Deletion of the MBP1 Gene, Involved in the Cell Cycle, Affects Respiration and Pseudohyphal Differentiation in Saccharomyces cerevisiae.

Mbp1p is a component of MBF (MluI cell cycle box binding factor, Mbp1p-Swi6p) and is well known to regulate the G1-S transition of the cell cycle. However, few studies have provided clues regarding its role in fermentation. This work aimed to recognize the function of the MBP1 gene in ethanol fermentation in a wild-type industrial Saccharomyces cerevisiae strain. MBP1 deletion caused an obvious decrease in the final ethanol concentration under oxygen-limited (without agitation), but not under aerobic, conditions (130 rpm). Furthermore, the mbp1Δ strain showed 84% and 35% decreases in respiration intensity under aerobic and oxygen-limited conditions, respectively. These findings indicate that MBP1 plays an important role in responding to variations in oxygen content and is involved in the regulation of respiration and fermentation. Unexpectedly, mbp1Δ also showed pseudohyphal growth, in which cells elongated and remained connected in a multicellular arrangement on yeast extract-peptone-dextrose (YPD) plates. In addition, mbp1Δ showed an increase in cell volume, associated with a decrease in the fraction of budded cells. These results provide more detailed information about the function of MBP1 and suggest some clues to efficiently improve ethanol production by industrially engineered yeast strains. IMPORTANCE Saccharomyces cerevisiae is an especially favorable organism used for ethanol production. However, inhibitors and high osmolarity conferred by fermentation broth, and high concentrations of ethanol as fermentation runs to completion, affect cell growth and ethanol production. Therefore, yeast strains with high performance, such as rapid growth, high tolerance, and high ethanol productivity, are highly desirable. Great efforts have been made to improve their performance by evolutionary engineering, and industrial strains may be a better start than laboratory ones for industrial-scale ethanol production. The significance of our research is uncovering the function of MBP1 in ethanol fermentation in a wild-type industrial S. cerevisiae strain, which may provide clues to engineer better-performance yeast in producing ethanol. Furthermore, the results that lacking MBP1 caused pseudohyphal growth on YPD plates could shed light on the development of xylose-fermenting S. cerevisiae, as using xylose as the sole carbon source also caused pseudohyphal growth.

China produces approximately 3.8 million tons of sugarcane molasses annually as a byproduct of sugar processing. This molasses contains approximately 45 to 50% (wt/wt) fermentable sugars that can be converted to ethanol by fermentation. Saccharomyces cerevisiae is widely used for ethanol production from molasses (1, 2) because of its robustness under industrial fermentation conditions (3). However, numerous inhibitors in molasses and the high osmolarity conferred by sugars still greatly affect yeast cell growth and ethanol production (4), and high concentrations of ethanol during the late stage of fermentation are also harmful to cells (5). Therefore, yeast strains with high performance, such as high tolerance, rapid growth, which can shorten the fermentation time, and high ethanol productivity, are highly desirable for industrial-scale ethanol production.

Nitrogen and other nutrient levels early in fermentation are factors that are extremely important in determining yeast cell growth and a successful fermentation outcome (6–8). The nutrients of which a cell can be starved include carbon and nitrogen (9). With sufficient nutrients, wild-type S. cerevisiae cannot form pseudohyphae, but when cells are starved for nitrogen (10, 11), carbon (12), and especially fermentable sugars (13), they switch from a yeast form to a filamentous pseudohyphal form (11) and invade into agar (13). Filamentous/invasive growth allows sessile yeast cells to forage for scarce nutritional resources (11, 12).

We previously isolated two industrial strains, MF01 and MC15, from 1-year-old sugar mill waste in Nanning, China. MF01 was found to possess better fermentative capabilities and has been used for industrial-scale ethanol production with an annual output of 50,000 tons but showed slower growth than MC15 (14). Comparative genomics between these strains showed that several candidate regulatory genes are potentially associated with ethanol fermentation (14). Among these genes, this study focused on MBP1, a gene involved in the cell cycle.

Although MBP1 is well known for its role in the cell cycle, little is known about its function in ethanol fermentation, especially in industrial strains. In this study, we deleted MBP1 in the MF01 strain and focused on the phenotypes and ethanol productivity of the resulting mbp1Δ strain. We found that MBP1 deletion decreased the fermentation ability and unexpectedly caused pseudohyphal differentiation and respiration defects. We report here pseudohyphal differentiation of S. cerevisiae cultured in rich medium (yeast extract-peptone-dextrose; YPD) to our knowledge. We further present several hypotheses that might help to understand the mechanisms underlying our results.

RESULTS

Deletion of MBP1 decreases fermentability in molasses medium.

