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Comparison of expression systems for the extracellular production of mannanase Man23 originated from Bacillus subtilis B23

Microbial Cell Factories volume 12, Article number: 78 (2013) Cite this article

Abstract

Background

Mannanase is an enzyme that can catalyze random hydrolysis of beta-1,4-mannosidic linkages in the main chain of mannans, glucomannans and galactomannans which are the key polymers in hemicellulose. It has been used in a number of different industrial applications including food, feed, pharmaceutical, pulp/paper industries, and second generation biofuel. To optimize the expression system of mannanase Man23 gene, two kinds of vectors and host bacteria were determined and compared.

Results

Recombinants pHY-p43-man23 and pBPS-man23 were constructed and transferred into Bacillus subtilis WB600 and Brevibacillus brevis respectively. For mannanase Man23 gene, recombinant pHY-p43-man23 expressed in Brevibacillus brevis had higher production and activity. Compared to the wild-type Bacillus subtilis B23, the production of recombinant pHY-p43-man23 in B. brevis increased by 10 times and activity increased by 21.3%. pHY-p43-man23 in B. brevis had activity at the range of 20 ~ 70°C but its optimum temperature was 50°C and had activity from pH 4 ~ 10 but its optimum pH was around 7. This demonstrated the recombinant had improved stability as well.

Conclusions

Mannanase is an important industrial enzyme and combination of vector pHY-p43 and host Brevibacillus brevis is a novel expression system for a mannanase decoding gene. This work aims at exploring a better expression system of mannanase Man23 decoding gene for industrial application.

Background

β-Mannanase, an extracellular enzyme, has hemicellulase activity or the activities of both hemicellulase and cellulase [1]. Mannanase can catalyze random hydrolysis of beta-1,4-mannosidic linkages in the main chain of mannans, glucomannans and galactomannans which are the key polymers in hemicellulose [2]. It is widely used by industries including food processing, feed, oil mining, paper making, pharmaceutical, and second generation biofuel [3, 4]. It is especially involved in breaking down plant tissues by degrading mannan polymers in the cell walls [5].

Mannanases once were isolated from plants [6], marine mollusk [7], and a body of bacteria and fungi [8, 9]. According to the hydrophobic cluster analysis of reported mannanases, they have been classified into glycoside hydrolase (GH) families 5 and 26. In this paper, mannanase Man23 which originated from Bacillus subtilis B23 belongs to family 26.

Wild-type mannanase Man23 has high activity and stability. We found that the sites of H129, E159, H190, E191, W196, F197, W198, and W199 on mannanase Man23 are relevant to the activity and substrate binding. The mutations at the sites of H129, H190, and W198 increased activity by 3.5-, 2.2-, and 3.8-fold, respectively (Haiyan Z, Xu N, Yong Y, Wenjiao Y, Yongyao W: Engineering mannanase Man23 decoding gene from Bacillus Subtilis B23 by semi-rational design, submitted). Herein, in order to promote the production and stability for meeting its commercial usage, our team had a further study to optimize the expression system of mannanase Man23. We evaluated two vectors, pHY-p43 and pBKE50, and two host bacteria, Bacillus subtilis (B. subtilis) WB600 and Brevibacillus brevis (B. brevis), to figure out how the recombinant expression plasmids performed in the two novel hosts. This work provides insights into how an optimized expression system worked on mannanase Man23 gene and moreover, it throws a clue to select a more suitable expression system and a host bacterium for cellulase or hemicellulase gene.

Results

Comparison of gene man23 expressed in host B. subtilis WB600 and B. brevis

For the economical reason, it is necessary to construct the stable expression systems for producing recombinant proteins. At present, about 60% of the commercially available enzymes are produced by Bacillus species [10]. In comparison of Escherichia coli (E. coli), B. subtilis is an attractive host for enzyme production since it is nonpathogenic and has a high capacity of secreting extracellular proteins directly into the medium [11]. However, B. subtilis greatly reduces the production and intactness of the secreted proteins because of it secrets at least seven extracellular proteases [12]. A series of extracellular-protease-deficient Bacillus strains were improved as a cell factory for secreting target proteins.

B. subtilis WB600 is a six-extracellular-protease-deficient strain and it was shown that in this strain, protein degradation is minimized and the production of some proteins was improved compared to that in the wild-type [13].

