Summary
Here we describe a set of tools to facilitate the use of maltose and the MAL32 promoter for regulated gene expression in yeast, alone or in combination with the GAL1 promoter. Using fluorescent protein reporters we find that under non-inducing conditions the MAL32 promoter exhibits a low basal level of expression, similar to the GAL1 promoter, and that both promoters can be induced independently of each other using the respective sugars, maltose and galactose. While their repression upon glucose addition is immediate and complete, we found that the MAL32 and GAL1 promoter each exhibit distinct induction kinetics. A set of plasmids is available to facilitate the application of the MAL32 promoter for chromosomal modifications using PCR targeting and for plasmid based gene expression.
Introduction
In yeast, promoters that can be regulated – induced or repressed – as a function of conditions or via the addition of compounds have been established as powerful tools for research or biotechnological purposes. Several carbon source dependent promoters (Weinhandl et al. 2014) exhibit a high level of dependence on the composition of the growth medium, for example the sugar content. In particular, the GAL1 promoter (Finley et al. 2002) is strongly influenced by the presence of galactose (inducing) or glucose (repressing) in the medium. Induction of the promoter upon addition of galactose to cells grown on raffinose is fast and can be rapidly halted by the subsequent addition of glucose. This feature of the GAL1 promoter, induction and repression simply based on the addition of compounds, is relatively unique. Other regulatable promoters, such as the heterologous tet-promoter, can be regulated only in one direction, e.g. either induced or repressed upon the addition of a compound (Dingermann et al. 1992; Gossen and Bujard 1992). In order to reverse the regulation the stimulus needs to be removed, for example, by washing the cells with fresh medium, which is much less convenient. Thus, the GAL1 promoter (subsequently called GAL1pr) is the promoter of choice whenever short expression pulses are needed to study a specific process, such as when performing a functional analysis of cell cycle regulation. However, for a number of applications it would be useful to have an additional promoter that can be regulated in a similar manner.
The promoters of the maltose inducible and glucose repressible MAL genes seemed to be promising candidates (Weinhandl et al. 2014). For example the MAL62 promoter can be strongly induced by maltose comparable to the GAL1pr, but under non-inducing or repressing conditions the background expression from the MAL62 promoter was much higher compared to the GAL1pr (Levine, Tanouye and Michels 1992; Finley et al. 2002) which decreases its usability. Therefore we investigated the regulation of other maltose inducible and glucose repressible MAL-promoters in direct comparison with GAL1pr. Depending on the yeast strain, the fermentation of maltose is governed by up to five unlinked but similar loci, each consisting of 3 genes (Barnett 1976; Carlson 1987). Each locus contains an activator gene, a maltose permease and a maltase. The genes in the different loci are termed MALxy, and the nomenclature is such that the first digit denotes the locus (1, 2, 3, 4, or 6) whereas the 2nd digit denotes one of the three genes: MALx1 for maltose permease, MALx2 for maltase and MALx3 for the activator gene (Fig. 1) (Weinhandl et al. 2014). Regulated gene expression as a function of the addition of maltose has been well studied and involves the induction of the maltose permease and the maltase encoding genes from a single bidirectional promoter present in the intergenic region of these two genes (Needleman et al. 1984; Bell et al. 1995). The MALx3 gene upstream of MALx1 codes for a transcriptional activator, that regulates the expression of the bi-directional promoter (Chang et al. 1988).It is important to note that different yeast laboratory strains contain different numbers of MAL loci, but often none are functional for growth on maltose, rendering these strains unable to use maltose as a carbon source.Here we investigate the regulation of maltase and maltose permease gene promoters in direct comparison with GAL1pr. We then focus on the MAL32 promoter (subsequently called MAL32pr) and we outline how this promoter can be used, alone and in combination with GAL1pr.