We obtained a diploid mutant lacking MBP1 by the method described in Materials and Methods. To examine whether the lack of MBP1 alters the fermentation ability of S. cerevisiae, we tested the ability of yeast to ferment sucrose and sugarcane molasses. Upon fermentation with sucrose as the sole carbon source, the total residual sugar in the fermentation broth of the mutant (mbp1Δ) and the wild-type (WT) strains decreased from 25.86% ± 0.33% and 26.35% ± 0.76% to 0.11% ± 0.00% and 0.11% ± 0.00%, respectively, and the utilization rate of sucrose by both strains was 99.6% (Fig. 1A). The maximum ethanol concentration obtained with mbp1Δ using sucrose was 13.65% ± 0.03%, which was slightly lower than that of the WT, 14.47% ± 0.05% (Fig. 1B). However, when molasses was used as the sole carbon source, the total sugar with mbp1Δ and WT decreased from 19.87% ± 0.14% and 19.55 ± 0.26% at the beginning of feeding (0 h) to 3.88% ± 0.15% and 3.37% ± 0.07% at 64 h, respectively, and the utilization rate of molasses by mbp1Δ was 80.5%, lower than that by the WT (82.8%) (Fig. 1A). As shown in Fig. 1B, the maximum ethanol concentration with mbp1Δ was 13.77% ± 0.23%, which was slightly lower than that of WT (14.16% ± 0%).

FIG 1

Fermentability analysis. For the determination of total residual sugar (A) and ethanol production with different carbon sources (B), samples were collected as described in Materials and Methods. (A) One part of 6 M HCl was added to 10 parts of the fermentation broth and boiled for 15 min. After cooling quickly to room temperature, 1.2 parts of 20% NaOH was added. Total sugar was estimated by dinitrosalicylic acid method (62). Data shown represent mean ± standard deviation (SD) of data from three replicate fermentations. (B) The concentration of ethanol was analyzed using an Agilent gas chromatograph, model 6890N (Agilent Technologies Inc., USA) with a flame ionization detector. Data shown represent mean ± SD of data from three replicate fermentations. (C) For the determination of ethanol production under different aeration conditions, cells were grown and fed with molasses medium as described in Materials and Methods. Equivalents of the cells were then cultured with shaking (130 rpm) and without shaking, respectively. Samples were taken at 36, 47, 59, 64, and 72 h after feeding. Data shown represent mean ± SD of three replicate fermentations.

MBP1 deletion causes respiration defects and obviously decreases ethanol production under oxygen-limited conditions.

Since a lack of MBP1 might cause decreased adaptability in molasses, we paid more attention to fermentation in molasses medium under different aeration conditions. When molasses medium was cultured with shaking (130 rpm), there was little difference in the ethanol concentration between the mutant and parent strains. In contrast, when the medium was cultured without shaking, the ethanol production by the mutant was significantly lower than that by the parent strain, with 2.9%, 4.8%, 3.5%, 9.3%, and 4.0% decreased, respectively, at each measurement time (36, 47, 59, 64, and 71 h). The ethanol concentration of mbp1Δ was significantly higher under aerobic conditions (130 rpm) than under oxygen-limited conditions (0 rpm). However, ethanol production by the parent strain showed a limited difference between the two conditions, although there was slight enhancement under aerobic conditions (except at 64 h) (Fig. 1C).

Considering this surprising difference under different aeration conditions, we checked the respiratory intensity of the strain. The mbp1Δ strain showed obvious defects in respiratory intensity displayed by the reduction of 2,3,5-triphenyltetrazolium chloride (TTC), which was exceptionally apparent under aerobic conditions; this was 16.79% and 64.52% compared to that of the parent strain under aerobic conditions and with insufficient oxygen supply, respectively. Interestingly, under oxygen-limited conditions, the mutant showed 1.8 times the respiratory intensity under aerobic conditions, whereas this was 47.3% for the WT under aerobic conditions (Table 1).

TABLE 1

Respiration intensity

Strain	Rotation speed
	130 rpmb	0 rpmc,d
WTe	1.31 ± 0.49	0.62 ± 0.04
mbp1Δf	0.22 ± 0.02	0.40 ± 0.02

Respiration intensity was presented as OD490. The data represent the TTC absorbance after 4 h incubation.

Statistical comparison between WT and mbp1Δ: ns, P = 0.188508.

Statistical comparison between WT and mbp1Δ: *, P = 0.026926.

Although yeast cells produce a lot of carbon dioxide, cultivation without shaking does not guarantee that the medium was totally anaerobic (65). Thus, we indicated this cultivation as oxygen-limited condition.

Statistical comparison for WT between 130 rpm and 0 rpm: ns, P = 0.314887.

Statistical comparison for mbp1Δ between 130 rpm and 0 rpm: ***, P = 0.000243.

Deletion of MBP1 alters colony morphology and causes invasive growth.

Unexpectedly, the deletion of MBP1 resulted in surface invaginations and roughness at the periphery of the colony on the YPD plate, in contrast to normal smooth, lustrous colony surfaces (Fig. 2A, panels a and b). Microscopic examination revealed that mbp1Δ cells became long and grew as chains of cells in a filament, whereas the WT cells were separated into ellipsoidal yeast cells (Fig. 2A, panels c and d). Therefore, we further examined their growth in liquid medium. Microscopic analysis showed that mbp1Δ cells were elongated (Fig. 2A, panel f). The forward angle scattering (FSC) of WT and mbp1Δ was 988,262 ± 100,525 and 1,177,935 ± 83,402, respectively (Fig. 2B), showing an increase in mutant cell volume.