B. brevis is a naturally extracellular-protease-deficient strain and has been known to exhibit high productivity of heterologous proteins into the culture medium but produce little extracellular protease [14, 15], which enables a high recovery of the target proteins with minimal degradation. Thus it has been used as a good host for production of heterologous proteins. Importantly, these two hosts have the clearly-known metabolic background.

The gene man23 using pHY-p43 as the expression vector firstly was introduced into the two hosts B. subtilis WB600 and B. brevis. The production yield of total proteins and mannanase Man23 in different hosts was shown in Figure 1. In comparison to the wild-type, B. bacillus WB600 and B. brevis displayed a better ability to express gene man23. The production of total proteins in B. bacillus WB600 and B. brevis increased by 12% and 16%, meanwhile, the production of mannanase Man23 increased by 9.8-fold and 10.5-fold and mannanase activity increased by 21% and 21.3% respectively.

Figure 1
figure 1

The production of total proteins and mannanase expressed by pHY-p43- man23 in different hosts.

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SDS-PAGE was used to identify the secreted protein from different hosts and the result was shown in Figure 2. From the diagram, B. subtilis WB600 and B. brevis displayed their excellent and high-efficient production for mannanase Man23. Especially, B. brevis had a clearer electrophoresis background compared to WB600 and wild-type host, which suggested B. brevis produced more mannanase Man23 and less other proteins. Thus, the purity of mannanase Man23 from B. brevis was highest among the tested hosts. In comparison with B. subtilis WB600 and B. brevis, the total protein production in B. brevis was higher than B. subtilis WB600 by 3% and mannanase Man23 production was higher by 6.3%. Table 1 demonstrated the mannanase activity produced in B. brevis was higher than B. subtilis WB600 by 0.6%.

Figure 2
figure 2

SDS-PAGE of gene man23 expression products in different hosts. M: standard protein molecular weight marker; 1: crude extract of B. bacillus WB600; 2: crude extract of B. brevis; 3: crude extract of wild-type host; 4: crude extract of B. bacillus WB600 (with pHY-p43-man23); 5: crude extract of B. brevis (with pHY-p43-man23). The target band arrow pointed to is mannanase band.

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Table 1 Comparison of mannanase activity produced by pHY-p43- man23 in different hosts
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Considering the data above and mannanase purity, B. brevis has been used as the host for expressing gene man23 in our following work.

Comparison of the expression vectors pHY-p43 and pBKE50 for gene man23

Plasmid pBKE50 is a shuttle vector which includes the replication origin of pUB110 and the erythromycin-resistance gene of pGK12. Plasmid pHY-p43 is also a shuttle vector which includes the strong promoter P43. In our work, these two vectors were introduced to express gene man23 in B. brevis.

Mannanase Man23 encoding gene was identified to be 1100 bp and was registered on Genbank [16]. Gene man23 was cloned using primer P1 and P2 to add BamH I and EcoR I restriction sites for the link with vector pHY-p43 and using primer P3 and P4 to add BamH I and Kpn I restriction sites for the link with vector pBKE50.

Both recombinants, pHY-p43-man23 and pBPS-man23, had excellent performance when they transformed into the host B. brevis and the results about production yield and mannanase activity of these two recombinants were shown in Table 2. Apparently, both recombinants produced much more mannanase and higher activity. The amount of total proteins expressed by pHY-p43-man23 and pBPS-man23 was enhanced by 19% and 4% compared to the wild-type. Moreover, comparing to the wild-type, the amount of mannanase Man23 increased by 11.25-fold and 8.05-fold and the mannanase activity increased by 18% and 3.4% respectively. From the data, it can be easily figured out that pHY-p43-man23 had more proteins production by 14.45%, more mannanase production by nearly 40% and higher mannanase activity by 14% than pBPS-man23. For this reason, in our following work, pHY-p43 has been used as the vector to express gene man23.