Results and Discussion
We used the S288c derived strain ESM356-1 (Knop et al. 2005), which is a spore from the diploid strain FY1679 (Winston, Dollard and Ricupero-Hovasse 1995; Wach et al. 1997). S288c strains contain two MAL loci, MAL1 and MAL3, both containing non-functional activator genes (mal13 and mal33). We decided to investigate all promoters of these loci for regulation by maltose and other carbon sources. We constructed reporter strains expressing sfGFP, a bright and fast maturing GFP variant (Pédelacq et al. 2006), under the control of all promoters from the two MAL-loci and compared it to a GAL1 promoter reporter strain. We tested for expression of the reporter using growth on agar plates and colony pinning using a pinning robot. Promoter activity was quantified in n ≥ 20 colonies per strain using whole colony fluorescence measurements with the help of a fluorescent plate reader. In the presence of the MAL63 activator (on plasmid pRS415- MAL63 containing a functional MAL activator gene originating from the yeast strain RM11), specific induction of the promoter regulating the maltase and the maltose permease genes was observed (Fig. 2A, B). The achieved expression levels were in the range of 15 – 45% of those observed for GAL1pr. No induction of the activator (MAL13pr and MAL33pr) was observed. We found that MAL11pr and MAL12pr showed the highest expression levels when induced by maltose but also higher basal levels compared to MAL31pr and MAL32pr when repressed by glucose or uninduced on galactose/ raffinose. MAL31pr and MAL32pr both showed low expression levels when repressed or uninduced, however, MAL32pr exhibited two fold higher levels than MAL31pr when induced by maltose. Based on these results we decided to use MAL32p for further work.
Next, we tested for repression of the promoter using cells grown in liquid medium and a plasmid containing GFP fusions to MAL32pr or GAL1pr. This revealed comparable expression levels of both promoters on the respective carbon source (maltose or galactose) and full repression of both promoters in the presence of glucose (Fig. 3). We also tested a truncated MAL31pr variant (MAL31pr-short (Levine, Tanouye and Michels 1992)) and found properties comparable to the full length MAL32pr.
In contrast to these results obtained in liquid medium, we observed that the presence of glucose in maltose or galactose containing agar plates did not repress expression of the MAL32pr and GAL1pr constructs (data not shown). We attribute this to the fact that cell colonies on agar plates are 3D objects that receive their nutrients from the bottom. Therefore, we speculate that the cells at the top of the colony, where the fluorescence is measured using the plate reader, receive only maltose or galactose, because glucose, which is the preferred carbon source, is consumed completely by the cells underneath.
To explore the possibility to use both promoters simultaneously in experiments where orthogonal regulation of two genes is needed, we used cells harboring MAL32pr and GAL1pr fusions simultaneously, using liquid growth conditions and full induction with the corresponding carbon sources (> 15 hours of growth under inducing conditions). On maltose only the MAL32pr reporter was expressed, and on galactose only the GAL1pr reporter was expressed. In the simultaneous presence of maltose and galactose both reporter were expressed to levels reaching approximately 70% of the ones observed for ‘single sugar’ induction (Fig. 4). We analyzed this culture by flow cytometry and found that it consisted of a homogeneous population of cells where each cell expresses both reporters simultaneously (data not shown).
In a last series of experiments we used flow cytometry and liquid growth conditions to compare the induction and repression dynamics of both promoters. We integrated the GAL1pr or the MAL32pr upstream of a strain expressing NUP2-sfGFP. We choose NUP2 as a test case since we knew from unpublished work that overexpression or deletion does not compromise the fitness of the cell (data not shown). For GAL1pr the entire cell population showed homogeneous induction of the reporter upon galactose addition. The situation was different for MAL32pr. Here, induction did not occur uniformly in all cells simultaneously. Instead, up to 5 hours after the addition of maltose the populations still contained cells that had not (yet) induced the reporter. Only after prolonged growth in the presence of maltose for > 15 hours did all cells exhibited uniform expression (Fig.5A). Therefore MAL32pr cannot be used for short-term expression experiments where homogeneously induced cell populations are needed.
Glucose addition to cells on maltose or galactose medium respectively led to rapid shut down of both promoters and the cellular fluorescence decayed exponentially, indicating an immediate halt of the reporter expression and subsequent dilution of the reporter in the dividing cell population (Fig. 5B). No difference in the behavior between the GAL1 and MAL32 promoter was observed.
Taken together, our experiments show that MAL32pr is strongly induced by maltose in the presence of a functional MAL-activator and background expression from it under repressing or non-inducing conditions is minimal and comparable to GAL1pr. The MAL32pr can be used in combination with GAL1pr, provided that (i) a functional MAL- activator gene is present (which can be integrated into the genome or contained on a plasmid or PCR tagging cassette), (ii) induction of the MAL32pr is not time-critical, since complete induction in every cell in a culture takes up to 15 hours. While this latter property prevents the MAL32 promoter for applications where short induction pulses are needed, it still works for experiments where longer induction periods can be accommodated (e.g. over night growth).