FIG 2

Morphology and size analysis. (A) Wild-type (a and c) and mbp1Δ (b and d) cells were incubated for 3 to 5 days on YPD plates and visualized on petri plates (a and b) and then picked from the edge of colony and viewed by microscopy (c and d). Wild-type (e) and mbp1Δ (f) cells cultured in liquid medium were also checked by microscopy. (B) Synchronized cells were grown to exponential growth, diluted to 1 × 106 cells/ml, and analyzed (10,000 events collected per sample) by FSC using an Accuri C6 flow cytometer (Becton, Dickinson, USA) at the medium flow rate. Cell size was estimated by forward scatter area (FSC-A). Each FSC was determined from an average of data from duplicate experiments.

Deletion or overexpression of MBP1 caused a slow growth.

Two different vectors (pK and pKY) were constructed and introduced into the WT and mbp1Δ strains. Cells overexpressing MBP1 (transformed pKY; Fig. 3B, panels d and f) were larger than the controls (transformed with pK; Fig. 3B, panels c and e), and this manifested as aggregation. Furthermore, at 36 h, the optical density at 600 nm (OD600) value of the mbp1Δ strain was 94.0% that of WT, whereas those of WT/pKY and mbp1Δ/pKY were 82.2% and 86.5% those of WT/pK and mbp1Δ/pK, respectively (Fig. 3A). In the platform growth period, the absorbance (OD600) of WT/pKY was lower than that of WT/pK or WT, and the growth curves of both strains were close to parallel; mbp1Δ/pKY and mbp1Δ/pK followed the same patterns. Since overexpression and deletion cells were bigger than their respective controls, their cell density was even lower than that of the controls, based on comparisons with the OD600 data. The similar morphology (Fig. 3B, panels d and f) and growth rate (Fig. 3A) between WT/pKY and mbp1Δ/pKY cells might result from the overexpression of MBP1. To confirm this hypothesis, quantitative reverse transcription (qRT)-PCR analysis was performed. The relative expression levels of MBP1 were 32 and 94 in mbp1Δ/pKY and WT/pKY, respectively (Fig. 3C), corresponding to their OD600 value at 18 h (Fig. 3A), which was consistent with our hypotheses. Taken together, we concluded that both the overexpression and deletion of MBP1 caused slow growth (Fig. 3A) and an increase in cell volume (Fig. 2B; Fig. 3B).

FIG 3

Deletion or overexpression of MBP1 causes slow growth and altered cell morphology. (A) After cells were synchronized, the number of cells in each sample was determined by microscopy and equivalent of cells were harvested by centrifugation, resuspended in sterile water, and shifted to YPD containing 2% galactose, at a final concentration of 1 × 106 cells/ml. Samples were taken at 6-h intervals and absorbance was measured at 600 nm. WT/pK and mbp1Δ/pK harbored pYes/kanMX, and WT/pKY and mbp1Δ/pKY harbored pYes/kanMX/mbp1. In these vectors, MBP1 expression was controlled by GAL1 promoter. Data shown represent mean ± SD of data from three independent biological replicates. (B) Synchronized cells were incubated for 30 h in YPD plus 2% galactose and determined by microscopy. a: WT, b: mbp1Δ, c: mbp1Δ/pK, d: mbp1Δ/pKY, e: WT/pK, f: WT/pKY. Scale bars, 20 μm. (C) Synchronized cells were harvested after 18 h of cultivation in YPD plus galactose. Gene transcript levels were determined by the 2−ΔΔCt method (63) using PDA1 (Table 2) as a reference gene for normalizing MBP1 expression levels and WT as a reference sample.