Table 2 Comparison of the production yield and mannanase activity produced by different expression plasmids
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Biochemical characteristics of recombinant mannanase Man23 expressed by pHY-p43-man23 in host B. brevis

To obtain the details about recombinant mannanase Man23, herein we determined its biochemical characteristics. It had activity at the temperature range of 20 ~ 70°C and its optimum temperature is 50°C (Figure 3). When the recombinant Man23 had been maintained at different temperature for 20 hours, it displayed high stability at temperature of 20 ~ 40°C and reduced sharply at 50°C in 20 hours (Figure 3). Compared to the wild-type which had the optimum temperature 45°C and the activity range of 30 ~ 60°C, the recombinant mannanase Man23 displayed a broader temperature range with high activity and a better heat tolerance.

Figure 3
figure 3

Effects of temperature on activity and stability of recombinant mannanase Man23.

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Meanwhile, the optimum pH of wild-type was 6.5 and it had activity in the pH range of 4 ~ 9. Nevertheless, recombinant mannanase Man23 had activity in a broader pH range of 4 ~ 10 and its optimum pH shifted slightly to around pH 7 (Figure 4). When being reserved in the phosphate buffer of pH 5 ~ 7 for 20 hours, the recombinant Man23 still kept 90% of activity but when out of pH 5 ~ 7 it was not very stable (Figure 4).

Figure 4
figure 4

Effects of pH on activity and stability of recombinant mannanase Man23.

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The kinetic parameters of recombinant Man23 degrading locust bean gum were determined in 50 mmol/L phosphate buffer of pH 7.0 at 50°C. Through the Lineweaver-Burk Plot, the values of K m and V max were 0.38 mg · ml-1 and 301 μmol · mg-1 · min-1.

Discussion

Endo-1,4-β-Mannanase has been classified into two glycosyl hydrolase families, GH family 5 and 26, according to the amino acid sequence similarities and hydrophobic cluster [17]. From the sequence analysis, mannanase Man23 mentioned in this paper belongs to family GH26.

There have been some reports about the optimization of expression system and the characterization of recombinant mannanase as summarized in Table 3. The optimal pH, temperature and the stability of mannanases reported were varying depending on the sources. Some mannanases screened by Katrolia P. [18] and Songsiriritthigul C. [2] had similar enzyme characteristics with mannanase Man23 and mannanase screened by Vu TT [19] had similar optimum pH with mannanase Man23 but the latter had broader pH activity range and higher thermo-stability. The activity and kinetic parameters of the mannanases from different sources varied greatly mainly because there are lots of differences with the structure of these mannanases. Usually, some thermostable mannanases tend to have lower specific activity in comparison with their mesophilic counterparts [20]. When comparing to other mannanases, it worth to be noticed that different substrates and individual techniques whittled down the accuracy for evaluating mannanase activity.

Table 3 Properties of various mannanase recombinants
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From the references, mannanase encoding gene from different organisms was transformed to express in prokaryotic cells such as E. coli and B. subtilis and eukaryotic cells such as yeasts. Mannanase Man23 encoding gene was hardly secreted from E. coli, therefore E. coli would not be a good option if the secretary proteins were expected. Moreover, the secretion of proteins would simplify the extraction procedure. Both B. subtilis WB600 and B. brevis are effective hosts for secretary proteins since there are abundant of vectors and regulatory elements for Bacillus species to help proteins folding [33, 34]. B. brevis especially has its advantages to be the expression host for gene man23 because B. brevis can secrete disulfide-bond-promoting factors to help proteins folding [35]. In our previous work, mannanase Man23 was found one disulfide bond formed between Cys90 and Cys110. Actually, our results about two tested hosts demonstrate B. brevis is more suitable for gene man23 indeed. Eukaryotic cells usually have the capacity to express extracellular proteins efficiently. However, considering the economic reasons, prokaryotic cells have their advantages because of the shorter production period and the simpler extraction process compared to that of eukaryotic cells.

Each expression host has one or more applicative vectors. Some reported mannanase genes used their native expression vector, and while some were recombined into other vectors. Vector pJ27Δ88U was tested and suitable for use in B. subtilis 168. In our work, plasmid pBKE50 and pHY-p43 are the shuttle vectors of E. coli and Bacillus. For gene man23, the promoter p43 on the vector pHY-p43 showed high efficiency to manipulate mannanase Man23 encoding gene in B. brevis. It deserves the further researches on other applicable vectors for gene man23 expression in B. brevis.

