oleaginous yeast Y. lipolytica. Thus, we generated four RedStar2 expression plasmids (BBa_K2983175, BBa_K2983176, BBa_K2983177 and BBa_K2983178) able to integrate upon transformation, into a Y. lipolytica Po1d strain.
To be able to make comparisons with the expression driven by the pTef1 variant already in the registry (pTef1a, BBa_K2117000), the BBa_K2983175 was subject to site directed mutagenesis to restore the BsaI site and thus generate BBa_K2983174.
All these parts are summarized in Table 1.
|Table 1. Parts used for fluorescence measurements.|
|Promoter labels||Promoter’s part numbers||RedStar2 expression cassettes’ part numbers||Y. lipolytica genome integration cassettes' part numbers|
For pTef1 promoter characterization we decided to use the auxotrophic wild-type Y. lipolytica strain JMY195 , but also JMY2033 . JMY195 is a Po1d strain, thus, by the means of the Zeta sequences , the Y. lipolytica genome integration cassettes (table 1) will be inserted randomly. JMY2033 is a derivative of JMY195 that contains a zeta docking platform at the ura3-302 locus. In this strain, the insertion is not random, but site specific which limits the risks of multiple insertion of plasmidic constructions in the genome.
These two Y. lipolytica strains were transformed with the NotI digested RedStar2 expression plasmids (BBa_K2983174, BBa_K2983175, BBa_K2983176, BBa_K2983177 and BBa_K2983178). As a negative control, we also transformed them with the NotI digested empty YL-pOdd1 vector (BBa_K2983030). As positive control we used the JMY7621 stain  which contains a single genome copy of a RedStar2 expression cassette.
For fluorescence measurements, yeast cells were first grown overnight in rich YPD medium then diluted by 100x in YNB-glucose medium (containing 1.7 g/L yeast nitrogen base with amino acids and ammonium sulfate, 1.5 g/L NH4Cl, 50 mM KH2PO4-Na2HPO4 buffer pH 6.8, 10 g/L glucose and 0.1 g/L leucine) in an opaque wall 96-well polystyrene microplate, the COSTAR 96 (Corning). The plate was incubated at 28°C at 200 rpm and the fluorescence (λexcitation 558 nm and λemission 586 nm) and OD600nm were measured every 15 min during 300 cycles in a SynergyMx (BioTek) plate reader.
To compare the expression between each promoter, we rely on specific fluorescence . We measure the turbidity of the culture at 600 nm and the fluorescence of RedStar2, and determine the mean rate of fluorescence/OD600nm (SFU/h) increase during the exponential growth phase. This method allows quantifying RedStar2 expression in a manner independent of the length of the lag phase.
Using the calibration curves presented in Figures 2 and 3 (and as an excel file too), we converted the arbitrary units into Molecules of Equivalent Resorufin (MEResorufin) / particle (Figure 6).
Also, using the calibration curves presented in Figures 2 and 4 (and as an excel file too), we converted the arbitrary units into Molecules of Equivalent Rhodamine B (MERhB) / particle (Figure 7).
The results of the different pTef1 promoter strength quantifications are presented in Figures 5, 6 and 7 using different units of measure.
For nearly each construct, we obtained and analysed twice at least 3 clones (and up to 32), the majority of each displaying comparable specific fluorescence values similar to the value obtained for the positive control. However, a minority of clones were constantly displaying twice more SFU/h suggesting they have integrated 2 copies of the RedStar2 expression cassette. Indeed, the difficulty in using insertion of plasmid construction in the genomic approaches is to estimate and control the insertion site and the number of copies inserted into the genome. In the auxotrophic wild-type Y. lipolytica strain JMY195, our RedStar2 expression cassettes integrate randomly and the protein expression may vary depending on the insertion site. In the JMY2033 strain, the insertion occurs mainly at the zeta docking platform at the ura3-302 locus.
As can be easily observed from the results presented in Figures 5, 6 and 7, the different modifications of the pTef1 promoter sequence highlighted in Figure 1 do not have a drastic impact on its activity. The specific fluorescence values are similar between the different variants of pTef1 in both Y. lipolytica strains and independent of copy number / genome. To confirm these observations, we performed a two-tailed student test with an error threshold of 5% in order to compare the specific fluorescence averages in each strain and each construct. No statistically significant difference was observed between the different constructs in both strains and at both copy number / genome.
Similar observations were obtained when using hrGFP as a reporter instead of RedStar2. These results are presented in detail on the BBa_K2117001 and BBa_K2117005 parts’ Main Pages on the iGEM Registry.
In conclusion, we have successfully built 4 versions of the pTef1 promoter: pTef1c (BBa_K2983050), pTef1d (BBa_K2983051), pTef1e (BBa_K2983052) and pTef1f (BBa_K2983053) which are able to drive the expression of a reporter gene in the oleaginous yeast Yarrowia lipolytica at an equivalent strength as the part already present in the iGEM Registry, pTef1a (BBa_K2117000). Thus, we have made an improvement of the (BBa_K2117000), a version of pTef1 promoter not compatible with the Type IIS RFC.
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 Cavallius J, Zoll W, Chakraburtty K, Merrick WC. Characterization of yeast EF-1 alpha: non-conservation of post-translational modifications. Biochim Biophys Acta (1993) 1163, 75-80.
 Celińska E, Ledesma-Amaro R, Larroude M, Rossignol T, Pauthenier C, Nicaud JM. Golden Gate Assembly system dedicated to complex pathway manipulation in Yarrowia lipolytica. Microb Biotechnol (2017) 10, 450-455.
 Larroude M, Park YK, Soudier P, Kubiak M, Nicaud JM, Rossignol T. A modular Golden Gate toolkit for Yarrowia lipolytica synthetic biology. Microb Biotechnol (2019) 12, 1249– 1259.
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Sequence and Features
- 10Illegal SpeI site found at 1727
Illegal PstI site found at 1692
- 12Illegal NheI site found at 2705
Illegal SpeI site found at 1727
Illegal PstI site found at 1692
- 21Illegal BamHI site found at 304
Illegal XhoI site found at 1281
Illegal XhoI site found at 1314
- 23Illegal SpeI site found at 1727
Illegal PstI site found at 1692
- 25Illegal SpeI site found at 1727
Illegal PstI site found at 1692
Illegal NgoMIV site found at 1126
Illegal AgeI site found at 1023
- 1000Illegal SapI.rc site found at 2713
Illegal SapI site found at 1520