TABLE 2

Primers used in this study

Primer use	Primer name	Primer sequence (5′–3′)	Note
MBP1 gene knockout box amplification primers
	R	GTGCTTAACATTCCGAGACACAACGTAAATCCCAGAAACACAAGC	Upstream of MBP1
		GCAGGTCGACAACCCTTAAT	Upstream of Loxp
	F	CAGTATATGGATACATGTAAAGTTCCTCTATTTATGTATATTTTA	Downstream of MBP1
		GCCACTAGTGGATCTGATATCACC	Downstream of Loxp
MAT locus verification primers
MFa or MFα verification	MATF	AGTCACATCAAGATCGTTTATGG	Downstream of MATF
MFa verification	MAT a	ACTCCACTTCAAGTAAGAGTTTG	Within MATa
MFα verification	MATα	GCACGGAATATGGGACTACTTCG	Within MATα
KanMX gene integrity verification primers
mbp1Δ::Kanr verification	Ka	CAGCATCCATTAGCCGTTAG	Upstream of MBP1
	Kb	ATTCCGACTCGTCCAACATC	Within KanMX
mbp1Δ::Kanr verification	Kc	AGGTCTAGAGATCTGTTTAGCTTGC	Within KanMX
	Kd	CACAGAAAAAGCACTGCTTACTG	Downstream of MBP1
MBP1 gene integrity verification primers
WT verification	056wa	ATGGAATACCTGCAAGATAC	Upstream of MBP1
	056wb	TGCAATAACACTTGTGGTAG	Within MBP1
WT verification	056wc	GGATCTACGAGGGGAAGCAG	Within MBP1
	056wd	CACTGTCTTGGGTGACGACG	Downstream of MBP1
Overexpressiona
pKY construction	MBP1-F	GGGGTACCGCATGTCTAACCAAATATACTCAGCG	Kpn I
	MBP1-R	ACATGCATGC TCCGATAATGTTCCAAAGGAAGC	Sph I
pK construction	Kan-F	CTAGCTAGCTAGGTCTAGAGATCTGTTTAGCTTG	Nhe I
	Kan-R	GGAATTCCATATGATATTAAGGGTTCTCGAGAGCTC	Nde I
qRT-PCR
MBP1	F	AAAAGCTGGAATACAGGCAAACGG
	R	TGAGCCAATTCCAACCTTTCCAG
PDA1	F	CTGTTGGTCAGGAGGCCATTGC
	R	CCAGAACGGCTTTCACTGAGGC

The protected base is shown as italic, and the restriction enzyme cutting site is underlined.

MBP1 deletion causes growth inhibition in the presence of stress.

To provide more proof that MBP1 contributes to cellular fitness, we determined the strains’ tolerance to ethanol. First, the strains were treated with ethanol at different concentrations for different times. It was found that mbp1Δ showed tolerance weaker than that of the WT after 3 h of treatment with 17% ethanol, as well as with longer treatment with less ethanol (Fig. 4A). Their growth rates were then checked. Both strains showed similar growth without ethanol in the liquid medium. In contrast, the OD600 of mbp1Δ was obviously lower than that of the WT after 40 h of culture with 9% ethanol (Fig. 4B). Taken together, we propose that a lack of MBP1 greatly affects the fermentation rate, especially in the late stage of fermentation, since biomass content governs the fermentation rate (6). To gain more insight into cellular fitness, we determined the content of trehalose and the activity of enzymes involved in tolerance. Consistent with tolerance, after culture with 9% ethanol, the contents of trehalose and the activities of CAT, POD, SOD, and ADH in mbp1Δ were 49%, 80%, 24%, 37%, and 73% lower, respectively, than those in the WT, but no significant difference was observed between the strains without ethanol (Fig. 5). Furthermore, we assessed the sensitivity of yeast cells to cell wall inhibitors and found that mbp1Δ was more susceptible to SDS and Congo red (Fig. 6A). These results indicate that MBP1 plays a role in maintaining cell wall integrity, which helps to optimize the cell survival response to stress and the fermentation ability.

FIG 4

The mutant showed a tolerance weaker than that of the WT. (A) A total of 2 × 106 overnight cells were inoculated into 1 ml YPD with ethanol at different concentrations and cultured for 3, 4, and 5 h, respectively. A total of 2 μl of each treated culture was spotted in rows on YPD plates. After the spots dried, the plates were incubated for 2 to 3 days. The treatment time and strain are indicated at the left of each panel, while the concentrations of ethanol are listed above. (B) A total of 1 × 106 overnight cells were reinoculated into 10 ml YPD and YPD plus 9% ethanol, respectively, for growth. Samples were taken at 8-h intervals. Data shown represent mean ± SD of data from two replicate fermentations.

FIG 5

Content of trehalose and activity of enzymes involved in tolerance. (A to D) Overnight cells were cultured in 50 ml YPD with or without 9% ethanol in the final concentration of 1 × 106 cells/ml and harvested by centrifugation after 48 h cultivation. Data shown represent mean ± SD of data from two or three replications. (E) After 54 h cultivation with or without ethanol, equal weight (38.5 g) of cells in each sample was collected. Trehalose was extracted using 0.5 M trichloroacetic acid and measured by the anthrone method (64). The amount of trehalose was determined using a standard curve of amounts of trehalose plotted against OD620. Data shown represent mean ± SD of data from two replications.

FIG 6

Sensitivity to cell wall inhibitor (A) and budding index (B). (A) Cells were grown in YPD medium to log phase (2 × 107 cells/ml) and serially diluted 10-fold, and 2 μl each of the 10-fold dilutions of cultures for each strain was spotted onto solid medium supplemented with inhibitor and cultured for 2 to 3 days. The strains and dilution times are indicated at the left and the top of the picture, respectively. (B) Synchronized cells were inoculated into 5 ml YPD with the final concentration 2 × 106 cells/ml. Samples were taken at 8-h intervals and the number of budded cells (Nbudded) and total cells (Ntotal) in each sample was determined. Budding index is equal to Nbudded/Ntotal. Data shown represent mean ± SD of data from two replicate fermentations.

DISCUSSION

Clues for industrial strain development.