Conclusions

The system composed of vector pHY-p43 and host B. brevis is a novel expression system for mannanase encoding gene. Our results demonstrate that this novel system is efficient for expressing and secreting mannanase Man23 encoding gene, which deserves to be considered for indus-trial applications. Additionally, this expression system could be adopted for producing other enzymes as well.

Methods

Extraction of genomic DNA and plasmid DNA

Genomic DNA was extracted by SDS method [36] and plasmid DNA was extracted by alkaline lysis method [37].

Cloning of mannanase Man23 encoding gene

Through the sequence alignment with high homology, two couples of primers were designed to clone mannanase Man23 encoding gene from the whole DNA of wild-type. One couple used to clone the decoding gene linked with vector pHY-p43 is P1:5′-CGCGGATCCATGCCTACTAAGT-3′ (underline is BamH I restriction site) and P2:5′-CGGAATTCTGATTCAGCTATCTGTG-3′ (underline is EcoR I restriction site). The other couple used to clone the decoding gene linked with vector pBKE50 is P3:5′- CGCGGATCC ATGCCTACTA AGT-3′ (underline is BamH I restriction site)and P4:5′-GGGGTACCTGATTCAGCT ATCTGTG-3′ (underline is Kpn I restriction site).

The PCR reaction is 94°C for 5 min, followed by 30 cycles of 94°C for 30 s; 56°C for 30 s; 72°C for 1 min, then 72°C for 10 min, 4°C thereafter. Cloning products were detected and recycled according to reference [38].

Construction of expression plasmid pHY-p43-man23

Plasmid pHY-p43-man23 was constructed from plasmid pHY-p43 and gene man23 with BamH I and EcoR I restriction sites. The plasmid pHY-p43 (CICIM MMB0050) was purchased from CICIM-CU. The procedure of construction was represented in Figure 5.

Figure 5
figure 5

The construction of expression plasmid pHY-p43- man23.

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Construction of expression plasmid pBPS-man23

Plasmid pBPS-man23 was constructed from plasmid pBKE50 and gene man23 with BamH I and Kpn I restriction sites. Plasmid pBKE50 was constructed basing on initial plasmids pKF3 [39] and pUB110 [40]. After digestion and re-link, the intermediate plasmid pKF33 was linked with erythromycin-resistance gene (Emr) to form plasmid pKF34. Another couple of primers, P5 and P6, were designed to clone the decoding gene of the promoter and signal peptide of B. brevis. P5 is 5′-CCCAAGCTTCGTGAG AATGCGTACCAAA-3′ (underline is Hind III restriction site) and P6 is 5′-TCCCCCGGGCGAAAGCCATGGGAGCAAC-3′ (underline is Sma I restriction site). The PCR reaction was 94°C for 5 min, followed by 30 cycles of 94°C for 40 s; 60°C for 30 s; 72°C for 50 s, then 72°C for 5 min, 4°C thereafter. The decoding gene of the promoter and signal peptide (PS) of B. brevis and plasmid pKF34 were digested with Hind III and Sma I and then linked together to form the shuttle vector pBKE50. The details of construction procedure were represented in Figure 6.

Figure 6
figure 6

The construction of expression plasmid pBPS- man23. MLS: multiple clone sites; cat-5: chloramphenicol resistance gene; Emr: erythromycin resistance gene; ori: replication of E. coli; rep: replication of B. brevis; PS: decoding gene of the promoter and signal peptide of B. brevis.

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Transformation and expression of the recombinant plasmids

B. bacillus WB600 and B. brevis are both the Bacillus species hosts, therefore the approaches recombinant plasmids transforming into the hosts are similar and elaborated as following.

The host cells were shaking cultured in T2 medium [41] overnight at 37°C and then cultures were refreshed into 5 ml of T2 medium by 1% of incubation amount and continued culturing till the late stage of logarithmic growth. The host cells were collected and suspended in 5 ml of 50 mmol/L Tris–HCl (pH 7.5) for a while and then cultured in 5 ml of 50 mmol/L Tris–HCl (pH 8.5) at 37°C for one hour. The host cells were collected into 0.5 ml of TP medium (phosphate buffer (1.905 g KH2PO4, 0.852 g Na2HPO4, 100 ml) mixed with 2 × T2 medium in proportion of 1:1) and at the same time, 100 μl of TE/TP buffer (TE buffer(10 mmo1/L Tris–HCl, pH 7.5 and l mmo1/L EDTA) mix with TP medium in proportion of 1:1) blended with 20 ul recombinant plasmids of 10 ng/ul and 1.5 ml PEG solution (PEG6000 400 g, 500 ml phosphate buffer). The mixture was incubated at 37°C for 10 min and then the host cells were recollected into 1 ml MT medium (MgCl2 in T2 medium with final concentrate of 20 mmol/L) and agitated at 37°C for 30 min. After antibiotics Amp of 50 ug/ml and Tet of 40 ug/ml were added into MT medium, the cultivation was continued for another 2 h. The plate cultures with 100 ug/ml of Amp and 60 ug/ml of Tet were used successively to screen individual colonies.