The diversity of MAL genes and the number of MAL-loci in different S. cerevisiae strains and also in other yeast species has been explored to some extent (e.g. see (Vidgren, Ruohonen and Londesborough 2005; Brown, Murray and Verstrepen 2010). However for practical reasons, e.g. when planning to use the MAL32pr for experimental work, it is only required to know whether a particular yeast strain contains a functional MAL-activator gene, whether it is able to grow on maltose, and whether the MAL32pr is induced. To obtain corresponding information for any yeast strain, the plasmids pMaM440 (containing a MAL32pr-sfGFP) and pMaM454 (containing a MAL32pr-sfGFP and the MAL63 activator) can be used. In Table 1 we demonstrate this for a number of frequently used laboratory strains of diverse origin. The obtained results emphasize that laboratory strains indeed differ with respect to maltose growth and induction.
To facilitate the use of the MAL32pr we have also constructed some tools. For N-terminal tagging of genes, tagging cassettes harboring a selection marker (kanMX, hphNT1 or natNT2) and the MAL32pr can be used together with S1-/S4-primers (Janke et al. 2004) (Fig. 6B (ii), pMaM446/448/447). For induction of the promoter a yeast strain containing a functional MAL activator is needed (see Table 1). Since BY4741 is widely used as a laboratory strain, we have constructed a BY4741 strain with a marker free integration of the MAL63 activator (YMaM991). For strains without a functional MAL activator, tagging with the MAL32pr and integration of MAL63 can be done simultaneously together with a selection marker (Fig. 6B (i), pMaM458/456/460). For marker free integration into a strain without functional MAL activator a tagging cassette only containing the MAL32pr and MAL63 can be used (Fig. 6B (iii), pMaM462). In this case selection for positive transformants needs to be done on YP + 2 % maltose + Antimycin A (3 mg/L), which enhances the selection of fermentatively growing transformants with a functional MAL activator over non-transformed cells that can only grow by respiration of maltose without MAL63 (Fukuhara 2003)). One has to note that tagging efficiencies are dependent on the cassette features and their homology to the genome. For cassettes including MAL32pr or GAL1pr the tagging efficiency is about 50 %, for cassettes containing MAL32pr plus MAL63 the efficiency goes down to 5 - 10 %. In addition to the tagging cassettes, centromeric plasmids based on pRS415 (Sikorski and Hieter 1989) harboring the MAL32pr with and without MAL63 are available (Fig. 6A (ii)/(i), pMaM453/449).
Materials and Methods
Yeast strains, plasmids and growth conditions
Yeast cells were grown according to standard methods (Sherman, 2002). Cultures were grown at 30°C to logarithmic phase (OD600 between 0.5 and 1.0 corresponding to 0.5−1=107 cells/ml) unless otherwise stated. See Table 2 for a list of strains. For construction of yeast strains, standard methods were used. For chromosomal fluorescent protein reporter fusions, a one-step PCR targeting procedure was used to chromosomally introduce the fluorescent protein 3’- to the selected promoter region, while fully maintaining the integrity of the target locus, according to the method described in Huber et al. (2014) (Huber et al. 2014). For plasmids (Table 3), standard cloning procedures were used (Greene and Sambrook 2012). A list of primers used in this study can be found in Table 4.
Fluorescence measurements by plate reader and flow cytometry
To measure the fluorescence of colonies expressing the fluorescent protein fusions to different regulatory expression sequences, yeast colonies were pinned using a RoToR pinning robot from Singer Instruments (UK). For background subtraction of the autofluorescence of the cells we used colonies of a strain that did not express the corresponding fluorescent proteins (cells containing empty plasmids). Fluorescence was measured using a TECAN M1000 pro and appropriate settings for excitation and emission wave-lengths and gain levels for detection sensitivity. For flow cytometry a BD FACS Canto II (BD Bioscience) was used. Cells were grown to logarithmic phase (approx. 5×106 cells/ml) for at least 6 hours on synthetic complete medium containing the indicated sugar (2 % w/v each).
Acknowledgements
We thank Anton Khmelinskii for discussion and comments on the manuscript. Part of the work was funded through the DFG Grant SFB 1036.