S. cerevisiae is an industrial strain that is important for bioethanol production. Numerous studies have been conducted to improve the performance of ethanol production (15–18). Most studies have focused on laboratory strains (19, 20), which might contain many naturally occurring mutations during cultivation (21), thus reducing reference value for industrial strains. The merits of industrial yeast have also been reported (22).

This study focused on wild-type industrial strains and uncovered the role of MBP1 in ethanol fermentation. Deletion of MBP1 decreases the utilization rate of molasses. The difference in the utilization rate of molasses might result from the difference in adaptation to a complex environment between the mutant and its parent strain, since molasses medium was more complex than sucrose medium. Furthermore, MBP1 loss decreased the content of trehalose and the activity of enzymes involved in tolerance. Trehalose accumulation is responsible for sustaining cell viability and is highly correlated with ethanol production (6). Our results suggest that MBP1 participates in the regulation of genes involved in trehalose biosynthesis and enzymes related to tolerance. Unexpectedly, mbp1Δ showed filamentous growth on YPD plates, generally caused by the starvation of nitrogen (10, 11) or carbon (12, 13). In addition, filamentous growth was also observed in a recombinant industrial strain using xylose as the sole carbon source (unpublished data). These results could shed light on the development of ethanol- and xylose-fermenting S. cerevisiae with better performance, which is important for developing an economical microbial conversion process of lignocellulosic biomass into bioethanol (23).

Several kinds of MBP1-based approach could potentially be used for the construction of yeast strain with high performance, such as CRISPR-Cas9 and homologous recombination, by which two strains with high performance were obtained via replacement of PHO4 (14) and CDC15 (unpublished data), respectively. Further research could check whether changes in the expression levels of Mbp1p could improve the ethanol productivity in a complex environment, although the overexpression caused a slow growth in medium without stress/inhibitor (Fig. 3A).

Phenotype affected by MBP1 deletion.

To the best of our knowledge, the phenotypic consequence of MBP1 deletion was first described by Bean et al. (24) in a W303 strain background. The mbp1Δ mutant showed a 20% increase in cell volume, associated with a 5% increase in budded cells among haploid yeast during exponential growth (24). However, according to Porter et al. (25), the loss of MBP1 in haploid yeast leads to a decrease in the proportion of budded cells in the first doubling time but an increase during 1.3 to 1.8 doubling times. Herein, the mbp1Δ mutant showed a 19.2% increase in cell volume (Fig. 2A, panels e and f; Fig. 2B), as reported by Bean et al. (24), but a decrease in budding index throughout the test (Fig. 6B), consistent with the report that large cell size impairs cell proliferation (26). MBP1 loss may delay cell division relative to cell growth and cause cells to be arrested in G1 and grow to their maximal size, since cell size is a sensitive indicator of cell cycle progression overall (27). More phenotypic differences have been reported. For example, some studies found that mbp1Δ swi4Δ strains failed to survive (24, 28), whereas another study obtained a swi4Δ mbp1Δ strain (29). Moreover, no apparent growth defects were observed in both swi4Δ mbp1Δ and mbp1Δ haploid strains in a BY4741 strain background (29), but minor growth defects were observed in mbp1Δ/mbp1Δ Candida albicans cells (30). In this study, the lack of MBP1 altered colony morphology (Fig. 2A, panel b) and caused invasive growth (Fig. 2A, panel d). The reasons for these discrepancies related to MBP1 deletion were likely due to different genetic backgrounds. For example, some laboratory strains (S288C and W303) fail to form pseudohyphae, resulting from a naturally occurring mutation in the FL08 gene (21).

Significantly, MBP1 deletion caused a slow growth, and so did the overexpression of MBP1. The slow growth phenotype could not be rescued by the overexpression, which might be attributed to an overdose of MBP1. In addition, previous work has found that high overexpression of MBP1 is lethal (31), unlike our results. The difference in viability of cells after overexpression of MBP1 may also result from the difference in MBP1 dosage or genetic background.

The role of MBP1 in pseudohyphal growth.

To the best of our knowledge, the requirements for pseudohyphal growth were first described in detail based on nitrogen starvation, an a/α diploid form, and BUD genes that regulate the budding pattern (11). However, contradictory results have been observed. For example, both haploid and diploid S. cerevisiae can form pseudohyphae in response to carbon limitations in the presence of sufficient nitrogen (12). Similarly, fermentable sugar depletion also causes invasive growth in haploid yeasts (13). In this study, the homozygous diploid mutant (mbp1Δ) unexpectedly showed invasive pseudohyphal growth on YPD plates (Fig. 2A, panels c and d). The fundamental cellular basis for invasive pseudohyphal growth could be assumed.

The processes involved in the filamentous phase consist of polar budding, cell elongation, incomplete cell separation, and invasive growth (11) and are regulated by multiple pathways (32). Theoretical considerations predicted that MBP1 was possibly associated with a gene that links it to filamentation-regulated genes. Some results support our hypothesis. First, deletion of genes, involved in the cell cycle and regulated by MBF, cause abnormal budding (33). Second, MAPK induces cell elongation by regulating CLN1 (34), a gene essential for pseudohyphal growth (35, 36). In addition, there is some interaction between MBP1 and CLN1 (37). Taken together, it might be possible that MBP1 serves as a transcriptional repressor, repressing the transcription of CLN1.