Isolation of native and recombinant mannanase Man23

Crude proteins were prepared from supernatant after centrifuge and then successively purified through salting-out, molecular sieve chromatography Sephadex G-100 and ion-exchange column chromatography. The isolation procedure was carried out according to reference [42].

Determination of recombinant mannanase activity and biochemical characteristics

Protein concentration was measured using the Bradford assay [6]. Mannanase activity assay was improved from the method of reducing sugar assay [43, 44]. One unit of enzyme activity was defined as the amount of enzyme liberating 1 μmol mannose per minute at 50°C and pH 6.8. The activity formula was as follows:

Mannanase activity(U/ml) = 5.56CeVde/VjeVst

5.56 the mole value of 1.0 mg mannose, μmol

Ce amount of mannose produced from hydrolysis, mg

Vde metered volume of enzyme solution, ml

Vje volume of enzyme solution added into the reaction mixture, ml

Vs volume of substrate solution, ml

t time, min

Specific activity of mannanase (units per milligram) = 5.56CeVde2/CpVjeVst

Cp amount of total proteins, mg

The optimal temperature of mannanase Man23 was evaluated by the activity assay at 20, 30, 40, 50, 60, 70, 80, 90°C for 10 min. The assay was performed with 1 ml mannanase solution (~1.0 mg/ml) at pH 6.8 and 50 mmol/L phosphate buffer.

The optimal pH was evaluated by the activity assay in different pH values of 50 mmol/L phosphate buffer for 10 min and temperature was maintained at 50°C. The mannanase amount was same as above.

Thermostability of mannanase Man23 was measured by incubating the samples for 20 hours at different temperatures and then plotting the residual activity versus the incubation time. The pH tolerance was measured by incubating the samples for 20 hours at different pH and then plotting the residual activity versus the incubation time.

Electrophoresis analysis of protein samples

The proteins extracted from wild-type, B. bacillus WB600 and B. brevis were analyzed by SDS-PAGE [45]. Marker was purchased from TIANGEN biotech co., LTD and it includes six bands of 97.4, 66.2, 43.0, 31.0, 20.1 and 14.4 Ku.

Statistical analysis

Data were presented as the mean ± standard error of the mean. Results were compared with the analysis of variance and Fisher’s protected least-significant difference tests, with a significance of P < 0.05.

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Authors and Affiliations

  1. College of Bioscience and Biotechnology, Hunan Agricultural University, Changsha, 410128, China

    Haiyan Zhou, Yong Yang, Xu Nie, Wenjiao Yang & Yongyao Wu

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  1. Haiyan Zhou
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  2. Yong Yang
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  3. Xu Nie
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  4. Wenjiao Yang
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Correspondence to Yongyao Wu.

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The authors declare that they have no competing interests.

Authors’ contributions

HZ conceived and designed the study, carried out the molecular genetic studies, and drafted the manuscript. YY and XN carried out the genetic studies and the determinations. WY participated in determinations and performed the statistical analysis. YW conceived of the study, participated in its design and helped to draft the manuscript. HZ, YY, XN, WY and YW reviewed and edited the manuscript. All authors read and approved the final manuscript.

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Zhou, H., Yang, Y., Nie, X. et al. Comparison of expression systems for the extracellular production of mannanase Man23 originated from Bacillus subtilis B23. Microb Cell Fact 12, 78 (2013). https://doi.org/10.1186/1475-2859-12-78

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  • DOI: https://doi.org/10.1186/1475-2859-12-78

Keywords

Microbial Cell Factories

ISSN: 1475-2859

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