However, since Mbp1p/MBF regulates many genes involved in the cell cycle (24, 28, 30, 32, 33, 38–40), MBP1 may associate with another gene linked to the filamentous phase, for example, CLN3. CLN3 has an antagonistic effect on pseudohyphal growth (35), and the inhibitory effect might be mediated through MBP1. Support for this hypothesis includes the interaction between them; CLN3 is an activator of MBF (39), and the role of CLN3 in the regulation of cell size and budding is partly dependent on MBF (39). Further evidence for their interaction might come from our results indicating that mbp1Δ showed an increase in cell volume (Fig. 2A, panels e and f; Fig. 2B) and a decrease in the budding index (Fig. 6B).

Cross talk between filamentous growth and cell wall integrity pathway.

Filamentous growth is a behavior more complex and globally regulated than is currently appreciated (32) and is regulated by MAPK pathways both positively and negatively (34). Cross talk among filamentous growth (FG) and other MAPK pathways, such as the pheromone response (32, 41, 42) and the high-osmolarity glycerol (32, 42), have been reported. Our results showed cross talk between FG and the cell wall integrity pathway (CWI) based on invasive growth (Fig. 2A) and sensitivity to cell wall inhibitors (Fig. 6A) in the mbp1Δ mutant. Further evidence is provided by the strong genetic interactions between MBP1 and SSE1 involved in CWI (29).

The effect of MBP1 deletion on respiration.

Although there was little difference in the final ethanol concentration between mbp1Δ and WT under aerobic conditions, a marked difference was observed under the condition of insufficient oxygen supply. Interestingly, the respiratory intensity of the mutant was stronger under oxygen-limited conditions than under aerobic conditions, whereas that of the parent strain was obviously lower. Nevertheless, the respiratory intensity of the mutant strain was lower than that of the parent strain under both conditions. Although the mechanism behind this phenomenon remains unclear, it could be speculated. The ability to grow under aerobic and anoxic conditions is one of the most relevant metabolic features of S. cerevisiae, and cells can obtain energy in both conditions by switching metabolism between respiration and fermentation. The switch between fermentation and mitochondrial respiration is regulated by glucose availability (43). The functionality of mitochondria is dependent on the carbon source (44), and mitochondrial respiration is regulated by SNF1 depending on the concentration of glucose (45, 46). In addition, SNF1 regulates MBF-dependent transcription (47, 48) and cyclin CLB5 (48, 49), which is also regulated by MBF (33). Taken together, we surmise that MBP1 might affect respiration by interacting with SNF1. Further evidence for their interaction is demonstrated by the previous report that SNF1 is involved in invasive growth (13) and affects cell integrity (50), as well as our similar results caused by the MBP1 deletion (Fig. 2A; Fig. 6A). However, MBP1 might affect respiration with other genes linked to mitochondria, since it has been reported that MBP1 regulates the activity of genes involved in mitochondria, such as YDR263C (DIN7) (51, 52) and YMR307W (GAS1) (51).

Conclusion.

MBP1 deletion caused a decrease of tolerance and an obvious decrease in the final ethanol concentration under oxygen-limited conditions. This provided clues regarding the role of MBP1 in fermentation and could help to efficiently improve ethanol production by industrially engineered yeast strains. Furthermore, we are not aware of any prior reports of pseudohyphal differentiation of S. cerevisiae cultured in rich medium. Although the cellular mechanisms underlying the pseudohyphal growth were not clear, we proposed several hypotheses that were helpful for uncovering the mechanisms. Nevertheless, our hypotheses about the interaction between MBP1 and other genes needed to be tested. Since filamentous growth was also observed in the yeast using xylose as the sole carbon source (unpublished data), our results could also shed light on the development of xylose-fermenting S. cerevisiae.

MATERIALS AND METHODS

Strain and culture conditions.

Strain MF01 (MATa/MATα) is a wild-type diploid S. cerevisiae. Unless otherwise stated, the yeast strain was grown in YPD (2% Bacto peptone, 1% yeast extract, and 2% dextrose) at 30°C, with shaking (180 rpm), or YPD solidified with 2% agar.

Preparation of haploid strains.

For preparation of haploid strains, 0.1 ml of overnight cells was spread on a plate for sporulation (0.82% sodium acetate, 0.1% glucose, 0.25% yeast extract, 0.18% KCl, 2% agar) for 4 to 5 days. The spores were scraped and rinsed from the plate into sterilized water, collected by centrifugation, and washed twice with 0.85% NaCl. The pellets were resuspended in lysis buffer (7 mM Tris-HCl [pH 8.0], 1% β-mercaptoethanol, and 2% glusulase) and incubated overnight at 30°C, with 180 rpm shaking. The spore suspensions were then incubated at 58°C for 10 min, washed with 10 mM Tris-HCl (pH 8.0), resuspended in sterilized water, and spread on YPD plates, which were incubated for 2 to 3 days. The suspected haploid was validated using PCR (53).

Generation of MBP1 gene disruption cassette.

Plasmid pUG6 was used as a PCR template to generate the loxP–kanr–loxP gene disruption cassette (54). For the MBP1 disruption experiment, two oligonucleotides (Table 2, MBP1 gene knockout box amplification primers R and F) were used that carry a segment homologous to sequences left and right of the loxP–kanMX–loxP module on plasmid pUG6 at their 3′ end and a segment homologous to the MBP1 to be disrupted at their 5′ end. The PCR conditions for the disruption cassette were as follows: 94°C for 3 min; 94°C for 30 s, 68°C decreasing (the annealing temperature of each subsequent cycle was run at 1°C less than that of the preceding cycle) for 30 s, 72°C for 2 min for 15 cycles; 94°C for 30 s, 53°C for 30 s, 72°C for 2 min for 30 cycles; and a final step of 72°C for 10 min.

MBP1 gene disruption and verification.

Mating types a and α of MF01 were both subjected to transformations with loxP–kanMX–loxP, respectively, as described previously (55). The transformants were selected by adding Geneticin (G-418 sulfate) at 300 mg/liter in solid medium or 200 mg/liter in liquid YPD. MBP1 gene integrity verification was carried out with primers 056wa and 056wb or 056wc and 056wd, respectively (Table 2), using the following PCR protocol: 94°C for 5 min; 94°C for 30 s, 50°C for 30 s, 72°C for 2.5 min for 30 cycles; and 72°C for 10 min. Detection of the correct gene deletion of MBP1 was performed with primers Ka and Kb or Kc and Kd, respectively (Table 2), using the following PCR protocol: 94°C for 3 min; 94°C for 30 s, 55°C decreasing (the annealing temperature of each subsequent cycle was run at 1°C less than that of the preceding cycle) for 30 s, 72°C for 2 min for 10 cycles; 94°C for 30 s, 45°C for 30 s, 72°C for 2 min for 20 cycles; and 72°C for 10 min.

Mating.

Diploid strains were constructed as previously described (56) with modifications. Overnight strains of each haploid lacking MBP1 were mixed and pelleted by centrifugation, and the mixtures were resuspended in appropriate YPD and subjected to incubation for 3 to 4 h without shaking. The cells were filtered onto a 0.45-μm nitrocellulose filter and then rinsed with 5 ml of YPD. The filter was placed onto a YPD plate containing 8% dextrose and incubated for 3 to 5 h. The cells were rinsed with 5 ml of YPD and subjected to centrifugation. The cells were then resuspended, plated, and incubated for 2 to 3 days. The diploid strains were selected based on their appearance and validated using PCR (53).

Marker rescue.

The diploid kanr yeast strain with the relevant genotype mbp1:: loxP–kanMX–loxP/mbp1:: loxP–kanMX–loxP was transformed with plasmid pSH65. The transformants were selected on YPD plates supplemented with 50 μg/ml zeocin and then incubated in YPD containing 2% galactose for more than 2 h (54). A colony lacking the marker gene was selected by plating cells on YPD and replica plating the colonies onto YPD plus G418. Cells of continuous passage culture for 10 generations for the loss of pSH65 were selected based on their ability to grow on YPD but not on YPD plus zeocin. Correct loss of the kanr marker gene was verified by PCR using KanMX gene integrity verification primers (Table 2).

Fermentation.

The method for fermentation with sucrose was as follows: 2 × 108 overnight cells were inoculated into 25 ml sucrose medium (1% yeast extract, 2% Bacto peptone, and 23% sucrose, natural pH value) and grown for 32 to 34 h, followed by fermentation without shaking until 56 h, and samples were taken at 8-h intervals. The method for fermentation with molasses was as follows: 2 × 108 overnight cells were grown in 10 ml molasses medium (23 degrees Brix [°Bx] molasses, 0.2% urea, 0.02% phosphoric acid [pH 3.8 to 3.9]) for 12 h, and the same molasses medium (replacing 23°BX molasses with 55°BX molasses) was supplemented (feeding), after which the cells were grown for another 24 h, followed by fermentation without shaking for 40 h. Samples were taken at 8-h intervals from feeding (0 h) to the end of fermentation. After centrifugation, the supernatants of the samples were collected and stored at −20°C until use. Frozen supernatants were thawed before the determination of ethanol or total sugar.

Respiratory intensity assays.

Cells in the mid-log phase (8 to 10 h) were harvested by centrifugation and suspended in 1 ml YPD containing 0.1% of the respiratory indicator triphenyl tetrazolium chloride (TTC). Equal volumes of cells (1 × 108/ml) were incubated with shaking (130 rpm) and statically for 4 h. Cells were harvested by centrifugation and lysed in 1 ml lysing buffer (2% Triton X-100, 1% SDS, 100 mM NaCl, 10 mM Tris, 1 mM EDTA, ∼0.3 g quartz sand [60 to 80 mesh]) for 10 min at high speed on a high-speed vortex mixer. After centrifugation, the supernatant was collected, and the precipitate was extracted with 200 μl methanol by shaking for 5 min at high speed, followed by centrifugation, after which the supernatant was combined with the previous supernatant. The presence of reduced TTC was quantified by measuring the absorbance at 490 nm (57).

Sensitivity to cell wall inhibitors.

Detection of cell wall defects was performed as described previously (58) and was modified by replacing 0.03% sodium dodecyl sulfate (SDS) with 0.05% SDS.

Sampling of yeast cells and preparation of crude enzyme solution and enzyme assays.

Cells were harvested by centrifugation, washed with deionized water, resuspended in solutions of Tris, EDTA, and dithiothreitol (final concentrations of 100, 5, and 2 mM, respectively [pH 7.4]) (59, 60), and then quickly frozen (−80°C) until use.

After thawing, the samples were quickly ground to a fine powder in liquid nitrogen, followed by the addition of phenylmethylsulfonyl fluoride (PMSF) at a final concentration of 1 mM and mixing immediately. After centrifugation for 5 min at 4°C (13,520 × g), the supernatants were collected and the protein concentrations were determined using the Bradford Protein assay kit (Beyotime Biotechnology, Beijing, China). Peroxidase (POD) activity was determined as previously described (61). Catalase (CAT) activity was determined using a catalase assay kit (visible light; Nanjing Jiancheng Bioengineering Institute, Nanjing, China) by analyzing the complex compound generated from the reaction of H2O2 and ammonium molybdate at 405 nm. Total superoxide dismutase (T-SOD) activity was analyzed using the total superoxide dismutase assay kit (hydroxylamine method; Nanjing Jiancheng Bioengineering Institute, Nanjing, China). Alcohol-dehydrogenase (ADH) activity assay was initiated by adding crude enzyme to a reaction mixture containing glycine-potassium hydroxide (pH 9), ethanol, and NAD-trihydrate (final concentrations of 50, 100, and 1 mM, respectively). After 20 min of reaction at 30°C, ADH activity was determined by measuring the increase in absorbance at 340 nm using a DU800 spectrophotometer (Beckman, USA). One enzyme unit was defined as a change of 1 in the absorbance at 340 nm per minute per milligram of protein.

Construction of overexpression plasmid.

The plasmids (pKY) for overexpression were created by ligating the coding region of MBP1 with Kpn I (5′) and Sph I (3′) linkers added by PCR into pYES2. The coding region of MBP1 was amplified using the following PCR protocol: 94°C for 5 min; 94°C for 30 s, 55°C for 30 s, 72°C for 2 min 30 s for 30 cycles; and 72°C for 10 min. The control vector (pK) was created by ligating the loxP-kanMX-loxP disruption module with Nhe I (5′) and Nde I (3′) linkers added by PCR into pYES2. The PCR protocol was 94°C for 5 min; 94°C for 30 s, 55°C for 30 s, 72°C for 2 min for 30 cycles; and 72°C for 10 min.

Synchronization.

Overnight cells were inoculated into starvation medium (2% dextrose, 0.05 M KH2PO4) for 1 day to induce synchronization.

qRT-PCR analysis.

Cells were harvested by centrifugation, quickly frozen in liquid nitrogen, and stored frozen at −80°C until use or ground to a fine powder in liquid nitrogen. Total RNA was extracted using RNAiso Plus (TaKaRa Biotechnology Co., Ltd., Dalian, China). Genomic DNA digestion was carried out using Recombinant DNase I (TaKaRa) prior to purification with an RNA clean kit (Tiangen Biotech, Beijing, China). Single-stranded cDNA synthesis was performed using TransScript first-strand cDNA synthesis super mix (TransGen Biotech, Beijing, China) with approximately 3 μg RNA as a template. The products were diluted 10-fold and used as the templates for qRT-PCR amplification using SYBR Premix Ex Taq II (TaKaRa Biomedical Technology, Beijing, China). The qRT-PCRs were performed using an ABI 7500 system in an 8-cap strip, with each reaction mixture containing 10 μl of SYBR Premix Ex Taq II (2×), 0.8 μl of each forward and reverse primer (10 μM) (Table 2), 0.4 μl of ROX Reference Dye II (50×), 6 μl water, and 2 μl of diluted reverse transcription product (no more than 100 ng). The amplification protocol was 1 cycle at 95°C for 30 s and 40 cycles at 95°C for 5 s, 56°C for 30 s, and 72°C for 34 s. Fluorescence intensity was detected at 72°C in each cycle. A melting curve was generated by heating from 60°C for 1 min to 95°C for 30 s at 0.1°C/s. The specificity of the PCR product was verified by melt-curve analysis.

Statistics.

Statistical comparisons were made using the Student’s t test (two-tailed, paired) using Microsoft Excel. P values were considered significant as follows: *, P < 0.05; **, P < 0.01; ***, P < 0.001; ns (not significant), P > 0.05.